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NZHTA REPORT
November 2006
Volume 9 Number 4
Screening Strategies for Antenatal Down Syndrome
Screening
A systematic review of the literature
Rebecca O’Connell
Meagan Stephenson
Robert Weir
New Zealand
Health Technology Assessment
Department of Public Health and General Practice
Christchurch School of Medicine and Health Sciences
Christchurch, New Zealand
NEW ZEALAND HEALTH TECHNOLOGY ASSESSMENT (NZHTA)
Department of Public Health and General Practice
Christchurch School of Medicine and Health Sciences
Christchurch, New Zealand
Screening Strategies for Antenatal Down
Syndrome Screening
A systematic review of the literature
Rebecca O’Connell
Meagan Stephenson
Robert Weir
NZHTA REPORT
November 2006 Volume 9 Number 4
This report should be referenced as follows:
O’Connell, R. Stephenson, M. Weir, R. Screening strategies for antenatal Down syndrome
screening. NZHTA Report 2006; 9(4).
2006
New Zealand Health Technology Assessment (NZHTA)
ISBN
ISBN
ISSN
1-877235-93-8 (Print)
1-877235-94-6 (Web)
1174-5142
i
CONTRIBUTION BY AUTHORS
This report was authored by Rebecca O’Connell (Research Fellow), and Meagan Stephenson (Research
Fellow) who both conducted the critical appraisals and prepared the report. Dr Rob Weir (Director)
also contributed to the writing of the methods section.
ACKNOWLEDGEMENTS
Dr Rob Weir (Director) peer reviewed the final draft. Susan Bidwell (Information Specialist)
developed and undertook the search strategy and coordinated retrieval of documents. Catherine
Turnbull (Administrator) provided document formatting. Kay Hodgson assisted with retrieval of
documents.
Acknowledgment is made of the contribution of Professor Nicholas Wald, Director, Wolfson Institute
of Preventive Medicine, who undertook an external peer review of a late draft and provided valuable
comments on the report.
The Canterbury Medical Library assisted with the retrieval of articles.
NZHTA is a Research Unit of the University of Otago funded under contract to the New Zealand
Ministry of Health.
This report was commissioned by Karen Mitchell, Group Manager, National Screening Unit, of New
Zealand’s Ministry of Health. We thank the National Screening Unit staff at the Ministry of Health for
partially funding the review, assisting in developing the scope and providing background material for
the review.
DISCLAIMER
New Zealand Health Technology Assessment (NZHTA) takes great care to ensure the information
supplied within the project timeframe is accurate, but neither NZHTA, the University of Otago, nor the
contributors involved can accept responsibility for any errors or omissions. The reader should always
consult the original database from which each abstract is derived, along with the original articles,
before making decisions based on a document or abstract. All responsibility for action based on any
information in this report rests with the reader. NZHTA and the University of Otago accept no liability
for any loss of whatever kind, or damage, arising from reliance in whole or part, by any person,
corporate or natural, on the contents of this report. This document is not intended as personal health
advice. People seeking individual medical advice are referred to their physician. The views expressed
in this report are those of NZHTA and do not necessarily represent those of the University of Otago or
the New Zealand Ministry of Health.
This review was commissioned by Karen Mitchell, on behalf of the New Zealand Ministry of Health.
NZHTA is a Research Unit of the University of Otago and is funded under contract by the New Zealand
Ministry of Health.
COPYRIGHT
This work is copyright. Apart from any use as permitted under the Copyright Act 1994 no part may be
reproduced by any process without written permission from New Zealand Health Technology
Assessment. Requests and inquiries concerning reproduction and rights should be directed to the
Director, New Zealand Health Technology Assessment, Christchurch School of Medicine and Health
Sciences, P O Box 4345, Christchurch, New Zealand.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
ii
CONTACT DETAILS
New Zealand Health Technology Assessment (NZHTA)
Department of Public Health and General Practice
Christchurch School of Medicine and Health Sciences
PO Box 4345
Christchurch
New Zealand
Tel: +64 3 364 3696
Fax: +64 3 364 3697
Email: [email protected]
Web Site: http://nzhta.chmeds.ac.nz/
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
iii
EXECUTIVE SUMMARY
Background
This review was requested by the Ministry of Health to inform the policy process in assessing options
for antenatal Down syndrome screening and in determining whether a national antenatal screening
programme for Down syndrome should be established in New Zealand.
Aim
This review aimed to systematically appraise the international evidence for the use of technologies and
screening strategies for antenatal Down syndrome. Including:
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The validity of Down syndrome screening methods
Any difficulties implementing screening strategies
The impact of screening on amniocentesis and chorionic villus sampling
The safety of these procedures.
Data sources
The following databases were searched (using the search strategy outlined in Appendix 1):
Bibliographic databases
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Cinahl
Cochrane Register of Controlled Trials
Current Contents
Embase
Medline
PubMed (last 60 days)
Science Citation Index
Social Science Citation Index
Review databases
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ACP Journal Club
Cochrane Database of Systematic Reviews
Database of Abstracts of Reviews of Effectiveness
Health Technology Assessment database
NHS Economic Evaluation database
Other
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Clinicaltrials.gov
Current Controlled Trials
References of retrieved papers were scanned for relevant publications.
TRIP database
UK National Screening Committee Down’s Syndrome Screening Programme
Hand searching of journals, contacting of manufacturers, or contacting of authors for unpublished
research was not undertaken in this review. A complete list of the sources searched for this review is
given in Appendix 2.
Searches were limited to English language material published from January 2000 onwards. The
searches were completed on 10 August 2006.
Result of the search strategy
The search strategy for the validity of screening strategies and implementation difficulties yielded 1138
articles. From 219 articles identified as potentially eligible for inclusion, a final group of 66 papers
were selected for appraisal, all of which were primary research (including statistical modelling). The
search strategy for the impact of screening on invasive testing rates and the safety of those invasive
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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tests yielded 1116 articles. From 192 articles identified as potentially eligible for inclusion, a final
group of 35 papers were selected for appraisal, all but one of which were primary research.
Key results
Accuracy of screening methods
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Maternal age alone is not an appropriate screening test for DS.
Screening methods that combine tests in an independent manner are not recommended.
The quad test provided the best screening performance characteristics in the 2nd trimester
The combined test performed better than other 1st trimester tests and all 2nd trimester strategies,
and serum integrated screening had a similar performance to the combined test.
All other integrated and sequential screening strategies have improved performance compared to
either 1st trimester or 2nd trimester screening strategies.
Integrated screening performed better than both stepwise and contingent screening, with a lower
FPR for a fixed DR.
The performance of stepwise and contingent screening is similar.
Difficulties implementing any screening strategies
The following implementation difficulties were reported:
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NT measurement not successful or taking more time than expected,
NT requiring trained staff, high quality equipment and quality control,
women defaulting from 2nd trimester maternal serum screening,
need to adjust for maternal weight, and for false positive results in previous pregnancies
need for USS dating,
issues with serum marker reliability (assay drift, and inaccurate marker MoM),
inappropriate model parameters giving inaccurate risk estimates,
issues with screening in twin pregnancies.
Uptake of invasive testing following receipt of screening results
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Maternal age (<35 years versus ≥ 35 years) appears to be a factor in the uptake of invasive testing
following screening.
Women’s individual estimates of calculated risk appear to influence the uptake of invasive testing,
with an increase in the uptake of invasive testing as the likelihood of carrying a fetus with DS
increases.
Perceived accuracy of the screening test and social, ethnic and cultural factors may influence
uptake and it would be wise to conduct a local study of the acceptability of both screening and
invasive testing.
Changes in the rate of invasive testing with the introduction of a screening programme
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Overall, rates of invasive testing increased slightly with the introduction of screening programmes.
This was against the backdrop of a steeper rise in maternal age and the increase in invasive testing
was less than what would be expected if invasive tests were offered based on maternal age alone.
Changes in rates of invasive testing varied as a function of maternal age. Rates of invasive testing
decreased among older mothers (≥ 35 years) and increased among younger mothers (< 35 years)
with the introduction of a screening programme.
Rates of fetal loss associated with invasive testing procedures
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A high quality systematic review confirmed that a 1% increased risk of fetal loss (against a
background risk of 2%) following amniocentesis in a low risk population is the best estimate of the
rate of procedure-related loss.
The recommendations of the review were that prenatal diagnosis is safest performed in the second
trimester by amniocentesis, which is safer than both transcervical CVS and first trimester
amniocentesis. Transabdominal CVS is the safest method for first trimester prenatal diagnosis,
followed by transcervical CVS.
Conclusions
Amongst the papers identified to assess the validity of DS screening methods the evidence indicated
that integrated or sequential screening had superior screening performance compared with screening
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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confined to either the 1st or 2nd trimester, and these are the screening methods of choice, whether it be
the integrated test, or sequential methods (contingent and stepwise screening).
Studies considered in this review had different strengths and weaknesses. The best designs for
determining the validity of a screening method are observational studies (cohort and nested casecontrol studies) in which clinical intervention does not follow a positive screening result (for example,
where NT screening results are not used clinically until the results of second trimester screening are
available). Studies based on intervention are subject to the bias that some screen positive affected
pregnancies would abort spontaneously in the absence of screening and selective ToP. Such studies
will tend to overestimate the screening performance of the tests considered. Some of the evidence
comparing the validity of different screening methods was also obtained from case-control studies. In
these studies the sample will include cases (Down syndrome) and unaffected controls, and may not be
representative of the groups who would be tested in a screening programme. Some modelling papers in
this review used the same primary data, similar modelling techniques, and similar assumptions which
may mean the same or similar results are replicated.
In relation to the uptake of invasive testing procedures following screening for Down syndrome, it
appears that both maternal age and individual risk estimates are factors in women’s decisions to opt for
invasive testing or not. Other factors may also play a part in the uptake of both screening and invasive
testing, such as perceived confidence in the accuracy of the screening test, and the social-acceptability
of screening and invasive testing.
The overall rate of invasive testing may increase slightly with the introduction of a screening
programme but when examined by maternal age group, it appears that the rate of invasive testing
increases in younger mothers and decreases in older mothers. Long-term evaluations of populationbased screening programmes using integrated and sequential methods have not been completed as yet,
so the effects on invasive testing rates are unclear at this stage. Relative to a screening programme
based on maternal age alone, the introduction of first or second trimester screening methods decreases
the rate of unnecessary invasive procedures. Again, social, ethnic and cultural variability in the
acceptability of screening and invasive testing is a factor in the impact of screening policy changes.
Because of this variability, it would be wise to conduct a local study of the acceptability of screening
and invasive testing in older and younger mothers of different ethnic groups before implementing a
large-scale screening programme in New Zealand.
There are a number of considerations apart from the validity of a screening strategy which are
important when deciding between the different screening strategies including: acceptability of the
strategies to women and clinicians, compatibility with neural tube defect screening, and the availability
of accurate alternative screening methods if women do not present at the appropriate gestational age.
The implications for resources for training, monitoring, and quality control particularly for NT testing
would need to be carefully considered when determining whether a screening programme should
proceed. It would also be important to ensure software is available which will accurately determine an
individual’s risk of DS, including calculation of correct MoMs, adjustments (including for maternal
weight, and false positive results from previous pregnancies) and use of appropriate population
parameters for Gaussian distributions.
Mesh headings
Down syndrome, chromosomes-human-pair 21, pregnancy trimester-first, pregnancy trimester-second,
ultrasonography-prenatal, nuchal translucency measurement, prenatal diagnosis, mass screening,
amniocentesis, chorionic villi sampling
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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TABLE OF CONTENTS
CONTRIBUTION BY AUTHORS ......................................................................................................................I
ACKNOWLEDGEMENTS ...............................................................................................................................I
DISCLAIMER ...............................................................................................................................................I
COPYRIGHT ................................................................................................................................................I
CONTACT DETAILS ....................................................................................................................................II
EXECUTIVE SUMMARY .............................................................................................................................III
TABLE OF CONTENTS ............................................................................................................................... VI
LIST OF TABLES ..................................................................................................................................... VIII
LIST OF ABBREVIATIONS AND ACRONYMS ............................................................................................... IX
LIST OF ABBREVIATIONS AND ACRONYMS ............................................................................................... IX
GLOSSARY............................................................................................................................................. XIII
CHAPTER 1: BACKGROUND
1
NEED FOR SYSTEMATIC REVIEW ................................................................................................................1
SCREENING - GENERAL OVERVIEW ............................................................................................................2
AIM ...........................................................................................................................................................2
REVIEW SCOPE ..........................................................................................................................................2
REVIEW QUESTIONS ...................................................................................................................................3
DOWN SYNDROME SCREENING METHOD TERMINOLOGY ............................................................................3
STRUCTURE OF REPORT .............................................................................................................................5
CHAPTER 2: REVIEW METHODOLOGY
7
SELECTION CRITERIA .................................................................................................................................7
SEARCH STRATEGY ....................................................................................................................................8
STUDY SELECTION .....................................................................................................................................9
APPRAISAL OF STUDIES ...........................................................................................................................10
KEY OUTCOME MEASURES FOR PRIMARY STUDIES...................................................................................11
PART A
CHAPTER 3: ACCURACY OF FIRST TRIMESTER SCREENING STRATEGIES 15
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY ..............................................................................15
PRIMARY RESEARCH: STUDY RESULTS ....................................................................................................17
CHAPTER 4: COMPARISON OF SECOND TRIMESTER SCREENING
STRATEGIES
63
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY ..............................................................................63
PRIMARY RESEARCH: STUDY RESULTS ....................................................................................................64
CHAPTER 5: COMPARISON OF 1ST TRIMESTER STRATEGIES, 2ND
TRIMESTER STRATEGIES, INTEGRATED AND SEQUENTIAL METHODS.
85
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY ..............................................................................85
PRIMARY RESEARCH: STUDY RESULTS ....................................................................................................87
PART B
CHAPTER 6: CHANGES IN THE RATE OF INVASIVE TESTING
FOLLOWING THE INTRODUCTION OF SCREENING
135
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY ............................................................................135
PRIMARY RESEARCH: STUDY RESULTS ..................................................................................................138
CHAPTER 7: UPTAKE OF TESTING FOLLOWING SCREENING RESULTS
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
157
vii
CHAPTER 8: INVASIVE TESTING AND PROCEDURE-RELATED LOSS
185
SECONDARY RESEARCH ........................................................................................................................ 185
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY ............................................................................ 187
PRIMARY RESEARCH: STUDY RESULTS .................................................................................................. 188
CHAPTER 9: DISCUSSION
197
SUMMARY OF EVIDENCE ....................................................................................................................... 197
CONCLUSIONS ....................................................................................................................................... 198
REFERENCES
201
APPENDIX 1: SEARCH STRATEGIES
207
SEARCH STRATEGIES ............................................................................................................................. 207
SEARCHES FROM OTHER SOURCES ......................................................................................................... 211
APPENDIX 2: SOURCES SEARCHED
213
SOURCES SEARCHED ............................................................................................................................. 213
APPENDIX 3 RETRIEVED STUDIES EXCLUDED FOR REVIEW : PART A
215
APPENDIX 4: RETRIEVED STUDIES EXCLUDED FOR REVIEW: PART B
223
APPENDIX 5:
231
DESIGNATIONS OF LEVELS OF EVIDENCE ............................................................................................... 231
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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LIST OF TABLES
Table 1:
Criteria for assessing screening programmes ............................................................. 2
Table 2:
Down syndrome screening methods that use both first and second trimester
screening tests ............................................................................................................ 4
Table 3.
Assessment of validity of a diagnostic test............................................................... 11
Table 4.
Comparison of DRs and FPR, maternal age versus other screening strategies ........ 17
Table 5.
Comparison of DRs for a 5% FPR, combined test, nuchal translucency and
fβhCG + PAPP-A..................................................................................................... 18
Table 6.
Comparison of DRs and FPR for fixed cut offs (same for all tests unless
indicated), combined test, nuchal translucency and fβhCG + PAPP-A.................... 19
Table 7.
Comparison of FPRs for an 85% DR, combined test, nuchal translucency and
fβhCG + PAPP-A..................................................................................................... 20
Table 8.
Comparison of DRs and FPR, fβHCG and total hCG .............................................. 20
Table 9.
Comparison of DRs and FPR, fβHCG and PAPP-A ................................................ 21
Table 10.
Evidence table of primary research studies appraised investigating the accuracy
of first trimester combined screening compared to components .............................. 24
Table 11.
Comparison of DRs and FPRs, maternal age versus other screening strategies ....... 65
Table 12.
Comparison of performance of the quad test, triple test, and double test................. 66
Table 13.
Evidence table of primary research studies appraised investigating the accuracy
of second trimester screening compared to components .......................................... 69
Table 14.
Non-interventional studies comparing DRs and FPRs of 1st trimester NT (or
combined test) versus 2nd trimester strategies (and integrated, sequential, or
independent strategies)............................................................................................. 88
Table 15.
Comparison of the validity of fully (or serum) integrated screening, stepwise
screening, contingent screening, and screening combining tests (combined test
and quad test) in an independent manner ................................................................. 92
Table 16.
Evidence table of primary research studies appraised investigating the accuracy
of screening carried out in first and second trimesters ............................................. 97
Table 17.
Evidence table of primary research studies appraised investigating the rate of
invasive testing with the introduction of a screening programme .......................... 142
Table 18.
Uptake of invasive testing following 1st trimester screening.................................. 161
Table 19.
Uptake of invasive testing following 2nd trimester screening ................................. 163
Table 20.
Uptake of invasive testing following 1st and 2nd trimester screening...................... 164
Table 21.
Evidence table of primary research studies examining the uptake of invasive
testing following DS screening .............................................................................. 166
Table 22.
Evidence table of secondary research studies appraised investigating the rate
of fetal loss following invasive prenatal diagnostic procedures ............................. 186
Table 23.
Evidence table of primary research studies investigating the rate of fetal loss
following invasive prenatal diagnostic procedures ................................................ 191
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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LIST OF ABBREVIATIONS AND ACRONYMS
X/12
—
Months e.g. 6/12 = 6 months
X/40
—
Weeks of gestation e.g. 10/40 = 10 weeks of gestation.
+ve
—
Positive
-ve
—
Negative
1st T
—
First trimester
2nd T
—
Second trimester
95% CI
—
95 percent confidence interval
95th centile.
—
95th percentile
AFP
—
Alphafetoprotein
AC
—
Amniocentesis
ADAM
—
A Disintegrin and Metalloprotease
AMA
—
Advanced maternal age
ART
—
Assisted reproductive technology
BPD
—
Biparietal Diameter
CI
—
Confidence interval
Cinahl

Cumulative Index to Nursing and Allied Health Literature
CRL
—
Crown-rump length
CVS

Chorionic Villus Sampling
DM
—
Diabetes Mellitus
DNA

Deoxyribonucleic acid
DR
—
Detection rate (sensitivity)
DS
—
Down syndrome
EDD
—
Expected Date of Delivery
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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ELISA
—
Enzyme-Linked ImmunoSorbent Assay
fβhCG
—
Free beta hCG (human chorionic gonadotrophin)
FASTER

First and Second Trimester Evaluation of Risk
FMF

Fetal Medicine Foundation
FmHx
—
Family History
FNR
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false negative rate
FPR
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false positive rate
GA
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Gestational age
GP
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general practitioner
hCG
—
Human chorionic gonadotrophin
HhCG
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Hyperglycosylated hCG (also called ITA)
HTA

Health technology assessment
Hx

History
INAHTA

International Network of Agencies for Health Technology Assessment
IT
—
Invasive test/testing
ITA
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Invasive trophoblast antigen (also called HhCG)
LR
—
Likelihood ratio
LMP
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Last menstrual period
MA
—
Maternal age
MeSH
—
Medical Subject Headings
MSS
—
Maternal Serum Screen
MoH
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Ministry of Health (NZ)
MoM
—
Multiple of the Median
NHS

National Health Service (UK)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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NHMRC

National Health and Medical Research Council
NT
—
nuchal translucency
NZ

New Zealand
NZHTA

New Zealand Health Technology Assessment
ONTD

Open neural tube defect
OSCAR

One stop clinic for assessment of risk
OR

odds ratio
Paeds

paediatricians
PAPP-A

pregnancy associated plasma protein
PPV

positive predictive value
QA

quality assurance
QC

quality control
RCT

randomised controlled trial
RNZCGP

Royal New Zealand College of General Practitioners
RR
—
Relative risk
SA
—
South Australia
SD

standard deviation
Se

sensitivity
Sig diff

Significantly different
Sp

specificity
SPR
—
screen positive rate
SURUSS
—
Serum Urine and Ultrasound Screening Study
T18
—
Trisomy 18
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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TA
—
Transabdominal
TC
—
Transcervical
ToP

Termination of pregnancy
ThCG
—
Total hCG
TT
—
Triple test
TV
—
Transvaginal
uE3
—
unconjugated estriol
UK

United Kingdom
USA
—
United States of America
USS
—
Ultrasound scan.
WA
—
Western Australia
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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GLOSSARY
A prior pertaining to something which is designated in advance.
Age standardisation
A procedure for adjusting rates designed to minimise the effects of
differences in age composition when comparing rates for different populations
Amniocentesis an invasive prenatal diagnostic test performed in pregnant women to identify
chromosomal abnormalities in the fetus by karyotyping. A needle is inserted into the uterus and used to
remove a small amount of amniotic fluid from the sac surrounding the fetus.
Analyte
a substance or chemical constituent that is undergoing analysis. In this report analyte
is used to refer to the serum constituent undergoing analysis, e.g. hCG
Aneuploidy Having an abnormal number of chromosomes
Ascertainment bias (detection bias)
ascertained, diagnosed or verified.
Systematic differences between groups in how outcomes were
Bias
Deviation of results or inferences from the truth, or processes leading to such deviation. Any
trend in the collection, analysis, interpretation, publication, or review of data that can lead to
conclusions that are systematically different from the truth.
Blinded study A study in which observers and/or subjects are kept ignorant of the group to which
they are assigned. When both observers and subjects are kept ignorant, the study is referred to as
double blind.
Case-control study An epidemiological study involving the observation of cases (persons with the
disease, such as cervical cancer) and a suitable control (comparison, reference) group of persons
without the disease. The relationship of an attribute to the disease is examined by comparing
retrospectively the past history of the people in the two groups with regard to how frequently the
attribute is present. See also nested case control.
Chorionic villus sampling
an invasive prenatal diagnostic test performed in pregnant women
to identify any chromosomal abnormalities in the fetus by karyotyping.. A needle is used to remove a
small amount of chorionic villus tissue from the placenta. The needle may be inserted via the cervix
(transcervical) or abdomen (transabdominal).
Cohort study
The analytic method of epidemiologic study in which subsets of a defined population
can be identified who are, have been, or in the future may be exposed or not exposed in different
degrees, to a factor or factors hypothesised to influence the probability of occurrence of a given disease
or other outcome. Studies usually involve the observation of a large population, for a prolonged period
(years), or both.
Combined test First trimester DS screening test based on combining 1st T MSS (PAPP-A, and
fβhCG) and NT with maternal age.
Confidence interval The computed interval with a given probability, e.g. 95%, that the true value of
a variable such as a mean, proportion, or rate is contained within the interval. The 95% CI is the range
of values in which it is 95% certain that the true value lies for the whole population.
Confounder
A third variable that indirectly distorts the relationship between two other variables,
because it is independently associated with each of the variables.
Contingent screening All women have first trimester screening and are divided into three groups
based on results: high, intermediate and low risk. High risk women have diagnostic test; low risk
women are reassured and have no further screening. All others have second trimester screening tests.
For these women the results of first and second trimester testing is combined to produce one integrated
result.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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Cross-sectional study
A study that examines the relationship between diseases (or other health
related characteristics), and other variables of interest as they exist in a defined population at one
particular time.
Double test
Second trimester serum screening using AFP and hCG (fβhCG or total hCG) and
incorporating maternal age
Effectiveness A measure of the extent to which a specific intervention, procedure, regimen, or
service, when deployed in the field in routine circumstances, does what it is intended to do for a
specified population.
Evidence table A summary display of selected characteristics (e.g., methodological design, results) of
studies of a particular intervention or health problem.
False negative result A negative test result in a person who does have the condition being tested for.
False positive result A positive test result in a person who does not have the condition being tested
for.
Fetal Medicine Foundation (FMF) A registered charity (London, UK) which promotes research and
training in fetal medicine
Integrated screening
Any method which integrates measurements performed during the first
and second trimester of pregnancy into a single test result.
Integrated test
Unless otherwise qualified, ‘integrated test’ refers to the integration of nuchal
translucency and PAPP-A measurements in the first trimester with the quadruple test markers in the
second trimester. It is the also known as the fully integrated test
Invasive testing
used in this case to describe prenatal diagnostic tests, e.g. amniocentesis or
chorionic villous sampling, which involve removal of tissue or fluid from the placenta or uterus.
Generalisability (applicability, external validity)
Applicability of the results to other populations.
High risk groups
Usually refers to groups of women that have been identified as having a higher
than expected, or higher than average for the population as a whole, incidence of the disease in
question.
Incidence
The number of new events (cases; e.g. of disease) occurring during a certain period, in
a specified population.
Independent screening The practice of offering women who have had first trimester Down
syndrome screening a second trimester screening test without consideration of the first trimester results
Internal validity
bias.
The extent to which the design and conduct of a study are likely to have prevented
Matching
The process of making a study group and a comparison group comparable with respect
to extraneous factors.
Mean Calculated by adding all the individual values in the group and dividing by the number of
values in the group.
Median
Any value that divides the probability distribution of a random variable in half. For a finite
population or sample the median is the middle value of an odd number of values (arranged in ascending
order) or any value between the two middle values of an even number of values.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
xv
Meta-analysis
The process of using statistical methods to combine the results of different studies.
The systematic and organised evaluation of a problem, using information from a number of
independent studies of the problem.
Misclassification The erroneous classification of an individual, a value, or an attribute into a
category other than that to which it should be assigned.
Monte Carlo simulation A method of generating values from a known distribution using a computer
simulation for the purposes of experimentation
Multiple regression
simultaneously.
Any analysis of data that takes into account a number of variables
Negative predictive value (NPV) The probability a person does not have the disease when the
screening test is negative.
Nested case control study
A case control study in which cases and controls are drawn from the
population in a cohort study. That is, the case control study is “nested” within the cohort study design
so that the effects of some potential confounding variables are reduced or eliminated. A case control
study can also be nested into a case series study. See also case control study, cohort study, and case
series study.
Nuchal translucency
subcutaneous fluid-filled space at the back of the neck of a fetus.
Observational study
A study in which the investigators do not seek to intervene, and simply
observe the course of events.
Population-based screening programme A population-based screening programme is one in which
screening is systematically offered by invitation to a defined, identifiable population.
Positive predictive value (PPV) The probability a person actually has the disease when the screening
test is positive.
Prevalence The number of events in a given population at a designated time (point prevalence) or
during a specified period (period prevalence).
Primary care
First contact, continuous, comprehensive and coordinated care provided to
individuals and populations undifferentiated by age, gender, disease or organ system.
Primary research/study ‘Original research’ in which data are collected. The term primary
research/study is sometimes used to distinguish it from a secondary study (re-analysis of previously
collected data), meta-analysis, and other ways of combining studies (such as economic analysis and
decision analysis). (Also called original study.)
Quadruple test Second trimester serum screening using AFP, hCG (fβhCG or total hCG), uE3 and
inhibin and incorporating maternal age. Also referred to as the quad test.
Randomised controlled trial An epidemiologic experiment in which subjects in a population are
randomly allocated into groups to receive or not receive an experimental preventive or therapeutic
procedure, manoeuvre, or intervention. Randomised controlled trials are generally regarded as the
most scientifically rigorous method of hypothesis testing available in epidemiology.
Recall bias
Systematic bias due to differences in accuracy or completeness of recall or memory of
past events or experiences.
Reference standard
An independently applied test that is compared to a screening or diagnostic
test being evaluated in order to verify the latter’s accuracy. A reference standard, therefore, provides
an accurate or “truth” diagnosis for verification of positive and negative diagnoses
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
xvi
Relative risk (RR)
The ratio of the risk of disease or death among the exposed to the risk among
the unexposed. It is a measure of the strength or degree of association applicable to cohort studies and
RCTs.
Reliability
The degree to which results obtained by a measurement procedure can be replicated.
Lack of reliability can arise from divergences between observers or measurement instruments,
measurement error, or instability in the attribute being measured.
Risk factor
An exposure or aspect of personal behaviour or lifestyle, which on the basis of
epidemiologic evidence is associated with a health-related condition.
Screening - Screening is the examination of asymptomatic people in order to classify them as likely or
unlikely to have the condition that is the object of screening.
Secondary care
Surgical and medical services that are generally provided in a hospital setting.
In many cases, access to these services is by referral from a primary care health professional such as a
general practitioner.
Secondary research/study Re-analysis of previously collected data, meta-analysis, and other ways
of combining studies (such as economic analysis and decision analysis)
Sequential screening Screening where results of screening in 1st trimester are combined with 2nd
trimester screening in either an independent, contingent, stepwise or integrated manner (see separate
glossary entries)
Selection bias
Any error in selecting the study population such that the people who are selected to
participate in a study are not representative of the reference population or, in analytic studies the
comparison groups are not comparable.
Sensitivity analysis A method to determine the robustness of an assessment by examining the extent
to which results are affected by changes in methods, values of variables, or assumptions.
Sensitivity (Se)
Sensitivity is the proportion of truly diseased persons in a screened population who
are identified as diseased by a screening test. Sensitivity is a measure of the probability of correctly
diagnosing a case, or the probability that any given case will be identified by the test.
Specificity (Sp) The proportion of truly non-diseased persons who are so identified by a screening
test. It is a measure of the probability of correctly identifying a non-diseased person with a screening
test.
Stepwise screening
All women have first trimester screening and are divided into two groups
based on results: high and low risk. Those with a high risk result are offered diagnostic testing. All
others have second trimester screening tests. For these women the results of first and second trimester
testing are combined to produce one integrated result.
Statistical difference A result that is unlikely to have happened by chance. The usual threshold for this
judgement is that the results, or more extreme results, would occur by chance with a probability of less
than 0.05 if the null hypothesis was true. Statistical tests produce a p-value used to assess this.
Statistical modelling
See Monte Carlo simulation
Systematic review Literature review reporting a systematic method to search for, identify and
appraise a number of independent studies.
Triple test
Second trimester serum screening using AFP, hCG (fβhCG or total hCG), and
uE3 and incorporating maternal age
Trisomy
Presence of an extra chromosome in each cell
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
xvii
True negative
A test correctly identifies a person without the condition.
True positive
A test correctly identifies a person with the condition.
Variance
A measure of the variation shown by a set of observations, defined by the sum of the
squares of deviation from the mean, divided by the number of degrees of freedom in the set of
observations.
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Chapter 1: Background
Down syndrome (DS) or Trisomy 21 is a chromosomal abnormality resulting from an extra copy of
chromosome 21. It is the most common aneuploidy in live born infants, with a population incidence of
about 1 in 1000 births. The severity of the disorder can vary but outcomes may include severe
developmental delay, congenital heart defects and physical growth impairment. There is no national
data on the prevalence of DS in New Zealand but a yearly prevalence of 1.17 /1000 births has been
reported between the years 1997-2003 (Chang, 2006).
The risk of carrying a fetus with DS has been recognised as increasing with maternal age since the
1930’s. A maternal age of 35 years or more at the expected date of delivery has been used as the basis
for DS screening since the 1970s. Women older than this age cut-off are offered prenatal diagnosis of
DS by either amniocentesis, usually from 16 weeks gestation, or chorionic villus sampling from
approximately 11 weeks gestation (Nicolaides, 2004). Each of these tests carries a risk of fetal loss and
other complications, and this method of screening has been criticised as resulting in a high number of
unnecessary invasive procedures and procedure-related fetal losses. Additionally, screening based on
maternal age alone identifies only approximately 30% of affected fetuses (Chang, 2006), as most
children with DS are born to women under 35 years of age.
Efforts to develop screening methods to identify mothers at high risk of carrying an affected fetus have
focussed on nuchal translucency (NT) thickness and maternal serum biochemistry as well as the
presence of other sonographic markers. Abnormal levels of maternal alpha-fetoprotein (AFP),
unconjugated estriol (uE3) and human chorionic gonadotropin (hCG) levels were initially noted to be
associated with the presence of DS, and the importance of two other biomarkers, Inhibin-A and
pregnancy associated placental protein A (PAPP-A), were later identified. There has been considerable
debate however regarding the best combination of screening tests and whether they should be offered
in the first or second trimester, or both.
NEED FOR SYSTEMATIC REVIEW
Overseas screening
In Australia second trimester serum screening and first trimester serum in combination with nuchal
translucency measurements are the established standards of care, and have been utilised with increasing
rates of uptake since the 1980’s (Chang, 2006; O’Leary et al. 2006). The American College of
Gynaecologists (ACOG) recommend offering invasive testing to women older than 35 years and to
women with a positive maternal serum screen result (Slack et al. 2006). In the U.K., the National
Institute for Clinical Excellence (NICE) suggests all pregnant women should be offered screening for
Downs syndrome based on methods which provide at least a 60% DR and no more than a 5% FPR.
They recommend nuchal translucency, first or second trimester maternal serum screening, or a
combination of NT and serum screening (NICE, 2003).
Current New Zealand screening
Currently New Zealand has no formalised antenatal screening programme for DS. The Royal
Australian and New Zealand College of Obstetricians and Gynaecologists (RANZCOG) recommends
offering screening or prenatal diagnosis based on maternal age or having a previous affected pregnancy
(RANZCOG 2004). It is suggested that women who are not considered to be at increased risk should
be made aware of the availability of screening. The screening methods currently recommended by
RANZCOG are nuchal translucency; first trimester combined, or second trimester screening. These
tests, however, are not available in all localities, serum screening is not available free of charge, and
consequently they have had a low uptake in New Zealand in the past (Chang, 2006). Screening is
conducted on an ad hoc basis, mostly based on ultrasound scanning. In a recent report to the National
Screening Unit (Ministry of Health) entitled “Assessment of Antenatal Screening for DS in New
Zealand” it was recommended that invasive diagnostic testing based on age and nuchal thickness
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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screening alone should be urgently reviewed, and that a national screening programme should be
implemented based on “best practice” (Stone and Austin, 2006).
The National Screening Unit has commissioned New Zealand Health Technology Assessment
(NZHTA) to undertake a systematic review to assess options for DS screening in order to inform policy
on a national screening programme.
SCREENING - GENERAL OVERVIEW
The focus of this review is secondary prevention, specifically screening. The National Health
Committee (NHC) of New Zealand defines screening as “…a health service in which members of a
defined population, who do not necessarily perceive they are at risk of, or are already affected by, a
disease or its complications, are asked a question or offered a test to identify those individuals who are
more likely to be helped than harmed by further tests or treatments to reduce the risk of disease or its
complications” (NHC, 2003, p29). The effectiveness of a screening programme depends upon high
levels of coverage of the population. Criteria to inform the assessment of screening programmes in
New Zealand have been developed by the NHC (2003). These criteria are listed in Table 1 below.
Table 1:
Criteria for assessing screening programmes
1.
The condition is a suitable candidate for screening.
2.
There is a suitable test
3.
There is an effective and accessible treatment or intervention for the condition identified through early detection
4.
There is high quality evidence, ideally from randomised controlled trials, that a screening programme is effective
in reducing mortality or morbidity.
5.
The potential benefit from the screening programme should outweigh the potential physical and psychological
harm (caused by the test, diagnostic procedures and treatment).
6.
The health care system will be capable of supporting all necessary elements of the screening pathway, including
diagnosis, follow-up and programme evaluation.
7.
There is consideration of social and ethical issues.
8.
There is consideration of cost-benefit issues.
The scope of this review is narrow and limited to partially addressing criterion two, and criteria five
and six.
AIM
To systematically identify and appraise international evidence for the antenatal use of technologies and
screening strategies for DS.
REVIEW SCOPE
The review scope was developed in consultation with the Director of the NZHTA and the National
Screening Unit.
There are two parts to the review. Part A is concerned with the validity of DS screening methods and
with any difficulties implementing screening strategies. Part B is concerned with the impact of
screening on amniocentesis and chorionic villus sampling, and the safety of these procedures.
For Part A, studies were included for appraisal if they reported comparisons of the DR and FPR of
screening using any of the following screening methods: maternal age, first trimester serum screening,
first trimester nuchal translucency screening, second trimester serum screening, or screening combining
the results of 1st and 2nd trimester screening (Cuckle et al. 2005). The scope also includes any
difficulties implementing any of the screening strategies. These difficulties include: successful
measurement, limitations of access, quality control issues, reliability of different strategies, and
incomplete application of screening strategies.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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For Part A, the search was limited to full reports published in English and published between January
2000 and 29 June 2006. Full details of inclusion and exclusion criteria are provided in the next chapter.
For Part B, studies were included for review if they reported the proportion of women tested by
amniocentesis and chorionic villus sampling after different DS screening results, how the introduction
of DS screening programmes impacted on testing rates, what proportion of fetal loss is associated with
testing, and what interventions are available that reduce the risk of fetal loss from these procedures.
The search was limited to full reports published in English and published between January 2000 and
7th August 2006. Full details of inclusion and exclusion criteria are provided in the next chapter.
REVIEW QUESTIONS
Part A
1.
What is the case DR for a given FPR resulting from antenatal screening for DS for the following
screening strategies/combinations of tests:
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maternal age (MA)
first trimester serum screening
second trimester serum screening
first trimester nuchal translucency screening
integrated first and second trimester screening
sequential first and second trimester testing: Independent screening
sequential first and second trimester testing: Stepwise and contingent screening.
2.
What difficulties have been experienced in the implementation of any of the following screening
strategies/combinations of tests:
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maternal age
first trimester serum screening
second trimester serum screening
first trimester nuchal translucency screening
integrated first and second trimester screening
sequential first and second trimester testing: independent screening
sequential first and second trimester testing: stepwise and contingent screening.
Part B
3.
In relation to amniocentesis and chorionic villus sampling for the detection of DS:
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what proportion of women are tested by amniocentesis or CVS following receipt of a high risk
result on screening
what proportion of women are tested by amniocentesis or CVS following receipt of a low risk
result on screening
what proportion of women are tested by amniocentesis or CVS without having had a screening test
what impact does the introduction of a screening programme have on testing rates
what is the proportion of fetal loss associated with testing
what interventions are available that reduce the risk of fetal loss from testing.
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DOWN SYNDROME SCREENING METHOD TERMINOLOGY
The terms used in the literature to describe Down syndrome screening methods that use both first and
second trimester screening tests vary. Some refer to all these methods as sequential methods (Cuckle et
al. 2005). Others refer to only the stepwise and the contingent screening methods as sequential
methods, i.e. excluding the integrated test (Malone et al. 2005). In some papers the “stepwise” strategy
is known as the “sequential” strategy (Palomaki et al. 2006).
We have chosen to adopt the terminology of the FASTER study (Malone et al. 2005) and SURUSS
(Wald et al. 2003b). Any method combining the results of tests taken in the first and second trimesters
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
4
into one test (with first trimester results held until completion of second trimester testing) is an
integrated screening method (fully integrated or serum integrated). A screening method which discloses
and acts upon the results of first trimester screening, and then offers a proportion of women (based on
risk cut-offs) a second trimester screening test is termed sequential screening. Sequential screening
strategies describe both stepwise and contingent screening methods.
The terminology does have some drawbacks. The peer reviewer of this document has highlighted the
fact that sequential screening methods offer an integrated test to women who have second trimester
screening. However, it may be confusing to use the overarching term “integrated screening”, as well as
having an “integrated test”.
Table 2 describes the four conventional screening methods that combine information from both first
and second trimester screening tests.
Table 2:
Down syndrome screening methods that use both first and second trimester screening
tests
Screening method
(overarching term)
1st Trimester
tests
2nd Trimester tests
Description of screening strategy
Serum integrated
(integrated)
PAPP-A
Quad test
All women have first and second trimester screening
tests. Results are held until completion of second
trimester screening when all results are combined
into one result
Fully integrated or
integrated test
(integrated)
NT and PAPP-A
Quad test
All women have first and second trimester screening
tests. Results are held until completion of second
trimester screening when all results are combined
into one result.
Stepwise (sequential)
Combined test
Quad test
All women have first trimester screening and are
divided into two groups based on results: high and
low risk. Those with a high risk result are offered
diagnostic testing. All others have second trimester
screening tests. For these women the results of first
and second trimester testing are combined to
produce one integrated result.
Quad test
All women have first trimester screening and are
divided into three groups based on results: high,
intermediate and low risk. High risk women have
diagnostic test; low risk women are reassured and
have no further screening. All others have second
trimester screening tests. For these women the
results of first and second trimester testing is
combined to produce one integrated result.
(NT, PAPP-A, and
either fβhCG or
total hCG)
Contingent (sequential)
Combined test
(NT, PAPP-A, and
either fβhCG or
total hCG)
In addition, sometimes a screening method employs the same strategy as a conventional integrated or
sequential screening method but different tests are used. For instance, measuring NT in the first
trimester and then offering those with a high risk result a diagnostic test, and those with a low risk a 2nd
trimester double test. This method uses the same strategy as the stepwise screening method and in this
review this is described as combining tests in a “stepwise manner”.
In some appraised studies women were offered a first trimester screening test then women who were
screen negative were offered a second trimester screen without consideration of the first trimester
results. This practice of combining tests in an independent manner leads to erroneous risk estimates
(Wald 2006c) and is not recommended.
For definitions of all other Down syndrome screening methods please refer to the glossary.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
5
STRUCTURE OF REPORT
This report is divided into two Parts (A and B) and chapters. Chapter 2 (Review Methodology) includes
the selection criteria (study inclusion and exclusion criteria), the search strategy, and outcomes
considered for Part A and Part B of the report.
The results section of the review includes primary and secondary research considered for Part A
(Chapters 3, 4 and 5) and Part B (Chapters 6, 7, and 8) of the review. This section also provides an
overview of the appraised papers and evidence, as well as detailed evidence tables, which present each
appraised study’s methods, results, limitations, and authors’ conclusions. Chapter 9 (Discussion)
summarises results, briefly discusses methodological limitations in the area, and presents key
conclusions.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
7
Chapter 2: Review Methodology
SELECTION CRITERIA
PART A: Review questions 1 and 2
Study inclusion criteria
Publication type
Studies published between January 2000 and June 2006 inclusive, in the English language, including
primary (original) research (published as full original reports) and secondary research (systematic
reviews and meta-analyses) appearing in the published literature.
Context
Studies reporting on the comparison of the diagnostic accuracy of two screening strategies. Screening
strategies included maternal age, first trimester serum screening, first trimester nuchal translucency
screening, second trimester serum screening, and sequential or integrated screening.
Outcomes
Measures of case DRs for a given FPR are presented in the results as well as any implementation
difficulties. Implementation difficulties include unsuccessful measurement, limitations of access to the
screening test, quality control issues in conducting the test, reliability of different screening strategies
and incomplete application.
Study design
Systematic reviews or primary research comparing different screening strategies.
Sample size
Studies with samples of at least 100 participants.
Study exclusion criteria
Research papers were excluded if they:
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were not published in English
were “correspondence”, editorials, expert opinion articles, non-systematic reviews, conference
proceedings, or abstracts
reported animal studies
did not clearly describe their methods and results, or had significant discrepancies
had been superseded by a later publication with longer follow-up data and overlap in the patient
population.
PART B: Review question 3
Study inclusion criteria
Publication type
Studies published between January 2000 and August 7th 2006 inclusive, in the English language,
including primary (original) research (published as full original reports) and secondary research
(systematic reviews and meta-analyses) appearing in the published literature.
Context
Studies reporting the proportion of women tested by amniocentesis and chorionic villus sampling
following receipt of either a low risk or high risk result, and the proportion of women having these
procedures without antenatal DS screening. Also, studies reporting the impact of the introduction of a
screening programme on testing rates, studies reporting the proportion of fetal loss associated with
testing, and studies describing interventions that reduce the risk of fetal loss from these procedures.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
8
Outcomes
The proportion of women opting for invasive testing as a function of their screening result, the change
in overall proportion of tests with the introduction of a screening programme, proportion of fetal loss in
women who have an invasive test and those who do not, changes in the rate of fetal loss as a result of
risk factors.
Study design
Systematic reviews, randomised controlled trials, cohort studies, case control studies, cross sectional
studies and before and after designs.
Sample size
Studies with samples of at least 100 participants.
Study exclusion criteria
Research papers were excluded if they:
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were not published in English
were “correspondence”, editorials, expert opinion articles, non-systematic reviews, conference
proceedings, abstracts
reported animal studies
did not clearly describe their methods and results, or had significant discrepancies
had been superseded by a later publication with longer follow-up data and overlap in the patient
population.
SEARCH STRATEGY
A systematic method of literature searching and selection was employed in the preparation of this
review.
Searches were limited to English language material published from January 2000 onwards. The
searches were completed on 29th June and 7th August, 2006 for Part A and Part B respectively.
Principal sources of information
The following databases were searched (using the search strategy outlined in Appendix 1):
Bibliographic databases
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Cinahl
Cochrane Register of Controlled Trials
Current Contents
Embase
Medline
PubMed (last 60 days)
Science Citation Index
Social Science Citation Index
Review databases
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ACP Journal Club
Cochrane Database of Systematic Reviews
Database of Abstracts of Reviews of Effectiveness
Health Technology Assessment database
NHS Economic Evaluation database
Other
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Clinicaltrials.gov
Current Controlled Trials
References of retrieved papers were scanned for relevant publications.
TRIP database
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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UK National Screening Committee Down’s Syndrome Screening Programme
Hand searching of journals, contacting of manufacturers, or contacting of authors for unpublished
research was not undertaken in this review. A complete list of the sources searched for this review is
given in Appendix 2.
Search terms used: Review questions 1 and 2
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Index terms from Medline (MeSH terms): Down syndrome, pregnancy trimester-first, nuchal
translucency measurement, pregnancy trimester-second, exp prenatal diagnosis, pregnancyassociated plasma protein-A, chorionic gonadotropin-beta subunit-human, alpha-fetoproteins,
estriol-blood, inhibins-blood, ultrasonography-prenatal, maternal age, mass screening, false
positive reactions, false negative reactions.
Index terms from Embase: Down syndrome, fetus echography, first trimester pregnancy, second
trimester pregnancy, maternal serum, alpha fetoprotein, inhibin A, maternal age, exp prenatal
diagnosis, pregnancy associated plasma protein A, chorionic gonadotropin beta subunit, screening
test, mass screening, prenatal screening, screening.
The above index terms were used as keywords in databases where they were not available and in
those databases without controlled vocabulary.
Additional keywords (not standard index terms) were used in all databases: trisomy 21, papp-a,
beta hcg, uE3, unconjugated estriol, unconjugated oestriol, inhibin a, afp, ((integrated or sequential
or contingent or step-wise) adj (screen$ or test$)), screen$, test$.
Non English language references, letters and news items were excluded using database limits
where available.
Filters for study design were not used in the search in order to retrieve a wider range of references
from which the final selection of studies could be made.
Search terms used: review question 3
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Index terms from Medline (MeSH terms): Down syndrome, chromosomes-human-pair-21,
trisomy, amniocentesis, chorionic villi sampling, karyotyping.
Index terms from Embase: Down syndrome, trisomy 21, amniocentesis, chorion villus sampling,
karyotyping, fetus karyotyping.
The above index terms were used as keywords in databases where they were not available and in
those databases without controlled vocabulary.
Additional keywords (not standard index terms) were used in all databases: trisomy 21, chorionic
vill$,.
Non English language references, letters and news items were excluded using database limits
where available.
Filters for study design were not used in the search in order to retrieve a wider range of references
from which the final selection of studies could be made.
STUDY SELECTION
Studies were selected for appraisal using a two-stage process. Initially, the titles and abstracts (where
available) identified from the search strategy, were scanned and excluded as appropriate. The full text
articles were retrieved for the remaining studies and these were appraised if they fulfilled the study
selection criteria outlined above.
PART A: Review questions 1 and 2
There were 1138 studies identified by the search strategy. 219 full text articles were obtained after
excluding studies from the search titles and abstracts. A further 153 of these full text articles did not
fulfil the inclusion criteria and are presented in Appendix 3. Reasons for rejecting these papers for
appraisal are:
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outcomes did not include a comparison of two or more screening methods (74)
methods were not fully described (2)
papers were either a letter (1), or comment (12)
non-systematic review (3)
data in the study was superseded (1)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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sample size less than 100 (3)
did not fit the scope of the review for other reasons (could not extract DR and FPR from paper,
screening methods were outside the scope of the review) (57).
Therefore, 66 articles were fully appraised and are included in this report. Along with other cited
publications (e.g. those providing background material), these are presented in the References.
PART B: Review question 3
There were 1116 studies identified by the search strategy. 191 full text articles were obtained after
excluding studies from the search titles and abstracts. A further 156 of these full text articles did not
fulfil the inclusion criteria and are presented in Appendix 4. Reasons for rejecting these papers for
appraisal are:
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outcomes did not include the proportion of invasive tests requested or performed (41)
methods were not fully described (5)
papers were either a letter (1), or comment (24)
non-systematic review (3)
data in the study was superseded (6)
sample size less than 100 (8)
uncontrolled study (9)
did not fit the scope of the review for other reasons (screening methods were outside the scope of
the review, cost-effectiveness analysis of effect of invasive testing) (59).
Therefore, 35 articles were fully appraised and are included in this report, and presented in the
References.
APPRAISAL OF STUDIES
The evaluation initially classified studies according to National Health and Medical Research Council
(NHMRC, 2000) levels of evidence criteria, so as to rank them in terms of quality according to a predetermined “evidence hierarchy” (see Appendix 5). These evidence levels are only a broad indicator
of the quality of the research. The levels describe groups of research which are broadly associated with
particular methodological limitations.
However, these levels are only a general guide to quality because each study may be designed and/or
conducted with particular strengths and weaknesses. High level evidence is provided by a well
conducted randomised-controlled trial. NHMRC checklists of quality issues to consider in appraising
research studies were also used relevant to study design.
Summaries of appraisal results are shown in tabular form as Evidence Tables and include:
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source reference (authors, publication date) and country where study was principally conducted
study setting
design
evidence level (applying NHMRC criteria)
description of screening strategies
sample (patient characteristics including number of women and patient inclusion and exclusion
criteria)
eligible outcome measures used and verification of outcomes
results of analyses on eligible outcomes, including statistically tested comparisons and reporting
relevant statistical data
comments on the study’s limitations relevant to its internal and external validity
authors’ conclusions
reviewer’s conclusions.
Conclusions are drawn based on the study design and the specific problems associated with individual
studies.
Systematic reviews are described and critiqued in terms of their search strategy, inclusion/exclusion
criteria, data synthesis and interpretation. Note: that such papers were considered principally as
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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background information as they invariably do not use the same selection criteria as this review and do
not consider subsequently published research.
KEY OUTCOME MEASURES FOR PRIMARY STUDIES
Assessment of validity of a diagnostic or screening test
The diagnostic or screening test performance includes consideration of validity of the test. In the
context of screening for DS, the outcome measures of choice for the assessment of predictive
performance are the case DR and the FPR. The case DR is the proportion of women with Down’s
syndrome pregnancies who have positive results and is therefore equivalent to the sensitivity. The FPR
is 1-specificity.
These measures are calculated based on presentation of results as shown in Table 3.
Table 3.
Assessment of validity of a diagnostic test
Reference test
Diagnostic test
Positive
Negative
Total sample size
Positive
Negative
a
b
c
d
n1
n2
Based on Table 3, measures of validity, and 95 percent confidence intervals, were calculated using the
following formulae:
Sensitivity
= a/(a+c)
= a/n1
Confidence interval for sensitivity: p ± 1.96(pq/n1)1/2
Where p = a/(a+c)
q = c/(a+c)
FPR
= b/(b+d)
= b/n2
Confidence interval for FPR: p ± 1.96(pq/n2)1/2
Where p = b/(b+d)
q = b/(b+d)
If either n*p or n(1-p) was less than five, confidence intervals based on the normal approximation to
the binomial distribution, using the formulae above were considered unreliable and exact methods
based on the binomial distribution were used to calculate the confidence interval. Stata version 7.0 was
used for these calculations.
Assessment of quality
Assessment of quality was based on internationally accepted criteria (Irwig and Glaziou 1996; Irwig et
al. 1994; Jaeschke et al. 1994). These were:
ƒ
there was an independent blind comparison with a reference gold standard;
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
12
ƒ
ƒ
ƒ
ƒ
the results of the test and reference standard were assessed independently of each other;
the sample of patients in the study included an appropriate spectrum of patients similar to those in
whom the test is likely to be used in New Zealand;
the results of the test being evaluated did not influence the decision to perform the standard
reference test (verification bias); and
there was sufficient detail in the study report to permit replication of the test.
For most studies of the performance of DS screening the choice of reference standard depends on the
results of the screening test. Those with a positive screen will be offered an invasive diagnostic test
with either CVS or amniocentesis, and where the screen is negative infants will normally undergo a
paediatric examination to exclude DS. Therefore, the comparison with a reference standard will not be
an independent blinded comparison and there may be verification bias. As this is the case for the
majority of studies it has not been included as a limitation unless there are few details given of the
efforts to determine outcomes in live infants.
It should be noted however that the difference in timing of the application of the reference standard
makes it difficult to accurately determine the validity of antenatal DS screening methods. DS cases
detected by screening are detected earlier (usually in 1st or 2nd trimester) than those missed by screening
(at term), and DS fetuses are more likely to miscarry than unaffected fetuses. Many DS pregnancies
detected by screening and having a termination of pregnancy would have miscarried if they had not
been screened, and some DS pregnancies not detected by screening will not be known to investigators
as they will have spontaneous fetal loss (Wald et al. 2003b). Also, screening markers may
preferentially detect DS cases which are likely to miscarry. Results of studies that determine the
performance of screening at 1st trimester or 2nd trimester will have higher DRs than those based on
detecting all DS cases at term (Wald et al. 2003b). In reality this later situation will not occur as it
would require an observational study which would be unethical (Wald et al. 2003b).
Limitations of the review
This study has used a structured approach to review the literature. However, there were some inherent
limitations with this approach. Namely, systematic reviews are limited by the quality of the studies
included in the review and the review’s methodology.
This review has been limited by the restriction to English language studies. Restriction by language
may result in study bias, but the direction of this bias cannot be determined. In addition, the review has
been limited to the published academic literature, and has not appraised unpublished work. Restriction
to the published literature is likely to lead to bias since the unpublished literature tends to consist of
studies not identifying a significant result.
Papers published pre-2000 were not considered as these were thought to predate current DS screening
strategies.
The studies were initially selected by examining the abstracts of these articles. Therefore, it is possible
that some studies were inappropriately excluded prior to examination of the full text article. However,
where detail was lacking or ambiguous, papers were retrieved as full text to minimise this possibility.
This review was confined to an examination of the technical aspects of screening and diagnostic testing
and did not consider the acceptability, or any ethical, economic or legal considerations associated with
these interventions. Interventions were not assessed in terms of their impact on general quality of life.
No studies included in this review were conducted in New Zealand, and therefore, their applicability to
the New Zealand population and context may be limited and needs to be considered. However, as this
review was concerned with evidence around diagnostic accuracy and technical aspects of screening and
diagnostic testing, rather than wider issues which may be influenced by national characteristics, the
evidence should be mostly applicable to the New Zealand situation.
Although two researchers appraised the articles included in this review they did not cross validate the
data extraction and appraisal process.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
13
The review scope was developed with the assistance of National Screening Unit staff at the Ministry of
Health. It had the goal of providing information that would inform the policy process in determining
whether a national antenatal screening programme for DS should be implemented in New Zealand, and
if so which screening strategy should be used.
This review was conducted over a limited timeframe (June, 2006 to December, 2006).
This review has greatly benefited from the advice provided by the consultant peer reviewer. However,
it has not been exposed to wider peer review.
For a detailed description of interventions and evaluation methods, and results used in the studies
appraised, the reader is referred to the original papers cited.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
14
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
15
Chapter 3: Accuracy of First
Trimester Screening Strategies
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY
The search identified 27 eligible papers comparing the accuracy of first trimester screening strategies,
including single and combined test options. Below is an overview of study designs and aspects of
quality represented by these studies.
Full details of the papers appraised, including methods, key results, limitations and conclusions, are
provided in evidence Table 10 (pages 24-61). Studies with directly observed DRs and FPRs are
presented first, followed by studies where the results are estimations of performance using statistical
modelling. For each of these two groups of papers, studies are presented in chronological order of
publication within the table.
Study design, and grading
Of the 27 papers comparing first trimester screening all were based on primary research; there were no
papers based on secondary research that fitted the inclusion and exclusion criteria of the review
protocol. Twenty papers reported directly observed (or age standardised) performance, and seven
reported DRs and FPRs estimated by statistical modelling using Monte Carlo simulation.
Most DS screening strategies use a degree of statistical modelling to determine an individual’s risk.
Each marker level is converted to a multiple of the gestational age specific median (MoM) of
unaffected pregnancies (either from the study population or meta-analysis), and the likelihood ratio
(LR) is calculated from the overlapping multivariate Gaussian distributions of affected and unaffected
pregnancies (Cuckle 2003; Nicolaides 2004). The LR for each screening test is combined with the a
priori risk (maternal age specific risk of DS) to produce a risk estimate for each individual, which
becomes the result of the screening method (Morris and Wald 2005). A risk level cut-off is then used to
determine whether the screening result is positive or negative and hence the DR and FPR of the
particular screening method (Morris and Wald 2005).The accuracy of the risk estimate depends on the
parameters used in the model: the means, standard deviations, and correlation coefficients (Cuckle
2003). It is important that these parameters are obtained from meta-analysis of published results with
tailoring of variances and covariances to the local population (Cuckle 2003). This is especially true for
the parameters of unaffected pregnancies as individual studies will have a relatively small number of
cases.
Another use of statistical modelling is to estimate screening performance of different screening
strategies (Cuckle 2003). The papers described in this review as statistical modelling papers, use Monte
Carlo simulation to sample from the Gaussian distributions to estimate screening performance.
Of the 20 papers reporting directly observed performance, eighteen were cohort studies and two of
these were retrospective cohort studies (O'Leary et al. 2006; Spencer et al. 2003b). The sample sizes in
the cohort studies of routinely screened women ranged from 1836-30,564. A study of twin pregnancies
had a sample size of 200 (Gonce et al. 2005).
There were two case-control studies. One was a nested case-control study with a sample size of 139
(Marsk et al. 2006). The other case-control study had a sample size of 463 (Hallahan et al. 2000).
While all these studies were graded III-2 as per NHMRC, the ideal design for determining the DR and
FPR of a screening strategy is a large prospective cohort (or nested case-control) study where all
women receive all screening methods being considered (Deeks 2001). Case-controls studies (other than
nested case-control studies) that recruit healthy participants without the disease, separately from cases,
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
16
will overestimate validity when compared to cohort studies with populations representative of a
routinely screened population (Deeks 2001).
Study setting and samples
The proportion of DS in the cohort studies of routinely screened women ranged from 0.14-0.95%.
While none of these studies were restricted to women of advanced maternal age or younger women,
there were variations in the maternal age distribution between studies. One paper screened women
attending a prenatal diagnosis centre and about half were having amniocentesis for AMA or other risk
factors (De Biasio et al. 2001). The paper had a relatively high mean maternal age (31 yrs + 8 months)
and a high proportion of DS in the sample (0.87%). As maternal age is associated with DS, studies in
populations with a larger proportion of older women may produce higher DR than studies in the
general population. For the results to be applicable to a given population the maternal age distribution
of the population in the study should be similar to that of the population in question. Note also that the
proportion of DS relates to DS detected in the 1st trimester and will be larger than that detected in 2nd
trimester or at term (because of the increase in spontaneous fetal loss in DS pregnancies).
Both of the case-control studies excluded cases of chromosomal disorders other than DS. The
proportion of DS in the nested case-control study was 22%, and in the other case-control study was
13.6%.
The majority of studies excluded multiple births. One study specifically looked at twin pregnancies
(Gonce et al. 2005), and one included twins in the analysis (Soergel et al. 2006). The issue of DS
screening in twin pregnancies (or multiples) is particularly important as twin pregnancies increase with
maternal age and assisted reproductive technology (ART) pregnancies are also more common with
advanced maternal age (Gonce et al. 2005). Screening for DS in twins is difficult as serum screening
does not provide an individual risk for each twin, and the serum results of an unaffected twin may
“normalise” the results of an affected twin (Gonce et al. 2005). It is especially important for screening
methods to be accurate as there is an increased chance of miscarriage with invasive diagnostic testing
(Gonce et al. 2005).
Only one study included screening in primary care (Niemimaa et al. 2001). Three of the single centre
studies were in university hospitals (Gonce et al. 2005; Soergel et al. 2006; Wojdemann et al. 2005).
These studies may produce results which are difficult to reproduce in regional hospital settings,
particularly where the screening strategy includes measurement of NT. As seen in the results section
(Difficulties implementing any of the screening strategies) it is important for NT to be measured in a
setting with high quality equipment, well conducted quality control programmes and staff who are
highly trained and who undergo regular audit.
Comparison screening methods
The screening methods compared in this chapter are:
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
MA as a screening test (cut-off ≥35 years unless specified)
PAPP-A
free βhCG (fβhCG)
total hCG (where papers include “hCG” this is assumed to be total hCG)
combination of PAPP-A + fβhCG (or total hCG)
NT measurement
combined test (NT, and PAPP-A + fβhCG)
ADAM12 (A Disintegrin and Metalloprotease 12)
Hyperglycosylated hCG (Hhcg) or Invasive Trophoblast Antigen (ITA)
AFP
repeat measures of PAPP-A and fβhCG at 10/40 and at 12/40
unless otherwise stated all screening strategies incorporate the individual’s maternal age.
All papers in this chapter used conventional methods to combine maternal age specific risks and
marker levels (LRs) to determine an individuals risk and therefore the DR and FPR (i.e. using
multivariate Gaussian distributions as described above).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
17
Outcomes
Where a large number of results for different risk cut-offs, fixed FPRs or DRs have been reported (e.g.
for modelling papers), a fixed FPR of 5% and/or a fixed DR of 85% have been selected for the
evidence table as this is the convention for reporting DS screening test performance. While studies
report DR for fixed FPR, in reality the cut-off chosen for screening programmes is an individual risk
(Benn and Donnenfeld 2005).
The majority of cohort studies include other chromosomal disorders as unaffected cases. In this way
their screening results will either be false positives or true negatives. While these cases are not strictly
false positives (as a positive screen is clinical relevant), for the purpose of this review and where it was
possible, figures were recalculated to include this subpopulation in the “unaffected” group (von
Kaisenberg et al. 2002).
PRIMARY RESEARCH: STUDY RESULTS
Accuracy of screening methods
Maternal age
Nine studies had results for maternal age alone as a screening test (see Table 4). In most studies,
maternal age was clearly inferior to the other strategies used. The exceptions were one study where
βHCG had a lower DR than maternal age for a fixed 5% FPR (Montalvo et al. 2005) and one other
study where maternal age had a higher DR but also a higher FPR than fβHCG alone and PAPP-A alone
(von Kaisenberg et al. 2002). Therefore, the comparative performance of maternal age and free βHCG
alone and PAPP-A alone was not clear in the latter study. Overall, the literature supported the low
predictive performance of maternal age compared with other screening strategies in the first trimester.
Table 4.
Comparison of DRs and FPR, maternal age versus other screening strategies
Reference
(Gasiorek-Wiens et al.
2001)
(Schuchter et al. 2002)
(von Kaisenberg et al.
2002)
(Wapner et al. 2003)
(Scott et al. 2004)
(Avgidou et al. 2005)
(Montalvo et al. 2005)
Test
MA
NT
MA
NT MoM >95%centile
NT + MA (MoM)
Combined
MA
NT
FβHCG
PAPP-A
Combined
MA
FβHCG + PAPP-A
NT
Combined
MA
FβHCG + PAPP-A
NT
combined
MA
NT
Combined
MA
PAPP-A
βHCG
NT
Combined
DR (%), (95% CI)
66.7
79.5
64.3
57.1
71.4
85.7
52.6
73.7
15.8
26.3
84.2
32.8
67.2
68.8
78.7
80
80
100
100
31.5
81.6
90.3
21.1
47.4
10.5
63.2
78.9
(60-73)
(74-85)
(39.1-89.4)
(31.3-83)
(30.2-75.1)
(53.9-93.5)
(6.5-46.1)
(66.3-88.1)
(24.6-37.6)
(76.2-87.0)
(86.2-94.5)
(6.1-45.6)
(24.9-69.8)
(1.3-33.1)
(41.5-84.9)
(60.6-97.3)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
FPR (%), (95% CI)
35.7 (35.0-36.3)
6.0 (5.7-6.3)
12.8
4.8 (4.2-5.4)
10
5 (4.5-5.7)
35.7 (34.1-37.2)
4.8 (4.1-5.5)
4.7 (4.0-5.3)
4.6 (3.9-4.3)
6.6 (5.8-7.5)
5
5
5
5
29
19
5.7
7.2
5
5
5
5
5
5
5
5
18
Table 4.
Comparison of DRs and FPR, maternal age versus other screening strategies
(continued)
Reference
(Soergel et al. 2006)
(Marsk et al. 2006)
Test
MA
NT
FβHCG + PAPP-A
Combined
MA
NT
Combined
DR (%), (95% CI)
63.6
81.8
87.5
87.5
67
94
94
(30.8-89.1)
(48.2-97.7)
(47.3-99.7)
(47.3-99.7)
(51-84)
(79-99)
(79-99)
FPR (%), (95% CI)
28.3
5.1
15.4
4.0
37
20
7
(27-30)
(4.3-6.0)
(13.8-16.9)
(3.2-4.8)
(28-46)
(13-28)
(2-12)
Combined versus NT and combined versus FβHCG + PAPP-A
Twenty-three studies were identified that included the combined test (fβhCG, PAPP-A and NT) and
had comparisons with NT and/or fβHCG + PAPP-A. These comparisons took different forms. In nine
studies, the DR for each screening strategy was presented for a 5% FPR. These results are summarised
in Table 5. The combined strategy consistently had a higher DR for the fixed FPR compared with the
two alternative strategies. It should be noted that in some of these studies there were a wide range of
other tests included. For studies in this table no conclusion could be made for the comparison of 1st
trimester MSS compared with NT.
Table 5.
Comparison of DRs for a 5% FPR, combined test, nuchal translucency and fβhCG +
PAPP-A
Reference
(Krantz et al. 2000)
(Crossley et al. 2002)
(Spencer et al. 2003b)
(Wapner et al. 2003)
(Avgidou et al. 2005)
(Montalvo et al. 2005)
(Gyselaers et al. 2005)
(Spencer et al. 2002)
(Palomaki et al. 2005)
Test
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Modelled
Combined
FβHCG + PAPP-A
NT
Modelled
Combined
FβHCG + PAPP-A
NT
DR (%) for 5% FPR (95% CI)
91
63
74
82 (65-93)
55 (39-70)
54 (37-71)
92 (74-99)1
68 (50-86)
76 (59-93)
78.7 (66.3-88.1)
67.2
68.8
90.3 (86.2-94.5)
Not given
81.6 (76.2-87.0)
78.9 (60.6-97.3)
Not given
63.2 (41.5-84.9)
73.6 (56.0-90.1)
61.5 (42.8-80.2)
42.3 (23.3-61.3)
88.9
69.5
73.5
84
67
Not given
In 15 studies a fixed cut off was used for the different tests, resulting in variation in both the DR and
the FPR. These studies are summarised in Table 6. The results presented in this table were also
consistent with improved performance of the combined strategy. For example, the DR of combined
screening was higher than or the same as that for fβHCG + PAPP-A while at the same time the FPR
was lower in the combined screening strategy in all 10 studies where this information was available.
When comparing the combined strategy with NT alone the DR of combined screening was higher than
or the same as that for NT testing while at the same time the FPR was lower in the combined screening
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
19
strategy in nine studies where this information was available. In four studies with estimates for
combined screening and NT the results were more difficult to interpret given a higher DR but also a
higher FPR from combined screening. In one study the combined and NT strategies had the same DR
(100%) but the combined strategy had a higher FPR (7.2% versus 5.7%), (Scott et al. 2004). In this
study there were only 5 cases of DS so the estimated DR may not be accurate. Also the median PAPPA was 0.88 MoM rather than 1 which will have increased the FPR for combined test. Once again it was
not possible to determine whether 1st (MSS) or NT has a better performance.
Table 6.
Comparison of DRs and FPR for fixed cut offs (same for all tests unless indicated),
combined test, nuchal translucency and fβhCG + PAPP-A
Reference
(De Biasio et al. 2001)
(Niemimaa et al. 2001)
(Schuchter et al. 2002)
(von Kaisenberg et al. 2002)
(Muller et al. 2003a)
(Wapner et al. 2003)
(Scott et al. 2004)
(Wojdemann et al. 2005)
(Gonce et al. 2005)
(Gyselaers et al. 2005)
(Soergel et al. 2006)
(Marsk et al. 2006)
(O'Leary et al. 2006)
(Christiansen and Olesen Larsen
2002)
(Christiansen and Jaliashvili
2003)
Test
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined (1:300)
FβHCG + PAPP-A
NT ≥ 95th centile
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Combined
FβHCG + PAPP-A
NT
Modelled
Combined
FβHCG + PAPP-A
NT
Modelled
Combined
FβHCG + PAPP-A
NT
DR (%), (95% CI)
87 (62-98)
69
62
80 (28-99)
75 (35-97)
60 (15-95)
85.7
Not given
71.4
84.2
Not given
73.7 (53.9-93.5)
73 (56-90)
69 (51-87)
62 (43-80)
85.2 (73.8-93.0)
85.2
82
100
80
100
91 (58.7-99.8)
73 (39-93.4)
75 (42.8-93.4)
100 (29-100)
Not given
100 (16-100)
80.8 (66-96)
80.8 (66-96)
42.3 (23-61)
87.5 (47.3-99.7)
87.5 (47.3-99.7)
81.8 (48.2-97.7)
94 (79-99)
Not given
94 (79-99)
83 (74-93)
85 (76-94)
73 (62-85)
FPR (%), (95% CI)
3.3 (2.5-4.1)
4.5
6.7
8.3 (6.9-9.6)
9.7 (8.5-11.0)
11.6 (10.0-13.2)
5 (4.5-5.7)
Not given
10
6.6 (5.8-7.5)
Not given
4.8 (4.1-5.5)
4.7 (4.1-5.3)
8 (7.3-8.7)
5 (4.4-5.6)
9.4 (8.8-10.1)
23.2
11.9
7.2
19
5.7
2.1 (1.8-2.5)
8.8 (8.1-9.5)
1.8 (1.5-2.1)
5.1 (0.7-9.5)
Not given
14.3 (7.4-21.2)
8.6 (
16.8 (16.1-17.4)
4.8 (4.5-5.2)
4.0 (3.2-4.8)
15.4 (13.8-16.9)
5.1 (4.3-6.0)
7 (2-12)
Not given
20 (13-28)
3.7 (3.5-4.0)
11.5 (11.1-11.9)
8.6 (8.2-8.9)
85.5
Not given
74.0
4.4
Not given
5.7
85.9
75.5
Not given
2.7
5.3
Not given
Other studies included results on the FPR given an 85% DR (see Table 7). These provide similar
predictive performance information to that provided by the DR for a given FPR. Specifically, if
combined has a higher DR than FβHCG + PAPP-A when both have a FPR of 5% then we would
expect the combined strategy to have a lower FPR than FβHCG + PAPP-A when the DR is fixed at
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
20
85% for both. Combined testing showed the best performance characteristics (compared with NT alone
and fβHCG + PAPP-A) in the four studies where this information was provided. Note, however, all
four of these studies were included in Table 5 so this is not telling us anything more about the
predictive performance compared with the data in Table 5.
Table 7.
Comparison of FPRs for an 85% DR, combined test, nuchal translucency and fβhCG
+ PAPP-A
Reference
Test
(Krantz et al. 2000)
Combined
1.4
FβHCG + PAPP-A
6.8
NT
3.4
(Avgidou et al. 2005)
FPR for an 85% DR
Combined
FβHCG + PAPP-A
2.9
NT
(Montalvo et al. 2005)
Combined
FβHCG + PAPP-A
8.2
(7.8-8.4)
8.6
(7.8-9.4)
Not given
65
NT
(Palomaki et al. 2005)
(2.7-3.0)
Not given
(64.0-66.4)
Modelled
Combined
5.6
FβHCG + PAPP-A
16
NT
Not given
fβhCG and total hCG
Four papers compared the performance of fβHCG and total hCG either alone or combined with PAPPA. (see Table 8). fβHCG had a higher estimated DR than total hCG when both tests had a fixed FPR of
5%.
Table 8.
Comparison of DRs and FPR, fβHCG and total hCG
Reference
Test
(Hallahan et al. 2000)
fβHCG
45
5
Total hCG
35
5
PAPP-A + fβHCG
67
5
PAPP-A + hCG
52
5
fβHCG
49.5
5
Total hCG
50.8
5
PAPP-A + fβHCG
88.9
5
PAPP-A + hCG
78.7
5
PAPP-A + fβHCG
64
5
PAPP-A + hCG
67
5
(Spencer et al. 2000a)
(Spencer and Cuckle 2002)
(Palomaki et al. 2005)
DR (%)
FPR (%)
Modelled
Modelled
Modelled
PAPP-A and fβhCG
Five studies were identified that presented estimates for the predictive performance of fβHCG and
PAPP-A (see Table 9). In all but one study PAPP-A was a better discriminator of DS than fβhCG.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
21
Table 9.
Comparison of DRs and FPR, fβHCG and PAPP-A
Reference
(Krantz et al. 2000)
(von Kaisenberg et al.
2002)
(Montalvo et al. 2005)
(Spencer and Cuckle
2002)
(Laigaard et al. 2003)
Test
fβHCG
PAPP-A
Free βHCG
PAPP-A
Free βHCG
PAPP-A
Free βHCG
PAPP-A
Free βHCG
PAPP-A
DR (%), (95% CI)
46
38
15.8
26.3
10.5 (1.3-33.1)
47.4 (24.9-69.8)
49.5
50.8
42.4
52.3
FPR (%), (95% CI)
5
5
4.7
4.6
5
5
5
5
5.1
5.1
Evidence regarding first trimester screening included in Chapter 5 evidence tables
Five studies included in Chapter 5 also have evidence relevant to this chapter (Cuckle et al. 2005;
Cuckle 2003; Malone et al. 2005; Rode et al. 2003; Wald et al. 2003b). None of this evidence
contradicted the conclusions of this chapter i.e. that the combined test is better than both NT and 1st T
MSS (PAPP-A and fβhCG) that fβhCG performs better than total hCG and that it is not possible to say
whether 1st T MSS or NT performs better.
Other tests
Muller et al. (2003a) added 1st trimester AFP to both FβHCG + PAPP-A and the combined tests. The
addition of AFP did not enhance test performance in this study.
The DR and screen positive rate (SPR) of ADAM12 was evaluated by Laigaard et al. (2003).
ADAM12 had improved performance compared with βHCG alone (DR 81.5% SPR 3.2% versus
βHCG alone: DR 59.9%, SPR 12.9%), and PAPP-A alone (DR of 66.2%, and FPR of 11.2%).
Palomaki et al. (2005) evaluated the use of serum ITA. In a key comparison they compared the DR of
ITA + PAPP-A and NT to the conventional combined test. With a fixed FPR of 5%, the DR of both
these screening methods was 84%. Spencer et al. (2002) also estimated the performance of ITA
(HhCG) in the 1st trimester and found ITA was unlikely to be of any additional value.
In another study a strategy involving repeat measures of PAPP-A and fβhCG at 10/40 and 12/40
showed a slight improvement in performance over the combined test where either the serum was taken
at 10/40 or it was taken at 12/40 (Spencer and Cuckle 2002). At a fixed 5% FPR the DR for the repeat
measures was 88.6% compared to 87.2% when serum was taken at 10/40, and 87.3% when serum was
taken at 12/40. The authors concluded that when women present twice in the 1st trimester this strategy
could be considered. However, there is no justification for taking two samples routinely (Spencer and
Cuckle 2002).
Christiansen (2002) evaluated a contingent screening strategy confined to the 1st trimester. This
involved all women having 1st trimester PAPP-A and βhCG prior to 11/40. Then only those with an
intermediate risk would have NT, and those with very high risk would have an invasive screen. The
reasoning was to explore the possibility of rationing NT. The 1st trimester contingent screening
strategy had a DR of 78.9% and a FPR of 4% compared to a combined screening which had a DR of
85.5% and a FPR of 4.4%. This performance would be achieved with only about 20% of women
requiring NT.
Difficulties implanting any of the screening strategies
Eleven studies gave details of any difficulties implanting screening strategies.
NT was successfully measured in all participants in a multicentre study but the investigators noted that
3-5% required TV USS for the measurement (Gasiorek-Wiens et al. 2001). In another study, NT could
not be measured in 2% (Schuchter et al. 2002). In a further study at least one image was obtained for
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
22
NT measurement in 72.9% of participants although only 51.9% successfully had all three images
measured, and staff felt more time was needed to measure NT (Crossley et al. 2002). In another study,
NT was too small to measure precisely so was assumed to be under 5mm (Muller et al. 2003a). In
another study a learning period was required for NT measurement (Wapner et al. 2003). This required
careful training, evaluation of competence and external quality control. In one study, 10 of 25 units
approached declined to participate due to lack of time/staff for USS, having USS equipment with
inadequate resolution, or having a large number of women booking in the community (Crossley et al.
2002).
One group investigated twin pregnancies (Gonce et al. 2005). In monochorionic twins they were unsure
whether the largest, smallest or average of the two NT measurements should be used.
There were also documented difficulties in obtaining both NT measurements and serum tests in one
study. This study measured NT in 7,580 but only 3,551 had serum samples taken as well (von
Kaisenberg et al. 2002).
In some studies, the marker MoMs were different from expected. For example, in Gonce et al. (2005),
the authors noted that twin serum levels should be double that for singleton pregnancies but the MoM
for fβHCG was only 1.57 and in Scott (2004) the MoM for PAPP-A was 0.88 rather than 1. In three
studies the distribution of NT measurements differed from the Fetal Medicine Foundation (FMF)
distributions (Gyselaers et al. 2005; Muller et al. 2003a; Wapner et al. 2003). The importance of using
correct parameters was noted in one study (Spencer et al. 2000a) which found that when PAPP-A +
total hCG samples were taken at 84-97 days and analysed using appropriate parameters (for gestational
age), this method achieved performance comparable to screening with PAPP-A and fβhCG.
Various types of assay methodology could be used for the serum tests. In one study an in-house polymonoclonal assay was used rather than an automated double monoclonal assay for the measurement of
PAPP-A (Christiansen and Jaliashvili 2003). The authors noted that the simplicity of the polymonoclonal approach was obtained at the expense of automation, which potentially increases the risk
of human error.
Summary of results
There was a high level of consistency supporting:
1.
2.
Poor performance of maternal age alone as a screening test compared with other screening
methods
improved performance of the combined test compared with either NT or fβHCG + PAPP-A (either
on the basis of a higher DR for a fixed FPR or a higher DR with a lower FPR).
There was also some support for fβHCG having better performance in the 1st trimester than total hCG,
and PAPP-A being a better discriminator of DS than fβhCG. There was no clear evidence to suggest
that either 1st trimester MSS or NT had superior screening performance.
Other tests were included in the studies appraised. There appeared to be some support for ADAM as a
marker for DS, and serum ITA showed promised as a screen but further research is required.
There were some difficulties noted with the screening tests. Most of the cited difficulties were with the
measurement of NT: either it was not able to be done in everyone, or the measurement was inaccurate
when assessed against standards such as the FMF standards. This may be because not all operators
were trained, or there was not enough time for measurement. There were also issues with serum marker
MoM being different from expected or problems when using inappropriate data for distribution
parameters.
Conclusion
The evidence appraised in this chapter showed that maternal age alone is not an appropriate screening
test for DS, that fβhCG performs better than hCG in the first trimester, and that in the first trimester the
combined test is the best DS screening method based on DR and FPR.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
23
There were some limitations to this evidence including some evidence based on case-control studies or
modelling papers based on data from case-control studies, and some studies having a retrospective
design. Most of the cohort studies were based in hospital settings: results (especially for NT) may not
be replicated in regional settings. Some samples were biased as not all women had all tests and in some
studies this was because women with large NT measurements had invasive diagnostic testing instead of
1st trimester MSS.
For screening confined to the first trimester the combined test is the screening method of choice. The
implications of resources for training, monitoring and quality control particularly for NT testing would
need to be carefully considered when determining whether a screening programme should proceed.
There are also quality control issues associated with determining risk. Correct medians are needed for
calculating MoMs and appropriate parameters are required for accurate risk calculations.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
24
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Krantz et al. 2000)
The study compared screening for
DS and T18 using fßhCG, PAPP-A,
fβhCG + PAPP-A, NT, fßhCG & NT,
PAPP-A & NT, and the combined
test.
Between September 1995-June 1998
blood samples collected from 10,251
women and dried as spots on filtered
paper.
Outcomes
DR and FPR of screening for
DS using fßhCG, PAPP-A,
fßhCG + PAPP-A , NT, fßhCG
& NT, PAPP-A & NT, and the
combined test was
extracted for this evidence
table. These results are
calculated based on the
age distribution of the USA
population (14-49 years).
Accuracy of screening
methods
Limitations
Fetal loss not accounted for which could
overestimate the DR. Using a fetal loss adjustment
(31% loss rate from late 1st T to term) the 3 not
detected by screening represents about 0.69% of
those alive at 1st T. Therefore 4 would have been
alive at 1st T (3/0.69 = 4) and the adjusted DR of
combined test= 30/34 = 88%.
Prospective cohort
study
Grade III-2
Analysed fβhCG and PAPP-A using
ELISA procedure. 7,801 samples
analysed at NTD labs (USA) and
2450 at Centro Di Diagnosi
Prenatale (Italy) using identical
reagents and procedures.
NT done according to FMF
guidelines and measured at
10+4/40-13+6/40 by FMF trained
ultrasonographers.
Marker values converted to MoM.
Labs developed separate MoMs to
account for interlab assay
variation.
LR calculated from multivariate loggaussian distributions of MoM in DS
and “unaffected”. Risks
determined by multiplying the LR
by MA associated risk of DS and
GA (Snijders et al. as referenced in
this paper), and the MA distribution
in USA.
GA = 9/40-13+6/40 based on USS or
LMP (if no USS). All pregnancies
apparently healthy singleton with no
DM.
Of 10,251 in study, 5,809 met the
criteria of the dates for NT and so
had successful NT measured as well
as MSS.
Spectrum of disease: 50 DS/10251 =
0.49%.
T18 = 20.
“Adverse fetal outcomes” (includes
other chromosomal disorders) = 75.
Of the unaffected (excludes DS, T18,
and other) having MSS
n= 10,106
Mean MA 31.6 ± 5.4 (SD)
Mean GA 11.65/40 ± 1.06 (SD)
Having NT and MSS
N= 5718
Mean MA 32.1 ± 5.7 (SD)
Mean GA 12.07/40 ± 0.85 (SD)
Of those with DS having MSS
n= 50
Mean MA 37.2 ± 4.9 (SD)
Mean GA 11.73/40 ± 1.16 (SD)
Having NT and MSS
n= 33
Mean MA 37.5 ± 4.4 (SD)
Mean GA 12.07/40 ± 0.88 (SD)
If MSS and NT not on same day, GA
taken as the later of the 2 GA’s.
For these figures it is
presumed T18 and other
chromosomal abnormalities
included as unaffected, but
unsure as DR and FPR only
given as %. CI’s were
therefore not calculated for
the evidence table.
The risk cut-off was varied
until it reached a fixed 5%
FPR. Also determined
performance at a fixed DR
of 70%.
Verification
No details given.
Expected number of DS
from the MA distribution was
48.9.
Age standardized, 5% FPR
fßhCG (1:145)
46%
PAPP-A (1:105)
38%
fβhCG + PAPP-A (1:140)
63%
NT (1:195)
74%
fßhCG & NT (1:240)
80%
PAPP-A & NT (1:185)
81%
Combined test (1:270)
91%
Age standardized, 70% DR
fßhCG (1:355)
15.8%
PAPP-A (1:395)
19.0%
fβhCG + PAPP-A (1:195)
6.8%
NT (1:90)
3.4%
fßhCG & NT (1:55)
2.3%
PAPP-A & NT (1:35)
2.3%
Combined test (1:15)
1.4%
Difficulties implementing any
of the screening strategies
None noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
There is also a possibility of not ascertaining all DS
cases born but not identified by screening.
However, in this study the DS ascertained is similar
to that expected based on MA and GA.
No details of how verifications obtained.
Unclear where parameters obtained for the
Gaussian distribution for LR. The paper presents
parameters for MSS markers and NT from 108 DS
(including an additional 58 analysed previously).
Two of the authors are employees of NTD labs and
one is the owner of NTD labs as well as the owner
of patents related to the use of fβhCG in DS
screening.
Author’s conclusion
1st T screening for DS and T18 is effective and offers
substantial benefits to clinicians and patients.
Reviewers’ conclusions
Despite limitations, this is a large well designed
study.
25
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Hallahan et al. 2000)
Comparison of screening with
fβhCG compared to intact hCG
(with and without MA) in 1st T
screening for DS.
fβhCG and intact hCG were
analysed in a total of 63 DS (35 liquid
serum and 28 dried blood) and 400
unaffected specimens (200 liquid
serum and 200 dried blood).
Outcomes
DR and FPR given are for
screening for DS using the
observed data (fixed 5%
FPR, or a fixed 60% DR), and
using Gaussian distribution
parameters from previous
studies and current study
combined with the MA
distribution of live births in
the USA.
Accuracy of screening
methods
Limitations
A case-control design is not the best design for
determining the validity of a screening test. The
design (DS and unaffected controls) means the
sample will not include fetuses with other
chromosomal disorders which are also likely to test
positive during DS screening.
Case-control study
Grade III-2
FßhCG was determined using inhouse ELISAs. Parameters for fβhCG
were obtained from previous
studies. For liquid samples these
were Brambati et al. 1997 and
Morssink et al. 1998 (as referenced
in this paper), and for dried
samples-ongoing prospective
analysis (Orlandi et al. 1997, Krantz
et al. in press, as reference in this
paper).
Intact hCG analysed using
commercial kit (Immulite system,
DPC).
Gestational day specific medians
calculated for liquid and dried
samples separately, and then MoM
calculated for the overall samples.
The MoM and the MA specific risk
used to determine the LR and the
individual risk of DS.
A meta-analysis (7 case-control
studies including this one) was
done for the distribution
parameters of intact hCG versus
fβhCG. Used studies where both
measured in same analyte set.
GA = 10-13/40.
100 (50 liquid, 50 dried) unaffected
pregnancy specimens selected for
each gestational week from USS
dated, white, non-diabetic,
singletons.
For DS, mean MA = 38 ± 5.09 (SD)
For unaffected controls, mean MA =
35.8 ± 5.71 (SD)
Spectrum of disease: 63 DS/463 =
13.6%
Presumably no other chromosomal
abnormalities in study.
Raw data not given, so
unable to calculate CI for
the DR and FPR.
Verifications
No details given.
DR for fixed FPR 5% using
observed parameters
Intact hCG alone
19%
fβhCG alone
27%
Intact hCG & MA
35%
fβhCG & MA
45%
FPR for fixed DR of 60% using
observed parameters
Intact hCG alone
30%
fβhCG alone
14.9%
Intact hCG & MA
17.7%
fβhCG & MA
10.5%
(No other details of sample given)
DR for fixed FPR 5% using
meta-analysis parameters
and USA age distribution
Intact hCG & MA
34%
fβhCG & MA
45%
Difficulties implementing any
of the screening strategies
None noted.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
There was little detail about the source of the
cases or controls-for example whether the cases
had been detected by a positive 1st T screen
using fβhCG.
The use of an in-house ELISA for fβhCG may limit
the reproducibility of the results unless the full
description of methods is available.
It is unclear whether those conducting the serum
analysis were blinded to the outcome.
Author’s conclusion
FβhCG is a better marker than intact hCG for DS in
1st T.
Reviewers’ conclusions
The design of the study and the possible biased
sample means that a further prospective study is
needed to verify the results. However, results do
seem to indicate that fβhCG is better at
discriminating between DS and unaffected
controls than intact hCG in 1st T DS screening.
26
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and verification
Results
Comments
(De Biasio et al. 2001)
The combined test was compared to
fβHCG + PAPP-A, and to NT.
Women attending the centre between
July 1998 and Jan 2000 were recruited.
Outcomes
All tests done on everyone.
Accuracy of screening
methods DR (CI), FPR (CI)
Limitations
Only described the participants (1836). The eligible
and source populations were not described.
Each screening method was well
described-could be replicated
Women were having AC or went on to
have TT.
DR and FPR for combined test
was compared to fβHCG +
PAPP-A, and to NT.
NT performed by TA USS at 10-13/40. 3
images obtained using standard
methods (Nicolaides et al. 1992-as
referenced in this paper).
The GA (from CRL) ranged from 10-13
+ 6/40 (median 12/40).
cut-off of 1:350
Combined
87% (62-98), 3.3 (2.5-4.1)
fβhCG + PAPP-A
69.2%, 4.5%
NT
61.5%, 6.7%
Prenatal diagnosis
centre
Genoa, Italy
Prospective cohort
study
Grade III-2
Immunoradiometric assays for MSS
were performed (Ortho-clinical
Diagnostics).
The risk of DS pregnancy estimated
from multivariate Gaussian
distribution (Wald and Hackshaw,
1997-as referenced in this paper),
using commercially available
software.
A regression analysis was performed
for NT and serum medians for
gestational age.
Median maternal age was 31yrs 8
months.
Spectrum of disease: 16/1836 DS =
0.87%
Participant Sample size = 1836.
The DR was for those with DS
and FPR was for those
unaffected by DS (i.e.
presumably all other
chromosomal disorders
considered to be
unaffected).
Difficulties implementing any of
the screening strategies
None noted.
Didn’t say how parameters obtained for the
Gaussian distribution, apart from medians for NT and
serum markers.
Unclear how many lost to follow-up or spontaneous
fetal loss before karyotyping or if these were
excluded from analysis.
Of the 992 participants who had TT doesn’t say how
outcome determined.
Figures in the paper were not
consistent so CI was not
calculated for this evidence
table.
No raw date to check anything but combined
screening. Also say 14/16 detected then in discussion
say 13 detected and that the screened population
was 1467 (not 1836 reported elsewhere).
Verification
Unclear if all tests were
compared with a valid
reference standard.
The DR is of DS found in 1st T. Does not account for
the fact that many of these (about 1 in 2) would be
lost anyway by miscarriage.
About half had invasive
diagnostic testing (IT) mostly
for AMA, and the rest had 2nd
T screen (TT) without a
description of outcome
verification.
The paper states that about 2
cases of DS would be
expected in 1,467
pregnancies and that
screening detected 13 DS. It is
not clear why these figures
differ from those reported
elsewhere.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Possibly the population is high risk as they were
attending a prenatal diagnosis centre and had AC
for AMA and other high risk situations. This limits the
applicability of the results. High percent DS in
population.
Author’s conclusions
“Our results confirm the value of the combined test in
first trimester screening for DS”
Reviewers conclusions
There are limitations which will affect the internal and
external validity of the study. However it appears that
combined screening performed better than fβHCG +
PAPP-A which in turn performed better than NT.
27
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and verification
Results
Comments
(Niemimaa et al. 2001)
Comparison of fβHCG + PAPP-A, NT,
and combined screening.
All pregnant women in Eastern and
Northern Finland in 1999 were invited
to participate during 1st visit to
midwives at 6/40-13/40.
Outcomes
DR and FPR determined for
cut-off of 1:250.
Accuracy of screening
methods
Limitations
Small number of DS cases (8 in total screened
population).
Antenatal clinics at
health centres-primary
and secondary care
Eastern and Northern
Finland
Prospective cohort
study
Grade III-2
NT by ultrasonographers trained in NT
measurement.
MSS analysis by commercial kits
(Wallac). Labs given clinical data
including NT thickness. Quality
control done regularly.
For each serum level the MoM was
calculated. Risk determined by
Wallac 1T risk calculation
programme (research version).
Cut-off of ≥ 3mm NT used for
intervention, but risk also calculated
by Wallac using MA, CRL and NT.
For serum screening the risk was
calculated using Wallac
programme.
Blood drawn in primary care and
maternity clinics of hospitals (university
and central).
MSS at 10– 13+6/40. GA mostly (82%)
based on USS, or based on LMP.
Presumed singleton.
2,515 had serum
17.5% >35 yrs which is = to the stats for
Finnish pregnant women.
Only 1,602 had NT as well as serum
Spectrum of disease: 8 DS/2525 =
0.32%
Also calculated DR for
combined screening with
fixed 5% FPR.
Verification
Contacted maternity clinics
and National Register of
Congenital Malformation,
and National Research and
Development Centre for
Welfare and Health to get
information on newborns
with DS.
Expected number DS
(according to national
Register of Congenital
Malformation) was 7.8.
DR (95%CI), FPR (95% CI)
Cut-off of 1:250
NT
60% (15-95), 11.6% (10.0-13.20)
Double
75% (35-97), 9.7% (8.5-11.0)
Combined
80% (28-99), 8.3% (6.9-9.6),
Fixed FPR 5% (Cut-off of 1:200)
Combined
80%
Difficulties implementing any of
the screening strategies
None noted.
2 cases of T18 (presumed included in
analysis as unaffected).
Corrections for weight but not
smoking or DM.
Not all tests were done on everyone. All had MSS
but not everyone had NT as well. This could be a
problem if this was based on risk (e.g. if those having
NT as well had higher or lower risk for DS).
Did not determine karyotype of fetal losses. Could
have missed DS and therefore true DR could be
lower.
Does not mention those lost to follow-up.
Lab was not blinded to the results of the NT.
However the serum marker results are not subject to
subjective interpretation.
Author’s conclusions
The study suggests that the combined test promises
better sensitivity than the current testing methods
(2nd T MSS) used in DS screening.
Reviewers conclusions
Some limitations which may decrease the accuracy
of the reported DR and FPR and the ability to
compare screening methods. However, it appears
that combined is better than NT alone, and that
fβHCG + PAPP-A is better than NT. However not all
had NT.
Serum results not given to women
(were used to determine medians)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
28
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Gasiorek-Wiens et al.
2001)
Comparison of screening by using
NT or MA alone.
Screening (June 1995-May 2000) of
those with EDD before August 2001.
Accuracy of screening
methods DR (95%CI), FPR (95%
CI)
(German speaking DS
screening group)
Centres included some specialist
perinatal diagnostic centres.
Limitations
Limited details of the study setting.
No details of the efforts to determine outcome for
fetal loss, or ToP or those lost to follow-up.
Multicentre
Tests could be replicated.
All those involved in the study had
FMF Certificate of Competence in
the 10-14/40 scan.
Outcomes
Outcomes were the
performance of screening
using NT (risk at term cut-offs
of 1:300 or 1:100), or MA (≥
35 years) alone.
Germany, Austria,
Switzerland
NT measured according to FMF
guidelines.
Prospective cohort
study
Risk for DS estimated using MA and
NT for CRL with the use of FMF
software.
Outcome available in 21,959 (92.2%).
Median MA 33yrs (range-15-49) &
36.1% ≥ 35 yrs (higher than general
population = 30 yrs and 18.1%)
Grade III-2
Screened 23,805 singletons.
The median GA 12/40 (range-10-14)
& median CRL = 61mm (range-3884)
Spectrum of disease: 210 DS/21959 =
0.95% DS.
The DR was for DS and the
FPR was for “normal”
pregnancies and did not
include any of the 274
pregnancies with other
chromosomal abnormalities.
Verification
CVS, AC, or birth of
phenotypically normal
infant or postnatal
karyotyping.
NT
(1:300) 87.6% (83-92), 13%
(12.6-13.5)
(1:100) 79.5% (74-85), 6.0%
(5.7-6.3)
Biased sample as many women would have had
a NT by own gynecologist and referred for further
investigation. This could over estimate the DR. High
NT in screened population.
MA (≥ 35 years)
66.7%(60-73), 35.7% (35.0-36.3)
Paper stated there was some self selection bias of
anxious women.
Difficulties implementing any
of the screening strategies
The paper did not include other chromosomal
disorders as unaffected which is the convention.
For comparison this would mean for NT (1:300) the
FPR = 14.0% and for MA alone = 35.8%
NT successfully measured in
all, but 3-5% needed TV USS
for NT measurement.
Also 274 cases of other chromosomal
disorders.
Of those where no outcome-258
spontaneous fetal loss, 125 ToP, 1,463
no antenatal follow-up.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Author’s conclusions
In Germany, Austria and Switzerland results of
screening for chromosomal defects by NT, in
centres with appropriately qualified sonographers
and using the FMF software are similar to those
reported in the UK using the same methods.
Reviewer’s conclusions
Despite a possibly biased sample which may limit
the applicability of the estimated DR and FPR,
screening using MA and NT appears better than
MA alone.
29
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Schuchter et al.
2002)
The study compared performance
of screening using MA, NT alone,
MA and NT, and combined test.
Between 1st Dec 1997 and 31st April
2000, all women with singleton
pregnancies, and GA 10-13 + 6/40
were invited for combined test.
Outcomes
The outcomes were DR and
FPR for screening for DS
based on MA alone, NT
(cut-offs of ≥ 2.5mm, and
MoM >95%), MA and NT,
and the combined test (risk
cut-off of 1:250).
Accuracy of screening
methods DR (95%CI), FPR
(95% CI)
Limitations
The denominator for the different screening
methods is unclear. Appears they have used the
number with outcome known for combined test,
but for MA alone have used the total who had
MSS and NT (4939), and for NT have used the total
having NT (5012) despite some of these having no
outcome documented. These were classified as
unaffected in the analysis. Some of the DR in text
disagreed with tables.
Hospital
Vienna, Austria
Prospective cohort
study
Grade III-2
Women invited for NT & CRL
measurement at 10/40-12+6/40. If
CRL <35mm another appointment
given. If >70mm offered Triple test
(only a few cases). NT by staff
experienced in NT measurement.
NT measured 3x by TA USS, using
standard methods.
PAPP-A and fβhCG analysed using
commercial kits (Ortho Clinical
Diagnostics).
Medians for NT, PAPP-A and fβhCG
(for GA) from study. Markers
converted to MoM. Risk calculated
based on MA and LR for markers
using commercial software
(Logical Medical systems).
5,012 had NT done.
4,939 had MSS of whom:
13 had spontaneous abortion
before 16/40, 4 had positive
combined test and no karyotyping
(2 of whom had NT >2.5mm).
Another 18 had no follow-up-1 with
positive combined test result.
14 spontaneous abortions at 1624/40, 3 with normal karyotype.
92 delivered at another hospital and
outcome unavailable.
In some cases the CI was
not calculated for this
evidence table as the
screened population
number was not clear.
Verification
311 of the whole
population had invasive
screen, 254 of whom had a
positive screen. Rest for
AMA (51) and for
malformations on
sonogram (6).
MA ≥ 35yrs
64.3% (39.1-89.4), 12.8%
NT ≥ 2.5mm
50% (24-76), 1.8% (1.4-2.2)
NT MoM >95%
57.1% (31.3-83), 4.8% (4.2-5.4)
NT MoM (with MA): 71.4%, 10%
Combined (1:250) 85.7%, 5%
(4.5-5.7)
Difficulties implementing any
of the screening strategies
About 2% could not measure
NT.
4802 known outcome.
Risk >1:250 used for counselling
during study. All those ≥ 35yrs or
with abnormal sonogram also
offered invasive diagnostic test.
Spectrum of disease: 14 DS/4802 =
0.29%
For the population age
distribution without
intervention the expected
number of DS at term was
8. However, screening at 12
weeks when more DS
viable.
In discussion do use a correction for the DR to
take account for fetal loss of DS pregnancies
between 10/40 and birth (48% of DS
pregnancies). This means 12 X 52% = 6.2 would
have survived. DR is therefore 6.2/6.2 +2 = 76%.
Local medians for NT and MSS markers when
these numbers are small especially for DS
medians.
Wide CI for DR as small number of DS cases.
Used the mean of 3 NT images not the largest
figure, and also mean CRL was only 48mm which
may have decreased performance of NT.
Author’s conclusions
The results make the combined test by far the
best test for the detection of DS in a low-risk
population.
Reviewers conclusions
Some limitations which limit the internal validity
especially the problem of those with no
outcomes being included, but authors did adjust
for fetal loss. Combined test does appear better
than NT which in turn appears better than MA
alone.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
30
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Crossley et al. 2002)
The study compared NT, fβHCG +
PAPP-A, and combined test.
Invited all pregnant women (1014/40) attending 15 routine
antenatal clinics over a two year
period to participate (n = 17,229).
Outcomes included DR for
FPR for DS screening by NT,
fβHCG + PAPP-A, and
combined test.
Accuracy of screening
methods DR (95%CI), for fixed
5%FPR
Limitations
Not clear how outcome determined e.g. for fetal
losses. Not clear if any lost to follow-up, and if so
whether they were presumed to be unaffected or
removed from analysis?
MA distribution about = to routinely
screened population. Median MA =
29.9 yrs (versus 29.1yrs) and 15% >35
years (versus 12.8%).
Verification
Of the DS cases, nine had
CVS (AMA or large NT), 23
AC (2nd T MSS or AMA) and
13 detected at birth (low
risk, or unscreened, or
declined diagnostic test).
Multicentre study at
15 maternity units.
Scotland, UK
Prospective cohort
study
Grade III-2
GA assessed by CRL or BPD. Where
CRL 31-94, or BPD <30mm, 3 x TA NT
measurements attempted. (TV USS
for NT was not part of the protocol).
Staff all trained by FMF in NT and
there was quality control.
fβhCG and PAPP-A assayed using
Kryptor analyser (Brahms). Subset of
2000 (including all affected) was
analysed using Delfia immunoassay
(Perkin-Elmer) for comparison.
(Results were strongly correlated).
Unaffected medians and other
distribution parameters for NT and
serum markers were derived from
the study population.
Marker levels converted to MoM for
GA and risk obtained from
Gaussian distribution. No results
were given to participating
women-all offered routine 2nd T
screen.
NT measurements were obtained in
72.9% of women and blood samples
in 98.4%.
Spectrum of disease: 45 DS/17,229 =
0.26 %
No details of lost to followup, or miscarriage before
outcome ascertained.
However says all outcomes
followed up.
States DS prevalence was
about that expected for this
population.
NT
54% (37-71)
Double
55% (39-70)
Combined (1:250)
82% (65-93)
Difficulties implementing any
of the screening strategies
15/25 units accepted study.
Declining units gave reasons
as: lack of time/staff for USS,
USS with inadequate
resolution, or large number
booking in community.
Success for NT = 72.9% (≥ 1
image) & 51.9% (3 images).
Best success during 11-13/40.
Most common reason for
failure= fetal position. “Not
enough time in appointment
for repeat attempts” And
“Need more than 10-15 mins.”
Used study data for parameters which may be
inappropriate, especially for DS as small sample.
MoM for DS NT (1.65) and fβhCG (1.58) which is
lower than expected. This may have decreased
the performance of screening.
Wide CI for DR as number of DS cases low
There was industry support as CIS and Perkin-Elmer
UK provided instrumentation and reagents.
Author’s conclusions
The authors felt they should include all DS in the
series when determining DR (and not just those
with NT and serum measured). Therefore DR = 62%.
NT in combination with appropriate serum markers
has the potential to detect over 80% of DS fetuses
in early pregnancy. However, NT measurement is
highly operator-dependent. It requires training,
external quality control and adequate time to
allow accurate measurement, otherwise
suboptimal performance will result.
Reviewers conclusions
Using own parameters for risk estimate may have
reduced the accuracy of the estimated DR and
FPR. Also some details of the study missing such as
how outcomes obtained and whether any loss to
follow-up. Does appear that combined is better
than NT and fβHCG + PAPP-A but the actual
figures for DR and FPR may not be precise.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
31
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(von Kaisenberg et al.
2002)
Compared combined test to MA,
NT, PAPP-A alone, and βhCG
alone.
The study began September 1998 &
included pregnancies with EDD
before November 2001.
Accuracy of screening
methods DR (95%CI), FPR
(95% CI)
fβhCG + PAPP-A 11-14/40.
All ultrasonographers had
certificate of competence from
FMF in the 11-14/40 scan.
Maternal serum (fβhCG and PAPPA) analysed at 11-14/40 using the
Kryptor analyser (Brahms) and
corrected for maternal weight.
The distributions for NT for CRL using
the 95th centile and 99th centiles
from FMF.
Distributions for serum markers
using the 95th centile and 5th
centile for fβhCG and PAPP-A
respectively from the data of this
study.
Risk of DS calculated from MA
related risk combined with LR from
NT and serum results using FMF
software.
3,864 singleton pregnancies 1114/40 with live fetuses screened. All
had MSS and NT.
Those with chromosomal
disorders other than DS (27)
analysed separately. The
total unaffected was 3505
and total screened after
removal of other
chromosomal disorders
=3524. For the purpose of
this evidence table the DR
and FPR for the combined
test (1:300) was also
calculated with the
chromosomal disorders
included as unaffected
(“other” included).
Limitations
Where there was a very high NT often had
invasive diagnostic test without MSS as
biochemical testing was a new policy. This means
the sample was biased as they were not included
in the study. The performance of the combined
test and the serum markers could therefore be
underestimated.
German speaking DS
screening group
Eight centres.
Germany
Prospective cohort
study
Grade III-2
Completed follow-up was available
in 3551 (91.8%).
Median MA = was 33 yrs (range-1546 yrs) & 35.8% ≥ 35 years.
Median GA at screening was 12/40
(range-11-14/40), and medial CRL
was 64mm (range-45-84mm).
Spectrum of disease: 19 DS/ 3551=
0.54% of the population screened
and followed up.
Verification
The choice of who got
which reference standard
was not blinded to test
results (those who had a
positive screen had CVS or
amniocentesis-verification
bias)
However, the reference
standard was not
discussed. Just says that
centre forwarded outcome
details with test results.
MA
52.6%(30.2-75.1), 35.7% (34.137.2)
NT ≥ 95th centile
73.7% (53.9-93.5), 4.8% (4.15.5)
fβhCG ≥ 95th centile
15.8%, 4.7% (4.0-5.3)
PAPP-A ≤ 5th centile
26.3% (6.5-46.1), 4.6% (3.9-4.3)
Combined (1:300)
84.2%, 6.6% (5.8-7.5)
Combined (1:100)
73.7% (53.9-93.5), 2.4% (1.92.9)
Difficulties implementing any
of the screening strategies
7580 had NT but only 3551 of
these had serum taken as
well. Only those with both
were included in the analysis.
Used local data for serum marker parameters
which could be biased for DS as sample size of DS
small.
Small number of DS means CI of the DR is very
wide.
When other chromosomal disorders included as
unaffected the combined test (1:300) had a FPR
of 7.3% (6.4-8.1) versus 6.6%.
Authors’ conclusions
In Germany the rates of screening for
chromosomal disorders by NT and MSS in centres
with qualified ultrasonographers are similar to
those reported in the UK using the same
methodology.
Reviewer’s conclusions
Small number of DS cases means the DR may not
be accurate. The accuracy of the DR is also
affected by the biased sample where many had
high NT and had invasive diagnostic testing and
were not included in the study.
However, it appears that combined screening
performs better than each of the serum markers
and NT. In this study NT appears better than the
serum markers individually. All screening methods
are better than MA alone.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
32
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Spencer et al.
2003b)
The study compared screening
for DS by NT, fβhCG + PAPP-A,
and the combined test.
During a 3 yr period (1st June 199831 May 2001) 12,339 women with
singleton pregnancies were
offered 1st T screening at the
OSCAR clinic.
Outcomes
The outcomes extracted
for this paper were the DR
and FPR for screening for
DS using NT, fβhCG +
PAPP-A or the combined
test at a risk cut-off of
1:300.
Accuracy of screening
methods
Limitations
It appears that the 98 lost to follow-up (but not
on the DS register) were included in the analysis
as “unaffected” pregnancies. This may over
estimate the DR.
It is assumed that the
other chromosomal
abnormalities were
included as “unaffected”
pregnancies for the
analysis.
DR (95%CI), FPR (95% CI)
Combined (1 :300)
92% (74-99), 5.2% (4.8-5.6)
OSCAR (One stop
clinic for assessment
of risk), maternity
unit, District General
Hospital
Essex, U.K.
Retrospective cohort
study
Grade III-2
In 1st year qualifying GA for
OSCAR = 10+3/40-13+ 6/40. Next
two years minimum GA
increased to 11/40. If less than
11/40 by CRL (45mm) given
another appointment. More than
13+6/40 (CRL = 85mm) offered
AFP and fßhCG (not in analysis)
NT carried out by staff with FMF
certificate of competence. NT
measured by TA USS as per FMF
guidelines. Completed in about
20 mins (99%). Less than 1% had
TV examination.
PAPP-A and fβhCG analysed by
Kryptor analyser (Brahms).
Patient specific risks calculated
by multivariate approach using
population parameters from
Spencer et al. 1999 (as
referenced in this paper) and MA
specific risks (Snijders et al. 1995
and 1999, as referenced in this
paper)
Cut-off for offer of invasive
screen was 1:300.
All women booking at Harold
Wood Hospital were offered
screening and given an
appointment to attend at about
12/40 for OSCAR. 97.5% accepted
offer=12,030
Median MA = 30 yrs (range-14.4 –
46 yrs).
Median weight = 65.8 kg, and
smoking in 18.1% (self reported,
1.1% unknown, rest 80.8% non
smokers)
Ethnicity-Mostly “white Caucasian”
(93.9%)
Median GA= 12 +2/40 (10+4/4013+6/40). Median CRL= 60mm
(range-38-84mm)
Excluded those > 13 + 6/40 on USS
(n=702), fetal death on USS
(n=233).
Total of 11,105
Spectrum of disease: 25 DS/11105=
0.23%
Verification
Pregnancy outcomes
were obtained from
delivery room records,
hospital database, and
child health records and
were cross checked with
the fetal database.
DR (95%CI) for fixed FPR 5%
NT
76% (59-93)
Double
68% (50-86)
Difficulties implementing
any of the screening
strategies
No difficulties noted
Paper states that 98 lost to
follow-up but were not on
DS register.
Based on MA distribution
and risk of DS at 12 weeks
would expect to see 26
cases.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Not clear how well fetal loss followed up and
no adjustment for fetal loss between screening
and term. Failure to ascertain all the DS
pregnancies will overestimate DR.
The lead author is an advisor to Brahms
Diagnostica on matters of prenatal screening.
CIS UK (Brahms Diagnostica was formally CIS)
funded some of the lab aspects of the OSCAR
clinic.
Authors’ conclusions
“The findings of the study confirm our
prediction that the combined test at 11-14/40
would identify about 90% of DS for a 5% FPR
which is far superior to the average sensitivity of
65% achievable by 2nd T MSS.”
Reviewer’s conclusions
Possible biases may overestimate the DR for this
1st T screening. However, large well designed
study which continues to show the trend that
combined test is superior to NT and fβHCG +
PAPP-A.
33
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Muller et al. 2003a)
The study compared NT, fβHCG +
PAPP-A (with & without AFP), &
combined test (with & without AFP).
All women booking January 1998June 2001 were invited to provide
blood sample and have NT USS 1113/40.
Observed and modelled DR
and FPR using NT, fßhCG +
PAPP-A , fßhCG + PAPP-A
plus AFP, combined test,
and combined test plus AFP.
The cut-off risk was 1 in 250
at term.
Accuracy of screening
methods
Limitations
Study population not well described. The paper
states that a total of 5694 women were included in
the study but not how many of those originally
invited, accepted. Unclear if sample biased.
Exclusion and inclusion criteria not stated. No
description of MA or GA of those screened. Not
everyone had all tests as evidenced by different
denominators. If this was based on risk it may bias
the results. Unclear how many screened by each
method, or how the denominator of each DR and
FPR calculation was derived.
(French Collaborative
Group)
9 centres-12 maternity
units.
Prospective cohort
study.
Grade III-2
Some statistical
modelling
NT performed by 60 staff: 2 FMF
trained, 30 trained by FMF trained
staff, 8 specific NT training, and 20
self taught. NT measured at 1114/40.
Serum samples taken and stored at
-20C. Retrospectively tested for
PAPP-A, fßhCG, and AFP using
fluorescent assay (Perkin Elmer).
Marker levels expressed as MoM for
GA (CRL). 87% had weight
available and had adjustment for
weight (Neveux et al. 1996 as
referenced in this paper).
Distribution parameters for
unaffected pregnancies from study
data (removal of outliers). DS mean
from study, but for serum markers SD
and correlation coefficients from
meta-analysis (Cuckle and Van Lith,
1999 as referenced in this paper).
The parameters used to obtain
observed and modelled DR and
FPR (as per Royston and Thompson,
1992, as referenced in this paper).
211 did not return after presenting
too early for NT, or presented too
late-removed from analyses.
A total of 5,694 singletons were
screened. (MA or GA of those
screened not given).
Spectrum of disease: 26 DS/5694=
0.46%
The 1st T serum not used clinically but
NT results were. When high NT result
(usually >3mm) women were offered
invasive prenatal diagnosis.
Those not scanned or with NT
considered to be normal were
offered T2 screening.
24 other chromosomal
disorders presumed
included as “unaffected” in
analysis.
Verification
As part of the National
Screening Programme
outcome sought for every
pregnancy.
Of 26 DS identified: 9
detected with high NT, 1
high risk and so had AC, 1
AMA and had invasive test,
14 2nd T screening, & 1 live
birth.
On the basis of MA 11 DS
births expected (as per
Cuckle, 1987). Assuming 45%
fetal loss this was consistent
with 26 found by screening.
Directly observed DR (95%CI),
FPR (95% CI)
NT
62% (43-80), 5% (4.4-5.6%)
PAPP-A, fßhCG
69%51-87), 8% (7.3-8.7)
PAPP-A, fßhCG, and AFP
69% (51-87), 8% (7.3-8.8%)
Combined test
73%(56-90), 4.7%(4.1-5.3)
Combined plus AFP
73%(56-90), 4.7 (4.1-5.3)
Modelled (DR, FPR)
NT
64%, 6%
PAPP-A, fßhCG
72%, 6.9%
PAPP-A, fßhCG, and AFP
73%, 6.9%
Combined test
81%, 4.5%
Combined plus AFP
81%, 4.5%
Difficulties implementing any
of the screening strategies
In 82 women the NT
measurement was too small to
measure precisely, and so
assumed to be under 0.5mm.
The study produced NT with
wider SD (0.16) than FMF
(0.12).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Unclear if karyotyping of spontaneous fetal losses,
or if anyone was lost to follow-up without the
outcome being obtained.
Stored samples were analysed, and NT was not
fully described which may limit the external validity.
DS mean for risk from observed data (only 26 DS).
Some industry support (Perkin-Elmer Life sciences)
Authors’ conclusions
In France 1st T screening with NT and MSS is likely to
achieve a high efficiency. This has important
implications for national screening policy.
Reviewer’s conclusions
Some design and quality issues limit the
applicability of the results. The small number of DS
(26) means the parameters for risk determination
may have been inaccurate and also produces
wide CI for the DR. However combined performed
better than MSS, which in turn was better than NT.
34
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Wapner et al. 2003)
Comparison of MA as a screen,
fβHCG + PAPP-A, NT, and
combined test
Women with singleton pregnancies
with GA 74-97days (CRL) offered
screening for DS & T18 by combined
test.
Accuracy of screening
methods DR (95%CI), FPR
(95% CI)
NT measured as per the FMF.
Sonographers FMF trained. Quality
monitoring. 3 NT measurements and
largest used to calculate the MoM
(using GA specific FMF standards)
and then LR for DS and T18 based
on FMF algorithm.
Exclusion criteria: recent significant
vaginal bleed, pregestational DM,
donor oocyte, indications for
prenatal diagnosis other than a risk of
trisomy.
Outcomes
The outcomes presented
are DR and FPR for MA,
fβHCG + PAPP-A, NT, and
combined test
Limitations
During the study two minor modifications were
made to the risk-assessment algorithm
corresponding to FMF changes in the algorithm,
and in updates of the median serum levels based
on our own data. Most (74%) screened based on
updated data. Results reported here are based on
risks calculated for the patients during the study.
There was no change in the rate of detection and
only a 0.1 % reduction in the FPR for DS when all
risks were recalculated using recent version.
BUN study
12 prenatal diagnostic
centres
USA, Canada
Prospective cohort
study
Grade III-2
Blood was taken and applied to
filter paper. Sent by mail to NTD
labs, New York.
ELISA for PAPP-A and fßhCG
performed.
Serum marker values were
converted to MoM for GA (using
medians from study data), and
these were converted into LR
calculated from Gaussian
distributions of unaffected and
affected populations (from previous
studies(Hallahan et al. 2000))
Patients risk calculated from
gestational specific risks according
to maternal age, multiplied by the
likelihood ratios for serum, NT
(combined using commercial
software).
Women given risks but
recommended continuation of
pregnancy until 2nd T screening
done
8816 women were eligible and
consented.
302 did not complete screening: 11
blood spot analyses failed, 4 NT not
visualised, 287 for scheduling or other
reasons.
102 were removed because of a
previous DS or T18 pregnancy, and
196 were removed because of
unknown outcomes (lost to followup).
8216 left for analysis. Of these the
mean MA at date of delivery =34.5 ±
4.6
GA at screening was 85.7 ± 5.7 day
Ethnicity = Black 4%, White 83%,
Hispanic 6%, Asian 5%, Other 2%
Spectrum of disease: 61DS /8216 =
0.74%
11 T18 included in the analysis as
unaffected.
Risk cut-off for DS was 1:270
at 12/40. Age standardised
using USA population 1997).
Unclear whether T18
included in unaffected for
analysis of screening
performance for DStherefore CI cannot be
calculated for this evidence
table (where it was not
provided)
Age standardised (2nd T 1:270)
MA
80.3%, 48%
fβhCG + PAPP-A
85.2%, 23.2%
NT
82%, 11.9%
Combined
85.2%(73.8-93.0), 9.4%(8.8-10.1)
Verification
Reference standard was
either invasive test with
karyotyping or evaluation of
the phenotype at birth.
Age standardised DR for Fixed
FPR fixed 5%
MA
32.8%
fβhCG + PAPP-A
67.2%
NT
68.8%
Combined
78.7% (66.3 -88.1)
Outcome of pregnancy was
determined by direct followup with the patient, and
through delivery records.
Combined better than serum
alone (p=0.006) but not
significantly better than NT
alone (p=0.28).
An effort was made to
determine the karyotype of
every fetus in pregnancies
that ended in spontaneous
fetal loss.
Modelled
Combined
1:337 78.8%, 5%
1:270 77.5%, 4.1%
All tests were done on everyone as
this was the basis for inclusion.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Medians were from study data.
Older population-Mean MA at date of delivery
=34.5 ± 4.6
Author’s conclusions
First-trimester screening for trisomy 21 and 18 on the
basis of MA, fβhCG and PAPP-A, and
measurement NT has good DR at an acceptable
FPR.
Reviewer’s conclusions
Well designed high quality study.
35
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
(Wapner et al. 2003)
.
BUN study
12 prenatal diagnostic
centres
USA, Canada
Prospective cohort
study
Grade III-2
Continued
Sample
Outcomes and
verification
Results
Of the 8216 in the analysis 90
had spontaneous fetal
losses. For 60 the karyotype
obtained (cytogenic
analysis). Others, phenotype
derived from pathological
analysis.
Difficulties implementing any
of the screening strategies
49 cases would be
expected based on the
maternal age.
For NT a learning period was
required for staff with
measurements becoming
more consistent over time. This
required stringent training,
evaluation of competence
and external quality control.
Women who were referred
because of increased NT
were not included, so
“ascertainment bias is
unlikely”.
Overall values for the MoM for
NT values were 9% lower than
the expected values from the
FMF. As the study progressed
the measurements converged
toward those of FMF.
11 blood spot analyses failed,
4 NT not visualised
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
36
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Scott et al. 2004)
Comparison of screening by MA,
NT, fβhCG + PAPP-A and
combined test.
All women with singleton
pregnancies referred to SUSW 1st
July 2000-3rd May 2002 for 1st T
screening offered NT, and MSS. GA
= 11-14/40 (CRL 45-84 mm).
Outcomes
The outcomes extracted for
this evidence table are the
DR and FPR for screening
for DS using MA alone (≥
35yrs), NT, fβHCG + PAPP-A,
and combined test.
It is not clear whether the
12 other chromosomal
disorders are included in
the unaffected group for
the analysis or removed,
therefore CI were not
calculated for this
evidence table.
Accuracy of screening
methods DR, FPR
Limitations
The patients were self selected to be an older
population.
Sydney Ultrasound for
Women (SUSW)-a
private practice
specialising in
obstetric ultrasound
Sydney
Prospective cohort
study
Grade III-2
Serum markers measured using
Kryptor analyser (Brahms
Diagnostica). 500 local samples
with USS dating used for Gaussian
distributions. The MoM was
corrected for maternal weight.
NT (and CRL) was measured
according to FMF standards. FMF
software used for GA specific risk.
Risk ≥1:300 = high risk. Patients
could opt for invasive testing even
if not screen positive.
Fetal NT and serum screen
successfully completed in all
cases.
Only included where MSS taken
before NT in order to remove the
chance large NT would be acted
on or small NT would have no further
screen.
2121 had both NT and MSS
completed. 68 had no outcome
(including 44 lost to follow-up and
23 spontaneous fetal loss and 1
ToP), so 2,053 included in the
analysis
Median MA = 32 yrs (range-15-44
yrs). 29% ≥35 yrs.
Median CRL = 61 mm (45-84) = GA
11-14 /40.
Spectrum of disease:
5 DS /2053 = 0.24%.
12 other chromosomal disorders.
verification
Data from pregnancies
were obtained from referral
doctors or patients via letter
phone or a feedback form.
MA (≥ 35yrs)
80%, 29%
NT
100%, 5.7%
fβHCG + PAPP-A
80%, 19%
combined
100%, 7.2%
The combined test FPR was
significantly lower than for
MA (p<0.01), and for fβHCG +
PAPP-A (p<0.01), but similar
for NT (p=0.07).
The differences in DR not
significant.
Difficulties implementing any
of the screening strategies
Median PAPP-A was 0.88
MoM rather than 1 which
would have increased the
FPR slightly (the PAPP-A in this
population would have been
more similar to DS resultsincreasing FPR).
When the program started it
used the data from FMF. New
curves were calculated using
local data. By the end of
study, PAPP-A MoM was low
and new medians calculated
using 15,000 patients. After
the study the PAPP-A and
fβhCG very close to 1. This
reduced the FPR for MSS from
19 to 14%.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Use local parameters for Gaussian distribution of
the serum markers.
Difficult to work out the denominator for the FPR
as only screen positive number given and not
clear whether this includes other chromosomal
disorders.
Author’s conclusions
A combination of MA, NT and MSS gives a high
DR for both DS and other chromosomal
abnormalities.
Reviews conclusions
Very small numbers especially for DS limits
external validity.
37
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Wojdemann et al.
2005)
Compared NT to fβHCG + PAPP-A,
and to combined test. Only NT used
as intervention marker.
March 1998-June 2001 13621 invited
to participate.
Outcomes
In the paper the FPR has
been calculated using all
screened as the
denominator (as opposed
to the unaffected). This
means the CI calculated for
this evidence table will not =
those calculated from the
paper.
Accuracy of screening
methods
Limitations
Small number of cases of DS means wide CI.
DR (95%CI) , FPR (95%CI)-risk
1 :250
NT
75% (42.8-93.4), 1.8%. (1.5-2.1)
Double
73% (39-93.4), 8.8% (8.1-9.5)
Combined
91% (58.7-99.8) , 2.1(1.8-2.5)
Not all had all tests.
Copenhagen First
Trimester Study
3 obstetric
departments of
University Hospital
Copenhagen,
Denmark
Prospective cohort
study
Grade III-2
NT and MSS at 11-14/40 (Most had
both-possible to choose one or
both). NT measured as per FMF. 13
staff measuring NT certified by FMF.
TA or TV USS (81% had both, 18% TA,
1% TV alone). GA using CRL. Internal
and external quality control. Risk of
DS based on NT, GA, and MA
assessed by ViewPoint Fetal
Database using delta-NT method.
Women with a risk 1:250 or more
offered karyotyping.
Bloods taken immediately after USS
and blinded to the results of other
test. Sent to Statens Serum Institut
and stored at -20C. PAPP-A and
fβhCG analysed using respectively
an in–house ELISA and commercial
kit (EG&G Life Sciences). Study data
(n=2702) used for serum marker
medians, and literature (Cuckle and
van Lith, 1999 as referenced in this
paper) for correlations and DS
medians.
LR for fβhCG + PAPP-A calculated
after weight adjustment and
multiplied by the MA specific risk of
DS at term (as per Cuckle et al.
1987 as referenced in this paper).
An adjustment was made to
determine risk at screening = MA
related risk/ 0.7 (to account for 30%
fetal loss from 1st T to birth). The risk
in combined test calculated by LR
NT X LR serum.
3680 not examined (2118 not
interested, 456 “want to but can’t”,
890 miscarriage, 216 other reasons).
Removed those without living fetuses,
or CRL not 38-82 mm (after 8 months
changed to 45-82mm = 11-13+6/40).
Removed those without NT
measured. Left 8995. 8622 of which
were singleton and included in the
analysis.
Mean MA = 29.3yrs, 10.8% >35yrs
versus 14% in general population (i.e.
this group younger).
6441 singletons at right GA and had
MSS after NT.
Spectrum of disease: 12/8622 = 0.14%
15 other chromosomal
abnormalities included as
unaffected in DS analysis.
Verification
Chromosomal analysis for all
second trimester
miscarriage and cross
check with chromosomal
labs. Infants all examined by
paeds. 96.2% followed up
through patient records.
Difficulties implementing any
of the screening strategies
None noted.
Fetal loss between 1st T &
20/40 = 47.
Estimated DS at birth in this
population is 1.3-1.7%. Of 9
diagnosed prenatally, 6
would have survived to term
(30% fetal loss rate) plus the
3 live births = 9 cases (birth
prevalence of 1%).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
The age distribution in study was low–this may have
been because women with AMA were entitled to
an invasive screen so opted for no screening.
No accounting for fetal loss between screening
and term, although 2nd T fetal loss had karyotyping.
Therefore DR may have been overestimated.
May not have ascertained all the DS when look at
expected birth prevalence.
Author’s conclusions
Results confirm that combined screening in nonselected population is better than other screening
methods. Believe their focus on quality meant that
they obtained low FPR.
Reviewers conclusions
Small numbers of DS means limited applicability of
DR especially as no adjustment for fetal loss in 1st T.
However, results suggest combined better than NT,
which is better than fβHCG + PAPP-A.
38
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Avgidou et al. 2005)
Compared MA as a screen to NT,
and combined test.
Those attending an OSCAR clinic
at FMF centre in London July 1999December 2003 were offered
screening by combined test at 1113 +6/40.
Outcome
The DR and FPR for DS
screening was calculated
with the other
chromosomal disorders
removed from analysis
leaving 30430.
Accuracy of screening
methods
Limitations
Older population limits the external validity and
may have increased the DR as the prevalence
of DS was high.
(supersedes Bindra
(2002))
OSCAR clinic
(provides pretest
counseling, MSS, USS
for NT, and post test
counselling in a 1
hour visit to a
multidisciplinary
clinic)
Essex, UK
Prospective cohort
study
Grade III-2
The serum markers were
analysed using the Kryptor
analyser (Brahms).
TA USS for NT and CRL by staff
with FMF certificate of
competence in the 11-14/40
scan.
Risks calculated by multivariate
approach using published
parameters (Spencer et al. 1999
as referenced in this paper) and
the MA and GA specific risk of DS
at screening (Snijders et al. 1999
as referenced in this paper). MA
specific risk multiplied by each LR
from NT and weight adjusted
MSS. Truncated LR.
Combined risk of 1:300 offered
invasive diagnostic test.
OSCAR was carried out in 31,904
singleton pregnancies 11-13+6/40.
No outcome in 53 ToP, 120
miscarriages, and 1167 were lost to
follow-up.
Outcome in 30564.
Median maternal age was 34 yrs
(15-49yrs), 48.5% ≥ 35 yrs. Median
CRL 63mm (45-84mm).
Spectrum of disease: 196 DS/
30564 = 0.64%
Other chromosomal abnormalities
in 134.
Analysis for DS screening = 30430
MA ≥ 35 yrs
Verification
Cytogenetics lab, letters
and phone calls to
women, or GPs or
maternity units where
delivered.
Estimated DS for MA and
GA distribution at
screening would have
been 192.
DR (95%CI) for 5% FPR
MA
31.5% (24.6-37.6)
NT
81.6% (76.2-87.0)
Combined
90.3% (86.2-94.5)
FPR (95%CI) for DR of 85%
MA
52.9% (52.3-53.4)
NT
8.2% (7.8-8.4)
Combined
2.9% (2.7-3.0)
Risk cut-off 1:300
Combined
93.4% (89.0-96.1), 7.5% (7.27.8)
Difficulties implementing
any of the screening
strategies
None noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
No details of how fetal losses were followed-up.
No adjustment for fetal loss ascertainment
Authors’ conclusions
The most effective method of screening for
chromosomal defects is by first-trimester fetal NT
and maternal serum biochemistry
Reviewer’s conclusions
Large sample all had all tests.
Good quality and well designed.
39
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Montalvo et al.
2005)
Compares MA, PAPP-A, βhCG,
NT, and combined test.
Routinely screened using
combined test in all women
presenting before 14/40.
Accuracy of screening
methods
Tertiary Hospital
NT measured using methods
described by Nicolaides. TA USS
unless NT could not be measured
then TV USS. GA confirmed by
CRL (10-13/40) and BPD (1314/40).
All results corrected for MA, race,
weight, height, smoking status,
and presence of DM.
PAPP-A and fβhCG measured
using Kryptor analyser (CIS Bio
International) Population
parameters for PAPP-A and
fβhCG from those published by
Wald and Hackshaw. Marker
levels converted to MoM for GA.
Outcomes
DR and FPR for screening
for DS by MA, PAPP-A,
βhCG, NT, and combined
test were determined after
removal of 24 other
chromosomal disorders.
Limitations
Does not describe the source population so
hard to determine if study population biased.
Reasons for declining screening were not
stipulated. Some may have had large NT and
decided not to have serum screen.
Madrid, Spain
Prospective cohort
study
Grade III-2
Risk due to MA was calculated as
per Cuckle et al. The “factor of
division” applied was 0.4554.
From these determined the MoM
for CRL.
Individual risks calculated by
multivariate approach. MA
specific risk multiplied by the LR
derived for the NT and weight
adjusted serum marker levels.
Recommend invasive diagnostic
test at risk cut-off of 1:270.
Patients could also elect to have
an invasive screen.
All singleton pregnancies where
outcome known were included.
4538 pregnancies completed
screening July 1999-October 2004
included in the analysis.
Mean age was 30 yrs (14-49yrs),
25.9% > 35yrs.
Mean GA when screened
(including for NT) = 11+5/40.
19 DS/4538 = 0.42%.
24 other chromosomal disorders.
Verification
Unclear number lost to
follow-up or efforts to
determine outcome of all
pregnancies.
No details of how
outcome determined for
screen negative
pregnancies.
DR (95%CI) for 5% FPR
MA
21.1% (6.1-45.6)
PAPP-A
47.4% (24.9-69.8)
FβhCG
10.5% (1.3-33.1)
NT
63.2% (41.5-84.9)
Combined
78.9% (60.6-97.3)
FPR for 85% DR
MA
58.4% (57.0-59.8)
PAPP-A
29.4% (28.1-30.7)
βhCG
67.3% (65.9-68.7)
NT
65% (64.0-66.4)
Combined
8.6% (7.8-9.4)
Combined (1:270)
78.9% (54-93.4), 3.6 %(3.04.1)
Difficulties implementing
any of the screening
strategies
No difficulties noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Unclear how outcomes determined or how
many lost to follow-up.
Removal of other chromosomal disorders will
decrease the FPR.
No mention of quality control for NT.
Authors’ conclusions
1st T screening is efficient and its use may be
appropriate in a tertiary hospital.
Reviewer’s conclusions
Possibly biased sample. Some quality issues
such as reporting of attempts to determine
outcome. Details lacking or not clear in paper.
40
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Gonce et al. 2005)
Compared NT to combined test
Prenatal unit at
University Hospital
First 22/12 of study NT used
clinically and combined test
results analysed retrospectively
after follow-up was complete.
Last 8/12 results of combined
used clinically (interventionally).
Also offered diagnostic test if ≥ 35
yrs.
July 2001-December 2003, 103
pregnant women with TWIN
pregnancies attending the
department for prenatal care or
referred for 1st T aneuploidy
screening enrolled in the study.
Outcomes
The outcomes extracted
for this evidence table
were the DR and FPR for
screening for DS by either
NT or the combined test.
Accuracy of screening
methods DR
Limitations
Population may be high risk (referred for
aneuploidy screening) therefore external
validity may be threatened
Inclusion: twin pregnancies with
both alive at 11-14 weeks.
Verification
25 women had an invasive
procedure: 10 for positive
screen (firstly NT then
combined in 2nd period),
10 AMA, 3 parental
anxiety, and 2 had other
high risk factors.
Barcelona, Spain
Prospective cohort
study
Grade III-2
Serum taken at 8-12/40 and
assayed fresh samples (Delfia,
PerkinElmer). USS at 11-14/40. CRL
and NT measured as per FMF
guidelines. Chorionicity
determined as per Sepulveda et
al. 1996 (as referenced in this
paper).
Serum and NT converted to MoM
for GA after correction for
presence of twins. Risk
determined using Delfia software
(Wallac, PerkinElmer) by both the
NT and combined test.
In dichorionic (taken as dizygotic)
considered as having an
individual risk. Risk calculated
using individual NT and serum
marker LR (adjusted for twins as
per Spencer 2000 as referenced
in this paper)
2 pregnancies lost to follow-up. 1
pregnancy diagnostic test
cancelled on the death of fetus at
risk (observed to have
exomphalos).
Of the 100 in analysis:
Mean MA 33.3 yrs (23-42,) 36% > 34
yrs.
56% were the result of ART and 12%
were monochorionic.
No other chromosomal
abnormalities in the sample.
Median GA at serum screen =
11/40 (7.3-13.5/40), and NT screen
= 12.5/40 (10.3-14.2/40)
Other outcomes from
delivery room records or
phoning those who did not
delivery in their hospital.
DR(95% CI), FPR (95% CI)
NT (detection of
pregnancies)
100%(16-100 ), 14.3% (7.421.2)
NT (detection of fetuses)
100% (29-100), 8.6 %(4.7-12.6)
Combined (detection of
pregnancies)
100%(16-100), 5.1% (0.7-9.5)
Combined (detection of
fetuses)
100% (29-100), 8.6 %(1.0-6.1)
(Difference between NT and
combined was not
significant)
Difficulties implementing any
of the screening strategies
Deciding which result to use
for NT in monochorionic twins
(the largest smallest or
average of 2 results). Should
both have same risk.
Spectrum of disease: 3 DS/ 200
1 monochorionic pregnancy both
affected and 1 dichorionic with 1
DS fetus.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Sample was well described but not the source
population or how recruited. Unclear if
consecutive patients were enrolled.
Very small sample size only 3 DS and 200 fetuses
in 100 women.
Very wide CIs.
Author’s conclusions
The 1st T combined test appears to be more
accurate than screening with NT alone in twin
pregnancies as it maintains the DR, reduces the
FPR and allows identification of the fetus at risk.
However when correction for twins made using
distribution of own data this reduction was less
apparent. The results should be confirmed in a
larger study.
Reviewers conclusions
Small sample. It appears that the performance
of the combined test in twins is better than NT
but further large prospective cohort studies
needed.
41
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Gonce et al. 2005)
For monochorionic pregnancies,
both fetuses considered to have
same risk. Risk calculated using
the largest NT and serum marker
levels after twin correction.
Prenatal unit at
University Hospital
Barcelona, Spain
Prospective cohort
study
Grade III-2
Sample
Outcomes and
verification
Results
Twin serum levels should be
about double singletons but
in this study while PAPP-A
MoM 1.96 the fβhCG 1.57
MoM.
Risk also recalculated using the
distribution parameters for
unaffected pregnancies in this
study.
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
42
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Gyselaers et al.
2005)
Compared screening by NT,
fβHCG + PAPP-A and by
combined test.
Population had a documented
underestimation of NT
measurement compared to the
FMF.
Between 1st January 2004-30th
April 2004 13267 1st T maternal
serum samples were analysed by
AML (a lab in Antwerp).
Outcomes
The outcomes extracted
for this evidence table
were the DR and FPR for
screening for DS by NT,
fβHCG + PAPP-A, and by
combined test.
This was calculated for a
12/40 risk cut-off of 1:200
and 1:300.
Accuracy of screening
methods
DR (95% CI), FPR (95%CI)
Limitations
37 fetal losses with no karyotype - may have
been some DS. Similar methods as many other
studies so comparison with other 1st T studies
may be ok.
264 obstetric
practices (mostly
private) in 35
centres.
Flanders, Belgium
Prospective cohort
study
NT was performed according to
FMF by those accredited by FMF,
but only 6/264 FMF accredited.
They measured 11.4% of the NT
values.
2700 local NT/CRL used to
determine MoM relative to the
FMF. FMF medians used to
calculate MoM.
Analysis of PAPP-A using ELISA
(DRG International) and fβhCG
using radioimmunoassay
(Biosource). Each result adjusted
for maternal weight, multiple
gestation, smoking, and
ethnicity-converted to MoM.
Used parameters reported by de
Graaf et al. 1999 as referenced in
this paper.
Risk calculation using the
algorithm reported by Wald et al.
1988 and Reynolds et al. 1989 (as
referenced in this paper).
Samples were obtained from
women attending 264
obstetricians in 35 centres in
Flanders. In this region 95% of
prenatal care is provided by
private obstetricians.
Information sent to AML included
CRL and NT.
Exclusion: those with chromosomal
disorders other than DS (n= 23),
fetal losses where karyotype
unknown (n=37). 13207 in
screening test analysis.
Spectrum of disease: 26 DS /13230
= 0.20%.
Verification
At least once per year
obstetrician reported
outcome of all screened
pregnancies. Non
responding obstetricians
were contacted by
phone.
The estimated birth
prevalence of DS from the
MA distribution and British
DS register = 19.4.
Considering 43%
spontaneous fetal loss
from 1st T to birth and no
intervention for the 17 ToP,
then 18.7 expected at
term in study population (9
live births plus 17 x0.75)
NT
1:200 38.5% (20.0-57), 3.2%
(2.9-3.5)
1:300 42.3% (23.3-61.3), 4.8%
(4.5-5.2)
DR for 5% FPR 42.3% (23.361.3)
fβHCG + PAPP-A
1:200 80.8% (66-96), 11.6%
(11.1-12.1)
1:300 80.8(66-96), 16.8%
(16.1-17.4)
DR for 5% FPR 61.5% (42.880.2)
Combined
1:200 76.9% (60.7-93.1), 5.5%
(5.1-5.9)
1:300 80.8 (65.6-95.9), 8.6%
(8.08DR for 5% FPR 73.6% (56.090.1)
Difficulties implementing
any of the screening
strategies
Recently had reported a
systematic underestimation
of the NT MoM in this
database compared to the
FMF. Majority of those
performing the NT
measurement did less than
50 over 3 yrs.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Results of age and NT poor. Did not use
regional centre or operator specific NT values.
MoM had poor correlation with FMF values.
Those with other chromosomal disorders
removed from analysis which may slightly
decrease the estimate of FPR compared to
other studies as most include these in the
unaffected cohort.
Not blinded. When bloods sent, NT values sent
as well.
Only 11.4% had access to NT measurements as
per FMF criteria.
Authors’ conclusions
The introduction of 1st T combined screening
with unspecified USS methodologies was very
easy. The performance was less than in single
centres using FMF scanning criteria but the
easy access to screening and the contribution
from serum markers were responsible for the
majority of DS detected in this population.
Reviewer’s conclusions
The results of the NT screening may not be
applicable as most staff were not FMF trained.
43
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Soergel et al. 2006)
Comparison of 1st T screening by
MA alone, fβHCG + PAPP-A, NT,
and combined test.
Those attending 1 of 3 centres
(maternity unit of university
hospital, or 2 private prenatal
diagnosis centres) June 1998October 2002 at GA 11-14/40 were
offered screening by NT and serum
markers (PAPP-A and fβhCG).
Outcomes
Outcomes were DR and
FPR for screening for DS
using MA, NT, or the
combined test. The paper
gave FPR as FP/total
screened-this was
recalculated using
FP/unaffected.
Accuracy of screening
methods
Limitations
301 had NT then did not have MSS as either the
NT was very low and decided not to have
serum screen or NT was very high and decided
to have invasive testing. This would bias the
sample and lead to a decreased performance
of the combined test (decreased DR).
University hospital
and 2 regional
private prenatal
diagnosis centres
Hanover, Germany
Prospective cohort
study
Grade III-2
NT measured using FMF criteria
when CRL 45-84mm.
All sonographers were FMF
trained.
Serum taken and sent to lab on
same day as NT. PAPP-A and
fβhCG levels analysed using
Kryptor analyser (Brahms).
Parameters in twin pregnancies
adjusted using approach of Wald
et al. 1991 as referenced in this
paper.
Risks calculated using FMF
computer algorithm with the PIA
Fetal Database programme
(ViewPoint). Uses MA specific risk
for GA as per Snijders et al. (as
referenced in this paper).
Given partial results based on NT
results and a priori risk before
serum screen.
Risk cut-off of 1:300 used to
recommend invasive screen.
4394 had screening and 409
refused to participate. Analysis
included those with CRL 45-84 mm
(11-14/40) and with known
pregnancy outcome. Total = 2497
includes 2423 singleton and 37
twins.
1450 did not have outcome
documented as: incomplete data,
refused to give details, wrong DOB
for fetus, or other reason.
All of the 2497 had MSS, 301 had
just NT, and 2196 had both NT and
MSS.
Median MA = 32.5yrs (16-44 yrs)slightly older than general German
obstetric population (29.7yrs).
26.4% ≥ 35.
Median GA at NT =12+4/40 and
median CRL = 62mm (45-84mm).
Spectrum of disease: 11 DS/2497 =
0.44%
13 other chromosomal
abnormalities.
Twins included so analysis
is per fetus rather than per
pregnancy.
Other chromosomal
abnormalities =
“unaffected.”
Verification
Invasive test or
questionnaires about birth
outcomes given to patient
or sent to gynaecologist.
Delivery room records
cross checked.
Risk 1:300
MA
63.6% (30.8-89.1), 28.3% (2730)
NT
81.8% (48.2-97.7) , 5.1% (4.36.0)
fβHCG + PAPP-A
87.5% (47.3-99.7), 15.4%
(13.8-16.9)
Combined
87.5% (47.3-99.7), 4.0% (3.24.8)
Difficulties implementing
any of the screening
strategies
None noted
Expected DS at birth = 6
(algorithm published by
Hecht and Hook, 1994 as
referenced in this paper).
Fetal loss 12 weeks-birth =
30% leading to an
adjusted prevalence of 9
at 12/40. (6 x 1/0.7 = 6 x
1.43 =8.6 at 12 weeks).
Ascertainment is probably
OK.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Small number of DS (8 in the group having both
screening methods).
Doesn’t state attempts to karyotyping any
fetuses lost between screening and term, nor
any adjustment.
Author’s conclusions
“This provides further evidence that 1st T
screening using a combined test is effective for
the detection of DS at 11-14/40 with DR of
about 90% for FPR of about 5%”.
Reviewers conclusions
Some bias in the sample may mean the
performance of the combined test is
underestimated.
44
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Marsk et al. 2006)
Comparisons were made
between screening by MA
alone, NT, and the combined
test.
The cases and controls were
identified from the Swedish NT trial
(n=39,572). This trial randomised
women to either a 1st T or 2nd T
USS. 47 pregnancies with DS were
identified from the early scan
group and 3 controls chosen for
each case.
Outcomes
DRs and FPRs for
screening for DS (risk
1:250) using MA alone, NT,
and the combined test.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
The aim of the study was not to determine an
accurate DR and FPR rather to determine
what extent adding MSS to NT in 1st T would
change the DR and FPR in individuals and
reduce the need for invasive testing.
Stockholm, Sweden
Nested case-control
study
Grade III-2
Stored (-70C) Serum which had
been taken for Rubella
screening was reanalysed.
fβhCG and PAPP-A analysed
using commercial kits (DelfiaPerkinElmer).
Risk calculated based on MoM
and MA using Lifecycle software
(Wallac).
The controls were randomised as
close as possible to the case in
time and geography and from
within 5 yrs of MA.
Only those living in the Stockholm
area were eligible.
Verification
No details given
MA
67%(51-84), 37%(28-46)
NT
94%(79-99), 20%(13-28)
Combined
94%(79-99), 7%(2-12)
Difficulties implementing
any of the screening
strategies
None noted
Excluded those refusing to
participate, with too little serum or
serum from before 8/40 or after
14/40.
33 controls (24%) excluded and 16
DS cases (34%) excluded.
MA of cases was 38.5 yrs ± 4 (SD)
versus 35.5 yrs ± 4 (SD) which was
statistically significant (p<0.01).
Storage time did not differ
between the two groups.
The study design (case control) limits the ability
to generalise the DR and FPR calculated in the
study. The spectrum of disease may not reflect
that in the general population. 29% of the
pregnancies in the sample were pregnancies
with DS, and the sample did not contain other
chromosomal disorders.
The sample may be biased if those refusing to
participate had a different DS risk compared
to those in the analysis (e.g. if NT
measurements differed).
Unclear how DS cases had been identified.
Also, no details of verification were given. This
is important if cases had been identified
through large NT.
Stored sera used for this retrospective analysis.
This may affect the performance of the MSS.
Sample size of 139
The small number in the sample is reflected by
the wide CI’s.
Spectrum of disease: 31DS/139=
22%
Equipment provided by PerkinElmer.
Author’s conclusions
The study confirms that when 1st T MSS is
added to NT and MA the number of women
screen positive decreases without a decrease
in the DR.
.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
45
Table 10.
Source
Country
Setting
Study design
Evidence Grading
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Comparison screening
strategies
Sample
Outcomes and
verification
Results
(Marsk et al. 2006)
Comments
Reviewers conclusions
The study did not aim to accurately determine
the DR and FPR for screening for DS. The
design and possible biases mean these results
should be regarded with caution.
Stockholm, Sweden
Nested case-control
study
Grade III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
46
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(O'Leary et al. 2006)
Compared 1st T screening for DS
using NT, fβHCG + PAPP-A, and
combined test in WA.
Between August 2001 and
October 2003, 26,641 women had
1st T combined screen in this
period.
Outcomes
Outcomes were the DR
and FPR for NT, fβHCG +
PAPP-A and combined
test.
Accuracy of screening
methods
Limitations
Retrospective nature of the study means there
may have been fetal loss bias and
overestimate of performance. Also sample may
have been biased by the proportion not
completing screening (removed from analysisno further details). These may have only had NT
and declined further screening because either
NT was very high (and had invasive screen) or
very low (and had no further testing)
13 independent and
government funded
ultrasound clinics
Western Australia
(WA).
Retrospective cohort
study.
Grade III-2
Screening NT data were
obtained from all 13 ultrasound
clinics undertaking screening
across WA between August 2001
and October 2003. NT was
measured as per FMF guidelines.
Two labs provided MSS data,
using either Kyrptor analyzer
(Brahms) (92% of data) or Wallac
(PerkinElmer).
Serum markers converted to
MoM (lab specific) and adjusted
for maternal weight.
Removed twins, and “incomplete”
screening (n = 3,946) and 415 no
outcome.
Those with no outcome may have
been ToPs, spontaneous fetal
losses, or relocations out of state.
Analysis was for 22,280 singleton
pregnancies between 11-13/40.
Median MA = 31 yrs (14-47).
Compared with 29 yrs for all WA
women giving birth in same
period. GA for NT = 12+4/40, and
for serum = 12+3/40.
Spectrum of disease: 60DS/22,280
= 0.27%
78 other chromosomal disorders.
The FPR given in the paper
was FP/"all screened”.
FP/unaffected was
calculated for this table.
Outcomes obtained by
linking screening data to
outcome data using
probabilistic recordlinkage.
Statewide data
collections (registries for
midwives notifications,
birth defects, and hospital
separations) combined
with providers screening
data.
DR (95%CI),FPR (95%CI)
(1:300)
NT
73% (62-85), 8.6% (8.2-8.9)
fβHCG + PAPP-A
85% (76-94), 11.5% (11.111.9)
Combined test
83% (74-93), 3.7% (3.5-4.0)
Difficulties implementing
any of the screening
strategies
None noted.
78 other chromosomal
disorders included in
analysis as unaffected.
Verification
As above review of
Midwives Notification
System and the Birth
Defects Registry between
August 2001-October 2003
(children were aged 3/1230/12).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
No adjustment for fetal loss between screening
and term.
Few details available for how risks calculated
(which parameters were used etc).
Authors’ conclusions
This study provides evidence that 1st T
combined screening performs well compared
to that predicted by clinical trials.
Reviewer’s conclusions
While the study appears well planned and the
sample was large and representative of the
general population, the design (retrospective)
makes it difficult to avoid bias such as
verification bias.
47
Table 10.
Source
Country
Setting
Study design
Evidence Grading
(O'Leary et al. 2006)
13 independent and
government funded
ultrasound clinics
Western Australia
(WA).
Retrospective cohort
study.
Grade III-2
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Birth Defects Registry
includes ToP for fetal
abnormalities and has
been validated.
All true positives for DS had
invasive screen.
Estimated DS for MA
distribution = 43.5. With
fetal loss from 12/40-birth
adjustment of 25% = 58
(95% CI 57-63) (Multiply
43.5 by 0.75 = 58).
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
48
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Spencer et al. 2000a)
The aim of the study was to clarify whether
total hCG is a marker of DS in 1st T of
pregnancy.
Three groups of women
comprised the study group.
Outcomes
DR for fixed 5% FPR for 1st
trimester screening with
AFP, total hCG, AFP + total
hCG, PAPP-A + total hCG,
and PAPP-A + fβhCG.
Accuracy of screening
methods (from text only % DR
given)
Limitations
Biased sample. Of the 130 DS some were already
screen positive by NT and 1st T MSS.
DR for fixed FPR 5%
1st T AFP
31%
1st T total hCG
31%
1st T AFP, total hCG
40%
1st T PAPP-A, total hCG
52%
1st T PAPP-A, free βhCG
67%
Some of the markers analysed on stored samples.
Case samples stored considerably longer than
control samples.
Statistical Modelling
Analysed AFP and total hCG in large series
of DS comparing these with other markers in
1st T.
Regression analysis to determine relationship
between marker level and gestational age.
Converted each level to MoM for the
gestational age. Performance modelled
using standard modelling techniques as per
Royston and Thompson. Observed
population parameters for AFP and total
hCG.
Observed parameters for total hCG and AFP
and Spencer et al. 1999 for others.
15,000 MoM generated for each marker
from the Gaussian distributions of the log
MoM affected and unaffected
pregnancies.
Values then used to calculate likelihood
ratios with MA specific risk of DS in1st T for a
population with a MA distribution of England
and Wales.
The first was women with
singleton pregnancies who
were referred to the Harris
Birthright Centre for fetal
karyotyping because of MA
and NT screening at 10-14
weeks high risk for DS.
2nd group women self
referred for assessment of
risk. Blood collected from
women at time of NT and
serum stored -20C (before
blinded retrospective
analysis). Gestational age
from CRL.
Outcome ascertained in all
women. 90 cases of DS part
of previous study.
To supplement these, third
group of 40 samples from
cases of DS from a Glasgow
centre part of the
Combined Ultrasound and
Biochemistry Study in
Scotland. In this series total
hCG AFP PAPP-A and
fβhCG all done at same
time.
Results also given for PAPPA + total hCG using GA
specific parameters.
Verification
Outcome obtained in all
pregnancies.
Controls resulted in the birth
of unaffected babies
DR using population
parameters specific to the
gestational age Fixed 5% FPR
total hCG & PAPP-A 70-83
days
47%
total hCG & PAPP-A 84-97
days
60%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Observed parameters for total hCG and AFP and
those from Spencer et al. 1999 (as referenced in
this paper) were adopted for other variables
Acknowledge the support of CIS in providing
reagents and instrumentation.
Author’s conclusion
“This median shift has significant implications for
interpreting previous studies and even more
significant implications for DRs. This observation
explains much of the confusion around total hCG
in the first trimester and shows the importance of
selecting analyte pairs and population
parameters appropriate to the time in gestation
when screening is performed.”
49
Table 10.
Source
Country
Setting
Study design
Evidence Grading
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Comparison Interventions
Sample
(Spencer et al. 2000a)
(total 130 DS cases)
Statistical Modelling
Median MA cases 37 (1745)
Gestational age at storage
time 86 days (43-97)
CRL 61mm (42-84)
Sample storage time 937
days (150-2317).
Continued
Outcomes and
verification
Results
Comments
Difficulties implementing any
of the screening strategies
Performance of PAPP-A + total
hCG worse using parameter
before 84 days.
Reviewers’ conclusions
When PAPP-A + total hCG analysed using
appropriate parameters screening performance
similar to PAPP-A, free βhCG at 84-97 days.
Controls 10-14/40 obtained
from samples taken as part
of the routine 1st T
screening in OSCAR clinic
(Harold Wood). PAPP-A and
free βhCG taken then
samples frozen -20C.
Further 90 specimens
obtained from the Glasgow
centre.
Total of 959 controls used to
establish medians and for
reference data.
Median MA controls 28.8
(15-45)
Gestational age storage
time 83 (42-97)
CRL 56mm (36-84)
Sample storage time 435
days (350-502)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
50
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Christiansen and
Olesen Larsen 2002)
The contingent screening was compared
to 1st T MSS, NT, and 1st T combined test.
Monte Carlo
simulation
The aim of the study was to assess the
discriminatory efficiency and costeffectiveness of a 1st T contingent
screening method compared to 1st T
combined screening.
The protocol involved all women having
1st T MSS (PAPP-A and β hCG) prior to
11/40 and only those with an
intermediate risk (including MA
associated risk) having NT and those with
very high risk having an invasive screen
(CVS). The reasoning was to explore the
possibility of rationing NT which requires
training, expensive equipment and
extensive quality control.
Sample
Outcomes and
verification
Results
Comments
Outcomes
DR and FPR of 1st T
Contingent
Screening, 1st T MSS, NT,
and combined test for a
fixed cut-off.
Accuracy of screening
methods
Limitations
Distribution of serological markers from three
different sources with no description of two of
these populations.
DR, FPR (risk cut-off for
double screen of 1:1000,
and final risk 1:400)
1st T Contingent
78.9%, 4%
PAPP-A + β hCG
74.2%, 9.6%
NT
74.0%, 5.7%
Combined test
85.5%, 4.4%
(Only 19.4% of women
offered NT testing.)
Distribution of 1st T serological markers
from literature (Cuckle) and 2nd T from
Wald (1994)
NT distribution from a large UK
multicentre study (Nicolaides).
MA distribution was standardised (Van
de Veen).
MA related risk of DS based on formula
from Cuckle and refers to risk at term.
Monte Carlo simulation used to evaluate
performance of different screening
methods.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Author’s conclusion
Contingent testing can reduce costs with a
small decrease in performance. Contingent
testing is attractive in areas where there is
restricted access to NT screening preventing
the introduction of 1st T screening. We have
shown here that NT screening need not be
applied to the whole population in order to
reach a satisfactory 1st T screening
performance.
Reviewers’ conclusions
As per authors’ conclusions this strategy shows
promise. Needs prospective cohort study.
51
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Christiansen and
Olesen Larsen 2002)
For estimates of the DR and FPR for
contingent screening firstly determined
the distribution of risk values after
serological screen. Used the published NT
distributions to determine the cut-off of
the serological marker risk, where no NT
measurement could reduce the final risk
to <1:400.
Monte Carlo
simulation
Continued
Sample
Outcomes and
verification
Results
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
52
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Spencer et al. 2002)
The aim of the study was to examine the
values of HhCG (hyperglycosylated) with a
sialic acid-specific lectin immunoassay in 1st
T of pregnancy.
Maternal serum samples
from unaffected and DS
pregnancies from women
attending Harold Wood
hospital. Collected as part
of research studies in to 1st
T screening since 1998 as
part of routine screening
OSCAR incorporating
PAPP-A, fβhCG, USS for CRL
and NT by FMF trained
ultrasonographers.
Outcomes
DR for fixed 5% FPR for
HhCG alone and in
combination with
conventional markers in a
population with the MA
distribution of pregnancies
in England and Wales 19971999.
Accuracy of screening
methods
Limitations
Means from small sample for HhCG
DR at fixed 5% FPR
ThCG
37.0%
HhCG
48.6%
ThCG & PAPP-A
49.0%
fβhCG
49.5%
PAPP-A
50.8%
HhCG & PAPP-A
61.2%
fβhCG & PAPP-A
69.5%
NT
73.5%
NT & ThCG
75.5%
NT, ThCG & PAPP-A
78.7%
NT & HhCG
79.9%
NT and fβhCG
80.1%
NT & PAPP-A
81.2%
NT, HhCG and PAPP-A
83.0%
NT, fβhCG and PAPP-A
88.9%
Controls and cases had different storage time. DS
stored longer and although not thawed since
collection may have influenced the results.
Statistical modelling
Results of a case-control study used for
model.
Maternal serum fβhCG, PAPP-A and ThCG
were measured using commercial kits
(Brahms).
Maternal serum HhCG measured at two
dilutions in singleton pregnancies using the
lectin immunoassay. Used the means of the
two results corrected for dilution in analysis.
Analysis of samples blinded to outcomes.
All marker levels converted to MoM for
unaffected pregnancies at the same
gestational age using previously described
relationships (Ong et al. 2000 and Spencer
et al. 2000a as referenced in this paper)
and for HhCG from this study.
Correction for maternal weight as per
Neveux et al. 1996 as referenced in this
paper.
Statistical modelling was performed (as
described by Royston and Thompson, 1992
as referenced in this paper) in order to
generate a series of 15000 random MoM
values for each marker from the Gaussian
distribution of the log10 MoM for DS and
unaffected pregnancies.
Maternal serum had been
stored at -20C.
224 unaffected and 54 DS
were retrieved from the
archive.
DS
MA 36.1 years (20-44)
Gestational age days 87
(73-97)
CRL 62mm (38-85)
Storage sample time 1187
days (147-2354)
Controls MA 30.4 (16-41)
Gestational age 84days
(70-96)
CRL 55mm(33-80)
Sample storage time 127
(116-1460)
Difficulties implementing any
of the screening strategies
None noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Authors’ conclusion
“Maternal serum HhCG is unlikely to be of
additional value when screening for DS in 1st T”
Reviewers’ conclusions
As per authors’ conclusions.
53
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Spencer et al. 2002)
The parameters for HhCG were derived
from this study, those for ThCG from
Spencer et al. 2000a, those for fβhCG and
PAPP-A and NT from Spencer et al. 1999 (as
referenced in this paper).
Statistical modelling
Continued
Sample
Outcomes and
verification
Results
These were used to calculate LR and
combined with MA specific risk of DS (using
Snijders et al. 1999) to calculate the DR in a
population with the MA distribution of
pregnancies in England and Wales 19971999.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
54
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Spencer and Cuckle
2002)
The aim of the study was to assess the within
person variability of 1st T MSS markers and to
see whether repeat measures of PAPP-A
and fβhCG during 1st T would increase DR.
Harold Wood Hospital Essex.
Outcomes
Compared screening using
one sample to using two
samples at 10/40 and
12/40, with and without NT.
Accuracy of screening
methods
Limitations
Estimates only for the DS correlation (no DS cases
in the sample).
Statistical Modelling
All women who book for maternity care are
offered an appointment at the OSCAR clinic
of 11/40.
At this appointment MSS is done and then
USS. Those having USS who are noted to
have CRL less than 45mm are given a further
appointment to attend for NT when GA is
between 11/40 and 13+6/40 (as the FMF
algorithm is based on data 11-14/40). A
further MSS is therefore taken at this repeat
appointment.
fβhCG and PAPP-A analysed using Kryptor
analyzer (Brahms). Samples analysed
straight away.
Converted to MoM using previously
established GA and maternal weight
adjustments. 261 pairs of data available
(unaffected fetuses) 10-13+6/40.
In routine practice about
8% initially attend when GA
too early for NT and so
need a repeat serum
sample.
261 pairs of data were
available for analysis over a
three year period. All were
unaffected pregnancies.
Median MA = 28.97.
95% Caucasian.
Median GA 1st sample:
10.7/40
Median 2nd sample: 12.6/40
DR For a fixed 5% FPR.
PAPP-A + β hCG at 10/40
67%
PAPP-A + β hCG at 10/40 & NT
87.2%
PAPP-A + β hCG at 12/40
67%
PAPP-A + β hCG at 12/40 & NT
87.3%
PAPP-A + β hCG at 10/40 & at
12/40
70.5%
PAPP-A + β hCG at 10/40 &
12/40 & NT
88.6%
Difficulties implementing any
of the screening strategies
None noted.
The standard deviation of fβhCG and PAPPA in each sample was estimated, and the
correlation between the markers, within and
between the two samples, was determined
excluding outliers.
Statistical modeling was used to predict DR
for a fixed FPR of 5%.
Modelling by numerical integration method
(as per Royston and Thompson) used to
model risks over a multivariate Gaussian
distribution of log marker levels and the
observed distribution of MA.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Small sample.
Authors’ conclusion
When women present twice in 1st T it might be OK
to include both measures. However, no
justification for taking two samples routinely.
Reviewer’s conclusions
As per authors conclusions.
55
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Spencer and Cuckle
2002)
NT parameters from FMF study (Nicolaides et
al. 1998 as reference in this paper).
Parameters for unaffected MSS markers
were from their own series and means taken
to be 1 MoM. For DS the SD and correlation
coefficients from a meta-analysis of the
difference between the variancecovariance matrices of affected and
unaffected pregnancies (as described by
Cuckle and van Lith 1999 as referenced in
this paper).
Statistical Modelling
Continued
Sample
Outcomes and
verification
Results
The means for DS for 1st and 2nd sample
taken as those for 10 and 12/40 respectively.
Assumed NT independent of MSS markers in
MoM.
MA specific risk derived from published
meta-analysis (Cuckle et al. 1987 as
referenced in this paper) and the MA
distribution was that of England and Wales
1994-1998. Truncation limits applied to the
MoM outside a certain range.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
56
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Christiansen and
Jaliashvili 2003)
The aim of the study was to determine the
performance of PAPP-A using a polymonoclonal assay to see whether it is as
efficient as double monoclonal assay in
discriminating between DS and unaffected
pregnancies.
Samples obtained through
1st T MSS screening
programme for syphilis and
other diseases from Statens
Serum Institute.
Outcomes
For this evidence table the
DR and FPR of PAPP-A in
combination with age,
βhCG and NT were
extracted from the paper.
Accuracy of screening
methods (DR,FPR)
Limitations
Data susceptible to biases typical of case control
studies: particularly selection bias.
Normal controls-i.e. no other chromosomal
disorders.
Monte Carlo
simulation
An in house poly-monoclonal assay for
PAPP-A was developed and performed as
detailed in the paper.
All PAPP-A measurements were converted
to the MoM of unaffected pregnancies for
the gestational age.
Distribution data for the other 1st T serum
markers (βhCG and NT) were obtained from
a recent meta-analysis (Cuckle and van
Lith 1999 as referenced in this paper).
DR in a population were estimated with a
Monte Carlo simulation using MA specific
risk (Cuckle et al. 1987 as referenced in this
paper) and a standardized age distribution
of women giving birth (van der Veen et al.
1997).
All simulations were done with 100,000
cases.
Truncation limits for PAPP-A were applied as
detailed in this paper.
39 DS and 167 controls with
normal pregnancy
outcome.
Samples collected as part
of another study. All
samples stored under
identical conditions.
Gestational age from LMP
and in most cases
confirmed by USS.
All DS diagnosed in 2nd T as
a result of screening or at
birth (i.e. would not be
biased by being screen
positive or negative cases
already by another serum
test).
Verification
All DS verified by
karyotyping.
No other information.
PAPP-A
Risk 1:100 50.1%, 2.3%
Risk 1:250 66.7%,6.4%
Risk 1:400 74.5%,10.2%
DR at 5% FPR 62%
PAPP-A, βhCG
Risk 1:100 61.8%, 2.1%
Risk 1:250 75.5%, 5.3%
Risk 1:400 81.3%, 8.1%
DR at 5% FPR 74%
PAPP-A, βhCG, NT
Risk 1:100 79.4%, 1.1%
Risk 1:250 85.9%, 2.7%
Risk 1:400 88.8%, 4.0%
DR at 5% FPR 90%
Difficulties implementing any
of the screening strategies
The simplicity of the detection
technology of the assay is
obtained at the expense of
the possibility of automation.
Automation reduces the risk
of human error. However felt
this could be suitable in smallmedian lab if results not
required within less than 5
hours.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Small sample for parameters of PAPP-A especially
for DS pregnancies.
Unclear if there was blinding to outcome.
Author’s conclusion
In conclusion we have described a high
performance PAPP-A assay.
Reviewers’ conclusions
Some limitations in design and information about
the population.
57
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Laigaard et al. 2003)
The aim of the study was to assess ADAM12
as a 1st T and 2nd T marker for DS.
Unaffected samples from
1st T pregnant women 154
obtained as part of routine
screening for DS in a
university hospital Denmark.
Screening at 8-13/40 and
also have USS.
Outcomes
The outcomes extracted
were the DR and SPR for
ADAM12, PAPP-A, fβhCG
and NT alone and
combined at risk cut-offs of
1:200 and 1:400.
Accuracy of screening
methods
Limitations
Very small samples e.g. for DS 1st T =18
All with age DR, SPR
In-house ELISA.
ADAM12
1:200 77.7%,1.5%
1:400 81.5%, 3.2%
No other details of length of time in storage or
details of MA, ethnicity gestational age.
Verification
All DS by karyotyping.
PAPP-A
1:200 52.3%, 5.1%
1:400 66.2%, 11.2%
Monte Carlo
simulation
An ELISA (enzyme-linked immunosorbent
assay) for the quantification of ADAM12 (A
disintegrin and metalloprotease) was
developed.
Median ADAM12 concentrations were
estimated for the gestational age. Marker
levels were converted to the MoM of
unaffected pregnancies. Compatibility with
the normal distribution assessed using normal
plots. Monte Carlo simulation done using a
standardised age distribution (van der Veen
et al. 1997 as referenced in this paper). The
MA specific risk was taken from Cuckle et al.
1987. The distribution parameters for PAPP-A,
βhCG and NT were taken from published
meta-analysis (Cuckle and van Lith, 1999).
Risks for cut-offs were 1:200 and 1:400 for
term. ADAM12 in DS did not differ from
unaffected in 2nd T so no further analysis
was done.
2nd T unaffected screening
sample obtained from 91
women in another
screening programme
(prenatal screen for severe
malformations and DS at
Statens Serum Institute).
Women 14-20/40-no further
analysis of 2nd T done.
All these samples 1st T and
2nd T were kept cool (4C)
before postage.
DS samples 1st T samples
n=18. Some were from the
same University hospital
programme (n=3) and were
identified as part of the
programme (i.e. already
screen positive) and 15
samples from the quality
control programme at
Statens Serum Institut
diagnosed (2nd T, n= 10) or
at birth ( n=5).
βhCG
1:200 42.4%, 5.1%
1:400 59.9%, 12.9%
NT
1:200 67.4%, 2.8%
1:400 74.3%, 5.9%
ADAM12 and βhCG
1:200 82.8%, 1.5%
1:400 86.3%, 3.1%
Only the 3 from University hospital were taken at
the same time as the controls and were recent
whereas the other 1st T DS samples (n=15) were
stored at -20C for many years.
Only 3 DS (and 154 unaffected) used for relation
between ADAM12 and PAPP-A and βhCG.
Used 15 DS from the Staten Serum Institut where
the same analysis had been done for βhCG and
PAPP-A.
No other details of length of time in storage or
details of MA, ethnicity gestational age.
Author’s conclusion
ADAM12 and βhCG and PAPPA
1:200 85.4%, 1.6%
1:400 88.7%, 3.0%
While further prospective studies are clearly
needed the data here suggest that ADAM12 is a
potentially valuable marker for use in prenatal
screening
ADAM12 and βhCG and PAPPA and NT
1:200 92.4%, 0.8%
1:400 94.1%, 1.5%
Reviewers’ conclusions
While results suggest the ADAM12 may be
discriminatory the study was potentially biased
and had a small sample (especially for DS). Needs
further large prospective studies.
Difficulties implementing any
of the screening strategies
None noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
58
Table 10.
Source
Country
Setting
Study design
Evidence Grading
(Laigaard et al. 2003)
Monte Carlo
simulation
Continued
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Comparison Interventions
Sample
Outcomes and
verification
Results
Only the 3 from University
hospital were taken at the
same time as the controls
and were recent whereas
the other 1st T DS samples
(n=15) were stored at -20C
for many years.
2nd T DS samples n=12 were
all from quality control
programme at Statens
Serum Institut diagnosed in
2nd T (n=8) or at birth (n=4).
(Biased as already positive
by 2nd T screening).
Gestational age from LMP
with most confirmed by USS.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
59
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Palomaki et al. 2005)
Compared screening using ITA (HhCG) in
the 1st T to using PAPP-A +fβhCG or PAPP-A
+hCG with and without NT. Also compares
screening in 1st T using DIA.
The maternal samples were
collected between 1994
and 1996 as part of a
previous trial. 16 centres in
California and elsewhere in
the USA recruited women
already scheduled to have
amniocentesis or CVS at 915/40.
Outcomes
The paper reports the
performance of ITA and
other 1st T serum markers at
various fixed FPR and fixed
DR and for various risk cutoffs. The performance is
also stratified by week of
gestation. For this evidence
table the data for DR and
FPR for 5% FPR, 85% DR and
cut-off of 1:250 has been
extracted. These are given
for weeks 11-13/40
combined.
Accuracy of screening
methods
Limitations
Model used data with a small sample and casecontrol design but appeared to be nested in
another study.
Statistical modelling
As part of an earlier observational study,
serum samples from 54 DS and 276 matched
unaffected controls were collected
between 9 and 15/40
Samples had been aliquoted and stored at 20 degrees C for 8 years. ITA was measured
and converted to weight-adjusted multiples
of the median (MoM). The distributions of
other 1st T markers are from a single
published study.
Serum collected before amniocentesis and
assayed for AFP, uE3, hCG, fβhCG and
PAPP-A then aliquoted and stored at -20C.
Case control series was constructed: 5
controls matched for each case of DS.
Matched for time in storage, MA,
gestational age, “race”, site where sample
obtained.
Mostly was for AMA.
Collected demographic
info including how dated,
weight, “race”, diabetic
status, gestational age
based on USS BPD or CRL,
and LMP
None had had serum
screen or NT in this
pregnancy.
54 DS and 276 matched
controls
9-15/40 gestation
For this study a “never thawed” aliquot was
available for 54 DS and 276 controls. These
330 samples sent (blinded) to Quest for ITA
measurement using automated
immunochemiluminometric assay (minimal
cross reactivity with hCG).
No further details of this
sample.
Verification
Amniocentesis
DR For a fixed 5% FPR (all with
MA and for 11-13/40
combined).
PAPP-A & fβhCG
67%
PAPP-A & hCG
64%
PAPP-A & ITA
67%
PAPP-A, fβhCG & NT
84%
PAPP-A, hCG and NT
84%
PAPP-A, ITA & NT
84%
PAPP-A, fβhCG, DIA & NT
88%
PAPP-A, hCG, DIA and NT
87%
PAPP-A, ITA, DIA & NT
87%
PAPP-A, fβhCG, & ITA
72%
PAPP-A, fβhCG, ITA, and NT
86%
PAPP-A, fβhCG, ITA, DIA and
NT
88%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Mostly AMA.
Some support from screening industry for the
study. Partially funded by Quest Diagnostics, and
Quest Diagnostics also assisted in the assaying of
the samples for various biomarkers. One author
worked for Quest.
Author’s conclusion
Serum ITA appears to be a useful first-trimester DS
marker that could replace fβhCG measurements
while maintaining performance.
Reviewers’ conclusions.
The use of ITA as a 1st T marker shows promise but
needs further investigation.
60
Table 10.
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Palomaki et al. 2005)
All results converted to MoM and corrected
for maternal weight (Neveux 1996).
Adjustments to the other variables and
population variables published elsewhere
(Wald et al. 1988 as referenced in this
paper).
Statistical modelling
Continued
SD of ITA in DS adjusted to take into
consideration the varying concentrations by
gestational week.
Correlation coefficients between ITA and
serum markers in 2nd T DS and unaffected
were derived after exclusion of outliers.
Correlation between NT and ITA in DS and
unaffected assumed to be zero.
Screening performance modelled for
combinations of serum ITA and other 1st T
serum markers with and without NT.
Modelling method based on overlapping
Gaussian distributions as described
elsewhere.
Used MA age distribution of the USA for
2000.
Sample
Outcomes and
verification
Results
FPR For a fixed 85% DR (all with
MA and for 11-13/40
combined).
PAPP-A & fβhCG
16%
PAPP-A & hCG
20%
PAPP-A & ITA
16%
PAPP-A, fβhCG & NT
5.6%
PAPP-A, hCG and NT
6.8%
PAPP-A, ITA & NT
5.6%
PAPP-A, fβhCG, DIA & NT
3.7%
PAPP-A, hCG, DIA and NT
3.7%
PAPP-A, ITA, DIA & NT
3.8%
PAPP-A, fβhCG, & ITA
12%
PAPP-A, fβhCG, ITA, and NT
4.3%
PAPP-A, fβhCG, ITA, DIA and
NT
3.2%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
61
Table 10.
Source
Country
Setting
Study design
Evidence Grading
(Palomaki et al. 2005)
Statistical modelling
Continued
Evidence table of primary research studies appraised investigating the accuracy of first trimester combined screening compared to components
(continued)
Comparison Interventions
Sample
Outcomes and
verification
Results
Risk cut-off of 1:250 DR, FPR (all
with MA and for 11-13/40
combined)
PAPP-A & fβhCG
78%,11%
PAPP-A & hCG
76%, 11%
PAPP-A & ITA
81%, 12%
PAPP-A, fβhCG & NT
85%, 5.8%
PAPP-A, hCG and NT
84%, 5.8%
PAPP-A, ITA & NT
86%, 6.3%
PAPP-A, fβhCG, DIA & NT
87%, 4.9%
PAPP-A, hCG, DIA and NT
87%, 5.1%
PAPP-A, ITA, DIA & NT
88%, 5.4%
PAPP-A, fβhCG, & ITA
82%, 9.9%
PAPP-A, fβhCG, ITA, and NT
87%, 5.6%
PAPP-A, fβhCG, ITA, DIA and
NT
88%, 5.1%
Difficulties implementing any
of the screening strategies
None noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
62
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
63
Chapter 4: Comparison of Second
Trimester Screening Strategies
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY
The search identified 13 eligible papers comparing the accuracy of second trimester screening
strategies. Below is an overview of study designs and aspects of quality represented by these studies.
Full details of the papers appraised, including methods, key results, limitations and conclusions, are
provided in evidence Table 13 (pages 69-84). Studies with directly observed DRs and FPRs are
presented first, followed by studies where the results are estimations of performance using statistical
modelling. For each of these two groups of papers, studies are presented in chronological order of
publication.
Study design, and grading
All 13 papers appraised in this chapter are based on primary research; there were no papers based on
secondary research that fitted the inclusion and exclusion criteria of the review protocol. Of the 13
papers comparing second trimester screening tests, ten reported directly observed comparisons of
performance, two of which also presented some results estimated by statistical modelling (Monte Carlo
simulation. Three other papers only reported comparisons of DR and FPR estimated by modelling.
Of the papers reporting directly observed comparisons, five studies used a cohort study design and
sample sizes ranged from 2,833-854,902. Two of these studies were retrospective analyses of screening
(Benn et al. 2003; Muller et al. 2002a). There were five case-control studies with sample sizes ranging
from 100 to 1128.
While all these studies were graded III-2 as per NHMRC, as discussed in chapter 2, the ideal design for
determining the DR and FPR of a screening strategy is a large prospective cohort study (or nested casecontrol study) where all receive the screening tests/methods being compared (Deeks 2001).
Study setting and samples
In one of the cohort studies the population consisted of women with twin pregnancies (Muller et al.
2003b). In this paper the proportion of DS in the analysis was 0.25%. In another cohort study the
population was high risk: all were having amniocentesis for advanced maternal age or because they
were considered high risk for other reasons (Huderer-Duric et al. 2000). Seventy three percent of
women in the population were aged 35 years and over, and the proportion of DS pregnancies in this
analysis was 0.42%. For the other three cohort studies the population was a routinely screened
population and the proportion of DS cases ranged from 0.11% to 0.19%. One of the cohort studies
removed other chromosomal disorders from the analysis, while for the remaining four papers it appears
they were included in the analysis as unaffected cases.
The proportion of DS in the case-control studies ranged from 6% to 17%. The samples in the casecontrol studies consisted of cases (DS) and unaffected controls. The papers either expressly excluded
other chromosomal disorders or it can be assumed there were no chromosomal disorders apart from DS
in the analysis.
Comparison screening methods
The screening tests/methods compared in this chapter are:
ƒ
ƒ
MA: either ≥ 38 years or ≥ 35 years.
Double test: AFP and hCG (fβhCG or total hCG)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
64
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
Triple test: AFP, hCG (fβhCG or total hCG) and uE3
Quad test: AFP, hCG (fβhCG or total hCG), uE3 and inhibin
Lens culinaris agglutinin-reactive AFP (expressed as a percentage of total AFP).
Human Placental Growth Hormone (hPGH)
Invasive trophoblast antigen (ITA) - formerly called hyperglycosylated hCG (HhCG).
hCG glycoforms (GlyhCG)
unless otherwise stated all screening strategies incorporate the individual’s maternal age.
Three case-control studies analysed some of the markers using stored samples. This may bias results if
there was a difference in storage times between cases and controls or if some markers were stored
where others were analysed using fresh samples. In one study (Baviera et al. 2004) hPGH was analysed
using stored specimens whereas TT markers were not (storage times were the same for cases and
controls), and in another study inhibin and uE3 were analysed using stored specimens and AFP and
hCG using fresh serum samples (case specimens were stored for a longer period) (Harrison and Goldie
2006). Two of the modelling papers used data from populations where stored samples had been used
either for one of the markers (Palomaki et al. 2004), or for all marker levels, but where population
parameters for one of the markers had been obtained from these samples, while the other parameters
were obtained from the literature (Talbot et al. 2003). In both these papers either cases or controls were
matched for storage time, or there was no difference in storage time between cases and controls.
All papers in this chapter except one used conventional methods to combine maternal age specific risks
and marker levels to determine an individuals risk and therefore the DR and FPR (i.e. using
multivariate Gaussian distributions). The paper in question established a unique scoring system, based
on the marker profile in relation to the median level of markers in unaffected pregnancies (Azuma et al.
2002). The scoring system did not incorporate the maternal age specific risk of DS.
Where details were given in the paper all serum markers were analysed using commercial kits and
individual risks were established using commercially available software.
Outcomes
Where a large number of results for different risk cut-offs, fixed FPRs or DRs have been reported (e.g.
for modelling papers) a fixed FPR of 5% and/or a fixed DR of 85% have been selected for the evidence
table. While studies report DR for fixed FPR in reality the cut-off chosen for screening programmes is
an individual’s risk (Benn and Donnenfeld 2005).
In the four of the five cohort studies it appears that any pregnancies affected by other chromosomal
disorders (e.g. trisomy 18) have been included as “unaffected” pregnancies for analysis of screening
accuracy, and so will contribute to false positive and true negative results. As discussed previously,
these cases are not strictly false positives (as a positive screen is clinical relevant), but it is appropriate
when calculating the performance of screening for DS to include these cases in the unaffected group.
PRIMARY RESEARCH: STUDY RESULTS
Accuracy of screening methods
Maternal age alone as a screening test.
Four studies had results for maternal age alone as a screen test. These results are presented in Table 11.
In two studies, maternal age was clearly inferior to any of the other strategies used: specifically the DR
was lower and the FPR was higher than for the other screening methods (Benn et al. 2003; Wald et al.
2003a). In one national study of the performance of maternal serum screening in the 2nd Trimester
(using triple test or double test), maternal age (≥ 38 years) had a lower DR (9.5%) compared to 2nd
trimester screening (73.5%) but a lower FPR ( 9.5% compared to 1.6%) (Muller et al. 2002a).
However, while the results for maternal age as a screening test could be extracted from the data this
was not the aim of the paper. As per the national policy those aged 38 years or older were offered
amniocentesis, and so only 1.7% of the population included in the study were over 38 years old (Muller
et al. 2002a). Another paper, a study of screening for DS in twin pregnancies, found that maternal age
as a screen (adjusted for twins) had a lower DR but a superior (lower) FPR compared to various double
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
65
test strategies (Muller et al. 2003b). Maternal age with a correction for the risk of DS in those with
dichorionic pregnancies had a DR equal to the double test but a higher FPR.
Overall, the literature supported the low predictive performance of maternal age compared with other
screening strategies in the second trimester.
Table 11.
Comparison of DRs and FPRs, maternal age versus other screening strategies
Reference
(Muller et al. 2002a)
(Wald et al. 2003a)
Test
TT & double (1:250)
MA ≥ 38 years
Quad (1:300)
MA ≥ 35 years
DR for fixed FPR of 5%
MA
Double
TT
Quad
(Benn et al. 2003)
(Muller et al. 2003b)
(twins)
DR for fixed FPR of 5%
& fetal loss adjustment
MA
Double
TT
Quad
Modelled (1:270)
MA ≥ 35 years
TT
Quad
Risk cut-off 1:250
MA ≥ 37 years
MA correct. dichorionic
Double-observed MoM
Double-twin median
Double- mono- or
dichorionic twin median
DR (%), (95% CI)
73.5 (70.1-76.2)
9.5 (8-11)
81 (72-89)
51 (41-62)
FPR (%), (95% CI)
6.85 (6.80-6.90)
1.6 (1.59-1.65)
7 (6.7-7.2)
14.3 (14.0-14.7)
26
61
66
75
5
5
5
5
(17-35)
(51-72)
(56-76)
(66-84)
24
57
62
70
5
5
5
5
53.3
79.3
83.8
17.1
10.4
9.9
27.3
54.5
54.5
54.5
54.5
(6-61)
(25-84)
(25-84)
(25-84)
(25-84)
6.5
24.4
7.6
7.9
7.6
(5.6-7.4)
(23-26)
(6.6-8.5)
(6.9-8.8)
(6.6-8.5)
Quad versus triple test and double test
Five studies were identified that included results for the validity of the quad test and had comparisons
with the triple test. Three papers also had results for the double test. The results for papers comparing
the quad test with the triple test and the double test are summarised in Table 12. These comparisons
took different forms. One study presented the results for a fixed cut-off of 1:250 (observed and
modelled), for a fixed 3% FPR, and for a fixed 75% DR (Harrison and Goldie 2006). Two papers just
gave results for a fixed 5% FPR (Palomaki et al. 2004; Wald et al. 2003a) and two papers provided
results for a 2nd trimester cut-off of 1:270 (Benn et al. 2003; Benn et al. 2001). It should be noted that
in some of these studies there were a wide range of other tests included.
The quad test consistently performed better than TT which in turn performed better than the double
test. The one exception to this was in a study where the quad test performed better than both TT and
double test except for the observed results for a cut-off of 1:250 where the DR was higher but the FPR
was also slightly higher (6.6 versus 6.7 ) for the quad test compared to the TT (Harrison and Goldie
2006).
A further study only had results for the TT and the double test but not the quad test ( and so was not
included in Table 12) (Huderer-Duric et al. 2000). In this study at a risk cut-off of 1:100 TT had a
clearly better DR but higher FPR compared to the double test.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
66
Table 12.
Comparison of performance of the quad test, triple test, and double test.
Reference
(Wald et al. 2003a)
(Benn et al. 2003)
(Harrison and Goldie
2006)
(Benn et al. 2001)
(Palomaki et al. 2004)
Test
DR for 5% FPR
Double
TT
Quad
Modelled (1:270 at
2nd T)
TT
Quad
Risk 1:250
Double
TT
Quad
DR (%), (95% CI)
61 (51-72)
66 (56-76)
75 (66-84)
79.3
83.8
63 (54-71)
70 (62-78)
72 (64-80)
3% FPR
Double
TT
Quad
52 (44-61)
55 (47-64)
56 (48-65)
75% DR
Double
TT
Quad
75
75
75
Modelled (1:250)
Double
TT
Quad
Modelled 2nd T risk
of 1:270
TT
TT LMP dating
TT USS dating
Quad
Quad LMP dating
Quad USS dating
Modelled DR for 5%
FPR
Double-LMP dating
Double- BPD dating
TT-LMP dating
TT-BPD dating
Quad-LMP dating
Quad-BPD dating
FPR (%), (95% CI)
5
5
5
10.4
9.9
7.0 (5.4-8.6)
6.6 (5.1-8.2)
6.7 (5.2-8.2)
3
3
3
13.2 (11.1-15.2)
10.3 (8.4-12.1)
9.9 (8.0-11.7)
64
67
70
7.6
7.2
6.7
74.6
70.4
77.4
79.3
76.4
81.3
8.4
9.05
7.96
7.38
8.15
6.86
65
67
67
72
77
79
5
5
5
5
5
5
Evidence regarding second trimester screening included in Chapter 5 evidence tables
Eight studies included in Chapter 5 also have evidence relevant to this chapter (Benn et al. 2005a;
Cuckle et al. 2005; Cuckle 2003; Knight et al. 2005; Malone et al. 2005; Rode et al. 2003; Wald et al.
2006a; Wald et al. 2003b). All eight of these papers confirmed that the quad test has a higher DR and
lower FPR than the TT and three papers (Benn et al. 2005a; Cuckle et al. 2005; Wald et al.
2003b)confirmed the conclusion that the TT performs better than the double test.
Other comparisons
In one paper, a case-control study, the performance of screening using TT with the addition of Lens
culinaris agglutinin-reactive AFP (AFP-L3) was compared to the conventional TT (using total hCG). It
also compared the performance of the conventional TT to screening with the TT using Lens culinaris
agglutinin-reactive AFP instead of the standard AFP (Azuma et al. 2002). The TT plus AFP-L3 had a
higher DR for all cut-offs than TT alone but a higher FPR. The TT with AFP-L3 instead of AFP had a
higher DR and lower FPR than the conventional TT. These results show AFP-L3 is a possible
additional 2nd trimester marker (Azuma et al. 2002).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
67
A case-control study compared the performance of the triple test using free βHCG compared to using
intact hCG (Sancken and Bahner 2003). Neither showed superior performance with fβhCG having a
slightly higher DR at a fixed 5% FPR (64% versus 55%), but having a lower DR and lower FPR (70%,
10%) than total hCG (79%, 12%) at a risk cut-off of 1:380. Another paper estimated the validity (with
statistical modelling) of the double test using fβhCG compared to using total hCG (Talbot et al. 2003).
For a fixed 5% FPR fβhCG plus AFP had a higher DR (66.4%) than total hCG plus AFP (59.4%).
The same paper compared these variations of the double test to screening with GlyhCG plus AFP (DR
was 53.1%) (Talbot et al. 2003). The case-control design and small sample size means there are some
limitations to the study, but GlyhCG does not appear to be any better than other forms of hCG already
in use.
Another case-control study compared the predictive performance of hPGH to the individual
components of the TT and compared the TT to screening with TT plus hPGH (Baviera et al. 2004), For
a fixed 5% FPR hPGH performed better than AFP (DR of 34.4% versus 25.8%), about the same as uE3
(35.5%), but worse than hCG (41.9%). When the conventional TT was compared to TT with the
addition of hPGF, the DR improved from 65.6% (95% CI 49-82) to 71.9% (95% CI 56-87) at a fixed
5% FPR (Baviera et al. 2004).
A case-control study compared the performance of screening with ITA to the components of the
conventional quad test. For a 5% FPR, ITA had a DR of 81% (95% CI 54-96), which was better than
the DR of AFP of 29% (95% CI 8-58), uE3 of 36% (95% CI 13-65), DIA of 36% (95% CI 13-65) and
hCG DR of 75% (95% CI 48-93). HCG performance (which correlates with ITA) was higher than
expected. These results could have been subject to bias or chance, and in this study ITA performance
may have been overestimated (Pandian et al. 2004). A further study estimated the performance of
screening ITA using modelling (Palomaki et al. 2004). When ITA replaced hCG in the triple test the
performance was similar: for a 5% FPR DR was 71% using ITA and 72% using hCG. When ITA
replaced DIA in the quad test the DR was 76% compared to 79% with the conventional quad test. The
quad test plus ITA had a DR of 83% (Palomaki et al. 2004).
Difficulties implanting any of the screening strategies
Five papers appraised in this chapter noted difficulties implementing any of the screening strategies.
Mostly these were quality control issues or issues with the reliability of serum marker measurements.
In one study (Harrison and Goldie 2006) inhibin-A was associated with considerable assay drift and
marked with-in batch imprecision which led the authors to state they had concerns with its use in its
present form.
In another study serum level results for two individuals had to be removed as they were outliers: a DS
pregnancy with a fβhCG of 29.7 MoM and a total hCG of 6.5 MoM, and an affected pregnancy with
fβhCG of 0.06MoM and total hCG of 0.05 MoM (Sancken and Bahner 2003). The authors stated that
dimeric hCG is thermally unstable during storage and transport and dissociated into fβhCG subunits
(Sancken and Bahner 2003). Analysis of stored specimens in this study could have distorted marker
levels compared to freshly analysed samples (Sancken and Bahner 2003).
A paper based on a twin population noted an apparent problem where the results of serum screening in
a twin with DS could be “normalised” by the results of an unaffected twin (Muller et al. 2003b). The
paper did not provide any data to support this statement.
Two papers noted problems determining an individual’s risk when dating was not accurate. One paper
compared various 2nd trimester screening methods using LMP or BPD dating (Palomaki et al. 2004).
Performance was worse if LMP dating was used compared to using BPD dating. Another found that
FPR of the quad test improved (reduced to 8.2% from 9.0) after correction for dating errors of more
than 10 days (Benn et al. 2003).
Another paper noted problems with screening accuracy (higher FPRs) when using the medians from
the software (as opposed to study population medians) (Huderer-Duric et al. 2000).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
68
Summary of results
There was a high level of consistency supporting:
ƒ
ƒ
poor performance of maternal age as a screening method compared with other screening
tests/methods
improved performance of the quad test compared with triple test and double test.
It was not possible to determine whether screening methods using fβhCG or total hCG had better
performance in 2nd trimester. fβhCG performed marginally better than hCG but there were only two
papers appraised that compared screening using these markers.
Markers other than standard 2nd trimester screening (hPGH, ITA, and AFP-L3) showed promising
results. However, further research is required using prospective cohort studies and using fresh serum
samples for analysis.
The difficulties implementing screening strategies included issues with the reliability of serum marker
measurements, problems with assay reliability, issues determining an individual’s risk when dating was
not accurate, and for one study difficulties with accuracy when using software medians to calculate risk
(as opposed to study population medians).
Conclusion
Some markers other than those used in conventional 2nd trimester screening showed promising
screening performance. These were hPGH, ITA, and AFP-L3. However, further research is required
using prospective cohort studies and using fresh serum samples for analysis
The quad test has the highest performance of all conventional screening strategies confined to the 2nd
trimester, followed by the triple test then the double test. Maternal age alone has a lower screening
performance than other screening methods and is not recommended as a screening test.
While some of the studies estimated DR and FPR using statistical modelling, there were also directly
observed data supporting this evidence. Other limitations included using case-control design
(especially for those considering new markers) and retrospective designs. However, the prospective
cohort studies included in this chapter also contributed to this evidence.
A population-based screening programme will need to include quality control measures to ensure
serum measurements are accurate. It will also need to consider the use of USS to correct for uncertain
dates, and to ensure software is able to accurately determine an individual’s risk of DS.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
69
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Huderer-Duric et al.
2000)
The comparison interventions were
the TT, compared to screening
using AFP and hCG (double test)
Between 1996-1998 a total of 2833
pregnant women (15-22/40) who
were enrolled in an antenatal care
programme had AC.
Outcomes
The outcomes extracted for
this table were the DR and
FPR for the TT and the
“double test” (AFP and
hCG) at risk cut-offs of
1:100, 1;200, 1:300. The
paper gives the DR of DS
and the specificity with a CI.
It appears that other
chromosomal disorders
have been removed from
this analysis (i.e. were not
included in the unaffected
group).
Accuracy of screening
methods DR% (95%CI), FPR%
(95%CI)
Limitations
The population was an older high risk population
as all were having AC. This may reduce the
external validity of the results. DR may be
overestimated.
The paper says that
introduction of their own
population specific means
reduced the overall FPR
from 27% to 18.6% (1:100),
from 38 to 26.7% (1:200) and
from 45% to 33% (1:300).
Difficulties implementing any
of the screening strategies
Higher FPR when used the
used software medians in risk
calculations.
Setting unclear
(although authors
from University School
of Medical, Zagreb,
Croatia.)
Zagreb, Croatia.
Prospective cohort
study
Grade III-2
MSS using Ortho-Clinical
Diagnostics assays. Markers
corrected for weight.
Risk determined using OrthoClinical Diagnostics software to
analyse MoM. First 986 used
software medians; next 1847 used
the study population medians.
Software corrects for MA, prior agebased risk for previous DS, and
gives risk at term.
In 2071 (73%) AC was indicated
because of AMA (35 years and
over).
762 were indicated for other reasons
or requested.
2.8% of total had previous DS, 0.8%
IDDM, 1.7% twins.
73% over the age of 34 years.
For most (98.2%) GA determined
from USS.
Mean GA =17.7/40
Spectrum of disease: 12 DS/2833 =
0.42%
12 cases of other chromosomal
disorders
Triple test
1:100 75% (43-95), 20% (19-22)
1:200 83% (52-98), 30% (28.531.9)
1:300 92% (62-100) 37% (34.938.5)
Double test
1:100 42% (14-70), 16% (14-18)
1:200 ?DR, 26% (24-27)
1:300 ?DR, 32% (31-34)
Verifications
All had amniocentesis.
Unclear if any fetal loss
between blood test and
AC.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Small number of DS cases (n=12).
Unclear how risks calculated for twins.
Few details about sample handling and storage
and methods for determining risk (parameters
used etc).
Unclear how some FPR figures calculated.
DR not available for comparison for all risk cut-offs
for double test.
Author’s conclusions
UE3 significantly contributes to DS detection with
cost of slightly reduced specificity. The 1:300 risk
cut-off caused an unfavorable compromise
between sensitivity and specificity.
Reviewers conclusions
May not be generalisable as high risk population.
Difficult to compare 2 screening methods as
unclear how some figures calculated and not all
DR are available. However in this study TT had a
clearly better DR but higher FPR compared to the
double test.
70
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Azuma et al. 2002)
Compared screening using the TT
(AFP, UE3, and hCG) with the
addition of Lens culinaris agglutininreactive AFP (AFP-L3), to the TT
alone. Also compared the
performance of conventional TT to
the TT with AFP-L3 instead of AFP.
No strategies included MA related
risk.
Retrospectively found 530 woman
without DS and 31 women with
fetuses affected by DS. Seen at the
hospital from 1989-1998.
Outcomes
The outcomes extracted for
this evidence table were
the
DR and FPR using different
cut-offs (scores of 5,4,3,2,
respectively) for TT with the
addition of AFP-L3
compared to TT.
Accuracy of screening
methods DR% (95%CI), FPR%
(95%CI)
Limitations
Excluded those other chromosomal abnormalities.
These are likely to have a positive screen for DS.
This will have reduced the FPR compared to
papers where these cases are included.
University hospital
Japan
Case-control study
Grade III-2
The authors established a scoring
index for each marker and
evaluated the screening
performance of screening using this
scoring method.
Gestation (dates from LMP and
corrected by USS).
Exclusions: DM, hepatic disease,
multiple pregnancies, major fetal
anomalies.
MA for cases 38 ± 3.9,
MA for controls 35.9 ± 4.8 years
(mean and SD)(p<0.05)
Samples taken at 14-20/40. AFP-L3measurement measured by
electrophoresis and expressed as a
percentage of total AFP.
GA cases 17.1 ± 1.8/40
GA controls 16.3 ± 1/40 (p<0.0001)
AFP, hCG, and UE3 measured by
commercial kits (Abbott Labs,
Wallak oy, Diagnostic Products
respectively). Marker levels then
expressed as MoM median based
on 4256 unaffected Japanese
pregnancies. A score of 1 or 2 was
assigned to an individual’s marker
profile based on the relationship
between the individual marker
MoM and the median value of
serum markers in unaffected
pregnancies.
Spectrum of disease: 31/561= 5.5%
Total = 561
Also compared TT using
hCG, uE3 and AFP-L3 to
conventional TT (hCG, uE3
and AFP).
Verification
All fetal karyotypes were
diagnosed by AC because
of either AMA, abnormal
screening results, or other
reasons.
TT & AFP-L3-score cut-off =5
35.5% (19-52), 1.3% (0.3-2.3)
TT & AFP-L3-score cut-off =4
83.9% (71-97), 5.1% (3.2-7.0)
TT & AFP-L3-score cut-off =3
90.3% (74-98),20.9%(17.5-24.4)
TT & AFP-L3-score cut-off =2
100%(89-100), 57.5% (53.361.8)
TT -score cut-off =5
16.1% (3-29), 0.2% (0.9-3.30
TT -score cut-off =4
35.5% (19-52), 1.3%(0.3-2.3)
TT -score cut-off =3
61.3% (44-78), 7.0% (4.8-9.2)
TT -score cut-off =2
90.3% (74-98), 35.3% (31.239.4)
No other chromosomal disorders.
HCG, uE3 and AFP-L3
80.6%, 6.6%
(TT) hCG, uE3 and AFP
61.3, 7%
Difficulties implementing any
of the screening strategies
No objective problems noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
As all had been diagnosed by AC for AMA and
abnormal screening results and various other
reasons, therefore sample would be biased and
could increase DR estimate.
Author’s conclusions
We confirmed that AFP-L3 is a useful marker for DS.
The method was not dependent on MA related
risk factor. Small database therefore it needs to be
confirmed by larger studies.
Reviewers conclusions
This scoring system needs validating in another
population. However these results show AFP-L3 is a
possible additional 2nd T marker.
71
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Muller et al. 2002a)
All labs used approved tests
(software and assay kit from the
same supplier).
The sample consisted of all pregnant
women who had a 2nd T serum
screen in France over 2 yrs (19971998).
Outcomes
The aim of paper was to
compare screening
performance for those
under 38 to those 38 years
and older using 2nd T MSS
(various TT or double test
methods).
Accuracy of screening
methods DR% (95%CI), FPR%
(95%CI)
Limitations
The study did not analyse different screening
methods separately.
MSS (TT, double)
73.5% (70.1-76.2), 6.85% (6.806.90)
Only 1.7% women in the analysis ≥ 38 yrs. Many of
those ≥ 38yrs would not have had 2nd T screening
as 38 years is the cut-off for offering AC in France.
MA ≥ 38 yrs
DR 9.5%(8-11), FPR 1.6% (1.591.65)
Fetal loss possibly not fully ascertained. No
national register of DS.
Nation-wide review of
medical records.
France
Retrospective cohort
study.
15% of labs used triple test (AFP,
UE3, hCG) (25% women).
85% of labs used the “double test”
(AFP & total hCG, or AFP and
fßhCG, or uE3 & hCG).
Grade III-2
The software all combined
maternal age risk with risks due to
the MSS markers.
Weight adjustment in 38 labs in
1997 and all labs in 1998.
Risk of 1:250 used in all labs.
Coincided with national decree in
1997 governing MSS including lab
practices obligations of practitioner
and patient, and reimbursement of
the cost of screening and
karyotyping.
1997 = 378,941 (52% of the total
pregnant women that year), 1998 =
475,961 (65% of total that yr). Total for
two yrs = 854,902. Less twins = 851,656
60 labs across France sent a
standard questionnaire.
GA in 98% = 14-17+ 6/40 in 98%.
In 98% GA confirmed by USS.
Spectrum of disease: = 977
DS/854,902 = 0.11%
For this evidence table
calculated performance of
MSS (all different methods)
compared to MA, by
removing twins and adding
together the two figures
(under 38 to those 38 years
and older).
Difficulties implementing any
of the screening strategies
None noted
Verification
For live births a
questionnaire was sent to
maternity units as all
newborns have pediatric
examination at 1/12, 3/12
and 6/12 after birth.
Questionnaire also sent to
all 80 cytogenetics labs
which perform pre and post
natal karyotyping.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Would have expected 1,027 DS out of those aged
< 38 yrs rather than 884 in this population.
However, some centres offered had 1st T NT
screening first -those with abnormal NT excluded
from 2nd T screening. This will decrease the DR of
the estimate of screening in 2nd T.
Author’s conclusions
Strict rule covering DS screening are of benefit to
patients, practitioners, and labs and ensure good
quality control and a high DR and low AC rate.
Reviewers conclusions
The sample is biased as many (especially over 38
yrs) will have had either 1st trimester NT screening
or AC. The results may have limited utility as they
are for serum screening as a whole rather than
one method. However, screening using MA alone
performs poorly compared to 2nd T serum
screening.
72
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Wald et al. 2003a)
Compared the performance of the
quad test (using total HCG, or more
usually fβhCG), to TT, double test,
and MA alone.
Between August 1996-September
2001 prospectively assessed the
quad test offered as routine
screening in 14 NHS hospitals.
Accuracy of screening
methods
Limitations
MA distribution of population not given but
presumed to be that of routinely screened
general population.
Serum markers taken 14-22/40 and
analysed at one centre.
All tests done in all pregnancies.
Outcomes
Outcomes were the
performance of the quad
test (risk cut-off of 1:300)
compared to MA alone ≥ 35
yrs.
UK
Prospective cohort
study
Grade III-2
Risk determined by аlpha software
(multivariate Gaussian model).
46,193 pregnancies had quad
screen done and MA recorded.
149 twins (no DS)
Risk of 1:300 considered screen
positive offered invasive testing.
In 79% GA determined by USS.
Spectrum of disease: 88 DS /46193 =
0.19%
The DR for quad test
compared to MA, the
double test and the TT at a
fixed 5% FPR.
This was repeated with an
adjustment for fetal loss
(23%) after 16/40.
Verification
Hospital records and
cytogenetic laboratories.
Expected DS at 16/40 =
expected at birth with
adjustment for fetal loss
16/40-term. 72 less 20 alive
at birth = 52. 52/1-0.23 = 68
plus 20= 88.
DR% (95%CI), FPR% (95%CI)
Quad test: 1:300
81% (72-89), 7% (6.7-7.2)
MA alone (≥ 35 years)
51% (41-62), 14.3% (14.0-14.7)
DR for fixed FPR of 5%
MA alone
26% (17-35)
Double test
61% (51-72)
triple test
66% (56-76)
Quad test
75% (66-84)
DR for fixed FPR of 5% & fetal
loss adjustment
MA alone
24%
Double test
57%
triple test
62%
Quad test
70%
Difficulties implementing any
of the screening strategies
None noted
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
No details of other chromosomal disorders in
sample but presumably left in analysis as
“unaffected”.
Unclear if all DS fetal losses ascertained however
fetal loss adjustment made.
Lead author is a director of logical Medical
systems (software for antenatal screening for DS)
and of Intema which holds rights to the Integrated
test.
Author’s conclusions
“The results from a routine screening service
confirm the value of an early 2nd T MSS over
screening using MA alone …and lends support to
the decision of the UK government to offer serum
screening to all pregnant women. Also confirms
that 2nd T quad is better than double or triple and
should be regarded as test of choice in this
period”
Reviewers conclusions
Small amount of detail in some sections but a
large well designed study which shows quad test
performs better than TT, double test, or MA alone.
73
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
Sample
Outcomes and
verification
Results
Comments
(Benn et al. 2003)
Compared the quad test
(observed and modelled) to MA,
double and TT.
All MSS quad test performed at the
health centre from November 1999
for 32 months were included.
Accuracy of screening
methods
AFP and hCG measured using
commercial kits (Bayer Corp), uE3
(Diagnostic Systems), and inhibin-A
(DSL).
Inclusion criteria: singletons, GA
14/40-21.9/40 at time of sample.
Limitations
Retrospective nature of the design means
outcomes may not have been determined for all
cases. However, adjustments made for fetal loss
and for expected DS for the MA distribution. This
highlights the problem of validating the DR in DS.
The prevalence changes through the pregnancy
(spontaneous fetal losses and ToPs) and difficult to
decide on denominator.
Adjustments for maternal weight,
race, and ethnicity have been
described elsewhere (see Benn et
al. 1995 and Benn et al. 1997 as
reference in this paper). No
adjustments for smoking. Median
values for all four analytes based
on data from this study and lab
data.
74% dated by USS, 25%- LMP, 1%
clinical exam.
Outcomes
As well as the observed
results for the quad test
(1:270 risk 2nd T) DR was
given for the quad test with
fetal adjustment (see
below) and with the
expected DS as
denominator (see
verification section).
A 2nd T risk of 1:270 used for screen
positive. MA specific risk for DS at
birth adjusted to 2nd T risk using a
factor of 0.76 for the survival of
affected and 0.985 for unaffected.
Spectrum of disease: 45 DS /23749 =
0.19%.
University of
Connecticut Health
Center, USA
Retrospective cohort
study
Grade III-2
Some statistical
modelling
During the study period revised
parameters used for screening
programme. However, for this
paper the same parameters
(means, SD, correlation
coefficients, and truncation limits)
used for all screened and revised
risks not used clinically.
The modelled DR and FPR
calculated by simulation using
mathsoft Inc software.
23749 had quad screen.
“Race” or ethnicity: 65% white, 19%
Hispanic, 12% black, 5% other (mostly
Asian).
The median MA at EDD was 27.8 yrs
and 17.1% ≥ 35 years.
12 DS live births. 12/0.76
(adjustment for fetal loss
from 2nd T to term) = 16. Plus
the 33 ToP= 49.
Also compared modelled
DR and FPR of MA alone
(>35 years), TT, and quad
test for a population with
the same attributes as the
study population. For the
quad test they adjusted for
fetal loss in both screen
positives and screen
negative women and using
the denominator of 54
(expected DS in this
population).
Verification
Cytogenetic lab reports,
genetic consultation
records, USS reports, and
follow-up from referring
physicians. (previously
validated methods).
Observed DR (95% CI) , FPR
(95% CI)
Risk of 1:270 at 2nd T.
Quad test No adjustment fetal
loss
86.7% (73.2-95), 9.0% (8.7-9.4)
DR Quad test with adjustment
85.8% (72.8-94)
DR Quad test with expected
denominator
77.7% (64.4-88)
Modelled DR, FPR
MA ≥ 35 years
53.3%, 17.1%
Triple
79.3%, 10.4%
Quad test
83.8%, 9.9%
Difficulties implementing any
of the screening strategies
After correction for major
dating errors (> 10 days) FPR
of quad = 8.2% (7.9-8.6).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
FPR different between observed and modelled
results which may reflect differences in parameters
for the analytes relative to published. This may be
due to differences in accuracy of dating,
population characteristics and assay conditions.
Author’s conclusion
The quad test meets or exceeds performance
expectation and appears to represent an
improvement over the triple test. Inhibin-A should
be widely available for 2nd T screening.
Reviewers’ conclusions
The study is limited by the retrospective design of
the study. However in this well conducted study,
quad test performed well in observed screening
and modelled results showed an improved
performance over TT and MA.
74
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Benn et al. 2003)
These were determined for those
dated by LMP and those dated by
USS then combined by calculating
averages weighted by the number
of women at each age and
method used for dating.
University of
Connecticut Health
Center, USA
Retrospective cohort
study
Grade III-2
Sample
Outcomes and
verification
Results
Expected DS based on MA
distribution = 54 cases.
Difference not sig diff
between 49 detected and
54 expected.
The modelling was based on a
population with MA distribution,
method of dating, and
“race”/ethnicity of those screened.
Some statistical
modelling
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
75
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Sancken and Bahner
2003)
Compared the performance of TT
using total hCG compared to
fβhCG.
34 serum samples from pregnancies
with DS and 189 controls matched
for GA.
Accuracy of screening
strategies:
fβhCG analysed by
immunoradiometric assay (CIS).
Others by a radioimmunoassay
(Ortho Clinical Diagnostics).
Removed two outliers. Left 33 DS and
188 controls= 221 in study.
Outcomes
DR and FPR for TT (without a
priori MA risk) using AFP, uE3,
and either total hCG, or
fβhCG.
Limitations
Case control study design means the population
may not be representative of a routinely screened
population. Other commonly confused disorders
removed (other chromosomal disorders).
Germany
Case-control study
Grade III-2
MoM from regression equations of
the controls with gestational days
as the regressing variable.
Multivariate discriminant analysis
was performed for the combination
of AFP, uE3, and hCG and for the
combination of AFP, uE3 and
fβhCG.
Mean MA was 34 yrs (19-43yrs) for
cases, and 29 yrs 17-44) for controls.
For both groups mean GA=17/40 (1522).
Spectrum of disease: 34DS /221 =
0.15%
No other chromosomal disorders.
Presumed singletons.
DR and FPR for TT (with a
priori MA risk) using AFP, uE3,
and either total hCG, or
fβhCG for a fixed 5% FPR
and with risk cut-off of 1:380.
Verification
Reference standard not
discussed nor whether the
cases were already screen
positive using total hCG or
fβhCG.
DR (95% CI), FPR (95% CI)
without MA ( ?risk cut-off)
TT -fβhCG
79% (65-93), 24% (18-30)
TT- total hCG
76% (61-90), 22% (16-28)
DR for fixed 5% FPR
TT-fβhCG
64%(47-80)
TT-total hCG
55% (38-72)
Risk cut-off of 1 :380 DR (95%
CI), FPR (95% CI)
TT-fβhCG 1:380
70% (54-85), 10% (5-14)
TT-total hCG 1:380
79% (65-93), 12% (8-17)
Difficulties implementing any
of the screening strategies
There were 2 outliers: one DS
(29.7 MoM fβhCG, 6.5 MoM
hCG), and one unaffected
(0.06MoM free βhCG, 0.05
MoM hCG).
Dimeric hCG is thermally
unstable during transport and
storage and dissociates into
fβhCG subunits.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
The removal of outliers. In clinical practice would
still need to have a risk estimate for these
individuals.
Unclear if serum specimens were retrospectively
analysed and if so if tests were performed blinded
to outcomes.
Author’s conclusions
For the observed cases none of the markers, hCG
or free βhCG, was superior in DS screening.
Problems with free ßhCG being unstable and
therefore an individuals risk misinterpreted means
the small increase in sensitivity may not justify using
it.
Reviewers conclusions
In this study fβhCG and total hCG performed
equally well. A case control study is not the best
design for diagnostic accuracy and a prospective
cohort study is needed in order to determine if
one marker is a better discriminator for DS.
76
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Muller et al. 2003b)
Compared five strategies for
screening for TWINS: MA, MA
corrected for risk of at least one DS
fetus in dichorionic pregnancies,
MSS (fβhCG and AFP) with
observed MoM ÷ 2, using median
values in twin population, and using
median values specific to mono- or
dichorionic twins.
Between Jan 1997 and June 2000,
3292 women with TWIN pregnancies
had 2nd T MSS at 14-22/40.
Outcomes
Outcomes were DR and FPR
for screening for DS using
MA alone, MA with twin
correction in dichorionic
pregnancies, double test
(fβhCG and AFP) with
observed MoM ÷ 2, double
test using median values in
twin population, and
double test using median
values specific to mono- or
dichorionic twins.
Accuracy of screening
methods DR (95% CI) , FPR
(95% CI)
Limitations
The setting of the study or what interventions
where based on in clinical practice was unclear.
MA alone
27.3% (6-61), 6.5% (5.6-7.4)
Small number of DS cases (n=15)
All methods had risk cut-off
of 1:250. For MA this meant
using cut-off of 37 yrs (1:250
risk in singletons) and then
where chorionicity known
correction as per Meyers et
al (as referenced in this
paper). For dichorionic twins
this leads to an offer of
invasive screen for those
with dichorionic twins for
women ≥ 34 years.
Double: median values-total
twin population
54.5% (25-84), 7.9% (6.9-8.8)
No details of setting.
France
Prospective cohort
study
Grade III-2
MSS analysed using PerkinElmer kit.
Risk using PerkinElmer software.
As the database increased, the
factor used to normalise serum
marker levels was corrected. In this
way the median concentration
observed in twins expressed in MoM
derived from singletons could be
used. Retrospective analysis of
serum level data. 2nd T MSS marker
(AFP and fβhCG) MoM calculated.
This was then ÷ 2, or medians
adjusted for twins, or medians
adjusted for chorionicity.
When risk of DS greater than 1:250
amniocentesis offered.
Median GA =15/40. Mostly (95%)
dates from 1st T USS.
Outcomes known in 3043 = 92.4%
Chorionicity in 1562 from 1st T USS
and the T or Lambda sign, or from
post natal placental examination.
Routine screening
Median MA = 30yrs (16-44).
Spectrum of disease: 15 DS /6086
fetuses = 0.25%
Four pregnancies with 2 fetuses
affected with DS, and 7 with one
fetus with DS.
Verification
No details.
Based on MA would expect
15-16 cases of DS.
MA corrected for dichorionic
pregnancies 54.5% (25-84),
24.4% (23-26)
Double: observed MoM ÷ 2
54.5% (25-84), 7.6% (6.6-8.5)
Double: median values for
mono- or dichorionic twins
54.5% (25-84), 7.6% (6.6-8.5)
Difficulties implementing any
of the screening strategies
Authors noted that a problem
with MSS for detection of DS in
twins is that an abnormal
result in an affected twin may
be normalised by an
unaffected twin’s marker
levels.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
No details of verification methods. May not be full
ascertainment of DS (fetal losses not accounted
for).
Author’s conclusions
Trisomy 21 second-trimester MSS is feasible in twins,
and is better than a policy based on maternal
age alone.
Reviewers conclusions
2nd T MSS using AFP and fβhCG performs better
than MA alone with no correction but not a lot
better than when MA corrected for risk of twins.
This method cannot indicate which is the affected
twin.
77
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Baviera et al. 2004)
Compared the TT (AFP, UE3, and
hCG) to the TT with the addition of
Human placenta growth hormone
(hPGH), and the performance of
the separate components of the TT
to hPGH.
32 stored samples (-70C) from 32
singletons with DS were retrieved.
Outcomes
The outcomes were the DR
for 5% FPR for hPGH, AFP,
uE3, hCG, TT, and TT plus
hPGH.
Accuracy of screening
strategies: DR, FPR
Limitations
The case control design is not the ideal design to
determine the performance of a screening test.
The spectrum of disease will not be that of a
routinely screened population. There will be no
other chromosomal disorders which will decrease
the FPR compared to studies which include these
as unaffected in their analysis.
Italy.
Case-control study
Grade III-2
All maternal samples had
previously had routine triple test
(Immulite) from 1999-2003 at 1520/40
hPGH Measured using a
commercial assay (Biocode).
hPGH Expressed as MoM. Gaussian
distributions for cases and controls
produced. Means and SD of the
hPGH marker and correlation
coefficients between markers
determined.
These were cases diagnosed with DS
by AC after positive TT (20), or AMA
(≥ 35 years) with negative triple test
(12). Of the 20 with positive TT, 5
were over 35 yrs.
Five matched singleton controls
(160).
MA, weight, specimen storage, GA,
and ethnicity not different between
groups.
Verification
All cases had AC. No details
of how control outcomes
verified.
DR For fixed FPR of 5%
hPGH
34.4% (18-51)
AFP
25.8% (11-41)
UE3
35.5% (19-52)
hCG
41.9%. (25-59)
Triple (AFP, UE3, and hCG)
65.6% (49-82)
AFP, UE3, hCG, and hPGH
71.9% (56-87)
Spectrum of disease: 32/192 = 17%
20/32 DS already positive by TT screening which
may bias the sample. Unclear if controls had
previously had positive or negative screen.
HPGH was analysed on stored sera while other
markers had already been analysed. Parameters
for hPGH were obtained from this study – i.e. a
small sample.
Author’s conclusions
Although the results are less significant than those
obtained with inhibin this marker could be
considered in screening for DS.
hPGH concentrations only weakly
correlated with other triple test
markers and these correlations
were taken into account when
determining the LR.
Reviewers conclusions
The design and sample size limits the ability to
accurately determine the performance of
screening with hPGH. It shows potential and this
should be confirmed in a prospective cohort
study.
Parameters for the other markers
from published data (Cuckle et al.
1995 as referenced in this paper).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
78
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Pandian et al. 2004)
Comparison of components of the
quad test i.e. AFP, uE3, hCG, and
DIA (dimeric inhibin-A) were
compared to serum ITA (previously
called hyperglycosylated hCG,
and usually measured in urine)
Blood collected from pregnant
women between 14-22/40. All were
singletons.
Outcomes
Compared the DRs for a
fixed 5% FPR for screening
using AFP, uE3, hCG, DIA,
and ITA
Accuracy of screening
strategies
Limitations
Case control design is not ideal design for
accuracy of screening. Small number of DS cases
(n=16).
Verification
All DS cases had
karyotyping after AC
AFP
29% (8-58)
UE3
36% (13-65)
HCG
75% (48-93)
DIA
36% (13-65)
ITA
81% (54-96%)
USA
Case-control study
Grade III-2
Samples analysed blind to clinical
information.
ITA results were determined by
automated
immunochemiluminometric assay.
Intra and interassay imprecision
determined (<3.5% and 7.4%).
DIA (diagnostic system
laboratories) and AFP, HCG, and
uE3 (immunlite 2000) were analysed
on the same day.
Estimates also modelled using
Gaussian distributions and maternal
age distribution for the USA in 2000.
Samples from the 16 with DS were
collected at the time of counseling
(Yale University). The diagnosis had
been made by AC.
All 16 DS had ITA and hCG done. For
two samples AFP, uE3, and DIA
results were not available.
Samples from 84 controls collected
from women undergoing 2nd T
screening (University of
Connecticut).
Spectrum of disease: 16 DS/100 =
16%
DR (95% CI) for a fixed FPR of
5%
The pair wise correlation
coefficients were calculated
between ITA and other
markers. The correlation
between ITA and HCG was
much higher than for others
(0.794 in controls). Both
markers may not be needed
in screening.
Difficulties implementing any
of the screening strategies
None noted.
No details of how outcomes determined for
controls.
Cases and controls at different sites-maybe
different handling of specimens. Cases
determined after AC - may affect marker levels.
Average GA for cases later than controls.
HCG performance (which correlates with ITA)
higher than expected. Could have been due to
bias or chance. Screening history reviewed for
referral bias- 8/16 DS from women ≥35 yrs. No
evidence these were screen +ve by MSS prior to
AC. Can’t exclude fact ITA performance may be
overestimated.
Quest diagnostics, and Nichols Institute
Diagnostics assisted in assaying the samples. One
of the authors works for Quest diagnostics.
Author’s conclusions
The current study found 2nd T serum ITA was a
good marker for DS % when gestational dating
was based on USS.
Findings should be confirmed in a larger study.
Reviewers conclusions
Some limitations due to study design and
numbers. Need to have a large prospective
cohort study.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
79
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Harrison and Goldie
2006)
Comparison of screening using
either double test, TT, or quad test
(all with total hCG).
128 case samples collected January
1993-December 2001.
Outcomes
The outcomes (DR and FPR)
were screening using the
double test, TT, and Quad
test. These are presented for
a risk cut-off of 1:250, DR at
a fixed FPR of 3%, and FPR
at a fixed DR of 75%.
Accuracy of screening
strategies
Limitations
Having only 55.3% confirmed by USS may have
decreased the performance of the tests. Hard to
compare to others where mostly or all GA
confirmed by USS.
Bristol, UK
Case-control study
Grade III-2
For DS samples, total hCG and AFP
analysed then stored at -40C until
completion of an annual audit,
then stored at -70C long-term. For
controls total hCG and AFP
determined then frozen (-40C) until
all outcomes known.
HCG and AFP not reanalysed.
Testing done with commercial kits
(Bayer Plc). Inhibin and UE3
analysed using Diagnostic Systems
Laboratories testing kits.
The control population comprised
1000 samples received
consecutively for DS screening (using
total hCG and AFP) between 1st
January and 20th February 2003. GA
15/40-17.6/40. GA from BPD in 55.3%
and remainder from reliable dates.
Median MA of cases at delivery = 33
yrs (19-42yrs).
Median MA of controls at delivery =
29 yrs (16-42 yrs).
Spectrum of disease: 128/1128 = 11%
All serum markers corrected for
maternal weight. Results expressed
as MoM. MA specific risks as per
Cuckle et al. 1987 (as referenced in
this paper). Risk estimates
calculated using NSC Prenatal
Screening Decision Support QAtools software. (uses multivariate risk
algorithm). Marker distribution for
AFP and hCG from literature (Wald
et al. 1988 - as referenced in this
paper). Distribution parameters for
uE3 and inhibin-A derived for this
study.
Assay drift was assessed by running
80 control samples across an assay
plate in forward then reverse
sequence.
Presume no other chromosome
disorders.
Presume singleton.
The 3% fixed FPR was
chosen as the National
screening committee in the
UK has set a target
performance for DS
screening of DR 75% for less
than 3% FPR by April 2007.
The performance was also
estimated using statistical
modeling.
Verifications
80 detected by the double
test (1:250 at term) and 48
missed (either live births or
miscarriages). None
identified by AC alone (i.e.
AMA) as these did not have
serum taken.
Risk 1:250 DR (95%CI), FPR
(95%CI)
Double
63 (54-71), 7.0(5.4-8.6)
TT
70 (62-78), 6.6 (5.1-8.2)
Quad
72 (64-80), 6.7 (5.2-8.2)
DR (95%CI) fixed 3% FPR
Double
52 (44-61)
TT
55 (47-64)
Quad
56 (48-65)
FPR (95%CI) fixed 75% DR
Double
13.2% (11.1-15.2)
TT
10.3% (8.4-12.1)
Quad
9.9 (8.0-11.7)
Modelled (1:250) DR, FPR
Double
64, 7.6
TT
67, 7.2
Quad
70, 6.7
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
For controls and cases different tests done at
different times-AFP and HCG then frozen samples
used for rest at later date.
Case blood collected some years earlier so frozen
for longer. Authors say this is not a problem as
stored under optimum conditions and subject to
only one thaw freeze cycle.
Problems with inhibin-A assay. Authors state they
have concerns about the use of this marker in its
present form. (No other assay available in UK
commercially).
Author’s conclusions
The NSC target of a DR of at least 60% with FPR <
5% may be achievable using TT and USS dating in
2nd T. The results suggest that the April 2007 target
of DR 75% and FPR < 3% is unachievable using
current 2nd T MSS.
Reviewers conclusions
Well designed and conducted study with clear
description of methods. Needs further analysis in
large prospective cohort study.
80
Table 13.
Source
Country
Setting
Study design
Evidence Grading
(Harrison and Goldie
2006)
Bristol, UK
Case-control study
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Difficulties implementing any
of the screening strategies
Inhibin-A was associated with
considerable assay drift and
marked within-batch
imprecision (intra-batch %
coefficient of variation = 17%).
Grade III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
81
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Benn et al. 2001)
The aim of the study was to determine the
extent to which additional DS pregnancies
may be identified through T18 screening,
and the extent to which T18 may be screenpositive for DS (cross-identification).
Statistical modelling
Randomly generated 100,000 sets of analyte
values corresponding to normal, DS and T18
pregnancies using the multivariate Gaussian
distribution generator in the statistical
computer package, S-Plus (mathsoft). This
program has been previously validated.
(Larsen et al. 1998-as referenced in this
paper).
For both the DS and unaffected populations
the means, SD and correlation coefficients
between the markers were determined by
Wald et al. 1994, 1996 and1997 (as
referenced in this paper).
Prior to the computation of the LR from the
randomly generated analyte values,
truncation limits were applied to the analyte
values as specified for DS calculations (Wald
et al. 1996 as referenced in this paper).
Sample
Outcomes and
verification
Results
Comments
Outcomes
For the purpose of this
evidence table the data for
the FPR and DR of triple test
(AFP, uE3, and hCG) and
quad test (addition of
inhibin) was extracted from
the paper.
Accuracy of screening
methods
Limitations
Performance of DS screening not the aim of the
study.
There were separate
simulations for pregnancies
dated by LMP and those
dated by USS, as well as a
simulation for a population
in which 60% of
pregnancies were dated
by USS and 40% on LMP.
DR, FPR (risk 1;270, 2nd T)
Triple test
74.6%, 8.4%
Triple test (LMP dated)
70.4%, 9.05%
Triple test (USS dated)
77.4%, 7.96%
Quad test
79.3%, 7.38%
Quad test (LMP dated)
76.4%, 8.15%
Quad test (USS dated)
81.3%, 6.86%
The risk cut-off was a 2nd T
risk of 1:270.
The MA distribution for the
model was that of the USA
population in 1998.
MA specific risk of DS was based on Bray et
al. 1998 (as referenced in this paper).
Adjustment to correct for prevalence of DS
in 2nd T was performed using a 0.8554 factor
obtained by comparing AC prevalence of
DS to GA specific prevalence curve (Cuckle
1999 and Benn and Egan 2000 as
referenced in this paper).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Author’s conclusion
Quad test appears to have a somewhat higher
FPR and DR than others have noted. This may be
due to the difference in MA distribution of the
population analysed and other minor differences
in the variables used in the model.
(Other conclusions were about cross
identification-the aim of this paper)
Reviewers’ conclusions
This model predicts that quad test with USS dating
of all pregnancies will perform better than TT.
82
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
(Talbot et al. 2003)
The study compared screening with different
forms of the double test (AFP and either hCG
glycoforms(GlyhCG), fβhCG, or total hCG).
Maternal serum samples
collected in 2nd T from DS
and unaffected women
attending Harold Wood
hospital (Spencer 1999-as
referenced in this paper).
Blood had been stored at 20C. From this archive
retrieved 50 DS and 279
unaffected samples.
Outcomes
Outcomes extracted for this
evidence table are the DR
for a 5% fixed FPR using
GlyhCG plus AFP,
compared to total hCG
plus AFP, and to fβhCG plus
AFP.
Accuracy of screening
methods
Limitations
Analysis of all samples using stored specimens.
Obtained population parameters for GlyhCG
from these results (small number and stored
samples). Parameters for other markers would
have been obtained from freshly analysed
samples.
Statistical modelling
HCG AFP and total hCG were analysed
using Kryptor (Brahms) and automated
immunofluorescent assays (Brahms).
The serum GlyhCG measured at two dilutions
in singletons using lectin immunoassay
described by Abushoufa et al. 2000 (as
referenced in this paper). The mean of the
two (after correction for dilution) used in the
analysis. Analysis for GlyhCG was blinded to
outcomes.
Each value converted to the MoM for the
GA using published parameters or for
GlyhCG from this study. Used observed
parameters for GlyhCG and those for total
hCG and fβhCG and AFP from Spencer et al.
2002 (as referenced in this paper).
All dated by CRL or BPD
(after 14/40).
Median MA 35 yrs DS and
30.4 yrs for controls
Model based on MA
distribution of England and
Wales 1997-1999
DR For a fixed 5% FPR.
GlyhCG, AFP
53.1%
Total hCG and AFP
59.4%
fβhCG, and AFP
66.4%
Difficulties implementing any
of the screening strategies
None noted
GA cases= 109 days. GA
controls =115 days.
Sample storage cases = 840
days. Sample storage
controls = 851.
Used regression analysis to determine the
relationship between marker levels and GA.
Corrected for maternal weight as per
Neveux et al. 1996 (as referenced in this
paper).
Performance of marker combinations
determined using standard modelling
techniques (Royston and Thompson, 1992 as
referenced in this paper). Monte Carlo
simulation used to generate 15,000 random
MoM for DS and unaffected pregnancies for
each marker based on the MA distribution of
England and Wales 1997-1999. From these
calculated the LR, and MA related risks used
to determine risk of DS at term. MA related
risks from Cuckle et al. 1987(as referenced in
this paper).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Author’s conclusion
Maternal serum GlyhCG, as measured by the
sialic acid-binding lectin immunoassay is unlikely
to be of additional value when screening for DS
in the second trimester.
Whether a more specific immunoassay could
improve clinical discrimination needs further
consideration.
Reviewers’ conclusions
The case-control design and small sample means
there are some limitations, but GlyhCG does not
appear to be any better than other forms
already in use.
83
Table 13.
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
(Palomaki et al. 2004)
The study compared the performance of
using serum ITA (or hyperglycosylated hCG)
in 2nd T multiple marker strategies with the
performance of using hCG, or dimeric
inhibin-A (DIA). ITA is a carbohydrate variant
of hCG.
Used stored serum from an
“unbiased group” of 5,345
women. Samples collected
1990-1992 during a previous
observational study
(Haddow et al. 1994 as
referenced in this paper).
Outcomes
The outcomes were
observed and modelled DR
at 5% FPR for ITA alone,
either with LMP dating or
BPD dating (without MA
specific risk in the
calculation of risk).
Accuracy of screening
methods
Limitations
Small sample, and data from a case control
study used for the model.
Statistical modelling
Serum collected before AC and assayed for
AFP, uE3, hCG then stored -20C.
Never thawed aliquot used for this series.
Samples sent (blinded) to Quest Diagnostics
for ITA measurement using automated
immunochemiluminometric assay (minimal
cross reactivity with hCG).
14 prenatal centres in
California and elsewhere in
USA recruited women at 1421/40, about to undergo
AC for reasons other than a
positive screening test
(mostly for AMA).
Results are also presented
for modelled DR for 5% FPR
replacing hCG, or DIA with
ITA in the TT or quad test,
and comparing the quad
test to quad plus ITA.
All results converted to MoM and corrected
for maternal weight (Neveux et al. 1996 as
referenced in this paper). Adjustments to the
other variables and population variables
published elsewhere (as referenced in this
paper). Correlation coefficients between ITA
and serum markers in 2nd T DS and
unaffected were derived after exclusion of
outliers.
None had had serum
screen in this pregnancy.
Used MA age distribution of
the USA for 2000.
Aliquots from same series
used for two previous
studies. Three cases and 7
controls had been used up.
Left 45 cases and 238
controls.
Verification
Amniocentesis
Modelling method based on over lapping
Gaussian distributions of DS and unaffected
pregnancy markers.
Matched for time in
storage, MA, GA, “race”,
and site where sample
obtained.
Observed (modelled) DR For a
fixed 5% FPR.
No details of MA but states that most of the
women having AC for AMA.
ITA alone-LMP dating
38% (45%)
ITA alone-BPD dating
40% (48%)
Used stored samples for ITA (and possibly DIA-no
details given)
Modelled DR For a fixed 5%
FPR for different methods of
dating.
Some support form screening industry for the
study. Partially funded by Quest Diagnostics, and
Quest Diagnostics also assisted in the assaying of
the samples for various markers. One author
works for Quest.
ITA -LMP dating
56%
ITA -BPD dating
58%
ITA, and AFP-LMP dating
62%
ITA, and AFP- BPD dating
65%
Double test (AFP & hCG) -LMP dating
65%
Double test (AFP & hCG) - BPD
dating
67%
TT (AFP, uE3, & hCG) -LMP
dating
67%
No further details of the
sample.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Author’s conclusion
This study indicates that serum ITA is an effective
marker for DS. It is highly correlated with both
hCG and free βhCG and could replace either of
them in a multiple marker method.
A lab may find it is more economical or easier to
use ITA than hCG and this should not change
performance. However, need to first look at ITA
screening for twins and T18 etc.
84
Table 13.
Source
Country
Setting
Study design
Evidence Grading
(Palomaki et al. 2004)
Statistical modelling
Continued
Evidence table of primary research studies appraised investigating the accuracy of second trimester screening compared to components
(continued)
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
TT (AFP, uE3, & hCG) BPD
dating
72%
ITA, AFP, & uE3-LMP dating
66%
ITA, AFP, & uE3- BPD dating
71%
ITA, AFP, uE3, & hCG -LMP
dating
70%
ITA, AFP, uE3, & hCG- BPD
dating
76%
Quad test -LMP dating
77%
Quad test -BPD dating
79%
ITA, AFP, uE3, & DIA -LMP
dating
77%
ITA, AFP, uE3, & DIA -BPD
dating
79%
ITA, AFP, uE3, DIA, & hCG -LMP
dating
80%
ITA, AFP, uE3, DIA, & hCG -BPD
dating
83%
Reviewers’ conclusions
Using data for the model from a case-control
study with a small sample limits the ability to
calculate an accurate DR and FPR. ITA does
appear to perform as well as hCG or DIA, but this
should be confirmed with a large prospective
cohort study with an unbiased sample.
Difficulties implementing any
of the screening strategies
Performance of screening
worse if used LMP dating
rather than BPD dating
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
85
Chapter 5: Comparison of 1 st
trimester strategies, 2 nd trimester
strategies, integrated and
sequential methods.
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY
The search identified 26 eligible papers comparing the accuracy of first trimester with second trimester
screening and/or comparison with screening where the results of screening in two trimesters are
combined (integrated or sequential screening). Below is an overview of study designs and aspects of
quality represented by these studies.
Full details of the papers appraised, including methods, key results, limitations and conclusions, are
provided in evidence Table 16 (pages 97-134). Studies with directly observed (or age standardised)
DRs and FPRs are presented first, followed by studies where the results only include estimations of
performance using statistical modelling. For each of these two groups of papers, studies are presented
in chronological order of publication.
Study design, and grading
All 26 papers appraised in this chapter are based on primary research; there were no papers based on
secondary research that fitted the eligibility of the review. Of the 26 papers appraised, twelve papers
reported directly observed (or age standardised) comparisons of performance, and fourteen papers only
reported comparisons of DR and FPR estimated by modelling. For further explanation of modelling see
Chapter Three Study design and grading.
Of the papers reporting directly observed comparisons (or age standardised), eleven were cohort
studies. Sample sizes for these studies ranged from 359-47,053. Four of these studies were
retrospective cohort studies, (Gyselaers et al. 2004a; Gyselaers et al. 2004b; Michailidis et al. 2001;
Schuchter et al. 2002) and one (Wald et al. 2003a) included analyses using data from a nested casecontrol study (sample size of 588). There was one case-control study with a sample size of 531
(Herman et al. 2002). While all these studies were graded III-2 as per NHMRC, as discussed in chapter
2, the ideal design for determining the DR and FPR of a screening strategy is a large prospective cohort
(or nested case-control) study where all women have all screening strategies being compared (Deeks
2001).
Study setting and samples
Of twelve studies reporting directly observed (or age standardised) data six were set in single centres
and six were multicentre studies. All studies except one were in hospital settings, (Knight et al. 2005)
and four single centre studies were set in university hospitals (Audibert et al. 2001; Dommergues et al.
2001; Herman et al. 2002; Michailidis et al. 2001).
The case-control study compared DS cases to “normal” controls, i.e. the study did not include cases of
other chromosomal disorders which will also be detected by DS screening (Herman et al. 2002). The
proportion of DS in this study was 4.3% (Herman et al. 2002).
In five of the cohort studies the population studied was a routinely screened population with the
proportion of DS in the sample ranging from 0.18-0.31%.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
86
Two of the papers screened women of AMA, one by design as the sample consisted of women 38 years
and over (proportion of DS = 2%), (Dommergues et al. 2001) and the other through referral bias-the
mean maternal age was 37 years and the proportion of DS in the study population was 0.78% (Babbur
et al. 2005).
In four studies the population contained fewer older women, two by design as they excluded either
women over 38 years (Audibert et al. 2001) or those over 37 years, (Rozenberg et al. 2002) or because
many women over 35 years old had invasive diagnostic screening without DS screening (Gyselaers et
al. 2004a; Gyselaers et al. 2004b).
The cohort studies all included other chromosomal disorders as unaffected (for some studies this is
presumed from the details in the paper).
Comparison screening methods
The screening tests/methods compared in this chapter were (see glossary for further details):
1.
Screening restricted to one trimester:
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
ƒ
MA ≥ 35 years
first trimester MSS (PAPP-A and either fβhCG or hCG)
first trimester combined test
second trimester double test
second trimester triple test (TT)
second trimester quad test
proform of eosinophil major basic protein (ProMBP) used in the TT (second trimester) instead of
uE3, and in the quad test instead of inhibin.
2.
Screening using repeat measures of the same serum analytes in first and second trimesters.
3.
Screening combining information from markers across two trimesters (sequential or integrated
screening). The conventional integrated and sequential screening methods were:
ƒ
ƒ
ƒ
ƒ
serum integrated screening (1st trimester PAPP-A and second trimester quad test)
(fully) integrated screening (1st trimester PAPP-A and NT and second trimester quad test)
stepwise screening (1st trimester combined test and second trimester quad test)
contingent screening (1st trimester combined test and second trimester quad test).
Integrated screening (serum integrated or fully integrated screening) involves all women having first
and second trimester screening tests. Results are held until completion of second trimester screening
when all results are combined into one result.
For stepwise screening all women have first trimester screening. Those with a high risk result are
offered diagnostic testing. All others have second trimester screening. For these women the results of
first and second trimester testing is combined to produce one integrated result.
For contingent screening all women have first trimester screening. High risk women have a diagnostic
test; low risk women are reassured and have no further screening. All others have second trimester
screening. For these women the results of first and second trimester testing is combined to produce one
integrated result.
In additional, sometimes a screening method employs the same strategy as a conventional integrated or
sequential screening method but different tests are used. For instance, measuring NT in the first
trimester and offering those with a high risk result a diagnostic test, and those with a low risk a 2nd
trimester double test. This method uses the same strategy as the stepwise screening method and in this
review this is described as combining tests in a “stepwise manner”.
In some appraised studies women were offered a first trimester screening test then women who were
screen negative were offered a second trimester screen without consideration of the first trimester
results. This practice of combining tests in an “independent manner” leads to erroneous risk estimates
(Wald 2006c) and is not recommended.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
87
ƒ
Unless otherwise stated all screening strategies incorporate the maternal age for each individual.
Three studies used stored serum specimens for the analysis. This may bias results if there was a
difference in storage times between cases and controls or if some markers were stored where others
were analysed using fresh samples. For one paper all markers were analysed using stored specimens
and cases and controls were matched for duration of storage (Wald et al. 2003b). Another paper
determined the performance of the serum integrated test using 1st trimester PAPP-A results from stored
serum (Knight et al. 2005). A further paper analysed ProMBP and Inhibin-A using stored specimens
while the analyses of other markers (fβhCG, hCG, uE3, AFP) were determined on fresh specimens
(Rode et al. 2003).
Where details were given in the papers most studies analysed serum markers using
commercial/automated kits and risk was established using commercially available software. One study
analysed PAPP-A using a manual ELISA, and ProMBP using an in-house (Statens Serum Institut)
ELISA (Rode et al. 2003).
All papers in this chapter used conventional methods to combine maternal age specific risks and
marker levels to determine an individual’s risk and therefore the DR and FPR (i.e. using multivariate
Gaussian distributions).
Outcomes
Where a large number of results for different risk cut-offs, fixed FPRs or DRs have been reported (e.g.
for modelling papers) a fixed FPR of 5% and/or a fixed DR of 85% have been selected for the evidence
table as this is the convention for reporting DS screening test performance (reference). While studies
report DR for fixed FPR in reality the cut-off chosen for screening programmes is an individual risk
(Benn and Donnenfeld 2005).
For practical reasons, in some cases where large numbers of results have been reported for serum or
NT measurements at different GAs, the results for timings which produced the best performance are
presented in the evidence tables.
PRIMARY RESEARCH: STUDY RESULTS
Accuracy of screening methods
Maternal age alone as a screening test
Two papers compared maternal age alone as a screen to other screening methods (Michailidis et al.
2001; Schuchter et al. 2002). In one study maternal age as a screen was clearly inferior to NT, triple
test and a screening method where NT and TT were combined in an independent manner (a positive
screen in either NT or TT constituted a positive screen) (Schuchter et al. 2002). In the other study
maternal age was inferior to NT and screening combining NT and double test in an independent
manner, but maternal age had a slightly higher DR than the double test (56.5% versus 50%) with a
higher FPR (21% versus 8.7%), (Michailidis et al. 2001). It should be noted however, that the double
test performance was determined after screening with NT in the first trimester that was interventional
and left only a few cases (n=4) to be detected by the double test (Michailidis et al. 2001).
Overall, the literature supported the low predictive performance of maternal age alone compared with
other screening strategies in the second trimester.
First trimester screening versus second trimester serum screening
One paper compared 1st trimester maternal serum screening alone (i.e. with no NT screening) to 2nd
trimester maternal serum screening (Gyselaers et al. 2004a). Results indicated that TT had a better
performance than 1st trimester MSS (fβhCG and PAPP-A). The paper had some limitations which may
reduce the accuracy of these findings. The design was a retrospective cohort study that compared
screening with two screening methods in two different populations at different times. There may have
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
88
been concurrent screening with other methods (NT during the period of 1st trimester MSS) which could
bias the samples.
Sixteen papers compared 1st trimester NT (or the combined test) to 2nd trimester serum screening
(double test, TT, or quad test). Five of these papers (Audibert et al. 2001; Babbur et al. 2005;
Michailidis et al. 2001; Rode et al. 2003; Schuchter et al. 2001) were interventional-i.e. the NT results
in the first trimester were acted upon before the 2nd trimester which biases the results (Wald et al.
2003b). Women with high NT results were offered diagnostic tests and did not have 2nd trimester serum
screening. This makes a comparison between NT and the 2nd trimester MSS invalid.
There were eleven non-interventional studies (or modelling based on non-interventional studies) that
compared screening with NT (or the combined test) to 2nd trimester MSS. The results of the 1st
trimester screening test were not acted upon and women proceeded to 2nd trimester screening. The
results of these studies are presented in Table 14.
The results consistently showed that 1st trimester screening strategies had similar performance to 2nd
trimester screening, apart from the combined test which in general performed better than all 2nd
trimester screening.
Table 14.
Non-interventional studies comparing DRs and FPRs of 1st trimester NT (or
combined test) versus 2nd trimester strategies (and integrated, sequential, or
independent strategies).
Reference
(Dommergues et al.
2001)
(Rozenberg et al.
2002)
?some intervention
(Wald et al. 2003b)
(SURUSS)
Test
NT ≥ 3mm
Double (1:250)
NT and double test
(independently)
Modelled (1:250)
NT
Double
NT & double (stepwise
manner)
Modelled 5% FPR (1:250)
NT
Double
NT & double (stepwise
manner)
Fixed 85% DR
NT
Combined
Double
TT
Quad
Serum integrated
Integrated
Fixed 5% FPR
NT
Combined
Double
TT
Quad
Serum integrated
Integrated
DR (%), (95% CI)
100 59-100
86 42-100
100 59-100
FPR (%), (95% CI)
3.3 (1.5-5.1)
33 (28-38)
35 (30-40)
53.4
68.8
80.6
4.6
7.8
5.3
54.6
59.7
79.8
5
5
5
85
85
85
85
85
85
85
20.0
6.1
13.1
9.3
6.2
2.7
1.2
60
83
71
77
83
90
93
5
5
5
5
5
5
5
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
(18.6-21.4)
(5.6-6.5)
(12.5-13.7)
(8.8-9.8)
(5.8-6.6)
(2.4-3.0)
(1.0-1.4)
89
Table 14.
Reference
(Malone et al. 2005)
(Faster trial)
Non-interventional studies comparing DRs and FPRs of 1st trimester NT (or
combined test) versus 2nd T MSS strategies (and integrated, sequential, or
independent strategies) (continued)
Test
Observed
Combined (1:150)
Combined (1:300)
Quad (1:300)
Combined and quad
(independent manner)
(1st T 1:150, 2nd T 1:300)
Age standardised FPR for
85% DR
NT
1st MSS
Combined
TT
Quad
Serum integrated
Integrated
(Lam et al. 2002)
(Cuckle 2003)
(Wright and Bradbury
2005)
Age standardised DR for
5% FPR
NT
1st MSS
Combined
TT
Quad
Serum integrated
Integrated
Stepwise (fixed 2.5% FPR
for each screening
component)
Modelled 5% FPR (1:320)
NT
Double
NT and double (Integrated
manner)
Modelled (1:250)
NT (11-13/40)
Combined
TT
Quad
PAPP-A combined with
quad (?integrated or
stepwise)
PAPP-A and NT
combined with quad
(?integrated or stepwise)
Modelled, 85% DR
Combined
Quad
Serum Integrated
Fully integrated
DR (%), (95% CI)
77
82
85
94
FPR (%), (95% CI)
(69-86)
(74-89)
(76-93)
(89-99)
85
85
85
85
85
85
85
70
70
87
69
81
88
96
95
(65-79)
(64-78)
(82-92)
(63-74)
(70-86)
(81-92)
(92-97)
(91-97)
69.3 (56-76.1)
73.2 (63.4-82.9)
85.7 (76.2-92.1)
3.2
5.6
8.5
11
(3.0-3.4)
(5.4-5.9)
(8.2-8.8)
(10.7-11.3)
20
16
3.8
14
7.3
3.6
0.6
(10-26)
(9.8-22)
(1.8-7)
(10-21)
(4.6-16)
(2.0-7.7)
(0.4-1.6)
5
5
5
5
5
5
5
4.9
5
5
5
70.6
81.6
65.1
69.2
76.1
2.4
2.0
4.7
4.1
3.2
88.1
1.5
85
85
85
85
6.1
6.2
2.7
1.2
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
90
Table 14.
Non-interventional studies comparing DRs and FPRs of 1st trimester NT (or
combined test) versus 2nd T MSS strategies (and integrated, sequential, or
independent strategies) (continued)
Reference
(Benn et al. 2005a)
(Cuckle et al. 2005)
(Benn and Donnenfeld
2005)
(Wald et al. 2006a)
Test
Modelled-UK policies
Combined (1:250)
Double (1:250)
TT (1:250)
Quad (1:250)
Contingent screening
(overall risk 1:250)
Modelled-USA policies
Combined (1:270)
TT (1:270)
Quad (1:270)
Contingent screening
(overall risk 1:270)
Modelled for 5% FPR
(using fβhCG)
NT
Combined
Double
TT
Quad
Serum Integrated
Fully integrated
Modelled
Combined
Quad
Stepwise
Modelled 5% FPR
(adjusted for previous
pregnancy)
Combined
TT
Quad
Serum integrated
integrated
DR (%), (95% CI)
FPR (%), (95% CI)
85.8
77.8
79.8
83.8
91.4
3.8
7.8
7.2
5.4
2.1
83.6
81.7
84.6
89.1
5.3
8.3
6.7
3.1
78
87
61
65
71
78
93
5
5
5
5
5
5
5
83.7
84.4
90.8
5.1
6.6
3.1
87
80
85
89
95
5
5
5
5
5
1st trimester screening and/or 2nd trimester screening compared with screening strategies
using first and second trimester tests.
All eleven studies in Table 14 (non-interventional studies comparing screening with NT/ combined test
with 2nd trimester MSS) also had results for a screening strategy using first and second trimesters tests
(integrated, sequential or independent screening). One of the studies was in a population where women
were of advanced maternal age and the proportion of DS was 2%, the sample size was only 359, and
there were only 7 DS cases (Dommergues et al. 2001). In this study, NT had a lower FPR and a DR
(100%) equivalent to screening in an independent manner. In another study screening combining
results in an independent manner had a higher DR and a higher FPR than screening confined to one
trimester (Malone et al. 2005). Most studies showed that screening in a stepwise, contingent or
integrated manner has an increased performance compared to screening in either trimester alone, and
that serum integrated screening has a similar performance to the 1st trimester combined test.
The five interventional papers not included in Table 14 confirmed these results. Two of these papers
included results for an independent approach (Audibert et al. 2001; Schuchter et al. 2001). In both these
studies independent screening had higher DRs but the FPR was higher than screening in either
trimester. Two papers gave results for screening in a stepwise manner (Audibert et al. 2001; Babbur et
al. 2005). In both studies this strategy had higher DRs than 1st or 2nd trimester screening but in one
paper the FPR was higher than for NT screening (4.1% versus 1.8%), (Babbur et al. 2005). In this study
TT had a particularly poor performance which may have been due to the samples being taken at 14/40
rather than 16/40 (Babbur et al. 2005). Also, comparisons were difficult in this paper as results were
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
91
presented for different cut-offs, fixed FPRs, or DRs. In another study the integrated test was compared
to the combined test and the quad test and the performance was better (higher DR for fixed 5% FPR)
than either method alone (Rode et al. 2003). In the last of these papers it was not clear how the tests
were combined for the results provided (Michailidis et al. 2001). However, the screening method
combining results for NT and the double test had a better DR and lower FPR than either screening
method alone (Michailidis et al. 2001).
Two other papers not included in Table 14 (as they did not also include results for 1st trimester
screening) compared screening in the 2nd trimester with a screening strategy using first and second
trimester tests.
One paper compared screening with 2nd trimester serum screening to a method combining NT and 2nd
trimester MSS (Gyselaers et al. 2004b). It was not clear how the strategy combined the results
(Gyselaers et al. 2004b). Screening performance decreased after the introduction of NT (Gyselaers et
al. 2004b). However, there were major limitations to this study. The study was based on two different
populations having two different screening strategies over different time periods (2nd trimester MSS
from 1992, NT from 1999), (Gyselaers et al. 2004b). The group having NT and 2nd trimester MSS
included a very small number of DS cases (n=9). The proportion of older women in the sample was
small as many of these women would have had an invasive test rather than screening (Gyselaers et al.
2004b). Women who had abnormal NT were probably removed as they would have had invasive
screen and not MSS. These limitations could explain the finding (which contradicts other studies) that
NT has a better performance than a sequential strategy combining NT and 2nd trimester MSS.
A prospective cohort study compared serum integrated screening to TT and quad test (Knight et al.
2005). When cut-offs were chosen so the DR was close to 70%, serum integrated screening had a lower
FPR (2%) than both quad test (3%) and TT (5%).
In general studies found that stepwise, contingent and fully integrated screening performed better
(higher DR and lower FPR) than screening in a single trimester and that screening combining tests in
an independent manner screening had an improved DR compared to screening in either trimester but
the FPR was higher. Serum integrated screening had a similar performance to 1st trimester combined
test and may be useful when staff trained in NT are not available (Wald et al. 2003b).
Comparison of performance of integrated and sequential screening strategies.
Ten papers were identified that compared integrated or sequential screening strategies. Seven of these
papers compared conventional integrated or sequential screening strategies: fully integrated (or serum
integrated), stepwise, or contingent screening. Some also presented results for screening where tests
were combined in an independent manner. The results of these papers are presented in Table 15.
Five papers compared stepwise screening to fully integrated screening (Cuckle et al. 2005; Hackshaw
and Wald 2001; Malone et al. 2005; Palomaki et al. 2006; Wald et al. 2003b). In most studies
integrated performed marginally better than stepwise screening. Where DR was fixed, integrated had a
decreased FPR. In one paper where the FPR was fixed at 5% integrated screening had a decreased DR
(93% versus 95% for stepwise), (Cuckle et al. 2005).
Three papers compared the fully integrated test to a conventional contingent strategy (Benn et al.
2005a; Cuckle et al. 2005; Palomaki et al. 2006). In one paper the results (FPR) varied depending on
the policy but in general integrated had a slightly better DR for the same risk cut-off (Benn et al.
2005a). In another paper at a fixed 5% FPR, integrated screening had a DR of 93% and contingent had
a DR of 94% (Cuckle et al. 2005). In the third paper for a fixed DR integrated screening had a lower
FPR (Palomaki et al. 2006).
Two papers directly compared contingent screening to stepwise screening. In one, at a fixed 5% FPR
contingent screening had a DR of 94% and stepwise had a DR of 95% (Cuckle et al. 2005). In the other
at a fixed risk cut-off stepwise had a DR of 90% and FPR of 1.7% whereas contingent screening had a
DR of 88% and a FPR of 1.4% (Maymon et al. 2005).
In the one paper that had a comparison between a screening method combining tests (combined test
and quad test) in an independent manner with sequential and integrated strategies, independent
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
92
screening had a lower DR (86%) compared to stepwise (95% with 1st trimester fβhCG), contingent
(94% with 1st trimester fβhCG) and fully integrated (93%) for a fixed FPR of 5% (Cuckle et al. 2005).
Three of the appraised papers only had results comparing non-conventional integrated or sequential
screening strategies (and so were not included in Table 15). One of these was a case-control study that
compared screening combining NT and TT in an independent manner (disclosure) versus an integrated
manner (non-disclosure), (Herman et al. 2002). The result showed the non-disclosure strategy had an
improved FPR but a decreased DR compared to the disclosure strategy (Herman et al. 2002). These
results contradict other results where DR is improved and FPR decreased by integrated screening
compared to independent screening. As discussed earlier, a case-control design is not ideal for
determining the validity of a screening method. The study also had limited details on how risk was
determined and the sample was biased by the fact that cases and controls were from different hospitals
and most of the cases had already been detected through NT screening (Herman et al. 2002).
Another paper aimed to compare the performance of screening (either with fβhCG, and AFP or with
fβhCG , AFP, and uE3) when different gestational dating policies were used (Rahim et al. 2002). It is
not clear when different samples were taken, but the GA for sampling was given as 13-21/40.
Screening with fβhCG, AFP, and uE3 had a slightly better DR (67.9% with a policy of scanning all
women for dating) compared to screening with fβhCG and AFP (63.2%), in agreement with the
evidence that combining first and second trimester tests improves performance of DS screening.
The third paper with a comparison of unconventional integrated or sequential methods compared a
three-stage contingent screening strategy with screening combining the same markers in an integrated
manner (Wright et al. 2006). The three stage screening strategy involves all women having 1st trimester
fβhCG and PAPP-A, and those with a very low risk would have no further screening (Wright et al.
2006). All other women would have NT (Wright et al. 2006). Those with a high risk when combined
with 1st MSS results would have an invasive diagnostic test, those with a low risk would have no
further testing, and those with an intermediate risk would have 2nd trimester quad test (Wright et al.
2006). This strategy achieved an 89.5% DR for a 1.9% FPR at the best risk cut-off. While the
integrated method had a higher DR and lower FPR (92.2%, 2.1%) most women having the contingent
strategy would only require 1st trimester screening, while for the integrated approach all women would
need testing in both trimesters (Wright et al. 2006).
Overall these papers suggest that fully integrated screening is marginally better than both stepwise and
contingent screening (with a lower FPR for a fixed DR) and that the validity of stepwise and contingent
screening is similar.
Table 15.
Comparison of the validity of fully (or serum) integrated screening, stepwise
screening, contingent screening, and screening combining tests (combined test and
quad test) in an independent manner
Reference
(Wald et al. 2003b)
(SURUSS)
(Malone et al. 2005)
(FASTER)
(Hackshaw and Wald
2001)
Test
Stepwise screening
(1:250 2nd T)
Integrated (risk cutoff set so DR =
stepwise)
Age standardised5% FPR
Serum integrated
Fully Integrated
Stepwise (2.5% FPR
for each screening
component)
Modelling-Stepwise
(5% FPR 2nd step),
integrated (same
DR)
Stepwise
integrated
DR (%), (95% CI)
93
FPR (%), (95% CI)
9.8
93
4.5
88
96
(81-92)
(92-97)
5
5
95
(91-97)
4.9
95
95
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
5 9.2
5 4.4
93
Table 15.
Reference
(Benn et al. 2005a)
(Cuckle et al. 2005)
(Maymon et al. 2005)
(Palomaki et al. 2006)
Comparison of the validity of fully (or serum) integrated screening, stepwise
screening, contingent screening, and screening combining tests (combined test
and quad test) in an independent manner (continued)
Test
Modelled-UK policies
Contingent screening
(overall risk 1:250)
Contingent screening
(overall risk 1:100)
Integrated testcontingent manner
(overall risk 1:250)
Integrated testcontingent manner
(overall risk 1:100)
Integrated test-non
disclosure (overall
risk 1:250)
Integrated test-non
disclosure (overall
risk 1:100)
Modelled-USA
policies
Contingent screening
(overall risk 1:270)
Contingent screening
(overall risk 1:130)
Integrated testcontingent manner
(overall risk 1:270)
Integrated test
combined in
contingent manner
(overall risk 1:130)
Integrated test-non
disclosure (overall
risk 1:270)
Integrated test-non
disclosure (overall
risk 1:130)
Modelled 5%FPR
Serum integrated
Integrated
Stepwise-fβhCG
Independent
manner-fβhCG
Contingent -fβhCG
Modelled
Stepwise
contingent
Modelled DR for 5%
FPR and integrated
set so same DR
Stepwise (1st T1:168, 2nd T-1:165)
Versus
Integrated (1:275)
Contingent (lower
risk 1:3250, 1st T
1:168, 2nd T 1:170)
Verus
Integrated
DR (%), (95% CI)
FPR (%), (95% CI)
91.4
2.1
88.2
1.1
91.9
2.2
88
1.0
92.1
2.2
88.3
1.0
89.1
3.1
86.2
1.9
90.5
3.4
86.8
1.8
90.7
3.4
87.0
1.8
78
93
95
86
94
5
5
5
5
5
90
88
1.7
1.4
89.9
5
89.9
3.1
89.8
5
89.8
3
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
94
Other comparisons
Two papers looked at the performance of screening when repeat measures of the same analytes were
taken in both trimesters. The first paper found that repeat measures of some markers (e.g. PAPP-A and
uE3 or total hCG) with and without NT performed better than combined screening, serum integrated
and fully integrated screening (lower FPR for a fixed 85% DR), (Wright and Bradbury 2005).
The authors of the second paper felt that the methods of the above study yielded “implausible riskestimates” when using repeat measures in several highly correlated markers (Wald et al. 2006b). To
overcome this issue they used ratios of the marker levels in 1st trimester and 2nd trimester which they
called the cross trimester (CT) ratios (Wald et al. 2006b). The modelled estimates of the DR for a 5%
FPR were higher for the integrated test when using CT ratios compared to the conventional integrated
test (using hCG-97.4% versus. 94.1%), (Wald et al. 2006b). The authors commented that while it
seems inconsistent that discrimination is improved if sampling of highly correlated analytes is repeated
across 2 trimesters, this is achieved because what is being measured is not two markers, but one
marker and the change in its concentration throughout a pregnancy (Wald et al. 2006b).
This paper also had results for the conventional integrated test using fβhCG compared to total hCG. For
a fixed 5% FPR the DR of the integrated test using fβhCG (94.2%) was similar to using hCG (94.1%),
and for a fixed DR of 85% the FPR of integrated using fβhCG (0.88%) was slightly lower than for hCG
(0.95%), (Wald et al. 2006b). There were no CI provided and these differences are too small to make a
conclusion on which is the most valid method.
One paper aimed to compare different combinations of 1st and 2nd trimester markers including a new
marker, the proform of eosinophil major basic protein (proMBP) (Rode et al. 2003). A combination of
AFP, hCG and ProMBP had a higher DR (79%) for a fixed 5% FPR than the conventional TT (AFP,
hCG and uE3-61%), and a combination of AFP, hCG, uE3 and ProMBP had a higher DR (83%) for a
fixed 5% FPR than the conventional Quad test (69%). The tests using ProMBP all had higher DR than
the combined test (76%), (Rode et al. 2003). As previously discussed the data were from a study where
-the NT was used clinically in the 1st trimester and nearly all women included in the analysis had a
negative NT screen which will bias the results in favour of 2nd trimester screening. The conventional
integrated test had a DR of 86% compared to a method combining NT, 1st trimester fβhCG, 2nd
trimester AFP and ProMBP which had a DR of 90%. While these results suggest that ProMBP may be
an important new marker for DS, there needs to be a larger prospective study using fresh samples to
confirm these results.
Difficulties implementing any of the screening strategies
Six papers noted problems with NT measurement. In one paper screening with NT was not achieved in
some women because either CRL corresponded to a gestational age outside the screening range, or
because NT was not able to be successfully measured (Audibert et al. 2001). In another paper
transvaginal USS (rather than transabdominal USS) had to be performed for 14% of NT measurements
(Michailidis et al. 2001).
A number of papers recorded the proportion of women in whom NT screening was unsuccessful: NT
screening failed or the measurements were suboptimal in 7% (Malone et al. 2005), for 0.22% NT could
not be measured successfully (Lam et al. 2002), 98.6% of women had successful NT measurement with
a mean duration of scan 12mins (range-5-26 mins), (Rozenberg et al. 2002), and for one study 9% of
pregnancies had no NT obtained within 20 mins (Wald et al. 2003b). This was worst before 10/40
weeks and after 14 weeks and best at 12/40) (Wald et al. 2003b). This last study also noted that the
failure rate decreased significantly over the study period, and also that the make and model of the USS
machine influenced the ability to get an image as did experience of the ultrasonographer (Wald et al.
2003b). In this study using only NT images that were judged satisfactory improved screening
performance (Wald et al. 2003b).
Four papers noted problems with serum screening-most commonly these were problems with
defaulting from 2nd trimester maternal serum screening (Audibert et al. 2001; Babbur et al. 2005;
Knight et al. 2005; Lam et al. 2002). In one study of 11,159 who agreed to participate, only about 80%
submitted both samples in the right gestational range (some had 1st trimester serum screening too early
or late, and others had no 2nd trimester serum screening due to fetal loss, declining to have screening,
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
95
changing residence/provider, having amniocentesis or ToP between trimesters or having 2nd trimester
serum screening too late), (Knight et al. 2005). This paper also had problems as they used a lower cutoff for 1st trimester screening of 8/40. As two of three didn’t have dates confirmed at this time and
PAPP-A had not been validated for before 8/40, these women had to have 2nd trimester serum
screening (Knight et al. 2005).
Two papers noted problems with combining results of screening in two trimesters. One noted issues
with matching samples from the two trimesters. This required extra work for lab staff (Knight et al.
2005). Another paper demonstrated through modelling how assuming tests were independent when
they were not could decrease the performance of stepwise screening: risks will be underestimated in
27% of DS cases and overestimated in 20% of unaffected (Benn and Donnenfeld 2005). In 10% of DS
the risk will be underestimated more than two fold and for 10% of unaffected cases the risk will be
overestimated more than 2 fold (Benn and Donnenfeld 2005).
Two papers commented on the importance of adjusting for certain factors in order to correctly
determine risk. One study showed that not adjusting for maternal weight meant a small increase in
FPR, and that not using USS for dating also increased FPR (Wald et al. 2003b). Another study
demonstrated that women who had false positive results in previous pregnancies had high FP rates in
subsequent pregnancies, and that these rates could be greatly reduced by adjustment for markers in
previous pregnancies (this adjustment slightly reduced DRs), (Wald et al. 2006a).
Summary of results
There was a high level of consistency supporting:
1.
Low performance of maternal age alone as a screening test compared to other screening strategies.
2.
NT and 1st trimester MSS having similar performance (FPR and DR) to 2nd trimester serum
screening.
3.
Combined test being a more valid screening test than all screening strategies in the second
trimester (and the first trimester-see Chapter 3).
4.
Serum integrated screening having a similar performance to combined screening.
5.
Screening combining tests in an independent manner increasing DR compared to screening in
either trimester alone, but having a higher FPR. This strategy is not recommended (Cuckle et al.
2005).
6.
Screening performance being improved if integrated or sequential methods (fully integrated,
stepwise, and contingent) are used rather than screening confined to one trimester.
7.
Fully integrated screening having a better performance than both stepwise and contingent
screening. Fully integrated screening has a lower FPR for a fixed DR.
8.
The validity of stepwise and contingent screening being similar.
There appears to be some support for improved performance using strategies which repeat measures of
the same analyte in the 1st and 2nd trimester. Another marker, ProMBP showed some promise but
further research is needed.
There were some difficulties noted with the screening tests. Mostly these were issues with NT: either
NT measurement was not successful in all women or it took more time than expected. There were also
a number of papers that noted the problem of women defaulting from 2nd trimester maternal serum
screening. Adjusting for maternal weight, dating using USS, and adjusting for false positive results in
previous pregnancies was noted to increase screening performance.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
96
Conclusion
Quality control of NT screening will be a major consideration if it is used in a population based
screening programme. The problem of women defaulting from 2nd trimester maternal serum screening
has implications for screening methods which depend on women having screening in both trimesters
(especially for integrated screening which only involves PAPP-A and NT, rather than the combined test
used by contingent and stepwise screening).
Combined screening is better than any other 1st trimester or 2nd trimester screening strategy. Screening
which combines tests in an independent manner may increase DR compared to screening confined to
either 1st or 2nd trimester but it will increase FPRs.
Fully integrated screening is marginally better than both stepwise and contingent screening with a
lower FPR for a fixed DR and that the validity of stepwise and contingent screening is similar.
However, most of this evidence is based on papers using statistical modelling as it is not possible to
both disclose and withhold results for the same individuals. These models make assumptions such as
the number of women who will return for 2nd trimester screening, which may not be accurate in the
real-world. Some modelling papers use the same primary data, similar modelling techniques, and
similar assumptions which may mean the same or similar results are repeated. Confirmation of the
performance of these strategies is required in large prospective cohort studies.
Overall, the evidence indicates that integrated or sequential screening has superior screening
performance for DS compared with screening confined to either 1st or 2nd trimester and any choice of
screening should be selected from these strategies (fully integrated, stepwise, or contingent screening).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
97
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Audibert et al. 2001)
Compared 1st T NT to screening with
2nd T double test (total hCG), or a
strategy which combined the 2
screening methods (1. having either
test positive, or 2. combined risk >
1:250).
May 1994 -December 1997 DS screening
(1st T NT USS and 2nd T double test)
routinely offered to women who
booked at the hospital.
Outcomes
The outcomes extracted for
this table are the DR and
FPR for DS screening for NT
and double test at different
cut-offs (NT ≥ 3mm, NT risk ≥
1:250, MSS risk ≥ 1:250) and
for combinations of the two
screening strategies: either
by a combined risk greater
than ≥ 1:250, or where NT ≥
3mm or MSS risk ≥ 1:250.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Women > 38 yrs were excluded-this is therefore a
low risk population.
NT ≥ 3mm
58% (30-86), 1.8% (1.4-2.3)
NT (1:250)
67% (35-90), 4.3% (3.7-4.9)
Double (1:250)
60% (26-88), 3.3% (2.7-3.8)
NT ≥ 3mm or MSS risk ≥ 1:250
(Independent manner)
90%(55-100 , 4.8% (4.1-5.5)
Combined risk ≥ 1:250
(stepwise manner)
90%(55-100, 2.6% (2.1-3.1)
This was an interventional study. Those positive by
1st T NT sometimes had IT and ToP before 2nd T. This
will decrease the DR of 2nd T MSS compared to 1st T
NT. Difficult to compared results with a nondisclosure strategy.
University Hospital
(Hôpital Antoine
Béclère)
France
Prospective cohort
study
Grade III-2
NT measured using standardised
methods by specially trained staff.
Cystic hygroma considered
increased NT. TA USS where possible
or TV USS. NT at 12-13/40.
5245 consecutive women scanned.
Exclusions (1080): twins (161), CRL
outside the range 38-84mm (303), NT not
measured or recorded (219), and MA
over 38 yrs (397) as these women were
routinely offered AC.
35 lost to follow-up.
AFP and total hCG were measured
(Ortho Clinical Diagnostics)
between 14-17+6/40. Cut-off risk of
1:250 risk (Prenata software, Ortho
Clinical diagnostics).
NT derived LR for each patient was
calculated using parameters from
Nicolaides et al. 1998 (as
referenced in this paper) and NT
distribution in this population.
To combine NT and MSS risks, MA
related risk and MSS LR multiplied by
NT LR.
Karyotyping suggested when NT ≥
3mm, MSS positive or abnormalities
on 2nd T USS.
4130 analysed.
Other chromosomal
disorders included as
unaffected.
Mean age 30.1 yrs (16-37).
3,790 had MSS (of whom 65 had positive
NT)
verification
7.6% had prenatal
karyotyping.
Most women who had abnormal NT also
had 2nd T MSS (before AC). Not possible
when women had CVS and requested
ToP before 14/40.
Fetal postmortem following
every ToP, spontaneous
abortion, or intrauterine
demise.
340 did not have MSS as declined test or
had fetal loss or ToP.
All newborns examined by
paeds and karyotyping in
those suspected of
chromosome abnormalities.
Spectrum of disease: 12DS/4130 = 0.29%
Difficulties implementing any
of the screening strategies
Successful screening was not
achieved because CRL
outside range (n= 303) or
because NT was not
measured (n=219).
340 did not have MSS as they
declined the test or had fetal
loss or ToP before 2nd trimester.
20 cases of chromosomal disorders
other than DS.
All those with an ongoing
pregnancy also had USS at 20-24
weeks.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
A better way to combine 2 tests is with an
algorithm based on MA, NT (related to CRL), and
MSS-none was available at time of study. The
method of combining risk as was done in this study
(MA and MSS-derived risk X NT-derived LR)
assumes NT and serum independent. This study
found no correlation between tests but some with
large NT not included. Needs further studies.
Authors’ conclusions
The results suggest that NT screening compares
favorably with MSS (double test) although there
was over-lap in CI’s which does not allow a firm
conclusion. NT also has the advantage of
confirming viability, dating, detecting multiple
pregnancies and structural abnormalities.
Reviewer’s conclusions
The study had excellent follow-up of pregnancy
outcomes. The intervention after 1st T NT meant the
sample is biased. The results of this study suggest
that combining the results of 1st T NT and 2nd T
double test is better than either method on its
own.
98
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Schuchter et al. 2002)
Compared screening with 1st T NT to
TT (AFP, uE3, and hCG) and a
combination of the two (where
positive results if screen positive by
either method).
NT done in 9,789 pregnancies and
9,642 also had TT over 5 year period
(January 1994-December 1998.
Outcomes
The performance of
screening using MA (≥
35yrs), NT, TT or combined
screening (either NT and/or
TT positive) is presented.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Retrospective design-may mean less
ascertainment of DS cases.
MA
47.4%(24.9-70), 10.6%(10.011.2)
NT
57.9%(35.7-80.1), 2.3%(2.0-2.6)
TT
91.7% (62-100), 5.2%(4.8-5.7)
Combined NT and TTindependent manner
94.7% (74-100), 7.0%(6.5-7.5)
Intervention study-some who were screen positive
in 1st T had IT and ToP and therefore did not have
2nd T MSS. Sample will be biased.
Danube Hospital
Vienna, Austria
Retrospective cohort
study
Grade III-2
The policy at the hospital was to
offer women NT (& CRL) at 1113/40. NT by TA USS or TV if not
feasible, using standardised
methods and trained staff. Rarely
needed to reschedule a visit for
repeat measure. GA using USS to
correct discrepancies between LMP
and CRL.
NT measured and for those with NT
≥ 3.5mm CVS performed. All others
asked to return for TT at 16/40.
TT using Ortho Clinical Diagnostics
kits. Risk factors using alpha
software (logical Medical Systems)
which takes MA into account.
Only the 9,342 women delivered at
this hospital used in the analysis as
outcome not followed-up if
delivered elsewhere. 9315 of these
also had 2nd T MSS.
Median age at delivery was 28 yrs
(range 15-46 years), and 10.7% ≥ 35
years.
Median CRL 48mm (range-3565mm).
Spectrum of disease: 19DS /9342 =
0.20%
12 with other chromosomal
abnormalities included as
unaffected.
Verification
Newborns all examined by
paeds. If suspected
chromosomal abnormality
karyotyping was done.
Difficulties implementing any
of the screening strategies
No objective problems noted.
Rarely needed to reschedule
a visit for repeat measure
(doesn’t say how many).
AC offered to those in whom NT 2.53.4 mm (had been told at the time
of NT), TT risk ≥ 1:250 and all women
≥ 35 years.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Small number of DS (n=19).
Author’s conclusion
The data suggest that the combination of NT
measurement in 1st T and the TT in the 2nd T is
associated with a very high DR of DS at a relatively
low screen positive rate (SPR).
Reviewers’ conclusions
The results show screening combining NT and 2nd T
TT has a better DR but higher FPR than TT or NT
alone. However this is an interventional studysome with high NT in 1st T did not have 2nd T TT.
99
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Michailidis et al. 2001)
Compared screening using NT to
screening with double test and to
screening combining NT and
double test. Some DS also detected
by USS soft markers.
Women routinely screened in a
single hospital setting. From data
base identified 9548 sequential
women who had 1st T USS after
January 1995 with EDD before 1st
January 2000.
Outcomes
Outcomes were the DR and
FPR for MA ≥ 35yrs, NT,
double test, or screening
combining NT and MSS.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Retrospective design.
Maternity unit of a
university hospital.
London, UK
Retrospective cohort
study
Grade III-2
1st T USS for NT, viability, CRL, and
number of fetuses and chorionicity.
GA corrected using CRL. NT
measured using standardised
methods. When NT could not be
measured by TA USS, TV scan
performed.
If NT above 99th centile (or structural
abnormalities) offered IT.
Women were offered the option of
2nd T double test (AFP, free β hCG).
AFP and free β hCG were
measured by radio-immunoassay
and immunoradiometric assays. The
risk for DS determined by screening
software (Screenlab, QC
technology) using LR method.
When risk at term >1:250 offered
invasive screen.
Retrospectively applied a formula
(Cuckle and Sehmi, 1999 as
referenced in this paper) and LR of
Nicolaides et al. 1998 (as
referenced in this paper) in order to
calculate combined risk based on
1st T and 2nd T screening and MA.
Excluded 309 with fetal demise, and
those presenting outside GA range
of 10-14/40 and those without NT
measurement. Left 8536 eligible.
7447 had outcome data.
Mean MA = 30.1 year (range-13-50
years). 21.3% ≥ 35 years.
The ethnicity was 75.6% Caucasian,
11% African and West Indian, 10.7%
Asian, and 2.7% Oriental.
Mean GA at NT was 12+5/40.
Spectrum of disease: 23 DS/7447 =
0.31%
23 other chromosomal disorders.
4864 also had 2nd T MSS (double
test). MA distribution not sig diff
between two groups. (21.97% > 35
yrs.) DS 4/4864 =0.08%.
Unclear how calculation
done for combining NT and
double test. Unclear the
denominator for this
calculation-CI therefore not
calculated for FPR.
Also used Cuckle and
Sehmi mathematical
formula to interpret double
test results when already
had 1st T screen.
Verification
Invasive testing offered to
those with positive NT
screen, USS showing
structural abnormality,
positive double test, MA
>37 yrs and requesting
invasive testing, Fmhx of
chromosomal
abnormalities, or maternal
anxiety. Overall 8.5% had
invasive screen.
MA ≥ 35 years
56.5%, (34.5-76.8), 21%(20.121.2)
NT fixed 5% FPR
82.6% (61.2-95.1)
Double test (1:250)
50% (6.8-93.2), 8.7%(7.9-9.5)
Combining NT and double
(?stepwise)
90.5% (69.6-98.8), 4.2%
Using correction for having 1st
T screening, double DR
increased and FPR decreased
(75%, 5%).
Difficulties implementing any
of the screening strategies
TV USS had to be performed
for 14% of NT measurements.
Pregnancy outcome from
hospital maternity
database, labour ward
records, or from patients
(outcome request letter).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Interventional study-results of 1st T NT were acted
on leaving only 4 cases of DS in those who had
double test. Difficult to compare the two
methods.
Raw data was not documented and confusing
text- difficult to check how figures calculated.
According to Hackshaw and Wald (Hackshaw
and Wald 2001) should only use the Cuckle and
Sehmi formula if all who had 1st T then have 2nd T
screening regardless of the result.
Author’s conclusion
1st T NT measurement is an effective screening test
for the prenatal detection of fetuses with DS.
Although the MSS in the 2nd T can detect
additional DS cases this may be outweighed by
the delay in diagnosis, the extra visits and cost so
that the right time for MSS is most likely to be in the
1st T.
Reviewers’ conclusions
Some biases may affect the accuracy of the DR
and FPR (especially for 2nd T MSS) and the ability to
compare with non-interventional studies. Difficult
to understand how the figures were calculated for
double test and combining NT and double test.
Results indicate that 1st T NT performs better than
double test but that combining the two increases
performance.
100
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Dommergues et al.
2001)
Compared screening by NT, 2nd T
double test, and combining results
of these two screening methods
(screen positive where either test
was positive). Also compared 2nd T
sonography, but these data were
not extracted for this review.
AMA-38 years and over.
Outcomes
The outcomes were the DR
and FPR for NT ≥ 3mm,
double test (1:250) and a
screen where either NT or
double test positive
constituted a positive
screen.
Accuracy of screening
methods DR (95% CI), FPR
(95% CI)
Limitations
Small number of DS cases (n=7).
University Hospital
(Hôpital Antoine
Béclère)
France
Prospective cohort
study
The study was non-interventional.
Women had MSS even where NT
was ≥ 3mm indicating need for AC
and in 3 women who had CVS.
Grade III-2
NT obtained at 10-14/40 using
standardised methods (as per
Nicolaides et al.) by staff trained in
NT measurement.
AFP and hCG analysed at 15-17/40
and risk calculated using Prenata
software, Ortho Clinical Diagnostics.
If NT ≥ 3mm or MSS >1:250 or if
structural anomalies on 2nd USS
recommended karyotyping.
The sample consisted of 359
consecutive women aged 38-47
seeking antenatal care before 14/40
in a maternity hospital between 1994
and 1997 who consented to have NT
and 2nd T MSS.
Follow-up in all 359 patients.
Disease spectrum = 7/359
= 2%
2 cases of other chromosomal
disorders-included in analysis as
unaffected
Verification
227 had karyotyping.
Follow-up included clinical
examination of all
neonates, cytogenetic
records when available,
and pathological
examination of all cases of
fetal loss or ToP.
NT ≥ 3mm
100% (59-100), 3.3% (1.5-5.1)
Double test (1:250)
86% (42-100), 33% (28-38)
Combining NT and double test
(independent manner)
100% (59-100), 35% (30-40)
Difficulties implementing any
of the screening strategies
No objective difficulties noted.
2 cases of fetal loss ≤ 22
weeks considered normal
on the basis of having no
significant structural
anomaly at post-mortem.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
AMA of the sample limits the generalisability of the
estimates of performance.
Few details of how risk calculated for double test
(where parameters obtained from)
Author’s conclusions
AC may be offered on a selective rather than
routine basis in women over 38yrs, based upon the
results of noninvasive screening tests”
Reviewers conclusions
The study has a small sample size and is limited to
women over 38 yrs. However the results indicate
that NT has a higher DR and lower FPR compared
to double test. A screening strategy where a
screening was positive if either NT or double tests
were positive had same DR as NT and higher DR
than double test, but higher FPR than NT or double
test alone.
101
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Rozenberg et al.
2002)
Comparing NT to double test
(fβhCG, AFP) and to screening
where either NT or double test
positive = a positive screen. Also
used modelling to compare NT and
double test to screening combining
NT and double test results (risk
1:250).
Six centers participated in the study
which was conducted between
March 1994 and December 1997. All
women having prenatal care at the
hospitals and requesting DS
screening were invited to
participate.
Outcomes
The observed DR and FPR
for NT ≥ 3mm, double test
(1:250), and screening
combining the two
(considered a positive test if
either NT or double test
positive).
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
While it was intended that all would have 2nd T
MSS some had only NT (possibly because of a
positive NT screen). Also some only had MSS.
Multicentre study: 2
tertiary referral centres
and 4 primary referral
centres.
Prospective cohort
study
Grade III-2
NT carried out 12-14/40. According
to the paper TV measured unless
position meant had to measure by
TA USS. Confirmed GA with CRL. NT
measured as per Nicolaides.
MSS at 14+1/40-17/40. Uniform
handling and storage of specimens.
fβhCG and AFP analysed using
ELISAs and commercial kits (CIS Bio).
Marker levels expressed as the
gestational specific MoM and risks
estimated from MA and MoM using
commercial software (CIS Bio) that
uses normal medians from a French
population at 14-17/40
AC advised when either NT ≥ 3mm
(procedure delayed until after
MSS), and when risk based on MSM
was ≥ 1:250 at term.
Retrospective analysis was done on
data collected in the study. NT and
MSS marker expressed as MoM
using own data set and risks
calculated based on published
parameters.
Eligible if 18-37 years, no Fmhx DS,
singleton, and intention to deliver at
participating hospital.
9444 screened over period.
326 outcome not known and
excluded from analysis (including
113 who miscarried before 24/40
without karyotyping)
9118 in analysis-of whom:
5506 had both USS and 2nd T MSS,
821 had only USS
2791 had only MSS.
The results were also
modelled for a population
with a mean maternal age
of 28 yrs and a coefficient
of variation of 16%.
Compared NT to double
test and to combined risk of
NT and MSS ≥ 1:250.
Verification
Amniocentesis when NT
more than 3mm or risk of
MSS more than 1:250.
About 8.6% invasive screen.
6327 had USS but only 6234 had
successful measurement of NT.
8297 had MSS.
Median MA 30.5 yrs.
Spectrum of disease: 21 DS /9118 =
0.23%
No details of how
pregnancy outcomes
verified or if fetal losses
were karyotyped.
NT ≥ 3mm
62%(41-83), 2.8% (2.4-3.2)
Double (1:250)
55%(33-77), 5.7% (5.2-6.2)
Combined screening
(independent manner)
81% (58-95), 8.4% (7.9-9.0)
modelled
DR, FPR(1:250)
NT
53.4%, 4.6%
Double
68.8%, 7.8%
NT & double (1:250)-stepwise
manner
80.6%, 5.3%
DR for 5% FPR (1:250)
NT (1:250)
54.6%
Double (1:250)
59.7%
NT & double (1:250)-stepwise
manner
79.8%
Difficulties implementing any
of the screening strategies
98.6% of women had
successful NT measurement.
Mean duration of scan 12mins
(5-26 mins)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Those over 37 yrs old excluded-low risk population
selected.
Authors felt that because the intervention was NT
≥ 3mm this may have meant that when NT < 3mm
did try as hard to be accurate-therefore results
not so good when converted to MoM.
Author’s conclusion
The study results suggest a 25% increase in the DR
of DS using a combination of NT measurement at
12-14/40 and MSS at 14-17/40 for a 5% falsepositive rate. However this delays risk assessment
and invasive testing by some weeks.
Reviewers’ conclusions
Some intervention. However, the results show that
double test was better than NT and that a
combined screening where risk from both NT and
double test combined was ≥ 250 performed the
best.
102
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
(Rozenberg et al.
2002)
Adjusted for maternal weight. Log
Gaussian modelling was carried out
using standard methods (Royston
and Thompson, 1992 as referenced
in this paper) to estimate the DR
and FPR using our parameters
applied to a population with a
mean maternal age of 28 years
and a coefficient of variation of
16%.
Multicentre study: 2
tertiary referral centres
and 4 primary referral
centres.
Prospective cohort
study
Sample
Outcomes and
verification
Results
Grade III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
103
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Herman et al. 2002)
Compared disclosure and nondisclosure approaches of
combining 1st T NT and TT.
508 consecutive “normal”
pregnancies (previously described
method of data collection-Herman
et al. 2000 as referenced in this
paper). Data collected
prospectively.
Outcomes
The DR and FPR of a
strategy combining NT and
TT results in an independent
manner and DR and FPR of
a strategy combining results
of these two tests in an
integrated or non-disclosure
manner. Applied an age
“adjustment risk technique”
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Case control study limits the spectrum of disease
and is not the ideal design to determine the
accuracy of a screening test. No cases of other
chromosomal disorders. Proportion of DS high4.3%. No details of MA.
Medical centre,
University Hospital.
Israel
NT done at 10-14/40 according to
Nicolaides et al. Risk based on FMF
software.
Case-control study
Grade III-2
2nd MSS at 16-19 weeks. LR for each
test used to calculate MA adjusted
FPR for non disclosure and
disclosure methods. MA a priori risk
from literature.
Estimated the FPR and DR by a
methodology of population
adjusted calculations previously
described in the literature (Pandya
et al. 1995 as referenced in this
paper), and using the MA
distribution of Israel in 2000.
Disclosure method either USS or
triple test risk ≥ 1:250. Tests
performed sequentially.
23 DS cases collected from various
sources: 8 from local 1st T NT
screening, 11 had NT elsewhere and
were referred to centre for ToP, 2
from neighbouring hospitals, 2
identified as DS after birth. Blood
taken before amniocentesis. Only
those with good NT images included.
Verification
No details other than 21/23
DS detected before birthmainly increased NT.
NT and TT-Disclosure method
(independent manner)
88.7%, 9.5%
NT and TT-Non
disclosure(integrated manner)
75.3%, 2.4%
Difficulties implementing any
of the screening strategies
No objective difficulties noted.
All had 1st T NT and 2nd T MSS.
Method of identifying
control pregnancy
outcomes was unclear.
Total 531
Spectrum of disease: 23/531= 4.3%
Possible bias as cases from different hospitals-tests
may not be done identically as controls, and tests
done at different times. Most DS (91%) had been
identified before birth mostly from NT screening.
No details of the testing kits.
Exact method of determining DR and FPR unclear
(used ‘a methodology of population adjusted
calculations’).
Author’s conclusion
The disclosure approach resulted in considerably
higher DR. The non-disclosure approach however
had a lower FPR.
No other details of population.
Reviewers’ conclusions
Biased sample. The result showed the nondisclosure strategy had a decreased DR but
improved FPR compared to the disclosure
strategy. These results are contradictory to other
comparisons where DR is usually improved by
integrated screening.
Non-disclosure if integrated figure ≥
1:250.
Risk derived from LR NT X LR TT.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
104
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Wald et al. 2003b)
The aim of the study was to
determine the most effective, safe
and cost-effective method of
screening for DS using NT, MSS, and
urine markers in the 1st and 2nd T.
Urine screening is outside the scope
of this review and therefore
methods and results are not
reported here.
25 maternity units in the UK and one
in Austria who were screening for DS
in 2nd T and who agreed to collect
observational date in 1st T. Most
started recruiting in September 1996
and ended April 2000.
Outcomes
The outcomes extracted for
this evidence table are the
FPR for a fixed 85% DR for
fully integrated, serum
integrated, combined test,
quad test, TT, double test,
and NT. The results are for
1st T NT and serum at 10/40
except for NT screening
results (NT at 12-13/40). Also
extracted results for fixed
FPR of 5%.
Accuracy of screening
methods
Limitations
High median inhibin compared to other studies so
had to use published data.
Serum urine
ultrasound scan
(SURUSS) study
UK.
Prospective cohort
study and nested
case-control study.
Grade III-2
Had USS at booking visit (CRL,
viability, and if possible at least 3 NT
measurements). Quality control of
images, and all ultrasonographers
trained in NT measurement. If NT ≥
3mm flagged to ensure 2nd T serum
screen done. Allowed up to 20 mins
to get image. NT measurement
standardised across centres and
ultrasonographers. NT MoM based
on ultrasonographer specific
medians and upper truncation limit
of 2.5 MoM used.
Two sets of serum samples (from
booking and from 2nd T) were
stored at -40C. DS samples and
those of matched controls retrieved
and analysed. If serum collected
before 14/40 = 1st T.
AFP, fβhCG, total hCG, uE3 and
PAPP-A measured using
fluoroimmunoassay (Perkin Elmer)
and Inhibin-A using ELISA (Oxford
Bioinnovation and Diagnostic
Systems). Analysis was blinded to
outcomes.
47053 women with singletons
presenting at 8-14/40 were recruited.
Data set used for performance of
screening was 43,712 singletons
recruited at 10-13/40. 39983 had NT,
40387 had 1st T serum, 37362 had
2nd T serum.
MA was median 29 years % ≥ 35 was
16%.
Spectrum of disease: 101/ DS 47053 =
0.21%. (or 0.22% if only include 96%
where outcomes documented).
For biochemical analysis 1090
controls and 101 DS were retrieved. 3
DS had no serum or urine screen
available-serum analysis based on
98 DS samples. Each DS was
matched with 5 singleton controls
(n= 490) according to centre, CRL
(or BPD), MA, and duration of
storage or sample.
When estimated using MA,
the MA specific risk of DS
was for a standard
population of England and
Wales 1996-1998.
The confidence intervals
were calculated using
Monte Carlo simulation.
Results for a number of
other marker combinations,
different GA, and for
different fixed FPR, and
fixed DR are presented in
the report.
FPR (95% CI) for 85% DR
Integrated
1.2 (1.0-1.4)
Serum integrated
2.7 (2.4-3.0)
Combined
6.1 (5.6-6.5)
Quad
6.2 (5.8-6.6)
TT
9.3 (8.8-9.8)
Double
13.1 (12.5-13.7)
NT
20.0 (18.6-21.4)
DR for 5% FPR
Integrated
93%
Serum integrated
90%
Combined
83%
Quad
83%
TT
77%
Double
71%
NT
60%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Not everyone had all tests done.
Analysis on stored samples.
One of the authors belongs to the institution which
holds the patent for the use of uE3 as DS marker.
Same author is a director of a company
producing a commercial software package for DS
screening interpretation (USS and serum markers).
Also director of company holding a patent
application for integrated test.
Author’s conclusion
Overall the integrated tests have the best
performance, if NT is not available should use
serum integrated, for women attending only in
2nd T quad is best, for those only wanting 1st T
screening combined is best.
NT, double and TT without combination with other
screening methods are not worthwhile.
105
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
(Wald et al. 2003b)
After observation that urine did not
add to the performance an
additional 600 controls that had 1st
T and 2nd T samples taken were
selected and sample analysed. This
was in order to estimate screening
performance where GA based on
dates compared to screening
based on USS (CRL). Together with
490 matched controls this meant
over 1,000 samples could be used
for distribution parameters for both
methods of dating.
Serum urine
ultrasound scan
(SURUSS) study
UK.
Prospective cohort
study and nested
case-control study.
Grade III-2
Continued
Despite 1st T screening being
observational, 5 DS pregnancies
had ToP before 14/40 weeks. About
3 of these would have continued to
2nd T without miscarriage. Therefore
two samples were selected at
random to remove from analysis to
avoid overestimation of median
marker levels in DS pregnancies
(intervention bias).
There were 26 live births of which 10
were screen –ves. This means that
13 would have been expected in
2nd T (1/0.77), and there would
have been about another 3 screen
–ves who would have been
miscarried. Need to include these
as there would have also been
screen +ves who had ToP, but
would have miscarried if left, or will
overestimate the DR. Therefore 3 of
these pregnancies sampled and
levels added to those already
included.
Sample
Outcomes and
verification
Results
Comments
Verification
Verification of outcomes in
6 ways:
Staff at local hospitals filled
out a SURUSS outcomes
form at delivery.
Cytogenetic lab info linked
to SURUSS records.
National DS register linked
to SURUSS records.
Info from local obstetric
outcome records.
Form sent to women with
request to return details of
outcome.
Individual searches of those
outcomes not otherwise
obtained.
DR, FPR
Stepwise screening (1:250)
93%, 9.8
Integrated (risk cut-off set so
DR = stepwise)
93%, 4.5%
Reviewers’ conclusions
Large well designed study with unbiased sample
(adjustments for intervention). Excellent
verification of outcomes.
Results show similar results for 1st T and 2nd T but
integrating markers were better. Integrated had
better performance than stepwise screening.
Follow-up continued until
31st May 2001.
Completeness of
ascertainment. Would
expect 81 live births if no
intervention (55 of 71 ToP
would have gone to
term=77% plus 26 live births
= 81).
From MA distribution would
expect 87.
Difficulties implementing any
of the screening strategies
Overall 9% of pregnancies
had no NT obtained within 20
mins (worst before 10/40
weeks and after 14 weeks).
Best at 12/40.
The failure rate decreased
significantly over the study
period.
DS with unacceptable images
were close to the MoM for the
unaffected pregnancies.
The make and model of the
USS machine influenced the
ability to get an image as did
experience of the
ultrasonographer.
Depended on the machine
used and experience of the
operator.
Using only NT images that
were judged satisfactory
improved screening
performance.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
106
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
(Wald et al. 2003b)
The DS used in analysis was 101 – 2
ToP plus 3 as above = 102
(adjustment for intervention bias).
Serum urine
ultrasound scan
(SURUSS) study
UK.
Prospective cohort
study and nested
case-control study.
For each marker the MoM was
calculated for each GA (using CRL
or BPD to estimated CRL). The
medians were calculated using
unaffected pregnancy serum
markers adjusted for maternal
weight. There was no correction for
ethnicity.
Sample
Outcomes and
verification
Results
Not adjusting for maternal
weight meant a small increase
in FPR.
Not using USS for dating
increased FPR.
Grade III-2
Continued
To estimate risk the parameters (SD,
means and correlation coefficients)
were derived from the study
population. Used a published MoM
for inhibin-A as it appeared
unexpectedly high in the study
population.
The risk of having a DS pregnancy
at 17/40 was calculated using the
maternal age specific risk of a live
birth (corrected by multiplication of
1/0.77 to allow for DS fetal loss from
mid term to term) and LR for the
markers obtained by the
overlapping of the Gaussian
distributions of DS and unaffected
pregnancies.
No planned intervention in 1st T.
Antenatal diagnostic tests were
based on routine 2nd T results
(double, TT, or quad).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
107
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Gyselaers et al.
2004b)
Compares screening with 2nd T MSS
to screening combining the results
of NT and 2nd T MSS.
Since 1992 2nd T MSS samples from
all geographic areas in Flanders
have been analysed by General
Medical Laboratory in Antwerp
(AML).
Outcomes
Performance (DR for fixed
FPR) of screening with 2nd T
MSS (?quad test)
compared to a strategy
combining MSS and NT.
Compared screening
accuracy for those who
had 2nd T MSS but did not
have NT (36,382) to those
who had NT and 2nd T MSS
(3274).(i.e. totally separate
populations).
Unclear how the two tests
combined (presume
stepwise manner).
Accuracy of screening
methods
Limitations
Comparing two populations having two different
screening strategies over different time periods
(2nd T MSS from 1992, NT from 1999). The group
having NT and 2nd T MSS had very small number
of DS (n=9).
Lab samples from all
geographic areas.
Flanders, Belgium
Retrospective cohort
study.
Grade III-2
2nd T serum: AFP (Diagnostic
Products Corporation) fβhCG
(BioSource), uE3 (Diagnostic
Systems Laboratories) PAPP-A
(BioSource). The cut-off for a
positive screen was 1:300.
A total of 2700 NT measurements
sent to FMF for audit and used to
calculated MoM.
The total number of MSS samples (1st
and 2nd T) analysed by AML over
the 10 years of the study (1992-2002)
was 78,365. 51.7% had compete
follow-up = 40,490.
Since 1999 AML have also registered
details of NT and CRL.
Those who had 2nd T MSS but did
not have NT =36, 382. Those who had
NT and 2nd T MSS = 3274. Those who
had 1st T MSS and NT = 834-no further
analysis.
Spectrum of disease: 108 DS /39656 =
0.27%
Chromosomal disorders other than
DS considered unaffected.
5.5% study population ≥ 35 years
compared with 8.9% of the general
population (p<0.001).
Verification
Outcomes of pregnancies
and newborns from
obstetricians after birth.
DR (95%CI), FPR (95%CI)
2nd T MSS
69.7% (61-79), 5.5% (5.3-5.7)
NT and 2nd T MSS ( ?stepwise
manner)
55.6%(21-86), 7.6% (6.7-8.5)
DR for 5% FPR
2nd T MSS
66.7% (57-76)
NT and 2nd T MSS
44.4% (14-79)
Difficulties implementing any
of the screening strategies
None noted.
Clinicians mailed every
year for collection of
missing data and
contacted in person if did
not respond.
Compared prevalence in
screened population to
prevalence in Belgium.
No other details of who got
AC-presumably all who
were screen positive.
No details if karyotyping
used in case of fetal loss.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Across the two groups the proportion of women
over 35 yrs was less than in the general
population. Some over 35 yrs would have had IT
without screening.
No details of why some women had NT from 1999.
Possibly some women had only NT and not MSS
over this period as high NT so referred for IT. Only
those with normal NT would have 2nd T MSS. This
will decrease the DR of screening in the group
having NT and 2nd T MSS.
Unclear how pregnancies dated or whether staff
trained in NT. Unclear what the 2nd MSS was.
Author’s conclusion
In Flanders the uptake of 2nd T MSS in women
over 35 yrs is low. The performance of screening
decreased after the introduction of NT.
Reviewers’ conclusions
Poor design (comparing two separate nonrandomised populations) and biased samples.
These limitations could explain the finding (which
contradicts other studies) that NT is better than a
strategy combining NT and quad test.
108
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Gyselaers et al.
2004a)
Compared screening with 1st MSS
(fβhCG) to screening with the TT
(total hCG).
Since 1992 2nd T MSS samples from
all geographic areas in Flanders
have been analysed by General
Medical Laboratory in Antwerp
(AML).
Outcomes
The outcomes extracted for
this evidence table are the
DR and FPR for 1st T MSS
(1:85) compared to the DR
and FPR of 2nd T MSS, the TT
(total hCG) with a risk cutoff of 1:300.
Accuracy of screening
methods
Limitations
The study populations are completely separate
i.e. different tests done on different populations.
Also screened at different time periods and details
of other concurrent screening (e.g. NT) or invasive
testing (women over 35 yrs) in these time periods
which could also bias sample.
Lab samples from all
geographic areas.
Flanders, Belgium
Retrospective cohort
study
Grade III-2
Immunoradiometric assay used for
AFP (Diagnostic Products
Corporation) and fβhCG
(BioSource), and uE3 assayed with
radioimmunoassay (Diagnostic
Systems Laboratories). PAPP-A
measured by ELISA (BioSource). The
cut-off for a positive screen was
1:300 for 2nd T MSS and 1:85 for 1st T
MSS.
2nd T MSS was obtained
between1992-1998 which was
before the introduction of 1st T
screening for DS, and 1st T MS were
taken 1999-2003.
A total of 40,419 2nd T MSS samples
performed over study period.
Spectrum of disease in this group =
60DS /40419 = 0.15%
A total of 7079 1st T MSS samples
performed over study period.
Spectrum of disease in this group =
13 DS /7079 = 0.18%
5.1% of those having 2nd T MSS were
≥ 35 years, and 8.6% of those having
1st T MSS were ≥ 35 years.
Chromosomal disorders other than
DS presumably considered
unaffected.
Verifications
Outcomes of pregnancies
and newborns from
obstetricians after birth.
DR (95%CI), FPR (95%CI)
1st T MSS (1:85)
61.5%(52-86), 5%(4.5-5.5)
2nd T MSS (1:300)
73.3%(62.1-84.5), 5.6%(5.4-5.8)
Difficulties implementing any
of the screening strategies
No objective difficulties noted.
Clinicians mailed every
year for collection of
missing data and
contacted in person if did
not respond.
Compared prevalence in
screened population to
prevalence in Belgium.
Those with risks as described
offered invasive screening.
In the two time periods
studied, the prevalence of
DS in Belgium was 0.14%
and 0.17% which correlated
well.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Few details about the study population (GA at
screening) and how risks calculated (parameters
used in Gaussian distributions).
No details of lost to follow-up (presume kept in the
analysis as unaffected).
No adjustment for viability bias-1st T screening
detects cases that may not be viable in 2nd T.
Small number of DS cases in 1st T group (n= 13).
Author’s conclusion
The performance of both 1st MSS and 2nd MSS at
MA ≥ 35 yrs (these results not extracted) in
Flanders is excellent, even without the
combination with NT or integration of 1st and 2nd
T screening. The simplicity of methods makes them
good options for aneuploidy screening at AMA,
until high quality combined or integrated
screening is accessible to all women in Belgium.
Reviewers’ conclusions
Poor design for screening performance and
biased samples. Results indicate TT had better DR
and similar FPR than 1st T MSS (fβhCG and PAPPA).
109
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Babbur et al. 2005)
Compared screening with NT to a
screening method combining LR of
NT and the LR of TT.
Sample consisted of 3,188 women
with singleton pregnancies
requesting screening for DS (August
2001-March 2004) who had a
combined NT and triple test.
Outcomes
For this evidence table the
performance of NT was
compared to the
performance of combining
TT with NT. This was
calculated firstly with only
those who had both tests
(2725) then for the overall
performance-including all
those who were screened
with either NT or MSS (in a
stepwise manner).
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
NT ≥ 3-mm
64%; (38.8-78.9), 1.8 (1.3-2.3)
Combining NT plus TT stepwise
manner (1:250)
67% (27.9-92.5), 2.7% (2.1-3.3)
Overall screening
performance stepwise manner
(1:250)
88% (68.8, 97.5), 4.1% (3.4-4.8)
TT FPR for fixed 88%DR
20%
TT DR for fixed 4.8%FPR
60%
Limitations
High-risk group-median MA = 37 yrs so DR likely to
be higher than in a routinely screened population.
Women’s hospital
Cambridge, UK.
Prospective cohort
study
Grade III-2
NT measured according to FMF
criteria when CRL 45-84 mm. 3
images obtained and largest NT
used in analysis. Offered invasive
testing if NT > 3mm (which was the
current policy in the department). If
less than 3mm or declined CVS
offered the combination of the NT
results and TT at 14 weeks (Had
screened at 14/40 not 16/40 since
2000).
For those having both 1st T and 2nd T
screen the risk was calculated
multiplying the MSS risk by the
likelihood ratio for the reported NT
(as per Cuckle and Sehmi, 1999 as
referenced in this paper). Offered
invasive testing if combined risk DS
at term of >1:250.
All TT assayed markers at same lab
with commercial kits (PerkinElmer,
Wallac Oy). Three markers used in
combination with MA to determine
the risk of DS.
All results expressed as MoM for
medians of unaffected
pregnancies of same GA based on
local population. Adjusted for
maternal weight.
Median MA was 37 years (19-46 yrs)
Attending for NT offered as a self –
paying service at a maternity
Hospital and an outreach clinic, and
those attending for NHS funded NT
for previous fetal abnormality.
Excluded those who had non-viable
pregnancy at USS.
3188 total. 2725 had MSS after NT
(85% of 3188). 463 did not have MSS.
Most of those with normal NT scan
proceeded to 2nd T triple.
Mid trimester (12-16 /40) prevalence
for DS was 7.8/1000
The FPRs given in the paper
are the SPRs (as per raw
data in the paper). For this
reason CI not calculated.
Verification
Cytogenetic data (invasive
testing) and neonatal tests
for all women who
delivered within East Anglia.
Authors were not notified of
any missed diagnoses in
women delivering outside
the area (did not have
access to these records).
Difficulties implementing any
of the screening strategies
12.4% did not attend for triple
test.
Unclear if fetal losses were
karyotyped.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
14/40 for TT instead of usual 16/40.
Interventional so hard to compare screening with
NT (or the combination) to studies where NT (or
combination) was not interventional.
No details of how TT risk determined or risk cut-offs.
Author’s conclusion
In a high-risk group the combination of NT with TT
offers DR at least as good as either test while
allowing disclosure of an abnormal NT at scan
and reducing the FPR. Importantly FPR is less than
5%, which is lower than TT alone.
Reviewers’ conclusions
High risk group but for this population screening
combining NT and TT performed better than NT
alone.
110
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Knight et al. 2005)
Compared serum integrated
screening to quad and TT.
Women in Maine receiving prenatal
care from one of 229 primary care
prenatal practitioners were recruited
for the study between August 2001
and August 2003. Recruited women
presenting 8-13/40. Told about delay
in interpretation until 2nd T.
Outcomes
Outcomes given are the DR
and FPR at different cut-offs
for TT, quad and serum
integrated screening. Also
included the serum
integrated FPR adjusted
after USS dating.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Not all received all tests and these were removed
from analysis- may have biased sample if they
were more or less likely to have DS. Those
removed included those with fetal loss. However
did use the more conservative figure of the
expected DS for denominator (DR).
Primary care
Maine, USA
Prospective cohort
study
Grade III-2
First serum sample taken then
stored at -20C. Second sample
taken 15/40.
Designed a lab form to facilitate
sample matching. Modified the labs
database to accommodate the
additional sample and added a
matching algorithm for linking info
from both samples.
2nd T MSS evaluated by the
algorithm to see if 1st T MSS had
been taken. Staff usually verified all
matches. Occasionally had to
contact primary care to obtain
further information. Sent reminder
faxes that 2nd T MSS was due.
In 2nd T combined the results of all
five tests with MA associated risk to
produce a single DS risk using a
published algorithm and
parameters (Haddow et al. 1998;
Knight et al. 1998; Wald et al. 1999
as referenced in this paper).
11159 agreed to participate. Less
950 who had 1st T too early or too
late, less 1436 where no 2nd T MSS as
(575 fetal loss, 459 declined, 236
elected AC, 133 changed
residence/provider, 29 ToP, 4 second
sample too late)
Left 8733
Spectrum of disease: 16/8773 =
0.18%
Mean MA 27.8 (SD 5.5) and MA ≥ 35
years 11.3%.
GA at 1st T screening =10/40, and 2nd
T screening 16.9/40.
Maternal ethnicity: non Hispanic
Caucasian=98%.
The DR has been
calculated using the
expected DS cases (17.8)
rather than the observed 16
cases. Paper also presents
“expected” results where
selected 2nd T risk cut-offs to
yield DR of about 70%unclear how these
calculated (?statistical
modelling).
Verification
Outcome information from
Bureau of Vital Records and
2 diagnostic labs
responsible for most
karyotyping in the region
(AC, 1st yr of life and
products of conception).
Triple test (1:270)
67%(43-84), 6.4 (5.9-6.9)
Triple (1:190)
62%(39-81), 4.6(4.2-5.1)
Quad (1:150)
56%(33-76), 3.3%(2.9-3.7)
Serum integrated (1:100)
79%(55-92), 3.2%(2.8-3.6)
When FPR was revised using
only unaffected pregnancies
that remained screen positive
after confirming dates with
USS the FPR decreased from
3.2% to 3.0%.
Expected
Triple (1:190)
69%, 5
Quad (1:150)
69%, 3
Serum integrated (1:100)
73%, 2
Difficulties implementing any
of the screening strategies
Those with 2nd T risk ≥ 1:100
considered screen positive and
managed accordingly.
Calculated DS risk for each woman
using either quad or TT correcting
the total DS cases for “trimester of
ascertainment bias” due to some
affected pregnancies with
negative screen having fetal loss
and not diagnosed.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
PAPP-A analysed on stored serum.
No details of commercial kits or software used for
analysis of data.
There was some support from the screening
industry as PAPP-A reagents were provided by
Diagnostic Systems Laboratories.
Author’s conclusion
“Integrated serum screening for DS was
successfully implemented in primary care settings;
screening performance was consistent with
predictions”. It is an accessible and acceptable
alternative to screening methods that require NT
measurement.
111
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
(Knight et al. 2005)
To do this calculated the expected
number of cases on the basis of MA
distribution in the screened
population and published age
specific risks of DS (Hecht and Hook
1996, as published in this paper)
and used this as the denominator
for the DR (17.8 cases rather than
the 16 ascertained in the study).
Primary care
Maine, USA
Prospective cohort
study
Grade III-2
Continued
Sample
Outcomes and
verification
Results
Comments
Also contacted genetic
counselors to confirm
known cases and identify
missed cases. Primary care
also contacted
occasionally.
Samples from 2 trimesters were
correctly matched in 99.9% of
women (98% by the computer
and 139 with input of lab staff,
requiring 15-30 mins per day).
In 6 cases no match could be
made (multiple providers,
name changes, and
sometimes multiple 1st T
samples). The matching was
the most demanding aspect
of implementation. The
process was successful but
required extra work.
Reviewers’ conclusions
Some issues with the implementation of the
integrated approach-having to match specimens
taken in both trimesters.
However serum integrated performed better than
quad and TT having a higher DR and slightly lower
FPR.
Those with positive screen
advised to have invasive
screen.
Of 11,159 who agreed to
participate 78.6% submitted
both samples in the right
gestational range.
950 had 1st T MSS too early or
too late, 1436 where no 2nd T
MSS as (575 fetal loss, 459
declined, 236 elected AC
(mostly as over 35 years), 133
changed residence/provider,
29 ToP, 4 second sample too
late)
Also using 8 week as the lower
cut-off for having a 1st T MSS
was a problem as most (2/3)
didn’t have dates confirmed
at this time. PAPP-A had not
been validated before 8/40 so
had to just use 2 T screen.
Later more emphasis was
placed on dating but still had
9% of samples taken too early.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
112
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
Sample
Outcomes and
verification
Results
Comments
(Malone et al. 2005)
Comparing stepwise screening to
serum integrated and fully
integrated screening. Also
evaluated the performance of the
following screening methods: NT, 1st
T MSS (PAPP-A and fβhCG),
combined screening, quad test,
and a screening method
combining tests (combined and
quad) in an independent manner.
MA taken into account in all the risk
calculations.
Recruited from 15 centres in the USA.
Outcomes
The outcomes extracted for
this evidence table are the
directly observed DR and
FPR for combined screening
(1:150, and 1:300), quad
test (1:300) and screening
combining tests in an
independent manner
screening (1st T 1:50 and 2nd
T 1:300). These are given
with and without the
inclusion of cystic hygroma.
Accuracy of screening
methods
Limitations
Women with cystic hygroma were removed from
the analyses so the results apply to populations
without cystic hygroma. (Including cystic hygroma
increased the DR.)
1st T risks determined by NT, PAPP-A,
free β hCG, and MA at 10+3/4013+6/40. Returned at 15-18/40 for
2nd T screening. 2nd T risk calculated
from AFP, uE3, total hCG, and
inhibin A and MA. The 1st T results
were not released until 2nd T to allow
an unbiased comparison of the two
approaches.
Patients with cystic hygroma
followed separately (included for
some comparisons). 134 had cystic
hygromas (with 25 DS).
Age standardised
performance is also
presented based on the
MA specific risk DS at term
corrected to early mid
trimester to allow for fetal
loss from this time until birth,
and applied to the 1999
USS distribution of MA.
These results are given for
NT, 1st T MSS, combined test,
serum integrated, fully
integrated, TT, and quad
with all 1st T screening at
11/40.
Age standardised FPR (95% CI)
for 85% DR
NT
20 (10-26)
1st T MSS
16 (9.8-22)
Combined
3.8% (1.8-7)
Triple
14% (10-21)
Quad
7.3%(4.6-16)
Serum integrated
3.6% (2.0-7.7)
Fully integrated
0.6%(0.4-1.6)
First- and secondtrimester evaluation of
risk (FASTER) trial.
USA
Prospective cohort
study
Grade III-2
NT measurement performed
according to standard methods by
trained staff. A minimum of 20
minutes reserved for NT
measurement, and could return for
further attempt. TV USS
measurement used if required.
Quality control conducted.
MSS markers converted into MoM
for GA (CRL). Adjusted for maternal
weight and ethnicity.
NT MoM centre specific and
distribution of NT measurements
based on all NT measurement in the
population including those with
cystic hygroma.
Inclusion criteria: MA ≥ 16 years,
singleton live fetus, CRL 36-79
(10+3/40- 13+6/40) at recruitment.
42,367 approached.
4,178 ineligible or refused.
Exclusions: Prior measurement of NT,
or anencephaly (n=22).
38,033 enrolled. Maternal
characteristics: mean (± SD) MA at
EDD was 30.1 ± 5.8 yrs, ethnicity
66.9% “white” 22.6% Hispanic, 5.3%
Black, 4.1% Asian and 1% other.
GA at 1st T screening: 44.8% were
12+0/40-12+6/40, 22.6% were
11+0/40-11+6/40, 29.1 were 13+0/4013+6/40, and 3.5% were 10+3/4010+6/40.
Outcomes were available for 36,873
Spectrum of disease: 92/36,873 =
0.25%
Removed 7% of NT measurements as
failed or inadequate. Complete 1st T
data available in 36,120. Complete
data for 1st T and 2nd T available in
33,546 (i.e. all tests done).
Directly observed DR (95%CI),
FPR (95%CI)
Combined (1:150)
77%(69-86), 3.2% (3-3.4)
Combined (1:300)
82%(74-89), 5.6%(5.4-5.9)
Quad (1:300)
85% (76-93), 8.5%(8.2-8.8)
independent screening
94% (89-99),11% (10.7-11.3)
The differences between
screening were less
apparent when FPR fixed at
5% rather than 1% because
the DR of all screening is
relatively high.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Although the study was not directly supported by
the screening industry, some of the authors hold
patents for screening tests and
directorships/ownership of companies involved in
screening.
Author’s conclusion
Where there is appropriate quality control for NT,
combined screening is a powerful tool for
detection of DS. Stepwise screening and fully
integrated screening are both associated with
high DR and acceptable FPR; the advantage of
earlier diagnosis with stepwise screening must be
weighed against the lower FPR with integrated
screening. Consideration of the costs associated
with different strategies and patient preferences
will help guide the choice between these
approaches.
Reviewers’ conclusions
Well designed and high quality paper. Direct
comparison with 1st and 2nd trimesters is possible.
The results showed 1st T screening for DS is highly
effective and that combined screening at 11/40
better than quad.
113
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening
strategies
(Malone et al. 2005)
Risk estimated by multiplying the
MA specific risk (Morris et al. 2002-as
referenced in the paper) by LR
obtained by the Gaussian
distributions of affected and
unaffected pregnancies (as per
Wald and Hackshaw. 2,000-as
referenced in this paper).
Distribution using published
parameters (Wald et al. 1999 and
Wald et al. 2000 as referenced in
this paper).
First- and secondtrimester evaluation of
risk (FASTER) trial.
USA
Prospective cohort
study
Grade III-2
Continued
After all screening complete
women given two risks; with cut-off
of 1:150 risk at term for 1st T and
1:300 risk at term for 2nd T screening.
Offered counselling and invasive
test if either was positive.
2nd T screening (standard of care)
cut-off chosen so that the
estimated rate of positive screens
would be similar to the current
screening practice (5%), and the 1st
T cut-off so the over-all rate of
screen positives would not be
excessive.
95% CI for screening estimates were
determined by “bootstrapping”
with 1000 DS dataset replications.
Sample
Outcomes and
verification
Results
Comments
Verification
Medical records were
reviewed by one paediatric
geneticist in situations
where DS suspected, or in
those with positive screen
but no karyotyping, and in
a random sample of all
others.
Age standardised DR (95% CI)
for 5%FPR
NT
70%(65-79)
1st T MSS
70%(64-78)
Combined
87%(82-92)
Triple
69% (63-74)
Quad
81%(70-86)
Serum integrated
88%(81-92)
Fully integrated
96% (92-97)
Combinations of measurements of markers from
both 1st T and 2nd T (fully integrated and
stepwise) yield higher DR and lower FPR than
markers from a single trimester. Serum integrated
screening was similar to 1st T combined and may
be useful when staff trained in NT are not
available.
DS status ascertained by
AC, fetal cord sample in
those with positive screen
but declined AC, and or
tissue sampling in
spontaneous fetal loss ToP
or stillbirth.
Completeness of
ascertainment estimated
by the expected number of
DS at 2nd T from MA
distribution and recent age
specific birth prevalence.
112 would be expected 117
found (25 in the cystic
hygroma group plus 92).
The differences between
combined screening and
either NT or 1st T MSS are
significant.
Stepwise setting a 2.5% FPR for
each screening component
95% (91-97), FPR 4.9%
Difficulties implementing any
of the screening strategies
7% failed or suboptimal NT
measurements.
To compare different screening
methods the differences between
pairs of tests were determined for
each data set replication and CI
determined for this measure.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Stepwise had a similar DR to integrated but with
higher FPR. Independent screening had a high
FPR and should not be used.
114
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Hackshaw and Wald
2001)
Compared integrated screening and stepwise screening
to illustrate the effect of reporting a risk in women who
have already had 1st T screening without taking into
account that the distributions are based on populations
where everyone had both 1st T and 2nd T screen.
Statistical modelling
Sample
The authors were concerned about the screening practice
where women who have a positive screening in 1st T are
offered a CVS and those with a negative screen are then
offered a screen in 2nd T.
Two problems occur: Firstly if the1st T results are not
available or are ignored the standard calculation of risk for
2nd T screening will not be accurate. Second if the results
are combined with 1st T result to produce a risk estimate,
this still does not allow for the fact that these women were
screen negative based on another test and this will also
give inaccurate risk estimates. The paper examines this
issue.
The parameters for the Gaussian distribution of markers in
DS and unaffected pregnancies were obtained from
published prospective data. Those relating to NT were from
a large cohort (Nicolaides et al. 1998 as referenced in this
paper). 1st T PAPP-A and fβhCG were from SURUSS (77 DS
and 383 unaffected). 2nd T AFP, uE3, total hCG, fβhCG and
dimeric inhibin-A based on 77 DS and 980 unaffected
pregnancies (Wald et al. 1994, 1996b, 2000 as referenced in
this paper). Correlation coefficients between NT and 1st T
markers taken to be zero (Spencer et al. 1999). Correlation
coefficients between 1st T markers and 2nd T AFP, uE3, and
hCG also taken to be zero (Lam et al. 1998, de biasio et al.
2000).
No published data for the correlation between 1st T
markers and 2nd T inhibin-A. As the correlations between
the others are very small it is likely to also be the case for
inhibin, and even if there were a small correlation unlikely to
have a big effect on the modelling.
Outcomes and
verification
Results
Comments
Outcomes
The overall DR and FPR
were estimated using
the 1st T and 2nd T
combined results with
revised MA specific risk
curves and revised
marker distributions.
Results of screening
across trimesters
combined in stepwise
manner-anyone screen
negative has 2nd
trimester screen and risk
at 2nd T takes 1st
trimester into account.
Accuracy of screening
methods
Limitations
Like all models makes assumptions that
may not be applicable in the real-world
e.g. that all who are screen positive are
offered and accept IT.
These were compared
to integrated test with a
cut-off chosen to yield
the same DR as the
stepwise approach. The
modelled integrated
test uses hCG in both
trimesters so it is the
same as in the stepwise
method.
The maternal age
specific risk curves
showed that the age
specific risks in those
who have had a
previous negative 1st T
screen were lower than
those who have not
been screened, as most
DS will have been
detected in 1st T.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Stepwise DR, FPR (cut-off set at
5%FPR 2nd step) and
integrated FPR for same DR.
NT (risk 1:350), double
Stepwise manner
88%, 9.9%
Integrated manner
88%, 6.4%
NT (risk 1:350), TT
Stepwise
91%, 9.9%
integrated
91%, 6.7%
NT (risk 1:350), Quad
Stepwise manner
93%, 9.9%
Integrated
93%, 6.0%
Combined (risk 1:400), Double
Stepwise manner
92%, 9.2%
integrated
92%, 6.1%
Combined (risk 1:400), TT
Stepwise manner
94%, 9.2%
Integrated
94%, 5.8%
Author’s conclusion
If women who are screen positive in the
1st T are offered IT while those who are
negative have 2nd T screening, the MA
specific risk and marker distributions used
to estimate risk in those who are screen
negative would need to be revised.
If the 1st T test result is not available or not
combined with the 2nd T result
(independent screening) there is a greater
chance of FPR.
If the markers are combined but the
revised MA specific risks and the revised
distributions are not taken into account
the risk will be too low and may reduce
the DR. This is because the distribution of
markers in screen negative women who
have DS fetuses will be closer to that of
affected pregnancies.
115
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Hackshaw and Wald
2001)
Estimated the correlation between two fβhCG samples
(unaffected and affected) from the correlation when
samples taken a few weeks apart in unaffected women,
and distribution of fβhCG across 2 trimesters. Same done for
correlation between 1st T fβhCG and 2nd T total βhCG.
Statistical modelling
Sample
Continued
Using the age distribution of England and Wales 1996-1998
and applying the MA related risk of DS at term (Cuckle et
al. 1987-as referenced in this paper), a hypothetical group
of 100,000 affected and 100,000 unaffected pregnancies
was produced using a Monte Carlo simulation. From this
was generated MoM for marker levels in unaffected and
affected pregnancies.
Outcomes and
verification
Results
Comments
The distribution of some
of the markers changed
for women who are
screen negative
compared to women
who are yet to be
screened.
1st T combined (risk 1:400),
Quad
Conventional Stepwise
screening
95%, 9.2%
integrated
88%, 4.4%
Similar problems when those having a
positive 1st T risk are then offered a 2nd T
screen to “double check” if they need an
invasive test.
This means that the risk
estimate will be wrong if
these are not taken into
account.
To determine the effect of 2nd T screening in women who
were previously screen negative had to firstly estimate:
The MA specific risk of having a DS birth in those who were
screen negative after 1st T screening.
The distribution of the markers (median, SD and correlation
coefficients of 1st T and 2nd T markers in affected and
unaffected women who were screen negative after 1st T,
and compared to those who had not been screened
before.
The risk of having a DS pregnancy in those who had
previously been screen negative in 1st T was illustrated
using women having the 2nd T triple test. Risks were
estimated based on: the assumption that women had not
been screened before in the same pregnancy; by
combining the 1st T and 2nd T markers with MA using the
inappropriate age specific risk curve; and also combining
the 1st T and 2nd T and MA and the revised (appropriate)
MA specific risk curve and revised marker distributions.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers’ conclusions
Even when use the correct MA distribution
and correct marker distribution stepwise
has a higher FPR than integrated.
116
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
(Lam et al. 2002)
Compared screening with NT to 2nd T double test and
integrated screening.
Modelling was based on
data from obstetric
clinics of 5 hospitals in
Hong-Kong, China.
Outcomes
Compared estimates of
DR and FPR obtained
from modeling for NT
alone (without MA), NT
and MA, double test,
and a screening
method which
integrated the results of
NT and double test and
only disclosed them
after all results were
available.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Removed those with other chromosomal
disorders-changes the spectrum of
disease and may reduce FPR compared
to studies where these are considered
“unaffected”.
Verification
Pregnancy outcome
from hospital records or
direct contact with
women after delivery.
Difficulties implementing any
of the screening strategies
For 0.22% (39/17590) could not
measure NT successfully.
Statistical modelling
Non-intervention trial. All in the analysis had both 1st T and
2nd T screening.
NT measured at 10-14/40 with TA USS (98.6%) or TV USS.
Measured using methods as per FMF by staff who had
undergone NT training. Regular audit carried out. The NT
measurements from the 2 best images were averaged. GA
by CRL at or before 13/40 or BPD at 13-14/40.
NT converted to MoM for the gestational day. NT not acted
upon unless USS showed gross features of hydrops fetalis.
Neither women nor obstetricians told of the results.
All had 2nd T MSS (hCG and AFP =double test) between 1520/40. DS risk from MSS disclosed and women with risk 1:250
or more offered invasive diagnostic test.
Women >35 yrs old or with other risk factors given the
option of CVS at 10-12/40 or AC at 15-20/40 but MSS still
taken few weeks after CVS or just before AC.
All markers expressed as MoM at given GA. AFP and hCG
adjusted for maternal weight using commercial software.
The DR and FPR of the screening methods were obtained
by the model based LR approach described by Royston
and Thompson, 1992 (as referenced in this paper).
Specifically all markers were logarithmically transformed
and multivariate Gaussian distribution fitted for affected
and unaffected pregnancies. Used MA distribution of Hong
Kong in 1994 and the age specific risks of DS to estimate DR
and FPR particular risk cut-offs.
95% CI obtained by parametric bootstrapping (n= 300).
Those attending clinics
at or before 14/40 who
agreed to DS screening
were recruited. NT was
measured for research
only and results were
not disclosed to women
or clinicians.
17,590 recruited January
1997-August 2000.
Removed 208 with other
chromosomal disorders
or major abnormalities.
Removed 39 where NT
measurement was
unsuccessful. Also
removed 1015 who
defaulted from 2nd T
MSS, and 91 who
miscarried between NT
and 2nd T MSS.
16237 left for analysis:
mean GA at USS 87
days, and at 2nd T
screening 16/40. Mean
MA unaffected =30.5yrs
(19% were ≥ 35 years).
Pregnancy outcome
ascertained in 15253.
Review of cytogenetic
labs performing
karyotyping for all 5
hospitals.
Of the 16237 in the
analysis 117 had CVS
(none had DS), and
1913 had AC.
Looked at estimated
number of DS at 2nd T
based on MA
distribution-about 38
similar to that found of
35.
Spectrum of disease:
35DS/15253 = 0.23%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
DR (95%CI) for fixed FPR 5%
NT alone
60.8 (41.7-69.4)
NT
69.3% (56-76.1)
Double test
73.2% (63.4-82.9)
Integration of NT and double
85.7% (76.2-92.1)
5.8% defaulted from 2nd T
screen (1015/17590).
Removed those not having 2nd T
screening. However, NT results weren’t
disclosed so should not have removed
women with large NT (and therefore cases
of DS) except hydrops fetalis, and possibly
any women who had CVS without MSS.
DS were ascertained at or beyond 2nd T so
hard to compare NT performance to other
studies that ascertained DS with NT
screening in 1st T. (Some of these would
have miscarried anyway).
NT non-interventional may not have cared
about precision as opposed to relying on
it clinically.
Unclear which population parameters
used for statistical modeling-presumably
from the prospective cohort study
Author’s conclusion
Despite the use of the double test 2nd T
MSS had a higher DR than NT. The
integration of NT and 2nd T MSS yielded the
best screening efficacy DS.
Reviewers’ conclusions
Non-interventional study so reasonably
valid comparison between 1st T and 2nd T
screening. Double test performed better
than NT but the integration of the two had
the best performance.
117
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
(Rahim et al. 2002)
The study aimed to determine the performance of a
compromise policy where women who were most likely to
have errors received a dating scan rather than all women
having a dating scan. Screening with two markers (fβhCG,
AFP) compared to 3 markers (uE3) for policies where all had
USS for dating, or restricted to those with uncertain dates or
dates unrecorded.
Study based on 14, 274
women with unaffected
singleton pregnancies
screened by LASS
January 1997-July 2001.
Outcomes
The outcomes were for
2 markers compared to
3 markers for different
policies for dating;
either using dates only,
using scan unless dates
reliable, or scanning all
women.
Accuracy of screening
methods
Limitations
Unclear when serum markers taken so
difficult to reproduce results or to classify
the screening methods as 2nd T or 1st T
screening. The aim of the study was not to
determine accurate DR and FPR for
different screening combinations but to
determine the best policy for dating.
Statistical modelling
All had MSS at 13-21 weeks: fβhCG, AFP, and uE3
(PerkinElmer). Some also had inhibin-A, NT and PAPP-A but
these markers were not used in the model.
For each woman marker MoM were calculated based on
USS and LMP. Serum markers adjusted for maternal weight
where available. Normal medians were those used
routinely by Leeds Antenatal Screening Service (LASS).
Standard statistical modeling used to predict DR for a fixed
5%FPR for different screening methods. Parameters for
unaffected from study data (correlation coefficients after
removal of outliers). DS parameters from unaffected
parameters with addition of meta-analysis values (Cuckle,
1995 as referenced in this paper).
Both LMP and USS
dating available for
12711, no LMP on form
for 1404, and no USS
information in 162. Of
those with LMP
available, 1693 listed as
uncertain, 547 pill
withdrawal periods,
1565 irregular cycles,
and 296 regular cycles
but abnormal length
(these were all classified
as unreliable).
Presumably markers
were across trimesters.
MA distribution was that
for England and Wales
1994-1998.
Verification
No details
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Dates only, DR for 5% FPR
fβhCG and AFP
57.6%
fβhCG, AFP, uE3
59.3%
Scan unless dates reliable, DR
for 5% FPR
fβhCG and AFP
61.1%
fβhCG, AFP, uE3
64.7%
Scan all women, DR for 5% FPR
fβhCG and AFP
63.2%
fβhCG, AFP, uE3
67.9%
Author’s conclusion
The study confirms that a policy of
universal scanning for dating increases the
DR and reduces the FPR compared with
using LMP. In this study over half of these
benefits could be achieved by restricting
USS dating to the 1/3 of women with
unreliable dates.
Reviewers’ conclusions
A combination of 3 markers (presumably
across trimesters) was better than using
only 2 markers. Unclear which markers
taken when or if some markers taken
across two trimesters (e.g. fβhCG).
118
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Cuckle 2003)
The aim of the paper was to update the parameters for DS
screening markers, specifically inhibin in 2nd T, combining 1st T
PAPP-A with 2nd T markers, and 1st T NT and 2nd T nuchal skinfold (NF) thickness (outside the scope of this review).
Statistical modelling.
Sample
All markers were expressed as MoM (GA specific) of
unaffected pregnancies and log transformed.
Used meta-analysis of published studies to derive the DS mean
and the differences in variance and covariance between
affected and unaffected pregnancies.
Except for NT only data from non-interventional studies were
used. Used 11 studies for NT, including 5 interventional studies.
Adjusted for this bias.
Outcomes and
verification
Results
Comments
Outcomes
The outcomes extracted
are the DR for 5% FPR and
DR and FPR (1:250) for NT,
combined, combined
plus 1st T uE3 and AFP, TT,
quad, and what appears
to be serum integrated
and fully integrated
methods.
Accuracy of screening methods
Limitations
Little information on correlation between 1st
T PAPP-A and 2nd T markers. More data
needed to calculate covariances for inhibin
and PAPP-A.
Paper presented results
for various fixed FPR, fixed
DR, and cut-offs for a
number of marker
combinations.
Other parameters from existing meta-analyses except for
mean for fβhCG across the 1st T when GA specific values were
regressed. The unaffected variance and covariance in
unaffected pregnancies from 29,516 women screened in
Leeds. The SD estimated from the Gaussian distribution and
covariance estimated after exclusion of outliers.
Results for β hCG better
than with total HCG for
both quad and triple testthe fβhCG results have
been extracted.
The existing and updated parameters were then used to
predict performance of screening policies using the numerical
integration method as described by Royston and Thompson,
1992-as referenced in this paper. The MA specific risk was from
Cuckle et al. 1987-as referenced in this paper, and the MA
distribution was taken to be Gaussian with mean MA 27yrs,
and SD 5.5 yrs.
For all the combinations,
the results were better
when the 1st T markers
were measured at 10/40
compared to 13/40-the
10/40 results have been
extracted.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
DR, FPR (1:250 cut-off)
NT (11-13/40)
70.6%, 2.4%
Combined
81.6%, 2.0%
Combined plus uE3 & AFP
84.0%, 1.8%
TT
65.1%, 4.7%
Quad
69.2%, 4.1%
1st T PAPP-A combined with
quad (?integrated or stepwise)
76.1%, 3.2%
1st T PAPP-A and NT combined
with quad (?integrated or
stepwise)
88.1%, 1.5%
DR for 5%FPR
NT (11-13/40)
76.1%
Combined
87.8%
Combined plus uE3 & AFP
90.5%
TT
66.1%
Quad
71.7%
1st T PAPP-A combined with
quad (?integrated or stepwise)
80.6%
1st T PAPP-A and NT combined
with quad (?integrated or
stepwise)
93.5%
Unclear whether results combining 1st and
2nd T screening relate to the disclosure or
non-disclosure method. Presume they were
combined in an integrated manner.
Author’s conclusion
The existing and updated meta-analysis
parameters are used to predict screening
performance for the related policies yielding
a DR for a 5% false-positive as high as 9093%.
Since multi marker serum screening for DS
was first introduced there has been a steady
increase in DR in relatively small increments
as new markers have been added. The
incorporation of USS markers has continued
and accelerated the process.
Reviewer’s conclusions
The results indicated that adding inhibin to
2nd T TT increased DR, that NT at 11-13/40
had better DR than any 2nd T serum
screening, and that combined test better
than NT. Adding 1st T uE3 and AFP to
combined test did not improve screening by
much.
Combining results of screening across
trimesters was better than any method
alone-presume this was the serum
integrated and fully integrated screening
method.
119
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
(Rode et al. 2003)
Compared screening using different combinations of 1st T
and 2nd T markers, including a new marker, the proform of
eosinophil major basic protein (proMBP).
Used 6,741 women from
the Copenhagen First
Trimester Study
(Wojdemann et al. 2001
as referenced in this
paper) who gave birth
prior to 1st April 2001
who all had NT 10-13/40.
Outcomes
The DR for a fixed 5%
SPR was extracted for 1st
T MSS, combined test,
conventional TT, TT with
ProMPB instead of uE3,
conventional quad,
quad using ProMBP
instead of inhibin,
integrated method, and
a method using 1st
βhCG, & NT and 2nd T
AFP & ProMBP.
Accuracy of screening
methods DR (95%CI), FPR
(95%CI)
Limitations
Data from interventional study. Sample of
195 women biased. Only 1/195 had
positive NT screen i.e. these were women
who had negative NT screen then 2nd T
serum screen-those with large NT would
have not continued screening.
Statistical modelling
Monte Carlo
simulation
The aim of the study was to investigate the distribution of
and correlation between1st and 2nd T serum markers and NT
in normal pregnancies and use these findings in
combination with published information on the distribution
of markers in DS pregnancies to assess the performance of
different screening strategies.
NT measured according to FMF. Those with risk > 1:250
based on NT and MA were offered invasive screen. One of
the 195 had positive screen.
PAPP-A determined using a manual ELISA. fβhCG
determined using commercial kit (AutoDelfia ™, EG&G, Life
Sciences). 2nd serum (AFP, hCG and uE3) analysed using
commercial kit (AutoDelfia ™, EG&G, Life Sciences).
These all done prospectively.
Of the 195 blood samples only 166 could be retrieved for
proMBP and inhibin analysis. Total proMBP using ELISA
developed by Statens Serum Institut Copenhagen. Inhibin
using an Inhibin-A Dimer Assay Kit (Oxford Bio-Innovation).
195 had both 1st T
(10+5/40-13+6/40) and
2nd T (14/40-20+2/40)
samples taken in same
pregnancy.
Singleton, live birth
outcomes, with no
malformations.
Only SPR was available.
This will be a good proxy
for the FPR in this
modelled population.
Median MA 32.2 yrs
(range-20.3-40).
Markers converted to GA (CRL) MoM. The correlation
between markers and regression analysis performed using
MoM. The distributions of MoM values determined for GA
intervals.
Monte Carlo simulation using S-Plus based software
(validated by Larsen et al. 1998-as referenced in this paper)
a standard distribution of MA (Van der Veen et al. 1997 as
referenced in this paper) and published information on
marker distribution in DS pregnancies (Cuckle and van Lith,
1999, and Wald et al. 1994;1996, as referenced in this
paper).
ProMBP distributions established in 16 DS samples obtained
from routine serum samples from Statens Serum Institute.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
DR for a fixed 5% screen
positive
1st T PAPP-A and fβhCG
56%
Combined test (β hCG)
76%
TT (hCG)
61%
2nd T AFP, hCG, and ProMBP
(instead of uE3)
79%
Quad (hCG)
69%
2nd T AFP, hCG, uE3, and
ProMBP (instead of inhibin)
83%
Integrated
86%
1st T βhCG, NT & 2nd T AFP &
ProMBP
90%
PAPP-A using a manual ELISA, and ProMBP
using an in-house ELISA. ProMBP and
inhibin-A on retrieved samples which had
been stored at -20C.
Very small sample used for the
parameters in unaffected pregnancies195 and only 166 had all tests.
ProMBP distributions established in 16 DS
obtained from routine serum samples from
Statens Serum Institute.
Used the correlation coefficients from
normal pregnancies in the DS matrices in
calculations. This was done as an increase
in correlation coefficients (up to 4 fold
trialled) did not change the estimated
performance of a given marker
combination , fix common position and
because data on correlation coefficient
between 1st T and 2nd T markers in DS
pregnancies are not yet available.
Authors’ conclusion
These results suggest that proMBP may be
an important new marker in DS screening
and, in particular, a good substitute for
inhibin A.
Reviewers’ conclusions
Needs further analysis with larger samples
for the parameters especially of proMBP.
120
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Wright and Bradbury
2005)
Compared combined test, quad test, serum integrated and
fully integrated screening to screening using highly
correlated repeated measures of serum markers taken in the
1st T and 2nd T of pregnancy.
Statistical Modelling
Sample
Estimates of means, SD, correlations of log MoM from SURUSS
(47,053 pregnancies and 101 cases DS).
MoM are estimated from USS dating and are corrected for
maternal weight.
MA related risk of DS- from published data (Wright and Bray,
2000-as referenced in this paper)
DR and FPR estimated for the maternal age distribution of
England and Wales 1996-1998 using Monte Carlo simulation
to sample 500,000 observations from the distribution of MoM
in DS and unaffected.
LR calculated for each observation and used to estimate
the DR and FPR for each MA.
Overall DR obtained by combining MA specific rates with
MA distribution.
Apart from the model for MA related risk of DS the
assumptions are the same as the MA risk model used in
SURUSS. The DR and FPR are identical to those in SURUSS (to
the number of decimal places presented).
Outcomes and
verification
Results
Comments
Outcomes
Outcomes were the FPR
for 85% DR for combined
test, quad test, serum
integrated and fully
integrated screening,
and screening using
highly correlated
repeated measures of
serum markers taken in
the 1st T and 2nd T.
Accuracy of screening
methods
Limitations.
The modeling makes assumptions based
on small sample of DS cases.
The notation ^2 means a
measure was taken in 1st
T then again in 2nd T.
The results presented are
for repeat measures of
PAPP-A, repeat
measures of PAPP-A and
uE3, repeat measures of
PAPP-A and total hCG,
repeat measures of
PAPP-A, uE3, and inhibin.
Results are also given
with the inclusion of 1st T
NT for some of these
screening methods.
Repeat measures of
other analytes are
available from the
paper, but those
presented had the best
screening performance.
In the repeat measures it
is assumed that
screening takes place at
10/40 for 1st T samples.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
FPR for 85% DR
Combined (βhCG)
6.1%
Quad (hCG)
6.2%
Serum integrated test
2.7%
Integrated test
1.2%
PAPP-A^2
2.3
PAPP-A^2, uE3^2
0.5%
PAPP-A^2, uE3^2 & NT
0.3%
PAPP-A^2, & total hCG^2
1.1%
PAPP-A^2, total hCG^2 & NT
0.6%
PAPP-A^2, uE3^2, & inhibin^2
0.3%
(The notation ^2 means a
measure was taken in 1st T
then again in 2nd T)
Authors also state that SURUSS parameters
affected by viability bias because of
intervention in the T2 (will optimistically bias
performance). However no studies are
observational as this would be unethicalneed to compare performance at 2nd T.
The modelled generated “implausible riskestimates” when using repeat measures in
several highly correlated markers (Wald
2006). To overcome this issue Wald et al.
used ratio of the marker levels in 1st T and
2nd T which they called the cross trimester
(CT) ratio.
Author’s conclusion
Certain combinations of highly correlated
markers (some of which have poor
discriminatory power individually) have
benefits over the established integrated
test. Would be good in situations where NT
not available. Drawback (as for the
integrated) is that all need repeat testing
in 2nd T.
The performance of repeated measures
screening tests, and acceptability should
be assessed in further prospective studies.
Reviewers’ conclusions
While there are some issues with the
methods used, repeat measures could be
an additional marker which could
potentially improve screening
performance.
121
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Benn et al. 2005a)
Compared contingent and integrated methods of
screening with different timings of markers, using fβhCG or
total hCG, and different risk cut-offs according to the
practice in the UK and USA.
Statistical Modelling
Sample
The aim of the study was to assess performance of different
protocols for contingent screening for DS. Modelled to
predict performance for programmes most likely to be
adopted in the UK and USA.
Statistical modelling applied to the parameters in the SURUSS
study. Multivariate Gaussian model used for distributions of
marker profiles for DS and unaffected pregnancies.
All markers expressed as the GA specific MoM of unaffected
pregnancies. The marker’s means, SD, and correlation
coefficients were obtained from SURUSS (based on
pregnancies expected to be viable 2nd T).
MA related chance of DS at term from the literature (Wright
and Bray, 2000 as referenced in this paper). Risk at 2nd T
calculated by allowing for 23% fetal loss between 2nd T and
term (Cuckle 1999 as referenced in this paper). MA
distribution from national statistics of England and Wales
2001 or USA 2000.
DR and FPR estimated using Monte Carlo simulation to
sample 500,000 observations from the modelled distributions.
LR ratios were calculated for each observation to derive MA
specific rates. Also calculated the early DR and FPR for those
with high risk in T1.
Outcomes
Results
Comments
Outcomes
Outcomes were the DR
and FPR for UK policies
for risk cut-offs at term
for UK and at 2nd T for
USA.
Accuracy of screening
methods DR, FPR
Limitations
Modelling as opposed to directly observed
DR and FPR although the method used has
been validated.
For the UK screening 1 T
MSS (fβhCG) taken at
10/40, NT 11/40, and 2nd
T serum 14-20/40. For the
USA contingent
screening 1st T serum
(total hCG) and NT
12/40, and 2nd T MSS 1420/40. For integrated
test, PAPP-A 10/40 & NT
at 11/40. (These timings
produced the best
results.)
st
For contingent method
the cut-offs for high and
low risk groups were for
the UK very high cut-off
1:20, very low cut-off
1:2000, (early DR, FPR =
62.5%, 0.3%); and for the
USA very high cut-off
1:30, very low cut-off
1:1300, (early DR, FPR =
61.7%, 0.6%).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
UK policies (DR, FPR)
Combined (1:250)
85.8%, 3.8%
Double (1:250)
77.8%, 7.8%
TT (1:250)
79.8%, 7.2%
Quad (1:250)
83.8%, 5.4%
Contingent screening (overall
risk 1:250)
91.4%, 2.1%
Contingent screening (overall
risk 1:100)
88.2%, 1.1%
Integrated test combined in
contingent manner (overall risk
1:250)
91.9%, 2.2%
Integrated test combined in
contingent manner (overall risk
1:100)
88%, 1.0%
Integrated test-non disclosure
(overall risk 1:250)
92.1%, 2.2%
Integrated test-non disclosure
(overall risk 1:100)
88.3%, 1.0%
Author’s conclusion
With appropriate patient counselling it
should be possible to provide highly
effective DS screening using contingent
protocols.
Reviewers’ conclusions
Contingent screening can provide most
patients with early reassurance or diagnosis
while providing additional testing for those
who will most benefit. Our model based on
the proposed protocols indicates this
strategy can be highly effective. For both
UK and USA policies over 60% of DS
detected in 1st T and less than 20% require
2nd T screening.
122
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Benn et al. 2005a)
Compared contingent and integrated methods of
screening The contingent screening used 2 serum markers as
opposed to just PAPP-A for integrate. This was to ensure that
women who decided to just have 1st T screening had best
available marker combinations. A four marker combination
was chosen for 2nd T screening for those who attended too
late for 1st T screening.
Statistical Modelling
Continued
Sample
Outcomes
Results
Results for other timings
and combinations of
markers are presented in
paper.
USA policies
Combined (1:270)
83.6%, 5.3%
TT (1:270)
81.7%, 8.3%
Quad (1:270)
84.6%, 6.7%
Contingent screening (overall
risk 1:270)
89.1%, 3.1%
Contingent screening (overall
risk 1:130)
86.2%, 1.9%
Integrated test combined in
contingent manner (overall risk
1:270)
90.5%, 3.4%
Integrated test combined in
contingent manner (overall risk
1:130)
86.8%, 1.8%
Integrated test-non disclosure
(overall risk 1:270)
90.7%, 3.4%
Integrated test-non disclosure
(overall risk 1:130)
87.0%, 1.8%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
123
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Cuckle et al. 2005)
The study compared the estimated performance of 17 DS
screenings strategies: 3 in 1st T, 6 in 2nd T, and 8 integrated
or sequential policies- 6 are not in use but are proposed or
trials underway and 2 used by default (combining results in
an independent manner).
Statistical modelling
Sample
1st T: NT at 11-13/40, combined test with PAPP-A and fβhCG
at 10-13/40, or hCG at 12-13/40. 2nd T: double test (with
either βhCG or total hCG) TT (with βhCG or total hCG),
quad test (with βhCG or with hCG).
The eight policies combining 1st T and 2nd T markers were:
Serum integrated screening
Fully integrated
step-wise (either fβhCG or total hCG in 1st T and either
fβhCG or total hCG in 2nd T)
screening combining tests in an independent manner (as
for step wise)
Contingent (using either fβhCG or hCG in 1st T and 2nd T)
All marker levels converted to MoM for GA. The risk was
estimated by combining the MA specific risk with LR for
marker profiles derived from the Gaussian distribution of DS
and unaffected pregnancies.
The distribution of risk was estimated by statistical modelling
as per Royston and Thompson, 1992 (as referenced in this
paper). The maternal age specific risk was from Cuckle et
al. 1987 (as referenced in this paper) and the maternal age
distribution was considered Gaussian with a mean of 27yrs
and a SD of 5.5 years. The risks for extreme marker values
were calculated after truncation as per Wald et al. (Wald
et al. 2003b)
Parameters for 2nd T obtained from two meta-analyses of
non–interventional studies. For AFP, uE3, hCG and βhCG this
was Cuckle, 1995 (as referenced in this paper) and for
inhibin this was Cuckle (Cuckle 2003)
Outcomes and
verification
Results
Comments
Outcomes
For this table the
comparisons were NT,
combined screening
with fβhCG or hCG,
double test with fβhCG
or hCG, TT with fβhCG or
hCG, quad test with
fβhCG or hCG, serum
integrated, fully
integrated, stepwise
with fβhCG or hCG for
1st T, independent with
fβhCG or hCG for 1st T,
and contingent
screening with fβhCG or
hCG for 1st T. The results
were the DR for a fixed
FPR.
Accuracy of screening
methods DR for 5% FPR
Limitations
Not a lot of information on between
trimester correlations in DS pregnanciesthese parameters will need to be
updated.
The performance is
reported with 1st T
serum and NT at 10/40
and 11/40 unless hCG
used when serum and
NT at 12 and 13/40.
For the stepwise policies
(where applicable) the
proportion of tests
considered positive
after 1st T screen set at
70%, and for contingent
screen the proportion
having 2nd T screening
set at 15%.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
NT 11/40
78%
Combined (fβhCG)-MSS 10/40,
NT 11/40
87%
Combined (hCG)-MSS & NT
12/40
83%
Double (fβhCG)
61%
Double(hCG)
56%
TT (fβhCG)
65%
TT (hCG)
60%
Quad (fβhCG)
71%
Quad (hCG)
67%
Serum Integrated
78%
Fully integrated
93%
Stepwise (1st T fβhCG)
95%
Stepwise (1st T hCG)
90%
Independent (1st T fβhCG)
86%
Independent (1st T hCG)
86%
Contingent (1st T fβhCG)
94%
Author’s conclusion
Modelling with meta-analysis derived
parameters provides a reliable guide for
policy and favours contingent screening
policy. The widespread use of calculate in
1st T and 2 T risks separately should be
abandoned.
Reviewers’ conclusions
High quality validated modeling using
parameters from large studies. Metaanalysis of non intervention or adjustment
for viability bias. Lots of detail about the
methods used.
The results were better for strategies using
fβhCG compared to total hCG in both
trimesters.
Combined screening was better than NT,
and both were better than all 2nd T
screening methods.
All integrated and sequential screening
was clearly better than screening in 1
trimester, except serum integrated which
has a similar performance to NT and was
inferior to combined, and independent
screening.
124
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Cuckle et al. 2005)
GA mostly based on USS.
Statistical modelling
1st T PAPP-A and fβhCG parameters from a published
meta-analysis of non-interventional studies (Cuckle and van
Lith, 1999 as referenced in this paper), extended to include
the gestational specific DS means from a more recent
meta-analysis (Spencer et al. 2002) as referenced in this
paper and in a large single study (Wald et al. 2003b)
Continued
Sample
Outcomes and
verification
The means at 10, 11, 12, and 13 /40 derived from the
weighted average from these 3 sources subjected to
regression.
About half of the data in the recent meta-analysis from
interventional studies using NT, PAPP-A, and fβhCG so
viability bias. Possibly this would mean a 1.5% reduction in
the mean PAPP-A level and a 1% increase in the mean
fβhCG and so to allow for bias authors adjusted the means
by these proportions.
Mean serum hCG at 12 and 13/40 from the weighted
average of data in the two recent studies (Spencer et al.
2002 as referenced in this paper and SURUSS) as were other
hCG parameters.
NT means for DS at 11, 12 and 13 weeks from a new metaanalysis of nine studies as referenced in this paper. Four
were intervention studies so subject to intervention bias and
one biased referral of women with increased NT.
FASTER biased as removed cystic hygroma. The results of
the 3 interventional studies adjusted for viability bias.
NT SD from 4 large prospective studies combined (Spencer
et al. 2003 as referenced in this paper).
Between trimester correlation coefficients from a new
meta-analysis from 5 studies as referenced in this paper.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Results
Comments
Contingent (1st T hCG)
88%
Stepwise screening using fβhCG in
combined test has best performance
(95%) based on DR and FPR followed by
contingent (94%) using fβhCG in
combined test and then fully integrated
(93%). Contingent has high DR with only
15% having 2nd T screening.
125
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
Sample
Outcomes and
verification
Results
Comments
(Maymon et al. 2005)
The aim of the study was to describe a method for deciding
whether an individual's 1st T DS screening test result justifies
further testing in the second trimester.
The illustrative sample:
Outcome
The modeled DRs and
FPRs for stepwise and
contingent screening
are presented.
Accuracy of screening
methods
Limitations
The illustrative sample size was small and
biased but this was only used to confirm
the probability of a positive 2nd T test
given the 1st T test results.
Statistical Modelling
For each 1st T test result the model estimated the
probability that the final results would be positive, and it
also generated 2 cut-off probabilities, above one where
women would be offered invasive screen, and below the
other women would be counselled that no further
screening would be needed.
The markers compared were 1st T fβhCG and PAPP-A and
2nd T quad (intact hCG).
Statistical modelling was used to estimate the distribution of
second-trimester marker profiles for a given first-trimester
profile and hence the probability of a final positive result,
using a 1:250 risk at term cut-off.
The Gaussian distributions were constructed for unaffected
and DS pregnancies for 1st T and 2nd T markers.
For a given profile of one marker the associated profile of
2nd T markers was determined. Using numerical integration
(Royston and thompson,1992). The probability of a positive
final result was determined given the MA and the first
trimester profile.
24 DS samples from
women referred to a
Medical Centre, in Israel
for late ToP. All had
been screened with NT
at 11-13/40 and 2nd T TT
and all had AC. Some
also had 1st T MSS
(PAPP-A and fβhCG)
and others were tested
retrospectively from
stored serum.
367 unaffected
singletons. Samples
collected from those
having sequential
screening at same
centre. All had been
screened with NT at 1113/40 1st T MSS (PAPP-A
and fβhCG) and TT and
all had AC.
For stepwise screening
all those with a ≥ 50%
chance final positive
have diagnostic test.
For contingent
screening all those with
≥ 50% chance final
positive have diagnostic
test, and below 3% no
further screen.
Verification
From phoning parents
and delivery medical
records.
The parameters used for DS and unaffected were from
SURUSS. GA from USS (CRL) and markers were weight
corrected. 1st T serum taken at 10/40, 2nd T serum at 1422/40 and NT measured at 11/40.
MA risk based on Cuckle et al. 1987 (as referenced in this
paper) and MA distribution taken as Gaussian with mean 27
yrs and SD of 5.5 yrs.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
DR, FPR
Step-wise
90%, 1.7%
Contingent
88% 1.4%
Difficulties implementing any
of the screening strategies
None noted
Author’s conclusion
Predicting the probability of a positive
final result from the first-trimester marker
profile has potential utility, either as a
decision aide for individual women or as a
formal part of screening policy in selecting
a subset of women for second-trimester
testing.
Reviewers’ conclusions
While this was not the aim of the study the
paper did have results for stepwise
screening versus contingent screeningstepwise screening had a marginally
higher DR and a slightly higher FPR
compared to contingent screening.
126
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Maymon et al. 2005)
A multi-variate log Gaussian model was used with
published parameters.
Sample
Outcomes and
verification
Statistical Modelling
Continued
To illustrate the method, the model was applied to a
published series of 24 DS and 367 unaffected pregnancies
to confirm the probability of a positive screen given first
trimester markers.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Results
Comments
127
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Benn and
Donnenfeld 2005)
The study compared combined test, quad test, and
stepwise screening using a strategy that takes into
consideration correlation between tests and one that
doesn’t.
Statistical modelling
Sample
If both trimester results considered independent then the a
priori risk at 2nd T is the LR from the 1st T, and the LRs are
multiplied together. Not all tests are fully independent so it is
important to take the correlation between markers into
account when calculating the LR.
Few labs have flexible software which have the capacity to
combine 1st T and 2nd T screening results into a
multivariable screening algorithm so it has been suggested
(Malone 2005 as referenced in this paper) that risks could
be provided based on the approximation that tests are
independent of each other.
Outcomes and
verification
Results
Comments
Outcomes
The DR and FPR have
been modelled for 1st T
combined screening,
2nd T quad test (with
total βhCG), and
stepwise strategy with
and without this
multivariate algorithm
(LRM).
Accuracy of screening
methods DR, FPR
Limitations
The paper states that more robust
estimates of DR and FPR based on the
simulation of larger numbers of cases with
additional test combinations are available
elsewhere.(Benn and Donnenfeld 2005).
1st T combined
83.7%, 5.1%
2nd T quad (with total βhCG)
84.4%, 6.6%
Stepwise (LRM)
90.8%, 3.1%
Risk cut-off was 1:270.
Model used the MA
distribution of the USA
for 2000.
The aim of this study is to compare this approach (LR1st T X
LR2nd T) with the approach that uses an algorithm that
takes the correlations into consideration (LRM).
Statistical parameters from SURUSS. Screening at 12/40 and
then 14-22/40. Dating was by USS and maternal weight
correction.
Monte Carlo simulation (software programme S-plus) to
generate 50,000 DS results and 50,000 unaffected result. For
each set of results the LR for 1st T and 2nd T were
calculated, as well as for all seven markers combined
(LRMA).
Combined the LR with MA specific risk of DS and the MA
distribution of the USA for 2000.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Stepwise (LR1st T X LR2nd T)
90.2%, 3.9%
Difficulties implementing any
of the screening strategies
Errors in determining risk if
assuming that 1st T and 2nd T
tests are independent when
they are not.
Risk will be underestimated in
27% of DS cases and
overestimated in 20% of
unaffected. In 10% of DS the
risk will be underestimated ≥ 2
fold, and for 10% of
unaffected the risk will be
overestimated ≥ 2 fold.
Author’s conclusion
We conclude that the correlations that
exist between first and second trimester
screening tests preclude the use of
second trimester risks derived from the
direct product of separate first and
second trimester screening.
Should not be offered screening across 2
trimesters unless can be combined using
this multivariate algorithm.
Reviewers’ conclusions
The study has highlighted importance of
taking the correlation between markers
into account when calculating the LR.
128
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Palomaki et al. 2006)
The aim of the study was to describe the choices and
tradeoffs inherent in 3 strategies that combine 1st T and
2nd T markers.
Monte Carlo
simulation
Sample
Compares three policies stepwise (1st T combined then 2nd
T quad), contingent, and integrated screening.
Parameters (means SD, and correlation coefficients) and
truncation limits for modelling taken from SURUSS. Data
from pregnancies viable at 2nd T.
Assumes that if a case is detected in 1st T, there is no
screen in 2nd T. The MA distribution is that of the USA in 2000
(median 27 years and 13% ≥ 35 years). The MA specific risk
is based on a published equation (Hecht and Hook 1996
as referenced in this paper). Adjusted for 43% loss in DS
between late 1st T and term, and 23% loss between early
2nd T and term.
Monte Carlo simulation to generate MA and the
associated 7 markers for a million hypothetical cases of DS
and million unaffected. For each of the “pregnancies” 1st T
risk then 2nd T risk is assigned.
Modelling programme has been used elsewhere and
validated by comparing the results to other independent
models in the literature.
Assume complete adherence i.e. all positive cases get
diag. test and no one who has positive 1st T screen then
requests 2nd T. No one drops out.
Compared their result to that of SURUSS at same cut-offs.
Minor differences may be due to hCG rather than fβhCG
and slight differences in the MA distribution and a priori
risks. Still they are nearly identical to those of SURUSS.
Use same type of hCG in 1st as in 2nd T as feel these had to
be kept the same when comparing strategies.
Outcomes and
verification
Results
Comments
Outcomes
Compares firstly
stepwise screening to
integrated screening.
DRs are given for
stepwise screening for a
fixed FPR (2% and 5%)
and different cut-offs.
The FPR and cut-offs set
so that the DR for fully
integrated screen is
same as for sequential
screening. Cut-offs
provided in brackets for
each test.
Accuracy of screening
methods
Limitations
Makes assumptions that may not occur in
“real-world screening” e.g. that there is
complete adherence to the policy i.e. all
positive cases get IT and no one who has
positive 1st T screen then requests 2nd T.
The cut-offs are the
level at or above which
women would be
offered IT.
Secondly compares
contingent screening to
integrated screening in
the same manner. The
DR for fixed FPR (2% and
5%) are given for
contingent screening,
then compared to the
FPR for integrated
screening when the DR
are the same as for the
contingent screening.
Stepwise versus integrated
Stepwise DR for 2% FPR (1st T1:63, 2nd T-1:65)
84.3%
Integrated FPR (1:100)
1.2%
Stepwise DR for 5% FPR (1st T1:168, 2nd T-1:165)
89.9%
Integrated FPR (1:275)
3.1%
Stepwise FPR 5% (1st T-1:41, 2nd
T-1:450)
92.3%
Integrated FPR (1:470)
4.8%
Contingent (those with risk
1:1500 or lower no further
screen) versus integrated
Contingent DR for 2% FPR (1st
T-1:63, 2nd T-1:70)
84.1%
Integrated FPR (1:95)
1.2%
Contingent DR for 5% FPR (1st
T-1:168, 2nd T-1:195)
89.5%
Integrated FPR (1:250)
2.8%
For contingent
screening the cut-off
under which women
have no further screen
is either set at 1:1500 or
1:3250.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Author’s conclusion
“Integrated screening is the most efficient
of the 3 screening strategies but possible
to select risk cut-offs for both stepwise
and contingent that minimize losses in
efficiency while maintaining early
detection and early completion. For all of
these strategies well designed
intervention trials are needed to
determine acceptability to women and
providers in primary care settings and to
assess real-world performance.”
Reviewers’ conclusions
Slightly different DR and fixed FPR so
difficult to compare all three at same
time. However results do show that
integrated performs better than either
stepwise screening or contingent
screening.
129
Table 16.
Source
Country
Setting
Study design
Evidence Grading
(Palomaki et al. 2006)
Monte Carlo
simulation
Continued
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Comparison screening strategies
Sample
Outcomes and
verification
Results
Contingent (those with risk
1:3250 or lower have no
further testing) versus
integrated.
Contingent DR for 2% FPR (1st
T-1:63, 2nd T-1:65)
84.2%
Integrated FPR (1:95)
1.2%
Contingent DR for 5% FPR (1st
T-1:168, 2nd T-1:170)
89.8%
Integrated FPR (1:270)
3%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
130
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Wald et al. 2006b)
Compared screening with Integrated to serum Integrated
screening methods with and without the use of the Cross
trimester (CT) ratios.
Monte Carlo
simulation
Sample
Used data from SURUSS in which the following analytes
were measured in both 1st T and 2nd T: AFP, uE3, fβhCG
and total hCG, PAPP-A and inhibin-A. Some are markers in
one trimester but not other (e.g. PAPP-A).
Results are for 74 DS pregnancies with pairs of 1st T and 2nd T
measures and 492 unaffected pregnancies (3 were
removed as they had imprecise GA).
NT performed in 1st T. Analytes measured in 1st T between
10-13/40 and those in 2nd T 14-22/40. Median interval
between two measures was 31 days when first measure
done at 11/40, 27 when first taken at 12/40 and 18.5 when
first taken at 13/40.
Analytes expressed as MoM for unaffected pregnancies at
same GA. The CT ratio expressed as MoM in 2nd T divided by
MoM 1st T. Medians of CT ratios in DS pregnancies
estimated for 10/40, 11/40, 12/40, and 13/40. SD and
correlation coefficients estimated from SURUSS (based on
GA using CRL and corrected for maternal weight).
Parameter estimates for individual markers are from SURUSS.
Truncation limits given in appendix for the serum markers,
and for NT in the text. NT lower truncation limit was 0.65
which is higher than for SURUSS (as per Morris and Wald
2005, as referenced in this paper).
Outcomes and
verification
Results
Comments
Outcomes
The performance of
screening using the CT
ratios was better when
the 1st T measurement of
NT and MSS was at
11/40 compared to 12
or 13/40. The results are
therefore given for 1st
trimester screening at
11/40.
Accuracy of screening
methods
Limitations
Small sample used to determine the
parameters (74 DS cases).
The outcomes extracted
for this evidence table
were those for each
Cross trimester (CT) ratio
when first of each pair
taken at 11/40.
All were good
discriminators except
AFP. The results for
integrated screening
(with fβhCG and total
hCG) are presented
with and without the use
of the CT ratios (for all
markers except AFP).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
DR for 5% FPR
CT ratio-PAPP-A
60%
CT ratio-total hCG
42%
CT ratio-uE3
31%
CT ratio-inhibin-A
30%
CT ratio-fβhCG
19%
CT ratio-AFP
10%
Without CT ratios, DR for 5% FPR
Integrated test (fβhCG)
94.2%
Integrated test (total hCG)
94.1%,
Without CT ratios, FPR for 85%
DR
Integrated test (fβhCG)
0.88%
Integrated test (total hCG
0.95%
With CT ratios DR for 5% FPR
Integrated test (fβhCG)
96.9%
Integrated test (total hCG)
97.4%
The first author has a patent interest in the
integrated test and with others holds a
patent for the use of uE3 as a 2nd T
screening marker for DS. He is also the
director of logical Medical Systems
(software for interpretation of DS
screening test results).
Author’s conclusion
The addition of CT ratios to an Integrated
test substantially improves the efficacy
and safety of prenatal screening for DS. It
is cost effective and could be usefully
introduced into screening programmes.
Reviewers’ conclusions
More data may be needed to refine
parameters. However it appears that CT
ratios have the potential to improve
integrated screening.
131
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Wald et al. 2006b)
Multivariate Gaussian distributions were specified for
different combinations of screening markers. Monte Carlo
simulation used these distributions to generate random
samples (500,000 DS and 500,000 unaffected). The risk of DS
pregnancy at mid-trimester determined by MA specific
rates of DS at term adjusted by multiplying by 1/0.77 (fetal
loss between mid-trimester and term). This MA specific rate
was multiplied by the LR for marker values obtained by the
over lapping Gaussian distribution of affected and
unaffected pregnancies.
Continued
Sample
Outcomes and
verification
DR and FPR calculated for a specific risk cut-off. The MA
distribution based on England & Wales from 1996 to 1998.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Results
With CT ratios, FPR for 85% DR
Integrated test (fβhCG)
0.32%
Integrated test (total hCG)
0.28%
Comments
132
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison screening strategies
(Wright et al. 2006)
Compared three stage contingent screening, to integrated
screening, and a strategy of using TT rather than quad in
the 2nd T stage of contingent screening.
Statistical modelling
Sample
For the 3 stage contingent strategy PAPP-A and fβhCG
would be measured at 10/40. The risk would be combined
with MA associated risk and those with very low risk would
be considered screen negative and would have no further
screen.
All remaining women would then get NT screen at 11/40
and risk would be determined using 1st T screen and MA.
Those with very low risk would have no further screening
and those with very high risk would have invasive testing.
Those with intermediate risk would continue to 2nd T
screening. The quad test (AFP, uE3, fβhCG, and inhibin)
would be measured at 2nd T. MA risk, and results from 1st T
and 2nd T screens would be combined to assess risk. This
would be used to determine whether screen positive or
screen negative at this stage.
The integrated strategy would involve all women receiving
all tests and being told the result after all screening
completed.
Outcomes and
verification
Results
Comments
Outcomes
Results for 3 stage
contingent screening,
integrated screening,
and a strategy of using
TT rather than quad for
the contingent strategy
were extracted for this
evidence table.
Accuracy of screening
methods DR , FPR
Limitations
Assumes all with high risk will receive the
additional testing. However there is a
relatively narrow GA window and some
may not present until 2nd T.
The paper used
modelling to determine
the best cut-off. This was
stage one 1:2000, stage
2 low risk 1:2000 high risk
1:20, stage 3 1:250.
These results are
presented in this table
compared to
integrated screening
(final risk cut-off of
1:250).
Means, SD, and correlation coefficients obtained from
SURUSS (Wald et al. 2004).
These parameters based on pregnancies expected to be
viable in 2nd T and assume no correlation between marker
values and viability. SURUSS truncation limits used.
Modelling based on data where GA confirmed by USS and
weight corrected.
Various rates estimated using a Monte Carlo simulation.
500,000 observations were drawn. LR calculated for each
set of markers at each stage and combined with MA
distribution of DS or unaffected pregnancies to derive DR
and FPR.
The MA associated risk of DS taken form published data
(Wright and Bray, 2000 as referenced in this paper). MA
distribution that of England and Wales 2002.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
3 stage contingent with quad
89.5%, 1.9%
3 stage contingent with TT
89.2%, 2.2%
PAPP-A and βhCG combined
with quad -integrated
manner(non-disclosure)
92.2%, 2.1
Author’s conclusion
3 stage contingent screening achieved
similar results to integrated screening while
only a fraction needed 2nd T results.
About 2/3 of pregnancies are screened
with 1st T MSS alone, 5/6 women
complete screening in 1st T, and 1st T DR is
over 60%. This is a logical approach for
allocation of NT where this resource is
limited.
The acceptability of this protocol and its
performance in practice should be tested
in prospective studies.
Reviewers’ conclusions
This strategy appears promising but there
needs to be a prospective study in order
to have data based on observed data.
133
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Wald et al. 2006a)
The aim of the paper was to determine the effect of
adjusting serum markers for values from a previous
pregnancy. Women with a FP MSS in one pregnancy have
an increased chance of a FP result in a subsequent
pregnancy.
Monte Carlo
simulation
Sample
The study compared performance of screening with TT,
compared to quad, combined, serum integrated and
integrated screening, adjusting and not adjusting for DS in
previous pregnancy.
For each screening marker the values of the MoM were
adjusted to take account of the values of a previous
pregnancy using the regression coefficient of the weight
adjusted MoM values in the current pregnancy regressed
on the value of the previous pregnancy.
Outcomes and
verification
Results
Comments
Outcomes
For the purpose of this
evidence table the DR
and FPR for Triple, quad,
combined, serum
integrated and
integrated screen for a
5% FPR and an 85% DR
were extracted. These
are presented as
unadjusted figures, and
figures adjusted for
previous pregnancy
results.
Accuracy of screening
methods
Limitations
MoM adjustment does not take into
account that the SD of adjusted MoM
values tend to be smaller and correlation
coefficients slightly different. However
virtually no gain using adjusted distribution
parameters.
All tests used fβhCG.
The regression coefficient for 1st T markers was estimated
using data from 401 women who had MSS in two
pregnancies screened at the Wolfson Institute of Preventive
Medicine. For 2nd T markers used previously reported
estimates of the regression coefficients (Wald et al. 2004a,
as referenced in this paper). These were based on 6,448
women screened at the Wolfson Institute of Preventive
Medicine.
Adjusted all screening markers. Did not adjust NT as the
regression coefficient was so small.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Women with previous
pregnancy. DR (adjusted DR)
For a fixed 5% FPR.
Triple
75% (adj 80%)
Quad
81% (adj 85%)
Combined
85% (adj 87%)
Serum integrated
86% (adj 89%)
Integrated
94% (adj 95%)
FPR (adjusted FPR) For a fixed
85% DR.
Triple
10% (adj 7.9%)
Quad
7.1% (adj 4.9%)
Combined
4.9% (adj 3.7%)
Serum integrated
4.7% (adj 2.9%)
Integrated
1.1% (adj 0.7%)
Assumed that the relationship between
markers across two pregnancies is the
same whether the second has DS where
first does not, or both were unaffected (no
data but authors presume this is a safe
assumption).
The first author has a patent interest in the
integrated test and with others holds a
patent for the use of uE3 as a 2nd T
screening marker for DS. He is also the
director of logical Medical Systems
(software for interpretation of DS
screening test results).
Author’s conclusion
The results show that adjusting the MoM
for those in a previous pregnancy
improves screening performance and
avoids recurrent FP. Should be used on all
women with previous pregnancy screen
(as long as not DS in first). Both false
positives and false negatives will be
reduced.
134
Table 16.
Evidence table of primary research studies appraised investigating the accuracy of screening carried out in first and second trimesters (continued)
Source
Country
Setting
Study design
Evidence Grading
Comparison Interventions
(Wald et al. 2006a)
DR and FPR estimated by Monte Carlo simulation. Weight
adjusted MoM and MA were simulated for a previous
pregnancy and current pregnancy for a sample of 100,000
affected (for DR) and 100,000 unaffected (for FPR)
pregnancies.
Monte Carlo
simulation
Sample
Outcomes and
verification
Continued
Distribution of ages among women who had two
pregnancies from Wald et al. 2004a (as referenced in this
paper). MA specific risk of DS from Morris et al. 2002 (as
referenced in this paper).
Means DS and correlation coefficients for markers in the
same pregnancy were from SURUSS. Based on GA by USS,
NT at 11/40 and weight adjusted.
The correlation coefficients for markers in different
pregnancies were calculated from 401 women as above.
Truncated limits for all markers in appendix (from Wald et al.
2003 as referenced in this paper and Morris (2005)).
MoMs were adjusted for serum marker results in previous
pregnancy. These results together with MA were used to
calculate risk of DS.
Also examined affect of adjusting MoM for those who had
previous FPR.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Results
Comments
Should also not adjust where previous
pregnancy was a twin or where previous
pregnancy had markers adjusted for
smoking and not smoker now.
Also probably no need to adjust where
women screened in last 10 months as
likely to have ended in miscarriage with
risk of extreme levels.
Simplify by using most recent pregnancy.
Should also truncate to avoid adjusting
using very extreme levels which may have
been associated with T18.
Reviewers’ conclusions
While this was not the aim of the study the
results show that the integrated tests is
superior to the serum integrated test
which is superior to the combined test
which in turn is superior to the quad test
and that the TT has the poorest
performance of these 5 screening
methods.
135
Chapter 6: Changes in the Rate of
Invasive Testing Following the
Introduction of Screening
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY
The search identified 11 eligible primary research studies. Below is an overview of study designs and
aspects of quality represented by these studies. Full details of the 11 papers appraised, including
methods, key results, limitations and conclusions, are provided in evidence Table 17 (pages 142-155).
Studies are presented in reverse chronological order of publication within each table.
Study designs and quality assessments
Of the 11 eligible studies investigating changes in the rate of invasive testing following the introduction
of population-based MSS programmes, all 11 were graded evidence level III-2. All 11 of these studies
were retrospective cohort studies with eight studies comparing rates of testing before and after the
introduction of screening programmes (Shohat et al. 2003; Zoppi et al. 2001; Benn et al. 2005b; Jou et
al. 2005; Benn et al. 2004; Chasen et al. 2004; Muggli and Halliday 2004; Cheffins et al. 2000), and
three comparing the invasive testing rates in hospitals or areas with differing screening policies (SmithBindman et al. 2003; Dixon et al. 2004; Wellesley et al. 2002).
The eight studies comparing the rate of invasive testing before and after the introduction of populationbased MSS screening programmes were of similar design but varied considerably in terms of the type
of screening programme introduced, the quality of the data sources and the duration of follow-up. Jou
et al. (2005) reported the rates of amniocentesis in mothers aged 35 years and over in Taiwan between
1993 and 2001. The authors utilised large national databases of birth defects, amniocentesis records,
and demographic descriptions of the population in Taiwan to report the numbers of births, the
proportion of infants born to older mothers, the live birth prevalence of DS and rates of amniocentesis.
The quality of these databases is mixed and there is no information reported regarding the uptake of the
screening programme. The registration of live births was not compulsory in Taiwan until 1997 (Chen
et al. 2005), which brings into question the quality of the birth data and, thereby, the accuracy of
calculating amniocentesis rates as a proportion of total births.
Benn et al. (2004) aimed to examine the overall effectiveness of a MSS programme in clinical practice
by investigating changes in the numbers of samples processed by the authors’ cytogenetics laboratory
over an 11-year period (1991-2002). A triple-analyte MSS programme was introduced in Connecticut
in 1991, expanded to include a fourth analyte in 1999 and utilised USS findings to modify risk from
1996 onwards. While the records used were complete, the authors could not be certain that the
proportion of the population screened by their laboratory had remained constant over the period of the
study and that any changes in invasive testing were not the result of people being referred to other
laboratories. Indications for invasive testing were reclassified by the authors into one category when
multiple indications were present. There is no information as to whether the reclassification was
conducted by someone blind to the screening policy in place when the test was requested. A second
study by Benn et al. (2005b) utilised a similar sample but over a 12-year period (1991-2003) and
focussed on the uptake of invasive testing in true-positive versus false-positive cases. While the
quality of data were generally good in both of these studies, the samples consisted of a proportion of
the pregnant population of Connecticut and lacks generalisability.
Chasen et al. (2004) compared the rates of invasive testing after the introduction of NT measurement in
a medical centre between 2000 and 2002. The quality of records was high, however, the sample was
small and based in one medical centre, and therefore may not be generalisable to other populations. In
addition, the authors chose to exclude terminated pregnancies and stillbirths from the sample and so the
study reports only on the invasive testing rate in women aged 35 years or older who delivered viable
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
136
infants. As a number of invasive tests will result in terminated pregnancies and miscarriages, this
design does not give an accurate indication of changes in the overall rate of invasive testing.
Two studies retrospectively examined the rate of invasive testing in large state-wide MSS programmes
in Australia. Muggli and Halliday (2004) examined changes in the rate of prenatal diagnostic tests
performed in Victoria between 1992 and 2002. Prior to 1997, risk assessment for DS was made based
primarily on maternal age ≥ 37 years of age, previous family history or increased risk of aneuploidy.
In 1997 second trimester MSS based on 4 analytes and maternal age was introduced, and a combined
serum and NT risk assessment was available from 2000. Similarly, Cheffins et al. (2000) reported rates
of invasive testing over an 11-year period (1986-1996) following the introduction of a 4-analyte MSS
programme in South Australia in 1991. Both of these studies utilised high quality databases, reported
rates of invasive testing for older and younger mothers, and included all invasive tests performed over
the period of study, rather than just those of mothers who had delivered viable infants. The inclusion
of all pregnancies in the state and all complete records of all invasive tests make these results highly
valid and more generalisable to other settings.
Shohat et al. (2003) investigated the rate of invasive testing relative to screening policies in the Israeli Jewish population between 1990 and 2000. National birth and cytogenetic databases were utilised. In
Israel the MSS triple screen was introduced to the public between 1990 and 1992 (free of cost), USS
screen at 14-16 weeks were available privately at a cost from 1992, and NT measurements privately
from 1996. Unfortunately, the availability of some tests privately and some publicly makes it difficult
to determine the effect of each change in policy on invasive testing rates. Furthermore, the authors
used a maternal survey of all women who gave birth on a single day in 2000 to estimate the uptake of
various screening options over the whole period of the study. Lastly, cultural differences in the
acceptability and uptake of screening and invasive testing in the Israeli population make the findings of
this study less generalisable to other settings.
Zoppi et al. (2001) compared the rates of prenatal diagnosis in two cohorts of women, one group
referred prior to nuchal translucency measurement (1995) and one after (1999). The study was set in
Italy and the two cohorts of women were both ≥ 35 years of age. In the 1995 cohort, 982 women were
given non directive counselling and offered invasive testing on the basis of AMA. In the 1999 cohort,
1386 women were given non directive counselling and offered IT on the basis of AMA and NT results.
The authors focused on the proportion of women who declined invasive testing after receiving
nondirective counselling where NT results were or were not discussed. Women who presented too late
for 1st trimester NT measurement were included in analyses of rates of invasive testing in the NT
group. Removing these women from analyses altered the findings. Potential cultural differences in the
acceptability and uptake of screening and invasive testing in Italy make the findings of this study less
generalisable to other settings.
Three studies compared the rates of invasive tests performed in areas or hospital districts with differing
screening policies. Dixon et al. (2004) compared two district hospitals, one with a maternal serum
screening programme (2 analytes) in place and one with MSS available by request. In the second
(Wellesley et al. 2002), eight district maternity units were divided into three groups based on their
screening policies. Group 1 (two hospitals) assessed risk for DS based on two maternal serum analytes
and an anomaly scan. Group 2 (three hospitals) assessed risk based on maternal age and a second
trimester anomaly scan. Group 3 (three hospitals) included nuchal translucency measurement in their
risk calculations, although the application of NT was not consistent across the three districts, being
offered either to all mothers, on the basis of age, or information was supplied to mothers regarding
private nuchal translucency measurement. The age distribution of the cohorts varied significantly in
both studies and, given that maternal age was used in some serum screening protocols to calculate risk,
this may have confounded the results. In Wellesley et al. (2002), the rates of invasive testing are
difficult to compare because there were variations between hospitals in the same group, regarding the
age at which testing was offered, the availability of services through the public health system, and the
age of the sample.
Smith-Bindman et al. (2003) examined the proportion of invasive testing in England and Wales over an
11 year period (1989-1999) and in relation to the dominant screening policies in different areas. Data
describing almost 6,000,000 births and 335,000 prenatal diagnostic referrals were included in the study.
Data sources for births and cytogenetic results were of high quality. The screening method which lead
to a prenatal diagnosis in DS cases was used as a proxy measure for screening methods employed in
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
137
different areas for different years (area-years). Using this inferred method, each area-year was
classified on the basis of the dominant screening method at the time and rates of invasive testing
compared.
Study settings and samples
Jou et al. (2005) examined the rate of invasive testing using a Taiwanese national database of all
deliveries to mothers aged 35 years and over between 1993 and 2001. (Shohat et al. 2003) utilised large
national datasets in Israel to examine rates of invasive testing, with a focus on the Jewish-Israeli
population. Two studies, both based in Australia, examined rates of invasive testing following the
implementation of a state-wide maternal screening programme. Muggli and Halliday (2004) utilised
two units which collect information on indications for every invasive procedure and every birth at or
after 20 gestational weeks in the state of Victoria. Rates of invasive procedures between 1992 and
2002 were compared. Cheffins (2000) evaluated the South Australian Maternal Serum Antenatal
Screening Programme (SAMSAS) between 1986 and 1996. Both of these studies included all invasive
tests performed in the sample over the period of study and reported their results separately for older and
younger mothers.
Four studies, three based in the United States and one in Italy, were based on records collected in
specific hospitals or cytogenetic laboratories. Benn et al. (2004; 2005b) reported the numbers and
indications of all AC and CVS samples processed by one cytogenetics laboratory in the state of
Connecticut between 1991 and 2002, and so included both older and younger mothers in the sample.
Chasen et al. (2004) reviewed the records of all women aged 35 years and over who delivered viable
infants at one hospital in New York State. Women who underwent a termination were excluded from
the study. (Zoppi et al. 2001) compared the proportion of invasive testing in two groups of women,
both aged ≥ 35 years, who were screened for DS risk based on maternal age alone or nuchal
translucency and maternal age.
Two studies (Dixon et al. 2004; Wellesley et al. 2002) utilised the records of maternity hospitals based
in neighbouring districts and both of these were based in England. Dixon et al. included all registered
pregnancies in two district hospitals in Gloucestershire, England between 1993 and 1999, and reported
rates of invasive testing separately for older and younger mothers. Wellesley included all women who
completed their pregnancies in one of eight hospitals in Wessex, England between 1994 and 1999.
While mothers of all ages were included in the sample, the results were reported as an average rate of
invasive testing across the period of study and not reported separately for each age group. (SmithBindman et al. 2003) reviewed the dominant screening policies and rate of invasive testing in England
and Wales from 1989-1999.
Study interventions, comparators and outcomes
All of the studies examined the rates of invasive testing in district, state, or national community
screening programmes.
In eight studies the rates of invasive testing were compared before and after the implementation of a
screening programme. In two cases a maternal screening programme utilising two analytes had been
introduced, in two cases nuchal translucency measurement had been introduced, and in the remaining
four studies a triple screen or quadruple screen had been introduced. The policy prior to the
implementation of these programmes was not specified in all cases, but in the studies which did
describe the previous policy it was generally based on maternal age (either ≥ 35 or ≥ 37 years), and
previous family history or risk of aneuploidy. Uptake of screening varied between samples and was
not reported in some cases.
Five of the studies reported the rates of testing for individual years of study. One study reported the
rate of testing for specific years during the period of the study because they corresponded to particular
changes in policy or uptake of screening. One study reported the average rate of testing across the 6year period of the study instead of including data for individual years.
Two of the studies compared the rates of invasive testing between maternity units with different
screening policies. In one study two district hospitals were compared, one with a maternal serum
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
138
screening programme (2 analytes) in place and one without. In the second, 8 district maternity units
were divided into three groups of districts with similar screening policies in place. Group 1 assessed
risk for DS based on two maternal serum analytes and an anomaly scan. Group 2 assessed risk based on
maternal age and a second trimester anomaly scan. Group 3 included nuchal translucency measurement
in their risk calculations, although the application of NT was not consistent across the three districts,
being offered either to all mothers, on the basis of age, or information was supplied to mothers
regarding private nuchal translucency measurement. One final study compared the rates of invasive
testing for different areas in each year of the study (area-years) (Smith-Bindman et al. 2003). The
dominant screening method in each area for each year of study was approximated using a proxy
measure of the method of screening in identified DS cases.
There were variations in the way data were reported. In five studies the rates of CVS and AC were
reported separately, in five studies a single rate of invasive testing (AC + CVS) was reported, and in
one study the numbers of invasive tests were reported rather than the rate. Four studies reported rates
of testing separately for older and younger mothers, three studies only included mothers aged 35 or
older, and four studies compared the overall proportion of invasive testing across age groups.
The rate of invasive testing was calculated as the number of tests performed or serum samples
analysed/ the total number of pregnancies or total pregnancies for that age group.
PRIMARY RESEARCH: STUDY RESULTS
Studies comparing the rate of invasive testing before and after implementing a MSS
programme
Seven studies compared the rate of invasive testing before and after the implementation of populationbased MSS programmes. One of the studies (Jou et al. 2005) examined the introduction of a two
analyte screen, one study (Benn et al. 2005b) compared rates before and after the introduction of a
three and four analyte screen, and two (Muggli and Halliday; 2005, Cheffins, 2000) the effectiveness
of a four analyte screen. One further study (Chasen, 2002) examined the effectiveness of using nuchal
translucency measurements to detect DS.
Two studies utilised high quality sources of data, included representative samples and examined the
rates of invasive testing over an acceptable period of time. Cheffins et al. (2000) evaluation of
SAMSAS included information about the rate of invasive testing, births to women aged 35 years and
older, and the uptake of a four analyte maternal serum screen in South Australia between 1986 and
1996. Overall, births to women of AMA (≥ 35 years) increased from 5.2% of total births in 1982 to
13.5% in 1996. There was an overall increase in the proportion of pregnant women undergoing
invasive testing from 4.9% in 1986 to 11.4% in 1996. When these rates were examined relative to
maternal age, the authors’ reported that the rate of invasive testing in older women had not changed
significantly since the introduction of maternal screening (51.0% in 1986 to 53.8% in 1996) whereas in
younger women it had increased from 1.7% to 4.8% over the same period. A comparison of
indications for referrals across time showed that indications based on maternal age alone had decreased
from 60.7% to 51.0% as a proportion of all tests. The proportion of tests referred on the basis of MSS
results increased from 9.5% to 35.7%.
Muggli and Halliday (2005), in their evaluation of a four analyte serum screening programme
introduced in Victoria in 1996, also noted a steady increase in the proportion of births to women of
AMA (≥ 37 years) giving birth over time, from 6.1% in 1992 to 11.2% in 2002. Prior to the
introduction of MSS in 1996, invasive tests were recommended based primarily on maternal age ≥ 37
years. During this period the rates of invasive testing increased from 5.9% in 1992 to 8.2% in 1996.
MSS was introduced for all women in the public health system in 1996. Overall rates of invasive
testing were 8.8% in 1998 and 7.9% in 2002. Among older women, the rate of invasive testing
decreased from 63.0% in 1992 to 42.7% in 2002, while the proportion of younger women undergoing
an invasive procedure increased from 2.2% to 3.6% over the same period.
A comparison of
indications for referrals between 1992 and 2002 showed that indications based on maternal age alone
decreased from 62.2% to 48.3% as a proportion of all tests. The proportion of tests recommended on
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
139
the basis of abnormal screening results (MSS or USS or both) increased from 6.9% to 35.4% of all
tests.
Benn et al. (2004) reported an overall decrease in the number of amniotic or chorionic villus samples
processed at a cytogenetics laboratory between 1991 and 2002 when, based on the age demographics of
the population, the expectation would have been that the number would have increased. In 1991 a
three analyte (AFP, uE3, hCG + MA) MSS programme was introduced to screen for DS and this was
expanded to include inhibin-A in 1999. There were however, a number of limitations in this study
which make generalisation of the findings to other populations difficult. The authors acknowledged
that they assumed the proportion of the population serviced by their laboratory had remained constant
over the period of study, and that it was possible that changes in the number of samples processed by
the lab were the result of changes in referrals to their lab, rather than due to screening policy change.
They noted that the numbers of samples processed remained within 19-22% of all Connecticut births
during this time. AMA as an indication for invasive testing decreased from 66% of all tests in 1991 to
45% in 2002, while tests referred on the basis of MSS results increased from 23% to 35% of all tests
over the same period of time. Given that indications for referral were reclassified if there were
multiple indications, it is difficult to determine the effect of individual changes in screening policy, and
the authors acknowledge this limitation. Furthermore, there is no information as to whether the person
who reclassified the indications was blind to the screening policy in place for each case.
A second study by Benn et al. (2005b) utilised a similar sample but over a slightly different timeframe
(1991-2003) and examined both the proportion of invasive tests performed in DS screen-positive
pregnancies and the proportion performed in false-positive pregnancies, over the period of the study.
There was a reduction in the utilisation of amniocentesis by screen-positive women from 70% in 1991
to 27.7% in 2003. When DS affected pregnancies and false-positive pregnancies were examined
separately, the authors found there was no significant change over time in the rate of AC in DS affected
pregnancies (average =73%), but in false-positives, the decline from 70% to 27% was significant.
There was no information about the change in rate of AC over time either overall or for older and
younger women.
Chasen et al. (2004) examined the rates of invasive testing in women aged 35 years or older who gave
birth at a New York based medical centre between 2000 and 2002. NT screening was introduced in
2000 and the authors compared the rate of AC and CVS between mothers who were screened and not
screened. Overall rates of IT decreased from 70.0% to 64.7% over the three year period of the study
(p<.001). A significantly greater proportion of women who underwent NT screening opted for CVS
(7.1%) than in those who did not take up NT screening (1.9%, p<.001). There was no difference in
rates of amniocentesis between the screened (64.1%) and unscreened groups (62.1%), or in overall
rates of invasive testing between screened (66.0%) and unscreened (69.3%) groups. However, the
follow-up was not long enough to provide a real indication of the change in invasive testing following
the introduction of screening.
Shohat et al. (2003) investigated the rate of invasive testing following the introduction of second
trimester maternal serum screening in 1990-1992, targeted ultrasound screening in 1992, and nuchal
translucency measurements in 1996. In older women, the rate of invasive testing decreased from 66.5
to 48.3% between 1990 and 2000. In women <35 years of age, the rate of invasive testing increased
from 5.7% to 13.8% over the same period. Overall there appears to have been an initial increase in
invasive testing rates between 1990 and 1993, followed by a leveling out and slight decrease between
1994 and 2000.
Zoppi et al. (2001) compared the rates of prenatal diagnosis in two cohorts of women, both ≥ 35 years
of age. In the 1995 cohort, 982 women were given non directive counselling and offered invasive
testing on the basis of AMA. In the 1999 cohort, 1386 women were given non directive counselling
and offered IT on the basis of AMA and NT results. A higher proportion of women accepted invasive
testing after screening based on maternal age alone compared to screening which included nuchal
translucency measurements (70.2% vs. 66.1%). However, this difference was not significant and 297
women who presented too late for NT screening were included in the calculation of invasive testing
uptake. It was possible to analyse the data excluding these women and when this was done, the rate of
invasive testing in the NT group was 77.9%, significantly higher than the AMA alone group. The
design of this study gives an indication of changes in the rate of testing following the implementation
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
140
of a new screening policy, but a much longer follow-up period is needed to get a real sense of the
impact of any change.
Jou et al. (2005) reported a substantial increase in AC rates between 1991 and 2002. During this period
there were, however, two important policy changes in Taiwan that potentially may have biased their
results. The registration of live births was not compulsory in Taiwan until 1997 (Jou et al. 2005),
which brings into question the quality of the birth data and, thereby, the accuracy of calculating
amniocentesis rates as a proportion of total births. Secondly, Chen et al. (2005) commented on the
implementation of a programme to promote prenatal diagnosis in older women in 1990 and a change in
family values to one of quality rather than quantity which may have made the use of more definitive
methods of prenatal diagnosis, such as AC or CVS, more popular.
Studies comparing the rate of invasive testing in health districts with differing DS screening
policies:
Three studies compared the rate of invasive testing in areas or health districts with differing screening
policies for DS.
Smith-Bindman et al. (2003) examined the proportion of invasive testing in relation to the dominant
screening policies in different areas in England and Wales over an 11 year period (1989-1999). High
quality data describing almost 6,000,000 births and 335,000 prenatal diagnostic referrals were included
in the study. The screening method which lead to a prenatal diagnosis in DS cases was used as a proxy
measure for screening methods employed in different areas for different years (area-years). Using this
inferred method, each area-year was classified on the basis of the dominant screening method at the
time and the rates of invasive testing compared. The number of invasive tests per DS case detected
were reported but the proportion of women undergoing invasive testing for each area-year was not.
The overall rate of invasive testing increased gradually from 4.4% in 1989 to 5.8% in 1999.
Dixon et al. (2004) compared two district hospitals, one with a maternal serum screening programme (2
analytes) in place and one with MSS available by request (1.6% of women requested MSS). The
overall rate of invasive testing in the district with a MSS programme was significantly higher (7.6%)
than in the district with MSS available only by request (4.4%, p < 0.001). When these rates were
examined as a function of age they showed that, among older mothers, the rate of invasive testing was
lower in the district with routine MSS (29%) than in the MSS by request district (38%). Among
mothers aged 25-34 years of age, the rate of invasive testing was higher in the district with MSS (4.8%)
than the district with MSS by request (0.61%). Unfortunately, the age distribution of the two cohorts
was different, with women in the district with MSS being significantly older than those in the district
with no MSS. Because maternal age was used in conjunction with MSS, gestational age and maternal
weight to calculate DS risk, it is possible that this population had a higher uptake of invasive testing as
a result of the age of the sample, rather than because of the introduction of the screening programme.
Rates of testing were presented as an average over the six-year period of the study so it is difficult to
determine how rates of testing changed over time as a result of the introduction of MSS.
Wellesley et al. (2002) utilised a similar design where eight district maternity units were divided into
three groups based on their screening policies. Group 1 (two hospitals) assessed risk for DS based on 2
maternal serum analytes and an anomaly scan. Group 2 (three hospitals) assessed risk based on
maternal age and a second trimester anomaly scan. Group 3 (three hospitals) included nuchal
translucency measurement in their risk calculations, although the application of NT was not consistent
across the 3 districts, being offered either to all mothers, on the basis of age, or information was
supplied to mothers regarding private nuchal translucency measurement. In the two districts offering
serum screening (Group 1) the average rate of invasive testing was 6.3%. In districts offering invasive
testing on the basis of MA (35+ or 37+) and an USS anomaly scan at 20 weeks (Group 2), the average
rate was 5.2%. In districts offering invasive testing on the basis of MA and NT (Group 3) the average
rate was 5.3%. However there was some variation between hospitals in the same group, for instance,
rates of testing in group 3 ranged from 2.8% to 7.7%. Interestingly, the district with the highest rate of
invasive testing had the oldest maternal population and the district with the lowest rate of invasive
testing had the youngest maternal population. The authors suggested that the proportion of women
who accept an invasive diagnostic test increases with age and risk even in populations with serum
screening in place. The rates of invasive testing are difficult to compare because there were variations
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
141
between hospitals in the same group in the age at which testing was offered, the availability of services
through the public health system, and the age distribution of the samples.
Conclusion
In general, the quality of appraised studies in this section of the report was not high. There were
limitations regarding sample selection and the setting of the study which may have biased the findings
in several of the studies or at least made them less applicable to other settings.
The uptake of screening varied and many older women still opted for direct invasive testing. Factors
such as the perceived accuracy of the test may affect women’s decisions regarding screening and
subsequent invasive testing. Screening uptake seemed to increase the longer a test had been used,
perhaps reflecting women’s confidence in the results. Unfortunately, none of the studies included in
this chapter evaluated the change in rates of invasive testing following the introduction of integrated or
sequential screening methods. While the performance of these methods in detecting Down syndrome
cases has been examined in short-term audits of community screening programmes, they have not yet
been implemented long enough to provide an indication of the long-term effects on invasive testing
rates.
Of the 11 studies included in this chapter, two were designed well enough to provide a reliable
indication of the impact of a screening programme on rates of invasive testing. In one study a four
analyte screen (AFP, uE3, α and β subunits of hCG) was introduced (Cheffins et al. 2000) and in the
other the quadruple test (Muggli and Halliday, 2005). Both of these studies were based in Australia
and used reliable, complete sources of data, followed the cohort for an appropriate length of time, and
reported their findings separately for older and younger mothers. It appears that overall rates of
invasive testing increased slightly after the introduction of screening against the backdrop of a steeper
rise in maternal age. If referrals for prenatal diagnosis had been made on the basis of maternal age
alone, the rates of invasive tests would have been expected to increase more than they did after
screening was introduced.
When the uptake of invasive testing was examined as a function of age, the pattern was one of a
decrease in older mothers and increase in younger mothers after the introduction of screening. In areas
with screening in place there was generally a decrease in rates of testing in older mothers and fewer
tests were recommended on the basis of maternal age alone, thereby decreasing the number of
unnecessary invasive procedures in that age group. If the proportion of older mothers accepting
invasive testing declines with the introduction of a screening programme, changing patterns in maternal
age are likely to be an important determinant of invasive testing rates if such a programme was to be
introduced. A limitation of this chapter was that none of the studies evaluated the effect of introducing
integrated or sequential screening strategies on the rate of invasive testing. The results from long-term
evaluations of population-based screening programmes utilising these strategies are not yet available.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
142
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
Source
Sample
Screening Strategies
Outcomes
Results
Comments
Benn et al. (2005b)
N= 109, 469 maternal serum tests
performed on singleton
pregnancies that were referred to
the authors’ cytogenetics
laboratory between September
1991 and December 2003.
September 1991:
Triple test introduced –
maternal serum AFP, hCG,
uE3 + MA
Utilisation of AC
Cytogenetic results
MSS provided to 109,469 women with
singleton pregnancies between 1991
and 2003
The presence of DS or other
aneuploidy identified at
birth
Age distribution:
≥ 35 years at delivery = 12.9% of
screened population
The proportion of births to
mothers ≥ 35 years
Changes in utilization of AC:
Screen positive women (all ages)
1991 = 70% AC
2003 = 27.7% AC
Authors Conclusions
Between 1991 and 2003 there was a marked
reduction in the utilization of AC by screen positive
women. This was true of women aged 35 or older
and those aged < 35 years. The overall reduction
in AC rates was confined to false-positive cases. In
affected pregnancies, there was no significant
change in the rate of AC (average 73%), but in
false-positives, the decline from 70% to 27% was
significant.
University of
Connecticut Health
Center Human
Genetics Laboratories
Retrospective cohort
Level of evidence III-2
Data were collected from
laboratory records regarding
utilization of AC, cytogenetic
results, presence of DS or other
aneuploidy.
Proportion of births to AMA women
collected from birth certificate
data
April 1999:
Inhibin-A added to serum
screening
2nd T cut-off of 1:270 used to
identify high risk pregnancies
January 1996:
2nd T USS used to modify
age-specific or post serum
screening risk
False positives (all ages)
1991 = 70%
2003 = 27%
Significant difference (p<.001)
Screen positive affected pregnancies
(all ages)
No significant difference in AC rate
between 1991 and 2003 (average
73%)
Proportion of AMA women who
received screening:
1991 = 58% of all AMA women
2003 = 83% of all AMA women
Reviewers Conclusions
Rates of AC uptake for screen positive affected
pregnancies fluctuated between 1991 and 2003.
The authors do not present the actual uptake for
this group but report that it was not a significant
difference. They include a figure comparing the
rate of uptake for affected and false positive
pregnancies and it appears that the AC rate for
unaffected pregnancies initially increased from
about 50% in 1991 to about 90% in 1996, followed
by an overall decline to about 70% uptake in 2003.
The authors present rates of AC averaged over
the period of the study and focus instead on the
difference between AC rates in screen positive
affected pregnancies and screened false positive
pregnancies. The study does not provide
information about the change in overall rate of
AC over time either overall or for older and
younger women.
The sample demographics were not reported in
enough detail to ascertain whether the
participants were representative of the
Connecticut pregnant population or whether the
results are generalisable to other populations.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
143
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Jou et al. 2005)
N= 1 331 616 deliveries between
1993 and 2001.
2nd T MSS for DS introduced
in 1994 using 2 analytes:
AFP and hCG
AFP and free beta-hCG
+ MA
AC rates per year in
women aged 35 years
and older
The proportion of pregnant women
aged 35 and older was 4.8% in 1993
and rose steadily to 8.3% in 2001.
Live birth prevalence of DS
in the Taiwanese
population
AC rate in pregnant women ≥35
years of age:
1993=25.3%
1994=35.0%
1995=41.3%
1996=46.1%
1997=53.3%
1998=56.7%
1999=69.2%
2000=75.8%
2001=70.7%
Authors Conclusions
The live birth rate of DS fell markedly from 0.63 per 1000
live births in 1994 to 0.21 per 1000 live births in 2001. This
sudden fall in live birth rates of infants with DS is mainly
due to the implementation and liberal use of the twomarker MSS test for DS during the 2nd T. We do not
know how many women underwent the test per year in
Taiwan but it is estimated that probably about 65-85%
of pregnancies were screened. AC rates may have
increased because the present policy in Taiwan still
indicates routine AC in women aged 35 years or older
and serum testing in other women. However the
efficacy of AC has been re-evaluated and the rate of
AC decreased in 2001.
Taiwan
Retrospective cohort
Level of evidence III-2
Taiwan has an average of
approximately 300,000 live births
per year.
Data sources:
Birth defects registration
(1993-2001)
Amniocentesis database
(1987-2001)
Demographic databases
(1991-2001)
Live birth rate of isolated
cleft palate (ICP) used as
an internal control
Reviewers Conclusions
There is not enough information provided in the study
to ascertain whether the screening programme was
responsible for the decrease in the live birth rate of DS,
or how the introduction of the screening programme
affected rates of AC.
There are no reliable data reported about the uptake
of screening. It is possible that screening was not as
widely accepted as the authors postulated and that
the introduction of screening merely raised awareness
of DS. Mothers may have been more likely to opt for
direct AC to obtain a definitive diagnosis about their
child as a result of this increased awareness. We have
no way of knowing whether mothers who opted for AC
had previously undergone MSS.
Policy changes in Taiwan during the period of the study
may have affected the rates of AC. Compulsory birth
registration was introduced in 1997 suggesting that the
birth data may not have been accurate prior to this
time, and if AC rates were calculated as a proportion
of all births, this may have affected their accuracy as
well.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
144
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Benn et al. 2004)
N = 18057 records regarding all
amniotic or chorionic villus samples
processed by the laboratory
between 1991 and 2002
1991 – high risk women
identified mostly on the basis
of MA (≥35 years), low
maternal serum maternal
AFP, or family hx
The numbers of invasive
tests ordered, indications
for testing, and results of
tests were compared for
each year of study.
Births:
1991
Live births = 48566
AMA births = 6 082 (12.5%)
September 1991:
Triple test introduced –
maternal serum AFP, hCG,
uE3 + MA
Trends in the use of
prenatal testing, referral
indications, and numbers of
abnormalities were
identified.
Authors Conclusions:
Against the background of an increase in the
number of women aged 35 years or older at
delivery, the number of invasive tests performed
decreased by 50% between 1991 and 2002. The
reduction of invasive tests is largely attributable to
the introduction of serum screening and 2nd T
ultrasonography to determine risk, instead of MA
alone. However, because indications for testing
were reduced to one indication per test, it is
difficult to determine the relative contributions of
each change in screening policy.
No new cytogenetics laboratories opened in the
area and the proportion of women receiving MSS
DS tests by our laboratory remained within 19.121.3% of the total Connecticut pregnant
population, suggesting that any changes in
referral numbers were not because patients were
referred to competing laboratories.
University of
Connecticut Health
Centre cytogenetics
laboratory
USA
Retrospective cohort
Level of Evidence: III-2
Numbers of referrals were reported
separately for DS cases and other
abnormal karyotypes.
Indications for prenatal dx:
1) fetal demise
2) abnormal USS
3) abnormal serum screening
results
4) family history of aneuploidy
5) maternal age of 35 years or
older
6) other
Multiple indications were reduced
to a single indication in the above
order of priority.
January 1996:
2nd T USS used to modify
age-specific or post serum
screening risk
April 1999:
Inhibin-A added to serum
screening
2002
Live births = 41690
AMA births = 9 040 (21.7%)
Numbers of prenatal diagnoses
performed each year:
1991
AC fluid samples = 1870
CVS samples = 118
Total = 1988/48566 = 4.1% (95% CI 3.9 –
4.3%) of total births
1996
AC fluid samples = 1581
CVS samples = 60
2002
AC fluid samples = 878
CVS samples = 55
Total = 933/41690 = 2.2% (95% CI 2.1 –
2.4%) of total births
Indications for referral:
AMA number (%age of referrals)
1991=1314 (66%, 95% CI 64 – 68%)
2002=423 (45%, 95% CI 42 – 49%)
MSS number (%age of referrals)
1991=455 (23%, 95% CI 21 – 25%)
2002=350 (38%, 95% CI 34 – 41%)
Abnormal USS number (%age referrals)
1991=72 (4%, 95% CI 3 - 4%)
2002=127 (14%, 95% CI 11 – 16%)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers Conclusions:
There is evidence of a decrease in the overall
number of invasive tests performed between
1991 and 2002 when, based on the age
demographics of the population, the expectation
would have been that the number of ITs would
have increased had AMA alone been used to
identify high risk mothers. During this period, MSS
to screen prenatally for DS risk was introduced but
this study cannot be used to demonstrate a
causal link between the introduction of screening
and the decrease in invasive tests performed.
Given that indications for referral were reclassified
if there were multiple indications, it is difficult to
determine the effect of individual changes in
screening policy, and the authors acknowledge
this limitation. Furthermore, there is no information
as to whether the person who reclassified the
indications was blind to the screening policy in
place for each case. It is also impossible to
determine the individual screening methods used
by individual practitioners in the state, which may
have varied widely and may or may not have
reflected the state policy on DS screening.
145
Table 17.
Source
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Sample
Screening Strategies
Outcomes
Results
(Benn et al. 2004)
Comments
The sample demographics were not reported in
enough detail to ascertain whether the
participants were representative of the
Connecticut pregnant population or whether the
results are generalisable to other populations.
University of
Connecticut Health
Centre cytogenetics
laboratory
This study gives an indication of the effects on the
rate of invasive testing of introducing MSS and 2nd
T USS screening for DS in a population. However
the results cannot reliably be used to predict
change in invasive testing rates with the
introduction of similar policies in other populations.
USA
Retrospective cohort
Level of Evidence: III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
146
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Chasen et al. 2004)
N= 4029 women aged 35 years or
older who delivered viable infants
between January 2000 to
December 31 2002
Main objective: assessing
the impact of NT screening
on the rate of CVS and AC
in women ≥35 years old
Rates of screening and IT
reported for six 6-monthly
periods between January
2000 and December 2002.
Median age at delivery = 37 years
NT screening introduced
April, 2000:
NT 11-14 weeks GA (as per
FMF protocol)
High risk cut off > 1:300
Measures:
NT screening rates
2nd T multiple marker
screening rates
CVS and AC rates
Rates of testing with and without NT
screening:
NT group:
CVS=1.9%
AC=64.1%
Overall IT=66.0%
Authors Conclusions
There was a decline in invasive testing that
coincided with the increasing use of NT screening.
Women who underwent NT screening were less
likely to have CVS than women who did not
undergo screening. Rates of AC stayed the same.
Different trends were noted in 35-39 year olds and
≥40 year olds. In 35-39 year olds, the declining
rates of both CVS and AC contributed to an
overall decline in invasive testing. In women aged
40 years and older, the rate of CVS declined
although the rate of AC increased, with a rate of
IT that did not change significantly over time.
USA
New York Weill Cornell
Medical Center
Hospital
Retrospective review
of hospital records –
USS database and
antepartum records
Level of evidence III-2
Exclusion criteria:
- women who underwent abortion
- women who were cared for by
physicians who did not deliver their
patients at the authors hospital
2nd T USS 18-20 weeks GA
No NT group:
CVS=7.1%
AC=62.1%
Overall IT=69.3%
Rates of testing by age group:
<40 years old
NT : AC=60.6%, CVS=1.8%
No NT : AC=61.8%, CVS=4.2%
≥40 years old
NT: AC=75.7%, CVS=2.4%
no NT: AC=63.7%, CVS=19.3%
Uptake of screening:
Rates of NT screening increased from
0% to 41.2% (p<.001) over the two year
period.
Overall rates of CVS decreased from
7.9% to 4.4% (p<.001) over the two
year period. Rates of CVS among
those who did not have NT screening
also decreased over the period of the
study from 7.9% to 6.5%(p=.02)
suggesting there was an overall trend
of a decrease in CVS regardless of
screening. There was no change in
AC rates but there was an overall
decrease in IT from 70.0% to 64.7%
(p<.001).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers Conclusions
Only women who delivered viable infants were
included in the sample so the results of this study
do not report the rates of IT in all women who
underwent screening. The authors acknowledge
this and explain that, because one of the
concerns about IT rates is exposure of unaffected
fetuses to IT, they felt that excluding aborted
fetuses was appropriate.
Only age-related demographic information was
reported for the sample so it is difficult to
determine how representative the sample was of
the wider population. Because the sample was
restricted to women ≥ 35 years of age, the findings
of the study have limited generalisability.
The authors acknowledged that other factors may
have contributed to changes in IT rates, including
better education of physicians and patients about
the use of 2nd T screening, and pointed out that
they could not be certain that there was a causal
relationship between NT screening and changes
in IT rates. In addition, the authors reported a
decrease in CVS rates over the period of the study
for those who did not undergo NT screening,
suggesting an external factor may have been at
least partially responsible for the decrease.
147
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Dixon et al. 2004)
N= 38,475 registered pregnancies in
two district hospitals between 1993
and 1999
Comparison of the impact
of different DS antenatal
screening policies on
detection and AC rates.
IT rates for each district and
maternal age group
Women who registered their
pregnancies in West Gloucestershire
were significantly younger than
women in East Gloucestershire.
Authors Conclusions
Our findings show that in Gloucestershire between
1993 and 1999, the double test identified a greater
proportion of pregnancies affected by DS than a
programme based on age-based AC and 20
week USS. The acceptance rate of the double
test suffered a steady decline from 67% in 1993-4
to 47% in 1998-1999. The highest acceptance rate
was 66% in the 25-34 year age group.
Gloucestershire,
England
Retrospective cohort
– review of records
(1993-1999)
Two district hospitals in
Gloucestershire with
different prenatal DS
screening policies.
Level of evidence III-2
District 1 – East Gloucestershire
N=14,863
< 25 years = 25%
25-34 years = 59%
>34 years = 16%
District 2 – West Gloucestershire
N=23,612
<25 years = 29%
25-34 years = 61%
>34 years = 10%
Data sources:
Regional cytogenetic laboratory
records, Gloucestershire community
pediatric service register, medical
records
East Gloucestershire:
May 1993-1999 offered an
opt-in MSS programme to
women ≥ 25 years. No NT
available but small minority
able to request NT privately.
MSS between 15-19/40
based on two analytes
(double test):
AFP
fßhCG
MSS + MA + GA + maternal
weight used to assign risk.
MSS risk cut-off May 1993 to
Jan 1994 was 1:250. Jan
1994 increased to 1:200
Women with a +ve MSS
result, history of aneuploidy
or >34 years MA were
offered AC or CVS.
West Gloucestershire:
No MSS unless requested by
woman or her doctor. Of
the pregnant population in
West Gloucestershire, 1.6%
had a double test.
Both districts offered AC if
DS-related anomalies were
found by a mid-gestation
scan.
DS cases for each district
and maternal age group
Fetal losses after IT
Uptake of IT following a
positive MSS result
Rate of Invasive testing:
The overall rate of IT in West
Gloucestershire (no MSS) was
significantly lower than East
Gloucestershire (MSS) (p<.001).
East Gloucestershire = 7.6% (95% CI
6.6-8.6%)
West Gloucestershire = 4.4% (95% CI
3.0-5.9%)
Rates of IT for each age group:
East Gloucestershire
<25 = 32/3806 = 0.8% (95% CI 0.6 –
1.1%)
25-34 = 425/8713 = 4.9% (95% CI 4.4 –
5.3%)
>34 = 671/2344 = 28.6% (95% CI 26.8 –
30.5%)
West Gloucestershire
<25 = 24/6875 = 0.3% (95% CI 0.2 –
0.5%)
25-34 = 87/14305 = 0.61% (95% CI 0.5 –
0.7%)
>34 = 931/2432 = 38.3% (95% CI 36.3 –
40.2%)
Rate of acceptance of screening:
East Gloucestershire (opt in MSS)
overall = 51%
<25 years = 16%
25 – 34 = 66%
>34 = 53%
West Gloucestershire (by request)
overall = 1.6%
Invasive testing acceptance rate
following a positive MSS result:
<25 = 87%
25-34 = 93%
>34 = 86%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Maternal age was the principal indication for IT in
West G. whereas a positive MSS result in women
aged 25-34 was the main indication and cause of
the significantly higher IT rate in East G. The rate of
IT in East G. was significantly higher than that in
West G.
Reviewers Conclusions
The higher rate of IT in East G. (MSS) seems to be
driven by the 25-34 year age group, who had the
highest uptake of MSS and among whom positive
MSS results were the main indication for IT. In
women aged > 34, positive MSS results and MA
were equally likely indications for IT.
It appeared that AMA women may be using the
screen programme to avoid AC.
Retrospective so relying on accurate records.
148
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Muggli and Halliday
2004)
Victoria, Australia
All women who received prenatal
dx before 25 weeks gestation in
Victoria, Australia between 1992
and 2002.
Retrospective analysis
of statewide datasets
Data were collected from the
following sources:
Aim: To describe patterns of
uptake of prenatal
diagnostic testing and
prenatal DRs for DS in
Victoria with regard to
maternal age and prenatal
screening practices.
Total number of prenatal diagnostic
tests:
Steady increase from 1992 – 1998
followed by an 8% decline from 2000
to 2002. The proportion of CVS was
about 40% over this period. Total
confinements were about 60000 per
year from 1992 – 2002.
Level of evidence III-2
Public Health Genetics Unit which
collects data on indications for
every CVS and AC procedure in
Victoria.
2nd T MSS screening
became available for all
women in 1997 using a four
analyte screen:
AFP
hCG
inhibin-A
uE3
+ MA
Authors Conclusions
Although the proportion of older mothers (≥ 37
years) has doubled in the past 10 years and in
2002 represented 11% of all women giving birth,
there has been a steady decrease in the utilization
of IT by older women. At the same time an
increasing number of younger women are being
referred for invasive testing following an increased
risk result of a screening test.
Perinatal Data Collection Unit
collects data on every birth on or
after 20 weeks gestation from all
maternity hospitals and home
births.
1st T combined serum and
NT was introduced in the
private sector only in 2000.
Comparisons focused on
the following years:
1992 – prenatal dx primarily
on basis of MA
1996 – introduction of 2nd T
MSS for all women in the
public sector
1998 – highest uptake of
prenatal dx
2002 – most current data
Two age groups
compared:
37 years and over at
expected date of delivery
36 years and younger at
expected date of delivery
Proportion of older women (≥ 37
years) giving birth:
1992=6.1%
1996=8.0%
1998=9.1%
2002=11.2%
Overall rate of IT (CVS or AC)(%,
95%CI)
1992=5.9% (5.8 – 6.1%)
1996=8.2% (7.9 – 8.4%)
1998=8.8% (8.6 – 9.1%)
2002=7.9% (7.7 – 8.1%)
Rate of IT for women 37 years or older:
1992=63.0% (61.5 – 64.5%)
1996=65.1% (63.7 – 66.4%)
1998=58.5% (57.2 – 59.8%)
2002=42.7% (41.5 – 43.8%)
Rate of IT for women 36 years or
younger:
1992=2.2% (2.1 – 2.3%)
1996=3.3% (3.1 – 3.4%)
1998=3.8% (3.7 – 4.0%)
2002=3.6% (3.4 – 3.7%)
Indications for invasive testing:
AMA alone decreased from 95.7% to
80.4% in older women, and from 62.2%
to 48.3% as a proportion of all tests.
The proportion of diagnostic tests
carried out in younger women with no
increased screening risk decreased
from 62.2% to 25.6%.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers Conclusions
High percentage of recruitment to the study.
Information about all births, IT rates in the state.
Applicable to a NZ setting.
Exact uptake of MSS was not reported but was
mentioned in the discussion as being less than 50%
over the period of the study, and approximately
46% in 2002.
149
Table 17.
Source
(Muggli and Halliday
2004)
Victoria, Australia
Retrospective analysis
of statewide datasets
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Sample
Screening Strategies
Outcomes
Results
As a proportion of all diagnostic tests it
decreased from 21.6% to 10.2%.
Overall increase from 6.9% to 35.4% of
all tests being prompted by an
abnormal screening result (either 2nd T
MSS or USS or both) between 1992 and
2002.
Level of evidence III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
150
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Wellesley et al. 2002)
N=155 501 women who
completed their pregnancies
between January 1994 and
December 1999.
Seven different screening
policies were used across
the eight districts. These
could be divided into 3
principle groups:
Wessex antenatally detected anomalies
register
Invasive procedure rates for each
district ranged from 2.8% to 7.7% from
1994 to 1999.
Group 1:
Serum screening offered to
all mothers:
AFP
fßhCG
1:250/1:300 cut-off = IT
offered
Routine scan at 16 or 12
weeks
Anomaly scan at 20 weeks
in one district
For 1998 only, the postcodes of women
who delivered in each district were
checked to make sure they were
allocated to the correct district.
Authors Conclusions
The authors found no evidence that serum and
NT screening improves the DRs or reduces rates
of invasive procedures. Across the region 15%
of pregnant women were aged ≥ 35 years
compared with the 5-7% assumed by modelling
studies of serum screening. Despite this high
proportion the rate of IT was only 5-7%, even in
districts that relied on MA screening. The authors
speculate that the proportion of women who
accept an offer of IT rises with increasing age
and risk.
In the districts offering routine MSS the uptake of
screening among older women was 40%, and
this has decreased progressively since it was
introduced in 1993. In these districts 40% of
women opted for direct AC and 20% declined
any test.
Wessex, England
Retrospective six year
survey (1994-1999)
Comparative audit
of screening in
adjacent health
districts to determine
whether serum
screening is justified
by an increase in DR
or a reduction in the
rate of invasive
procedures
Maternity units in
eight districts
7 different screening policies in the
8 districts.
Group 2:
MA main indication for IT
19-20 week anomaly scan
2 districts – 35 years and
over cut-off
1 district – 37 years and
over cut-off
Group 3:
IT offered to all women 35
years and over with
additional screening
offered.
NT was offered in one
district to all women and in
another to women aged ≥
34 years or by request in
younger women. A third
district provided a leaflet
with information about
private clinics offering NT
measurement and serum
screening.
An anomaly scan at 20
weeks was performed in all
3 districts.
One cytogenetics laboratory for the
region.
The district with an average of 2.8% IT
had the youngest maternal
population and the district with a
7.7% rate of IT had the oldest
maternal population.
IT rate per group:
Group 1: (MSS, anomaly scan in 1
district)
Average = 6.3% (range 5.9-6.7%)
Group 2: (MA + anomaly scan)
Average = 5.3% (range 4.2-6.8%)
Group 3: (MA + NT either to all
women, those ≥ 34 years or offered
privately + anomaly scan)
Average = 5.2% (range 2.8-7.7%)
Rates of IT are reported as an
average rate over the period of the
study (1994-1999), not separately for
each year.
Uptake of screening:
Group 1:
1993 = 85%
1999 = 55% in hospital A and 65% in
hospital B
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers Conclusions
The rates of IT for each district are difficult to
compare because even where districts had
similar screening policies, there were differences
in the age at which different services were
offered, the availability of services through the
public system, the age of the population, and
the uptake of screening options. For instance, in
the two districts offering MSS, the uptake of
screening was about 85% in 1993 but had
dropped to 55% in district A and 65% in district B
by 1999. Because the rates of IT are averaged
over the 6 year period of the study, it is difficult
to determine how the rates of IT changed with
decreases in the uptake of screening.
Age distribution of the population in each district
varied, which would have affected the offer of
IT (MA) and possibly uptake as well. The district
with the highest proportion of AMA women, had
the highest reported rate of IT and the district
with the lowest proportion of AMA women had
the lowest rate of IT.
Authors conclude that there was no difference
in rate of invasive testing between districts with
serum screening and districts without.
151
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Cheffins et al. 2000)
Women who had MSS between
1991 and 1996
AC and CVS offered to
women age 35 and older
since 1970’s.
Number of births
Overall proportion of pregnant women
undergoing IT (%age, 95% CI):
Total (AC + CVS)
1986 = 4.9% (4.6 – 5.2%)
1991 = 7.3% (6.9 – 7.6%)
1996 = 11.4% (10.9 – 11.8%)
Authors Conclusions
Against a background of increasing births to
women aged 35 years or older there was a
significant decrease in the birth rate of DS
following the introduction of MSS. There was an
increase from 7% to 84% of all women using a form
of prenatal testing (MSS/direct AC/CVS), with
approximately 7% using direct AC or CVS and 76%
using MSS. MSS availability has resulted in a large
proportion of women (approximately 83% of
younger women and 93% of older women in 1996)
having a prenatal test for DS, where previously
testing was rare.
South Australia (popn
1.48 million people,
20000 births per year)
Retrospective cohort
South Australian
Maternal Serum
Antenatal Screening
Programme (SAMSAS)
Level of evidence III-2
Women who had AC or CVS
between 1986 and 1996
Women who had births or
terminations of pregnancies with DS
between 1982 and 1996
Births to women ≥ 35 years:
1982 = 5.2%
1996 = 13.5%
SA prenatal screening policy
introduced in 1991:
AFP
uE3
alpha and beta subunits of
hCG
+ MA
Offered on a state-wide
basis in September 1992.
MSS well-established in
private sector by 1994 using
Amerlex-M, a three analyte
screen.
Risk cut-off for both tests was
1:405 (equal to the risk of a
woman aged 35 years at
delivery in South Australia).
At-risk women counseled
and offered AC for fetal
karyotyping.
Uptake of screening:
1991 = 17% (pilot
programme introduced)
1994 = 71% (Medicare
rebate introduced)
1996 = 76%
Higher in younger women (<
35) for all years.
Maternal
sociodemographic and
obstetric characteristics
Terminations performed
for DS
Numbers of screening
tests performed and
results of screening tests
AC rates by age
(provided by
Department of Chemical
Pathology, Women’s
and Children’s Hospital
who perform 80% of
tests).
Total AC and CVS rates
and indications.
Proportion of older women undergoing IT:
1986 = 51.0% (48.3 – 53.8%)
1991 = 52.8% (50.5 – 55.0%)
1996 = 53.8% (51.8 – 55.7%)
Proportion of younger women undergoing IT:
1986 = 1.7% (1.5 – 1.9%)
1991 = 2.6% (2.3 – 2.8%)
1996 = 4.8% (4.5 – 5.1%)
Indications for AC 1991 vs. 1996:
MSS increased from 9.5% to 35.7%
USS increased from 4.0% to 6.5%
MA decreased from 60.7% to 51.0%
Anxiety (< 35 yrs) decreased from 8.9% to
2.3%
Family history or past birth of birth defect
decreased from 7.1% to 2.3%
Proportion of women using direct AC (all
reasons except high risk MSS result):
1990: 5.3%
1996: 6.5%
Older women:
1990 = 42.1%
1996 = 40.1%
Younger women:
1990 = 1.8%
1996 = 1.2%
AC rates in screen +ve (high risk):
1491/1966=75.8%
<35 years = 80.3%
≥35 years = 65.0%
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
With the introduction of MSS the proportion of
women utilizing AC increased, particularly among
younger women, paralleling experience at other
centres. For younger women MSS offered a
chance for screening where none had been
offered before. For older women it provided an
opportunity to use a non-invasive test which might
indicate that AC is unnecessary. Counseling very
important prior to MSS, especially the informed
consent process. Counselling also required when
results of the screening are reported.
Reviewers Conclusions
High percentage of recruitment to the study.
Information about all births, IT rates in the state.
Applicable to a NZ setting. Women who screened
positive were told they had a 1 in 50 chance of
carrying a fetus with DS. One clinic performed 80%
of testing so high control over way testing carried
out but more information about how the results
were reported to mothers needed.
Still a high proportion of older mothers opting for
direct AC (all other indications except MSS), but it
is providing an option for older mothers who would
like to avoid AC. Prior to the introduction of testing
53% of older mothers had some form of prenatal
screening (AC or CVS) compared to 93% after (IT
or MSS).
152
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Zoppi et al. 2001)
Two groups of women referred for
prenatal diagnosis on the basis of
maternal age.
Group 1:
AMA
Acceptance of screening for
the NT group
Group 2:
NT at 10+3 – 13+6 weeks
Maternal choice of invasive
testing among the two groups
Group 1 (AMA alone)
690/982 = 70.2% (67.4 – 73.1)
underwent IT
CVS = 31% (27.6 – 34.5)
AC = 69% (65.5 – 72.4)
Authors conclusions
Knowledge of NT could lead to a decrease in the
demand for invasive diagnosis. Because
abnormalities are detected in the 1st trimester, this
might lead to a more frequent diagnosis by 1st T
transabdominal CVS for those undergoing IT.
One group presented to the
clinic before NT screening
had been introduced and
so were referred for testing
based on AMA alone. The
second group presented
when NT screening was
being offered between 10.3
and 13.6 weeks gestation.
Rate of diagnosis by CVS and
AC among the two groups
Prenatal diagnosis
clinic,
Italy
Group 1 (AMA alone)
N = 982
Retrospective cohort
Level of evidence III-2
Group 2 (AMA and NT)
N = 1386
1089 at appropriate gestational
age for NT screening
1088 accepted NT screen
NT offered at 10+3 – 13 +6 weeks
The age range of each group was
not reported. However the age
range of women accepting IT in
each group was:
Group 1
Median age = 38 (35 -46)
Group 2
Median age = 37 (35 – 48)
The two groups were both
given non-directive genetic
counseling, which included
information about maternal
and fetal risks associated
with AC and CVS (no PRL
ratios provided in the paper
but Tabor cited); techniques
and results; local
experiences and resources
by the same group of
geneticists.
221/982 = 22.5% (19.9 – 25.1) refused IT
68 miscarried before diagnosis and 3
terminated the pregnancies
Group 2 (AMA + NT)
1386 in total
1089 eligible for NT screen
1088/1089 accepted NT screen
Rates of uptake were reported in the
paper inclusive of the 297 women
who did not have NT measured
because they were outside the
gestational age range.
916/1386 = 66.1% (63.6 – 68.6)
underwent IT
CVS = 29% (26.1 – 32.0)
AC = 71% (68.0 – 73.9)
421/1386 = 30.4% (28.0 – 32.8) refused
IT
Rates of IT in women where NT was
measured:
848/1088 = 77.9% (75.5 – 80.4%)
Not possible to extract CVS and AC
data separately for this group.
47 women had a spontaneous
miscarriage and two terminated the
pregnancies prior to diagnosis
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
Not all of group 2 had NT measured as 297
women presented too late for the screen. Data
were available to calculate the rate of IT
excluding those women who presented after
13+6 weeks, and this showed a higher rate of IT
(77.9%) in the NT group compared to the AMA
group (70.2%).
The maternal and gestational ages of the two
groups were not reported, although the age
range of women in each group who opted for IT
was provided. However, the two original groups
of women may have presented at different
stages in pregnancy and, as uptake of IT can
vary as a function of gestational age, this may
have confounded the results (as may any
difference in age). The lack of information about
the age of the participants was a serious
limitation.
Potential cultural differences in the acceptability
of prenatal screening and diagnosis make the
results of this study less generalisable to other
settings. The design of this study gives an
indication of changes in the rate of testing
following the implementation of a new screening
policy, but a much longer follow-up period is
needed to get a real sense of the impact of any
change.
153
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
Shohat et al. (2003)
Prenatal screening policy
between 1990 and 2000:
Israel
N= 831,505 live births and 169,927
invasive tests performed between
1990 and 2000 in Israel.
Retrospective cohort review of nationally
collated databases
Births, numbers of invasive tests and
indications for IT in the Jewish
population in Israel from 1990-2000.
Data collected for whole
Israeli population but
findings reported
separately for Jewish and
non-Jewish women.
Level of evidence III-2
Data sources:
Demographic variables (maternal
age, ethnic origin, number of births
in Israel) obtained from the Central
Population Registry.
%age (95% CI)
Total IT rate in Israeli Jewish
population:
1990 = 11.3% (11.1 – 11.5)
1992 = 19.4% (19.1 – 19.6)
1994 = 23.8% (23.5 – 24.1)
1996 = 20.7% (20.4 – 20.9)
1998 = 20.3% (20.0 – 20.6)
2000 = 19.8% (19.6 – 20.1)
Authors conclusions
Between 1990 and 1995 there was an increase in
the number of invasive tests carried out and a
significant improvement in the percentage of DS
cases detected. This change in the use of invasive
testing seems to be the result of the introduction of
calculated DS risk based on MA and MSS.
Between 1995 and 2000, despite the introduction
of new methods for calculating DS risk (USS and
NT), there was no significant change in the rate of
invasive testing, which remains high compared to
other countries. Of interest is the difference
between the two age groups. While the uptake of
IT among women age less than 35 years was
almost the same between 1995 and 2000, the
uptake in women age ≥ 35 years declined from
61.6 – 48.3%. It may be that the introduction of
newer screening tests has increased anxiety in
younger women and helped older women decide
whether they require IT or not based on their
calculated risk of DS.
Live births data obtained from
National Registry for DS livebirths
Invasive testing data collected from
all 14 cytogenetic laboratories in
Israel and divided into 3 groups
based on indications:
• AMA (≥ 35 years)
• < 35 years with ≥ 1:386 risk of DS as
calculated by free 1st or 2nd T MSS
• low risk of DS who elected to have
IT.
1990-1992
2nd T triple screen introduced
(free of cost):
AFP
hCG
uE3
1992
14-16 weeks targeted USS
introduced (private, cost)
1996
NT with or without 1st T MSS
(PAPP-A + fßhCG (private,
cost)
Genetic counseling
available free of cost for
women with detected
abnormality or high risk DS
estimate
Invasive testing available
free of charge with following
indications:
≥ 35 years
≥1:386 risk of DS (at delivery)
based on age and MSS
Abnormal NT result (normally
>3mm)
IT available at cost for
women who request it
Total number of prenatal
tests
Utilization of screening
methods in 2000
DS cases detected
DS live births
Birth rate
IT rate per age group:
≥ 35 years
1990 = 66.5% (65.4 – 67.6)
1992 = 67.6% (66.5 – 68.6)
1994 = 62.2% (61.4 – 63.0)
1996 = 57.7% (56.9 – 58.5)
1998 = 51.9% (51.1 – 52.7)
2000 = 48.3% (47.6 – 49.1)
<35 years
1990 = 5.7% (5.5 – 5.8)
1992 = 14.0% (13.8 – 14.3)
1994 = 15.8% (15.5 – 16.1)
1996 = 13.4% (13.1 – 13.7)
1998 = 13.5% (13.3 – 13.8)
2000 = 13.8% (13.6 – 14.0)
Utilization of screening methods
(2000):
2nd T MSS = 60.9%
NT = 20.3%
USS (14-16 weeks) = 34.9%
Uptake of screening methods in 2000
measured using a maternal survey of
women in all maternity departments in
Israel on 1 day. Women also
questioned about IT, 2nd T marker test,
1st T MSS, USS (14-16 weeks), and NT
(10-13 weeks). 540 women
interviewed 70% Jewish
Proportion of women aged ≥ 35 years
old did not change significantly during
the study period (16.2 – 17.4%)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
Estimations of the uptake of prenatal screens were
calculated by interviewing women who gave birth
on a particular day in 2000. This doesn’t include
women who underwent screening but miscarried
or terminated pregnancies. It is likely that the
uptake of different screens would have changed
over the years. Without reliable data regarding
the use and uptake of screening methods, it is
difficult to determine how they might have
affected IT rates. Without indications for younger
and older women, it is difficult to determine why
rates of IT have changed in each group.
There are a very high number of nonrecommended invasive tests performed in Israel
(<1:386 risk) “most likely due to the social emphasis
placed on general health, and especially on the
health of children”. This suggests that cultural
differences in the acceptability of invasive testing
and disability may have influenced the rate of
invasive testing, making the results less
generalisable to other settings.
154
Table 17.
Source
Shohat et al. (2003)
Israel
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Sample
Screening Strategies
Outcomes
Results
Utilization of IT in the total Israeli
population was lower than that of the
Jewish population but showed the
same overall pattern.
Retrospective cohort review of nationally
collated databases
Level of evidence III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Comments
155
Table 17.
Evidence table of primary research studies appraised investigating the rate of invasive testing with the introduction of a screening programme
(continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
Smith-Bindman (2003)
N= 5,980,519 pregnancies in
England and Wales between 1989
and 1999
England and Wales divided
into 26 geographical areas
and the combination of
geographic area and year
(area-years) was the unit of
analysis for all comparisons
Total number of invasive
tests
Percentage (95% CI) of pregnancies
undergoing IT:
1989 = 4.4% (4.3 – 4.4)
1991 = 5.0% (4.9 – 5.0)
1993 = 5.7% (5.6 – 5.7)
1995 = 6.1% (6.1 – 6.2)
1997 = 6.4% (6.4 – 6.5)
1999 = 5.8% (5.8 – 5.9)
Authors conclusions
The current analysis has several limitations. NEQAS
estimates of the number of IT included some
duplicates and some tests for other conditions but
these are likely to be a very small percentage of
the total. Our proxy measure assumes that the
patterns of screening for diagnosed cases are a
reliable reflection of referral patterns; the analysis
in 2 geographic areas showed a close correlation
between the 2 measures (0.7). However the
categorization of area-years by their dominant
screening method will tend to underestimate the
differences between the screening methods
because our characterization of screening
patterns based only on DS cases almost certainly
overestimated the use of serum and US screening.
Additionally each area-year includes a mixture of
screening methods which accounts for some of
the variability in outcomes within each screening
category and might have limited our ability to
differentiate between the performance of USS and
serum screening. NT and 2nd T anomaly screens
combined. Lower number of ITs per case
detected when serum or USS used versus AMA.
England, and Wales
Retrospective cohort review of nationally
collated databases
Level of evidence III-2
Data sources:
National Office of Statistics
annual births, terminations
and stillbirths
annual maternal age-specific
population births for each
health authority
National DS cytogenetic register
(NDSCR)
UK national external quality
assessment scheme (UKNEQAS)
- annual audit of all cytogenetics
laboratories
Information on the dominant
method of screening for
each area-year and
invasive testing information
was linked.
Each area-year was
classified on the basis of the
dominant screening method
used for prenatal diagnosis
of DS cases.
1) Serum
2) ultrasound (1st or 2nd T)
3) AMA
4) mixed – no dominant
method
Rate of invasive testing per
year
Utilization of screening
methods per area-year
Total = 5.6% (5.6 – 5.6)
IT per DS case detected:
Serum = 60.7 (56.6-64.8)
USS = 52.0 (43.8 – 64.8)
AMA = 88.0 (80.1 – 95.9)
A general policy of offering invasive testing on
AMA alone is not justified.
Reviewers conclusions
Design of study measures number of ITs per case
detected for area-years. Authors acknowledge
that within each area-year there is variation in the
offering and uptake of each method of screening.
The design is therefore unable to indicate how
invasive testing rates change with the introduction
of screening because the screening policy for
each year was not consistent across England and
Wales and the percentage of invasive tests for
each area-year are not reported, just the number
of ITs per case detected.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
156
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
157
Chapter 7: Uptake of testing
following screening results
The search identified 18 eligible papers examining the uptake of invasive testing following positive or
negative screening results. Below is an overview of study designs and aspects of quality represented
by these studies. Full details of the 18 papers appraised, including methods, key results, limitations and
conclusions, are provided in evidence Table 21 (pages 166-184).
Study settings and samples
Of the 18 papers appraised, seven were reviews of multi-centre community-based screening
programmes and 11 were single centre studies set in hospitals or clinics. Of the 11 single centre
studies, eight were prospective cohorts and three were retrospective reviews of medical records (Marini
et al. 2002; de la Vega et al. 2002; Michailidis et al. 2001). Of the seven reviews of community-based
screening programmes, three were retrospective analyses of data collected prospectively as part of the
screening programme (Hadlow et al. 2005; Mueller et al. 2005; Chen et al. 2000), one was a
retrospective analysis of a large perinatal survey (Khoshnood et al. 2003) and three were prospective
studies which collected information from contributing hospitals or diagnostic centres (Platt et al. 2004;
Wald et al. 2003a; Saltvedt et al. 2005).
All seven of the multi-centre reviews of screening programmes included women of all maternal ages,
and sample sizes ranged from 8216- 308,000 screened women, of whom 403 - 16,792 had screen
positive results. One of these studies (Chen et al. 2000) did not report the number of women who were
screened as the study reviewed the records of screen positive women only. Of the 11 single centre
studies, four included women of all maternal ages, six examined the rates of invasive testing among
women of AMA only (≥ 35 years - Lam et al. 2000; Ilgin-Ruhi et al. 2005; Vergani et al. 2002; ≥ 38
years – Dommergues et al. 2001; Marini et al. 2002) or younger women (< 38 years - Audibert et al.
2001) and one did not report the age distribution of the sample.
Study design and quality
Reviews of community-based screening programmes
Khoshnood et al. (2003) used data from the National Perinatal Survey which collected information on
all births in a one week period in France (National Perinatal Survey, 1988). The sample was large
(n=13,478) however a number of women had missing data on either amniocentesis or serum screening
(n=1152) and were excluded from analyses. Women were divided into four age groups (<30, 30-34,
35-37, ≥ 38 years) and approximately 10% were aged ≥ 35 years. Because data were collected via a
retrospective interview, it could be subject to recall bias and this coupled with the proportion of
missing data makes it difficult to interpret the findings.
Chen et al. (2000) utilised the databases of a cytogenetics laboratory in Connecticut, USA and
retrospectively reviewed the records of almost 50,000 women who were referred to the laboratory for
second trimester MSS screening (AFP, hCG, uE3). Screening was offered to all women regardless of
age, the median age of the screened women was 27.5 years and 10.3% of the population were 35 years
or older at delivery. Women with a high risk result (1:270 or more) were offered invasive testing
(n=2879) and the uptake rates were reported as a function of risk estimate, maternal age, gestational
age, ethnicity and year of testing. Unfortunately amniocentesis information was not available for 10%
of the screened sample but these women were included in analyses and assumed not to have had
invasive testing. While this study was carried out retrospectively, the data sources were robust and
missing data were dealt with appropriately. Results of screening were reported back to women via their
practitioners and it is likely there was variation in the information they were provided regarding the
implications of their risk estimate and the risks involved with invasive testing. However, this provides a
more accurate reflection of the realities of community testing programmes. What is of more concern,
and was acknowledged by the authors, is that they cannot be certain that all screen positive women
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
158
were offered invasive testing. The population source, age distribution and size make the study results
applicable to other settings.
Platt et al. (2004) utilised a multi-centre prospective cohort of women undergoing sequential first and
second trimester screening for DS. First trimester serum (PAPP-A, fßhCG), NT and MA were collected
with all screen positive (≥1:270 cut-off) women and women aged 35 years or older offered invasive
testing. All women were offered second trimester serum screening (AFP, total hCG, uE3 + MA) and
high risk women (≥ 1:270 cut-off) were offered invasive testing. Rates of invasive testing were
reported for three groups of women: screen positive after first trimester screening; screen positive after
second trimester screening; low risk for both screens. The age distribution of the entire sample was not
reported in this paper, however approximately 39% of women who had both first and second trimester
screening were aged ≥ 35 years.
Saltvedt et al. (2005) randomly assigned women participating in the NUPP trial to receive either a scan
at 12-14 weeks gestation (12 week group) which included a measure of NT, or a scan at 15-20 weeks
(18 week group). Women in the 12 week group were offered prenatal diagnosis on the basis of NT and
women in the 18 week group were offered prenatal diagnosis primarily on the basis of maternal age (≥
35 years). The trial also evaluated the performance of the screening test in the detection of DS cases.
Almost 40,000 women from 8 maternity hospitals were included in the trial which was conducted over
a 3 year period in Sweden. The authors’ main concern was that the screening policies in each group
had not been adhered to strictly. Approximately 9% of women in the 12 week scan group did not have
NT measurements recorded and a small proportion of women in both groups requested and received
second trimester maternal serum screening. However, the authors also noted that this reflected the
realities of community-based screening.
Hadlow et al. (2005) conducted a retrospective audit of a first trimester community screening
programme in Western Australia, including analyses of the uptake of invasive testing in screen positive
women. Screening and cytogenetic records for 10,480 women who completed first trimester screening
based on the combined test were examined. High risk women (≥ 1:300 risk) were offered prenatal
diagnosis in consultation with their doctor. The proportion of acceptance of invasive testing was
reported for screen positive and screen negative women and some results were available for different
levels of estimated risk. The mean age of the sample was 30.7 years with 21% of women aged 35
years or older. There was a minimal loss to follow-up because Western Australia has a stable
population base and well-established state-wide data collection methods. All FMF accredited
sonologists and cytogenetic laboratories in WA agreed to provide information, suggesting the data
were complete. The authors acknowledged however, that they did not have information about the
number of women who were not screened because of technical difficulty, multiple pregnancy, or
gestational age.
Mueller et al. (2005) reported the rates of amniocentesis in women who were screened as part of the
Ontario MSS programme between 1993 and 1998. The Ontario MSS programme was a large
community-based programme which screened more than 300,000 women for DS risk using the triple
test (AFP, uE3, hCG) and maternal age. About half the pregnant population in Ontario opted for
screening and over 21,000 women screened positive (≥ 1:385 risk at term). (Mueller et al. 2005)
reported that amniocentesis information was not available for 23% of women who were excluded from
analyses, potentially producing biased estimates. AC uptake in relation to age, risk estimate and the
interaction between age and risk was reported for the 77% of screen positive women who did have
follow-up information about amniocentesis. The study provides an indication of the uptake of
amniocentesis following screening in a community-based programme, but the high proportion of
women lost to follow-up is of concern and decreases the validity of the findings.
Wald et al. (2003a) prospectively collected information from 46,000 women screened for DS risk using
the quadruple test (AFP, uE3, hCG, inhibin-A) and maternal age at term. This study was based in 14
hospitals in the UK between 1996 and 2001. There were 3271 women who screened positive (≥ 1:300)
and uptake of amniocentesis relative to risk estimate was reported.
Single centre cohort studies
Nicolaides et al. (2005) collected information from women who attended a private prenatal assessment
clinic between 1999 and 2003. More than 30,000 women were screened in the first trimester (11-13+6
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
159
weeks) for DS risk using the combined test (NT, free ßhCG, PAPP-A + maternal age). The median age
was 34 years with a high proportion of women (48.5%) aged 35 years or greater. Uptake of invasive
testing was reported for screen-positive (risk of ≥ 1:300) and screen-negative women, as well as for
each risk estimate group. While the design and description of the study are of good quality, the sample
may not be representative in that it consisted of women who presented early in their pregnancy to a
private clinic and their socioeconomic status may have been higher than the general population. High
quality information was available regarding risk estimates, maternal age, and the uptake of invasive
testing.
Michailidis et al. (2001) examined the uptake of invasive testing in 8536 women who screened positive
by either first trimester NT screening or second trimester maternal serum screening based on two
analytes. Complete outcome data were not available for 13% of the original sample so 7447 women
were included in the final analyses. NT measurements were completed at 10-14 weeks gestation and
women were informed of their results and offered prenatal diagnosis if they were above the 99th centile
or the screen showed structural abnormalities. There was not enough information presented in the
paper to ascertain whether the women who did not have second trimester screening refused screening,
were lost to follow-up, or did not continue their pregnancy into the second trimester because of
spontaneous miscarriage or termination.
Ilgin-Ruhi et al. (2005) conducted a prospective study of the uptake of screening and invasive testing
following screening results in women who presented at the authors’ clinic for prenatal diagnosis on the
basis of maternal age (35 years or older). Women were initially offered second trimester MSS (AFP,
hCG, uE3) with a high risk cut-off of 1:250. Uptake of invasive testing was reported for those who
declined screening, screen positive and screen negative women. The sample was relatively small and
the study was based in Turkey, making it more difficult to generalise these results to other settings.
A study by de la Vega et al. (2002) presents the same difficulties in sample size (n=555 screen positive
women), and a lack of generalisability because of potential cultural differences in the acceptability of
both screening and invasive testing. In this study, the medical records of Hispanic women who
presented to a high risk prenatal clinic in Puerto Rico were retrospectively reviewed. Women who had
tested screen positive for DS (> 1:250) were included in the study and were grouped based on their
indication for prenatal diagnosis. Women with more than one risk factor were excluded from the study
and the uptake of amniocentesis was reported for each group. The description of the methodology was
not detailed enough to ascertain what options women were offered following screening, what invasive
testing risks they were informed of, and what they were told about their individual risk for DS. The
age distribution of the sample and how many women were excluded because of multiple indications for
prenatal diagnosis was not reported. It was also not indicated whether grouping of women based on
their indications was blind to their invasive testing decision.
Spencer et al. (2000b) reported on the uptake of invasive testing in a prospective cohort of women who
presented for maternity care between 10 and 13+6 weeks GA at a maternity unit in Essex, England.
Women (n=4190) were given the option of first trimester screening using a combination of MSS (free ß
hCG + PAPP-A) and NT. The rate of invasive testing in screen positive women (n=253) was reported
overall and relative to risk estimate. Exact figures for uptake relative to risk estimate were not reported
and confidence intervals were unable to be calculated. The methods section was detailed and thorough
with the median age of the sample being 29 years and 6.1% of the sample aged ≥ 35 years.
Vergani et al. (2002) reported the rate of amniocentesis in 1486 women who underwent genetic
counselling on the basis of maternal age (≥ 35 years) at a maternity clinic in Italy. Data were collected
prospectively between 1990 and 1998. Women were initially seen at 10 - 14 weeks GA and were
counselled regarding their risk for DS and screening options. Women were offered an USS including
NT measurement and their attitudes to amniocentesis (in favour/against) were measured. Rates of
uptake were reported relative to ultrasound findings and women’s a priori preferences for/against
invasive testing. Potential cultural differences with regard to the acceptance of both screening and
invasive testing make the results of this study less generalisable to other settings.
O’Connell et al. (2000) reviewed the clinic and cytogenetic records of almost 19,000 women who
booked for first trimester assessment between May 1992 and April 1997 at Hull Maternity Hospital,
England. Women were screened for DS risk using the triple test (AFP, uE3, total hCG or free ßhCG).
Amniocentesis was available on request prior to serum testing but was not routinely offered on the
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
160
basis of maternal age. Women with a high risk result (1:250 or more) were informed of their options,
including invasive testing, by a consultant. Rates of invasive testing in screen positive, screen negative
and unscreened women were reported. While the rest of the study was adequately reported, no
information was provided about the age distribution of the sample, making it difficult to determine how
representative the sample was, and how generalisable the findings might be. Standardised information
was provided to women prior to testing but there was not enough detail in the study to know how
women were informed of their results after testing. Free ß hCG replaced total hCG in the screen from
May 1994 - April 1997. There was subsequently an increase in the proportion of screen positive
women and there may have been a change in the uptake of invasive testing, however rates of
acceptance were not reported separately for these two variations of the serum test.
Lam et al. (2000) conducted a prospective cohort study to examine the uptake of screening and the rate
of invasive testing in women of AMA (≥ 35 years). This study was based in Hong Kong between 1997
and 1999 and followed 3,419 women who reported for prenatal diagnosis on the basis of maternal age.
The authors standardised the information presented to women regarding screening and invasive testing
by including a video presentation and written information in the consultation. At the consultation
women were offered serum screening (AFP + total hCG) as an alternative to direct IT and screen
positive women (1:250 or greater risk) were offered amniocentesis. Amniocentesis was offered to
screen negative women if requested. Women who refused any screening or prenatal diagnosis were
excluded from the study. The sample was predominantly of Chinese ethnic origin (91%) and the
authors found that uptake varied as a function of ethnicity, making it difficult to generalise the findings
to other settings. The standardised and well-controlled nature of the screening and invasive testing
information presented to women may not reflect what would normally happen in clinical practice,
although it does represent an ideal situation. The number of women who refused any screening or
prenatal diagnosis was not reported, making it difficult to determine what proportion of the population
initially approached agreed to take part in the study.
Dommergues et al. (2001) conducted a prospective cohort study of the uptake of invasive testing in
women of AMA (38-47 years) following first and second trimester screening using a combination of
NT and MSS (AFP + hCG). A NT screen was performed at 10-14 weeks, MSS at 15-17 weeks and an
USS at 21-23 weeks. Women who were designated to be high risk on the basis of either their NT (≥
3mm) or MSS (≥ 1:250) or an abnormal USS were recommended to have an amniocentesis while low
risk women were given the option of no amniocentesis. MSS was performed in all women regardless
of their NT result. The rates of uptake of invasive testing were reported for screen positive and screen
negative women, as well as for each combination of screening results (both NT and MSS +ve; NT ve/MSS +ve; NT +ve/MSS -ve; both NT and MSS -ve). The sample was small (n=359) and was
restricted to women of AMA in France, where the DS screening policy offers direct AC to women aged
38 years and over, a little older than the age 35 years cut-off in many other countries. However,
Audibert et al. (2001) reported the results for women less than 38 years old in the same population.
The mean age of this sample was 30 years with 14% aged 35 - 37 years of age. The uptake of invasive
testing was reported for screen positive and screen negative women and for each combination of risk
group.
Marini et al. (2002) reviewed the records of a cytogenetics laboratory to examine the screening results
and subsequent decision to accept or decline invasive testing in women aged 35 years or older.
Women were included in the study if they had been screened for DS risk using the 2nd trimester triple
test (AFP, uE3, βhCG). A calculated risk of 1:270 or greater was considered screen positive. The rate
of invasive testing in screen positive and screen negative women was reported. As this study was a
retrospective review of laboratory records it relied on an assumption that the laboratory records were
accurate.
Study results
Of the eighteen studies included in this part of the review, 11 were prospective cohort studies and
seven were retrospective reviews of previously collected records.
The screening strategies employed by the studies included reviews of the uptake of invasive testing
following screening by first trimester methods (MSS + NT/NT alone, n = 4), second trimester methods
(triple = 5; quad=1; NT = 2; double = 1), or a combination of first and second trimester methods (n=4).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
161
One study reviewed the records of women who had been screened for DS risk using a variety of
methods (de la Vega et al. 2002).
Uptake of invasive testing following 1st trimester screening
Four studies examined the rates of invasive testing following results of 1st trimester screening (see
Table 18). Three of these studies utilised NT measurements in combination with maternal serum
markers, one utilized NT alone and all four included women of all maternal ages.
One of these studies was a review of a community-based screening programme. Hadlow et al. (2005)
reported a 62% uptake of invasive testing in screen positive women and a 2.7% uptake in screen
negative women. The rate of invasive testing increased with an increase in estimated risk of DS from
75.8% with a risk of ≥1:100 to 88.3% with a risk of ≥ 1:50.
Three further studies reported on the rates of invasive testing in hospital or clinic settings. Two studies
followed singleton pregnancies and reported 78 - 82% rate of uptake in screen positive women
(Nicolaides et al. 2005; Spencer et al. 2000b). Nicolaides et al. also reported that 4.6% of screen
negative women opted for invasive testing and that uptake rates varied as a function of age, with a
higher proportion of older women (7.4%) than younger women (2.2%) opting for invasive testing
following negative screening results. Saltvedt et al. (2005) compared the uptake of invasive testing in
women screened as high risk using either a 12 week scan including NT or an 18 week anomaly scan.
The results indicated that overall fewer women in the 12 week scan group (8%) underwent invasive
testing compared to women in the 18 week scan group (11%, p < 0.001). When the uptake of invasive
testing was examined in screen positive women, the findings indicated that 73% of women with high
risk NT measurements opted for invasive testing. In the 18 week scan group 52% of women ≥ 35 years
opted for invasive testing.
Table 18.
Uptake of invasive testing following 1st trimester screening
Reference
Maternal Age of
Sample
Uptake following positive screening
result (%, 95% CI’s)
Hadlow et al.
(2005)
Mean = 30.7
years
overall = 62
<25 - ≥ 35 years
Spencer et al.
(2000b)
Mean = 29 years
Saltvedt et al.
(2005)
Nicolaides et al.
(2005)
(57-67)
Uptake following a negative
screening result
<1:300 = 2.7
(2.4-3.0)
Overall = 4.6%
(4.3-4.8)
≥ 1:100 = 75.8
≥ 1:50 = 88.3
≥ 1:300= 81.8
(77.1 – 86.6)
Median = 30.1
years
12 week group = 73.4
(69.9 – 77.0)
18 week group = 51.7
(50.0 – 53.4)
Median = 34
years
1:1 - 1:150=~85
Range = 15-49
years
1:300-1:500~20
≥ 35 = 12.7%
1:151 to 1:300=~65
≥ 35 = 76.2
(74.4 – 78.1)
≥ 35 = 7.4
(6.9 – 7.8)
< 35 = 82.5
(79.4 – 85.6)
< 35 = 2.2
(2.0 – 2.5)
Uptake of invasive testing following 2nd trimester screening
Nine studies (Table 19) reported the rates of uptake of invasive testing in women who were screened
using 2nd trimester screening methods (triple=5; quad=1; NT = 2; double = 1). In five studies women
were screened with the triple test (AFP, hCG, uE3) and rates of uptake ranged from 36 - 85% following
a screen positive result, and 0.05 - 42% following screen negative results. Two of these were large
reviews of screening programmes (Mueller et al. 2005; Chen et al. 2000) and found an increase in
uptake of invasive testing with an increase in estimated DS risk. Both of these studies also found a
higher uptake of invasive testing in women < 35 years of age compared to women of AMA.
Wald et al. (2003a) found a 60% overall uptake of invasive testing in women screened with the
quadruple test (AFP, hCG, uE3, inhibin-A) and that uptake increased with increasing risk estimate.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
162
Lam et al. (2000) reported the rates of invasive testing in an AMA population screened with the double
test (AFP, total hCG) finding 60.9% of screen positive women, 5.3% of screen negative women, and
47.1% of women who opted for no testing, chose invasive prenatal diagnosis. Marini et al. (2002)
examined the records of AMA women (≥ 35 years) who underwent second trimester maternal serum
screening at the authors’ cytogenetics laboratory over a 6 year period. Of screen positive women, 48%
accepted the offer of invasive testing, while in the screen-negative group, 13% opted for invasive
testing. Khoshnood et al. (2003) used data from the National Perinatal Survey which collected
information on all births in a one week period in France in 1998 and found an increase in uptake of
invasive testing with maternal age and education. Vergani et al. (2002) found that 36% of screen
positive and 31% of screen negative women over the age of 35 years opted for invasive testing
following the results of NT screening.
Of the studies which examined 2nd trimester screening methods, three (Ilgin-Ruhi et al. 2005; Lam et
al. 2000; Vergani et al. 2002) were subject to possible bias in the cultural acceptability of both
screening and invasive testing. These studies were set in Turkey, Hong Kong and Italy and the public
acceptability of screening and prenatal diagnosis in these societies might have affected the uptake of
screening and/or invasive testing following screening results, making the findings less generalisable to
other settings. One study (Khoshnood et al. 2003) was subject to recall bias because the data were
collected via a retrospective maternal interview and screening or invasive testing data were missing for
8% of the sample. All three of the studies reviewing screening programmes (Mueller et al. 2005; Wald
et al. 2003a; Chen et al. 2000) noted an increase in uptake of invasive testing with an increase in
estimated DS risk. Two of these also examined uptake relative to maternal age and found that among
screen positive women, a higher proportion of younger women than older women opted for invasive
testing, although the difference between the two groups was less than 10%.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
163
Table 19.
Uptake of invasive testing following 2nd trimester screening
Reference
Maternal Age of
Sample
Uptake following positive screening
result (%, 95% CI’s)
Uptake following a negative
screening result (%, 95%
CI’s)
O’Connell et al.
2000
Mueller et al. 2005
Not included
85
0.05
(0.01 – 0.09)
Mean = 34 years
Range = 15-50
years
Overall = 65.7
Chen et al. 2000
Wald et al. 2003a
Mean = 27.5
years
Range = 13-48
years
All maternal ages
Distribution not
reported.
>1:100 = 73.3
1:100-1:149 = 69.1
1:150-1:199 = 67.7
1:200-1:249 = 63.4
1:250-1:299 = 62.8
1:300-1:385 = 58.6
Overall = 52
1:1 to 1:10 = 72.2
1:11 to 1:30 = 57.6
1:31 to 1:60 = 61.4
1:61 to 1:134 = 55.1
1:135 to 1:270 = 47.7
Overall = 60
(82-88)
(71.9 – 74.7)
(67.1 – 71.0)
(65.8 – 69.6)
(61.4 – 65.4)
(60.8 – 64.7)
(57.1 – 60.1)
(60.3 – 84.2)
(49.3 – 65.8)
(55.5 – 67.2)
(51.7 – 58.4)
(45.3 – 50.2)
Relative to DS risk:
>1:50 = 74.5
1:250-1:300 = 43.1
(67.3 – 81.7)
(38.8 – 47.5)
60.9
(55.4 – 66.4)
5.3
(4.2– .4)
48%
(44.7 – 51.4)
12.9
(11.2-14.5)
Khoshnood et al.
2003
Range = 35-47
years
Maternal age
range:
Less than 30 –
38 and older
Education level:
>12 years = 13.6
</=12 years = 9.5
(12.6-14.5)
(8.9-10.2)
Vergani et al.
2002
≥ 35 years only
Mean = 38.9
36
Ilgin-Ruhi et al.
2005
≥ 35 years only
Mean=38.2
75
Lam et al. 2000
Marini et al. 2002
Uptake
following no
screening (%,
95% CI’s)
1.8 (1.4-2.3)
≥ 35 years only
47.1 (45.5 –
48.8)
35 – 37 year olds
with >12 years
education = 51%
≥ 38 years =
81.7%
31
32.9 – 50.8
42
(68.9 – 81.6)
73.3 (60.4 –
86.3)
Uptake of invasive testing following 1st and 2nd trimester screening
Four studies reported the rates of uptake of invasive testing in women who were screened using a
combination of 1st and 2nd trimester screening methods (Table 20). Dommergues et al. (2001) and
Audibert et al. (2001) reviewed the results of women from the same screening cohort but reported on
different age groups. Women were screened using NT in the 1st trimester followed by MSS in the 2nd
trimester, with results available to women after MSS. MSS was performed in all women regardless of
their NT result. The uptake of invasive testing was 59% following a positive NT or MSS result in
women <38 and 81% in women ≥ 38 years of age. In both age groups the uptake of invasive testing
varied depending on the source of the positive result. Younger women were more likely to opt for
screening after NT (71%) than MSS (48%) while older women showed a 79% uptake with a positive
MSS result and 71% with a positive NT result. In both age groups there was 100% uptake of invasive
testing when both NT and MSS results were above the cut-off. Among younger screen negative
women, 4.7% opted for invasive testing, whereas 53% of older screen negative women opted for
invasive testing.
Michailidis et al. (2001) examined the uptake of invasive testing in 8536 women who screened positive
by either first trimester NT screening or second trimester maternal serum screening based on two
analytes. NT measurements were completed at 10-14 weeks gestation and women were informed of
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
164
their results and offered prenatal diagnosis if they were above the 99th centile or the screen showed
structural abnormalities. Of the 122 women who screened positive in the first trimester, 105 (86.1%)
opted for invasive testing. Of the remaining 7325 women, 4864 (66%) were screened in the 2nd
trimester for AFP and free ßhCG levels. Of the women who did undergo 2nd trimester screening,
44.5% of screen positive women opted for invasive testing, with an overall invasive testing rate in
screen positive women of 53.7%. The mean maternal age in this population was 30.1 years with 21%
of the sample aged 35 years and over, suggesting that it may not reflect the age distribution in the
general population. The prevalence of DS in the 2nd trimester screening sample was 0.08%, suggesting
it may have been comprised of women who were mostly at low risk of DS and possibly explaining the
lower uptake of invasive testing.
Platt et al. (2004) investigated the uptake of invasive screening in women who were screened in the 1st
trimester using NT and maternal serum levels and in the second trimester using the triple serum test.
First trimester results were disclosed to women prior to offering a choice of invasive testing, second
trimester testing or no further screening or diagnosis. A small number of women were screen positive
in the first and second trimesters, of whom 40.5% accepted invasive testing. 57.1% of women who
were screen positive in the first trimester and 44.4% of women who screened positive in the second
trimester accepted invasive testing, and 5.1% of women who were negative for both screens opted for
invasive testing. A higher proportion of older women (8.3%) than younger women (3.5%) in this
group opted for invasive testing.
Table 20.
Uptake of invasive testing following 1st and 2nd trimester screening
Reference
Audibert et al.
(2001)
Dommergues et
al. (2001)
Platt et al. (2004)
Michailidis et al.
(2001)
Maternal Age of
Sample
Mean = 30.1
years
< 38 years
Range = 38-47
years
All ages included
Distribution not
reported
Mean maternal
age = 30.1 years
(range 13 – 50)
Uptake following positive screening
result (%, 95% CI)
59
(52.1 – 65.3)
Uptake following a negative
screening result (%, 95% CI)
NT –ve, MSS –ve= 4.7 (4.0-5.3)
81
(74 - 88)
NT –ve, MSS –ve = 53
(46.8– 59.7)
1st T screen:
+ve: = 57.1
-ve = 15.3
(53.7 – 60.5)
(14.5 – 16.2)
Negative both screens
= 5.1
(4.4 – 5.8)
≥ 35 years = 8.3
< 35 years = 3.5
(6.8 – 9.8)
(2.8 – 4.3)
2nd T screen:
+ve both screens
= 40.5
1st T –ve/2nd T +ve=
44.4
1st T screen= 86.1
(29.4 – 51.7)
2nd T screen= 44.5
(39.7 – 49.2)
(39.3 – 49.4)
(79.9 – 92.2)
Summary of results
The variability in screening methods, age of the participants, setting of the studies, method of analyses,
and reporting of risk estimates utilised by the 18 appraised studies makes a comparison of the rates of
uptake difficult. While it is not possible to report an accurate overall proportion of uptake for screen
positive and screen negative women, there were two key trends in levels of uptake.
Maternal age appears to be an influential factor in the uptake of invasive testing. Four studies included
maternal age as a factor in their analyses, however, two studies reported a higher uptake of invasive
testing in older women (≥ 35 years) and two a higher uptake in younger women. Some of the
variability in these findings may be due to their setting as one of these studies was set in a private
prenatal testing clinic (Nicolaides et al. 2005), two were large reviews of community screening
programmes (Mueller et al. 2005; Chen et al. 2000) and one was based on findings from a maternal
survey (Khoshnood et al. 2003). In the smaller single-centre studies women were provided with
intensive and standardised counselling regarding the implications of their individual risk estimates and
the risks involved with prenatal testing, however, this is not reflective of the realities of communitybased screening.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
165
The individual level of risk estimate appears to influence women’s decisions regarding the uptake of
invasive testing. Five studies included exact risk estimates as a factor in their analyses with all five
reporting that as the calculated risk estimate and, therefore, the likelihood of carrying a DS fetus
increased, the proportion of women opting for invasive testing increased. Four of these studies were a
combination of large multi-centre evaluations of community screening programmes with a fifth set in a
single centre. In three of the studies women were screened using 2nd trimester methods and in two
studies 1st trimester methods. The effect of risk estimate appears to be fairly consistent and robust.
Three of these studies were able to examine the effect of risk estimate for each age group. All three of
these found a higher uptake of invasive testing among younger versus older screen positive women.
Conclusions
The decision whether to opt for a potentially risky invasive diagnosis following screening results is
obviously a very complex one. It appears that both maternal age and the individual calculated risk
estimate are factors in women’s decision-making but it is probable that many other factors also play a
role. The perceived accuracy of the test may be influential as uptake did vary, although not
predictably, depending on the method of screening used. This is probably in part related to the
gestational age of the fetus. Younger women and older women may be using screening for different
purposes. Younger women may not perceive themselves to be at risk so a negative screening result is
enough to reassure them and deter them from opting for an invasive test. In older mothers, who are
aware of the age-related risk of Down syndrome, the screening may be used as a way of avoiding
invasive testing. A higher proportion of these women decline invasive testing after receiving a positive
screening result, particularly one close to the cut-off.
Social, cultural, religious and ethnic factors may also influence the acceptability of both screening and
invasive testing but this again was not consistent across studies. In some cultures, dominant religious
beliefs may make termination of the pregnancy unacceptable, and lessen the demand for invasive
testing. In other cultures where population growth is high and families are limited in the number of
children they produce, the uptake of invasive testing and prenatal diagnosis may be higher. Because of
this cultural variability it would be wise to conduct a local study of the acceptability of screening and
invasive testing before implementing a large-scale screening programme. Both older and younger
women and women from different ethnic backgrounds should be included in the study, and consistency
in the quality of counselling regarding individual risk estimates and the implications of a positive or
negative diagnosis monitored. It would be very difficult to maintain consistency across all
practitioners; however, standardised information packs for both practitioners and patients might
increase the quality of pre-screen and post-screen counselling.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
166
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Hadlow et al.
2005)
N= 10480 women who
completed FTS in Western
Australia during the two year
period of the audit
1st T screening:
NT 11-14 weeks GA (FMF
protocol) plus
MSS based on free ßhCG
and PAPP-A
No risk reported on MA +
MSS alone
Numbers of screen +ve
women (≥ 1:300 risk)
Numbers of screen -ve
women (<1:300 risk)
%age (95% CI)
Proportion of screen +ve women:
403/10436 = 3.9% (3.5-4.3%)
Authors conclusions
Authors comment on the stable population base so
minimal loss to follow-up, small number of laboratories
who all cooperated, and well-established state-wide
data collection methods.
Western Australia
(25,000 annual
births)
Community-based
first trimester
screening
programme
Retrospective
cohort (audit of a
screening
programme)
Level of evidence
III-2
Age distribution:
Mean age = 30.7 years
<25 years, 9.5%
25-29 years, 29.4%
30-34 years, 39.9%
35+ years, 21.2%
Different from general
population demographics
Risk reported to woman
and referring doctor.
Prenatal dx offered in
liaison with doctor if risk of
1:300 or more.
Percentage in each
group accepting or
declining diagnostic
testing
Uptake of IT:
Screen positive (≥ 1:300 risk)
250/403 = 62% (57-67%)
Screen negative (< 1:300 risk)
271/10033 = 2.7% (2.4 – 3.0%)
By risk group
≥ 1:100 = 75.8%
≥ 1:50 = 88.3%
Median GA=12 weeks 3 days
Full pathology records available
for 10 436 women (99.6%) and
full birth or pregnancy
termination records were
available for 10 274 women
(98.4%).
USS performed in multiple community sites because
1st T screening coordinated over a very wide
geographical area. However the USS examinations
were performed or supervised by 4 experienced and
accredited sonologists.
The rate of diagnostic testing (CVS/AC) in the high
risk group (risk 1:300 or higher) was 62%. The rate of
diagnostic testing in the low risk group was 2.7%. The
likelihood of diagnostic testing increased with level of
risk, with 75.8% of women with a risk of ≥ 1:100 and
88.3% of women with a risk ≥ 1:50 proceeding to
testing.
Reviewers conclusions
Risks were reported to women and their doctors and
a decision regarding diagnostic testing made in
liaison with the doctor. It is possible that there was
variation between doctors regarding the information
women were provided about the risks associated
with invasive testing and what her calculated DS risk
meant, and that this may have influenced the
uptake of IT. The quality of the birth and invasive
testing records and the community-based setting
make this study a good source of information about
uptake rates in clinical practice.
Study included data from all 9
FMF accredited USS practices
and both the laboratories
offering 1st T screening analysis
in the state.
Exclusion criteria:
Gestation outside 11 weeks 1
day to 13 weeks 6 days
Cases with incomplete screens
or missing demographic
information were excluded.
The proportion of uptake relative to risk was reported
but not n for each group, so confidence intervals
could not be calculated for these groups.
The authors acknowledged that, because this was a
retrospective audit, they could not determine the
proportion of women not screened because of
technical difficulty, multiple pregnancy, or wrong
gestational dates. Consequently, the rates of
screening uptake are not reported, although the
authors did report that Western Australia has
approximately 25,000 births each year.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
167
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Ilgin-Ruhi et al.
2005)
N=340 women aged 35 and
older, referred from other
centres for IT based on AMA
2nd T MSS (3 analytes)
AFP
hCG
UE3
1:250 risk cut-off
Uptake of screening
Uptake of screening:
295/340 86.8% accepted screening
45/340 (13.2%) declined MSS (these women
were considered high risk for some analyses)
Authors conclusions
Following screening high risk women had a higher
rate of AC than low risk women. In a population of
women who all could have had AC based on
maternal age, only 63.5% of them opted to do so.
The rate of AC in women who did not have any
serum screening was higher than the low risk
screened women. This may mean they decided to
accept AC before genetic counseling. The mean
age of women who had Ac was not significantly
different from those who declined AC, but the
women who declined AC were further along in their
pregnancies.
Medical Genetics
Department,
Ankara University
Medical School,
Turkey
Prospective
cohort
Level of evidence
III-2
Mean age = 38.2 years +/-2.4
(median = 38)
Women were screened at 16-20
weeks GA
Mean GA = 19.2+/- 1.7
(median=19)
USS – not sure which
markers used in this study
Sometimes only hCG and
uE3.
16-20 gestational weeks
Genetic counseling offered
to referred women which
included information on:
Advice regarding AMA and
DS risks
How MSS and USS are used
to evaluate DS risk
DRs, false-positive and
false-negative rates
Risk cut-off levels for MSS
AC risks
In some cases counseling
required 1-2 additional
sessions for couples to
come to a decision
Couples asked to choose
initially whether to take up
USS and MSS screening.
Couples then asked to
decide whether to take up
AC.
Uptake of AC within the
no MSS and MSS groups.
Further analyses of AC
uptake based on results of
MSS and USS screen (high
risk or low risk).
For some analyses, no MSS
and MSS groups were
reported separately.
Some couples declined
MSS and these cases
(n=45) were considered
High Risk based on MA for
analyses comparing
invasive testing in high risk
versus low risk groups.
Overall rate of AC (%age, 95% CI):
63.5% (58.4 – 68.6%)
Uptake of AC with screen or no screen:
No screen
Accept = 73.3% (60.4 – 86.3%)
Decline = 26.7% (13.7 – 39.6%)
Screen
Accept = 62.0% (56.5 – 67.6%)
Decline = 38.0% (32.4 – 43.5%)
Uptake of AC by MSS risk group:
Low risk:
N=123
44.7% (35.9 – 53.5) accept AC
High risk:
N=172
74.4% (67.9 – 80.9) accept AC
Screen negative either MSS or USS
N=117
42% (32.9 – 50.8) accept AC
Screen positive either MSS or USS
N=178
75% (68.9 – 81.6) accept AC
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
The data suggested that screening by non-invasive
methods would decrease the requirement of AC
over time.
Reviewers conclusions
The method section was a little unclear about the
content of the MSS and USS markers.
The sample was relatively small and as a result the
confidence intervals are relatively wide for analyses
with smaller group sizes. The study was based in
Turkey and focused on women age 35 and above,
restricting the generalization of these results to other
settings.
Women referred from many doctors but receiving
counseling from one source so the information they
are receiving is consistent but possibly not a realistic
reflection of what might happen in a large scale
community-based screening programme.
168
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Mueller et al.
2005)
N= 16792 women who screened
+ve in the Ontario MSS
programme and for whom AC
uptake data were available.
Total screened = 308,298
2nd T MSS based on 3
biochemical markers:
AFP
uE3
hCG
+ MA
AC uptake relative to risk,
ethnicity and MA
6 risk groups:
>1:100
1:100-1:149
1:150-1:199
1:200-1:249
1:250-1:299
1:300-1:385
Median risk = 1:202
Risk range 1:8 to 1:385
%age, (95% CI)
Overall AC uptake in screen +ve:
11033/16792 = 65.7% (65.0 – 66.4%)
Caucasian = 67%
Asian = 66.6%
Black = 48.6%
Authors conclusions
The overall uptake of AC was 66%. Uptake in women
<35 was higher than that for older women. The risk
estimate also seemed to influence women’s
decisions regarding AC. As expected, the rate of
uptake declined with a decrease in risk estimate.
There was a greater change in uptake relative to risk
among women ≥ 35 years of age. The uptake of AC
in ≥ 35 year old women was less than that of women
< 35 years old at every risk level except > 1:100. Older
women and younger women have different
motivations for using screening. Older women seem
to use screening to avoid AC if possible. Younger
women do not perceive themselves at risk so use
screening for reassurance. When not reassured they
take the step of AC to get a definitive answer.
Canada
Ontario MSS
programme
between October
1993 and
September 1998
Retrospective
cohort (review of
MSS programme
database)
Level of evidence
III-2
<35 years, n=9779
≥ 35 years, n=7013
Median MA = 34 years (range
15-50 years)
Total screen +ve = 21823
AC data not available for 5031
(23%)
MSS database set up to audit
the MSS programme. Collected
demographic information,
screening results, utilization of
genetic services and
pregnancy outcomes.
Ontario prenatal care policy:
All pregnant women eligible for
MSS
Women who are screen +ve for
DS are offered AC
Women who are aged 35 years
or older can opt for AC without
screening
Screen +ve women receive
genetic counseling including
information about the risks of IT
Screening between 15 and
20 weeks GA
Risk cut off:
1:385 at term
All women received a
specific risk figure
regardless of their age and
screening result
2 age groups:
<35
≥35
3 ethnic groups:
Caucasian, 71.3%
Asian, 14.5%
Black, 6.8%
AC uptake relative to
magnitude of change
between age-specific risk
and MSS risk calculated
as:
(MSS risk-age risk)/age risk
AC uptake relative to risk estimate:
>1:100 = 73.3% (71.9 – 74.7%)
1:100-1:149 = 69.1% (67.1 – 71.0)
1:150-1:199 = 67.7% (65.8 – 69.6%)
1:200-1:249 = 63.4% (61.4 – 65.4%)
1:250-1:299 = 62.8% (60.8 – 64.7%)
1:300-1:385 = 58.6% (57.1 – 60.1%)
Screen +ve AC uptake relative to age:
<35 = 69.8% (68.9 – 70.7%)
≥35 = 60.1% (58.9 – 61.2%)
Similar patterns of uptake for all ethnic
groups with women <35 having higher
uptake rates than ≥35 year olds.
AC uptake relative to age and risk:
< 35 year olds
1: 100 = 73.6% (71.6 – 75.7%)
1:101–1:200 = 73.0% (71.3 – 74.7%)
1:201–1:300 = 69.6% (67.9 – 71.3%)
1:300–1:385 = 64.1% (62.3 – 66.0%)
≥ 35 year olds
1: 100 = 73.0% (71.0 – 74.9%)
1:101–1:200 = 62.3% (60.1 – 64.4%)
1:201–1:300 = 52.4% (50.1 – 54.7%)
1:300–1:385 = 47.8% (45.1 – 50.5%)
Separating highest risk into smaller groups:
>1:20, 1:20-1:49, 1:50-1:99 showed similar
uptake across all risk groups and age groups.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
About half the pregnant women in Ontario opted for
screening during the period of the study. There were
ethnic group differences in uptake of screening and
AC. This screening programme is state-funded so
these differences should not be related to SES.
Reviewers conclusions
Overall, women were more likely to opt for AC with a
higher risk estimate. In younger women, the
difference was not significant between all risk levels.
In older women there was a significant difference in
uptake between all risk levels and the change in
uptake was greater than that of younger women.
The proportion of >35year olds (16%) who were
screened is similar to that of the general pregnant
population, so the authors feel many women of AMA
are opting for screening.
169
Table 21.
Source
(Mueller et al.
2005)
Canada
Ontario MSS
programme
between October
1993 and
September 1998
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Sample
Screening Strategies
Outcomes
Results
Comments
Difference between age-risk and MSS risk:
These comparisons were only included for
women ≥ 35 years of age. The uptake of AC
increased gradually as the MSS risk increased
over the age-specific risk. When MSS risk was
20 times higher than age-specific risk, there
was a slight decrease in uptake.
AC data were missing for 23% of screen +ve women
who were lost to follow-up. Follow-up forms not
received for these women and they may have
miscarried, terminated their pregnancy, moved or
used another genetic centre. The authors excluded
these women from analyses but had they been
included and assumed not to have had AC, the
overall uptake of AC in screen +ve women would
have been 51% rather than the 66% that was
reported. Without age, ethnicity or risk estimate
information for the women lost to follow-up, it is
difficult to determine how their exclusion may have
affected the findings.
Retrospective
cohort (review of
MSS programme
database)
Level of evidence
III-2
Continued
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
170
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Interventions
Outcomes
Results
Comments
Saltvedt et al.
(2005)
N=39572 pregnancies
randomized to either 1st T NT or
2nd T USS by maternal age
Women who agreed to
participate were
randomized to either:
Pregnancy outcome
Comparison between groups:
The two groups did not differ in
demographic characteristics
Recruited women from an
unselected population of
pregnant women between
March 1999 and October 2002.
Eight Swedish maternity
hospitals included.
12-14 weeks scan including
NT.
Fetal karyotyping was
offered according to NT
screening; an anomaly
detected during any scan
or increased risk based on
history.
Authors conclusions
The 12 week scan policy was associated with many
fewer invasive tests per antenatally detected DS
case than the 18 weeks scan policy.
The two policies were not strictly adhered to but this
reflects the situation in real life. Neither pregnant
women nor health personnel adhere blindly to
recommended policies. There is no way of
preventing people from seeking a second opinion.
Almost 60% of the amniocenteses in the 12 week
scan group were performed because of parental
worry in the absence of medical risk factors. This
probably reflects the fact that women did not trust
the new NT method. Some women requested and
got 2nd T MSS but it is impossible to determine how
many retrospectively.
Multicentre RCT
NUPP trial, Sweden
Level of evidence
II
Eligibility criteria:
Ability to understand the
information about the trial
Gestational age at booking
≤13+2 weeks
12 week scan group:
N= 19796
Mean = 30.1 years
19.3% ≥ 35 years
18 week scan group:
N=19776
Mean = 30.2 years
19.4% ≥ 35 years
Declined to participate:
N= 10061
Mean = 29.7
19.0% ≥ 35 years
Sample size calculated based
on assumed prevalence of DS
and number of cases needed
to detect a difference between
groups.
Cut-off ≥ !:250
Peformance of each of
the screening policies
Uptake of IT following a
positive result for each of
the screening groups
Uptake of IT following a
negative result for each of
the screening groups
Indication for karyotyping
15-20 weeks anomaly scan.
Fetal karyotyping offered to
women ≥ 35 years old,
women with an anomaly
detected during any scan,
or increased risk based on
history.
2nd T MSS was not a routine
offer but was infrequently
performed by request
Randomization was
performed at the USS units
using internet-based
software.
Randomization was done
block-wise and stratified for
maternal age (<35 or ≥ 35
years).
%age (95% CI)
Uptake of IT:
12 week scan group (NT)
Overall = 8.0% (7.7 – 8.4)
Screen positive = 73.4% (69.9 – 77.0)
Number of invasive tests per detected DS
case = 38
18 week scan group (AMA)
Overall = 10.7% (10.3 – 11.1)
Screen positive = 51.7% (50.0 – 53.4)
Number of invasive tests per detected DS
case = 85
Indication for fetal karyotyping:
12 week scan group (NT)
NT high risk = 26.9%
Age ≥ 35 years = 7.3%
MSS = 1.1%
Anxiety = 57.8%
18 week scan group (AMA)
NT high risk = 0%
Age ≥ 35 years = 79.7%
MSS = 3.1%
Anxiety = 7.7%
Scans performed by 46
midwives with certification
by the FMF.
Confirmation of anomalies
and counseling provided
by 26 obstetricians.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
The authors acknowledged that there may have
been variability in the adherence to screening
policies in the two groups. This is a potential source of
bias, but they are also correct in saying it reflects the
realities of community-based screening where
people can and do seek second opinions. It would
seem from the indications for fetal karyotyping that
only a small proportion (1-3%) of women had MSS but
there is no way of knowing exact numbers.
The two groups did not differ in any demographic
characteristics and were representative of the
general population.
171
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Interventions
Outcomes
Results
Comments
(Nicolaides et al.
2005)
N=30564 singleton pregnancies.
All women attended the Fetal
Medicine Centre between July
1999 and December 2003.
1st T combined screen
NT
Free ßhCG
PAPP-A
MA
Rate of invasive testing
with varying levels of risk
Results of screening:
30564 women screened
2565/30564 = 8.4% screen positive
Composite risk calculated
based on NT + MSS results
Uptake of invasive testing
within older and younger
women with varying
degrees of risk
Authors conclusions
There was an exponential relationship between
estimated risk for DS and uptake of IT with the rate of
IT increasing as risk estimate increased. There was a
marked increase in the rate of invasive testing once
the risk was 1:300 or more, and this may be because
women are made aware during the consultation that
this is the risk cut-off point for offering IT. There was
also an effect of maternal age whereby more older
women than younger women opted for invasive
testing when their risk level was less than 1:300.
However, more than 90% of older women chose to
avoid IT when their risk level was less than 1:300.
Pregnant women are able to use risk information to
make informed decisions about IT for DS and should
be given the opportunity to do so.
Private prenatal
care clinic,
London, England
Prospective
cohort
Level of evidence
III-2
MA range 15-49 years
Median MA = 34 years
≥ 35 years = 48.5%
Screened at 11 – 13+6 weeks
Median GA = 12 weeks
1. Information leaflet
informing women of the PRL
rate of invasive testing (1%)
and that a DS risk of 1:300
or more was considered
high.
2. Screening carried out via
USS – NT and CRL and
screening of serum for
levels of fßhCG and PAPPA.
3. Women were counseled
with regards to their
individual risk for DS and
asked to decide whether to
accept or decline IT.
Proportion of women in
each risk category
%age (95% CI)
Uptake of invasive testing:
Overall
3277/30564 = 10.7% (10.4 – 11.1%)
Uptake relative to age:
< 35 = 5.1% (4.8 - 5.5%)
≥ 35 = 16.7% (16.1 – 17.3)
Screen positive
77.6% (76.0 – 79.2%)
Screen negative
4.6% (4.3-4.8%)
Uptake relative to risk:
1:50 or more = 95%
1:51 to 1:100=~83%
1:101-1:150=~75%
1:151 to 1:200=~70%
1:201 to 1:250=~63%
1:251 to 1:300=~60%
1:300-1:500~20%
Uptake relative to risk and age:
≥35 years
1:300 or more = 76.2% (74.4-78.1%)
Less than 1:300 = 7.4% (6.9-7.8%)
<35 years
1:300 or more = 82.5% (79.4-85.6%)
Less than 1:300 = 2.2% (2.0-2.5%)
Reviewers conclusions
There was a relationship between risk estimate and
AC uptake in that, as the likelihood of carrying a fetus
with DS increased, the proportion of women opting
for invasive testing increased. Unfortunately these
proportions are estimates because the uptake and
number in each risk group were not presented in
tables and the figure is difficult to read.
Consequently, confidence intervals could not be
calculated for the uptake relative to risk estimate.
All the women in this study attended one fetal
medicine clinic in London. Age distribution was
reported but no other demographic information,
making it difficult to determine how representative
these women are of the general population and how
generalisable the results would be to other settings.
In addition, the sample was older than that included
in other similar studies with a median age of 34 years,
and a high proportion of the women (48.5%) age 35
and older. It is also plausible that they might be of a
higher SES than the general population given that
they were visiting a private clinic for their prenatal
care.
In this study all women received standardized
information regarding the PRL risk for invasive testing
and the interpretation of their estimated DS risk. The
results therefore are possibly not reflective of the
reality of a community-based screening programme.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
172
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Platt et al. 2004)
N= 8216 women undergoing
sequential first and second
trimester screening for DS and
trisomy 18
1st T screening:
MA
PAPP-A
Free ßhCG
NT
≥1:270 screen +ve
Numbers of screen
positive women after 1st T
screening
1st T screening:
N= 8205
813 screen +ve
7392 screen –ve
All screen +ve and all
women 35 years or older
offered IT
Proportion of women
screened in 2nd T using
multiple marker MSS.
All women who continued
their pregnancy into 2nd T
offered 2nd T MSS:
AFP
Total hCG
uE3
Numbers of 2nd T screen
positive women
Authors conclusions
With the disclosure of their 1st T screen results, many
women still request 2nd T MSS. Sequential screening
following 1st T screening provides patients the
maximal number of options to make informed
decisions. Test results were disclosed with decisions
regarding 2nd T screening and prenatal diagnosis left
to the patient and physician. Invasive testing at <15
weeks was performed in 7.5% of screened patients,
with 28% of screen +ve and 5% of screen –ve opting
for IT at <15 weeks.
Women aged 35 years and older seem to have
undertaken screening for various reasons (information
to help them decide between CVS and AC,
thorough evaluation of their risk before IT). To make
screening most effective it is equally important to
understand patients’ preferences and to consider
their perceptions of risks based on g.a. and
willingness to use various methods.
USA
12 participating
prenatal
diagnostic centres
Prospective
cohort multicentre screening
programme
Level of evidence
III-2
11 cases of T18 removed
leaving n=8205 women in
sample
Age distribution of women who
underwent both 1st and 2nd T
screening:
N=4325
38.9% aged ≥ 35 years
Uptake of IT in 1st T screen
+ve women
Maternal age-related 2nd T
risk used in MSS calculation
≥1:270 = screen +ve
1st T screening results not
incorporated into 2nd T
calculation
Uptake of IT in women
who screened +ve in 2nd
T
1st T and 2nd T screening:
N=4325
2098 1st T screen –ve women declined or
results unavailable for 2nd T screening
+ve both screens = 74
-ve 1st +ve 2nd = 374
%age (95% CI)
Uptake of IT
1st T +ve and no 2nd T screen
+ve: 464/813 = 57.1% (53.7 – 60.5)
-ve: 1134/7392 = 15.3% (14.5 – 16.2)
Overall IT at ≤ 15 weeks GA
612/8205 = 7.5% (6.9 – 8.0)
+ve both screens
30/74 = 40.5% (29.4 – 51.7)
1st T –ve/ 2nd T +ve
166/374 = 44.4% (39.3 – 49.4)
Screen –ve both screens
194/3771 = 5.1% (4.4 – 5.8)
≥ 35 years = 8.3% (6.8 – 9.8)
< 35 years = 3.5% (2.8 – 4.3)
Reviewers conclusions
The uptake rates of IT after 1st T screen actually
reflect all women except those who had 2nd T
screening. Some of the women had missing data or
did not have information available for all 2nd T
analytes so were included in this group. May have
had AC for other reasons – family hx, anxiety, other
abnormal scan.
The authors acknowledged that they could not
control how results were presented to women by their
practitioner or what advice they were given
regarding their individual risk estimate, uptake of 2nd
trimester screening or potential risks of IT.
Age distribution of the original sample not reported in
this paper.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
173
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Khoshnood et al.
2003)
N= 12326 women who gave
birth in France in a 1-week
period in 1998 (National
Perinatal Survey, 1998)
French prenatal testing
policy:
2nd T USS with NT
2nd T serum screening
normal care
High risk women and all
women aged 38 years and
older offered reimbursed
AC
Reason for AC:
Provided retrospectively,
each woman could
provide 2 reasons from
serum screening, USS
finding, MA, other,
unknown.
Uptake of screening
8569/12326 = 69.5% screened
Authors conclusions
Altogether 11.1% of women had an AC. The
proportion of women who had an AC as greater for
women with higher levels of education. Irrespective
of screening or level of education, the proportion of
women who had an AC increased with advancing
maternal age.
For both maternal education groups the effect of
screening on AC was approximately 2 to 3 fold higher
for women younger than 35 years compared with
those 35 years and older. In general the odds of an
AC were substantially higher for women who had
screening compared with those who refused
screening.
Birth records from
a sample of all
births in France in
1998
Retrospective
cohort
Level of evidence
III-2
Excluded:
N=1152 (8.6%) women with
missing data regarding either
AC or serum screening
Data collected from:
1. face-to-face interview with
women after childbirth
2. medical records
Missing data 5% interview, 1%
medical records
Tested the hypotheses that:
1. as MA increases, women
will be more likely to opt for
IT without screening
2. as level of education
increases, women will be
more likely to opt for IT
without screening first
MA groups (at 14 weeks
g.a)
Less than 30
30-34
35-37
38 and older
Level of education:
<12 years
≥12 years
ORs comparing
proportion of AC with
screening vs. no screening
for each age group and
level of education group.
Logistic regression used to
adjust ORs for MA, marital
status, parity, ethnicity.
Logistic regression used to
examine the effects of
accepting versus
declining serum screening
on the odds of AC.
%age (95% CI)
Overall uptake of AC
1452/12326 = 11.8% (11.2 – 12.3%)
Age distribution:
Education level:
>12 years = 13.6% (12.6-14.5)
≤12 years = 9.5% (8.9-10.2)
Proportion of AC increased with MA
irrespective of screening or level of
education.
The proportions of women who opted for AC
with no screening were 51% for 35-37 year
old women with >12 years education, and
81.7% for ≥38 year old women.
OR of AC by maternal age and education:
Maternal education ≤ 12 years
<30 years = 2.7 (1.9 – 3.9)
30-34 years = 3.4 (2.0 – 5.9)
35 – 37 years = 1.2 (0.8 – 2.0)
≥38 years = 1.4 (0.7 – 2.4)
Maternal education>12 years
<30 years = 1.5 (1.0 – 2.4)
30-34 years = 1.5 (1.0 – 2.2)
35 – 37 years = 0.7 (0.4 – 1.1)
≥38 years = 0.7 (0.3 – 1.6)
Reason for AC:
35-38+ year olds, biggest indication was MA
followed by serum screening
<30-35 year olds, biggest indication was
serum screening followed by other or
ultrasound results.
Reviewers conclusions
Data were collected via a retrospective interview
and could be subject to recall bias. This, coupled
with the proportion of missing data (8.6% of women
were missing information about their serum screening
or amniocentesis), makes it difficult to interpret the
findings. The paper does not specify what type of
information was missing about serum screening but in
some it was whether serum screening was performed
or not (4.1%). These women were excluded from
analyses. The authors did not measure the use of
CVS but this is available under same conditions as AC
in France.
The study assumed that all women were offered the
same screening as per French prenatal testing policy.
There was a slightly lower proportion of <30 year olds
in >12 years education group (57.8% vs. 65.4%) and a
higher proportion of 30-34 year olds in >12 years
education group (30.4% vs. 24.4%). It is possible that
maternal age may have been confounded with level
of education and more educated women had their
children later. The difference in AC uptake between
the < 12 years and >12 years education groups may
have been due to differences in maternal age.
The confidence intervals for the odds of having an
AC relative to accepting or refusing serum screening
were wide suggesting small size for some of the
groups.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
174
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Interventions
Outcomes
Results
Comments
(Wald et al.
2003a)
Screening results
3271/46193 = 7.1% screen positive using MSS
AC or CVS uptake relative
to risk of DS calculated by
quadruple test
6659/46193 = 14.4% screen positive based
on MA alone
Data collected
from 14 UK
hospitals as part of
the routine care
offered by the UK
National Health
Service
2nd T MSS (4 analytes):
AFP
uE3
hCG
inhibin-A
+ MA at term
DR
False-positive rate
UK
46193 pregnancies screened for
DS risk at 14 UK hospitals
between August 1996 and
September 2001.
Compared performance of
quadruple test (AFP, uE3, hCG,
inhibin-A), triple test (inhibin-A
omitted) and double test
(inhibin-A and uE3 omitted) in
the same sample.
Screening between 14 and
22 weeks.
Performance of each
screening method was
compared for each
woman, so each woman
acted as her own control.
Authors Conclusions
Uptake of amniocentesis increased with increasing
risk Only 43% of women with risks of 1 in 250-300 had
an amniocentesis, whereas 74% did so if they had
risks higher than 1 in 50. Among women who tested
positive and had affected pregnancies, 87% had an
amniocentesis.
The influence of an anomaly scan in women with
screen-positive results might have led to a lower
overall uptake of amniocentesis than anticipated
(60%). The uptake of serum screening could not be
established because the number of women who
were offered such testing was not recorded.
Prospective
cohort
Included 149 twin pregnancies
Risk cut-off:
1:300 or greater
Uptake of AC in screen +ve women:
Overall = 60%
Relative to DS risk:
>1:50 = 74.5% (95% CI 67.3 – 81.7%)
1:250-1:300 = 43.1% (95% CI 38.8 – 47.5%)
Increase in IT with increasing risk (trend test
p< 0.0001).
Level of evidence
III-2
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers Conclusions
The overall study design and quality of the data
sources was high. The findings regarding an
increased rate of AC with higher estimated risk seem
robust. However, the report did not contain enough
information to calculate confidence intervals for the
overall rate of AC in screen positive women. There
was also no information about the uptake of AC in
screen negative women or women who declined
screening. The age distribution of the sample was not
reported in this paper.
175
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Interventions
Outcomes
Results
Comments
(de la Vega et al.
2002)
N=555 women referred for
estimation of DS risk between
January 1999 and December
2000.
Sample divided into groups
based on the indications for
prenatal diagnosis:
Uptake of AC was
calculated for each
group.
Uptake of AC for the total sample =
336/555=60.5%
Authors conclusions
The results suggest women are influenced by the
method of risk assessment more than their calculated
risk estimate. Patients in the sonographic marker
group chose AC more frequently than patients who
were offered AC based on maternal age or serum
screening results. Sonographic markers may be a
better method in Hispanic populations.
University Hospital
high risk prenatal
clinic, San Juan,
Puerto Rico
Hispanic
population
Women who had been
screened and identified as
having a calculated DS risk of ≥
1:250 were included in the
sample.
Retrospective
cohort review of
records
The sample was divided into
four groups based on the risk
factor detected.
Level of evidence
III-2
Women with more than one risk
factor were excluded from
analyses.
MA (35 years or older)
Abnormal serum screening
(either low AFP or triple
marker screening)
2nd T USS marker
Previous child with
chromosomal anomaly.
Uptake of AC per risk factor:
% (95% CI)
MA = 61.4% (55.8 – 67.0%)
Abnormal serum = 54.0%( 47.1 – 61.0%)
USS markers = 72.9%( 60.3 – 85.5%)
Family hx = 84.2%( 67.8 – 100%)
records of referred women
reviewed
risk calculated. If 1:250 or
more, included in study
risk factor identified
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
This study presents the same difficulties in sample size
(n=555 screen positive women), and a lack of
generalisability because of potential cultural
differences in the acceptability of both screening
and invasive testing. The confidence intervals for
uptake of invasive testing for each risk factor were
wide and overlapping, indicating that there was no
significant difference in uptake of IT between any of
the groups. In this study, the medical records of
Hispanic women who presented to a high risk
prenatal clinic in Puerto Rico were retrospectively
reviewed. Women who had tested screen positive
for DS (> 1:250) were included in the study and were
grouped based on their indication for prenatal
diagnosis. The description of the methodology was
not detailed enough to ascertain what options
women were offered following screening, what
invasive testing risks they were informed of, and what
they were told about their individual risk for DS. The
age distribution of the sample and how many
women were excluded because of multiple
indications for prenatal diagnosis was not reported. It
is also not indicated whether grouping of women
based on their indications was blind to their invasive
testing decision.
176
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Vergani et al.
2002)
N= 1486 women who
underwent genetic counselling
on the basis of MA (≥ 35 years)
between January 1990 and
December 1998.
Women’s views regarding IT
measured before USS
screening was undertaken.
Women’s preference for
AC a priori
Women’s preferences regarding AC
following genetic counselling and prior to
ultrasound:
103/1471 (7%) undecided
501/1368 in favour of AC
867/1368 against AC
Authors conclusions
Most studies looking at women’s decision-making
regarding IT, involve populations who have already
agreed to screening so are only relevant to these
populations. Secondly, many are retrospective
questionnaires or surveys and are more likely to
exclude those women who are not interested in
prenatal screening or diagnosis. They are also subject
to recall bias.
Hospital San
Gerardo, Monza,
Italy
National Health
Service funded
prenatal
evaluation and
diagnosis
Prospective
cohort
Level of evidence
III-2
Mean MA=38.9+/-2.1 years
1471/1486 (99%) underwent
genetic ultrasound
4645 deliveries for women aged
35 years and older
Genetic counselling at 11.4+/5.6 weeks
Ultrasound at 17.2+/-1.5 weeks
98% Caucasian
Are you inclined to have an
amniocentesis?
Yes/No/Undecided
Initial session occurred at
10-14 weeks.
Age-related risks of DS
discussed
MA, family hx, medical hx,
SES recorded.
Accuracy and risks of
available diagnostic tests
discussed.
Tests offered:
2nd T USS for structural
anomaly and markers of
aneuploidy (including NT)
2nd T genetic sonogram for
DS
AC
Women’s attitudes to AC
measured at end of session.
Results of genetic
sonogram
SES
Anamnestic
Decision to have AC or
not following
ultrasonographic findings
% (95% CI)
Uptake in IT following USS screening:
Normal findings:
N=966
31% (28 – 34) accept
69% (66 – 72) decline
Abnormal Findings:
N=402
36% (32 – 41) accept
64% (59 – 68) decline
AC uptake relative to a priori preference:
In favour:
N=501
83% (80 – 86%) accept
17% (14 – 20) decline
Against:
N=867
3% (2 – 5) accept
97% (95 - 98) decline
Women’s preference for/against AC prior to USS was
the strongest influence on their subsequent decision
whether to take up AC. Generally women did not
change their mind after receiving their USS results. 7%
of women who were against AC prior to their USS,
opted to have an AC after receiving results. Women
who had an a priori preference for AC tended to be
older than women who were against AC. They
conclude that ‘intensely personal values’ determine
uptake of AC
Reviewer’s conclusions
There were low uptake rates of AC in general. This
could be partially due to cultural preferences against
invasive testing as this was an Italian sample. It could
also be due to a lack of trust in the screen which is
less reliable than other methods.
The authors acknowledged that the sample included
only women who were referred to one genetic
counselling service, about 1/3 of women who
delivered at the hospital. The others would have
received genetic counselling at other clinics.
Representativeness of the sample is therefore an
issue.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
177
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Dommergues et
al. 2001)
N=359 consecutive pregnancies
in women presenting for
antenatal care before 14 weeks
NT 10-14 weeks
Numbers of women
screening positive for
each screening method
Screening results
Either positive MSS or positive NT = 130
Authors conclusions
A complete obstetrical and/or neonatal follow-up
was obtained in all 359 women. Results indicate that
a significant number of women of AMA chose not to
have an AC when noninvasive tests were reassuring.
However, nearly half of the women considered low
risk by NT, MSS and 2nd T sonography chose to have
an AC. Conversely, not all women considered high
risk by MSS elected to have AC. These discrepancies
may be in part related to the way different
practitioners gave the information to patients over
the study period, or to differences in the perception
of the patients. Although standardized written
information was given, it is impossible to control the
way the information sheet was commented on and
to determine the influence of the counselor on the
decision. AC may be offered on a selective rather
than routine basis in women over 38 based upon the
results of screening.
Prospective
cohort
Maternity Hospital,
France
Level of evidence
III-2
Age distribution 38 – 47 years
Excluded women who did not
consent to NT or MSS
2nd T MSS (2 analytes) 15 –
17 weeks:
AFP
hCG
2nd T USS 21-23 weeks
Low risk = NT < 3mm + MSS
derived risk < 1:250 +
normal USS
High risk = either positive NT
or MSS result or abnormal
USS
MSS was performed in all
women regardless of their
NT result
Negative for both MSS and NT = 229
Uptake of IT following a
positive result
Uptake of IT following a
negative result
Uptake of IT
Overall uptake
227/359 = 63% (95% CI 58 – 68%)
Screen positive
105/130 = 81% (95%CI 74-88%)
Screen negative
122/229 = 53% (95% CI 47-60%)
Uptake of IT for each screening measure
NT +ve, MSS +ve = 12/12 = 100%
NT+ve, MSS –ve = 5/7 = 71%
NT –ve, MSS +ve = 88/111 = 79%
NT –ve, MSS –ve = 122/229 = 53%
Low risk women were given
the option of not having an
AC.
High risk women were
recommended to have AC
A standardized information
sheet was provided to all
women and included
information regarding the
age-related risk of DS,
descriptions of MSS, NT and
USS methods of detecting
DS, and risks associated
with IT.
Reviewers conclusions
This study was a comparison of AC uptake and
pregnancy outcomes in women who screened high
or low risk for DS using MSS, 1st T NT and 2nd T USS.
Standardised written information was provided to
women about age-related risk of DS and risks
associated with IT. The authors acknowledge that
there may have been practitioner differences in the
way that information was communicated and it is not
clear whether women were informed of their
calculated MSS risk or just whether a positive or
negative result was obtained. While this means there
may have been variation in the information provided
to women, this is probably an accurate reflection of
what would occur in a community screening
programme and should not be seen as a limitation of
the study.
Information regarding the uptake of IT was obtained
for all women from cytogenetic records.
The sample is small and restricted to women over 38
years making the results less generalisable to other
settings.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
178
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Michailidis et al.
2001)
N= 8536 pregnant women who
presented at 10-14 gestational
weeks or having had a NT
measurement
NT screening at 10-14
weeks (n=7447)
Proportion of women who
opted for IT following an
abnormal NT result
Total rate of invasive testing:
632/7447 = 8.5%
Authors conclusions
The use of 1st T sonography had two effects on
biochemical screening: 1. a lower than usual uptake
of the test(66%), 2. taking into account the NT
measurements in our counseling and providing
women with a combined risk resulted in low uptake
of invasive tests, especially at the risk bands 1:250 –
1:100 (30 - 42%) A limitation of the study is that we
evaluated a combination of 1st and 2nd trimester
screening tests, although we acted upon the
abnormal results of the first test.
London, England
Maternity unit of a
university hospital
Full outcome data available for
7447 (87%)
Retrospective
cohort review of
records
Mean maternal age = 30.1
years (range 13 – 50)
≥ 35 years = 21.1%
Level of evidence
III-2
Mean gestational age at NT
screen = 12 + 5 weeks
Screening and invasive testing
data collected from hospital
database
Pregnancy outcome data from
maternity hospital records or
patients themselves
Positive screen results
disclosed to women
(above 99th centile or
structural abnormalities)
All women offered 2nd T
screening by midwife –
counseled, standardized
written information
2nd T MSS (2 analytes)
AFP
F ßhCG
N= 4864 women who went
on to 2nd T screening
Proportion of women who
opted for IT following
abnormal 2nd T screen
result
NT screening
N=7447
Screen +ve = 122
Rate of invasive testing
105/122 = 86.1% (95 % CI 79.9 – 92.2%)
MSS screening
N= 4864
Screen positive = 425
Rate of invasive testing
189/425 = 44.5% (95% CI 39.7 – 49.2)
No significant difference in age distribution
of this population
Prevalence of DS in this group was 0.08%
Risk cut-off >1:250
Ultrasound scan performed
if over risk cut-off
Counseling regarding
results included a
combined risk estimate
based on 1st T NT, MA, 2nd T
serum, and sonographic
markers.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
There was incomplete data for 13% of the original
sample.
Women who screened positive with MSS were given
an USS to detect soft sonographic markers and their
counseling included their combined risk (NT, MSS,
USS). So the uptake in screen positive women
actually reflects women who were given 2nd T MSS
and USS rather than those who screened over 1:250
for MSS risk. The uptake of 2nd T screening was low,
although the rates of uptake were calculated by
assuming all women who screened negative using NT
continued their pregnancy into the 2nd T. It would be
useful to report the number of terminations,
spontaneous miscarriages, or women lost to follow-up
in the NT screen negative group to get a better sense
of the uptake of 2nd T screening and the rates of
invasive testing in all groups (1st T negative/ 2nd T
positive and negative both screens).
179
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Interventions
Outcomes
Results
Comments
(Marini et al. 2002)
N= 2456 maternal serum
samples from women of AMA
referred for analysis at the
authors laboratory.
2nd T triple test:
AFP
uE3
ßhCG
Result of screening:
Positive screen result
(indicating increased risk
for either DS, ONTD or
trisomy 18)
Result of screening
841/2456 (34%) = positive
1615/2456 (66%) = negative
Authors conclusions
The majority of patients receiving negative screening
results did not request AC. More than half of all
patients receiving positive results declined AC.
Inclusion criteria
AMA cases selected from all
samples analysed 1994-1999 (n=
22 532)
Women screened for DS,
ONTD, T18 at the same time
Cytogenetics
laboratory, Texas,
USA
Retrospective
review of
laboratory records
over a 6 year
period
Level of evidence
III-2
MA range 35-47.3 years
GA range 15-22.9 weeks
Positive screen = 1:270 or
greater.
Rate of invasive testing in
screen positive women
Rate of invasive testing in
screen negative women
Uptake of invasive testing
% (95% CI)
Screen positive
AC = 404/841 = 48.0% (44.7 – 51.4%)
No AC 437/841 = 52.0% (48.6 – 55.3)
Screen negative
AC 208/1615 = 12.9% (11.2 – 14.5)
No AC = 87.1% (85.5 – 88.8)
Exclusion criteria: AMA women
undergoing screening for Open
Neural Tube Defects using AFP
only
Decisions made by AMA patients regarding AC may
not always correlate clinically with maternal serum
screening results. Understanding the reasons for
these decisions may improve service delivery to all
pregnant patients. An understanding of the decisionmaking process is also necessary in order to provide
women with full informed consent.
Reviewers conclusions
This study was a retrospective review of laboratory
records and thus was subject to potential bias in the
quality of data regarding screening and AC results.
As the authors acknowledge, clinicians vary in the
way they explain the results of screening and the
potential risks of IT to patients. As this was a review of
records, no information was available about the
contents of consultations or whether the laboratory or
individual obstetricians or midwives were responsible
for reporting results to women.
There is also no information provided regarding
whether women were told their exact risk estimate or
just that they were above the cut-off.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
180
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Audibert et al.
2001)
N = 4165 women undergoing
screening for DS by NT
measurement (10-14 weeks GA)
and MSS (14-18 weeks)
NT 10-14 weeks
Numbers of women
screening positive for
each screening method
Screening results
Either positive MSS or positive NT = 213
Authors conclusions
7.6% of screened women had antenatal karyotyping.
Surprisingly, in women at low risk for maternal age, NT
measurement and MSS, 4.7% still opted for AC.
Almost half of these tests were indicated by an
abnormal 2nd T scan.
Prospective
cohort
Maternity Hospital,
France
Level of evidence
III-2
35 (0.8%) lost to follow-up
Final NT group = 4130
Final NT + MSS group = 3790
Inclusion criteria:
MA less than 38 years (the
results for MA ≥ 38 years are
reported in Dommergues et al.
2001)
Exclusion criteria: MA ≥ 38 years;
twin pregnancy; CRL < 38mm or
>84 mm; NT not measured or
not recorded
Mean MA = 30.1 years (range
16-37 years)
14% 35 – 37 years
2nd T MSS (2 analytes) 15 –
17 weeks:
AFP
hCG
2nd T USS 21-23 weeks
Low risk = NT < 3mm + MSS
derived risk < 1:250 +
normal USS
High risk = either positive NT
or MSS result or abnormal
USS
MSS was performed in all
women regardless of their
NT result
Negative for both MSS and NT = 3599
Uptake of IT following a
positive result
Uptake of IT following a
negative result
Uptake of IT
Overall uptake
315/4130 = 7.6% (95% CI 6.8 – 8.4%)
Screen positive
125/213 = 58.6% (95%CI 52.1– 65.3%)
Screen negative
169/3599 = 4.7% (95% CI 4.0 – 5.4%)
Uptake of IT for each screening measure
NT +ve, MSS +ve = 4/4= 100%
NT+ve, MSS –ve = 59/83 = 71%
NT –ve, MSS +ve = 62/130 = 48%
NT –ve, MSS –ve = 169/3599 = 4.7%
Low risk women were given
the option of not having an
AC.
High risk women were
recommended to have AC
A standardized information
sheet was provided to all
women and included
information regarding the
age-related risk of DS,
descriptions of MSS, NT and
USS methods of detecting
DS, and risks associated
with IT.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
This study was a comparison of AC uptake and
pregnancy outcomes in women who screened high
or low risk for DS using MSS, 1st T NT and 2nd T USS.
This study included only women aged <38 years of
age, however the proportion of women over 35 years
(14%) was not unusually small.
Standardised written information was provided to
women about age-related risk of DS and risks
associated with IT. The authors acknowledge that
there may have been practitioner differences in the
way that information was communicated and it is not
clear whether women were informed of their
calculated MSS risk or just whether a positive or
negative result was obtained. While this means there
may have been variation in the information provided
to women, this is probably an accurate reflection of
what would occur in a community screening
programme and should not be seen as a limitation of
the study.
181
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Interventions
Outcomes
Results
Comments
(Chen et al. 2000)
n = 2879 women with screen
positive results who were
screened between April 1993
and December 1998
2nd T triple test offered to all
women regardless of MA:
AFP
hCG
uE3
High risk cut-off:
2nd T DS risk of 1:270 more
AC uptake (lab records)
2879/49772 (5.78%) women were screen +ve
Pregnancy follow-up
(from referring physician)
Uptake of AC in screen +ve women:
Overall = 52.0%
Authors conclusions
The greater the reported patient-specific risk, the
greater the utilization of AC. Women selected AC
when screening was performed earlier.
Logistic regression model
applied to identify the
influence of various
factors on the uptake of
AC:
Maternal age at delivery
Risk identified by
screening
Gestational age
Maternal weight
Method of determining
GA
Ethnicity
%age (95% CI)
By MA:
14-19 = 41.8% (30.9 - 52.6)
20-24= 48.0% (40.5 – 55.4)
25-29 = 52.6% (47.6 – 57.7)
30-34 = 58.9% (55.8 – 61.9)
35-39 = 48.7% (45.5 – 51.9)
40-48 = 42.5% (36.6 – 48.4)
University of
Connecticut
Health Center
maternal serum
screening
laboratory
Retrospective
cohort review of
records
Level of evidence
III-2
Mean MA = 33.5 years
Gestational age at screening =
14.0-21.9 weeks
Mean GA = 16.6 weeks
Mean DS risk = 1:73
Screened population:
n = 49772
Mean age = 27.5 years (range
13-48 years)
10.3% age 35 or more
70.7% White
10.3% Black
16.2% Hispanic
2.8% Other
Excluded:
AFP serum testing only
Multiple pregnancies
Women with insulin-dependent
diabetes
10.3% of screen +ve women
were tested through other
laboratories or had no follow-up
information and were assumed
not to have had AC.
Data collected from
cytogenetic laboratory records
and hospital records
Women ages 35 or older
were also able to opt for
direct AC
Laboratory findings
reported to women via
referring physicians, who
received an indication of
whether the test was
positive or negative and
also a patient-specific risk.
Assumed that all screen
+ve women were offered
AC
< 35 = 55.5% (53.1 – 57.9)
≥ 35 = 47.3% (44.5 – 50.1)
By risk:
1:1 to 1:10 = 72.2% (60.3 – 84.2)
1:11 to 1:30 = 57.6% (49.3 – 65.8)
1:31 to 1:60 = 61.4% (55.5 – 67.2)
1:61 to 1:134 = 55.1% (51.7 – 58.4)
1:135 to 1:270 = 47.7% (45.3 – 50.2)
By GA:
15/40 = 53.8%
17/40 = 50.3%
19/40 = 38.5%
21/40 = 6.5%
By ethnicity:
White = 54.6%
Black = 41.6%
Hispanic = 41.0%
By year:
1993 = 70.3%
1994 = 53.4%
1995 = 57.6%
1996 = 53.0%
1997 = 44.0%
1998 = 36.4%
Regression results:
Odds ratios presented for each factor in the
model.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Different ethnic groups showed different rates of
uptake of AC.
Year of testing also influenced uptake with a trend
towards declining AC between 1993 and 1998.
Maternal age influence on AC was complex.
Screening test may be used by older women to avoid
AC. Those who are going to have AC anyway, may
proceed directly to it.
Reviewers conclusions
Assumed that every screen positive woman was
offered AC but as the consultation was done by
referring physicians, the authors couldn’t control this
(acknowledged by them). Physicians were not
asked whether they offered AC. Also no control over
what information the patients received regarding
their risk or AC risk (acknowledged by authors).
Authors also suggest that decrease in AC over time
may be because of an increase in the use of genetic
sonogram to check for markers following MSS. This
may have resulted in a reduction in the need for AC.
182
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(O'Connell et al.
2000)
N= 18890 women who booked
for first trimester assessment
between May 1992 – April 1997
(total = 18890) and were
subsequently screened in the
2nd T
2nd T Triple test:
AFP
uE3
total hCG (May 1992 –
March 1994)
fßhCG (May 1994 – April
1997)
Rates of IT uptake in
screen positive and
screen negative women.
Uptake of screening
Screened = 14827/18890 = 78%
No screen = 4063/18890 = 22%
Rates of IT uptake in
women who were not
screened.
Results of screening
Screen +ve = 586/14827 = 4%
Screen –ve = 14241/14827 = 96%
Authors conclusions
The information women are given may influence how
they respond to prenatal diagnostic testing. 15% of
women who tested positive did not want IT and a
very small proportion of women with a negative
screening result opted for AC.
England
Hull Maternity
Hospital
Retrospective
review of a
screening cohort
Level of evidence
III-2
Data collected from antenatal
clinic records.
IT data collected from the
regional cytogenetics
laboratory records
1:250 risk cut-off
Individual counseling with a
midwife prior to testing. A
standardised information
sheet, which included a
description of the triple test
and options following
testing, was discussed with
patients and then provided
for further consideration.
Uptake of IT
Uptake of IT for screen +ve group:
IT = 498/586 = 85% (95% CI 82 – 88%)
No IT = 88/586 = 15% (95% CI 12 – 18%)
Uptake of IT in screen –ve group:
IT = 7/14241 = 0.05% (95% CI 0.01 – 0.09%)
Uptake of IT with no screening:
IT = 75/4063 = 1.8% (95% CI 1.4 – 2.3%)
AC not routinely offered on
the basis of MA.
AC performed prior to triple
test if requested
Women who tested positive
via MSS were informed in
person by a community
midwife and then met with
a consultant to discuss
options.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
There is no information provided about the age
distribution of the sample, which makes it difficult to
determine how well they represent the general
population. There was also no information about
whether any screen negative women were lost to
follow-up. It is possible that some of these screen
negative women were lost to follow-up and sought
prenatal diagnosis at another cytogenetics lab.
Standardised information was presented to women
prior to MSS but there is no information about the
information presented to women who screened
positive and negative. There may have been
variation in the information they were provided
regarding IT risks and the implications of their
calculated DS risk, which may have influenced their
decision whether to opt for IT. This information in
combination with the maternal age distribution might
help to explain the very low IT rate in the screen
negative group.
There was an increase in screen positives from 2.9%
(May 1992 – April 1994) to 5.7% (May 1994 – April
1997) when free ßhCG replaced total hCG in the
serum screen. The reliability of the screening test may
effect women’s decisions to opt for AC or not
following screening, and so it would have been useful
to present the rate of IT as a function of the two
variations of the serum screen or as a function of
year.
183
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Lam et al. 2000)
N= 3419 women ≥ 35 years of
age who reported for prenatal
diagnosis of DS on the basis of
AMA between Jan 1997 –
October 1999.
Women referred for
prenatal diagnosis on the
basis of AMA.
Uptake of screening by
year
Uptake of screening
1807/3419 = 52.9% (95% CI 51.2 – 54.5%)
opted for screening
Authors conclusions
Overall half of women aged ≥ 35 years chose serum
screening and this proportion increased with time.
The data show that the screening would become
more popular with time when people became more
confident and familiar with the procedure. Among
the screen positive cases, AC uptake was about 60%.
Another study (Lam et al. 1998a) by the same authors
reported on uptake in <35 year olds in the same
population and found 90% of screen positive women
opted for AC. There was a difference in screening
uptake depending on ethnic origin. This probably
represents the difference in values assigned to each
pregnancy outcome by people of difference ethnic
origin, cultural background and religious belief.
Hong Kong
Prospective
cohort
Level of evidence
III-2
Women were recruited to the
study and so women who
declined any form of screening
and diagnosis were excluded,
as well as women with other
high-risk factors (e.g. previous
chromosomally abnormal
pregnancies).
IT data were collected from
cytogenetic laboratory records
in the participating hospitals
Age distribution
35-36 years = 51%
37-38 years = 27%
39-40 years = 14%
>40 years = 7%
Detailed counseling,
leaflets and video
presentation including
information about agerelated DS risk, the use and
effectiveness of serum
screening, the use of and
risks related to IT.
Women offered serum
screening (total hCG and
AFP) as an alternative to
direct IT. Risk cut-off ≥ 1:250
Screen positive women
offered AC
Uptake of IT in screen
positive women
Uptake of IT in screen
negative women
1516 (AC) + 96 (CVS) = 1612/3419 = 47.1%
(95% CI 45.5 – 48.8%) opted for direct IT
Uptake of screening by year
1997 = 38.8%
1998 = 54.6%
1999 = 63.4%
Uptake of IT
Screen positives
184/302 = 60.9% (95% CI 55.4 – 66.4%)
Screen negatives
80/1505 = 5.3% (95% CI 4.2 – 6.4%)
Screen negative women
given detailed scan at 1820 weeks and AC
performed if requested
Reviewers conclusions
This study reports the uptake rates of IT following MSS
in pregnant women aged ≥ 35 years. The sample
was predominantly Chinese (91%) with a small
proportion of Filipino (5%) and Caucasian (1.3%)
women. Uptake rates of MSS varied according to
ethnic origin with a lower rate of uptake in women of
Chinese origin. This makes it difficult to generalise the
findings to other populations.
The information provided to women regarding the
implications of serum screening and invasive testing
was standardized and thorough. However, this may
not reflect the realities of clinical practice and may
overestimate the amount of information women
would actually be provided within a community
screening programme.
It is difficult to determine from the methods section
whether all women who booked for prenatal
diagnosis in this period were recruited to the study
and offered serum screening.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
184
Table 21.
Evidence table of primary research studies examining the uptake of invasive testing following DS screening (continued)
Source
Sample
Screening Strategies
Outcomes
Results
Comments
(Spencer et al.
2000b)
N= 4088 women accepted
screening after booking for
routine antenatal care over a 1
year period (1998-1999).
1st T combined NT + MSS
screen.
Uptake of 1st T screening
Uptake of screening:
4088/4190 (97.6%) opted for 1st T screening.
8% (n=348) had 2nd T screening (AFP + f
ßhCG)
Authors conclusions
The rate of acceptance of CVS was related to the DS
risk reported. Women with risks of ≥ 1:100 were 3
times more likely to accept CVS than those in the risk
group 1:200 to 1:300.
District General
Hospital maternity
unit,
England
Prospective
cohort
Level of evidence
III-2
Included singleton pregnancies
only
All women were screened
between 10+3 and 13+6 weeks
GA
Median age = 29 years
≥ 35 = 12.7%
≥ 37 = 6.1%
Screening was predominantly
1st T but some women
presented too late for NT
measurement and so only had
2nd T MSS (8%).
1. Consultation with midwife
and standardised written
information about available
tests and the clinic service.
2. If prenatal screening is
opted for:
MSS (fßhCG + PAPP-A if
prior to 14 weeks GA. If ≥ 14
weeks GA, AFP measured
instead of PAPP-A.)
NT
Uptake of IT following
screening.
After exclusions for GA or fetal death,
n= 3762 women who had 1st T screening.
Screening results:
≥ 1:300 = 253/3762 = 6.7%
Uptake of invasive testing:
207/253 = 81.8% (95% CI 77.1 – 86.6)
CVS = 200
AC = 7
3. MSS results entered into
database and composite
risk score produced.
4. Counselor/midwife
discusses risk report with
patient. Women with
increased risk for DS
referred for CVS or AC.
High risk cut-off:
1:300 or more
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
The methods section was detailed and thorough with
the median age of the sample being 29 years and
6.1% of the sample aged ≥ 35 years. In a
subsequent paper focusing on twin pregnancies from
the same sample (Spencer and Nicolaides, 2003) the
screening population was described as being
predominantly white Caucasian and from a relatively
affluent London borough.
The authors reported that the rate of uptake varied
depending on the level of risk estimate. However,
exact figures for uptake relative to risk estimate and
the numbers in each risk group were not reported
and confidence intervals were unable to be
calculated.
In this study all women received standardized
information regarding the PRL risk for invasive testing
and the interpretation of their estimated DS risk. The
results therefore are possibly not reflective of the
reality of a community-based screening programme.
185
Chapter 8: Invasive Testing and
Procedure-Related Loss
SECONDARY RESEARCH
The search strategy identified one relevant systematic review. The methods and conclusions are
described in Table 22 (page 186).
The report by the Cochrane Collaboration (Alfirevic et al. 2006) aimed to compare the safety and
accuracy of second trimester amniocentesis (after 15 completed weeks of gestation), early
amniocentesis (before 15 completed weeks of gestation), transcervical and transabdominal chorionic
villus sampling. The review included all 14 randomised comparisons of these methods of invasive
testing, including one RCT (Tabor, 1986). Quasi-randomised studies were excluded and the review
was graded as being of evidence level II. Outcome measures included the accuracy of the method,
technical difficulties related to sampling, pregnancy complications, pregnancy outcomes, and neonatal
complications.
In relation to fetal loss, the authors found the only RCT (Tabor, 1986∗) reported a 1% increase in total
pregnancy loss in the 2nd trimester AC group compared to no testing (3.2% versus 2.2%, ns), and a
0.8% greater risk of spontaneous miscarriage (2.1% versus 1.3%, relative risk (RR) 1.6, 95% CI 1.02 to
2.52). This was in a low risk population. One study compared early versus 2nd trimester
amniocentesis∗ (CEMAT, 1998) and found a 1.7% higher risk in total pregnancy loss with early
amniocentesis (7.6% versus 5.9%).
Four trials compared transcervical (TC) or transabdominal (TA) CVS with 2nd trimester AC (MRC,
1991; Canada, 1992; Denmark, 1992; Borrell, 1999)∗, finding total pregnancy loss to be 3.5% higher
following TC CVS than 2nd trimester amniocentesis (14.5 vs. 11%) but no difference between TA
CVS and AC.
Conclusions
The quality of this review was high in terms of both the studies included and the evaluation of included
studies. The reviewers concluded that the finding of a 1% increased risk of fetal loss (Tabor, 1986) is
still the best estimate of procedure-related loss in low-risk women. The recommendations of the
review were that prenatal diagnosis is safest performed in the second trimester by amniocentesis, which
is safer than both transcervical CVS and first trimester amniocentesis. Transabdominal CVS is the
safest method for first trimester prenatal diagnosis, followed by transcervical CVS.
∗
As cited by Alfirevic et al. (2006)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
186
Table 22.
Evidence table of secondary research studies appraised investigating the rate of fetal loss following invasive prenatal diagnostic procedures
Source
Search method
Selection Criteria
Results
Comments
(Alfirevic et al. 2006)
Cochrane
Collaboration
Search: Cochrane
Pregnancy and
Childbirth Group trials
register(March 2003)
which contains trials
identified from:
Cochrane Central
Register of Controlled
Trials (CENTRAL)
Monthly searches of
Medline
Handsearches of 30
other journals and
conference
proceedings
Weekly current
awareness search of
37 journals
All randomised
comparisons of late
amniocentesis, early
amniocentesis and
chorionic villus sampling
(either transabdominally or
transvaginally) with each
other or with no testing
have been included.
14 studies appraised:
Second trimester amniocentesis versus no testing (Tabor, 1986)
Early versus 2nd trimester amniocentesis (CEMAT, 1998)
CVS versus 2nd trimester amniocentesis (MRC, 1991; Canada, 1992;
Denmark, 1992; Borrell, 1999)
Transabdominal versus transcervical CVS (USNICHD, 1992; Brambati,
1991; Bovicelli, 1986; Tomassini, 1988)
Early amniocentesis versus CVS (Copenhagen, 1997; Leiden, 1998;
Kings, 1996)
Ultrasound assisted amniocentesis (Nolan, 1981)
Authors conclusions
In a low risk population with a background pregnancy loss of
around 2%, a 2nd T AC will increase this risk by another 1%. The
increase in spontaneous miscarriages following 2nd T AC compared
with controls was statistically significant (2.1% vs. 1.3%). Early AC is
not a safe alternative to 2nd T AC because of increased pregnancy
loss (7.6% vs. 5.9%). Transcervical CVS carries a significantly higher
risk of pregnancy loss (14.5% vs. 11%) and spontaneous miscarriage
(12.9% vs. 9.4%) than 2nd T AC. One study compared
transabdominal CVS with 2nd T AC and found no significant
difference in total pregnancy loss (6.3% vs. 7%).
Cochrane
Database of
Systematic Reviews
Level of evidence II
Cochrane Central
Register of Controlled
Trials (The Cochrane
Library, Issue 1, 2002)
searched using the
terms
‘amniocentesis*ME’,
‘amniocentes*’,
‘chorionic-villisampling*ME’, and
‘chorion*vill*’.
Databases searched:
Cochrane library,
Embase, Medline,
PsychLIT. Also
searched reference
lists of identified
studies, and
contacted experts in
the field to identify
further references.
Quasi-randomised studies
were excluded.
All trials were assessed for
methodological quality
using the criteria in the
Cochrane Handbook
(Clarke 2000) but there
were no other planned
exclusions based on quality.
Types of intervention:
2nd T amniocentesis (after 15
completed weeks of
gestation)
Early amniocentesis (before
15 completed weeks
gestation (i.e. ≤ 14 weeks 6
days)
Transabdominal,
transcervical, or
transvaginal CVS
Data extracted and analysed on an ‘intention to treat’ basis.
Weighted estimate of relative risk calculated for each outcome.
Chi-square test of heterogeneity used to determine whether a fixed
effects (no heterogeneity) or random effects (unexplained
heterogeneity) model was used to pool results.
Fetal Loss:
The only RCT (Tabor, 1986) reported a 1% increase in total
pregnancy loss in the 2nd T AC group compared to no testing (3.2%
versus 2.2%, ns), and a 0.8% greater risk of spontaneous miscarriage
(2.1% versus 1.3%, 95% CI 1.02 to 2.52). This was in a low risk
population.
One study compared early versus 2nd trimester amniocentesis
(CEMAT, 1998) and found a 1.7% higher risk in total pregnancy loss
with early amniocentesis (7.6% versus 5.9%).
Four trials compared transcervical (TC) or transabdominal (TA) CVS
with 2nd T AC (MRC, 1991; Canada, 1992; Denmark, 1992; Borrell,
1999), finding total pregnancy loss to be higher following TC CVS
than 2nd trimester amniocentesis but no difference between TA CVS
and AC.
Outcome measures
included the accuracy of
the method, technical
difficulties related to
sampling, pregnancy
complications, pregnancy
outcomes, and neonatal
complications.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers conclusions
Methodologically sound review process – two reviewers assessed
eligibility and trial quality and performed data extraction.
Studies were graded based on their method of randomization (A –
adequate, B – unclear, and quasi-randomised studies, graded C,
were excluded). There were no other planned exclusions based on
methodological quality. Because of this, some of the studies
included in the review have methodological flaws which make the
interpretation of their findings more difficult. However, several
studies of very high quality, including 1 RCT (Tabor, 1986), were
included and their findings should be considered good estimates
of the risk associated with each of the invasive tests they
examined.
187
PRIMARY RESEARCH: STUDY DESIGNS AND QUALITY
The search identified five eligible primary research studies. Below is an overview of study designs and
aspects of quality represented by these studies. Full details of the five papers appraised, including
methods, key results, limitations and conclusions, are provided in Table 23 (pages 191-195).
Study design
Of the five studies included in this part of the review, four were retrospective cohort studies (Scott et
al. 2002; Muller et al. 2002b; Antsaklis et al. 2000; Antsaklis et al. 2002), and one was a prospective
case-control study (Mungen et al. 2006).
Study setting
Of the four retrospective cohort studies, three were single centre studies. Two were set in maternity
hospitals in Greece (Antsaklis et al. 2000; Antsaklis et al. 2002)) and one in a prenatal diagnosis clinic
in Australia (Scott et al. 2002). One multi-centre study (Muller et al. 2002b) utilised a large
community-based maternal serum screening programme in France which collected data from 6
cytogenetic laboratories. The prospective case-control study was conducted in the perinatology unit of
a university hospital in Turkey (Mungen et al. 2006).
Samples
The sample sizes of the three single-centre cohort studies ranged from 365 – 9,200 and the case-control
study included 2068 participants and 2068 matched controls. Inclusion and exclusion criteria varied
depending on the sample and interventions. Younger (<35 years) and older (≥ 35 years) women (13 –
52 years) were included in three studies, while two studies examined fetal loss in either older (Scott et
al. 2002) or younger (Antsaklis et al. 2000) women.
Scott et al. (2002) examined rates of fetal loss in women referred for counselling about prenatal
diagnosis mostly on the basis of AMA. These women chose whether to have an invasive procedure and
which invasive procedure to have following counselling. Groups were not randomised and all women
were high risk for DS, in most cases on the basis of maternal age. No other exclusion criteria were
mentioned.
Antsaklis (2002) reviewed the records of women with multiple pregnancies who underwent AC or
CVS at their clinic between 1977 and 2000. No exclusion criteria were applied. Antsaklis (2000)
examined the procedure-related loss in 20-34 year old women who were referred for a variety of
reasons. Women in the study or control groups with multiple pregnancies, uterine abnormalities,
intrauterine contraceptive devices in situ or a serious history of second trimester miscarriage were
excluded from the study. The control group consisted of women who were screened but were
considered low risk for DS or NTD.
Muller et al. (2002b) utilised a large community screening programme which screened almost 55,000
women over a 3 year period. Of those women, 3472 opted for amniocentesis. The control group
consisted of 47,000 women who opted not to have amniocentesis, some of whom had calculated DS
risks above the cut-off (n=2418). The study group consisted of women who screened positive for DS
risk, mostly on the basis of elevated maternal serum levels, and opted for prenatal diagnosis. The
control group was all women who were screened but did not opt for AC. No exclusion criteria were
applied, 7.35% were lost to follow-up, and the age and serum levels of the study and control groups
differed significantly.
Mungen et al. (2006) applied strict inclusion and exclusion criteria to both cases and controls. Controls
and cases were matched one-to-one for maternal age, parity, and number of prior spontaneous
abortions. Matched pairs were excluded if either woman was lost to follow-up, had a fetus with an
abnormality or underwent repeat AC. Women with medical complications or elevated maternal serum
levels were excluded from the study.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
188
Interventions
Four of the five studies in this section of the review included a comparison of second trimester (15-24
gestational weeks) amniocentesis with no invasive testing, with one study also including a comparison
of 2nd trimester amniocentesis with 1st trimester CVS and CVS with no invasive testing (Scott et al.
2002). One study compared fetal loss in women with multiple pregnancies who underwent 2nd
trimester amniocentesis versus CVS (Antsaklis et al. 2002). This study reviewed data collected
between 1977 and 2000, during which time it is likely technology and procedure-related counselling
changed.
In most studies amniocentesis was performed under concurrent ultrasound guidance at 15-22 weeks
gestation using a 20-22 gauge needle.
Outcomes
Most studies collected pregnancy outcome data from obstetric units and information regarding fetal
loss from clinic databases. In Muller et al. (2002b), data were collected from six cytogenetic
laboratories and contributing maternity units. Antsaklis (2000) collected information regarding risk
factors for spontaneous miscarriage via a maternal interview. The interview was about retrospective
and potentially sensitive topics (previous abortions, miscarriages and pregnancy complications) and
could have been subject to recall or reporting bias. Two of the authors reviewed the maternal
interviews and the presence or absence of risk factors was recorded. Information as to whether the
interviewers or reviewers were blind to whether the woman had or did not have amniocentesis was not
provided.
The measure of fetal loss varied between studies. Two of the studies measured fetal loss within 28 or
30 days of the procedure or inclusion in the study for the control group (Antsaklis et al. 2002; Mungen
et al. 2006). Four of the studies measured fetal loss up to a particular gestational week, varying
between 22 and 28 weeks (Scott et al. 2002, Antsaklis et al. 2000; Muller et al. 2002b, Mungen et al.
2006). One study also compared losses occurring any time during the pregnancy (Mungen et al. 2006).
PRIMARY RESEARCH: STUDY RESULTS
Studies comparing 2nd trimester amniocentesis with no invasive testing
Four studies compared the rates of fetal loss in women who had a 2nd trimester amniocentesis
procedure and women who had no invasive testing.
Mungen et al. (2006) found no difference in rates of fetal loss either within 30 days of the procedure or
inclusion in the study, or before 28 weeks gestation in women who underwent AC or did not. Cases
and controls were matched one-to-one for maternal age, parity, and number of prior spontaneous
abortions. Matched pairs were excluded from analysis if either woman was lost to follow-up, had a
fetus with an abnormal karyotype or a major malformation, or underwent repeated AC because of
culture failure. Women with medical complications or elevated maternal serum levels were excluded
from the study. The sample size was sufficient to detect differences of 1% or greater (80% power at a
significance level of 0.05). However, the magnitude of increased fetal loss related to invasive testing is
typically estimated to be between 0.5 -1%. This study was well designed but the sample size was not
appropriate to examine these small differences and the authors’ concluded that they could only say
from their study that the increased fetal loss in women who had an amniocentesis was less than 1% if
there was any difference.
Antsaklis et al. (2000) compared the rates of fetal loss before 28 weeks gestation in 20-34 year old
women who underwent amniocentesis versus controls who did not. There were no significant
differences between the study and control group in mean maternal age, mean number of previous
pregnancies, history of abortion, or previous bleeding in current pregnancy. There was no information
regarding gestational age in each of the groups. There was a significant difference (p<.01) in the fetal
loss rate before 28 weeks in the control group (1.5%) compared to the AC group (2.1%).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
189
Antsaklis et al. (2000) also investigated the effects of predisposing risk factors on rates of fetal loss.
When patients had a previous history of abortion or bleeding in the current pregnancy, there was a
significant difference between the rate of fetal loss in the amniocentesis (5.9% and 6.9%) versus no
amniocentesis (3.8% and 3.5%) groups. When risk factors were not present, there was no difference in
fetal loss between the two groups (AC=0.96%, no AC = 0.93%). Data regarding the presence or
absence of risk factors were collected by maternal interview and included retrospective information of
a sensitive nature (e.g. previous abortions) and so may have been subject to recall or report bias.
There was no mention of whether interviewers were blind to the group allocation of each patient.
Muller et al. (2002b) utilized a large (n=54, 902) community-based maternal serum programme to
compare the fetal loss rates in screened women who had a 2nd trimester amniocentesis with those who
did not. The authors found a 0.8% increased risk of fetal loss in women who underwent 2nd trimester
amniocentesis (1.12%) compared to those who did not (0.42%). However, there were significant
differences between the two groups in mean maternal age (AC=33 years, no AC = 29 years) and
maternal serum levels, with the AC group being selected based on a higher than 1:250 risk for DS.
Both maternal age and elevated serum levels are associated with a higher rate of spontaneous
miscarriage. The rate of fetal loss in the AC group included eight fetal losses which occurred prior to
the procedure, thus overestimating the rate of loss following the procedure. Excluding these eight
cases would have produced a fetal loss rate of 0.89% (95% CI 0.58 – 1.21), 0.47% higher than the
control group. There was also a 7% loss to follow-up in this study.
Scott et al. (2002) retrospectively reviewed the records of 2366 women referred for prenatal diagnosis
at their clinic between 1995 and 1997. Women were mostly referred on the basis of age ≥ 35 years and
following genetic counselling were offered the options of 2nd trimester AC, 1st trimester CVS or no
invasive testing. Other complications or risk factors were not described and it is likely that women
with lower overall risk of DS were more likely to opt for no invasive testing, and that women with a
high risk for DS, based on maternal age and other factors, could be more likely to opt for early
diagnosis with CVS. Alternatively, women at high risk of miscarriage might have been more likely to
opt for a 2nd trimester AC procedure, with relatively lower risk, rather than CVS. Total fetal losses
after the initial consultation (9-10 weeks) and before 22 weeks were compared and the authors reported
a fetal loss rate of 8.4% in the control group and 3.1% in the AC group. Women were not randomly
allocated to groups.
Studies comparing 2nd trimester amniocentesis with CVS
Two studies compared 2nd trimester amniocentesis with CVS.
Scott et al. (2002) examined spontaneous miscarriages after AC or CVS and before 22 weeks
gestational age and found a lower rate of fetal loss in the AC group (0.36%) compared to the CVS
group (1.85%). However self-selection of groups meant that there is a possibility that lower risk
women opted for AC. Transabdominal and transcervical CVS were also compared with a slightly
higher rate of fetal loss in the transcervical CVS group (2.16% vs. 1.65%). However, the method of
entry in CVS procedures was non-randomised and decided based on operator preference.
Antsaklis et al. (2002) compared the rate of fetal loss in multiple pregnancies for women who opted for
AC or CVS. There was no difference between the two groups in the rate of miscarriages either within
four weeks of the procedure or after four weeks. However, the size of the sample (n=365) was most
likely too small to detect differences of less than 1% so the results are inconclusive.
Conclusion
The findings of the five studies included in this section were inconclusive. There were several
limitations in the studies including non-randomised allocation to groups, failure to exclude or control
for existing conditions and significant differences between the study and comparison groups in age and
maternal serum levels. In the best designed study, a matched case-control study of a low risk
population, the sample size was too small to detect differences of the magnitude typically found in
studies of procedure-related loss. The authors concluded that the difference, if any, between the
amniocentesis and no amniocentesis group was less than 1%.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
190
The ideal study would randomly allocate women at risk for aneuploidy to undergo amniocentesis,
chorionic villus sampling or no invasive testing. This would be unacceptable nowadays for ethical
reasons and the only fully randomised study of this kind was conducted twenty years ago (Tabor
(1986) as cited by Alfirevic (2006). The 1% increased risk of fetal loss following amniocentesis found
in Tabor still stands as the best indication of procedure-related loss in a low risk population. The
findings of the systematic review (Alfirevic et al. 2006) were that prenatal diagnosis is safest
performed in the second trimester by amniocentesis, which is safer than both transcervical CVS and
first trimester amniocentesis. Transabdominal CVS is the safest method for first trimester prenatal
diagnosis, followed by transcervical CVS.
No studies were identified in the search which investigated interventions to reduce rates of fetal loss.
However, best practice guidelines recommend the use of concurrent ultrasound guidance and welltrained and experienced operators for both amniocentesis and CVS (RANZCOG, 2004).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
191
Table 23.
Evidence table of primary research studies investigating the rate of fetal loss following invasive prenatal diagnostic procedures
Source
Setting
Sample
Interventions
Outcomes
Results
Comments
(Mungen et al.
2006)
Cases were 2068 women with
singleton pregnancies who
underwent 2nd T AC.
AC at 15-22 weeks GA
Case-control study
Perinatology
unit of a
university
hospital
AC group:
Indications for AC
MSS = 53%
AMA = 38%
Authors conclusions
In our study there were no significant
differences in fetal loss rates and major
pregnancy complications between the
study and control groups.
Level of evidence
III-2
February 1998 –
June 2002
Fetal loss
Premature delivery
Small for gestational age
infants
Preeclampsia/eclampsia
Placental abruptions
Caesarean deliveries
Istanbul, Turkey
Controls were 2068 women
selected from pregnant women
with singleton pregnancies who
either were not candidates for
AC or declined the procedure
for various reasons.
Controls and cases matched
one-to-one for maternal age,
parity, number of prior
spontaneous abortions
Matched pairs were excluded
from analysis if either woman
was lost to follow-up, had a
fetus with an abnormal
karyotype or a major
malformation, or underwent
repeated AC because of
culture failure.
Exclusions applied to both study
and control groups:
Medical complications
(hypertension, renal disease,
pre-gestational diabetes etc.)
Elevated maternal serum levels
22 gauge needle
Continuous ultrasound
guidance
Compared for study and
control groups
Mean gestational age at AC:
17.5 +/- 1.9 weeks
Majority of procedures
performed between 15 and 18
weeks
Mean maternal age
31.1 +/- 5.9 years
Control group:
Mean maternal age
30.9 +/- 5.7 years
Fetal loss within 30 days of AC or
inclusion in the study (%, 95% CI):
AC group = 0.4% (0.1 – 0.6)
Control = 0.3% (0.07 – 0.5)
Difference = 0.1% (not sig.)
Fetal loss before 28 weeks:
AC group = 1.5%
Control = 1.3%
Difference = 0.2% (not sig.)
Total fetal loss rates including
spontaneous abortions and
intrauterine fetal deaths/stillbirths:
AC group = 2.3% (1.6 – 2.9)
Control = 2.0% (1.4 – 2.6)
Difference = 0.3% (not sig.)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Our study had sufficient power to detect
a 1% increase in fetal loss rate, therefore,
we can conclude that increased risk of
fetal loss resulting from 2nd T AC, if any, is
less than 1%.
There was no significant difference in total
fetal loss rates between the women who
underwent one needle insertion and
those requiring two punctures.
Reviewers comments
The authors acknowledged that the
sample size was calculated on the
assumption that AC related fetal loss risk
was 1% and the background loss rate
after 15 weeks gestation was 2%. The
sample size did not have sufficient power
to detect differences less than 1%.
192
Table 23.
Evidence table of primary research studies investigating the rate of fetal loss following invasive prenatal diagnostic procedures (continued)
Source
Setting
Sample
Interventions
Outcomes
Results
Comments
(Antsaklis et al.
2002)
Single centre
maternity
hospital fetal
medicine unit,
1977-2000
n=365
1977 - 1990 women offered
AC or fetal blood sampling
based on gestational age
Total Fetal loss
1977-2000
365 AC in twin pregnancies
347 included in analyses
Authors conclusions
Our data suggest that both AC and
transabdominal CVS are equally safe,
however, it is well recognised that the
latter requires a more advanced level of
expertise.
Retrospective
cohort
Level of evidence
III-2
University
hospital
Athens, Greece
Data obtained
from maternity
units,
obstetricians, or
patients
themselves
Women with multiple gestations
who attended the unit for
prenatal diagnosis between
1977 and 2000
1 case lost to follow-up
17 ongoing pregnancies
12 cases have incomplete
pregnancy outcome data
Mean maternal age = 36.2
years (19-52)
1986 - 2000 patients
presenting in the 1st
trimester also offered
option of CVS
All patients were counseled
regarding the risks of
miscarriage/preterm
delivery and options if their
results were abnormal
Detailed ultrasound
performed prior to
procedure - number of
fetuses and placental and
cord placement
Miscarriages within 4
weeks of procedure
Miscarriages more than 4
weeks after procedure
7 cases prior to 14 weeks (early
AC)
340 between 16-21 weeks GA
(2nd T AC)
Indications for AC:
AMA
Previous hx of aneuploidy
Abnormal serum biochemistry
Increased NT
Abnormal sonographic findings
All procedures carried out
by 5 operators
Miscarriages within 4 weeks of
procedure:
AC
10/335 = 2.98%
CVS
1/44 = 2.27%
No significant difference
AC
Ultrasound guided for all
procedures
22 gauge needle
Transplacental entry in
some cases where it could
not be avoided
Miscarriages more than 4 weeks
after procedure:
AC
4/335 = 1.19%
CVS
1/44 = 2.27%
No significant difference
CVS
Transabdominal in all cases
21 gauge needle and
chorionic villi aspirated
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
The procedure-related risk was similar for
both groups of AC and CVS. CVS
appears to be as safe as AC and offers
the advantage of earlier detection of
defects.
Reviewers comments
Sample size is not big enough to detect
differences of the magnitude typically
found in studies of procedure-related loss.
Technology and/or advice regarding
procedure-related complications may
have changed between 1977-2000 but
the authors make no mention of any
changes in uptake or complications in
relation to the year of procedure.
Early AC is associated with a higher rate
of fetal loss than 2nd T AC – better to
exclude early AC from analyses.
193
Table 23.
Evidence table of primary research studies investigating the rate of fetal loss following invasive prenatal diagnostic procedures (continued)
Source
Setting
Sample
Interventions
Outcomes
Results
Comments
(Muller et al.
2002b)
Maternal serum
screening
programme
54,902 women with singleton
pregnancies
MSS:
AFP
fßhCG /total hCG
Fetal loss before 24
gestational weeks
AC group:
N= 3472
MSS high risk = 3151
Maternal anxiety or minor
sonographic markers = 321
Authors conclusions
The total rate of adverse outcome in the
Ac group was 1.52% and 0.66% in controls,
suggesting that AC carries an additional
risk of 0.86%.
Control group:
N=47 004
MSS high risk = 2418
MSS low risk = 44 586
Indications for AC may have selected
patients at higher risk of adverse outcome
because high maternal serum markers are
associated with adverse outcomes.
% (95% CI)
Fetal loss prior to 24 weeks:
AC group = 1.12% (1.08 – 1.15)
but 8 fetal deaths were
ascertained by USS prior to AC
and included in these rates
Reviewers comments
The authors acknowledged that the two
groups differed significantly in maternal
age (33 vs. 29 years), and that higher
rates of adverse outcomes are observed
in older patients.
Control = 0.42% (0.41 - 0.43)
Elevated maternal marker serum levels
are also associated with higher rates of
spontaneous miscarriage. The higher rate
of fetal loss in the AC group could have
been due to serum levels rather than the
AC procedure. A comparison of the fetal
loss rate in women who had high risk
serum levels but declined AC and those
who accepted AC would have been a
better comparison. However it is possible
that those women who declined AC were
closer to the cut-off (i.e. lower risk) than
those who accepted AC.
Retrospective
cohort
Level of evidence
III-2
6 accredited
laboratories
between 19971999
France
Data sources:
Data sheet
completed for
each patient by
obstetrical units
Median maternal age = 29
years (range 13-44 years).
97.8% < 35 years
4039 (7.35%) lost to follow-up
387 excluded because of
severe fetal abnormalities
Study group:
N=3472 women who had an AC
following screening for DS risk
Mean maternal age = 33 years
Control group:
N= 47004 women who elected
not to have an AC following
screening for DS
Mean maternal age = 29 years
2418 of these women had a DS
risk of ≥ 1:250 but opted for no
AC.
DS risk calculated by MA +
MSS
1:250 risk cut-off screen
positive women were
offered an amniocentesis.
AC performed under
ultrasound guidance using
a 20 gauge needle
AC between 15-24
gestational weeks (median
18 weeks)
Premature delivery
between 24 and 28 weeks
Difference = 0.8%
Premature delivery between 24
and 28 weeks:
AC group = 0.40% (0.39 – 0.41)
Control = 0.24% (0.23 – 0.25)
Total adverse outcome:
AC group = 1.52%
Control = 0.66%
Included losses diagnosed by USS prior to
AC in the calculation of fetal losses so
1.12% likely to be an overestimation
(acknowledged by authors)
Karyotype of fetal death cases not
reported. Cannot ascertain loss of normal
fetuses as a result of AC.
Initial sample 54 902 women of which 4039
(7.35%) were lost to follow-up. The authors
acknowledged that this could be a
source of bias but felt that it was not likely
to have affected results in this study.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
194
Table 23.
Evidence table of primary research studies investigating the rate of fetal loss following invasive prenatal diagnostic procedures (continued)
Source
Setting
Sample
Interventions
Outcomes
Results
Comments
(Scott et al. 2002)
Retrospective
cohort
Specialised
prenatal
diagnosis
practice
N= 2366 women
Women referred for counseling
about prenatal diagnosis
Following genetic
counseling, women chose
between no invasive
testing, undergoing AC or
undergoing CVS.
There were no significant differences
in maternal age or gestational age
at consultation between any of the
three groups.
Level of evidence
III-2
Sydney,
Australia
Total fetal loss (includes
miscarriages after
consultation but prior to
procedure and
terminations but not fetal
losses after 22 weeks
gestation)
Authors conclusions
Total loss rate for the AC group was
0.36% (procedure-related loss and
spontaneous loss). PRL is less than
0.36% but we cannot establish how
much less. The spontaneous
miscarriage rate was high (8.4%) in this
group of women, who were largely of
advanced maternal age. The
procedure-related loss rate for AC was
less than 1/280. The miscarriage rate
after transabdominal CVS appeared
less than for transcervical CVS but this is
not statistically significant.
Data sources:
Referring
doctors and
hospital records
Indication for prenatal diagnosis
AMA (≥ 35 years) in most cases
53 women (2.2%) were lost to
follow-up
Three groups:
No invasive testing (n=346)
Mean MA = 35.6 years
Mean GA (at time of
consultation) = 9.53 weeks
CVS (n=1128)
Mean MA = 38.5 years
Mean GA (at time of
consultation) = 9.44 weeks
AC (n=839)
Mean MA = 37.9 years
Mean GA (at time of
consultation) = 10 weeks
CVS
• performed under
ultrasound guidance
• 10 - 12 weeks GA
• transabdominally (19
gauge needle) or
transcervically
depending on operator
preference.
AC
• performed under
ultrasound guidance
• from 14+6 weeks GA
• 22 gauge needle.
Spontaneous miscarriage
rates for each group
Miscarriages defined as
fetal loss up to 22 weeks
GA (allowing 6 weeks or
more from any
procedure)
% (95% CI)
Total fetal losses:
No invasive test
29/346 = 8.4% (5.5 – 11.3)
CVS
71/1128 = 6.3% (4.9 – 7.7)
AC:
26/839 = 3.1% (1.9 – 4.3)
Spontaneous miscarriages after
procedure before 22 weeks GA:
AC
3/829 = 0.36% (-0.04 – 0.77)
(excludes 10 miscarriages prior to
procedure)
Transabdominal CVS
11/665 = 1.65 % (0.68 – 2.62)
Transcervical CVS:
9/416 = 2.16 (0.77 – 3.56)
Total CVS:
20/1081 = 1.85% (1.05 – 2.65)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
Reviewers comments
Greater risk of spontaneous
miscarriage earlier in gestation so
authors compared total loss from the
time of the initial consultation.
Because CVS and AC procedures
were carried out at different
gestational ages and fetal loss was
measured up to 22 weeks, there was a
longer period of time after a CVS
procedure for losses to occur.
Not a randomized study – sample
opted for no testing, AC or CVS. The
known PRL was 1/200 for AC and
higher for CVS at the time of the study,
and it is possible that lower risk patients
were attracted to AC rather than CVS
(acknowledged by authors). Those
with previous miscarriages or bleeding
may have decided against prenatal
testing. Transabdominal and
transcervical CVS was carried out
based on ‘operator preference’.
Higher risk women possibly allocated to
TA CVS. Confidence intervals were
wide due to a small sample size and
small differences between groups.
195
Table 23.
Evidence table of primary research studies investigating the rate of fetal loss following invasive prenatal diagnostic procedures (continued)
Source
Setting
Sample
Interventions
Outcomes
Results
Comments
(Antsaklis et al.
2000)
Maternal fetal
medicine unit
All procedures carried out
by 1 of 4 people
Retrospective
cohort
Athens, Greece
Study group:
N=3910 women referred for
prenatal diagnosis between
1992-1997. Women aged 20-34
years at EDD
3 risk factors were
identified by the authors
as being potentially
responsible for increased
perinatal loss:
- hx of 3 or more 1st T
abortions or 1 2nd T
abortion
- bleeding or spotting
before AC
- AC
No significant differences
between the study and control
group in mean maternal age,
mean number of previous
pregnancies, at least 1 induced
abortion, at least 1 spontaneous
abortion, ≥ 3 previous abortions,
previous bleeding in current
pregnancy
Authors conclusions
Authors - both study patients and control
women were in the same age group and
thus equally prone to chromosomally
abnormal fetuses. Both groups were
screened during the 2nd T and had the
same exclusion criteria.
1992-1997
Level of evidence
III-2
Indications for prenatal
diagnosis in study group:
Anxiety
Abnormal MSS result
Abnormal sonographic findings
Maternal infection with
toxoplasma or cytomegalovirus
Fetal karyotyping
DNA analysis
Known metabolic disease
Exclusions:
Women with multiple
pregnancies
Women with known uterine
abnormalities
Women with intrauterine
contraceptive devices in situ
Serious maternal hx of 2nd T
miscarriage
Control group:
n=5324 women who were
screened for DS between 16
and 20 weeks GA between
1992 and 1997. Women aged
20-34 years at EDD.
Only pregnancies considered at
low risk for DS or NTD were
included.
AC
Continuous ultrasound
guidance
Complete anatomic fetal
survey prior to procedure
21 gauge needle
Control group
MSS at 16-20 weeks GA
AFP, ßhCG, uE3
Risk Factors:
Data regarding risk factors
were collected by a
maternal interview.
Medical secretary and
midwives carried out
interviews which were
reviewed by 2 of the
authors.
The interview collected
information regarding:
Gravidity
Parity
History of 1st T spontaneous
and induced abortions
2nd T complications
Any sign of threatened
abortion in current
pregnancy
Presence/absence of risk
factors in control and
study groups was
recorded
Fetal losses before 28
weeks GA in study and
control groups
Fetal loss in study and
control groups with regard
to the presence or
absence of risk factors
Fetal losses before 28th week:
AC
79/3696 = 2.1% (95% CI 1.7-2.6)
No AC
80/5324 = 1.5% (95% CI 1.2-1.8)
Significant (p<.01)
Previous bleeding
AC 31/527 = 5.9%
No AC 28/723 = 3.8%
Previous abortions
AC 18/258 = 6.9%
No AC 12/334 = 3.5%
No predisposing factors
AC 30/3125 = 0.96%
No AC 40/4267 = 0.93%
The background risk in our population
after the 16th week of pregnancy was
1.5%. Our study and control groups were
comparable in terms of age, background
factors and time of entry into the study.
There was a 2.1% loss rate among women
who had 2nd T AC, leaving a procedurerelated loss rate of 0.6%. This risk is directly
related to risk factors such as previous hx
of abortions or bleeding during current
pregnancy. There was a statistically
significant difference between the study
group and controls when these factors
were present. When these predisposing
factors were not present, there was no
significant difference in fetal losses
between the study and control groups.
Reviewers comments
Data regarding the presence or absence
of risk factors were collected by maternal
interview and included retrospective
information of a sensitive nature (e.g.
previous abortions). May have been
subject to recall bias. There was no
mention of whether Interviewers and
reviewers were blind to the group
allocation of each patient.
Indications for AC group included risk
factors associated with higher
spontaneous miscarriage (maternal serum
levels). However, 35% of women in this
group had an AC procedure due to
anxiety.
Other exclusion criteria were
the same as those applied to
the study group
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
196
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
197
Chapter 9: Discussion
SUMMARY OF EVIDENCE
Aim of the review
This review aimed to systematically appraise the international evidence for the antenatal use of
technologies and screening strategies for DS. Specific aims included assessing the validity of DS
screening methods, any difficulties implementing screening strategies, the impact of screening on
amniocentesis and chorionic villus sampling, and the safety of these procedures. Part A considered the
validity of screening methods and difficulties implementing screening strategies. Part B considered the
impact of screening on invasive testing and the safety of these procedures.
Result of the search strategy
The search strategy for Part A yielded 1138 articles. From 219 articles identified as potentially eligible
for inclusion, a final group of 66 papers were selected for appraisal, all of which were primary research
studies. The search strategy for part B yielded 1116 articles. From these 192 articles identified as
potentially eligible for inclusion, a final group of 35 papers were selected for appraisal, all but one of
which were primary research
Key results
Accuracy of screening methods
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Maternal age alone is not an appropriate screening test for DS.
Screening methods that combine tests in an independent manner are not recommended.
The quad test provided the best screening performance characteristics in the 2nd trimester.
The combined test performed better than other 1st trimester and all 2nd trimester strategies, and
serum integrated screening had a similar performance to the combined test.
All other integrated and sequential screening strategies have improved performance compared to
either 1st trimester or 2nd trimester screening strategies. Fully integrated screening performed
marginally better than both stepwise and contingent screening, with a lower FPR for a fixed DR.
The performance of stepwise and contingent screening is similar.
Difficulties implementing any screening strategies
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NT measurement not being successful or taking more time than expected.
NT requiring trained staff, high quality equipment, and quality control.
Women defaulting from 2nd trimester maternal serum screening.
Need to adjust for maternal weight, and for false positive results in previous pregnancies.
Need for USS dating.
Issues with serum marker reliability (assay drift, and inaccurate marker MoM).
Inappropriate model parameters giving inaccurate risk estimates.
Unique issues with screening in twin pregnancies.
Uptake of invasive testing following receipt of screening results
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Maternal age (<35 years versus ≥ 35 years) appears to be a factor in the uptake of invasive testing
following screening. Younger and older women may perceive their risk differently and utilise DS
screening for different reasons.
Women’s individual estimates of calculated risk appear to influence the uptake of invasive testing,
with an increase in the uptake of invasive testing as the likelihood of carrying a fetus with DS
increases.
Perceived accuracy of the screening test and social, ethnic and cultural factors may influence
uptake and a local study of the acceptability of both screening and invasive testing is needed.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
198
Changes in the rate of invasive testing with the introduction of a screening programme
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Overall, rates of invasive testing increased slightly with the introduction of screening programmes.
This was against the backdrop of a steeper rise in maternal age and the increase in invasive testing
was less than what would be expected if invasive tests were offered based on maternal age alone.
Changes in rates of invasive testing varied as a function of maternal age. Rates of invasive testing
decreased among older mothers (≥ 35 years) and increased among younger mothers (< 35 years)
with the introduction of a screening programme.
Safety of amniocentesis and chorionic villus sampling
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A high quality systematic review confirmed that a 1% increased risk of fetal loss (against a
background risk of 2%) following amniocentesis in a low risk population is the best estimate of the
rate of procedure-related loss.
The recommendations of the review were that prenatal diagnosis is safest performed in the second
trimester by amniocentesis, which is safer than both transcervical CVS and first trimester
amniocentesis. Transabdominal CVS is the safest method for first trimester prenatal diagnosis,
followed by transcervical CVS.
CONCLUSIONS
Amongst the papers identified to assess the validity of DS screening methods the evidence indicated
that integrated and sequential screening had superior screening performance compared to screening
confined to either 1st or 2nd trimester. The choice of screening method should be selected from
integrated or sequential strategies (fully integrated, contingent or stepwise screening).
The gestational age at which the serum sample is taken or NT measured, has an affect on the validity of
the screening test. For example in the SURUSS study (Wald et al. 2003b) the combined test performed
better at 10/40 than at 13/40. The evidence for the optimum timing of screening tests was not
considered as part of this review, but this would need careful consideration by policy makers when
implementing a Down syndrome screening programme.
The optimum risk cut-off, for determining whether a screening result was screen positive or screen
negative, is also outside the scope of this review. The cut-offs for contingent screening is particularly
complicated as a first trimester high and low risk cut-off, and a 2nd trimester cut-off need to be
determined, and each will effect screening performance.
Papers that compared the same screening method before and after an adjustment (e.g. for maternal
weight) were not included in the review unless they also included a comparison with another screening
method fitting the review protocol criteria. Possible adjustments in Down syndrome screening include:
maternal weight, which is now a standard component of screening strategies (Spencer et al. 2003a);
smoking status (Spencer et al. 2004); and ethnicity (Spencer et al. 2005).
The evidence considered for the assessment of validity of DS screening tests exhibited methodological
limitations including:
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case-control studies used to determine validity of screening methods (therefore sample not
necessarily representative of the potential screening population)
studies with small sample sizes (and therefore small number of DS cases) which will limit the
accuracy of the estimates of DR and FPR
no details of parameters used or inappropriate parameters used for Gaussian distribution
no blinding of investigators to pregnancy outcomes (case-control studies and retrospective analysis
of stored samples)
use of intervention studies particularly in comparing 1st trimester and 2nd trimester screening (for
example where NT used clinically before 2nd trimester)
population already screened for DS by another method
not accounting for all fetal loss and/or few details of how live birth outcomes were obtained
some modelling papers using the same primary data, similar modelling techniques, and similar
assumptions which may mean the same or similar results are replicated.
The omission of studies published prior to 2000 may cause publication bias, as some of these papers
will contain evidence relevant to this review. However, integrated screening was not described until
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
199
1999 (Wald et al. 2006c), and the majority of papers comparing integrated and sequential screening
with each other and/or with first and second trimester methods have been published during or after the
year 2000.
There are a number of considerations apart from the validity of a screening strategy which are
important when deciding between integrated or sequential screening strategies. While integrated
screening may have a better performance it does have some practical disadvantages when compared to
sequential screening strategies. One potential drawback is the need to withhold results of 1st trimester
screening until the 2nd trimester, and the resulting delay in diagnosis of DS until the 2nd trimester. This
may not be acceptable to women or clinicians (Lam et al. 2002). Another consideration is that all
women will need both 1st and 2nd trimester screening for integrated screening, while for stepwise and
contingent screening most DS cases will be detected in the 1st trimester and fewer women will need to
have 2nd trimester screening (Palomaki et al. 2006).
Another consideration is that if women default from 2nd trimester screening and the intention has been
for them to have integrated screening, they will only have had a PAPP-A and NT assayed in the 1st
trimester, as opposed to contingent or stepwise screening when they would have had the combined test.
However, fβhCG could be measured in any left over serum sample in this instance, allowing a
combined test to be completed (Wald et al. 2006c).
Stepwise and contingent strategies also have some disadvantages. For both stepwise and contingent
strategies women will be given more than one risk estimate which may be confusing and distressing
(Lam et al. 2002). While integrated screening avoids detecting DS cases that would have miscarried
between 1st trimester and 2nd trimester (Lam et al. 2002), stepwise or contingent strategies will detect
these cases and will involve ToPs that may not have been necessary. The design of contingent
screening is complicated and screening planners need to choose three risk cut-off levels for this
screening: a very low and very high cut-off based on 1st trimester results, and a final cut-off based on
all markers after 2nd trimester serum screening (Benn et al. 2005a; Wright et al. 2006). Also, integrated
screening has the advantage of allowing all women to have 2nd trimester screening for neural tube
defects as all women will have AFP in the 2nd trimester (Lam et al. 2002).
Sequential screening and integrated screening have not yet been implemented in large population-based
screening programmes (Wald et al. 2006c) and so some issues with their implementation may not yet
be apparent. Policy makers may need to await the results of any evaluation of the implementation of
such screening programmes.
The implications of resources for training, monitoring and quality control particularly for NT testing
would need to be carefully considered when determining whether a screening programme should
proceed. It has been suggested that in the UK, implementation of a screening programme including NT
measurement may be difficult due to a shortage of well trained ultrasonographers and because of issues
with quality assurance (Neilson and Alfirevic 2006).
It will also be important to ensure software is able to accurately determine an individual’s risk of DS,
including calculation of correct MoMs, adjustments (including for maternal weight, false positive
results from previous pregnancies) and use of appropriate population parameters for Gaussian
distributions. Also, USS should be used to estimate gestational age.
Amongst the papers identified to assess the uptake of invasive testing following a positive or negative
screening result for DS risk, it appears that both maternal age and individual risk estimates are both
factors in women’s decisions to opt for invasive testing or not. Younger and older mothers may
perceive their level of risk differently and so utilise screening for different reasons. These perceptions
and motivations may then effect the decisions they make based on their screening results. Other factors
may also play a part, such as perceived confidence in the accuracy of the screening test, and there
seems to be culturally-based variation in the uptake of both screening and invasive testing.
The overall rate of invasive testing seems to increase slightly with the introduction of a screening
programme but when examined by maternal age group, it appears that the rate of invasive testing
increases in younger mothers and decreases in older mothers. If the proportion of older mothers
accepting invasive testing declines with the introduction of a screening programme, changing patterns
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
200
in maternal age are likely to be an important determinant of invasive testing rates if such a programme
was to be introduced. Long-term evaluations of population-based screening programmes using
integrated and sequential methods have not been completed as yet, so the effects of these strategies on
invasive testing rates are unclear at this stage. Relative to a screening programme based on maternal
age alone, the introduction of first or second trimester screening methods decreases the rate of
unnecessary invasive procedures. Again, social, ethnic and cultural variability in the acceptability of
screening and invasive testing is a factor in the impact of screening policy changes. Because of this
variability, a local study investigating the acceptability of screening and invasive testing in older and
younger mothers of different ethnic backgrounds is needed before implementing a large-scale
screening programme in New Zealand.
The findings of the papers identified to assess the rate of fetal loss associated with invasive prenatal
diagnosis were inconclusive. There were several limitations in the studies including non-randomised
allocation to groups, failure to exclude or control for existing conditions and significant differences
between the study and comparison groups in age and maternal serum levels. The only completely
randomised study found a 1% increased risk of fetal loss following second trimester amniocentesis and
this estimate still stands as the best indication of procedure-related loss in a low risk population. Other
complications have been investigated in relation to amniocentesis and CVS, such as infection, amniotic
fluid leakage, vaginal bleeding, needle injury to the fetus and orthopaedic problems in infancy and
childhood; however these were beyond the scope of this review. No studies were identified in the
search which investigated interventions to reduce rates of fetal loss. However, best practice guidelines
recommend the use of concurrent ultrasound guidance and well-trained and experienced operators for
both amniocentesis and CVS (RANZCOG, 2004). The recommendations of a systematic review
(Alfirevic et al. 2006) included information about the most appropriate procedure for each gestational
age and the relative safety of each method of needle insertion (transcervical or transabdominal).
While this review is concerned with the validity of screening strategies and difficulties implementing
screening, there are a number of other considerations when deciding on which screening strategy to use
for DS screening. These include cost, availability of different screening tests, and the acceptability of
screening for clinicians and women, including the acceptability for women of different ethnicities. A
woman’s decision to undergo screening or invasive testing could be influenced on a societal level by
cultural, ethnic, religious, and social factors and on a personal level by previous pregnancy history,
personal values and beliefs, and the advice of family, friends and her health provider. Another
consideration is the gestational age at which women need to attend for screening. In the USA, only
75% to 80% of women present in the first trimester for antenatal care (Fuchs and Peipert 2005). In New
Zealand women choose a lead maternity carer (usually a midwife rather than a GP) and if this choice is
delayed beyond the appropriate gestational window there will be major implications for DS screening.
There are also other promising screening tests/diagnostic tests which policy makers should be aware of.
Other ultrasound markers such as absence of nasal bone, abnormal ductus venosus flow, and tricuspid
regurgitation are being assessed (Neilson and Alfirevic 2006) and researchers are continuing to
investigate the use of fetal cells in maternal circulation as a “non-invasive” diagnostic test for antenatal
DS.
Further research should address limitations in study design demonstrated in this review. Where
possible, research on the accuracy of screening for DS should be based on large prospective cohort
studies (or nested case-control studies). However, the current evidence based on the accuracy of
screening supports the use of fully integrated, contingent or stepwise screening. If women present in
the 2nd trimester the quad test is best and if women request screening only in the 1st trimester, the
combined test has the best performance (Wald et al. 2003b).
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
201
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SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
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Appendix 1: Search Strategies
SEARCH STRATEGIES
Medline
1
2
3
4
5
6
7
8
9
10
11
12
13
14
15
16
17
18
19
20
21
22
23
24
25
26
27
28
29
30
31
32
Downs syndrome/ (5152)
trisomy 21.mp. (1407)
1 or 2 (5529)
Pregnancy Trimester, First/ (3620)
Nuchal Translucency Measurement/ (138)
Pregnancy Trimester, Second/ (3504)
exp prenatal diagnosis/ (18671)
Pregnancy-Associated Plasma Protein-A/ (362)
Chorionic Gonadotropin, beta Subunit, Human/ (1289)
alpha-Fetoproteins/ (2914)
estriol/bl (293)
inhibins/bl (753)
papp-a.tw. (290)
beta hcg.tw. (903)
uE3.tw. (97)
(unconjugated oestriol or unconjugated estriol).tw. (201)
inhibin a.tw. (599)
afp.tw. (2476)
((integrated or sequential or contingent or step-wise) adj (screen$ or test$)).mp. (270)
ultrasonography, prenatal/ (10659)
Maternal Age/ (4280)
or/4-21 (31726)
mass screening/ (25674)
False Positive Reactions/ (6544)
false negative reactions/ (4337)
(screen$ or test$).mp. (846205)
or/23-26 (850494)
3 and 22 and 27 (1439)
limit 28 to english (1314)
limit 29 to yr=2000-2006 (784)
(letter or news).pt. (318032)
30 not 31 (712)
Medline 2
1
2
3
4
5
6
7
8
9
10
11
12
13
Downs syndrome/ (5207)
trisomy 21.mp. (1424)
Chromosomes, Human, Pair 21/ (1693)
trisomy/ (2631)
3 and 4 (153)
1 or 2 or 5 (5640)
amniocentesis/ (1581)
Chorionic Villi Sampling/ (720)
chorionic villus.mp. (101)
exp Karyotyping/ (11568)
or/7-10 (13229)
6 and 11 (649)
limit 12 to yr=2000-2006 (367)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
208
Embase
1
2
3
4
5
6
7
8
9
10
11
12
13
14
15
16
17
18
19
20
21
22
23
24
25
26
27
28
29
30
31
32
Downs syndrome/ (5796)
trisomy 21.mp. (2002)
1 or 2 (6917)
fetus echography/ (5445)
First Trimester Pregnancy/ (5389)
Second Trimester Pregnancy/ (3712)
Maternal Serum/ (1089)
Alpha Fetoprotein/ (4868)
Inhibin A/ (691)
papp-a.tw. (550)
beta hcg.mp. (873)
uE3.tw. (110)
(unconjugated oestriol or unconjugated estriol).tw. (200)
Maternal Age/ (4165)
(nuchal translucency or nuchal fold).tw. (877)
exp Prenatal Diagnosis/ (20616)
Pregnancy Associated Plasma Protein A/ (410)
Chorionic Gonadotropin Beta Subunit/ (2095)
((integrated or sequential or contingent or stepwise) adj (screen$ or test$)).tw. (316)
inhibin a.tw. (1921)
or/4-20 (37859)
Screening Test/ (17624)
Mass Screening/ (5299)
(screen$ or test$).mp. (795108)
Prenatal Screening/ (2369)
screening/ (18303)
or/22-26 (795108)
3 and 21 and 27 (1612)
limit 28 to yr=2000-2006 (1039)
limit 29 to english (929)
letter.pt. (203923)
30 not 31 (848)
Embase 2
1
2
3
4
5
6
7
8
9
10
11
Downs syndrome/ (5916)
Trisomy 21/ (1684)
1 or 2 (6902)
exp amniocentesis/ (3374)
chorion villus sampling/ (983)
chorionic vill$.mp. (1306)
karyotyping/ (2675)
fetus karyotyping/ (251)
or/4-8 (7120)
3 and 9 (814)
limit 10 to yr=2000-2006 (551)
Cochrane Central Register of Controlled Trials
1
2
3
4
5
6
7
8
9
Downs syndrome/ (121)
trisomy 21.mp. (15)
1 or 2 (123)
Pregnancy Trimester, First/ (339)
Nuchal Translucency Measurement/ (2)
Pregnancy Trimester, Second/ (334)
exp prenatal diagnosis/ (383)
Pregnancy-Associated Plasma Protein-A/ (3)
Chorionic Gonadotropin, beta Subunit, Human/ (40)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
209
10 alpha-Fetoproteins/ (73)
11 estriol/bl (22)
12 inhibins/bl (33)
13 papp-a.tw. (7)
14 beta hcg.tw. (61)
15 uE3.tw. (1)
16 (unconjugated oestriol or unconjugated estriol).tw. (10)
17 inhibin a.tw. (68)
18 afp.tw. (76)
19 ((integrated or sequential or contingent or step-wise) adj (screen$ or test$)).mp. (31)
20 ultrasonography, prenatal/ (222)
21 Maternal Age/ (143)
22 or/4-21 (1355)
23 down$ syndrome.mp. (179)
24 3 or 23 (180)
25 22 and 24 (28)
26 limit 25 to yr=2000-2006 (11)
Cochrane Central Register of Controlled Trials 2
1
2
3
4
5
6
7
8
9
10
11
12
13
Downs syndrome/ (124)
trisomy 21.mp. (15)
Chromosomes, Human, Pair 21/ (14)
trisomy/ (12)
3 and 4 (2)
1 or 2 or 5 (128)
amniocentesis/ (88)
Chorionic Villi Sampling/ (50)
chorionic villus.mp. (0)
exp Karyotyping/ (88)
or/7-10 (172)
6 and 11 (7)
limit 12 to yr=2000-2006 (3)
Cinahl
1 Downs syndrome/ (1171)
2 trisomy 21.mp. (59)
3 down$ syndrome.tw. (863)
4 or/1-3 (1280)
5 (screen$ or test$).mp. (182249)
6 false positive$.mp. or false negative$.tw. [mp=title, subject heading word, abstract,
instrumentation] (1714)
7 (false positive$ or false negative$).mp. (1881)
8 or/5-7 (182762)
9 Pregnancy Trimester, First/ (410)
10 Pregnancy Trimester, Second/ (381)
11 exp Prenatal Diagnosis/ (2412)
12 exp Ultrasonography, Prenatal/ (1119)
13 (nuchal translucency or nuchal fold).mp. (51)
14 pregnancy associated plasma protein a.mp. (12)
15 papp-a.mp. (7)
16 Gonadotropins, Chorionic/ (201)
17 beta hcg.tw. (29)
18 Alpha Fetoproteins/ (131)
19 ESTRIOL/bl [Blood] (21)
20 inhibin a.mp. (9)
21 (uE3 or unconjugated oestriol or unconjugated estriol).tw. (16)
22 afp.tw. (74)
23 Maternal Age/ (591)
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
210
24
25
26
27
28
29
30
(integrated or sequential or contingent or step wise).tw. (8005)
or/9-24 (11580)
4 and 8 and 25 (252)
limit 26 to yr=2000-2006 (184)
limit 27 to english (183)
letter.pt. (33692)
28 not 29 (179)
Cinahl 2
1
2
3
4
5
6
7
8
9
10
11
12
13
Downs syndrome/ (1187)
trisomy 21.mp. (60)
Chromosomes, Human, Pair 21/ (0)
trisomy/ (0)
3 and 4 (0)
1 or 2 or 5 (1205)
amniocentesis/ (314)
Chorionic Villi Sampling/ (95)
chorionic villus.mp. (1)
exp Karyotyping/ (60)
or/7-10 (391)
6 and 11 (80)
limit 12 to yr=2000-2006 (58)
Psychinfo
1
2
3
4
5
6
7
8
exp Downs syndrome/ (933)
trisomy 21.mp. (44)
1 or 2 (938)
amniocentesis.mp. (45)
karyotyping.mp. (10)
chorion$ vill$.mp. (3)
or/4-6 (56)
3 and 7 (8)
Current Contents
1.
2.
3.
4.
5.
6.
7.
8.
9.
10.
11.
12.
13.
14.
15.
16.
17.
18.
19.
20.
21.
22.
Downs syndrome
Down’s syndrome
Trisomy 21
#1 OR #2 OR #3
Screen*
Testing
Tests
#4 AND (#5 OR #6 OR #7)
First trimester OR second trimester
Nuchal translucency OR nuchal fold
Pregnancy associated plasma protein a OR papp-a
(Human chorionic gonadotropn SAME beta) OR beta hcg
Alpha fetoproteins OR alha foetoproteins OR afp
Inhibin a
(integrated OR sequential OR continugent OR stepwise) SAME (screen* OR test*)
Prenatal SAME (ultrasonography OR ultrasound)
Unconjugated estriol OR uncongugated oestriol or ue3
Maternal age
#9 OR #10 OR #11 OR #12 OR #13 OR #14 OR #15 OR #16 OR #17 OR #18
#8 AND #19
false positive OR false negative
#8 AND #21
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
211
23. #20 OR #22
Current Contents 2
1.
2.
3.
4.
5.
6.
Downs syndrome OR trisomy 21
Amniocentesis
Karyotyp*
chorionic villus OR chorionic villi OR chorionic villus
#2 OR #3 OR #4
#1 AND #5
SEARCHES FROM OTHER SOURCES
In databases and all other sources without controlled vocabulary combinations of the index terms and
additional keywords from the above strategies were used in the search.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
212
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
213
Appendix 2: Sources searched
SOURCES SEARCHED
Bibliographic databases
Medline
Embase
Cinahl
Psychinfo
Current Contents
Cochrane Central Register of Controlled Trials
Index New Zealand
PubMed (last 60 days)
Review databases
ACP Journal Club – via Ovid
Cochrane Database of Systematic Reviews – (Wiley Interscience version)
Database of Abstracts of Reviews of Effectiveness - http://www.crd.york.ac.uk/crdweb/
NHS Economic Evaluation database http://www.crd.york.ac.uk/crdweb/
Health Technology Assessment database http://www.crd.york.ac.uk/crdweb/
Evidence-based collections
TRIP Database http://www.tripdatabase.com
ATTRACT http://www.attract.wales.nhs.uk
NHS Technology Assessment Programme http://www.hta.nhsweb.nhs.uk/
(UK) National Institute for Health & Clinical Excellence http://www.nice.org.uk
Other
UK National Screening Committee Down’s Syndrome Screening Programme
http://www.screening.nhs.uk/downs/home.htm
Clinical Trials.gov http://www.clinicaltrials.gov
Current Controlled Trials http://www.controlled-trials.com
References of retrieved papers were scanned for relevant publications
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
214
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
215
Appendix 3 Retrieved studies
excluded for review : Part A
Anonymous. (2003). First trimester ultrasound identifies more cases of Down syndrome than second
trimester maternal serum screening and is more cost effective. Research Activities, 273, 8-9.
Acacio, G. L., Barini, R., Pinto Junior, W., Ximenes, R. L., Pettersen, H., & Faria, M. (2001). Nuchal
translucency: an ultrasound marker for fetal chromosomal abnormalities. Sao Paulo Medical
Journal = Revista Paulista de Medicina, 119, 19-23.
Akbas, S. H., Ozben, T., Alper, O., Ugur, A., Yucel, G., & Luleci, G. (2001). Maternal serum
screening for Down's syndrome, open neural tube defects and trisomy 18. Clinical Chemistry
& Laboratory Medicine, 39, 487-490.
Bahado-Singh, R., Shahabi, S., Karaca, M., Mahoney, M. J., Cole, L., & Oz, U. A. (2002). The
comprehensive midtrimester test: high-sensitivity Down syndrome test. American Journal of
Obstetrics & Gynecology, 186, 803-808.
Bahado-Singh, R. O., & Cheng, C. S. (2004). First trimester prenatal diagnosis. Current Opinion in
Obstetrics & Gynecology, 16, 177-181.
Bahado-Singh, R. O., Mendilcioglu, I., Rowther, M., Choi, S. J., Oz, U., Yousefi, N. F., & Mahoney,
M. J. (2002). Early genetic sonogram for Down syndrome detection. American Journal of
Obstetrics & Gynecology, 187, 1235-1238.
Bahado-Singh, R. O., Oz, U., Shahabi, S., Mahoney, M. J., Baumgarten, A., & Cole, L. A. (2000).
Comparison of urinary hyperglycosylated human chorionic gonadotropin concentration with
the serum triple screen for Down syndrome detection in high-risk pregnancies. American
Journal of Obstetrics & Gynecology, 183, 1114-1118.
Ball, R. H. (2004). Invasive fetal testing. Current Opinion in Obstetrics & Gynecology, 16, 159-162.
Beaman, J. M., & Goldie, D. J. (2001). Second trimester screening for Down's syndrome: 7 years
experience. Journal of Medical Screening, 8, 128-131.
Benn, P. A., Egan, J. F. X., & Ingardia, C. J. (2002). Extreme second-trimester serum analyte values in
Down syndrome pregnancies with hydrops fetalis. Journal of Maternal-Fetal & Neonatal
Medicine, 11, 262-265.
Bersinger, N. A., Vanderlick, F., Birkhauser, M. H., Janecek, P., & Wunder, D. (2005). First trimester
serum concentrations of placental proteins in singleton and multiple IVF pregnancies:
Implications for Down syndrome screening. Immuno-Analyse et Biologie Specialisee, 20, 2127.
Bersinger, N. A., Wunder, D., Vanderlick, F., Chanson, A., Pescia, G., Janecek, P., Boillat, E., & et al.
(2004). Maternal serum levels of placental proteins after in vitro fertilisation and their
implications for prenatal screening. Prenatal Diagnosis, 24, 471-477.
Bianchi, D. W. (2004). Circulating fetal DNA: its origin and diagnostic potential-a review. Placenta,
25 Suppl A, S93-S101.
Biggio, J. R., Jr., Morris, T. C., Owen, J., & Stringer, J. S. (2004). An outcomes analysis of five
prenatal screening strategies for trisomy 21 in women younger than 35 years. American
Journal of Obstetrics & Gynecology, 190, 721-729.
Bindra, R., Heath, V., Liao, A., Spencer, K., & Nicolaides, K. H. (2002). One-stop clinic for
assessment of risk for trisomy 21 at 11-14 weeks: a prospective study of 15 030 pregnancies.
Ultrasound in Obstetrics & Gynecology, 20, 219-225.
Borrell, A., Casals, E., Fortuny, A., Farre, M. T., Gonce, A., Sanchez, A., Soler, A., et al. (2004). Firsttrimester screening for trisomy 21 combining biochemistry and ultrasound at individually
optimal gestational ages. An interventional study. Prenatal Diagnosis, 24, 541-545.
Borruto, F., Comparetto, C., Acanfora, L., Bertini, G., & Rubaltelli, F. F. (2002). Role of ultrasound
evaluation of nuchal translucency in prenatal diagnosis. Clinical & Experimental Obstetrics &
Gynecology, 29, 235-241.
Brigatti, K. W., & Malone, F. D. (2004). First-trimester screening for aneuploidy. Obstetrics &
Gynecology Clinics of North America, 31, 1-20.
Brizot, M. L., Carvalho, M. H., Liao, A. W., Reis, N. S., Armbruster-Moraes, E., & Zugaib, M. (2001).
First-trimester screening for chromosomal abnormalities by fetal nuchal translucency in a
Brazilian population. Ultrasound in Obstetrics & Gynecology, 18, 652-655.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
216
Canini, S., Prefumo, F., Famularo, L., Venturini, P. L., Palazzese, V., & De Biasio, P. (2002).
Comparison of first trimester, second trimester and integrated Down's syndrome screening
results in unaffected pregnancies. Clinical Chemistry & Laboratory Medicine, 40, 600-603.
Celentano, C., Guanciali-Franchi, P. E., Liberati, M., Palka, C., Fantasia, D., Morizio, E., Calabrese, et
al. (2005). Lack of correlation between elevated maternal serum hCG during second-trimester
biochemical screening and fetal congenital anomaly. Prenatal Diagnosis, 25, 220-224.
Centini, G., Rosignoli, L., Kenanidis, A., Talluri, B., Pasqui, L., Scarinci, R., De Simone, S., et al.
(2004). Can a selective use of amniocentesis replace the routine procedure for advanced
maternal age? Italian Journal of Gynaecology & Obstetrics, 16, 27-31.
Centini, G., Rosignoli, L., Scarinci, R., Faldini, E., Morra, C., Centini, G., & Petraglia, F. (2005). Reevaluation of risk for Down syndrome by means of the combined test in pregnant women of
35 years or more. Prenatal Diagnosis, 25, 133-136.
Cha, D. H., Khosrotehrani, K., Bianchi, D. W., & Johnson, K. L. (2005). The utility of an erythroblast
scoring system and gender-independent short tandem repeat (STR) analysis for the detection
of aneuploid fetal cells in maternal blood. Prenatal Diagnosis, 25, 586-591.
Chasen, S. T., Sharma, G., Kalish, R. B., & Chervenak, F. A. (2003). First-trimester screening for
aneuploidy with fetal nuchal translucency in a United States population. Ultrasound in
Obstetrics & Gynecology, 22, 149-151.
Chen, C. P., Lin, C. J., & Wang, W. (2005). Impact of second-trimester maternal serum screening on
prenatal diagnosis of Down syndrome and the use of amniocentesis in the Taiwanese
population. Taiwanese Journal of Obstetrics & Gynecology, 44, 31-35.
Chen, M., Lam, Y. H., Lee, C. P., & Tang, M. H. Y. (2004). Ultrasound screening of fetal structural
abnormalities at 12 to 14 weeks in Hong Kong. Prenatal Diagnosis, 24, 92-97.
Cheng, C. C., Bahado-Singh, R. O., Chen, S. C., & Tsai, M. S. (2004). Pregnancy outcomes with
increased nuchal translucency after routine Down syndrome screening. International Journal
of Gynaecology & Obstetrics, 84, 5-9.
Cheng, P. J., Chu, D. C., Chueh, H. Y., See, L. C., Chang, H. C., & Weng, D.-H. (2004). Elevated
maternal midtrimester serum free beta-human chorionic gonadotropin levels in vegetarian
pregnancies that cause increased false-positive Down syndrome screening results. American
Journal of Obstetrics & Gynecology, 190, 442-447.
Christiansen, M., Hogdall, E. V., Larsen, S. O., & Hogdall, C. (2002). The variation of risk estimates
through pregnancy in second trimester maternal serum screening for Down syndrome.
Prenatal Diagnosis, 22, 385-387.
Christiansen, M., Larsen, S. O., Oxvig, C., Qin, Q. P., Wagner, J. M., Overgaard, M. T., Gleich, G. J.,
et al. (2004). Screening for Down's syndrome in early and late first and second trimester using
six maternal serum markers. Clinical Genetics, 65, 11-16.
Christiansen, M., & Norgaard-Pedersen, B. (2005). Inhibin A is a maternal serum marker for Down's
syndrome early in the first trimester. Clinical Genetics, 68, 35-39.
Cicero, S., Bindra, R., Rembouskos, G., Spencer, K., & Nicolaides, K. H. (2003). Integrated ultrasound
and biochemical screening for trisomy 21 using fetal nuchal translucency, absent fetal nasal
bone, free beta-hCG and PAPP-A at 11 to 14 weeks. Prenatal Diagnosis, 23, 306-310.
Cole, L. A., Sutton, J. M., & Stephens, N. D. (2003). Invasive trophoblast antigen (ITA): a new highsensitivity test for detecting gestational Down syndrome. Journal of Clinical Ligand Assay,
26, 121-128.
Comas, C., Antolin, E., Torrents, M., Mun~oz, A., Figueras, F., Echevarria, M., Gomez, O., et al.
(2001). Early screening for chromosomal abnormalities: new strategies combining
biochemical, sonographic and doppler parameters. Prenatal & Neonatal Medicine, 6, 95-102.
Comas, C., Torrents, M., Munoz, A., Antolin, E., Figueras, F., & Echevarria, M. (2002). Measurement
of nuchal translucency as a single strategy in trisomy 21 screening: should we use any other
marker? Obstetrics & Gynecology, 100, 648-654.
Crossley, J. A., Aitken, D. A., Waugh, S. M., Kelly, T., & Connor, J. M. (2002). Maternal smoking:
age distribution, levels of alpha-fetoprotein and human chorionic gonadotrophin, and effect on
detection of Down syndrome pregnancies in second-trimester screening. Prenatal Diagnosis,
22, 247-255.
Cuckle, H., Aitken, D., Goodburn, S., Senior, B., Spencer, K., Standing, S., & UK National Down's
Syndrome Screening Programme, L. A. G. (2004). Age-standardisation when target setting
and auditing performance of Down syndrome screening programmes. Prenatal Diagnosis, 24,
851-856.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
217
Cusick, W., Buchanan, P., Hallahan, T. W., Krantz, D. A., Larsen, J. W., Jr., & Macri, J. N. (2003).
Combined first-trimester versus second-trimester serum screening for Down syndrome: a cost
analysis. American Journal of Obstetrics & Gynecology, 188, 745-751.
DeVore, G. R. (2001). The genetic sonogram: its use in the detection of chromosomal abnormalities in
fetuses of women of advanced maternal age. Prenatal Diagnosis, 21, 40-45.
DeVore, G. R., & Romero, R. (2002). Genetic sonography: a cost-effective method for evaluating
women 35 years and older who decline genetic amniocentesis. Journal of Ultrasound in
Medicine, 21, 5-13.
DeVore, G. R., & Romero, R. (2003). Genetic sonography: an option for women of advanced maternal
age with negative triple-marker maternal serum screening results. Journal of Ultrasound in
Medicine, 22, 1191-1199.
Dixon, J., Pillai, M., Mahendran, D., & Brooks, M. (2004). An assessment of the Down syndrome
antenatal screening policies of East and West Gloucestershire between 1993 and 1999.
Journal of Obstetrics & Gynaecology, 24, 760-764.
Dormandy, E., Hooper, R., Michie, S., & Marteau, T. M. (2002). Informed choice to undergo prenatal
screening: a comparison of two hospitals conducting testing either as part of a routine visit or
requiring a separate visit. Journal of Medical Screening, 9, 109-114.
Drysdale, K., Ridley, D., Walker, K., Higgins, B., & Dean, T. (2002). First-trimester pregnancy
scanning as a screening tool for high-risk and abnormal pregnancies in a district general
hospital setting. Journal of Obstetrics & Gynaecology, 22, 159-165.
Egan, J. F., Benn, P., Borgida, A. F., Rodis, J. F., Campbell, W. A., & Vintzileos, A. M. (2000).
Efficacy of screening for fetal Down syndrome in the United States from 1974 to 1997.
Obstetrics & Gynecology, 96, 979-985.
Egan, J. F., Malakh, L., Turner, G. W., Markenson, G., Wax, J. R., & Benn, P. A. (2001). Role of
ultrasound for Down syndrome screening in advanced maternal age. American Journal of
Obstetrics & Gynecology, 185, 1028-1031.
Falcon, O., Auer, M., Gerovassili, A., Spencer, K., & Nicolaides, K. H. (2006). Screening for trisomy
21 by fetal tricuspid regurgitation, nuchal translucency and maternal serum free beta-hCG and
PAPP-A at 11 + 0 to 13 + 6 weeks. Ultrasound in Obstetrics & Gynecology, 27, 151-155.
Fortuny, A., Borell, A., Casals, E., Seres, A., Sanchez, A., & Soler, A. (2005). First trimester
aneuploidy screening combining biochemical and ultrasound markers. Ultrasound Review of
Obstetrics & Gynecology, 5, 9-17.
Ghisoni, L., Ferrazzi, E., Castagna, C., Levi Setti, P. E., Masini, A. C., & Pigni, A. (2003). Prenatal
diagnosis after ART success: the role of early combined screening tests in counselling
pregnant patients. Placenta, 24, S99-S103.
Goldberg, J. D. (2004). Routine screening for fetal anomalies: expectations. Obstetrics & Gynecology
Clinics of North America, 31, 35-50.
Green, J. M., Hewison, J., Bekker, H. L., Bryant, L. D., & Cuckle, H. S. (2004). Psychosocial aspects
of genetic screening of pregnant women and newborns: A systematic review. Health
Technology Assessment (Winchester, England), 8, iii-87.
Hadlow, N. C., Hewitt, B. G., Dickinson, J. E., Jacoby, P., & Bower, C. (2005). Community-based
screening for Down's Syndrome in the first trimester using ultrasound and maternal serum
biochemistry. BJOG: An International Journal of Obstetrics & Gynaecology, 112, 1561-1564.
Harris, A. H. (2004). The cost effectiveness of prenatal ultrasound screening for trisomy 21.
International Journal of Technology Assessment in Health Care, 20, 464-468.
Has, R., Kalelioglu, I., Ermis, H., Ibrahimoglu, L., Yuksel, A., Yildirim, A., & Basaran, S. (2006).
Screening for fetal chromosomal abnormalities with nuchal translucency measurement in the
first trimester. Fetal Diagnosis and Therapy, 21, 355-359.
Herman, A., Dreazen, E., Herman, A. M., Batukan, C. E., Holzgreve, W., & Tercanli, S. (2002).
Bedside estimation of Down syndrome risk during first-trimester ultrasound screening.
Ultrasound in Obstetrics & Gynecology, 20, 468-475.
Hsu, J. J., Chiang, C. H., Hsieh, C. C., & Hsieh, T. T. (2004). The influence of image magnification in
first-trimester screening for Down syndrome by fetal nuchal translucency in Asians. Prenatal
Diagnosis, 24, 1007-1012.
Hulten, M. (2004). Combined serum and nuchal translucency screening in the first trimester achieves
85% to 90% detection rate for Down and Edward syndromes. Evidence-Based Healthcare, 8,
82-84.
Hung, J. H., Fu, C. Y., Yuan, C. C., Chen, C. L., Yang, M. L., Shu, L. P., & Wu, C. C. (2003). Nuchal
translucence incorporated into a one-stage multifactorial screening model for Down syndrome
prediction at second-trimester pregnancy. Ultrasound in Medicine & Biology, 29, 1667-1674.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
218
Hwa, H. L., Yen, M. F., Hsieh, F. J., Ko, T. M., & Chen, T. H. (2004). Evaluation of second trimester
maternal serum screening for Down's Syndrome using the Spiegelhalter-Knill-Jones (S-KJ)
approach. Journal of Perinatal Medicine, 32, 407-412.
Jaques, A. M., Collins, V. R., Haynes, K., Sheffield, L. J., Francis, I., Forbes, R., & Halliday, J. L.
(2006). Using record linkage and manual follow-up to evaluate the Victorian maternal serum
screening quadruple test for Down's syndrome, trisomy 18 and neural tube defects. Journal of
Medical Screening, 13, 8-13.
Jou, H. J., Shyu, M. K., Chen, S. M., Shih, J. C., Hsu, J. J., & Hsieh, F. J. (2000). Maternal serum
screening for down syndrome by using alpha-fetoprotein and human chorionic gonadotropin
in an asian population. a prospective study. Fetal Diagnosis & Therapy, 15, 108-111.
Kennelly, M., Carroll, S., & Parland, P. M. (2004). Nuchal translucency audit: low uptake of invasive
testing in screen positive cases. Irish Medical Journal, 97, 304-305.
Kim, M. H., Park, S. H., Cho, H. J., Choi, J. S., Kim, J. O., Ahn, H. K., Shin, J. S., et al. (2006).
Threshold of nuchal translucency for the detection of chromosomal aberration: comparison of
different cut-offs. Journal of Korean Medical Science, 21, 11-14.
Kim, S. K., Bai, S. W., Chung, J. E., Jung, Y. N., Park, K. H., Cho, D. J., Kim, J. W., Yang, Y. H., et
al. (2001). Triple marker screening for fetal chromosomal abnormalities in Korean women of
advanced maternal age. Yonsei Medical Journal, 42, 199-203.
Kishida, T., Hoshi, N., Hattori, R., Negishi, H., Yamada, H., Okuyama, K., Hanatani, K., et al. (2000).
Efficacy of maternal serum screening in the prenatal detection of fetal chromosome
abnormalities in Japanese women. Fetal Diagnosis & Therapy, 15, 112-117.
Krantz, D., Goetzl, L., Simpson, J. L., Thom, E., Zachary, J., Hallahan, T. W., Silver, R., et al. (2004).
Association of extreme first-trimester free human chorionic gonadotropin-beta, pregnancyassociated plasma protein A, and nuchal translucency with intrauterine growth restriction and
other adverse pregnancy outcomes. American Journal of Obstetrics & Gynecology, 191, 14521458.
Krantz, D. A., Hallahan, T. W., Macri, V. J., & Macri, J. N. (2005). Maternal weight and ethnic
adjustment within a first-trimester Down syndrome and trisomy 18 screening program.
Prenatal Diagnosis, 25, 635-640.
Kremensky, I., Jordanova, A., Michaylova, E., Todorova, A., Ivanova, M., Petkova, R., Andonova, S.,
et al. (2000). Laboratory diagnosis of inherited disorders and congenital anomalies in
Bulgaria. Balkan Journal of Medical Genetics, 3, 13-21.
Lai, T. H., Chen, S. C., Tsai, M. S., Lee, F. K., & Wei, C. F. (2003). First-trimester screening for Down
syndrome in singleton pregnancies achieved by intrauterine insemination. Journal of Assisted
Reproduction & Genetics, 20, 327-331.
Lambert-Messerlian, G., Dugoff, L., Vidaver, J., Canick, J. A., Malone, F. D., Ball, R. H., Comstock,
C. H., et al (2006). First- and second-trimester Down syndrome screening markers in
pregnancies achieved through assisted reproductive technologies (ART): a FASTER trial
study. Prenatal Diagnosis 26, 672-8 Epub ahead of print.
Lambert-Messerlian, G. M., & Canick, J. A. (2004). Clinical application of inhibin a measurement:
prenatal serum screening for Down syndrome. Seminars in Reproductive Medicine, 22, 235242.
Leung, T. Y., Spencer, K., Leung, T. N., Fung, T. Y., & Lau, T. K. (2006). Higher median levels of
free beta-hCG and PAPP-A in the first trimester of pregnancy in a Chinese ethnic group.
Implication for first trimester combined screening for Down's syndrome in the Chinese
population. Fetal Diagnosis & Therapy, 21, 140-143.
Lewis, S. M., Cullinane, F. M., Carlin, J. B., & Halliday, J. L. (2006). Women's and health
professionals' preferences for prenatal testing for Down syndrome in Australia. Australian and
New Zealand Journal of Obstetrics and Gynaecology, 46, 205-211.
Lewis, S. M., Cullinane, F. N., Bishop, A. J., Chitty, L. S., Marteau, T. M., & Halliday, J. L. (2006). A
comparison of Australian and UK obstetricians' and midwives' preferences for screening tests
for Down syndrome. Prenatal Diagnosis, 26, 60-66.
Lim, K. I., Pugash, D., Dansereau, J., & Wilson, R. D. (2002). Nuchal index: a gestational age
independent ultrasound marker for the detection of Down syndrome. Prenatal Diagnosis, 22,
1233-1237.
Liu, S. S., Lee, F. K., Lee, J. L., Tsai, M. S., Cheong, M. L., She, B. Q., & Chen, S. C. (2004).
Pregnancy outcomes in unselected singleton pregnant women with an increased risk of firsttrimester Down's syndrome. Acta Obstetricia et Gynecologica Scandinavica, 83, 1130-1134.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
219
Locatelli, A., Piccoli, M. G., Vergani, P., Mariani, E., Ghidini, A., Mariani, S., & Pezzullo, J. C.
(2000). Critical appraisal of the use of nuchal fold thickness measurements for the prediction
of Down syndrome. American Journal of Obstetrics & Gynecology, 182, 192-197.
MacRae, A. R., Gardner, H. A., Allen, L. C., Tokmakejian, S., & Lepage, N. (2003). Outcome
validation of the Beckman Coulter access analyzer in a second-trimester Down syndrome
serum screening application. Clinical Chemistry, 49, 69-76.
Malone, F. D. (2005). Nuchal translucency-based Down syndrome screening: barriers to
implementation. Seminars in Perinatology, 29, 272-276.
Malone, F. D., Ball, R. H., Nyberg, D. A., Comstock, C. H., Saade, G. R., Berkowitz, R. L., Gross, S.
et al. (2005). First-trimester septated cystic hygroma: prevalence, natural history, and pediatric
outcome. Obstetrics & Gynecology, 106, 288-294.
Malone, F. D., D'Alton, M. E., & Society for Maternal-Fetal, M. (2003). First-trimester sonographic
screening for Down syndrome. Obstetrics & Gynecology, 102, 1066-1079.
Marical, H., Douet-Guilbert, N., Bages, K., Collet, M., Le Bris, M. J., Morel, F., & De Braekeleer, M.
(2006). Second-trimester prenatal screening for trisomy 21 using biochemical markers: A 7year experience in one cytogenetic laboratory. Prenatal Diagnosis, 26, 308-312.
Marsis, I. O. (2004). Screening for Down syndrome using nuchal translucency thickness and nasal
bone examination at advanced maternal age in Jakarta: A preliminary report. Journal of
Medical Ultrasound, 12, 1-6.
Matias, A., Montenegro, N., & Blickstein, I. (2005). Down syndrome screening in multiple
pregnancies. Obstetrics & Gynecology Clinics of North America, 32, 81-96.
Maymon, R., Betser, M., Dreazen, E., Padoa, A., & Herman, A. (2004). A model for disclosing the first
trimester part of an integrated Down's syndrome screening test. Clinical Genetics, 65, 113119.
Maymon, R., Jauniaux, E., Holmes, A., Wiener, Y. M., Dreazen, E., & Herman, A. (2001). Nuchal
translucency measurement and pregnancy outcome after assisted conception versus
spontaneously conceived twins. Human Reproduction, 16, 1999-2004.
Maymon, R., Sharony, R., Grinshpun-Cohen, J., Itzhaky, D., Herman, A., & Reish, O. (2005). The best
marker combination using the integrated screening test approach for detecting various
chromosomal aneuploidies. Journal of Perinatal Medicine, 33, 392-398.
Maymon, R., & Shulman, A. (2002). Serial first- and second-trimester Down's syndrome screening
tests among IVF-versus naturally-conceived singletons. Human Reproduction, 17, 1081-1085.
Maymon, R., & Shulman, A. (2004). Integrated first- and second-trimester Down syndrome screening
test among unaffected IVF pregnancies. Prenatal Diagnosis, 24, 125-129.
Meier, C., Huang, T., Wyatt, P. R., & Summers, A. M. (2002). Accuracy of expected risk of Down
syndrome using the second-trimester triple test. Clinical Chemistry, 48, 653-655.
Monni, G., Zoppi, M. A., Ibba, R. M., Floris, M., Manca, F., & Axiana, C. (2005). Nuchal translucency
and nasal bone for trisomy 21 screening: single center experience. Croatian Medical Journal,
46, 786-791.
Mueller, V. M., Huang, T., Summers, A. M., & Winsor, S. H. M. (2005). The effect of fetal gender on
the false-positive rate of Down syndrome by maternal serum screening. Prenatal Diagnosis,
25, 1258-1261.
Muller, F., Dreux, S., Lemeur, A., Sault, C., Desgres, J., Bernard, M. A., Giorgetti, C., et al. (2003).
Medically assisted reproduction and second-trimester maternal serum marker screening for
Down syndrome. Prenatal Diagnosis, 23, 1073-1076.
Muller, F., Dreux, S., Oury, J. F., Luton, D., Uzan, S., Uzan, M., Levardon, M., & Dommergues, M.
(2002). Down syndrome maternal serum marker screening after 18 weeks' gestation. Prenatal
Diagnosis, 22, 1001-1004.
Nicolaides, K. H. (2004). Nuchal translucency and other first-trimester sonographic markers of
chromosomal abnormalities. American Journal of Obstetrics & Gynecology, 191, 45-67.
Nicolaides, K. H., Bindra, R., Heath, V., & Cicero, S. (2002). One-stop clinic for assessment of risk of
chromosomal defects at 12 weeks of gestation. Journal of Maternal-Fetal & Neonatal
Medicine, 12, 9-18.
Nicolaides, K. H., Spencer, K., Avgidou, K., Faiola, S., & Falcon, O. (2005). Multicenter study of firsttrimester screening for trisomy 21 in 75 821 pregnancies: Results and estimation of the
potential impact of individual risk-oriented two-stage first-trimester screening. Ultrasound in
Obstetrics & Gynecology, 25, 221-226.
O'Callaghan, S. P., Giles, W. B., Raymond, S. P., McDougall, V., Morris, K., & Boyd, J. (2000). First
trimester ultrasound with nuchal translucency measurement for Down syndrome risk
estimation using software developed by the Fetal Medicine Foundation, United Kingdom--the
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
220
first 2000 examinations in Newcastle, New South Wales, Australia. Australian & New
Zealand Journal of Obstetrics & Gynaecology, 40, 292-295.
O'Connell, M. P., Holding, S., Morgan, R. J., & Lindow, S. W. (2000). Biochemical screening for
Down syndrome: patients' perception of risk. International Journal of Gynaecology &
Obstetrics, 68, 215-218.
Odibo, A. O., Stamilio, D. M., Nelson, D. B., Sehdev, H. M., & Macones, G. A. (2005). A costeffectiveness analysis of prenatal screening strategies for Down syndrome. Obstetrics &
Gynecology, 106, 562-568.
Onda, T., Tanaka, T., Yoshida, K., Nakamura, Y., Kudo, R., Yamamoto, H., Sato, A., et al. (2000).
Triple marker screening for trisomy 21, trisomy 18 and open neural tube defects in singleton
pregnancies of native Japanese pregnant women. Journal of Obstetrics & Gynaecology
Research, 26, 441-447.
Orlandi, F., Rossi, C., Allegra, A., Krantz, D., Hallahan, T., Orlandi, E., & Macri, J. (2002). First
trimester screening with free beta-hCG, PAPP-A and nuchal translucency in pregnancies
conceived with assisted reproduction. Prenatal Diagnosis, 22, 718-721.
Palomaki, G. E., Knight, G. J., Roberson, M. M., Cunningham, G. C., Lee, J. E., Strom, C. M., &
Pandian, R. (2004). Invasive trophoblast antigen (hyperglycosylated human chorionic
gonadotropin) in second-trimester maternal urine as a marker for down syndrome: preliminary
results of an observational study on fresh samples. Clinical Chemistry, 50, 182-189.
Panburana, P., Ajjimakorn, S., & Tungkajiwangoon, P. (2001). First trimester Down Syndrome
screening by nuchal translucency in a Thai population. International Journal of Gynaecology
& Obstetrics, 75, 311-312.
Parano, E., Falcidia, E., Grillo, A., Takabayashi, H., Trifiletti, R. R., & Pavone, P. (2001). Fetal
nucleated red blood cell counts in peripheral blood of mothers bearing Down syndrome fetus.
Neuropediatrics, 32, 147-149.
Perenc, M., Dudarewicz, L., & Kaluzewski, B. (2000). Utility of the triple test in the detection of
abnormalities of the feto-placental unit. Medical Science Monitor, 6, 994-999.
Perni, S. C., Predanic, M., Kalish, R. B., Chervenak, F. A., & Chasen, S. T. (2006). Clinical use of
first-trimester aneuploidy screening in a United States population can replicate data from
clinical trials. American Journal of Obstetrics & Gynecology, 194, 127-130.
Pertl, B., & Bianchi, D. W. (2001). Fetal DNA in maternal plasma: emerging clinical applications.
Obstetrics & Gynecology, 98, 483-490.
Platt, L. D. (2005). First-trimester risk assessment: twin gestations. Seminars in Perinatology, 29, 258262.
Platt, L. D., Greene, N., Johnson, A., Zachary, J., Thom, E., Krantz, D., Simpson, J. L., et al. (2004).
Sequential pathways of testing after first-trimester screening for trisomy 21. Obstetrics &
Gynecology, 104, 661-666.
Prefumo, F., & Thilaganathan, B. (2002). Agreement between predicted risk and prevalence of Down
syndrome in first trimester nuchal translucency screening. Prenatal Diagnosis, 22, 917-918.
Raty, R., Virtanen, A., Koskinen, P., Anttila, L., Forsstrom, J., Laitinen, P., Morsky, P., et al. (2002).
Serum free beta-HCG and alpha-fetoprotein levels in IVF, ICSI and frozen embryo transfer
pregnancies in maternal mid-trimester serum screening for Down's syndrome. Human
Reproduction, 17, 481-484.
Rice, J. D., McIntosh, S. F., & Halstead, A. C. (2005). Second-trimester maternal serum screening for
Down syndrome in in vitro fertilization pregnancies. Prenatal Diagnosis, 25, 234-238.
Roberts, D., Walkinshaw, S. A., McCormack, M. J., & Ellis, J. (2000). Prenatal detection of trisomy
21: combined experience of two British hospitals. Prenatal Diagnosis, 20, 17-22.
Rosen, D. J., Kedar, I., Amiel, A., Ben-Tovim, T., Petel, Y., Kaneti, H., Tohar, M., et al. (2002). A
negative second trimester triple test and absence of specific ultrasonographic markers may
decrease the need for genetic amniocentesis in advanced maternal age by 60%. Prenatal
Diagnosis, 22, 59-63.
Rosen, T., & D'Alton, M. E. (2005). Down syndrome screening in the first and second trimesters: what
do the data show? Seminars in Perinatology, 29, 367-375.
Rozenberg, P., Bussieres, L., Chevret, S., Bernard, J. P., Malagrida, L., Cuckle, H., Chabry, C., et al.
(2006). Screening for Down syndrome using first-trimester combined screening followed by
second-trimester ultrasound examination in an unselected population. American Journal of
Obstetrics and Gynecology 199, 1379-1387 Epub ahead of print.
Rudnicka, A. R., Wald, N. J., Huttly, W., & Hackshaw, A. K. (2002). Influence of maternal smoking
on the birth prevalence of Down syndrome and on second trimester screening performance.
Prenatal Diagnosis, 22, 893-897.
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221
Sabria, J., Cabrero, D., & Bach, C. (2002). Aneuploidy screening: ultrasound versus biochemistry.
Ultrasound Review of Obstetrics & Gynecology, 2, 221-228.
Saltvedt, S., Almstrom, H., Kublickas, M., Valentin, L., Bottinga, R., Bui, T. H., Cederholm, M., et al..
(2005). Screening for Down syndrome based on maternal age or fetal nuchal translucency: a
randomized controlled trial in 39,572 pregnancies. Ultrasound in Obstetrics & Gynecology,
25, 537-545.
Sau, A., Langford, K., Auld, B., & Maxwell, D. (2001). Screening for trisomy 21: the significance of a
positive second trimester serum screen in women screen negative after a nuchal translucency
scan. Journal of Obstetrics & Gynaecology, 21, 145-148.
Schielen, P. C., van Leeuwen-Spruijt, M., Belmouden, I., Elvers, L. H., Jonker, M., & Loeber, J. G.
(2006). Multi-centre first-trimester screening for Down syndrome in the Netherlands in
routine clinical practice. Prenatal Diagnosis 26, 711-718 Epub ahead of print.
Skotko, B. (2006). Comparing three screening strategies for combining first- and second-trimester
Down syndrome markers. Obstetrics and Gynecology, 107, 1170.
Smith-Bindman, R., Hosmer, W., Feldstein, V. A., Deeks, J. J., & Goldberg, J. D. (2001). Secondtrimester ultrasound to detect fetuses with Down syndrome: a meta-analysis. JAMA, 285,
1044-1055.
Snijders, R. (2001). First-trimester ultrasound. Clinics in Perinatology, 28, 333-352.
Sorensen, T., Larsen, S. O., & Christiansen, M. (2005). Weight adjustment of serum markers in early
first-trimester prenatal screening for Down syndrome. Prenatal Diagnosis, 25, 484-488.
Souter, V. L., & Nyberg, D. A. (2001). Sonographic screening for fetal aneuploidy: first trimester.
Journal of Ultrasound in Medicine, 20, 775-790.
Spencer, K. (2001). Age related detection and false positive rates when screening for Down's syndrome
in the first trimester using fetal nuchal translucency and maternal serum free betahCG and
PAPP-A. BJOG: An International Journal of Obstetrics & Gynaecology, 108, 1043-1046.
Spencer, K. (2005). First trimester maternal serum screening for Down's syndrome: an evaluation of
the DPC Immulite 2000 free beta-hCG and pregnancy-associated plasma protein-A assays
Annals of Clinical Biochemistry, 42, 30-40.
Spencer, K., Bindra, R., Cacho, A. M., & Nicolaides, K. H. (2004). The impact of correcting for
smoking status when screening for chromosomal anomalies using maternal serum
biochemistry and fetal nuchal translucency thickness in the first trimester of pregnancy.
Prenatal Diagnosis, 24, 169-173.
Spencer, K., Bindra, R., & Nicolaides, K. H. (2003). Maternal weight correction of maternal serum
PAPP-A and free beta-hCG MoM when screening for trisomy 21 in the first trimester of
pregnancy. Prenatal Diagnosis, 23, 851-855.
Spencer, K., Bindra, R., Nix, A. B., Heath, V., & Nicolaides, K. H. (2003). Delta-NT or NT MoM:
which is the most appropriate method for calculating accurate patient-specific risks for
trisomy 21 in the first trimester? Ultrasound in Obstetrics & Gynecology, 22, 142-148.
Spencer, K., Crossley, J. A., Aitken, D. A., Nix, A. B., Dunstan, F. D., & Williams, K. (2003). The
effect of temporal variation in biochemical markers of trisomy 21 across the first and second
trimesters of pregnancy on the estimation of individual patient-specific risks and detection
rates for Down's syndrome. Annals of Clinical Biochemistry, 40, 219-231.
Spencer, K., Heath, V., El-Sheikhah, A., Ong, C. Y., & Nicolaides, K. H. (2005). Ethnicity and the
need for correction of biochemical and ultrasound markers of chromosomal anomalies in the
first trimester: a study of Oriental, Asian and Afro-Caribbean populations. Prenatal
Diagnosis, 25, 365-369.
Spencer, K., Liao, A. W., Ong, C. Y., Geerts, L., & Nicolaides, K. H. (2001). First trimester maternal
serum placenta growth factor (PIGF)concentrations in pregnancies with fetal trisomy 21 or
trisomy 18. Prenatal Diagnosis, 21, 718-722.
Spencer, K., & Nicolaides, K. H. (2003). Screening for trisomy 21 in twins using first trimester
ultrasound and maternal serum biochemistry in a one-stop clinic: a review of three years
experience. BJOG: An International Journal of Obstetrics & Gynaecology, 110, 276-280.
Spencer, K., Spencer, C. E., Power, M., Moakes, A., & Nicolaides, K. H. (2000). One stop clinic for
assessment of risk for fetal anomalies: a report of the first year of prospective screening for
chromosomal anomalies in the first trimester. BJOG: An International Journal of Obstetrics &
Gynaecology, 107, 1271-1275.
Stenhouse, E. J., Crossley, J. A., Aitken, D. A., Brogan, K., Cameron, A. D., & Connor, J. M. (2004).
First-trimester combined ultrasound and biochemical screening for Down syndrome in routine
clinical practice. Prenatal Diagnosis, 24, 774-780.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
222
Summers, A. M., Farrell, S. A., Huang, T., Meier, C., & Wyatt, P. R. (2003). Maternal serum screening
in Ontario using the triple marker test. Journal of Medical Screening, 10, 107-111.
Toyama, J. M., Brizot, M. L., Liao, A. W., Lopes, L. M., Nomura, R. M. Y., Saldanha, F. A. T., &
Zugaib, M. (2004). Ductus venosus blood flow assessment at 11 to 14 weeks of gestation and
fetal outcome. Ultrasound in Obstetrics & Gynecology, 23, 341-345.
Tsai, M. S., Huang, Y. Y., Hwa, K. Y., Cheng, C. C., & Lee, F. K. (2001). Combined measurement of
fetal nuchal translucency, maternal serum free beta-hCG, and pregnancy-associated plasma
protein A for first-trimester Down's syndrome screening. Journal of the Formosan Medical
Association, 100, 319-325.
Van Den Berg, M., Timmermans, D. R. M., Kleinveld, J. H., Garcia, E., Van Vugt, J. M. G., & Van
Der Wal, G. (2005). Accepting or declining the offer of prenatal screening for congenital
defects: Test uptake and women's reasons. Prenatal Diagnosis, 25, 84-90.
van den Berg, M., Timmermans, D. R. M., ten Kate, L. P., van Vugt, J. M. G., & van der Wal, G.
(2005). Are pregnant women making informed choices about prenatal screening? Genetics in
Medicine, 7, 332-338.
Vandecruys, H., Faiola, S., Auer, M., Sebire, N., & Nicolaides, K. H. (2005). Screening for trisomy 21
in monochorionic twins by measurement of fetal nuchal translucency thickness. Ultrasound in
Obstetrics & Gynecology, 25, 551-553.
Viora, E., Masturzo, B., Bastonero, S., Errante, G., Sciarrone, A., Grassi Pirrone, P., & Campogrande,
M. (2003). Efficiency and intra-operator's variability of nuchal translucency measurement.
Importance of operator's experience. Italian Journal of Gynaecology & Obstetrics, 15, 69-73.
Wapner, R. J. (2005). First trimester screening: the BUN study. Seminars in Perinatology, 29, 236-239.
Wasant, P., & Liammongkolkul, S. (2003). Prenatal genetic screening for Down syndrome and open
neural tube defects using maternal serum markers in Thai pregnant women. Southeast Asian
Journal of Tropical Medicine & Public Health, 34 Suppl 3, 244-248.
Wayda, K., Kereszturi, A., Orvos, H., Horvath, E., A, P. A., Kovacs, L., & Szabo, J. (2001). Four years
experience of first-trimester nuchal translucency screening for fetal aneuploidies with
increasing regional availability. Acta Obstetricia et Gynecologica Scandinavica, 80, 11041109.
Wilson, R. D., & Genetics Committee of the Society of Obstetricians and Gynaecologists of Canada
(2005). Cell-free fetal DNA in the maternal circulation and its future uses in obstetrics.
Journal of Obstetrics & Gynaecology Canada: JOGC, 27, 54-62.
Wright, D., Bradbury, I., Benn, P., Cuckle, H., & Ritchie, K. (2004). Contingent screening for Down
syndrome is an efficient alternative to non-disclosure sequential screening Prenatal
Diagnosis, 24, 762-766.
Yamamoto, R., Azuma, M., Hoshi, N., Kishida, T., Satomura, S., & Fujimoto, S. (2001). Lens culinaris
agglutinin-reactive alpha-fetoprotein, an alternative variant to alpha-fetoprotein in prenatal
screening for Down's syndrome. Human Reproduction, 16, 2438-2444.
Zoppi, M. A., Ibba, R. M., Floris, M., Manca, F., Axiana, C., & Monni, G. (2005). Nuchal translucency
measurement at different crown-rump lengths along the 10- to 14-week period for Down
syndrome screening. Prenatal Diagnosis, 25, 411-416.
Zoppi, M. A., Ibba, R. M., Floris, M., & Monni, G. (2001). Fetal nuchal translucency screening in
12495 pregnancies in Sardinia. Ultrasound in Obstetrics & Gynecology, 18, 649-651.
Zoppi, M. A., Ibba, R. M., Putzolu, M., Floris, M., & Monni, G. (2000). Assessment of risk for
chromosomal abnormalities at 10-14 weeks of gestation by nuchal translucency and maternal
age in 5,210 fetuses at a single centre. Fetal Diagnosis & Therapy, 15, 170-173.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
223
Appendix 4: Retrieved studies
excluded for review: Part B
Abbott, M. A., & Benn, P. (2002). Prenatal genetic diagnosis of Down's syndrome. Expert Review of
Molecular Diagnostics, 2, 605-615.
Alfirevic, Z., & Neilson, J. P. (2004). Antenatal screening for Down's syndrome. British Medical
Journal, 329, 811-812.
American College of Obstetricians and Gynecologists (2001). ACOG Practice Bulletin. Clinical
management guidelines for obstetrician-gynecologists. Prenatal diagnosis of fetal
chromosomal abnormalities. Obstetrics & Gynecology, 97, Suppl 1-12.
Anonymous. (2003). Risk and Down's screening. Bandolier, 10, 6.
Anonymous. (2005). Sequential pregnancy screening. ACOG Clinical Review, 10, 4-5.
Antsaklis, A. (2003). Invasive genetic studies in multiple pregnancy. Balkan Journal of Medical
Genetics, 6, 41-47.
Audibert, F., Mairovitz, V., & Frydman, R. (2002). Alternatives to amniocentesis for advanced
maternal age. [French]. Gynecologie, Obstetrique & Fertilite, 30, 562-566.
Avgidou, K., Papageorghiou, A., Bindra, R., Spencer, K., & Nicolaides, K. H. (2005). Prospective
first-trimester screening for trisomy 21 in 30,564 pregnancies. American Journal of Obstetrics
& Gynecology, 192, 1761-1767.
Babbur, V., Lees, C. C., Goodburn, S. F., Morris, N., Breeze, A. C., & Hackett, G. A. (2005).
Prospective audit of a one-centre combined nuchal translucency and triple test programme for
the detection of trisomy 21. Prenatal Diagnosis, 25, 465-469.
Bahado-Singh, R. O., Oz, A. U., Gomez, K., Hunter, D., Copel, J., Baumgarten, A., & Mahoney, M. J.
(2000). Combined ultrasound biometry, serum markers and age for Down syndrome risk
estimation. Ultrasound in Obstetrics & Gynecology, 15, 199-204.
Ball, R. H. (2004). Invasive fetal testing. Current Opinion in Obstetrics & Gynecology, 16, 159-162.
Beaman, J. M., & Goldie, D. J. (2001). Second trimester screening for Down's syndrome: 7 years
experience. Journal of Medical Screening, 8, 128-131.
Benacerraf, B. R. (2000). Should sonographic screening for fetal Down syndrome be applied to low
risk women? Ultrasound in Obstetrics & Gynecology, 15, 451-455.
Benn, P., & Donnenfeld, A. E. (2005). Sequential Down syndrome screening: the importance of first
and second trimester test correlations with calculating risk. Journal of Genetic Counseling, 14,
409-413.
Benn, P. A. (2002). Advances in prenatal screening for Down syndrome: II first trimester testing,
integrated testing, and future directions. Clinica Chimica Acta, 324, 1-11.
Benn, P. A., Fang, M., Egan, J. F., Horne, D., & Collins, R. (2003). Incorporation of inhibin-A in
second-trimester screening for Down syndrome. Obstetrics & Gynecology, 101, 451-454.
Benn, P. A., Kaminsky, L. M., Ying, J., Borgida, A. F., & Egan, J. F. X. (2002). Combined secondtrimester biochemical and ultrasound screening for Down syndrome. Obstetrics and
Gynecology, 100, 1168-1176.
Biggio, J. R., Jr., Morris, T. C., Owen, J., & Stringer, J. S. (2004). An outcomes analysis of five
prenatal screening strategies for trisomy 21 in women younger than 35 years. American
Journal of Obstetrics & Gynecology, 190, 721-729.
Bindra, R., Heath, V., Liao, A., Spencer, K., & Nicolaides, K. H. (2002). One-stop clinic for
assessment of risk for trisomy 21 at 11-14 weeks: a prospective study of 15 030 pregnancies.
Ultrasound in Obstetrics & Gynecology, 20, 219-225.
Blackwell, S. C., Abundis, M. G., & Nehra, P. C. (2002). Five-year experience with midtrimester
amniocentesis performed by a single group of obstetricians-gynecologists at a community
hospital. American Journal of Obstetrics & Gynecology, 186, 1130-1132.
Borrell, A., Casals, E., Fortuny, A., Farre, M. T., Gonce, A., Sanchez, A., Soler, A., Cararach, V., &
Vanrell, J. A. (2004). First-trimester screening for trisomy 21 combining biochemistry and
ultrasound at individually optimal gestational ages. An interventional study. Prenatal
Diagnosis, 24, 541-545.
Brigatti, K. W., & Malone, F. D. (2004). First-trimester screening for aneuploidy. Obstetrics &
Gynecology Clinics of North America, 31, 1-20.
SCREENING STRATEGIES FOR ANTENATAL DOWN SYNDROME SCREENING
224
Canick, J. A., Saller, D. N., Jr., & Lambert-Messerlian, G. M. (2003). Prenatal screening for Down
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Appendix 5:
DESIGNATIONS OF LEVELS OF EVIDENCE
Level I
Evidence obtained from a systematic review (or meta-analysis) of relevant randomised
controlled trials.
Level II
Evidence obtained from at least one randomised controlled trial.
Level III. 1
Evidence obtained from pseudorandomised controlled trials (alternate allocation or
some other method).
2
Evidence obtained from comparative studies (including a systematic reviews of such
studies) with concurrent controls and allocation not randomised, cohort studies, case
control studies or interrupted time series with a control group).
3
Evidence obtained from comparative studies with historical control, two or more
single-arm studies or interrupted time series without a parallel control group.
Level IV Evidence obtained from case series, either post-test or pretest/post-test.
*Modified from NHMRC (2000).
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