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University of Iowa
Iowa Research Online
Theses and Dissertations
Spring 2013
Investigating the genetics Of thyroid stimulating
hormone in newborns
Farah Yacoub Alul
University of Iowa
Copyright 2013 Farah Yacoub Alul
This dissertation is available at Iowa Research Online: http://ir.uiowa.edu/etd/2434
Recommended Citation
Alul, Farah Yacoub. "Investigating the genetics Of thyroid stimulating hormone in newborns." PhD (Doctor of Philosophy) thesis,
University of Iowa, 2013.
http://ir.uiowa.edu/etd/2434.
Follow this and additional works at: http://ir.uiowa.edu/etd
Part of the Genetics Commons
INVESTIGATING THE GENETICS OF THYROID STIMULATING HORMONE IN
NEWBORNS
by
Farah Yacoub Alul
An Abstract
Of a thesis submitted in partial fulfillment
of the requirements for the Doctor of
Philosophy degree in Genetics
in the Graduate College of
The University of Iowa
May 2013
Thesis Supervisor: Professor Jeffrey C. Murray
1
ABSTRACT
Endocrine disorders are substantial contributors to neonatal morbidity and
mortality and, of these, congenital hypothyroidism (CH) is the most common (Kumar et
al. 2009). CH is a common and preventable cause of mental retardation with an incidence
of approximately 1 in 2,350 live births (Hinton et al. 2010). In Iowa, the Iowa Neonatal
Metabolic Screening program (INMSP) uses thyroid stimulating hormone (TSH) to
screen for CH at birth. However, TSH is highly variable among healthy newborns as well
as adults, leading to false positive results in some cases. Previous studies have observed
that adult TSH variability is under strong genetic regulation with estimated heritability of
up to 65% (Panicker et al. 2008). Additionally, there have been multiple studies
examining genetic factors associated with adult TSH levels.
TSH heritability has never been estimated in the neonatal period and we aimed to
determine the heritability in neonates and compare it to heritability estimates in adults.
We examined 381 twin pairs obtained from the INMSP. Heritability was estimated using
multilevel mixed-effects linear regression adjusting for factors affecting TSH levels;
gestational age, gender, weight and age at time of sample collection. We estimated
neonatal TSH heritability to be 58% with a P-value of 2x10-5, which mirrors adult
heritability estimates, and provides direct evidence for a strong genetic contribution to
TSH variability at birth.
We next examined genetic factors that may contribute to the observed heritability.
Genetic contribution to TSH variation has been studied extensively in adults, but not in
neonates. We genotyped a population of Iowa neonates; term (n=827) and preterm
(n=815), for 45 single nucleotide polymorphisms (SNPs) that we selected based on
reported genetic associations with adult TSH levels from the literature, as well as other
candidate genes. TSH values were obtained from the INMSP. Analysis of variance was
performed to identify genetic associations with TSH concentrations. The strongest
2
association identified was rs4704397 in the PDE8B gene (p=1.3x10-4), followed by
rs965513 (p=6.4x10-4) on chromosome 9 upstream of the FOXE1 gene. Both of these
SNPs met statistical significance after correction for multiple testing. Our results
demonstrated for the first time two genetic associations with neonatal TSH levels that
replicate findings with adult TSH levels, and these findings could have clinical
implications for the early prediction of risk for adult diseases and conditions associated
with thyroid hormone levels.
Finally, we aimed to identify the etiologic variants that may be responsible for the
observed associations by fine mapping adjacent enhancer elements. This was done in two
stages; first we sequenced 58 term neonates with TSH levels at both ends of the normal
distribution to identify associated variants, then we replicated the findings in an
additional population of 306 term neonates. None of the observed variants were
statistically significant for an association with TSH levels, however, one of the rare
variants (rs112053411) identified was detected in three neonates, all in the upper
distribution of TSH levels including one infant that was later diagnosed with CH. This
rare variant is worth pursuing in a larger study population and in functional studies.
Together this work has advanced our knowledge of the genetic basis of TSH variation in
the neonatal period, as well as provided insight into the early prediction of risk for
adulthood thyroid related diseases through shared genetic associations between adults and
neonates.
Abstract Approved: ____________________________________
Thesis Supervisor
____________________________________
Title and Department
____________________________________
Date
INVESTIGATING THE GENETICS OF THYROID STIMULATING HORMONE IN
NEWBORNS
by
Farah Yacoub Alul
A thesis submitted in partial fulfillment
of the requirements for the Doctor of
Philosophy degree in Genetics
in the Graduate College of
The University of Iowa
May 2013
Thesis Supervisor: Professor Jeffrey C. Murray
Copyright by
FARAH YACOUB ALUL
2013
All Rights Reserved
Graduate College
The University of Iowa
Iowa City, Iowa
CERTIFICATE OF APPROVAL
_______________________
PH.D. THESIS
_______________
This is to certify that the Ph.D. thesis of
Farah Yacoub Alul
has been approved by the Examining Committee
for the thesis requirement for the Doctor of Philosophy
degree in Genetics at the May 2013 graduation.
Thesis Committee: ___________________________________
Jeffrey C. Murray, Thesis Supervisor
___________________________________
Alexander G. Bassuk
___________________________________
Terry A. Braun
___________________________________
Josep M. Comeron
___________________________________
John M. Dagle
To my beloved family.
ii
ACKNOWLEDGMENTS
There are so many people that have helped and supported me and without whom
this work would not have been possible. First I would like to thank Dr. Jeff Murray for
giving me this amazing opportunity. When I first came to Iowa I was very fortunate to
work as a research assistant in Dr. Murray’s lab and that paved the way for me to enter
the Genetics Program. Dr. Murray goes above and beyond for his students and no one can
wish for a better mentor. I would also like to thank Dr. Kelli Ryckman. Kelli was like a
second mentor to me and I learned so much from her, as well as a great friend. I am sure I
would not be where I am today if it weren’t for Kelli’s support.
I would like to thank the members of my thesis committee: Dr. John Dagle, Dr.
Alex Bassuk, Dr. Terry Braun, and Dr. Josep Comeron for valuable insight and advice in
every meeting, and Dr. Anne Kwitek for her role in my comprehensive exam. I am also
thankful for the support of Dr. Dan Eberl, Anita Kafer, Isabelle Hardy, and Linda Hurst
from the Genetics Program.
I was very fortunate to work in one of the biggest labs on campus, so there are so
many people to thank. I would like to start with Tamara Busch for answering my never
ending questions, Elizabeth Leslie and Leah Biggs for all your help with comps. Thanks
to Allison Momany and Lauren Fleener for being great friends and making me laugh
every day, you two are the best bench neighbors ever. I am also very grateful to Lauren
Fleener, Osayame Ekhaguere and Elwood Cook; without your help I would still be
processing blood spot cards today. I am very thankful to all past and present Murray lab
members, you all make coming to work every day something to look forward to: Nancy
Weathers, Adela Mansilla, Aline and Raul Petrin, Jennifer Standley, Brandon Alleman,
Bruce Bedell, Lindsey and Dana Rhea, Azeez Butali, Zhonglin Jia, Hodad Naderi, Jinsil
Kim, Aimee Buhr, Satoshi Suzuki, Dee Even, Nancy Davin, Erin Brothers-Smith, Sarah
Barten, and Susie McConnell. I would also like to thank my grad school colleagues and
iii
great friends, Lily Paemka and Dina Ahram, I was fortunate to go through this journey
with you.
I would like to thank all of the families that participated in our research, without
them none of this would be possible. I am also very grateful to people at the State
Hygienic Lab especially Dr. Stanton Berberich for providing samples, and the University
of Iowa DNA Facility especially Dr. Kevin Knudtson, Mary Boes and Garry Hauser, for
providing me with work space, machines and support when results didn’t turn out as
expected. I would like to thank Drs. Zuhair Amr and Abdelkader Battah from Jordan,
without their guidance I would not have made it to grad school to begin with. And I
would especially like to thank Dr. Adel Afifi for introducing me to Dr. Murray when I
first came to Iowa, and for being an exceptional supporter of new graduates coming to the
United States from abroad.
Finally, I am very grateful for my family. I owe everything good that happened to
me to my parents Yacoub and Eman Alul, they have been exceptionally supportive and
loving my whole life and I wish one day I can be to my children half the parent they were
to me. I also want to express my gratitude to my sisters Lubna and Haya, my
grandmothers Amal and Nahida, and my aunts May and Azza for the endless support and
love. Last but not least, I would like to express my honest gratitude to my husband Taher
and my son Bashir. They were with me every step of the way, and witnessed this whole
experience with me first hand. Taher’s unconditional love and support was what got me
through the ups and downs throughout this journey. He always pushes me for more and
expects me to excel. And Bashir always helps me forget any troubled experiment the
minute I pick him up from daycare. I owe all of this and much more to you all.
iv
ABSTRACT
Endocrine disorders are substantial contributors to neonatal morbidity and
mortality and, of these, congenital hypothyroidism (CH) is the most common (Kumar et
al. 2009). CH is a common and preventable cause of mental retardation with an incidence
of approximately 1 in 2,350 live births (Hinton et al. 2010). In Iowa, the Iowa Neonatal
Metabolic Screening program (INMSP) uses thyroid stimulating hormone (TSH) to
screen for CH at birth. However, TSH is highly variable among healthy newborns as well
as adults, leading to false positive results in some cases. Previous studies have observed
that adult TSH variability is under strong genetic regulation with estimated heritability of
up to 65% (Panicker et al. 2008). Additionally, there have been multiple studies
examining genetic factors associated with adult TSH levels.
TSH heritability has never been estimated in the neonatal period and we aimed to
determine the heritability in neonates and compare it to heritability estimates in adults.
We examined 381 twin pairs obtained from the INMSP. Heritability was estimated using
multilevel mixed-effects linear regression adjusting for factors affecting TSH levels;
gestational age, gender, weight and age at time of sample collection. We estimated
neonatal TSH heritability to be 58% with a P-value of 2x10-5, which mirrors adult
heritability estimates, and provides direct evidence for a strong genetic contribution to
TSH variability at birth.
We next examined genetic factors that may contribute to the observed heritability.
Genetic contribution to TSH variation has been studied extensively in adults, but not in
neonates. We genotyped a population of Iowa neonates; term (n=827) and preterm
(n=815), for 45 single nucleotide polymorphisms (SNPs) that we selected based on
reported genetic associations with adult TSH levels from the literature, as well as other
candidate genes. TSH values were obtained from the INMSP. Analysis of variance was
performed to identify genetic associations with TSH concentrations. The strongest
v
association identified was rs4704397 in the PDE8B gene (p=1.3x10-4), followed by
rs965513 (p=6.4x10-4) on chromosome 9 upstream of the FOXE1 gene. Both of these
SNPs met statistical significance after correction for multiple testing. Our results
demonstrated for the first time two genetic associations with neonatal TSH levels that
replicate findings with adult TSH levels, and these findings could have clinical
implications for the early prediction of risk for adult diseases and conditions associated
with thyroid hormone levels.
Finally, we aimed to identify the etiologic variants that may be responsible for the
observed associations by fine mapping adjacent enhancer elements. This was done in two
stages; first we sequenced 58 term neonates with TSH levels at both ends of the normal
distribution to identify associated variants, then we replicated the findings in an
additional population of 306 term neonates. None of the observed variants were
statistically significant for an association with TSH levels, however, one of the rare
variants (rs112053411) identified was detected in three neonates, all in the upper
distribution of TSH levels including one infant that was later diagnosed with CH. This
rare variant is worth pursuing in a larger study population and in functional studies.
Together this work has advanced our knowledge of the genetic basis of TSH variation in
the neonatal period, as well as provided insight into the early prediction of risk for
adulthood thyroid related diseases through shared genetic associations between adults and
neonates.
vi
TABLE OF CONTENTS
LIST OF TABLES ............................................................................................................. ix
LIST OF FIGURES ........................................................................................................... xi
CHAPTER1 INTRODUCTION ..........................................................................................1
Significance ......................................................................................................1
The Thyroid Gland ...........................................................................................2
Thyroid Hormones ............................................................................................3
Thyroid Follicles ...............................................................................................4
Hypothalamic-Pituitary-Thyroid Axis ..............................................................4
Thyroid Stimulating Hormone ..........................................................................5
Embryological Development of the Thyroid Gland .........................................5
Molecular Aspects of Thyroid Morphogenesis ................................................6
Thyroid Function in the Fetus...........................................................................7
Thyroid Function in the Neonate ......................................................................7
Full Term Newborns..................................................................................7
Preterm Newborns .....................................................................................8
Disorders of Thyroid Function .........................................................................8
Transient Hypothyroxinemia of Prematurity.............................................8
Congenital Hypothyroidism ......................................................................9
Newborn Screening ........................................................................................10
Etiology of Congenital Hypothyroidism ........................................................12
Transient Congenital Hypothyroidism ....................................................12
Permanent Congenital Hypothyroidism ..................................................13
Adult Onset Hypothyroidism ..........................................................................14
Genetics of Thyroid Stimulating Hormone ....................................................15
Genome Wide Association Studies .........................................................16
Candidate Gene Studies ...........................................................................19
Main Thyroid Related Genes...................................................................20
Purpose of Study .............................................................................................22
Hypothesis ...............................................................................................23
Specific Aims ..........................................................................................23
CHAPTER 2 THE HERITABILITY OF METABOLIC PROFILES IN
NEWBORN TWINS ......................................................................................33
Abstract ...........................................................................................................34
Introduction.....................................................................................................34
Methods ..........................................................................................................37
Study Population .....................................................................................37
Enzymatic Assays ....................................................................................37
Tandem Mass Spectrometry ....................................................................38
Determination of Zygosity ......................................................................38
Statistical Analysis ..................................................................................39
Analysis of Ratios....................................................................................41
Results.............................................................................................................42
Discussion .......................................................................................................43
vii
CHAPTER 3 GENETIC ASSOCIATIONS WITH NEONATAL THYROID
STIMULATING HORMONE LEVELS ........................................................57
Abstract ...........................................................................................................58
Introduction.....................................................................................................58
Methods ..........................................................................................................60
Study Population .....................................................................................60
Marker Selection and Genotyping ...........................................................61
Statistical Analysis ..................................................................................62
Haplotype Analysis .................................................................................63
Results.............................................................................................................63
Discussion .......................................................................................................65
CHAPTER 4 CHARACTERIZATION OF FOXE1 AND PDE8B ENHANCER
REGIONS FOR A ROLE IN NORMAL VARIATION IN
NEONATAL TSH LEVELS ..........................................................................83
Abstract ...........................................................................................................83
Introduction.....................................................................................................84
Materials and Methods ...................................................................................86
Study Population .....................................................................................86
Selection of Studied Regions...................................................................88
Genotyping ..............................................................................................88
Statistics ...................................................................................................89
Results.............................................................................................................90
Sequencing ..............................................................................................90
TaqMan....................................................................................................91
Discussion .......................................................................................................91
CHAPTER 5 CONCLUSIONS AND FUTURE DIRCTIONS .......................................101
Conclusions...................................................................................................101
Future Directions ..........................................................................................107
REFERENCES ................................................................................................................110
viii
LIST OF TABLES
Table 1-1 Summary of GWAS data for TSH.....................................................................24
Table 2-1 List of analytes examined. .................................................................................47
Table 2-2 List of markers used for zygosity testing and population allele
frequencies.........................................................................................................48
Table 2-3 Heritability estimates for all twin pairs. ............................................................49
Table 2-4 Heritability estimates for twin pairs excluding TPN, abnormal screens,
gestational age <34 weeks, and MZ twin pairs that are >20% discrepant
in weight. ...........................................................................................................51
Table 2-5 Demographic characteristics of twin pairs. .......................................................53
Table 2-6 Heritability estimates for analyte ratios. ............................................................54
Table 3-1 List of genotyped markers. ................................................................................70
Table 3-2 Demographic Characteristics of Cohorts...........................................................72
Table 3-3 Association statistics for all genotyped SNPs with neonatal TSH level for
all combined populations. P-values reported in this table are from
ANOVA and non-parametric analysis. .............................................................73
Table 3-4 Association statistics for all genotyped SNPs with neonatal TSH level for
individual population cohorts. P-values reported in this table are from
ANOVA and non-parametric analysis. .............................................................75
Table 3-5 TSH means and standard deviations for PDE8B and FOXE1 significant
SNPs. .................................................................................................................77
Table 3-6 TSH means and standard deviations for marginally significant SNPs. .............78
Table 3-7 SNP haplotypes in the FOXE1 gene that are significantly associated
(p<0.001) with natural log transformed TSH levels..........................................79
Table 3-8 SNP haplotypes in the TSHR gene that are significantly associated
(p<0.001) with natural log transformed TSH levels..........................................80
Table 4-1 Potential FOXE1 and PDE8B enhancer regions studied. ..................................95
Table 4-2 Primer sequences and PCR conditions for sequencing FOXE1 and
PDE8B enhancer regions...................................................................................96
ix
Table 4-3 List of SNPs selected for further investigation after sequencing. .....................97
Table 4-4 List of all sequence variants detected in the sequencing of 58 newborns. ........98
x
LIST OF FIGURES
Figure 1-1 Thyroid gland. . ................................................................................................25
Figure 1-2 Iodine organification and thyroid hormone synthesis. .....................................26
Figure 1-3 Hypothalamic-pituitary-thyroid axis regulation. ..............................................27
Figure 1-4 Three month old infant with untreated congenital hypothyroidism. . ..............28
Figure 1-5 A Manhattan plot of the TSH level GWAS done in 2008 by ArnaudLopez et al. ......................................................................................................29
Figure 1-6 A Manhattan plot of the TSH level GWAS done in 2010 by Panicker et
al. . ...................................................................................................................30
Figure 1-7 A Manhattan plot of the TSH level GWAS meta-analysis done in 2012
by Rawal et al. . ...............................................................................................31
Figure 1-8 A Manhattan plot of the TSH level GWAS meta-analysis done in 2013
by Porcu et al. . ................................................................................................32
Figure 2-1 Heritability of analyzed metabolites and analyte ratios. . ................................55
Figure 2-2 Environment and genetic contribution to metabolites in the β-oxidation
pathway and the pathway for catabolism of branched-chain amino acids.......56
Figure 3-1 Association statistics for all genotyped SNPs with neonatal TSH level
for combined populations. ...............................................................................81
Figure 3-2 Association statistics for all genotyped SNPs with neonatal TSH level
for individual populations. ...............................................................................82
Figure 4-1 FOXE1 potential enhancer regions. .................................................................99
Figure 4-2 PDE8B potential enhancer regions. ...............................................................100
xi
1
CHAPTER1
INTRODUCTION
Significance
Endocrine disorders are substantial contributors to neonatal morbidity and
mortality and, of these, congenital hypothyroidism (CH) is the most common (Kumar et
al. 2009). CH is a common and preventable cause of mental retardation with an incidence
of approximately 1 in 2,350 live births (Hinton et al. 2010). Early treatment with
thyroxine (T4) with subsequent supplementation for life produces excellent results for
both growth and development (Wilcken and Wiley 2008; Hinton et al. 2010). CH is
screened for at birth through detection of T4, thyroid stimulating hormone (TSH), or both
(Wilcken and Wiley 2008). Unfortunately, newborn screening for CH has the highest
number of false positive results with repeated testing costs of more than two million
dollars annually (Kwon and Farrell 2000). False positive results can cause significant
stress for parents of these infants, and also result in an increased financial burden in
follow up testing costs (Kwon and Farrell 2000). The false positive result rate is usually
higher in newborn screening programs that use T4 as a primary analyte (0.30%) compared
to programs that use TSH (0.05%) (Kaye et al. 2006b). In Iowa, the Iowa Neonatal
Metabolic Screening program uses TSH only to screen for CH (Pass and Neto 2009).
Furthermore, TSH is extremely sensitive to serum thyroid hormone levels, which makes
it the test of choice for clinicians to diagnose most cases of thyroid dysfunction (Stathatos
2012).
TSH is highly variable among healthy newborns; this is one of the factors
contributing to the false positive rate for this test when used in newborn screening
programs. Additionally, TSH varies greatly by gestational age and birth weight and
shows lower levels in premature or low birth weight newborns (Kirsten 2000). In healthy
adult subjects, TSH has considerable variability between individuals, whereas this
2
variability is much less in the same individual when TSH is measured repeatedly over an
extended period of time (Panicker et al. 2010). Previous studies have observed that adult
TSH variability is under strong genetic regulation; studies have estimated a heritability of
up to 65% (Panicker et al. 2008). However, no studies have examined the heritability of
neonatal TSH levels. Furthermore, there have been multiple studies examining genetic
factors associated with adult TSH levels but no studies have examined the genetics of
neonatal TSH levels. Therefore, a better understanding of the normal variation in TSH
may improve the sensitivity of its use in newborn screening and help minimize the rate of
false positive results, as well as provide a better understanding of the thyroid profile and
disorders in newborns.
Understanding variation in TSH levels and the genes responsible may be
particularly important in a population at risk for abnormal TSH levels such as preterm
infants. Preterm infants manifest even higher TSH variability than term infants owing to
the postnatal changes in thyroid function due to the premature interrupted exposure to
maternal thyroid hormones as well as an immature hypothalamic-pituitary axis (HPA)
(Hinton et al. 2010). Thyroid hormones also play a key role in neonatal as well as adult
normal physiology, affecting almost all tissues and maintaining healthy status of all
human systems including cognition, cardiovascular function, skeletal health, and
balanced energy and metabolic status (Panicker 2011). Understanding the shared genetic
associations with TSH levels in both the neonatal period as well as through adulthood
will be useful for earlier prediction of risk to adult diseases that are affected by TSH
levels.
The Thyroid Gland
The thyroid is a butterfly-shaped endocrine gland located in the neck immediately
below the larynx and anterior to the trachea (Figure 1-1) (Kirsten 2000; Stathatos 2012).
The thyroid gland consists of two lateral lobes connected by narrow thyroid tissue called
3
the isthmus (Figure 1-1). The two thyroid lobes contain spherical structures called
follicles (Kirsten 2000). The thyroid follicle is the functional part of the thyroid gland
consisting of the thyroid hormone synthesizing follicular cells (De Felice and Di Lauro
2011; Stathatos 2012). During human embryological development, the thyroid is the first
endocrine structure to develop (Kratzsch and Pulzer 2008). It is also one of the largest
endocrine glands, weighing about 15 to 20 grams in human adults (Kirsten 2000). The
thyroid gland secretes thyroid hormones that are vital for the normal physiology of
virtually every organ system in the human body (Kirsten 2000; Panicker 2011).
Thyroid Hormones
The thyroid gland is necessary for normal human physiology, plays a vital role in
almost all tissues, and influences most bodily functions through the secretion of its two
major thyroid hormones; thyroxine (T4) and triiodothyronine (T3) (Kirsten 2000; Panicker
2011). Of these two thyroid hormones, T3 is considered to be the primary thyroid
hormone since it is more potent, but T4 is more abundant (Kirsten 2000). Under normal
conditions, thyroid gland output is about 90% T4 and 10% T3 (Stathatos 2012). Thyroid
hormone synthesis requires the presence of iodide; the sodium/iodide transporter (NIS)
transports iodide from the blood into thyrocytes against its concentration gradient since
the thyroid gland maintains a 20-40 times higher concentration of free iodide than that in
the plasma (Figure 1-2) (Targovnik et al. 2010). Iodide is then transferred from
thyrocytes into the colloid via an apical anion channel (Grasberger and Refetoff 2011).
Iodide undergoes oxidation and is then covalently linked to tyrosine residues of
thyroglobulin, this process is called iodine organification (Stathatos 2012), resulting in 3monoiodotyrosine (MIT) and 3,5-diiodotyrosine (DIT) which bind to form the hormones
T3 and T4; these steps are catalyzed by the enzyme thyroid peroxidase (TPO) (Figure 1-2)
(Targovnik et al. 2010; Cangul et al. 2012a). The resulting thyroglobulin containing MIT,
DIT, T3 and T4, called the mature thyroglobulin, is stored in the colloid and undergoes
4
proteolysis in the lysosome to release predominantly T4 and a small amount of T3 (Figure
1-2) (Targovnik et al. 2010; Grasberger and Refetoff 2011). The released MIT and DIT
undergo deiodination to release iodide which is recycled and used in further hormone
synthesis (Targovnik et al. 2010; Grasberger and Refetoff 2011). Since the potent T3 is
only secreted in small amounts form the thyroid, it is predominantly produced in
peripheral tissues by deiodination of T4 catalyzed by one of three identified enzymes;
Type-1, Type-2, and Type-3 iodothyronine deiodinases (Targovnik et al. 2010).
The production of thyroid hormones is regulated by three major parts: the thyroid
follicle in the thyroid gland, the hypothalamus and the pituitary gland through the action
of the hypothalamic-pituitary-thyroid axis (Stathatos 2012).
Thyroid Follicles
Thyroid follicles are the functional units of the thyroid gland, each follicle is a
cystic structure consisting of a single layer of epithelial cells, termed thyrocytes or
follicular cells, that make up the wall structure of the follicle (Stathatos 2012). Each
follicle is filled with the colloid, a thick sticky matter mostly consisting of thyroglobulin,
which is a large glycoprotein that stores thyroid hormone (Kirsten 2000; Stathatos 2012).
The thyroid gland produces thyroid hormones and stores considerable amounts of them in
the colloid’s thyroglobulin until they are needed by the body (Kirsten 2000).
Hypothalamic-Pituitary-Thyroid Axis
The hypothalamic-pituitary-thyroid (HPT) axis regulates various functions both
during development as well as in adult life through the regulation of thyroid function
(Costa-e-Sousa and Hollenberg 2012; Schmaltz 2012). The hypothalamus secretes
thyrotropin-releasing hormone (TRH) which in turn stimulates the anterior pituitary gland
to secrete thyroid-stimulating hormone (TSH), which stimulates thyroid hormone
production and is essential for thyroid function regulation (Figure 1-3) (Stathatos 2012).
The HPT axis is mainly regulated by a negative feedback system between its three
5
components to ensure equilibrium of serum thyroid hormone levels (Schmaltz 2012).
Small changes in serum thyroid hormone levels affect the HPT axis; high serum thyroid
hormone levels directly inhibit TRH production, whereas low levels stimulate increased
production of TRH in the hypothalamus leading to stimulation of TSH synthesis and
increased thyroid hormone production (Figure 1-3) (Stathatos 2012). Since TSH is
extremely sensitive to serum thyroid hormone levels, it is the test of choice for clinicians
to diagnose most cases of thyroid dysfunction (Stathatos 2012).
Thyroid Stimulating Hormone
A very important regulator of thyroid function is TSH which stimulates the
thyroid gland resulting in secretion of thyroid hormones (Stathatos 2012). TSH effect is
exerted through a specific receptor, the TSH receptor (TSHR), found on the thyrocyte
membrane (Stathatos 2012). TSHR activation results in intracellular effects mediated by
adenylyl cyclase stimulation leading to increased levels of the intracellular secondary
messenger, cyclic adenosine monophosphate (cAMP), which eventually results in
modulation of gene expression in the thyrocytes (Szkudlinski et al. 2002; Stathatos
2012). This ultimately results in an increase in iodine uptake and organification,
increased hormone production and release, as well as promotion of thyroid growth
(Szkudlinski et al. 2002).
Embryological Development of the Thyroid Gland
Thyroid gland embryologic development starts at human embryonic day 22, with
the appearance of the thyroid placode, originating from the embryonic endoderm layer
(Stathatos 2012). The thyroid placode is considered the first morphological evidence for
the thyroid, and is formed by a thickening of the endodermal layer in an area overarching
the aortic sac (De Felice and Di Lauro 2011). However, recent molecular evidence
suggests that 12 to 24 hours before the thickening occurs, specific transcription factors
that are critical for thyroid development, such as NK2 homeobox 1 (NKX2-1) and paired
6
box 8 (PAX8), are expressed in a group of single layered endodermal area cells leading to
their differentiation (De Felice and Di Lauro 2011). This differentiation through a
specific gene expression program is considered the first event in thyroid development (De
Felice and Di Lauro 2011). It is hypothesized that this monolayer of committed cells
recruits other cells to form the multilayer thyroid placode (De Felice and Di Lauro 2011).
The formed thyroid placode then extends into the underlying mesenchyme and migrates
in a dorsal and posterior direction to form the thyroid bud (De Felice and Di Lauro 2011).
The primitive thyroid gland continues to expand to form the two lobes of the thyroid
(Stathatos 2012). When the thyroid cells reach their final destination anterior to the
trachea, precursors of thyroid follicular cells are organized into follicles with activated
terminal differentiation program leading to the expression of specific genes that devote
the cells to the synthesis of thyroid hormones (De Felice and Di Lauro 2011). This
process of thyroid morphogenesis is typically finalized after 49 days when the bilobed
thyroid begins to form follicles and is visible anterior to the trachea (Kratzsch and Pulzer
2008). The fetal thyroid steadily increases in volume in the further course of gestation,
and is capable of concentrating iodide and synthesizing thyroid hormone at about 11 to
13 weeks of gestation (Kratzsch and Pulzer 2008; Stathatos 2012). This specific sequence
of embryologic events is necessary for the normal development of the thyroid gland, and
any defect in these events can lead to developmental thyroid anomalies that result in
disease such as CH (Stathatos 2012).
Molecular Aspects of Thyroid Morphogenesis
Thyroid gland morphogenesis and development depends on numerous genes (De
Felice and Di Lauro 2011). During this process, regulating mechanisms can be divided
into two groups; cell-autonomous and mesoderm-derived (Fagman and Nilsson 2011).
Cell-autonomous regulation is activated through the transcription factors NKX2-1,
FOXE1, PAX8, and HHEX co-expressed by the endoderm layer progenitor cells that are
7
committed to forming the thyroid placode (Fagman and Nilsson 2010; Fagman and
Nilsson 2011). Mesoderm-derived regulation is mediated by mesoderm cells, surrounding
the developing thyroid, expressing the transcription factor TBX1, which is not expressed
in thyroid progenitor cells, as well as mesoderm-derived fibroblast growth factors which
are essential for correct thyroid development (De Felice and Di Lauro 2011; Fagman and
Nilsson 2011).
Thyroid Function in the Fetus
Thyroid hormones are crucial for fetal neurodevelopment (Shields et al. 2011),
and the fetus relies on maternal thyroid hormones, especially during the early stages of
pregnancy (Julvez et al. 2013). During development and up until the second trimester,
the primitive thyroid gland is mainly nonfunctional, and fetal neurodevelopment is solely
dependent on maternal thyroid hormones that enter the fetal circulation across the
placenta (Schmaltz 2012). After the 12th week of gestation and until delivery, fetal TSH
and T4 levels increase, whereas T3 levels remain relatively low (Kratzsch and Pulzer
2008). As thyroid hormone production from the fetus is increasing, the placenta starts to
restrict the permeability of maternal thyroid hormones (Schmaltz 2012). However, there
is evidence that in fetuses with CH, substantial transfer of maternal T4 across the placenta
takes place even during late gestation (Vulsma et al. 1989; Shields et al. 2011).
Thyroid Function in the Neonate
Full Term Newborns
Following delivery, the neonate undergoes a series of changes to adapt to the
extrauterine environment including changes in thyroid function (Kirsten 2000; Schmaltz
2012). The dramatic decrease of temperature that the newborn experiences at delivery,
results in a surge of TRH and TSH (Schmaltz 2012). TSH levels rise in the first 30
minutes after delivery and, in turn, induce increased production of T4 and T3 in the first
8
36 to 48 hours of life (Kirsten 2000). The cold-induced postnatal TSH surge does not last
long and TSH levels start to decrease due to the feedback inhibition by T4, and within the
second day of life, TSH levels return to normal (Kratzsch and Pulzer 2008; Schmaltz
2012). The surge in thyroid hormones T4 and T3 fades by six weeks of life (Schmaltz
2012).
Preterm Newborns
The hypothalamic-pituitary-thyroid (HPT) axis of preterm newborns is immature
and the degree of immaturity depends on gestational age (Kratzsch and Pulzer 2008).
Consequently, the cold-induced postnatal TSH surge is blunted in preterm newborns and
thyroid hormone levels are decreased (Kirsten 2000). These changes in thyroid function
vary between preterm newborns depending on gestational age, and thyroid hormone
levels usually reach levels seen in term newborns by 38 to 42 weeks post-conceptional
age (Kirsten 2000).
Disorders of Thyroid Function
Transient Hypothyroxinemia of Prematurity
In the preterm infant, thyroid function undergoes postnatal changes related to an
immature hypothalamic-pituitary-thyroid (HPT) axis, along with the interrupted exposure
to maternal thyroid hormone and thyroid releasing hormone from the placenta (LaFranchi
1999). Due to immature HPT function T4 is lower in preterm infants compared to
neonates born at term, and there is a direct correlation between the serum T4 level and the
degree of prematurity (LaFranchi 1999; Kratzsch and Pulzer 2008). Preterm neonates
with abnormal thyroid function may have transient hypothyroxinemia of prematurity
(THOP), hence, it is essential to take gestational age and birth weight into consideration
when making the differentiation between THOP and true cases of thyroid disorders such
as congenital hypothyroidism (CH) (Hinton et al. 2010). THOP affects 35-50% of
9
preterm newborns (Berbel et al. 2010) and is characterized by low T4 levels and low to
normal TSH levels (Schmaltz 2012). THOP is strongly correlated with adverse
neurodevelopmental outcomes (La Gamma and Paneth 2012). However, thyroid hormone
replacement therapy of newborns with THOP is controversial and is still under
investigation (Kratzsch and Pulzer 2008; La Gamma and Paneth 2012; Schmaltz 2012).
Congenital Hypothyroidism
Congenital hypothyroidism (CH) is defined as deficient thyroid hormone
production since birth (Abduljabbar and Afifi 2012). CH is a common and preventable
cause of mental retardation with an incidence rate of approximately 1 in 2,350 live births
(Hinton et al. 2010). Early treatment with T4 with subsequent supplementation for life
produces excellent results for both growth and development (Rose et al. 2006; Hinton et
al. 2010). The timing of diagnosis is crucial; the later the treatment is started, the worse
the neurodevelopmental outcome and IQ will be (Kaye et al. 2006b). Infants with CH
appear to be protected during the first few weeks of life due to the maternal thyroid
hormone that crosses the placenta to the fetus (Kaye et al. 2006b; Abduljabbar and Afifi
2012), the best outcome is when treatment is started by two weeks of age (Rose et al.
2006). If treatment is not started, or significantly delayed, clinical features include facial
puffiness, large tongue, hoarse cry, hypothermia, hypotonia, skin mottling, prolonged
jaundice, poor feeding, constipation, lethargy, large fontanels, abdominal distention, and
umbilical hernia (Figure 1-4) (Kaye et al. 2006b; Abduljabbar and Afifi 2012; Schmaltz
2012).
CH incidence is different between ethnicities; it is higher in Hispanics, Asians,
and Native Americans and lower in blacks (Hinton et al. 2010; Abduljabbar and Afifi
2012). The variable incidence rates in different ethnicities suggests the involvement of
genetic factors that have not been discovered yet (Rastogi and LaFranchi 2010). CH
incidence is also affected by gender where it is twice as common in females compared to
10
males (Rose et al. 2006; Hinton et al. 2010). The cause for the increased risk in females
is not well known but is thought to be related to autoimmune risk, which is generally
more common in females (Kaye et al. 2006b; Rastogi and LaFranchi 2010). Newborns
with Down syndrome also have increased CH risk at approximately 1 in 140 (Kaye et al.
2006b).
Newborn Screening
CH is detected shortly after birth through newborn screening. Newborn screening
is a critical public health program started in the 1960s (Wilcken and Wiley 2008).
Newborn screening programs are designed to detect inborn disorders that, if left
untreated, can lead to early mortality or lifelong morbidity and disability (Center for
Disease Control 2001; Watson et al. 2006). It is mandatory to offer newborn screening to
all infants born in the United States, however, parents have the right to opt-out of the
screening (Kaye et al. 2006a; Watson et al. 2006). Screening is done shortly after birth,
usually within the first 48 hours of life (Watson et al. 2006), using blood spotted on a
special card through a heel prick (Kaye et al. 2006a). The timing of newborn screening
sampling is important since most screened analytes have normal ranges that vary
considerably within the first hours or days of life (Wilcken and Wiley 2008). For
example, the TSH surge that occurs immediately after birth may result in a high rate of
false positive results for CH screening when sampling is done before 48 hours of life
(Kaye et al. 2006a).
Approximately 4 million newborns are screened in the United States every year,
and of those 3,000 are identified with a severe condition (Center for Disease Control
2001). Newborn screening programs vary between states in the conditions screened for
and the technology used (Kaye et al. 2006a) There were no national standards for
newborn screening programs until 2006, when the American College of Medical Genetics
(ACMG) published a report with guidelines for state newborn screening programs after
11
being commissioned to do so by the Maternal and Child Health Bureau (Watson et al.
2006).The ACMG recommends mandated screening for 29 identified disorders (Watson
et al. 2006). The disorders screened for include hereditary metabolic disorders (amino
acid disorders, fatty acid oxidation disorders, and organic acid disorders), congenital
endocrinopathies, hemoglobinopathies, and cystic fibrosis (Center for Disease Control
2001; Kaye et al. 2006a). Furthermore, many infants are screened for congenital hearing
loss as part of the newborn screening program (Kaye et al. 2006a). The Iowa Neonatal
Metabolic Screening Program (INMSP) screens for all 29 disorders recommended by the
American College of Medical Genetics and an additional 14 metabolic conditions making
it one of the most comprehensive newborn screening programs in the United States
(National Newborn Screening and Genetics Resource Center 2013).
CH screening was added to existing newborn screening programs in the mid
1970s (Kaye et al. 2006b). CH is screened for at birth in the newborn screening program
through detection of T4, TSH, or both (Wilcken and Wiley 2008). There is no consensus
on a single best CH screening protocol; 131 newborn screening programs worldwide use
TSH for CH screening and 75 use a T4/TSH screening protocol, but all screening is done
using an immunoassay technique (Pass and Neto 2009). Each screening method misses
certain CH syndromes, and the best protocol is simultaneous testing of T4 and TSH at the
same time, which is implemented in 5 states, but was considered expensive and time
consuming until the recent development of multi-analyte assays that can test several
biomarkers in the same assay well simultaneously (Pass and Neto 2009). The Iowa
Neonatal Metabolic Screening Program (INMSP) uses TSH only for CH screening (Pass
and Neto 2009).
Unfortunately, newborn screening for congenital hypothyroidism has the highest
number of false positive results with repeated testing costs of more than two million
dollars annually (Kwon and Farrell 2000). It was estimated that only 3.9% of screen
positive newborns are true positives who get diagnosed with CH (Pass and Neto 2009).
12
The false positive result rate is usually higher in newborn screening programs that use T4
as a primary analyte (0.30%) compared to programs that use TSH (0.05%) (Kaye et al.
2006b). However, most newborn screening programs in the United States still use T4 as
the primary analyte, and an advantage of this is the ability to identify infants with
secondary hypothyroidism that have no TSH surge, or infants with delayed TSH surge
such as preterm infants, both of which would be missed in programs that measure TSH as
the primary analyte (Kaye et al. 2006b). Preterm infants account for the largest
percentage of newborns with false positive CH screening results due to their low T4
levels resulting from the immature HPT axis (Kaye et al. 2006b).
All newborns with T4 level below the 10th percentile in the newborn screening
programs that use T4 as an initial analyte, get a follow-up TSH screen (Kaye et al.
2006b). If final newborn screen results for CH are abnormal, the infant must be recalled
immediately for follow-up confirmatory serum testing of thyroid function (Kaye et al.
2006b; Rastogi and LaFranchi 2010). Confirmatory serum testing includes TSH, free or
total T4, and a binding protein measure such as T3 resin uptake, and is usually done
around one to two weeks of age (Rastogi and LaFranchi 2010). Once a CH diagnosis is
confirmed, treatment should be started immediately, and then additional optional
diagnostic studies may be done to determine the underlying etiology of CH (Kaye et al.
2006b).
Etiology of Congenital Hypothyroidism
Congenital hypothyroidism (CH) is a heterogeneous disorder and is classified into
two forms; transient and permanent (Abduljabbar and Afifi 2012).
Transient Congenital Hypothyroidism
Transient CH is a temporary thyroid hormone deficiency that is present at birth,
but normal thyroid hormone production is recovered during the first months or years of
life (Abduljabbar and Afifi 2012). Transient CH etiology is classified into maternal or
13
neonatal factors. Maternal factors include transplacental passage of antithyroid
medications, TSH receptor antibodies, and iodine deficiency or excess (Rastogi and
LaFranchi 2010). Neonatal factors include iodine deficiency or excess, heterozygous
mutations in DUOX2 and DUOXA2 genes leading to transient or permanent CH, and
congenital liver hemangiomas (Rastogi and LaFranchi 2010; Abduljabbar and Afifi
2012). Transient CH is more common in iodine deficient parts of the world such as
Europe where the incidence is reported to be 1 in 100, whereas in the United States, an
iodine sufficient country, the incidence is 1 in 50,000 (Rastogi and LaFranchi 2010).
Permanent Congenital Hypothyroidism
Permanent CH is, by definition, a persistent thyroid hormone deficiency that
requires thyroid hormone replacement therapy for life (Abduljabbar and Afifi 2012).
Permanent CH etiology is classified into primary or secondary.
Primary Congenital Hypothyroidism
Primary CH causes include abnormal development of the thyroid gland (thyroid
dysgenesis, agenesis, or ectopy), abnormal thyroid hormone production from a
structurally normal gland (thyroid dyshormonogenesis), and TSH binding or signaling
defects (Rose et al. 2006; Rastogi and LaFranchi 2010). In iodine sufficient countries,
abnormal thyroid gland development is the most common cause of CH accounting for 8085% of CH cases (Hinton et al. 2010; Rastogi and LaFranchi 2010). Thyroid dysgenesis
CH is mostly sporadic; only 2% of cases have a known causing mutation in one of the
genes necessary for thyroid development (NKX2.1, NKX2.5, PAX8, or FOXE1), whereas
the remaining 98% of cases have an unknown cause (Rastogi and LaFranchi 2010;
Abduljabbar and Afifi 2012). In the cases with a mutation in one of the genes encoding a
transcription factor, CH may be present as part of a syndrome; for example FOXE1
mutations lead to Bamforth-Lazarus Syndrome (Rastogi and LaFranchi 2010).
14
The remaining ~15% of CH cases have a molecular defect in one of the genes in
the thyroid hormone biosynthesis pathway most commonly inherited as autosomal
recessives (Abduljabbar and Afifi 2012). Most commonly the defect is in a gene affecting
the activity of the enzyme thyroid peroxidase such as DUOX2, DUOXA2, and SLC26A4.
Rarely, cases of dyshormonogenesis result from a mutation in the gene encoding the
sodium/iodide transporter (SLC5A5) (Rastogi and LaFranchi 2010).
Secondary or Central Congenital Hypothyroidism
Secondary CH, also called central CH, generally results from TSH production
defects, and is most commonly part of congenital hypopituitarism (Rastogi and LaFranchi
2010). In rare cases, certain genetic mutations result in secondary CH; these include
mutations in the thyrotropin releasing hormone (TRH) receptor gene leading to TRH
resistance, and mutations in the gene encoding the TSH β subunit leading to TSH
deficiency(Rastogi and LaFranchi 2010).
Adult-Onset Hypothyroidism
Adult-onset hypothyroidism results from inadequate thyroid hormone production
or action. It is a common disorder affecting about 0.3% of the population in the United
States, and it is more prevalent in women, the elderly, and certain ethnic groups. Just like
congenital hypothyroidism (CH), adult-onset hypothyroidism may be transient or
permanent, and can be primary, resulting from thyroid gland abnormalities, or secondary,
resulting from abnormalities in the hypothalamic-pituitary-thyroid axis (Almandoz and
Gharib 2012). The most common cause of hypothyroidism worldwide is iodine
deficiency, however, in iodine sufficient areas, autoimmune disease, known as
Hashimoto’s thyroiditis, is the leading cause (Vanderpump 2011). Hypothyroidism
symptoms are often subtle but may include fatigue, muscle aches, constipation, dry skin,
cold intolerance, and vocal changes (Almandoz and Gharib 2012). If left untreated,
hypothyroidism can affect blood pressure, lipid levels, fertility, cognition, and
15
neuromuscular function (Gaitonde et al. 2012). The best laboratory test for
hypothyroidism is serum thyroid stimulating hormone (TSH) measurement, if it is found
to be elevated, it is followed by a serum free thyroxine (FT4) measurement.
Hypothyroidism is diagnosed based on elevated serum TSH levels with low serum FT4
levels, and is treated with thyroid hormone replacement therapy (Almandoz and Gharib
2012; Gaitonde et al. 2012).
Genetics of Thyroid Stimulating Hormone
The hypothalamic-pituitary-thyroid axis is complexly regulated both by genetic as
well as physiological factors, leading to the individuality of thyroid hormone and TSH
levels in each subject both in normality and in thyroid dysfunctional states (Midgley et al.
2013). This is observed in the distribution of TSH levels in the population versus in an
individual; it was found that TSH has a wide population reference range whereas the
range is much narrower in the same individual TSH levels over a period of time
(Andersen et al. 2002; Panicker 2011; Hoermann and Midgley 2012; Midgley et al.
2013). Several studies tried to estimate the genetic contribution to this individuality in
TSH levels through twin-based or family-based study designs (Panicker 2011). TSH
heritability was estimated to vary from 32% (Samollow et al. 2004), to 64% (Hansen et
al. 2004), and to a maximum of 65% (Panicker et al. 2008). Heritability is defined as the
proportion of the phenotypic variation in a trait that is attributable to genetic factors. The
heritability of a given phenotype can be estimated from the difference of trait variation
between monozygotic and dizygotic twin pairs (Boomsma et al. 2002). There have been
several genome-wide association studies (GWAS) as well as candidate-gene studies to
identify the genes that are responsible for the heritability of TSH levels and thyroid
function.
16
Genome-Wide Association Studies
Genome-wide association studies (GWAS) are designed to search for common
genetic variants that are associated with complex traits or diseases through the
genotyping of hundreds of thousands to millions of single nucleotide polymorphisms
(SNPs) across the genome in hundreds or even thousands of individuals (Manolio 2010).
GWAS allow for interrogating the entire genome without a prior hypothesis or
premeditated candidate gene selection (Dube and Hegele 2013). SNPs that are found to
be associated with a trait or disease in GWAS are typically not the causative variant, but
are surrogates for most other variants, and potentially the causative variant, in nearby loci
through linkage disequilibrium (LD) (Dube and Hegele 2013). LD implies that SNPs are
transmitted from one generation to the next in blocks, and genotyping a few SNPs in each
block, called tag SNPs, can capture the variation of most other SNPs within that block
(Manolio 2010). This LD phenomenon is the result of the low recombination rate of
approximately 1 crossover per 100 megabases per generation (Altshuler et al. 2008).
However, the transition from a GWAS significantly associated SNP to the identification
of the specific etiologic variant that is tagged by the GWAS signal is still challenging
(Dixon et al. 2011).
To date, six GWAS and two meta-analyses have been published with TSH level
as one of the phenotypes studied (Table 1-1) (Hwang et al. 2007; Arnaud-Lopez et al.
2008; Gudmundsson et al. 2009; Lowe et al. 2009; Panicker et al. 2010; Gudmundsson et
al. 2012; Rawal et al. 2012; Porcu et al. 2013). The GWAS by Hwang et al. (2007)
studied 810 individuals form the Framingham Heart Study for genetic association with
mean TSH levels from two measurements. Two of the top three significantly associated
SNPs are intergenic on chromosome 7 and the third SNP is in an intron of HACE1
(Hwang et al. 2007).
The second TSH related GWAS was done by Arnaud-Lopez et al. (2008) on
4,300 Sardinians, and the strongest identified association was for an intronic SNP in
17
PDE8B (Figure 1-5). This association was successfully replicated in an additional 4,158
individuals form Sardinia, Tuscany, and the Old Order Amish (Arnaud-Lopez et al.
2008). The PDE8B gene encodes a high affinity adenosine 3’,5’-cyclic monophosphate
(cAMP)-specific phosphodiesterase to regulate the level of cAMP in cells and plays a
vital role in signal transduction (Hayashi et al. 1998; Lakics et al. 2010). In the ArnaudLopez et al. paper, the authors suggest that since cAMP is necessary for thyroid-hormone
secretion due to TSH stimulation; when PDE8B catalyzes the hydrolysis and inactivation
of cAMP in the thyroid gland, it results in decreased generation of thyroid-hormone T4
and T3 resulting in the negative feedback loop to act on producing more TSH (ArnaudLopez et al. 2008).
The third GWAS done by Lowe et al. (2009) on over 2,800 Micronesian
individuals found a novel significant association for 10 SNPs in a region on chromosome
9 encompassing the gene encoding thyroid transcription factor 2 (TTF-2, now known as
FOXE1) with TSH levels. This was the first report of an association for this locus with
the variation of TSH levels, which is interestingly, a strong biological candidate gene
(Lowe et al. 2009). FOXE1 gene encodes a transcription factor that is essential for the
initiation of thyroid differentiation at the embryonic stage (Parlato et al. 2004). Mutations
of the FOXE1 gene may result in thyroid dysgenesis leading to congenital
hypothyroidism (Castanet and Polak 2010). FOXE1 also plays an important role in
regulating the transcription of different thyroid-specific genes resulting in regulation of
thyroid-hormone synthesis (Gudmundsson et al. 2009). This GWAS also replicated the
PDE8B finding reported previously in Caucasians by Arnaud-Lopez et al. (2008).
Next, Gudmundsson et al. (2009) studied the genetic association with serum TSH
levels in a population of ~12,000 Icelanders for two SNPs that were previously found to
be significantly associated with thyroid cancer in a GWAS. The two intergenic SNPs
were found to be significantly associated with serum TSH levels; one is on chromosome
9 and the other is on chromosome 14, with FOXE1 and NKX2-1 being the nearest genes
18
respectively (Gudmundsson et al. 2009). NKX2-1 and FOXE1 are plausible candidates
given their involvement in thyroid gland development; both genes encode transcription
factors necessary for proper thyroid organogenesis and are referred to as thyroid
transcription factor 1 and 2 (TTF1 and TTF2) respectively (Gudmundsson et al. 2009).
The fifth GWAS done by Panicker et al. (2010) on 2,014 twins from the United
Kingdom identified a novel locus on chromosome 1, near CAPZB gene, to be
significantly associated with serum TSH levels (Figure 1-6). This finding was
successfully replicated in an independent cohort of 1,093 Australian individuals
(Panicker et al. 2010). CAPZB gene encodes the beta subunit of an actin binding protein
that helps regulate the growth of the actin filament. It is known to be expressed in the
thyroid, brain, and pituitary, making it a plausible candidate for involvement in pituitarythyroid axis regulation, however, the mechanism is not known yet (Panicker et al. 2010).
The sixth GWAS done by Gudmundsson et al. (2012) on 27,758 Icelandic
individuals reported 22 SNPs to be significantly associated with serum TSH levels at a pvalue <5x10-8. Of the loci previously identified to be associated with TSH levels; the
PDE8B locus (Arnaud-Lopez et al. 2008), the chromosome 9 and chromosome 14 loci
(Gudmundsson et al. 2009), and the chromosome 1 locus (Panicker et al. 2010), were
replicated in this GWAS (Gudmundsson et al. 2012).
Rawal et al. (2012) performed a meta-analysis of two GWAS, with a total sample
size of 3736 individuals of European ancestry, to identify genetic associations with TSH
levels. The meta-analysis results showed statistically significant associations with four
loci (Figure 1-7), two of which replicate previous GWAS findings for PDE8B on
chromosome 5 (Arnaud-Lopez et al. 2008), and CAPZB on chromosome 1 (Panicker et
al. 2010). The third locus is in an intergenic region on chromosome 16, near MAF, that
region was previously found in a GWAS to be associated with thyroid volume and goiter
(Teumer et al. 2011). The forth locus is on chromosome 4 upstream of NR3C2, and this is
the first report of an association between this locus and TSH levels (Rawal et al. 2012).
19
NR3C2 encodes the mineralocorticoid receptor that mediates the actions of aldosterone
and functions as a transcription factor. It is highly expressed in the thyroid gland, and the
authors hypothesize that it may be involved in regulating the expression of thyroid
specific genes involved in the transduction of the received TSH/cAMP signal (Rawal et
al. 2012). All four loci were successfully replicated in 3,727 individuals of European
ancestry (Rawal et al. 2012).
Recently, Porcu et al. (2013) performed a large meta-analysis of GWAS to
identify genetic variants associated with serum TSH in over 26,000 euthyroid European
individuals from 18 studies. The authors reported 19 loci to be significantly associated
with TSH levels (Figure 1-8). Four loci replicate previous GWAS findings for PDE8B
(Arnaud-Lopez et al. 2008), CAPZB (Panicker et al. 2010), NR3C2 and chromosome 16
region, near MAF (Rawal et al. 2012), whereas the remaining 15 loci are novel (Porcu et
al. 2013).
Candidate-Gene Studies
Candidate-gene studies select genes that are suspected to play a role in thyroid
physiology based on biological information, the selected genes are then studied and fine
mapped for associations (Panicker 2011). Candidate-gene studies identified a
polymorphism in the TSH receptor gene (TSHR) to be associated with adult serum TSH
levels (Hansen et al. 2007). However, this finding was not replicated in GWAS (Panicker
2011). The lack of reproducibility for candidate-gene studies in GWAS is a common
occurrence in complex traits and diseases. A possible explanation for this is publication
bias, which refers to the higher likelihood of publication for positive results compared to
negative results, implying the possibility that those were not true associations, but rather
false positive findings (Bosker et al. 2011). However, other explanations are that
phenotyping of complex traits and diseases across different studies may vary, and that
complex traits and diseases are affected by gene-gene and gene-environment interactions
20
that may be different across populations, and all this variability may lead to the lack of
reproducibility (Bosker et al. 2011). Therefore, it has been argued that GWAS, at this
point, are not designed to definitively exclude the role of possible candidate genes in
complex traits or diseases (Michel et al. 2010).
Many other biologically plausible genes, such as the genes encoding thyroid
hormone receptors (THRA and THRB) and thyroid hormone transporter (MCT8) have
been studied in candidate-gene studies but have not shown significant associations
(Panicker 2011). The three genes encoding the three iodothyronine deiodinases (DIO1,
DIO2, and DIO3) have also been studied because of their vital role in thyroid function,
but no association with serum TSH levels was found (Panicker 2011).
Main Thyroid Related Genes
PDE8B
The phosphodiesterase 8B (PDE8B) gene is located on chromosome 5. It is
expressed most abundantly in the thyroid gland where it has threefold higher level than in
the next highest tissue (Lakics et al. 2010). It is expressed at lower levels in some other
tissues including the brain, spinal cord, and placenta (Hayashi et al. 1998). The PDE8B
gene encodes a high affinity adenosine 3’,5’-cyclic monophosphate (cAMP)-specific
phosphodiesterase that catalyzes hydrolysis of cAMP to regulate its level in cells, and
therefore plays a vital role in signal transduction (Hayashi et al. 1998; Lakics et al. 2010;
Panicker 2011). Mutations of PDE8B result in the autosomal-dominant striatal
degeneration (ADSD) disease (Appenzeller et al. 2010). However, a study of a large
family with ADSD did not find any thyroid function abnormalities in affected individuals
(Kuhlenbaumer et al. 2004). PDE8B mutations were also found in patients with adrenal
hyperplasia and Cushing syndrome (Horvath et al. 2008).
21
NKX2-1
NK2 homeobox 1 (NKX2-1) gene, also called thyroid transcription factor 1
(TTF1), encodes a transcription factor that is necessary for the regulation of thyroid
specific gene expression as well as thyroid morphogenesis (Parlato et al. 2004).
Mutations in this gene are associated with congenital hypothyroidism due to thyroid
dysgenesis (Rastogi and LaFranchi 2010). A role of NKX2-1 in regulating TSH level is
supported by two GWAS (Gudmundsson et al. 2009; Gudmundsson et al. 2012).
FOXE1
Forkhead box E1 (FOXE1) gene, also called thyroid transcription factor 2 (TTF2),
is located on chromosome 9. FOXE1 encodes a transcription factor that is essential for
the initiation of thyroid differentiation at the embryonic stage (Parlato et al. 2004).
Mutations of the FOXE1 gene may result in thyroid dysgenesis leading to both familial as
well as cases of syndromic congenital hypothyroidism in the Bamforth-Lazarus
Syndrome, Online Mendelian Inheritance in Man (OMIM) #241850 (Online Mendelian
Inheritance in Man 2013), a rare inherited disorder characterized by CH, cleft palate, and
spiky hair (Castanet and Polak 2010). FOXE1 also plays an important role in regulating
the transcription of different thyroid-specific genes resulting in regulation of thyroidhormone synthesis (Gudmundsson et al. 2009).
TSHR
Thyroid stimulating hormone receptor (TSHR) gene is located on chromosome 14.
The protein encoded by the TSHR gene is the TSH receptor (TSHR). TSHR is present on
thyroid cells, and when activated by TSH secreted from the pituitary gland, intracellular
cAMP is upregulated resulting in activation of various cellular processes ending with an
increased production of thyroid hormone (Stathatos 2012). TSHR activating mutations
cause several types of hyperthyroidism (Hebrant et al. 2011). TSHR loss of function
22
mutations may lead to an autosomal recessive form of thyroid dysgenesis (Cangul et al.
2012b).
CAPZB
F-actin-capping protein subunit beta (CAPZB) gene encodes the beta subunit of an
actin binding protein that helps regulate the growth of the actin filament. It was found to
be associated with TSH levels in two GWAS and two meta-analyses (Panicker et al.
2010; Gudmundsson et al. 2012; Rawal et al. 2012; Porcu et al. 2013). It is known to be
expressed in the thyroid, brain, and pituitary, making it a plausible candidate for
involvement in pituitary-thyroid axis regulation, however, the mechanism is not known
yet (Panicker et al. 2010; Panicker 2011).
Purpose of Study
It is well established that genetic variants play an important role in defining
thyroid function throughout life, both in health as well as in disease states. The role of
genetics has been extensively studied through GWAS and candidate-gene studies, and
several genes have been identified to be associated with the variation of thyroid function
between individuals. Elucidating the genetic basis of thyroid function variability is
currently an area of interest not only to advance our understanding of thyroid physiology,
but also to further the understanding of adult conditions related to thyroid function. For
example, low serum TSH levels are associated with an increased risk of atrial fibrillation
in adults over 60 years old (Sawin et al. 1994). Thyroid hormone levels within the normal
physiological range have also been shown to affect bone mass and density in healthy men
aged 25-45 years (Roef et al. 2011), as well as in men and women above 55 years of age
(van der Deure et al. 2008). Furthermore, some of the genetic variation reported to be
associated with thyroid function was also found to be associated with several other
clinical and developmental phenotypes (Panicker 2011). For example, variants in DIO2
23
were found to be associated with osteoarthritis, and variants in TSHR were found to be
associated with bone density, insulin resistance, and longevity (Panicker 2011).
Although there have been many significant new findings in the genetics of thyroid
function over the past decade, we are still at the beginning and there are more genes and
pathways yet to be discovered (Panicker 2011). Furthermore, most studies address
thyroid function in adulthood and none in the neonatal phase. The purpose of this study is
to examine genetic associations with thyroid function, namely TSH level variation, in the
neonatal period. This will enhance our understanding of thyroid function in newborns, as
well as potentially identify avenues for the early prediction of adult diseases that are
associated with thyroid function genetic variants.
Hypothesis
Genetic polymorphisms within biologically relevant pathways, including
neuroendocrine pathways, are associated with the normal variation of TSH levels in
neonates.
Specific Aims
Specific Aim 1: Estimate the heritability of TSH level using newborn blood spot
cards of monozygotic and dizygotic twin pairs.
Specific Aim 2: Identify SNPs associated with normal variation in TSH
measurements, obtained from the Iowa Neonatal Metabolic Screening Program, in
euthyroid preterm and term infants.
Specific Aim 3: Fine mapping of potential FOXE1 and PDE8B enhancer regions
to identify genetic variants that are associated with normal variation in neonatal TSH
measurements.
24
Table 1-1 Summary of GWAS data for TSH
GWAS
Associated Locus
Candidate Gene in
Region
P-Value
Hwang et al. 2007
7p21
6q16
7p15
Intergenic
HACE1
Intergenic
4 x 10-6
7 x 10-6
8 x 10-6
Arnaud-Lopez et al.
2008
5q13
PDE8B
1 x 10-11
Lowe et al. 2009
9q22
5q13
FOXE1
PDE8B
1 x 10-6
3 x 10-4
Gudmundsson et al.
2009
9q22
14q13
FOXE1
NKX2-1
3 x 10-14
3 x 10-2
Panicker et al. 2010
1p36
CAPZB
3 x 10-8
Gudmundsson et al.
2012
5q13
9q22
1p36
14q13
PDE8B
FOXE1
CAPZB
NKX2-1
3 x 10-62
4 x 10-31
4 x 10-26
1 x 10-16
Rawal et al. 2012
5q13
4q31
16q23
1p36
PDE8B
NR3C2
MAF
CAPZB
3 x 10-27
3 x 10-10
6 x 10-10
2 x 10-8
Porcu et al. 2013
5q13
1p36
16q23
4q31
PDE8B
CAPZB
MAF
NR3C2
2 x 10-56
4 x 10-21
9 x 10-18
9 x 10-16
25
Figure 1-1 Thyroid gland. Anterior view of the thyroid gland showing its location below
the larynx and anterior to the trachea.
Source: (Kirsten 2000). Reprinted with permission from Springer Publishing Company:
Neonatal Network, Volume 19, Number 8, Endocrine Series #6, Figure 1.
26
Figure 1-2 Iodine organification and thyroid hormone synthesis.
Source: (Stathatos 2012). Reprinted with permission from Elsevier.
27
Figure 1-3 Hypothalamic-pituitary-thyroid axis regulation.
Source: (Stathatos 2012). Reprinted with permission from Elsevier.
28
Figure 1-4 Three month old infant with untreated congenital hypothyroidism. (A) This
picture demonstrates hypotonia. (B) This picture demonstrates facial puffiness, large
tongue, large fontanels, and skin mottling. (C) This picture demonstrates abdominal
distention, and umbilical hernia.
Source: (Rastogi and LaFranchi 2010). Reprinted with permission from BioMed Central.
29
Figure 1-5 A Manhattan plot of the TSH level GWAS done by (Arnaud-Lopez et al.
2008). SNPs are arranged by chromosome number and plotted on the X-axis. The Y-axis
is the –log10 of the association p-value.
Source: (Arnaud-Lopez et al. 2008). Reprinted with permission from Elsevier.
30
Figure 1-6 A Manhattan plot of the TSH level GWAS done by (Panicker et al. 2010).
SNPs are arranged by chromosome number and plotted on the X-axis. The Y-axis is the –
log10 of the association p-value.
Source: modified from (Panicker et al. 2010). Reprinted with permission from Elsevier.
31
Figure 1-7 A Manhattan plot of the TSH level GWAS meta-analysis done by (Rawal et
al. 2012). SNPs are arranged by chromosome number and plotted on the X-axis. The Yaxis is the –log10 of the association p-value. The upper horizontal line indicates the
genome-wide threshold of statistical significance of p-value of 5 x 10-8.
Source: (Rawal et al. 2012). Reprinted with permission from Oxford University Press.
32
Figure 1-8 A Manhattan plot of the TSH level GWAS meta-analysis done by (Porcu et al.
2013). SNPs are arranged by chromosome number and plotted on the X-axis. The Y-axis
is the –log10 of the association p-value. The horizontal line indicates the genome-wide
threshold of statistical significance of p-value of 5 x 10-8. The loci that reached genomewide significance are highlighted in green.
Source: Modified from (Porcu et al. 2013). Reprinted form PLOS Genetics, no
permission required under the Creative Commons Attribution License.
33
CHAPTER 2
THE HERITABILITY OF METABOLIC PROFILES IN NEWBORN
TWINS
The following manuscript was published in Heredity, 2013; 110: 253-258.
Additional authors include Daniel Cook, Oleg Shchelochkov, Lauren Fleener, Stanton
Berberich, Jeffrey Murray, and Kelli Ryckman.
The objective of the work described in this chapter is to estimate the heritability
of thyroid stimulating hormone (TSH) and other metabolites routinely measured in
newborns. TSH heritability of up to 65% has been estimated in adults; however, to-date
has not been reported in neonates. Our study is the first to assess heritability of TSH
levels in the neonatal period, as well as the first to use newborn blood spot card
measurements to estimate the genetic heritability of any trait, illustrating the utility of
stored newborn blood spot cards as a valuable resource for genetic studies. We estimated
the heritability of neonatal TSH at 58% which is consistent with the previous reports of
TSH heritability in adults. This study provides direct evidence for a strong genetic
contribution to TSH variability at birth.
Drs. Jeffrey Murray and Kelli Ryckman provided oversight for all aspects of the
project, provided input into study design and assisted in the writing and editing of the
manuscript. Dr. Ryckman also performed statistical analysis with the assistance of Daniel
Cook. Dr. Oleg Shchelochkov provided valuable insight into newborn screening and
editing the manuscript. Lauren Fleener performed TaqMan genotyping. Dr. Stanton
Berberich provided input into the study design and access to study samples and data. I
was involved in study design, literature review, performed DNA extraction from newborn
blood spot cards for all twin samples and assisted in the analysis. I also wrote the
manuscript, revisions, and responses to reviewer critiques.
34
Abstract
Identifying genetic and metabolic biomarkers in neonates has the potential to
improve diagnosis and treatment of common complex neonatal diseases, and potentially
lead to risk assessment and preventative measures for common adulthood illnesses such
as diabetes and cardiovascular disease. There is a wealth of information on using fatty
acid, amino acid, and organic acid metabolite profiles to identify rare inherited congenital
diseases through newborn screening, but little is known about these metabolic profiles in
the context of the “healthy” newborn. Recent studies have implicated many of the amino
acid and fatty acid metabolites utilized in newborn screening in common complex adult
diseases such as cardiovascular disease, insulin resistance, and obesity. To determine the
heritability of metabolic profiles in newborns, we examined 381 twin pairs obtained from
the Iowa Neonatal Metabolic Screening Program. Heritability was estimated using
multilevel mixed-effects linear regression adjusting for gestational age, gender, weight
and age at time of sample collection. The highest heritability was for short chain
acylcarnitines, specifically butyrylcarnitine (C4) (h2=0.66, P=2x10-16),
methylmalonylcarnitine (C4-DC) (h2=0.83, P<10-16) and isovalerylcarnitine (C5)
(h2=0.61, P=1x10-9). Thyroid stimulating hormone (TSH) (h2=0.58, P=2x10-5) and
immunoreactive trypsinogen (IRT) (h2=0.52, P=3x10-9) also have a strong genetic
component. This is direct evidence for a strong genetic contribution to the metabolic
profile at birth and that newborn screening data can be utilized for studying the genetic
regulation of many clinically relevant metabolites.
Introduction
Metabolomics is the study of metabolites, small molecules that make up the
building blocks of cellular processes (Goonewardena et al. 2010). Metabolomics is a
rapidly developing field of great importance in understanding the physiology of dynamic
cellular processes and for diagnosis of human diseases. Better understanding of the
35
metabolic profiles present in the immediate postnatal period is important for their short
term contribution to diagnosis as well as for the long term prediction of outcomes.
Metabolic profiles of the neonate, defined by levels of amino acid, organic acid, and fatty
acid oxidation metabolites, may be correlated with metabolic conditions in adulthood,
such as obesity, diabetes and cardiovascular disease through the phenomenon of
metabolic programming (Srinivasan and Patel 2008).
Understanding the genetic contribution to metabolic profiles, particularly in the
neonate, may provide insight into complex diseases and their risks. The underlying
genetic contribution to metabolic traits has been studied in plants (Keurentjes et al.
2006), mice (Ferrara et al. 2008), and more recently, in adult humans (Shah et al. 2009).
However, to-date, we are aware of no studies examining the heritability of metabolic
traits related to amino acid and fatty acid oxidation in the neonatal period.
Population-based metabolic profiling is most commonly implemented in Statemandated neonatal screening programs used to detect numerous endocrine and metabolic
disorders at birth. Levels of amino acids, including branched-chain amino acids, and
acylcarnitines are measured to detect newborns with rare disorders that are treatable, if
detected early (Wilcken and Wiley 2008). Some hormones and enzyme activities are also
measured including thyroid stimulating hormone (TSH), immunoreactive trypsinogen
(IRT), and 17-hydroxyprogesterone (17-OHP) to detect disorders such as congenital
hypothyroidism, cystic fibrosis, and congenital adrenal hyperplasia respectively (Center
for Disease Control 2001; Khoury et al. 2003; Votava et al. 2005). In addition to
detecting disorders at birth, branched-chain amino acids have been associated with adult
diseases including type 2 diabetes and cardiovascular disease (Shah et al. 2010; Wang et
al. 2011).
There are several genome-wide association studies that have identified genetic
loci associated with metabolite measurements from adult human blood and/or urine
samples (Gieger et al. 2008; Illig et al. 2010; Suhre et al. 2011a; Suhre et al. 2011b;
36
Kettunen et al. 2012). While initial results are promising, less effort has been devoted to
identifying the underlying heritability of metabolic traits in humans at different times of
development, particularly at birth. The heritability of biomarkers for amino acid and fatty
acid oxidation is virtually unexplored in adults or neonates with the exception of a single
study examining an extensive panel of metabolic markers from adult plasma samples
(Shah et al. 2009). The authors demonstrated high heritability among several amino acids
and acylcarnitines in eight multiplex families with a family history of premature
cardiovascular disease (Shah et al. 2009). A recent study by Kettunen et al. examined the
heritability for amino acids, lipoproteins, lipids, and some other metabolites such as
glucose and urea in adult serum samples; however, the paper does not investigate
acylcarnitines which are important for fatty acid oxidation (Kettunen et al. 2012). An
additional study by Nicholson et al. investigates the genetic and environmental
contribution to human metabolic profiles, and the authors report estimations of familial
variation for different metabolite measurements; however they state that their sample size
is insufficient for heritability estimations (Nicholson et al. 2011). A few other studies
have shown a high degree of heritability in adult hormone measurements, particularly,
adult serum levels of TSH where heritability estimates ranged from 32% (Samollow et al.
2004) to 64% (Hansen et al. 2004) to 65% (Panicker et al. 2008).
In this study, we obtained twin samples from the Iowa Neonatal Metabolic
Screening Program (INMSP) to determine the heritability of hormone, enzyme,
acylcarnitine, and amino acid measurements measured during routine newborn screening.
Understanding the heritability of these analytes at birth may increase our understanding
of physiologic processes and metabolic programming in various adulthood diseases.
Furthermore, identifying the heritable components of the metabolome, particularly in the
neonatal period, may pave the way for future genetic association studies that may provide
insight into the physiology of different cellular processes, as well as the biology of
complex neonatal and adulthood diseases.
37
Methods
Study Population
Metabolic data for 47 analytes from routine newborn screening were obtained
from the University of Iowa State Hygienic Laboratory (SHL) for 243 same-sex twin
pairs (130 male-male twin pairs and 113 female-female twin pairs) and 165 male-female
twin pairs born in 2009 (Table 2-1). Twins were identified by the SHL based on both
infants having the same birth date, gestational age, mother’s first name and facility
identification number. Newborn dried blood spots (DBS) were obtained from a heel stick
24-72 hours after birth. DBS specimens were collected, dried and handled according to
the Clinical Laboratory Standards Institute (CLSI) guideline (Hannon et al. 2007). DBS
specimens were transported to the SHL within 5 days of collection, and evaluated for
quality at the time of arrival by trained technical staff. Blood spot cards were obtained for
DNA extraction and zygosity testing for all same-sex twin pairs. Approval for use of the
de-identified data and blood spot cards was granted by the Iowa Department of Public
Health and a waiver of consent was obtained from the Institutional Review Board of the
University of Iowa (IRB#200908793). DNA was extracted from one dried whole blood
spot using the AutoGen (Holliston, MA, USA) QuickGene-810 nucleic acid extraction
machine with the DNA Tissue Kit (catalogue number DT-S) and following
manufacturer’s recommendations.
Enzymatic Assays
Quantification of 17-hydroxyprogesterone (17-OHP), TSH and IRT were
determined by solid phase, time-resolved fluoroimmunoassay from dried newborn blood
spots using Perkin Elmer’s AutoDELFIA® platform (Waltham, MA, USA). Galactose-1phosphate uridyl transferase (GALT) was determined by a semi-quantitative enzymatic
assay by Perkin Elmer (Waltham, MA, USA) based on the Beutler method.
38
Tandem Mass Spectrometry
Tandem mass spectrometry is performed in neonatal screening to detect levels of
amino acids and acylcarnitines. Screening procedures in Iowa are based on previously
established methodology (Chace et al. 2001; Turgeon et al. 2008; Chace et al. 2009).
Briefly, a derivatization method is used in which butyl esters of acylcarnitines and amino
acids are prepared from the extracts. For succinylacetone, hydrazine derivatives are
prepared. Tandem mass spectrometry is performed with Waters Quattro Micro triple
quadrupole tandem mass spectrometers, equipped with an electrospray ionization source
operated in the positive ion mode. Sensitivity and resolution checks on the instruments
are performed daily and calibration and mass accuracy adjustments are done 2 – 3 times
per year. Multiple reaction monitoring (MRM) mode is used to scan for specific mass ion
intensities. Concentrations are obtained from the ratio of ion intensity (cps) at the mass
that represents a specific analyte compared with its isotopically labeled internal standard
and correcting for blood volume in a 1/8 inch DBS punch. Both internal and external
spiked control specimens, a normal control specimen, and a blank are analyzed with each
batch of specimens. The external spiked control specimens are obtained from Newborn
Screening Quality Assurance Program at the Centers for Disease Control.
Determination of Zygosity
Zygosity was determined based on concordance of genetic markers by genotyping
20 markers with high heterozygosity (~0.5) (Table 2-2) that were not in linkage
disequilibrium with one another. Genotyping was performed using the TaqMan®
chemistry genotyping system (Applied Biosystems, Foster City, CA, USA). All SNP
genotyping assays were available and ordered using the Assay-on-Demand service from
Applied Biosystems. These genotyping assays included primers to amplify the region
containing the SNP of interest and two TaqMan Minor Groove Binder probes that are
specific to the polymorphic variant alleles at the site labeled with different fluorescent
39
reporter dyes, FAM and VIC. All reactions were performed using standard conditions
supplied by Applied Biosystems. Following thermocycling, fluorescence levels of the
FAM and VIC dyes were measured and genotypes were scored using the Sequence
Detection Systems 2.2 software (Applied Biosystems). Genotypes were uploaded into a
Progeny database (Progeny Software, LLC, South Bend, IN, USA) containing the
phenotypic data for subsequent statistical analysis.
Using the following equation (Nyholt 2006), we determined that there was a
>99% power to accurately differentiate between monozygotic (MZ) and dizygotic (DZ)
twin pairs using >10 markers with minor allele frequencies between 0.2 and 0.5.
𝑀(𝐷𝑍) =
1
1
1
𝑃𝑟𝑜𝑏(𝑧0 ) + 𝑃𝑟𝑜𝑏(𝑧1 ) + 𝑃𝑟𝑜𝑏(𝑧2 )
2
4
4
1
1
1
= 4 𝑀0 + 2 𝑎2 + 4
1
1
1
= 4 ∑𝑛𝑖=1(𝑝𝑖 )4 + ∑𝑛𝑖=1 ∑𝑛𝑗=𝑖+1(2𝑝𝑖 𝑝𝑗 )2 + 2 ∑𝑛𝑖=1(𝑝𝑖 )2 + 4
Of the 243 pairs, we identified 109 as DZ (r2 = 0.4-0.8) and 107 as MZ (r2>90%).
All discordant sex twin pairs (N=165) were considered DZ. We excluded 27 pairs
because of one or both twins having low genotyping efficiency that is <10 markers
(N=18) or questionable zygosity that is r2<0.4 (N=5) or r2=0.81-0.9 (N=4). The utility of
DNA extracted from DBS cards is challenging because of the very low DNA yield
resulting from these small punches as starting material. This lower quality and quantity of
DNA is most probably contributing to the low genotyping efficiency that we observed for
some of the samples.
Statistical Analysis
Demographic characteristics were compared between DZ and MZ twin pairs. Chi
square tests were used to compare categorical variables (gender, total parenteral nutrition,
and abnormal screen) and Wilcoxon Rank sum tests were used to compare continuous
traits (gestational age, weight, and age at screening). Heritability was estimated with
40
multilevel mixed-effects linear regression adjusting for confounders known to influence
analyte measurements including gender, age at time of sample collection, gestational age
and birth weight. P-values from the additive genetic component are presented.
Heritability was estimated from the division of the beta coefficient of the additive
component over the sum of the additive, shared environment and residual coefficients.
Measurements outside the lower limits of detection (LOD) were given a value of LOD.
17-OHP, TSH and GALT had 10.9%, 5.6% and 0.1% of values, respectively, that were
outside the LOD. GALT also had 59 (7.7%) measurements that were outside the upper
limits of detection; these values were assigned as the upper limits. One amino acid (ASA)
and eight acylcarnitines (C5:1, C6-DC, C14:2, C14-OH, C16:1-OH, C16-OH, C18-OH
and C18:1-OH) had little to no variability (standard deviation ≤ 0.01) and, therefore, were
excluded from heritability analysis. Succinylacetone was also excluded as >20% of the
measurements were missing. For each analyte, outliers were excluded if values were
outside of the mean±4 standard deviations. Equal numbers of DZ and MZ twin pairs were
excluded for deviations ±4 standard deviations from the mean (P=0.58). The outliers may
be due to neonatal illness that we could not account for since we did not have access to
medical records. With the exception of C3, which had no outliers, 1-7 twin pairs (0.3%1.8%) were excluded for all other analytes. To normalize measurement distributions each
analyte was transformed with the natural logarithm. Of the 37 analytes examined, 21
were normally distributed (P>0.01) after transformation; however MET and C18:1
required additional removal of 15 and 5 twin pair outliers respectively and results from
these analytes should be interpreted accordingly. For ARG, LEU, PHE, VAL, C5, C10:1,
C12:1, C14:1, C16:1, TSH and 17-OHP normal distribution was attained for the residuals
from linear regression adjusting for relevant covariates including age at time of
collection, birth weight, gestational age and gender. The residuals were used in
heritability analyses for these analytes. TSH, PHE and C10:1 required additional removal
of 36, 13 and 1 twin pair outliers respectively and results from these analytes should be
41
interpreted accordingly. GALT, C12 and C5-DC were analyzed with the natural log
transformed measurement and IRT and C10 were analyzed with the residuals; however,
all deviated from normality (p<0.01). Additionally we ran heritability measurements on
natural log transformed analyte measurements excluding twin pairs <34 weeks gestation,
with one or both twins having received an abnormal screen, with one or both twins on
total parenteral nutrition and MZ twin pairs where the birth weight was >20% discordant.
This was an attempt to control for infants with medical complications that could interfere
with analyte measurements. As this was a population-based de-identified retrospective
examination of data we were not able to connect our measurements to medical record
information to obtain more detailed information on the severity or type of illness. Results
were similar (Tables 2-3 and 2-4); therefore, the full model including all available twin
pairs are presented in the results and discussion below.
Analysis of Ratios
There were eight amino acid ratios and 13 acylcarnitine ratios included in the
measurements reported with the newborn screen (Table 2-1). We estimated heritability
for these ratios as described above for the single analytes. C4/C2, C5/C2, C5-DC/C16
and C16-OH/C16 were excluded due to low variability (standard deviation ≤ 0.01).
Outliers were excluded if values were outside of the mean±4 standard deviations; 1-7
twin pairs (0.3%-1.8%) were excluded for all ratios. Equal numbers of DZ and MZ twin
pairs were excluded for deviations ±4 standard deviations from the mean (P=0.54). To
normalize measurement distributions each ratio was transformed with the natural
logarithm. Of the 17 analytes examined, 8 were normally distributed (P>0.01) after
transformation; however ASP/HOMOCIT and LEU/PHE required additional removal of
5 and 2 twin pair outliers and results from these analytes should be interpreted
accordingly. For C14:1/C12:1, CIT/ARG, TYR/PHE normal distribution was attained for
the residuals from linear regression adjusting for relevant covariates including age at time
42
of collection, birth weight, gestational age and gender. The residuals were used in
heritability analyses for these analytes. CIT/ARG required additional removal of 4 twin
pair outliers respectively and results from these analytes should be interpreted
accordingly. C4/C3 was analyzed with the natural log transformed measurement, C8/C10
was analyzed with the residuals, C5-DC/C8 was analyzed with the natural log
transformed measurement after removal of 5 twin pairs and MET/PHE was analyzed with
the residuals after removal of 2 twin pairs; however, all still deviated from normality
(p<0.01) and should be interpreted with caution.
Results
Heritability analyses were performed on a total of 381 twin pairs (274 DZ and 107
MZ) (Table 2-5). The DZ and MZ twin pairs were not statistically different from each
other when comparing their mean gestational age, total parenteral nutrition, abnormal
newborn screening result, weight, and age at screening (Table 2-5). The gender of the
two groups differed marginally between DZ and MZ twin pairs (P=0.06), with slightly
more female MZ twin pairs compared to DZ (Table 2-5).
Heritability measurements were significant after correction for multiple testing
(p<0.001) for 10 analytes (Figure 2-1A, Table 2-3). C4-DC of the short chain
acylcarnitines had the highest heritability (h2=0.83, P<10-16). Other short chain
acylcarnitines with high heritability included C2 (h2=0.50, P=7x10-9), C3 (h2=0.44,
P=2x10-6), C4 (h2=0.66, P=2x10-16),C4-OH (h2=0.31, P=4x10-5), and C5 (h2=0.61,
P=1x10-9). Free carnitine C0 also had a significant heritability of (h2=0.45, P=4x10-9).
The environmental component was significant (p<0.001) for all analytes except C4-DC
and C5. However, in most cases where shared environment was also significant, the
proportion of variability explained by the genetic component exceeded the proportion
explained by shared environment. TSH (h2=0.58, P=2x10-5) and IRT (h2=0.52, P=3x10-9)
also had a significant heritability measurement after correction for multiple testing. The
43
shared environment was significant for IRT (P=5x10-4) but not TSH (P=0.29). The
heritability of 17-OHP (h2=0.31, P=1x10-3) was marginally significant with strong shared
environment (P=7x10-7). The only amino acid significant after correction for multiple
testing was glutamate (h2=0.35, P=5x10-4), the shared environment was also significant
(P=1.0x10-5). There was a strong genetic component for the ratios PHE/TYR (h2=0.51,
P=6.4x10-6), TYR/PHE (h2=0.59, P=6.6x10-7), C3/C2 (h2=0.64, P=8.7x10-13), C4/C3
(h2=0.61, P=2.9x10-12) and C5/C3 (h2=0.40, P=4.2x10-6) (Figure 2-1B, Table 2-6).
Of special interest, are the results of the environment and genetic contribution to
metabolites in the β oxidation pathway (Figure 2-2A). We observe a stronger
environmental component for the variation in the long-chain and medium-chain
acylcarnitine measurements. Whereas for short-chain acylcarnitines the environmental
contribution decreases as the genetic contribution increases. We also observed the same
trend of decreasing environmental and increasing genetic contribution for the pathway
that represents the catabolism of the branched-chain amino acids (valine and total
leucine) into C3-DC and C4-DC (Figure 2-2B).
Discussion
High-throughput technologies that integrate genomics and metabolomics are
advantageous for providing insight into the pathophysiology and genetics of complex
human diseases (Goonewardena et al. 2010). Hence, it is important to recognize the
heritability of a particular metabolic measurement before investing in intensive genetic
characterization. To our knowledge, this is the first evaluation of the heritability of a
large panel of enzyme, acylcarnitine, and amino acid biomarkers in the neonatal period,
in addition to being first to use newborn blood spot cards to estimate the genetic
heritability. Our findings of high heritability for the acylcarnitines C2, C3, C4-OH and
C5 as well as the amino acid glutamate were consistent with a previous report examining
the heritability of metabolites in adults with a family history of premature cardiovascular
44
disease (Shah et al. 2009). These similarities are noteworthy not only because so few
studies report heritability estimates for acylcarnitines, but also because there is recent and
compelling evidence for the importance of acylcarnitines as biomarkers for
cardiovascular disease, obesity, and type 2 diabetes in adulthood (Mihalik et al. 2010;
Shah et al. 2010).
Interestingly, our highest heritability was found with C4-DC which in addition to
being elevated in diabetics, was also associated with poor glycemic control, implicating
this metabolite as a strong biomarker for gluco- and lipotoxicity in type 2 diabetes
(Mihalik et al. 2010). Furthermore, the same three metabolite classes (that is short-chain
acylcarnitines, C4-DC, C4-OH) were reported to be significantly associated with adverse
outcomes after coronary artery bypass grafting (Shah et al. 2012). Hence, these
metabolites can be used as biomarkers of risk to predict performance after coronary
artery bypass grafting (Shah et al. 2012). Our study suggests that the levels of potentially
important biomarkers of adult diseases are heritable at birth. Therefore, identifying
genetic variants associated with these metabolites at birth may provide important
screening tools to identify diseases developed later in life.
Also noteworthy is the significant finding of TSH heritability in neonates. TSH is
one of the two analytes used in newborn screening to detect primary congenital
hypothyroidism (CH) (Wilcken and Wiley 2008). As a major player in thyroid function,
TSH has great influence on both neonatal as well as adult normal physiology, affecting
almost all tissues and maintaining healthy status of all human systems including
cognition, cardiovascular, skeletal, and metabolic function (Panicker 2011). Our finding
of significant heritability for TSH in newborn twins (h2=0.58, P=2x10-5) agrees with
previous reports of TSH heritability estimates in adult serum measurements, ranging from
0.32 (Samollow et al. 2004) to 0.64 (Hansen et al. 2004) to 0.65 (Panicker et al. 2008) in
different studies. This finding of high TSH heritability, both in neonates as well as adults,
45
suggests that thyroid function is mainly controlled by genes throughout life, and hence,
neonatal screening results of TSH might help predict adult thyroid diseases later in life.
We also find relevance in these results with respect to neonatal metabolic
screening programs. The State of Iowa Neonatal Metabolic Screening Program is one of
the few that uses the C3/C2 ratio, for which we found strong heritability (h2=0.64,
P=8.7x10-13), to screen for methylmalonic and propionic acidemias. We have identified
patients with confirmed metabolic disorders based on elevated C3/C2 ratios in the
presence of C3 below the threshold defined by the newborn screening program. This is
consistent with the observation that the C3/C2 ratio has a strong genetic component with
little environmental input. This suggests that the C3/C2 ratio may be a useful primary
screening marker for methylmalonic and propionic acidemias as it is primarily defined by
genetic influence.
We are aware of the limitations in our study. Some of the studied metabolites had
large confidence intervals; that may be due to our modest sample size. Furthermore, we
were not able to connect our measurements to medical record information to obtain more
detailed information on neonatal illness, we attempted to control for this by estimating
the heritability excluding twin pairs <34 weeks gestation and twin pairs where one or
both twins were on total parenteral nutrition and observed little difference compared to
the model where all twin pairs were included (Table 2-3 and Table 2-4). Another
limitation to our study was that we had no information on self-identified ancestry.
However, in 2009 86.9% of the births in Iowa were Caucasian. However, it would be
interesting for future studies to replicate these results in other races and age groups. We
identified high heritability for TSH, and short-chain acylcarnitines all of which are
important biomarkers of adult diseases. Our study illustrates the utility of having IRB
reviewed access to stored, de-identified newborn dried bloodspot samples as these results
will guide further studies addressing the predictive ability of metabolic biomarkers in
46
common complex adult diseases as well as characterizing the genes underlying these
observed heritabilities.
47
Table 2-1 List of analytes examined.
17-Hydroxyprogesterone (17OHP-ng/mL)
Acylcarnitines (cont)
Galactose-1-Phosphate Uridyl Transferase (GALT-U/gHb)
Tetradecenoylcarnitine (C14:1)
Trypsinogen I Free (IRT-umol/L)
Tetradecadienoylcarnitine (C14:2)
Thyroid Stimulating Hormone (TSH-mIU/L)
3-Hydroxytetradecanoylcarnitine (C14-OH)
Acylcarnitines (umol/L)
Palmitoylcarnitine (C16)
Carnitine free (C0)
Palmitoleylcarnitine (C16:1)
Acetylcarnitine (C2)
3-Hydroxypalmitoleylcarnitine (C16:1-OH)
Propionylcarnitine (C3)
3-Hydroxypalmitoylcarnitine (C16-OH)
Malonylcarnitine (C3-DC)
Stearoylcarnitine (C18)
Butyrylcarnitine+Isobutyrylcarnitine (C4)
Oleoylcarnitine (C18:1)
Methylmalonylcarnitine (C4-DC)
3-Hydroxyoleoylcarnitine (C18:1-OH)
3-Hydroxybutyrylcarnitine (C4-OH)
Linoleoylcarnitine (C18:2)
Isovalerylcarnitine+Methylbutyrylcarnitine (C5)
3-Hydroxystearoylcarnitine (C18-OH)
Tiglylcarnitine (C5:1)
Amino Acids (umol/L)
Glutarylcarnitine (C5-DC)
Alanine (ALA)
3-Hydroxyisovalerylcarnitine (C5-OH)
Arginine (ARG)
Hexanoylcarnitine (C6)
Argininosuccinate (ASA)
Methylglutarylcarnitine (C6-DC)
Citrulline (CIT)
Octanoylcarnitine (C8)
Glutamate (GLU)
Octenoylcarnitine (C8:1)
Leucine (LEU)
Decanoylcarnitine (C10)
Methionine (MET)
Decenoylcarnitine (C10:1)
Phenylalanine (PHE)
Dodecanoylcarnitine (C12)
Succinylacetone (SUAC)
Dodecenoylcarnitine (C12:1)
Tyrosine (TYR)
Tetradecanoylcarnitine (C14)
Valine (VAL)
48
Table 2-2 List of markers used for zygosity testing and population allele frequencies.
Chromosome
Marker
Position
CEU
CHB
JPT
YRI
1
rs581886
57539683
0.424 C
0.458 A
0.419 C
0.314 A
3
rs427832
149949053
0.491 G
0.226 G
0.273 G
0.372 A
4
rs3804099
154844106
0.45 C
0.339 C
0.267 C
0.372 T
4
rs8752
175649052
0.424 C
0.315 T
0.366 T
0.263 T
5
rs33383
142690179
0.481 T
0.247 C
0.2 C
0.41 C
5
rs4869315
96255028
0.455 A
0.494 A
0.372 A
0.451 G
6
rs2734335
32001923
0.487 G
0.387 G
0.151 G
0.496 G
8
rs2446432
67280862
0.492 A
0.378 C
0.375 C
0.333 C
8
rs4360312
4785152
0.46 T
0.217 C
0.198 C
0.265 T
10
rs2256588
81674775
0.483 A
0.5 G
0.467 A
0.2 G
10
rs4751996
118387884
0.431 A
0.284 G
0.256 G
0.44 A
11
rs1055574
17472409
0.482 G
0.274 G
0.291 G
0.389 G
12
rs2139573
101302904
0.474 C
0.267 C
0.295 C
0.3 C
17
rs2239907
23749871
0.46 T
0.271 T
0.221 T
0.451 C
17
rs4968779
58886303
0.5 G
0.125 G
0.25 G
0.217 A
19
rs1529729
11024562
0.473 C
0.256 C
0.174 C
0.279 C
21
rs6518251
45841556
0.487 T
0.476 T
0.448 T
0.363 T
22
rs738992
31540005
0.496 T
0.44 C
0.446 C
0.317 T
22
rs84460
35855677
0.335 G
0.363 G
0.372 G
0.442 G
X
rs2070584
47331463
0.473 T
0.458 G
0.43 G
0.424 G
Table 2-3 Heritability estimates for all twin pairs.
Enzyme
h2 (95% CI)
Genetic
Coefficient
Genetic Pvalue
Environment
Coefficient
Environment Pvalue
Standard
h2
GALT
0.07 (2.0x10-3-0.77)
3.5x10-3
0.57
0.02
7.4x10-7
0.30
IRT
0.52 (0.35-0.68)
0.11
3.0x10-9
0.07
5.0x10-4
0.47
-3
0.20
-7
7.0x10
0.19
0.03
0.29
0.37
17-OHP
0.31 (0.16-0.51)
0.13
1.2x10
TSH
0.58 (0.32-0.80)
0.13
1.7x10-5
-3
-8
0.11
ALA
0.06 (1.1x10 -0.81)
0.01
0.61
0.05
2.4x10
ARG
0.22 (0.07-0.49)
0.07
0.05
0.15
1.9x10-7
0.10
-6
0.40
0.29
CIT
0.23 (0.08-0.51)
0.02
0.04
0.03
8.2x10
GLU
0.35 (0.18-0.56)
0.02
5.2x10-4
0.02
1.0x10-5
LEU
-20
4.9x10
-16
MET
0.21 (0.05-0.54)
PHE
3.2x10
-20
TYR
0.36 (0.16-0.63)
-22
-18
(8.6x10 -2.8 x10 )
-22
-18
(9.4x10 -1.1x10 )
-8
-21
3.7x10
1.00
0.05
<1x10
0.02
0.10
0.05
2.6x10-5
-21
-15
1.3x10
1.00
0.02
8.7x10
0.06
5.5x10-3
0.05
4.5x10-3
-3
-14
-0.07
0.08
0.12
0.38
2.4x10-4
VAL
0.02 (7.8x10 -1.0)
1.3x10
0.87
0.06
2.4x10
C0
0.45 (0.31-0.60)
0.05
3.8x10-9
0.04
1.0x10-6
0.64
-9
0.04
-4
1.8x10
0.68
0.05
4.3x10-5
0.38
C2
0.50 (0.33-0.67)
0.05
6.6x10
C3
0.44 (0.27-0.61)
0.06
1.7x10-6
-10
0.13 (0.02-0.47)
0.02
0.21
0.09
2.6x10
C4
0.66 (0.49-0.80)
0.10
2.2x10-16
0.03
8.7x10-3
2.3x10-3
0.66
49
C3DC
Table 2-3 Continued
C4DC
C4OH
C5
C5DC
C5OH
C6
C8
C8:1
C10
C10:1
C12
C12:1
C14
C14:1
C16
0.83 (0.58-0.95)
0.31 (0.18-0.48)
0.61 (0.41-0.78)
0.03 (1.4x10 -1.0)
-21
6.0x10
-13
-12
-8
-22
-19
(1.3x10 -1.4x10 )
(7.9x10 -1.3x10 )
(1.4x10 -2.5x10 )
0.04 (4.4 x10 -0.83)
2.6x10
-14
-12
(1.3x10 -5.3x10 )
0.31 (0.14-0.56)
0.14 (0.03-0.49)
0.27 (0.11-0.52)
1.1x10
1.4x10
0.02
0.03
0.24
4.0x10
-3
0.02
-16
-4
-13
0.10
-9
3.6x10
0.15 (0.04-0.44)
3.2x10
3.6x10
0.02
-6
-10
0.06
-5
0.02
0.20 (0.10-0.37)
4.2x10
<1x10-16
0.07
0.09 (0.02-0.39)
-15
0.08
6.5x10
8.4x10
-11
8.7x10
-22
8.8x10
-3
9.9x10
-14
0.03
0.03
0.03
0.17
-3
0.84
0.09
1.00
0.11
1.00
0.17
1.00
0.09
0.66
0.13
1.00
6.6x10
0.06
0.07
0.13
-16
7.9x10-3
0.26
-3
0.20
0.04
0.11
0.01
0.04
0.39
0.70
-9
0.32
0.42
-16
0.06
5.6x10
-15
0.27
5.4x10
-8
-0.15
3.1x10
-11
-0.03
<1x10
-16
-0.10
<1x10
-16
-0.11
<1x10
-16
-0.28
-13
-0.10
-16
-0.08
1.0x10
-4
0.16
1.3x10
-8
-0.01
1.2x10
-5
0.24
-10
-1.0x10-3
<1x10
5.0x10
<1x10
C16:1
0.10 (0.01-0.51)
0.02
0.31
0.09
2.0x10
C18
0.31 (0.14-0.55)
0.03
5.1x10-3
0.04
5.2x10-5
0.39
0.03
-3
0.02
0.04
0.33
C18:1
C18:2
0.43 (0.21-0.68)
0.10 (0.01-0.51)
0.02
1.0x10
0.32
0.13
2.7x10
-11
0.19
50
The genetic coefficient and P-value represent the additive genetic component and the environment coefficient and P-value represent
the shared environment component. Standard heritability was also calculated with the log transformed measurement and no covariate
adjustment using 2*(rMZ-rDZ) where r is the standard correlation coefficient for MZ and DZ twins.
51
Table 2-4 Heritability estimates for twin pairs excluding TPN, abnormal screens,
gestational age <34 weeks, and MZ twin pairs that are >20% discrepant in weight.
Enzyme
h2 (95% CI)
Genetic
Coefficient
Genetic
P-value
Environment
Coefficient
Environment
P-value
GALT
2.8x10-13 (4.6x10-13-1.7x10-11)
1.52x10-14
1.00
0.03
<1x10-16
IRT
0.63 (0.41-0.8)
0.14
2.2x10-9
0.05
0.03
-6
0.11
2.7x10-5
OHP
0.43 (0.27-0.61)
0.12
1.6x10
TSH
0.5 (0.25-0.75)
0.11
4.4x10-4
0.05
0.09
0.36
0.04
3.8x10-6
-3
ALA
0.13 (0.01-0.63)
9.7x10
ARG
0.36 (0.18-0.59)
0.09
1.1x10-3
0.10
6.3x10-5
CIT
0.41 (0.19-0.67)
0.03
1.7x10-3
0.02
7.3x10-3
GLU
0.35 (0.16-0.6)
0.02
3.1x10-3
0.02
1.9x10-4
LEU
0.13 (0.01-0.68)
6.9x10-3
0.39
0.02
7.0x10-5
MET
0.28 (0.09-0.62)
0.02
0.05
0.03
1.9x10-3
PHE
0.14 (6.6x10-3-0.81)
5.3x10-3
0.48
0.01
0.02
TYR
0.47 (0.24-0.72)
0.07
5.3x10-4
0.04
0.04
VAL
0.26 (0.09-0.56)
0.02
0.04
0.03
4.3x10-5
C0
0.51 (0.35-0.66)
0.06
5.7x10-11
0.04
2.8x10-5
C2
0.52 (0.34-0.7)
0.06
2.4x10-8
0.04
1.1x10-3
C3
0.57 (0.37-0.75)
0.07
1.9x10-8
0.04
7.4x10-3
C3DC
0.18 (0.06-0.42)
0.03
0.04
0.10
1.5x10-10
C4
0.65 (0.45-0.81)
0.11
3.5x10-12
-16
0.04
0.01
-3
C4DC
0.87 (0.5-0.98)
0.09
6.7x10
C4OH
0.4 (0.25-0.56)
0.08
7.0x10-7
0.09
8.8x10-7
C5
0.69 (0.43-0.87)
0.07
1.4x10-8
0.01
0.29
C5DC
0.23 (0.12-0.38)
0.06
5.7x10-4
0.17
5.3x10-13
C5OH
0.28 (0.14-0.46)
0.03
8.6x10-4
0.06
4.3x10-9
C6
0.22 (0.05-0.63)
0.03
0.16
0.05
3.8x10-4
C8
0.34 (0.19-0.53)
0.06
9.2x10-5
0.09
1.3x10-7
C8:1
0.24 (0.14-0.38)
0.03
8.0x10-5
0.09
1.7x10-13
C10
0.34 (0.2-0.52)
0.09
6.9x10-5
0.14
1.2x10-7
C10:1
0.25 (0.12-0.45)
0.03
4.0x10-3
0.08
6.3x10-10
C12
0.22 (0.08-0.5)
0.04
0.04
0.10
3.4x10-7
5.1x10
0.65
52
Table 2-4 Continued
C12:1
0.26 (0.13-0.44)
0.12
1.1x10-3
0.26
5.6x10-10
C14
0.42 (0.2-0.67)
0.05
1.4x10-3
0.03
7.2x10-3
C14:1
0.35 (0.19-0.56)
0.08
4.5x10-4
0.10
6.5x10-6
C16
0.37 (0.18-0.62)
0.04
2.2x10-3
0.04
9.5x10-4
C16:1
0.23 (0.09-0.48)
0.04
0.02
0.08
1.1x10-7
C18
0.42 (0.21-0.67)
0.05
6.6x10-4
0.03
4.8x10-3
C18:1
0.39 (0.17-0.68)
0.03
5.8x10-3
0.03
0.02
C18:2
0.28 (0.12-0.54)
0.05
0.01
0.09
4.0x10-6
The genetic coefficient and P-value represent the additive genetic component and the
environment coefficient and P-value represent the shared environment component.
53
Table 2-5 Demographic characteristics of twin pairs.
DZ (n=274)
MZ (n=107)
Gender of Twin Pair
Pvalue
0.06*
Female-Female
45 (16.4%)
58 (54.2%)
Male-Female
165 (60.2%)
0 (0%)
Male-Male
64 (23.4%)
49 (45.8%)
Gestational Age of Twin Pair/weeks
35.6 (2.5)
35.7 (2.3)
1.00
TPN (one or both twins)
29 (10.6%)
9 (8.4%)
0.53
Abnormal screen (one or both twins)
42 (15.3%)
19 (17.8%)
0.56
Weight/grams (averaged for each twin pair)
2 397.9 (496.9)
2 364.7 (465.8)
0.19
Age at screening/hours (averaged for each twin
pair)
35.2 (11.8)
35.2 (13.0)
0.55
TPN, total parenteral nutrition.
*P-value determined comparing only Male-Male and Female-Female twin pairs.
Table 2-6 Heritability estimates for analyte ratios.
Enzyme
h2 (95% CI)
Genetic
Coefficient
Genetic
value
ARG/ORN
0.34(0.2-0.52)
0.06
ASP/HOMOCIT
0.33(0.13-0.62)
CIT/ARG
P-
Environment
Coefficient
Environment
P-value
6.1x10-5
0.08
3.4x10-8
0.03
0.01
0.03
3.8x10-3
0.17(0.04-0.47)
0.04
0.12
0.13
1.3x10-8
LEU/ALA
2.7x10-13(6.5x10-15-1.1x10-11)
1.4x10-14
1.00
0.03
0.00
LEU/PHE
0.17(0.04-0.46)
5.5x10-3
0.11
0.02
2.8x10-9
MET/PHE
0.04(1.8x10-5-0.99)
2.2x10-3
0.79
0.03
2.9x10-7
PHE/TYR
0.51(0.3-0.72)
0.09
6.4x10-6
0.04
0.03
-7
0.02
0.16
TYR/PHE
0.59(0.36-0.79)
0.10
6.6x10
C0/C16
0.14(0.03-0.43)
0.01
0.15
0.05
2.0x10-11
C0/C18
0.21(0.06-0.5)
0.02
0.07
0.04
9.5x10-7
C3/C2
0.64(0.45-0.79)
0.07
8.7x10-13
0.02
0.02
-12
0.04
6.5x10-3
C4/C3
0.61(0.43-0.76)
0.09
2.9x10
C5/C3
0.4(0.24-0.57)
0.05
4.2x10-6
0.05
4.1x10-6
C5DC/C8
0.11(0.03-0.35)
0.01
0.14
0.08
0.00
C8/C10
0.14(0.02-0.58)
6.8x10-3
0.29
0.02
1.3x10-5
C14:1/C12:1
0.06(1.0x10-3-0.77)
5.5x10-3
0.61
0.06
2.9x10-11
C14:1/C16
0.38(0.2-0.59)
0.05
3.8x10-4
0.05
1.1x10-4
54
The genetic coefficient and P-value represent the additive genetic component and the environment coefficient and P-value represent
the shared environment component.
55
Figure 2-1 Heritability of analyzed metabolites and analyte ratios. (a) Heritability of
analyzed metabolites. The y-axis is the negative log10 of the P-value for additive genetic
component and the heritability estimate is on the x-axis. Confidence intervals around the
heritability point estimates are in light gray bars. IRT, TSH, 17-OHP and GALT are
represented as dark gray squares, amino acids are represented as medium gray circles and
acylcarnitines are represented as light gray triangles. (b) Heritability of analyte ratios.
The y-axis is the negative log10 of the P-value for additive genetic component and the
heritability estimate is on the x-axis. Confidence intervals around the heritability point
estimates are in light gray bars.
56
Figure 2-2 Environment and genetic contribution to metabolites in the β-oxidation
pathway and the pathway for catabolism of branched-chain amino acids. (a) Environment
and genetic contribution to metabolites in the β-oxidation pathway. The x-axis is a list of
the even-chain acylcarnitines, the y-axis is the negative log10 of the P-value for the
correlation coefficients. The dotted line represents the genetic component and the solid
line represents the environmental component. (b) Environment and genetic contribution
to metabolites along the pathway that represents the catabolism of the branched-chain
amino acids (valine and total leucine) into C3-DC and C4-DC. The x-axis is a list of the
metabolites, the y-axis is the negative log10 of the P-value for the correlation
coefficients. The dotted line represents the genetic component and the solid line
represents the environmental component.
57
CHAPTER 3
GENETIC ASSOCIATIONS WITH NEONATAL THYROID
STIMULATING HORMONE LEVELS
The following manuscript was published online on February 27, 2013 in Pediatric
Research. Additional authors include Oleg Shchelochkov, Stanton Berberich, Jeffrey
Murray, and Kelli Ryckman.
Thyroid stimulating hormone (TSH) is known to be largely controlled by genetic
factors. In the previous chapter, we presented that TSH heritability in neonates was 58%.
Genetic factors playing a role in regulating TSH levels have been extensively studied in
adults through genome-wide association and candidate-gene studies. However, the
genetic factors involved in neonatal TSH variability have never been studied. In this
study, we identified for the first time two genetic associations with neonatal TSH levels
that replicate findings with adult TSH levels. This finding may have clinical implications
for the early prediction of risk for adult diseases and conditions associated with thyroid
hormone levels.
Dr. Oleg Shchelochkov provided valuable insight into TSH use as a marker for
congenital hypothyroidism and was involved in editing the manuscript. Dr. Stanton
Berberich provided insight on the study design and study samples and data. Drs. Jeffrey
Murray and Kelli Ryckman provided oversight for all aspects of the project, provided
input into study design and assisted in the writing and editing of the manuscript. Dr. Kelli
Ryckman also performed the statistical analyses. I reviewed the literature and selected all
study markers. I performed part of the DNA extraction and trained Dr. Osayame
Ekhaguere, Lauren Fleener, and Daniel Cook to complete additional DNA extraction
from newborn blood spot cards. I optimized a new protocol for Fluidigm genotyping that
had not been used in our lab before and performed all the genotyping presented in this
58
study. I performed bioinformatic analyses and assisted in statistical analyses. I also wrote
the manuscript, revisions, and responses to reviewer critiques.
Abstract
Background: Elevations or deficits in thyroid hormone levels are responsible for a
wide range of neonatal and adult phenotypes. Several genome-wide, candidate-gene and
meta-analysis studies have examined thyroid hormones in adults; however, to our
knowledge no genetic association studies have been performed with neonatal thyroid
levels. Methods: A population of Iowa neonates; term (n=827) and preterm (n=815),
were genotyped for 45 single nucleotide polymorphisms. Thyroid stimulating hormone
(TSH) values were obtained from the Iowa Neonatal Metabolic Screening Program.
Analysis of variance was performed to identify genetic associations with TSH
concentrations. Results: The strongest association was rs4704397 in the PDE8B gene
(p=1.3x10-4), followed by rs965513 (p=6.4x10-4) on chromosome 9 upstream of the
FOXE1 gene. Both of these SNPs met statistical significance after correction for multiple
testing. Six other SNPs were marginally significant (p<0.05). Conclusions: We
demonstrated for the first time two genetic associations with neonatal TSH levels that
replicate findings with adult TSH levels. These SNPs should be considered as early
predictors of risk for adult diseases and conditions associated with thyroid hormone
levels. Furthermore, this provides a better understanding of the thyroid profile and
potential risk for thyroid disorders in newborns.
Introduction
Endocrine disorders are substantial contributors to neonatal morbidity and
mortality and, of these; congenital hypothyroidism (CH) is the most common (Kumar et
al. 2009). CH is a common and preventable cause of mental retardation with an incidence
rate of approximately 1 in 2,350 live births (Hinton et al. 2010). Early treatment with
thyroxine (T4) with subsequent supplementation for life produces excellent results for
59
both growth and development (Wilcken and Wiley 2008; Hinton et al. 2010). CH is
screened for at birth through detection of T4, thyroid stimulating hormone (TSH), or both
(Wilcken and Wiley 2008).
In the preterm infant, thyroid function undergoes postnatal changes related to an
immature hypothalamic-pituitary axis (HPA), along with the interrupted exposure to
maternal thyroid hormone and thyroid releasing hormone from the placenta. Due to
immature HPA function T4 is lower in preterm infants compared to neonates born at
term, and there is a direct correlation between the serum T4 level and the degree of
prematurity (LaFranchi 1999). Preterm neonates with abnormal thyroid function may
have transient hypothyroxinemia of prematurity, and be misreported as true cases of CH
(Hinton et al. 2010). Hence, it is essential to take gestational age and birth weight into
consideration when making the differentiation between transient hypothyroidism and true
cases of CH (Hinton et al. 2010).
Among healthy subjects, TSH shows considerable variability between individuals,
whereas this variability is much less in the same individual when TSH is measured
repeatedly over an extended period of time (Panicker et al. 2010). Previous studies have
observed that TSH variability is under strong genetic regulation; studies have estimated
heritability of up to 65% for variation in adult serum TSH (Panicker et al. 2008). In
addition, there have been several genome-wide association studies (GWAS) reporting
multiple genetic variants associated with TSH levels in adults (Hwang et al. 2007;
Arnaud-Lopez et al. 2008; Panicker et al. 2010; Rawal et al. 2012). Furthermore in
candidate-gene studies the Asp727Glu polymorphism in the TSH receptor gene (TSHR)
is associated with adult serum TSH levels, which further supports a genetic contribution
in assessing the variation of TSH (Hansen et al. 2007). To our knowledge no studies have
examined candidate SNPs with neonatal TSH measurements. We genotyped term and
preterm infants for 45 SNPs in 24 candidate genes that are known to play a role in TSH
production or metabolism and examined these polymorphisms for associations with TSH
60
levels measured at birth as part of the Iowa Neonatal Metabolic Screening Program.
Understanding variation in TSH levels and the genes responsible may be particularly
important in a population at risk for abnormal TSH levels such as preterm infants.
Methods
Study Population
Study samples were obtained from two sources. The first was from the University
of Iowa SHL where we obtained de-identified residual dried blood spots on a population
of Iowa neonates; term (n=827) and preterm (n=413). Approval for use of the deidentified data and blood spot cards was granted by the Iowa Department of Public
Health and a waiver of consent was obtained from the Institutional Review Board at the
University of Iowa (IRB#200908793). All subjects had TSH measurements between day
1 and 3 of life and had not received a transfusion prior to sample collection. Preterm birth
was defined as birth before 37 completed weeks of gestation. Gestational age was
determined from the records obtained from the SHL. Quantification of TSH was
performed at the SHL using CLIA (Clinical Laboratory Improvement Amendments)
certified methods. TSH was determined by solid phase, time-resolved
fluoroimmunoassay from dried newborn blood spots using PerkinElmer’s AutoDELFIA
platform (Waltham, MA). DNA was extracted from one dried whole blood spot for all
term samples and two dried whole blood spots for all preterm samples using the AutoGen
(Holliston, MA) QuickGene-810 nucleic acid extraction machine with the DNA Tissue
Kit (AutoGen) and following manufacturer’s recommendations.
The second source was from the University of Iowa Hospitals and Clinics NICU.
Preterm infants admitted to this NICU were either born in house or transferred from
referring units within the first 28 days of life. Preterm birth was also defined as birth
before 37 completed weeks of gestation. Gestational age was determined from the first
day of the last menstrual period. Gestational age was confirmed through obstetrical
61
judgment and if uncertain, ultrasound measurements were used for confirmation. All
families provided signed informed consent (UI IRB199911068) to be included in a
repository of samples designed to provide DNA and limited epidemiologic data to study
complications of newborn infants (Steffen et al. 2007). Preterm infants from singleton
births, without congenital anomalies, with gestational ages between 22 to 36 weeks
(n=402) were included in this study, and early preterm infants (<34 weeks gestation)
were overrepresented from their population frequency due to the referral patterns of our
NICU. TSH measured by the SHL as part of routine neonatal screening was linked to the
sample and medical record data. DNA was extracted from cord blood, discarded venous
blood or buccal swab for all infants. All DNA was extracted using standard protocols.
Marker Selection and Genotyping
We chose a total of 45 SNPs encompassing 24 candidate genes and eight
intergenic loci. The list of genes and SNPs genotyped are in Table 3-1. SNPs were
chosen either based on their previously reported associations with adult serum TSH
levels, or based on thyroid biology and candidate genes from the literature. In the first
case, we chose the exact SNPs that were reported to be associated. In the second case, we
chose SNPs from the HapMap database (http://hapmap.ncbi.nlm.nih.gov/) based on their
ability to tag the surrounding SNPs in the candidate gene. All SNPs were genotyped
using TaqMan assays (Applied Biosystems, Foster City, CA) on the EP1 SNP
Genotyping System and GT48.48 Dynamic Array Integrated Fluidic Circuits (IFCs)
(Fluidigm, San Francisco, CA). All SNP genotyping assays were available and ordered
using the Assay-on-Demand service from Applied Biosystems. These genotyping assays
included primers to amplify the region containing the SNP of interest and two TaqMan
Minor Groove Binder probes that are specific to the polymorphic variant alleles at the site
labeled with different fluorescent reporter dyes, FAM and VIC. All reactions were
performed using standard conditions supplied by Fluidigm. Following thermocycling,
62
fluorescence levels of the FAM and VIC dyes were measured using the EP1 Reader
(Fluidigm) and genotypes were scored using the Fluidigm Genotyping Analysis software
(Fluidigm). Genotypes were uploaded into a Progeny database (Progeny Software, LLC,
South Bend, IN) containing the phenotypic data for subsequent statistical analysis.
Genotyping efficiency was >98% for all markers with the exception of rs9322817 in
HACE1 (93.5%) and rs1014968 in TSHR (90.8%). Forty-three individuals with
genotyping efficiency <95% (i.e. missing data on >2 markers) were excluded from
further analysis. Additionally, only 16 individuals had an abnormal (TSH≥25.0 mIU/L)
level on initial screen. In order to avoid potential confounding, these individuals were
excluded leaving 404 SHL preterm neonates, 799 term neonates and 380 NICU neonates
for analysis.
Statistical Analysis
Demographic characteristics were compared between cohorts using Chi-square
tests for categorical traits and Wilcoxon rank sum tests for continuous traits. All
demographic factors listed in Table 3-2, year of sampling and TSH assay lot were
individually associated (P≤0.001) with the natural log transformed TSH measurement in
the combined (N=1,583) sample cohort using analysis of variance (ANOVA). Step-wise
modeling was used to determine a final list of covariates for inclusion when testing
association between SNP genotype and TSH level. Gestational age (P=5.55x10-19), age at
time of sampling (P=1.63x10-42), gender (P=1.52x10-8) and year of sampling (P=7.36x104
) were all significantly associated with TSH in the final model; birth weight (P=0.02),
assay lot (P=0.09) and TPN (P=0.25) were not included in the final model due to
marginal significance. Hardy-Weinberg Equilibrium (HWE) was evaluated for each
marker using Fisher exact tests for all cohorts. All markers were tested for association
with the natural log transformed TSH measurement adjusting for gender, gestational age,
age at time of sampling and year of sampling using ANOVA in the combined cohort
63
(N=1,583). A Bonferonni significance threshold of P=0.001 (0.05/45 markers) was used
to correct for multiple testing. Sub-analyses were performed in each cohort separately to
determine individual population effects. All analyses were performed in STATA software
version 12.0 (StataCorp LP, College Station, TX).
Haplotype Analysis
Haplotype analysis of SNPs in the same gene or region was used to evaluate
regional associations with natural log transformed TSH levels. Haplotype analysis was
performed with linear regression adjusted for gender, gestational age, age at time of
sampling and year of sampling in the combined cohort. Haplotype analysis was
performed using sliding windows of 2, 3, and 4 SNPs along a gene or region of interest.
Haplotype analyses were performed in PLINK software
(http://pngu.mgh.harvard.edu/purcell/plink/) (Purcell et al. 2007).
Results
Analysis was performed on a total of 1,583 neonates (404 University of Iowa
State Hygienic Laboratory (SHL) preterm neonates, 799 term neonates, and 380
University of Iowa Hospitals and Clinics Neonatal Intensive Care Unit (NICU) neonates)
(Table 3-2). The three cohorts were not statistically different from each other when
comparing their gender (Table 3-2). Differences between mean TSH level, gestational
age, and birth weight were statistically significant between all three cohorts (Table 3-2).
Difference in mean for age at screening was statistically significant between SHL preterm
and NICU preterm but not between SHL term and SHL preterm cohorts (Table 3-2).
Difference in total parenteral nutrition was statistically significant between SHL term and
SHL preterm but not between SHL preterm and NICU preterm cohorts (Table 3-2).
Association results for all genotyped single nucleotide polymorphisms (SNPs) in
combined populations are shown in Figure 3-1 and Table 3-3. Association results for all
genotyped SNPs in individual populations are shown in Figure 3-2 and Table 3-4.
64
Eight SNPs were nominally significantly associated with neonatal TSH levels in
all study populations combined (p<0.05) (Table 3-5, Table 3-6, and Figure 3-1).The
strongest association was rs4704397 in the PDE8B gene (p=1.3x10-4), followed by
rs965513 (p=6.4x10-4) on chromosome 9 upstream of the FOXE1 gene. Both of these
SNPs met statistical significance after correction for multiple testing (corrected
significance threshold set at p<0.001). While none of the associations in the individual
populations met the significance threshold after correction for multiple testing, the
strongest associations remained rs4704397 in the PDE8B and rs965513 near FOXE1
(Figure 3-2). Each copy of the minor A allele for rs4704397 in PDE8B was associated
with an increase in TSH levels in both term and preterm infants (Table 3-5), as well as an
increase of 0.6 mIU/L in TSH levels in the combined cohort. For SNP rs965513 in
FOXE1 each copy of the minor A allele was associated with a decrease in TSH levels in
both term and preterm infants (Table 3-5), as well as a decrease of 0.2-0.7 mIU/L in TSH
levels in the combined cohort. Two other SNPs in FOXE1 (rs1443432 and rs3021523)
showed marginal (p<0.05) significance with TSH levels. Each copy of the G allele of
rs1443432 and each copy of the C allele of rs3021523 were associated with a decrease in
TSH levels in both term and preterm infants (Table 3-5), as well as a decrease of 0.2-0.5
and 0.2-0.6 mIU/L in TSH levels in the combined cohort respectively. Haplotype analysis
revealed significant associations of specific allele combinations with TSH levels. Near
the FOXE1 gene, the presence of the AT and GT haplotypes at rs965513 and rs1443433
was significantly associated with either a decrease or increase of TSH levels, respectively
(p=4.2x10-4 and p=4.6x10-4) (Table 3-7).
The four remaining SNPs were marginally significant with TSH levels; rs9308765
on chromosome 2 (p=0.01), rs657152 in the ABO gene (p=0.02), rs4892386 in the
SLC16A2 gene (p=0.01), and rs1527680 in the PPP1R9A gene (p=0.04). However, the
association between these SNPs and TSH levels were not always in the same direction in
the three studied cohorts, and further investigation is needed to confirm the associations
65
(Table 3-6). While there were no significant single locus associations with TSH levels in
TSHR in any of the cohorts the presence of the AGT haplotype at rs10149689,
rs4903957, and rs11159483, the GTT haplotype at rs4903957, rs11159483, and
rs2075179, the AGTT haplotype at rs10149689, rs4903957, rs11159483, and rs2075179,
and the GTTA haplotype at rs4903957, rs11159483, rs2075179, and rs12885526 were
significantly associated with TSH levels (p=7.9x10-4, p=6.2x10-4, p=4.2x10-5, and
p=7.8x10-4 respectively) (Table 3-8).
Discussion
Elucidating the genetic basis of TSH variability is currently an area of interest to
further the understanding of adult conditions related to TSH levels. For example, low
serum TSH levels are associated with an increased risk of atrial fibrillation in adults over
60 years old (Sawin et al. 1994). Thyroid hormone levels within the normal physiological
range have also been shown to affect bone mass and density in healthy men aged 25-45
years (Roef et al. 2011), as well as in men and women above 55 years of age (van der
Deure et al. 2008). Thyroid hormones also play a key role in neonatal as well as adult
normal physiology, affecting almost all tissues and maintaining healthy status of all
human systems including cognition, cardiovascular function, skeletal health, and
balanced energy and metabolic status (Panicker 2011). This is particularly relevant in
preterm infants were the variability of TSH is particularly high because of postnatal
changes in thyroid function due to premature interrupted exposure to maternal thyroid
hormones as well as an immature HPA (Hinton et al. 2010). Understanding the shared
genetic associations with TSH levels in both the neonatal period as well as through
adulthood will be useful for earlier prediction of risk to adult diseases that are affected by
TSH levels.
In this light, we aimed to identify genetic polymorphisms that may play a role in
TSH variation, especially, in preterm infants. We observed genetic associations that have
66
an effect on TSH levels in either or both term and preterm infants. However, most of our
nominally significant associations were found in the term population, and these
associations reached multiple testing correction levels of significance in all populations
combined. This may be due to the wide range of variability in TSH levels of preterm
infants due to immature HPA and the skewed nature of our preterm population where
early preterm infants are overrepresented. Our most significant association was with SNP
rs4704397 in PDE8B gene (p=1.3x10-4). Each copy of the minor A allele was associated
with an increase of 0.6 mIU/L in TSH levels in the combined cohort. This finding is
consistent with what has previously been reported in adult serum TSH levels (ArnaudLopez et al. 2008). The PDE8B gene is expressed most abundantly in the thyroid gland
where it has threefold higher levels than in the next highest tissue (Lakics et al. 2010). It
is expressed at lower levels in some other tissues including the brain, spinal cord, and
placenta (Hayashi et al. 1998). The PDE8B gene encodes a high affinity adenosine 3’,5’cyclic monophosphate (cAMP)-specific phosphodiesterase to regulate the level of cAMP
in cells and plays a vital role in signal transduction (Hayashi et al. 1998; Lakics et al.
2010). Common genetic variants in PDE8B may affect steroid hormone physiology, such
as levels of TSH. For example, an intronic SNP in PDE8B (rs4704397) that was
identified in the genome-wide association study by Arnaud-Lopez et al. (2008) associated
with adult serum TSH levels was then reported to be associated with subclinical
hypothyroidism during pregnancy (Shields et al. 2009), as well as with TSH levels in
obese children (Grandone et al. 2012). Interestingly, we found the same SNP to be
associated with TSH levels in both preterm and term infants suggesting that this gene
plays an important role in regulating TSH levels at birth as well as thyroid function
throughout life. All four studies (adult serum TSH level (Arnaud-Lopez et al. 2008),
pregnancy TSH level (Shields et al. 2009), obese children TSH level (Grandone et al.
2012), and this newborn TSH level study) came to the same finding that each copy of the
minor A allele was associated with an increase in TSH levels. In the Arnaud-Lopez et al.
67
paper, the authors suggest that since cAMP is necessary for thyroid-hormone secretion
due to TSH stimulation; when PDE8B catalyzes the hydrolysis and inactivation of cAMP
in the thyroid gland, it results in decreased generation of thyroid-hormone T4 and T3
resulting in the negative feedback loop to act on producing more TSH (Arnaud-Lopez et
al. 2008). Hence, genetic variation in PDE8B may affect PDE8B activity resulting in
altered cAMP, TSH, and probably other downstream effects. In the Arnaud-Lopez et al.
paper, all exons in the PDE8B gene were sequenced in 40 patients to identify a possible
etiologic variant in linkage disequilibrium with the intronic rs4704397; however, no
coding variants were identified (Arnaud-Lopez et al. 2008). Further investigation and
sequencing of this gene will be needed in adult and newborn samples to identify the
regulatory regions causing the association between PDE8B and thyroid levels.
We also found SNPs rs965513 and rs1443432 near the FOXE1 gene (p=6.4x10-4
and 0.02 respectively) and SNP rs3021523 in the FOXE1 gene (p=0.03), to be associated
with TSH levels in all the populations combined. Although, only rs965513 meets
multiple testing correction level of significance while the other two SNPs are only
marginally significant, this may be secondary to the moderate, but not complete, linkage
disequilibrium (LD) with each other (rs965513, rs1443432: D’=0.863, r-squared =0.519;
rs965513, rs3021523: D’=0.835, r-squared=0.48) and where rs965513 and rs1443433
also have strong effects as part of a haplotype associated with TSH levels. FOXE1 gene
encodes a transcription factor that is essential for the initiation of thyroid differentiation
at the embryonic stage (Parlato et al. 2004). Mutations of the FOXE1 gene may result in
thyroid dysgenesis leading to both familial as well as cases of syndromic congenital
hypothyroidism in the Bamforth-Lazarus Syndrome, Online Mendelian Inheritance in
Man (OMIM) #241850 (Online Mendelian Inheritance in Man 2013), a rare inherited
disorder characterized by CH, cleft palate, and spiky hair (Castanet and Polak 2010).
FOXE1 also plays an important role in regulating the transcription of different thyroidspecific genes resulting in regulation of thyroid-hormone synthesis (Gudmundsson et al.
68
2009). Both of two SNPs, rs965513 near FOXE1 (Castanet and Polak 2010) and
rs1443434 in FOXE1 gene (Medici et al. 2011), have been previously shown to be
associated with adult serum TSH levels. Our replication of this finding with newborn
TSH levels further implicates involvement of this locus in determining TSH levels in
newborns; indicating that this association is present at birth.
We further identified four haplotypes in the TSHR gene to be significantly
associated with TSH levels. The protein encoded by the TSHR gene is the TSH receptor
(TSHR). TSHR is present on thyroid cells, and when activated by TSH secreted from the
pituitary gland, intracellular cAMP is upregulated resulting in activation of various
cellular processes ending with an increased production of thyroid hormone (Stathatos
2012). SNPs in the TSHR gene were previously found to be associated with adult serum
TSH levels in a GWAS reported by Arnaud-Lopez et al. (2008). We did not find an
association with single SNPs in the TSHR gene; however we found SNP haplotypes to be
associated with newborn TSH levels.
One limitation of this study is that we were not able to connect TSH
measurements to medical record information to obtain more detailed information on
neonatal illness or race for the SHL preterm and term cohorts. However, in 2009 86.9%
of the births in Iowa were Caucasian, suggesting that the majority of our samples are
from Caucasians. Another limitation was that we do not have follow up data on our study
cohort to check for development of conditions later in life. On the other hand, our study
illustrates the utility of having IRB reviewed access to stored, de-identified newborn
dried bloodspot samples for genetic studies. It is also, to our knowledge, the first study to
examine genetics of TSH levels in newborns. Unraveling the genes that affect TSH levels
will enhance our understanding of the genetic regulation and physiology of the thyroid
and the pituitary-thyroid axis as well as the genes that may be involved in different
thyroid diseases. This knowledge may be used to help individualize thyroid related
treatments according to the individual’s specific genotype. Recognizing TSH variation
69
and the genetic factors affecting it early in infancy may be a useful adjunct in population
screening for the early prediction and possible treatment or prevention of adult diseases
and conditions affected by TSH levels.
70
Table 3-1 List of genotyped markers.
Marker
Gene
Location
Chr.
Position
MAF
rs10917469
-
Intergenic
1
19843576
0.19
rs1321108
TSHB
Promoter
1
115572365
0.5
rs4849179
PAX8
Intron
2
113985170
0.42
rs877202
PAX8
Intron
2
114019129
0.26
rs9308765
-
Intergenic
2
119043209
0.11
rs2288629
EPHA4
Intron
2
222307310
0.16
rs1505287
THRB
Intron
3
24412690
0.37
rs784490
TTC21A
Intron
3
39173530
0.24
rs1976324
-
Intergenic
3
87212806
0.31
rs10493147
HSPA4L
Intron
4
128737499
0.24
rs2545308
-
Intergenic
4
181637915
0.44
rs27178
PDE4D
Intron
5
58587025
0.46
rs4704397
PDE8B
Intron
5
76518442
0.48
rs9342104
CGA
Intron
6
87798512
0.44
rs6942231
HACE1
Intron
6
105191814
0.45
rs9322817
HACE1
Intron
6
105232233
0.4
rs2983521
PDE10A
Intron
6
166057203
0.2
rs10486365
TMEM196
Intron
7
19801364
0.1
rs6977660
TMEM196
Intron
7
19805480
0.14
rs10499559
-
Intergenic
7
22109459
0.16
rs10486653
NPSR1
Intron
7
34711663
0.2
rs1527680
PPP1R9A
Promoter
7
94534886
0.15
rs2252696
SLA
Intron
8
134063532
0.43
rs7865184
ZDHHC21
Intron
9
14687867
0.45
rs10512065
GNAQ
Intron
9
80625644
0.13
rs965513
-
Intergenic
9
100556109
0.37
rs1443433
-
Intergenic
9
100579219
0.19
rs1443432
-
Intergenic
9
100583195
0.47
rs894673
FOXE1
Promoter
9
100612270
0.47
rs3021523
FOXE1
Coding exon-synon
9
100616583
0.29
rs4460498
FOXE1
Downstream
9
100620412
0.46
rs4128956
MED27
Intron
9
134818509
0.38
71
Table 3-1 Continued
rs657152
ABO
Intron
9
136139265
0.38
rs944289
-
Intergenic
14
36649246
0.41
rs10149689
TSHR
Promoter
14
81415800
0.46
rs4903957
TSHR
Intron
14
81448511
0.32
rs11159483
TSHR
Intron
14
81501311
0.25
rs2075179
TSHR
Coding exon-synon
14
81562998
0.1
rs12885526
TSHR
Intron
14
81574429
0.36
rs1991517
TSHR
Coding exon-missense
14
81610583
0.1
rs945006
DIO3
3'UTR
14
102029277
0.12
rs3908399
-
Intergenic
20
12901275
0.27
rs6030171
PTPRT
Intron
20
40994094
0.31
rs500243
SLC16A2
Intron
X
73676685
0.37
rs4892386
SLC16A2
Intron
X
73718735
0.32
Chr: chromosome, MAF: minor allele frequency, UTR: untranslated region.
72
Table 3-2 Demographic Characteristics of Cohorts.
a
SHL term
(N=799)
SHL preterm
(N=404)
NICU preterm
(N=380)
P-valuea
P-valueb
TSH level (mIU/L)
8.9±4.5
7.4±4.5
5.9±3.8
<0.001
<0.001
Male Gender
454 (56.8%)
230 (56.9%)
222 (58.4%)
0.97
0.67
Gestational Age
(weeks)
40.0±0
34.0±2.6
31.2±3.1
<0.0001
<0.0001
Birth weight
(grams)
3,489.9±434.0
2,405.1±695.3
1,773.4±712.3
<0.0001
<0.0001
Age at screening
(hours)
36.4±10.6
37.6±12.8
29.5±7.0
0.68
<0.0001
Total parenteral
nutrition
2 (0.3%)
51 (12.6%)
38 (10.0%)
<0.001
0.25
P-values for differences between SHL term and SHL preterm.
b
P-values for differences between SHL preterm and NICU preterm.
73
Table 3-3 Association statistics for all genotyped SNPs with neonatal TSH level for all
combined populations. P-values reported in this table are from ANOVA and nonparametric analysis.
SHL Combined
(N=1,203)
Preterm Combined
(N=784)
All Populations
(N=1,583)
SNP
ANOVA NP
ANOVA
NP
ANOVA
NP
rs10917469
0.7528
0.3101
0.2791
0.2005
0.9458
0.7193
rs1321108
0.9158
0.6954
0.303
0.7759
0.4175
0.8148
rs4849179
0.2598
0.4742
0.2782
0.481
0.2721
0.1839
rs877202
0.5271
0.6602
0.165
0.4215
0.1831
0.4164
rs9308765
0.052
0.3822
0.0841
0.2538
0.0142
0.1066
rs2288629
0.1125
0.45
0.224
0.4296
0.048
0.8108
rs1505287
0.6627
0.3227
0.649
0.9471
0.4997
0.2211
rs784490
0.4193
0.2856
0.1671
0.2018
0.5526
0.528
rs1976324
0.3268
0.6366
0.8745
0.8343
0.8638
0.9436
rs10493147
0.546
0.358
0.0701
0.0443
0.1836
0.1079
rs2545308
0.9677
0.8922
0.5966
0.5533
0.7198
0.9349
rs27178
0.9619
0.8553
0.2537
0.1269
0.5674
0.3666
rs4704397
0.0012
0.00037
0.0032
0.0074
0.000131
0.000198
rs9342104
0.6594
0.8155
0.4234
0.4766
0.9504
0.8611
rs6942231
0.0812
0.539
0.369
0.1698
0.6181
0.4383
rs9322817
0.0609
0.438
0.2374
0.1315
0.3853
0.2407
rs2983521
0.2517
0.3254
0.6611
0.7188
0.4708
0.7915
rs10486365
0.3561
0.1761
0.8154
0.6479
0.8889
0.2256
rs6977660
0.2457
0.1685
0.0844
0.1737
0.266
0.0699
rs10499559
0.7201
0.6735
0.8018
0.5151
0.6427
0.4651
rs10486653
0.7473
0.5105
0.3012
0.5109
0.8398
0.9275
rs1527680
0.2204
0.1149
0.041
0.0707
0.0408
0.0154
rs2252696
0.863
0.8943
0.9006
0.4825
0.8176
0.6244
rs7865184
0.4494
0.6661
0.7593
0.1664
0.9355
0.4005
rs10512065
0.3765
0.08
0.062
0.0229
0.3937
0.047
rs965513
0.002
0.0237
0.0163
0.0786
0.00064
0.0039
rs1443433
0.8521
0.8393
0.666
0.5086
0.8468
0.61
rs1443432
0.0466
0.0874
0.2357
0.451
0.0229
0.0285
rs894673
0.2178
0.4816
0.8799
0.851
0.2518
0.6393
rs3021523
0.0884
0.0927
0.0437
0.1423
0.0324
0.047
74
Table 3-3 Continued
rs4460498
0.1777
0.406
0.7991
0.8849
0.1892
0.5
rs4128956
0.0679
0.2111
0.366
0.6094
0.1854
0.7661
rs657152
0.0493
0.1728
0.0928
0.2228
0.0173
0.0742
rs944289
0.4915
0.3661
0.6303
0.7263
0.8397
0.8868
rs10149689
0.3957
0.2723
0.216
0.4152
0.1642
0.2357
rs4903957
0.6061
0.1911
0.8394
0.6728
0.4663
0.3086
rs11159483
0.2454
0.2215
0.1874
0.09
0.1936
0.1026
rs2075179
0.7826
0.9824
0.8474
0.9097
0.7666
0.9981
rs12885526
0.559
0.4342
0.9649
0.7441
0.7106
0.831
rs1991517
0.7395
0.9231
0.0433
0.1712
0.3744
0.6739
rs945006
0.8651
0.2766
0.267
0.5691
0.7954
0.61
rs3908399
0.044
0.1776
0.8479
0.3134
0.3641
0.2268
rs6030171
0.8891
0.6489
0.5915
0.6862
0.7144
0.4469
rs500243
0.128
0.0756
0.4275
0.797
0.1428
0.0968
rs4892386
0.0073
0.0095
0.0582
0.2294
0.0143
0.0583
75
Table 3-4 Association statistics for all genotyped SNPs with neonatal TSH level for
individual population cohorts. P-values reported in this table are from ANOVA and nonparametric analysis.
SHL Term (N=799)
SHL Preterm (N=404)
NICU Preterm (N=380)
SNP
ANOVA
NP
ANOVA
NP
ANOVA
NP
rs10917469
0.348
0.0724
0.4504
0.534
0.511
0.3517
rs1321108
0.9127
0.6842
0.9386
0.6803
0.0795
0.1883
rs4849179
0.5091
0.3613
0.4075
0.9425
0.4809
0.4565
rs877202
0.5594
0.5593
0.5057
0.971
0.2645
0.2225
rs9308765
0.0358
0.1824
0.2488
0.6247
0.2044
0.1287
rs2288629
0.2654
0.6044
0.643
0.2896
0.3443
0.6087
rs1505287
0.5449
0.2636
0.5706
0.4703
0.597
0.3648
rs784490
0.5856
0.2744
0.1172
0.1133
0.6059
0.6838
rs1976324
0.4701
0.6724
0.1757
0.1484
0.078
0.1744
rs10493147
0.9838
0.8336
0.306
0.173
0.2324
0.1562
rs2545308
0.6793
0.7623
0.8728
0.8949
0.5124
0.3412
rs27178
0.7575
0.762
0.9138
0.5949
0.1517
0.2181
rs4704397
0.0184
0.000578
0.0571
0.0677
0.0369
0.0658
rs9342104
0.443
0.7448
0.9974
0.956
0.1363
0.1017
rs6942231
0.1881
0.4229
0.5255
0.2947
0.063
0.1078
rs9322817
0.1088
0.486
0.5335
0.1997
0.0924
0.1997
rs2983521
0.2401
0.2857
0.5563
0.9692
0.8259
0.8154
rs10486365
0.6508
0.7737
0.4753
0.5017
0.4047
0.5013
rs6977660
0.9095
0.8635
0.0868
0.1208
0.0691
0.254
rs10499559
0.2781
0.2987
0.8155
0.4067
0.9108
0.6107
rs10486653
0.4469
0.6107
0.6649
0.8594
0.0976
0.1143
rs1527680
0.3504
0.4786
0.2706
0.2082
0.0275
0.0453
rs2252696
0.906
0.8397
0.6661
0.371
0.5509
0.2777
rs7865184
0.5114
0.3136
0.6618
0.7817
0.2243
0.0353
rs10512065
0.8573
0.9703
0.0316
0.0055
0.9892
0.9895
rs965513
0.0052
0.048
0.1351
0.4406
0.143
0.2477
rs1443433
0.2695
0.1495
0.4106
0.216
0.9807
0.7001
rs1443432
0.079
0.0707
0.5559
0.9126
0.3595
0.3215
rs894673
0.1014
0.3248
0.8757
0.8254
0.9111
0.9866
rs3021523
0.3693
0.4695
0.1325
0.2279
0.2819
0.424
rs4460498
0.0998
0.3012
0.8457
0.8253
0.8716
0.9881
76
Table 3-4 Continued
rs4128956
0.1921
0.2677
0.3602
0.489
0.4252
0.4105
rs657152
0.119
0.2615
0.3384
0.5335
0.177
0.3247
rs944289
0.9647
0.9142
0.1661
0.1728
0.739
0.4829
rs10149689
0.6685
0.515
0.5691
0.5821
0.3845
0.6665
rs4903957
0.542
0.2547
0.6337
0.4733
0.4111
0.2773
rs11159483
0.7336
0.509
0.1675
0.0578
0.7113
0.9163
rs2075179
0.7537
0.6832
0.9833
0.782
0.8505
0.9743
rs12885526
0.2137
0.1706
0.8077
0.2871
0.853
0.7218
rs1991517
0.4723
0.5476
0.0356
0.258
0.3726
0.517
rs945006
0.4875
0.252
0.6699
0.6907
0.4003
0.4448
rs3908399
0.0187
0.1441
0.6776
0.8059
0.3069
0.085
rs6030171
0.6954
0.6168
0.9116
0.8281
0.3811
0.7481
rs500243
0.3088
0.0431
0.462
0.1649
0.6851
0.5981
rs4892386
0.1641
0.0067
0.0346
0.0094
0.6943
0.8527
Table 3-5 TSH means and standard deviations for PDE8B and FOXE1 significant SNPs.
Gene
SNP
PDE8B
rs4704397
FOXE1
SHL term (N=799)
SHL preterm (N=404)
NICU preterm (N=380)
All Cohorts
Mean(SD) P-value
Mean(SD)
Mean(SD)
P-value
P-value
0.04
1.3x10-4
0.14
6.4x10-4
0.36
0.02
0.28
0.03
0.02
P-value
0.06
AA
10.2±4.5
8.0±4.6
6.2±3.9
GA
8.7±4.6
7.5±4.6
6.2±3.9
GG
8.4±4.3
6.7±4.3
5.3±3.5
-3
rs965513
5.2x10
0.14
AA
9.0±5.0
6.6±3.9
5.1±3.4
GA
8.5±4.3
7.1±4.3
5.8±3.7
GG
9.3±4.6
7.7±4.8
6.2±3.9
rs1443432
0.08
0.56
AA
9.3±4.5
7.6±4.8
6.1±3.9
AG
8.6±4.4
7.3±4.5
5.9±3.8
GG
8.8±4.9
7.1±3.8
5.1±3.2
rs3021523
0.37
0.13
CC
8.5±4.4
6.8±3.2
5.6±2.5
TC
8.7±4.4
6.9±4.6
5.7±3.5
TT
9.1±4.6
7.6±4.6
6.1±4.0
77
Table 3-6 TSH means and standard deviations for marginally significant SNPs.
Gene
SNP
Chr 2
rs9308765
ABO
SLC16A2
SHL term (N=799)
SHL preterm (N=404)
NICU preterm (N=380)
All Cohorts
Mean(SD)
Mean(SD)
Mean(SD)
P-value
P-value
0.20
0.01
0.18
0.02
0.69
0.01
0.03
0.04
P-value
0.04
P-value
0.25
AA
6.7±2.9
8.5±4.1
5.1±3.4
GA
9.5±5.1
7.6±4.6
6.7±4.3
GG
8.8±4.4
7.3±4.5
5.7±3.6
rs657152
0.12
0.34
GG
8.6±4.2
7.0±4.2
5.6±3.4
GT
9.0±4.6
7.5±4.6
5.9±3.8
TT
9.8±5.3
8.0±5.2
6.9±4.7
rs4892386
0.16
0.03
CC
8.8±4.5
6.8±4.2
6.0±3.9
TC
8.1±3.9
8.7±5.0
5.5±3.2
TT
9.8±4.7
7.9±4.7
5.7±3.7
PPP1R9A rs1527680
0.35
0.27
AA
8.9±4.6
7.1±4.2
5.7±3.7
GA
9.0±4.3
8.3±5.1
6.2±3.6
GG
9.6±4.5
7.3±5.6
8.9±6.0
78
79
Table 3-7 SNP haplotypes in the FOXE1 gene that are significantly associated (p<0.001)
with natural log transformed TSH levels.
SNPs
Gene
Haplotype
Frequency
Beta
P-value
FOXE1
rs965513 - rs1443433
AT
0.23
-0.08
4.2x10-4
GT
0.62
0.07
4.6x10-4
Frequency: frequency of haplotype indicated. Beta: beta coefficient for linear regression
model; positive value indicates the haplotype is associated with an increase in TSH level,
negative value indicates the haplotype is associated with a decrease in TSH level. P-value
= p-value for association between natural log transformed TSH and a specific haplotype
composed of the alleles listed.
80
Table 3-8 SNP haplotypes in the TSHR gene that are significantly associated (p<0.001)
with natural log transformed TSH levels.
SNPs
Gene
Haplotype
TSHR
rs10149689-rs4903957-rs11159483
AGT
TSHR
0.06
-0.16
7.9x10-4
0.05
-0.16
6.2x10-4
0.03
-0.28
4.2x10-5
0.05
-0.17
7.8x10-4
rs10149689-rs4903957-rs11159483-rs2075179
AGTT
TSHR
P-value
rs4903957-rs11159483-rs2075179
GTT
TSHR
Frequency Beta
rs4903957-rs11159483-rs2075179-rs12885526
GTTA
Frequency: frequency of haplotype indicated. Beta: beta coefficient for linear regression
model; positive value indicates the haplotype is associated with an increase in TSH level,
negative value indicates the haplotype is associated with a decrease in TSH level. P-value
= p-value for association between natural log transformed TSH and a specific haplotype
composed of the alleles listed.
81
Figure 3-1 Association statistics for all genotyped SNPs with neonatal TSH level for
combined populations. The X-axis is a list of all genotyped markers. The Y-axis is the log10 of the p-value from the ANOVA analysis. The horizontal dashed lines represent the
p-value cutoffs; * p-value = 0.05, ** p-value = 0.001. The solid line is for all populations
combined. The dashed line is for the SHL preterm and SHL term combined. The dotted
line is for the SHL preterm and the NICU preterm combined.
82
Figure 3-2 Association statistics for all genotyped SNPs with neonatal TSH level for
individual populations. The X-axis is a list of all genotyped markers. The Y-axis is the log10 of the p-value from the ANOVA analysis. The horizontal dashed lines represent the
p-value cutoffs; * p-value = 0.05, ** p-value = 0.001. The solid line is for the SHL term
population. The dashed line is for the SHL preterm population. The dotted line is for the
NICU preterm population.
83
CHAPTER 4
CHARACTERIZATION OF FOXE1 AND PDE8B ENHANCER
REGIONS FOR A ROLE IN NORMAL VARIATION IN NEONATAL
TSH LEVELS
The following manuscript is being prepared for submission. Additional authors on
this manuscript include Jeffrey Murray, and Kelli Ryckman.
In this study, we followed up on the two most significantly observed associations
with thyroid stimulating hormone (TSH) levels in newborns (Chapter 3). We sought to
identify the etiologic variants that may be responsible for the observed associations by
fine mapping adjacent enhancer elements. This was done through sequencing of a small
population of term neonates followed by replication of findings in a larger population of
term neonates. We adapted the extreme phenotype sampling approach by selecting
infants with newborn screening TSH levels that are on either extreme of the TSH
distribution (<2.2 – 25.0 µIU/ml) to increase the power of identifying the rare causal
variants.
Drs. Jeffrey Murray and Kelli Ryckman provided oversight for all aspects of the
project and provided input into study design. I conducted all the experiments and analysis
reported in this chapter. I also wrote the manuscript.
Abstract
Background: Thyroid stimulating hormone (TSH) levels are highly variable and
largely controlled by genetic factors. Several genome-wide association studies (GWAS)
have identified variants associated with TSH levels; however, the causative variants
responsible for GWAS signals are unknown. Methods: A population of term Iowa
neonates (n=58) with TSH levels at both ends of the normal distribution (<2.2 – 25.0
µIU/ml) were sequenced in six potential enhancer regions for two of the genes most
associated with TSH levels; FOXE1 and PDE8B. Identified variants were genotyped in
84
an additional population of 306 term newborns that were also at the two extreme ends of
the TSH level distribution. Results: We identified 12 common and three rare variants in
sequencing; and although none of these variants were statistically significant with TSH
levels, one of the rare variants (rs112053411) identified was interestingly found in three
neonates, all in the upper distribution of TSH levels including one infant that was later
diagnosed with congenital hypothyroidism. Conclusions: Variants identified were not
statistically significant for an association with TSH levels; however, one of the rare
variants (rs112053411) identified only in neonates in the upper distribution of TSH
levels is worth pursuing with functional studies as well as further replication in
individuals with thyroid disorders.
Introduction
In healthy adult subjects, thyroid stimulating hormone (TSH) has considerable
variability between individuals, whereas this variability is much less in the same
individual when TSH is measured repeatedly over an extended period of time (Panicker
et al. 2010). Likewise, newborn TSH levels are highly variable and this variability is
largely controlled by genetic factors (Alul et al. 2013a; Alul et al. 2013b). In the previous
work reported in chapters two and three, we have estimated the heritability of TSH levels
in newborns to be 58% which mirrors previous heritability estimates for adult serum TSH
levels (Panicker et al. 2008), and we identified genetic variants that are associated with
neonatal TSH levels. The identified variants (rs965513 upstream of FOXE1 and
rs4704397 in intron 1 of PDE8B) replicated previous genome-wide association studies
(GWAS) for adult TSH levels; however, the causative variants responsible for the
reported associations have not yet been identified.
These two variants; rs965513 and rs4704397, have been extensively studied and
found to be significantly associated with various thyroid related traits in various studies,
hence, pursuing the causative variants responsible for these associations is justified. As
85
for rs965513 which was found to be associated with adult TSH level in GWAS
(Gudmundsson et al. 2012), it has been repeatedly found to be associated with thyroid
cancer (Gudmundsson et al. 2009; Gudmundsson et al. 2012; Jones et al. 2012; Tomaz et
al. 2012) and with hypothyroidism (Denny et al. 2011). Whereas rs4704397 that was
initially identified in the GWAS by Arnaud-Lopez et al. (2008) to be associated with
adult serum TSH levels, was later reported to be associated with subclinical
hypothyroidism during pregnancy (Shields et al. 2009), as well as with TSH levels in
obese children (Grandone et al. 2012). Identifying the causative variant responsible for
these associations is important to better understand the etiology of these thyroid
conditions.
In this study, we sequenced potential enhancer regions for the two most
significant genes from the previous association study; FOXE1 and PDE8B, to examine
possible causative variants. We chose the extreme phenotype sampling approach for
study population selection. The extreme phenotype approach has been used to search for
rare causal variants in complex traits by selecting individuals at both extremes of a
continuous trait distribution spectrum. The principle is that rare causal variants with large
effect sizes on the phenotype of interest will be enriched in one of the two tails of the
distribution leading to an increased minor allele frequency in this particular study group
and therefore an increased power in identifying the rare causal variants compared to
random sampling from the entire distribution (Lamina 2011; Emond et al. 2012; Barnett
et al. 2013). We also chose a unique approach for the selection of potential enhancer
regions of interest by utilizing the recently published data by the Encyclopedia of DNA
Elements (ENCODE) (Dunham et al. 2012). The ENCODE project was designed to
comprehensively describe all functional elements of the human genome. The most
striking finding of the ENCODE project was that about 80% of the human genome is
functional and mostly comprises regulatory elements such as enhancers (Dunham et al.
2012). Enhancer elements are critical for the regulation of gene expression and authors
86
from the ENCODE project found that previously reported GWAS single nucleotide
polymorphisms (SNPs) are enriched in the identified regulatory elements in this project
including enhancers (Dunham et al. 2012). ENCODE findings have a great impact on
biomedical research, shed light on the importance of enhancer elements, and provide new
insight for the search of causative variants after association studies.
In this study, we sequenced potential enhancer regions based on ENCODE data,
in a group of 58 term newborns that are at the two extreme ends of the TSH level
distribution (<10th and >90th percentile). We identified three rare variants in sequencing
results. To follow up on the identified rare variants, we used the TaqMan chemistry to
genotype them in an additional population of 306 term newborns that are also at the two
extreme ends of the TSH level distribution (<5th and >95th percentile).
Materials and Methods
This study was conducted in two phases. The first phase is the sequencing of
potential FOXE1 and PDE8B enhancer regions in a small population of 58 term neonates.
The second phase pursues sequencing results of interest in a larger population of 306
term neonates by using the TaqMan genotyping system (Applied Biosystems, Foster
City, CA).
Study Population
For this study, we used the extreme phenotype sampling approach by selecting
infants with newborn screening thyroid stimulating hormone (TSH) levels that are on
either extreme of the TSH distribution (<2.2 – 25.0 µIU/ml). Study samples were
obtained from two sources. The first source was from the University of Iowa Hospitals
and Clinics Newborn Nursery. Only singleton term neonates (n=58) with gestational ages
between 37 and 42 weeks were included in this study. Infants with TSH levels below the
10th (n=30) or above the 90th (n=28) percentile of the TSH distribution were chosen. Only
1 individual had an abnormal (TSH≥25.0 µIU/ml) level on the initial screen. Gestational
87
age was determined from the first day of the last menstrual period. Gestational age was
confirmed through obstetrical judgment and if uncertain, ultrasound measurements were
used for confirmation. All families provided signed informed consent (UI
IRB199911068) to be included in a repository of samples designed to provide DNA and
limited epidemiologic data to study complications of newborn infants (Steffen et al.
2007). TSH measured by the State Hygienic Laboratory (SHL) at the University of Iowa
as part of routine neonatal screening was linked to the sample and medical record data.
DNA was extracted from cord blood, discarded venous blood, or buccal swab for all
infants. All DNA was extracted using standard protocols.
The second source was from the University of Iowa SHL where we obtained deidentified residual dried blood spots from a population of Iowa newborns as part of the
newborn screening program. Only singleton term neonates (n=306) with gestational ages
between 39 and 41 weeks were included in this study. Infants with TSH levels below the
5th (n=154) or above the 95th (n=152) percentile of the TSH distribution were selected.
Approval for use of the de-identified data and blood spot cards was granted by the Iowa
Department of Public Health and a waiver of consent was obtained from the Institutional
Review Board at the University of Iowa (IRB#200908793). All neonates had TSH
measurements obtained between day 1 and 3 of life and had not received a transfusion
prior to sample collection. All neonates with a presumptive positive screening result were
excluded from this study. Quantification of TSH was performed at the SHL using CLIA
(Clinical Laboratory Improvement Amendments) certified methods. TSH was determined
by solid phase, time-resolved fluoroimmunoassay from dried newborn blood spots using
PerkinElmer’s AutoDELFIA platform (Waltham, MA). DNA was extracted from one
dried whole blood spot for all samples using the AutoGen (Holliston, MA) QuickGene810 nucleic acid extraction machine with the DNA Tissue Kit (AutoGen) and following
manufacturer’s recommendations.
88
Selection of Studied Regions
We selected six potential enhancer regions for FOXE1 and PDE8B genes based
on ENCODE data (Table 4-1) using the University of California, Santa Cruz (UCSC)
Genome Browser (Kent et al. 2002; Rosenbloom et al. 2013). The specific UCSC
Genome Browser ENCODE tracks used were the “Layered H3K27Ac” track which is for
an activating acetylation mark on seven cell lines from ENCODE, one of the histone
modification marks often found near active regulatory elements and believed to
differentiate between active and inactive enhancers, and the “DNase Clusters” track
which is for DNaseI hypersensitive sites in 125 cell types from ENCODE, marking
accessible chromatin which is often found in regulatory DNA regions (Dunham et al.
2012). The mammalian, primate, and vertebrate conservation tracks form UCSC Genome
Browser were also used to see if the picked regions were conserved (Figure 4-1 and
Figure 4-2). Potential enhancer regions were chosen in the vicinity of the two most
significantly associated SNPs with neonatal TSH levels in the work reported in Chapter
three (rs965513 near FOXE1, and rs4704397 near PDE8B) (Figure 4-1 and Figure 4-2).
These two SNPs are also among the top GWAS associated SNPs with adult TSH levels
and adult thyroid disorders (Arnaud-Lopez et al. 2008; Gudmundsson et al. 2009; Shields
et al. 2009; Denny et al. 2011; Grandone et al. 2012; Gudmundsson et al. 2012; Jones et
al. 2012; Tomaz et al. 2012).
Genotyping
Sequencing
Primers used to amplify all enhancer regions were designed with Primer 3. Primer
sequences and PCR conditions for amplifying the regions of interest for the sequencing
of enhancer regions are listed in Table 4-2. Amplified regions in the form of PCR
products were sent for sequencing using an ABI 3730XL (Functional Biosciences, Inc.,
Madison, WI). The six potential FOXE1 and PDE8B enhancer regions were sequenced in
89
58 term neonates in the forward direction. All identified rare variants were confirmed by
sequencing in the reverse direction. Chromatograms were transferred to a UNIX
workstation, base-called with PHRED (v.0.961028), assembled with PHRAP
(v.0.960731), scanned by POLYPHRED (v.0.970312), and viewed with the CONSED
program (v.4.0).
TaqMan
We selected three SNPs to follow up on with TaqMan genotyping based on
sequencing results (Table 4-3). We chose to follow up on all three rare SNPs, minor
allele frequency (MAF) < 1%, identified in sequencing, and none of the common SNPs
since they were all not significantly associated. SNPs were genotyped using the TaqMan
chemistry (Applied Biosystems, Foster City, CA). All SNP genotyping assays were
available and ordered using either the Assay-on-Demand or Assays-by-Design service
from Applied Biosystems. These SNP genotyping assays included primers to amplify the
region containing the SNP of interest and two TaqMan Minor Groove Binder probes that
are specific to the polymorphic variant alleles at the site labeled with different fluorescent
reporter dyes, FAM and VIC. PCR reactions were performed using standard conditions
supplied by Applied Biosystems. Following thermocycling, fluorescence levels of the
FAM and VIC dyes were measured using the Applied Biosystems 7900HT Fast System
and genotypes were scored using the Sequence Detection System (SDS) software
(Applied Biosystems). Genotypes were uploaded into a Progeny database (Progeny
Software, LLC, South Bend, IN) containing the phenotypic data for subsequent analysis.
Genotyping efficiency was >98% for all markers.
Statistics
Given that we used the extreme phenotype approach for study population
selection, we treated TSH levels as a dichotomous trait by grouping all sequenced
neonates with low TSH values (n=30) into one group and all sequenced neonates with
90
high TSH values into another group (n=28). To determine if any of the observed
sequence variants is associated with newborn TSH levels, we compared the frequency of
each sequence variant between the low TSH group and the high TSH group with Fisher’s
exact test. We excluded any sample with poor sequencing quality (PHRED Quality Score
<30) for a given variant from analysis for that specific variant.
For the three SNPs genotyped using TaqMan assays, testing for association of
with TSH levels in a group of 306 neonates was performed as mentioned above.
Results
Sequencing
A total of 58 infants were sequenced for six FOXE1 and PDE8B enhancer regions
to search for potential etiologic sequence variants that may be associated with newborn
TSH levels. A total of 15 known sequence variants were detected; 14 of which are SNPs
and one deletion/insertion variation (DIV) of 8 base pairs (Table 4-4). Of the 15
identified sequence variants, 12 are common (MAF > 1%), were not found to be
associated with newborn TSH levels (p-value > 0.05), and will not be pursued any
further. The remaining 3 SNPs are rare (reported MAF < 1% in the 1000 genomes
project) and each SNP was identified in one sample only. SNPs rs148044470 in PDE8B
Enhancer 1 and rs117811946 in FOXE1 enhancer region 1 were each found in an infant
with TSH level below the 10th percentile. SNP rs112053411 in FOXE1 enhancer region 3
was found in an infant with TSH level above the 90th percentile. The TSH level for this
infant was interpreted as borderline in the newborn screen for congenital hypothyroidism
(CH). After sequencing and identifying this SNP, we searched the medical record and
found that this infant was later diagnosed with CH based on follow-up serum testing in
the clinic. We then sequenced this infant’s parents and found that this SNP is transmitted
from the mother who is also heterozygous for it and was diagnosed with hypothyroidism.
91
TaqMan
A total of 306 infants were genotyped with TaqMan assays for the three rare
SNPs identified in sequencing (rs148044470, rs117811946, and rs112053411) to increase
the power of detecting an association with TSH levels. SNP rs148044470 was identified
in two samples, one from the low TSH group and one from the high TSH group. SNP
rs117811946 was identified in five samples, two from the low TSH group and three from
the high TSH group. SNP rs112053411 was identified in two samples, both from the high
TSH group. All three SNPs were not found to be associated with newborn TSH levels (pvalues 1.0, 0.68, and 0.50 respectively).
Discussion
The genetic contribution to TSH variability is widely studied due to the
importance of TSH level in normal human physiology. There have been six successful
GWAS, to date, identifying a number of loci to be associated with TSH variability
(Hwang et al. 2007; Arnaud-Lopez et al. 2008; Gudmundsson et al. 2009; Lowe et al.
2009; Panicker et al. 2010; Gudmundsson et al. 2012). One of the most interesting
associated loci is a region in intron 1 of PDE8B, which has been found to be the most
significantly associated locus (p-value=1.95x10-56) in the most recent meta-analysis of
TSH level related GWAS (Porcu et al. 2013). An attempt to identify the functional
variant responsible for this association by sequencing all PDE8B exons was unsuccessful,
suggesting that the causative variant is likely in a noncoding region (Arnaud-Lopez et al.
2008). A second interesting locus is an intergenic region on chromosome 9q22, with
FOXE1 being the nearest gene, found in a GWAS of TSH level to be one of the most
significantly associated loci (p-value=4.3x10-31) (Gudmundsson et al. 2012). The
causative variant responsible for this association has not been identified either since most
GWAS identify associated regions but not the causative variants. It has been observed
that about 40% of GWAS significantly associated SNPs are located in intergenic regions,
92
and another 40% are in introns (Manolio 2010). Furthermore, research from the
ENCODE project has shown that previously reported GWAS SNPs are enriched in the
identified regulatory elements in this project including enhancers (Dunham et al. 2012).
Examples of diseases known to be caused by enhancer variants include α-thalassemia,
preaxial polydactyly, holoprosencephaly, and nonsyndromic cleft lip (Epstein 2009).
Therefore, comparing GWAS associated loci for a given trait, such as TSH levels, with
reported ENCODE regulatory regions may help identify narrower loci that are functional
and worth pursuing with fine mapping techniques. Fine mapping a given region to
identify causative variants may be done through sequencing which enables the
identification of rare variants that are missed in GWAS and may have a more extreme
phenotype.
In this light, we decided to further investigate these two loci (PDE8B and
FOXE1), which were also the most significantly associated with newborn TSH level in
the work previously reported in Chapter 3. We aimed to fine map six potential enhancer
regions identified by ENCODE that were also in the vicinity of the above mentioned
GWAS hits to identify potential causative variants. Only term newborns were selected to
minimize TSH variability due to gestational age and birth weight factors. We identified a
total of 15 known variants in sequencing the first population of 58 newborns. Of the 15
identified variants, 12 are common (MAF > 1%) and were not found to be associated
with newborn TSH levels (p-value > 0.05). The remaining 3 SNPs are rare (MAF < 1%)
and each SNP was identified in one sample only.
Our most interesting finding is SNP rs112053411 in the FOXE1 enhancer region
3 identified in an infant with an initial TSH level above the 90th percentile. The TSH level
for this infant was interpreted as borderline in the newborn screen for CH. However, after
identifying this SNP through sequencing, we examined the medical record for this infant
and found that the infant was later diagnosed with CH based on follow-up serum testing
in the clinic. We also discovered that the infant’s mother is on thyroid hormone
93
replacement therapy. After sequencing this infant’s parents, we found that the mother is
also heterozygous for this SNP. Whether the mother had CH or adult-onset
hypothyroidism is not known, however, the fact that both mother and infant are
hypothyroid and heterozygous for this rare SNP is intriguing. When we further examined
this SNP with TaqMan genotyping, it was identified in two infants from the high TSH
group (n=152) and in none of the infants in the low TSH group (n=154). Although this
finding was not statistically significant for an association with TSH levels (p-value =
0.50), this may be due to the modest study population size and lack of power to detect an
association for SNPs with small effect sizes. Furthermore, given that this SNP is very rare
with MAF of 4 in a thousand, and yet it was detected in a total of two infants in TaqMan
genotyping, all with high TSH levels, from a small population size of 306, it can be
argued that this SNP is worth pursuing further in a larger population. Although the
observed MAF for this SNP in our population of 306 infants is not statistically
significantly different from the reference MAF (p-value = 0.63), it is still observed almost
two times more than expected making it an interesting finding. If this SNP shows
statistical significance for association with TSH levels in future larger studies, or is
shown to affect enhancer activity in functional studies, then this SNP might have
important clinical implications. Especially since there has been recent evidence that
infants with elevated TSH in newborn screening (blood spot TSH > 20 µIU/ml), but are
not diagnosed with CH, are at an increased risk of developing persistent subclinical
hypothyroidism later in childhood (Leonardi et al. 2008). Identifying infants who are
likely to develop thyroid problems later in childhood is critical for early detection and
treatment.
The two other rare SNPs identified are rs148044470 in PDE8B Enhancer 1 and
rs117811946 in FOXE1 enhancer region 1, each found in an infant with TSH level below
the 10th percentile. However, after doing TaqMan genotyping of 306 infants, the two
94
SNPs were found in infants from both the low and the high TSH groups, and therefore
are unlikely to be associated with TSH levels (p-values 1.0 and 0.68 respectively).
This study has a few limitations; first, we do not have access to the medical
records for SHL studied infants since we only obtained their de-identified data and blood
spot cards. Therefore, we were not able to connect TSH measurements to medical record
information to obtain more detailed information on neonatal illness or race. However, in
2009 86.9% of the births in Iowa were Caucasian, suggesting that the majority of our
samples are from Caucasians. Another limitation was that we do not have follow up data
on our study cohort to check for development of thyroid conditions later in life. As
mentioned above, studies have shown a high rate of persistent subclinical hypothyroidism
developing later in childhood for infants with elevated TSH in newborn screening (blood
spot TSH > 20 µIU/ml), but are not diagnosed with CH (Leonardi et al. 2008). Having
that information would have been valuable to check for an association with our studied
SNPs. And finally, our small study size does not give us enough power to detect variants
with low effect sizes for a trait such as TSH level which is a highly polygenic and
complex trait.
95
Table 4-1 Potential FOXE1 and PDE8B enhancer regions studied.
Region
Location (UCSC Genome Browser
February 2009 build)
Distance from top GWAS
associated SNP
FOXE1
Enhancer 1
chr9:100,564,149-100,565,129
8 kb downstream of rs965513
FOXE1
Enhancer 2
chr9:100,565,744-100,566,698
10 kb downstream of rs965513
FOXE1
Enhancer 3
chr9:100,535,465-100,536,666
19 kb upstream of rs965513
PDE8B
Enhancer 1
chr5:76,587,369-76,588,272
69 kb downstream of rs4704397
PDE8B
Enhancer 2
chr5:76,541,540-76,541,997
23 kb downstream of rs4704397
PDE8B
Enhancer 3
chr5:76,597,139-76,598,388
79 kb downstream of rs4704397
Source: (UCSC Genome Browser).
96
Table 4-2 Primer sequences and PCR conditions for sequencing FOXE1 and PDE8B
enhancer regions.
Amplicon
Primer Sequence
Annealing
Temperature
Product
Size
FOXE1
Enhancer 1
F
R
CGTTCTTCCTTTTCACTTGCT
TCTGTTCTTTTTCCCTTTTGG
55
843
FOXE1
Enhancer 2
F
R
GACAGGTGGCCTCGCATC
TGTCCCACTCCATCCCTCTC
62
955
FOXE1
Enhancer 3
F1
R1
F2
R2
GGGAAGTATGGTGGGAACCT
GCTACAGTTGGGTCTGGAAAC
GACATTCTCGCCTTTCACACT
TTCCAATAACAGTCCTCCGATT
62
910
56
511
PDE8B
Enhancer 1
F
R
AATCTTTCGCTGGCTTGGAC
CACAACATACGCCTTCCTGA
61
867
PDE8B
Enhancer 2
F
R
GCCTGCCTCATTTCCTCTTT
GAGTCCCCACGAACAACCTA
61
779
PDE8B
Enhancer 3
F1
R1
F2
R2
TCTGTTTCTTTGCCCATCAA
GCCATCGTCTTGCTAACTCTG
CGGCAGTGTCTATTATCAGTGG
CAGGTAGGGAAGTCGGTGTG
61
900
61
945
97
Table 4-3 List of SNPs selected for further investigation after sequencing.
SNP
Base
change
Region
MAF
Reason SNP was chosen
rs117811946 C/G
FOXE1
Enhancer 1
0.004
SNP was found in sequencing in one
neonate with TSH below the 10th percentile
rs112053411 C/G
FOXE1
Enhancer 3
0.004
SNP was found in sequencing in one
neonate with TSH above the 90th percentile
that was later diagnosed with congenital
hypothyroidism
rs148044470 A/T
PDE8B
Enhancer 1
0.002
SNP was found in sequencing in one
neonate with TSH below the 10th percentile
Table 4-4 List of all sequence variants detected in the sequencing of 58 newborns.
Region
Sequence
variation name
in dbSNP
Variation
class
Change
Minor allele
frequency
(MAF)
Location (UCSC Genome
Browser February 2009
build)
Number of newborns
with variant (low and
high TSH group)
Fisher’s exact test pvalue for association
with TSH level
FOXE1
Enhancer 1
rs79229991
SNP
(A/C)
0.03
chr9:100,564,393
5 (3 and 2)
1.0
rs57077725
SNP
(C/T)
0.04
chr9:100,564,512
5 (3 and 2)
1.0
rs117811946
SNP
(C/G)
0.004
chr9:100,564,806
1 (1 and 0)
1.0
FOXE1
Enhancer 2
rs77394667
SNP
(A/G)
0.13
chr9:100,565,813
18 (11 and 7)
1.0
rs114804130
SNP
(C/G)
0.10
chr9:100,566,031
12 (8 and 4)
0.74
FOXE1
Enhancer 3
rs112053411
SNP
(C/G)
0.004
chr9:100,536,171
1 (0 and 1)
0.49
rs62573974
SNP
(C/T)
0.34
chr9:100,536,542
33 (15 and 18)
0.62
rs141224302
DIV
(8bp del)
0.34
chr9:100,536,606100,536,613
33 (15 and 18)
0.62
PDE8B
Enhancer 1
rs148044470
SNP
(A/T)
0.002
chr5:76,587,716
1 (1 and 0)
1.0
PDE8B
Enhancer 2
rs57774448
SNP
(G/C)
N/A
chr5:76,541,674
19 (10 and 9)
1.0
PDE8B
Enhancer 3
rs10066802
SNP
(A/G)
0.44
chr5:76,597,461
27 (10 and 17)
0.33
rs76281411
SNP
(C/T)
0.22
chr5:76,597,627
18 (8 and 10)
0.79
rs11745130
SNP
(A/G)
0.16
chr5:76,597,857
24 (13 and 11)
0.81
rs35689253
SNP
(A/G)
0.32
chr5:76,597,887
35 (19 and 16)
0.83
rs1382893
SNP
(C/T)
0.13
chr5:76,598,292
9 (4 and 5)
1.0
98
Figure 4-1 FOXE1 potential enhancer regions. The GWAS signal rs965513 is shown in green and the three selected enhancer regions
are shown with UCSC Genome Browser ENCODE regulation tracks to demonstrate enhancer signals.
99
Figure 4-2 PDE8B potential enhancer regions. The GWAS signal rs4704397 is shown in green and the three selected enhancer regions
are shown with UCSC Genome Browser ENCODE regulation tracks to demonstrate enhancer signals.
100
101
CHAPTER 5
CONCLUSIONS AND FUTURE DIRCTIONS
Conclusions
Congenital hypothyroidism (CH) is defined as thyroid hormone deficiency
present at birth. It is a common and preventable cause of mental retardation and is
screened for at birth in the newborn screening program by thyroid stimulating hormone
(TSH) or thyroxine measurements. TSH is considered the most informative marker of
thyroid function and is the test of choice for clinicians for the diagnosis of most thyroid
disorders. However, TSH is highly variable and manifests a wide reference range in the
general population leading to some challenges in its interpretation in newborn screening
as well as its later use as a clinical diagnostic test of thyroid function. This variability in
TSH is largely controlled by genetic factors and this has been extensively studied in
adults, however, no studies have addressed neonatal TSH variability. The work in this
thesis is focused on exploring whether TSH variability is largely controlled by genetic
factors in the neonatal period as it is in adults, as well as investigating these genetic
factors in both term and preterm neonates.
The genetic factors controlling adult TSH variability have been widely studied
through heritability studies, candidate-gene studies, and genome-wide association studies
(GWAS). GWAS have no a priori hypotheses and therefore have the advantage of
discovering loci that would not be suspected to be associated based on known biology.
Hence, several novel loci have emerged from GWAS associated with adult TSH levels;
however, the causative variants responsible for the reported associations were not
identified. This work addresses all of these areas but in relation to neonatal TSH
variability rather than adult. We estimated heritability, replicated previous genetic
associations reported in GWAS, and investigated functional variants that may be
responsible for GWAS signals.
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In case of TSH heritability; adult TSH heritability was estimated to vary from
32% (Samollow et al. 2004), to 64% (Hansen et al. 2004), and to a maximum of 65%
(Panicker et al. 2008). TSH heritability has never been determined in the neonatal period;
therefore, we examined 381 twin pairs obtained from the Iowa Neonatal Metabolic
Screening Program. We estimated neonatal TSH heritability to be 58% with a P-value of
2x10-5. TSH is known to be largely affected by age, and the use of age-dependent
reference ranges for TSH is strongly advocated, with infants, children, adolescents, and
adults being in separate groups (Kratzsch et al. 2008). Therefore, it can be argued that
different genetic and environmental factors are responsible for this age-dependent
variation, resulting in different heritabilities across different age groups. Furthermore,
there are examples from the literature where heritability estimates vary between different
age groups, such as the variable heritability estimates of lipid and lipoprotein levels
across three age groups in the same study (Iliadou et al. 2001).
Our study is the first to estimate heritability of TSH levels in the neonatal period,
as well as the first to use newborn blood spot card measurements to estimate the genetic
heritability of any trait, illustrating the utility of stored newborn blood spot cards as a
valuable resource for genetic studies. The estimated heritability of 58% in this study
mirrors previous reports of adult TSH heritability, and provides direct evidence for a
strong genetic contribution to TSH variability at birth, suggesting that thyroid function is
mainly controlled by genes throughout life. This may have clinical implications in
utilizing neonatal TSH measurements to predict the risk of adult diseases later in life. For
example, TSH level variation even within the normal physiological range in euthyroid
adults has been associated with bone mineral density (van der Deure et al. 2008), mean
platelet volume possibly affecting thrombosis (Kim et al. 2013b), and cholesterol and
triglycerides (Roos et al. 2007; Garduno-Garcia et al. 2010). And since TSH is largely
controlled by genetic factors, it can be argued that neonatal TSH levels may reflect TSH
103
levels in adulthood and provide early prediction of childhood and adult thyroid
abnormalities.
Given that TSH individual levels are highly heritable, efforts were directed
towards identifying the genes responsible for this heritability. Several GWAS as well as
candidate-gene studies were successful in identifying both specific genes as well as
intergenic loci with unknown function to be associated with adult TSH levels. However,
no studies addressed the genetic variation associated with neonatal TSH levels, and as
mentioned previously different genes may play a role at different stages for a given trait.
Therefore, we aimed to replicate major genetic associations with adult TSH levels from
the literature in a population of term and preterm neonates, as well as study other
candidate genes that are biologically plausible to control TSH levels but were not found
to be significantly associated in adult TSH studies. Our results replicated two of the most
important adult GWAS findings (Arnaud-Lopez et al. 2008; Gudmundsson et al. 2012),
the first was for rs4704397 in the PDE8B gene (p=1.3x10-4), and the second was
rs965513 (p=6.4x10-4) on chromosome 9 upstream of the FOXE1 gene. Both of these
SNPs met statistical significance after correction for multiple testing. Our results
demonstrate the importance of these two loci in determining TSH levels in the newborn
period, emphasizing their role at birth and in adulthood. However, thyroid function
undergoes marked changes during puberty to adapt to the increased energy expenditure in
response to body and sexual development (Fleury et al. 2001). Therefore, additional
studies in late childhood and adolescence are needed to ensure their involvement
throughout life, and it could be speculated that additional genetic factors may be
responsible for the observed thyroid function changes during puberty.
Additionally, these two SNPs have been extensively studied and found to be
significantly associated with various thyroid related diseases in various studies. For
example, rs965513 has been repeatedly found to be associated with thyroid cancer
(Gudmundsson et al. 2009; Gudmundsson et al. 2012; Jones et al. 2012; Tomaz et al.
104
2012) and with hypothyroidism (Denny et al. 2011). For thyroid cancer, each copy of the
minor A allele for SNP rs965513 near FOXE1 was associated with an increased risk of
thyroid cancer (Gudmundsson et al. 2009; Gudmundsson et al. 2012; Jones et al. 2012;
Tomaz et al. 2012). The minor A allele is also the allele found to be associated with a
decrease of 0.2-0.7 mIU/L in TSH levels in our term and preterm combined cohort,
which mirrors adult findings. It has been speculated that lower TSH levels may lead to
poor differentiation of thyroid epithelium, resulting in an increased risk of malignant
transformation (Gudmundsson et al. 2012). As for rs4704397, it was reported to be
associated with subclinical hypothyroidism during pregnancy (Shields et al. 2009), as
well as with TSH levels in obese children (Grandone et al. 2012). Therefore, the
identified association of these two SNPs with TSH levels at birth sheds light on the
possibility of using these two SNPs as biomarkers for the early prediction of risk for adult
diseases and conditions associated with thyroid hormone levels.
Finally, we aimed to identify the causative variants that may be responsible for
the observed associations with rs4704397 in intron 1 of the PDE8B gene and rs965513 in
an intergenic region on chromosome 9 upstream of the FOXE1 gene. Both these variants
have been identified in adult TSH GWAS (Arnaud-Lopez et al. 2008; Gudmundsson et
al. 2012) but the functional variants responsible for these associations are unknown.
Identifying the real functional variants tagged by the associated SNP after GWAS has
always been a challenge. Often, functional variants are unsuccessfully searched for in the
nearest gene. This is the case with rs4704397 in intron 1 of the PDE8B gene where all
exons were sequenced but the causative variant was not identified (Arnaud-Lopez et al.
2008). This implies that the causative variant may be in intergenic regions that function
as regulatory elements controlling gene expression, such as enhancers. The search for
etiologic variants in noncoding regulatory regions can be argued for especially after the
Encyclopedia of DNA Elements (ENCODE) project reported that GWAS significantly
associated SNPs are enriched in the identified regulatory elements in this project
105
including enhancers (Dunham et al. 2012). We chose to fine map six enhancer regions for
our two genes of interest PDE8B and FOXE1 to identify functional variants that may be
affecting enhancer activity resulting in differential gene expression and variable TSH
levels. None of the identified variants were statistically significant for an association with
TSH levels; however, one of the rare variants was only identified in neonates with TSH
levels above the 95th percentile of the distribution, one of whom was diagnosed with CH,
making this variant worth pursuing with functional studies.
There are several challenges to identifying genetic factors responsible for the
variation observed in a complex trait such as TSH level. First, although there have been
several successful GWAS and candidate-gene studies identifying variants associated with
adult TSH levels, all identified loci together do not account for the entire observed
variability in TSH levels. For example, it is reported that the most significantly associated
SNP with TSH levels in PDE8B gene (rs4704397) is responsible for 2.3% of the
observed variation in TSH levels (Arnaud-Lopez et al. 2008). Furthermore, the most
recent meta-analysis of GWAS for TSH variation reported that all 19 significantly
associated loci account for only 5.64% of the total trait variance observed (Porcu et al.
2013).Therefore, it is evident that there are more genes and variants yet to be identified to
explain the remaining missing heritability. It has been suggested that missing
heritabilities of complex traits may be within a large number of unidentified variants each
with a small effect size making their identification hard in small study cohorts (Manolio
et al. 2009). Another possibility is the role of rare variants, each with larger effect sizes,
however also difficult to detect in traditional GWAS and candidate-gene association
studies (Manolio et al. 2009). And finally, missing heritabilities may be explained by
structural variants, gene-gene, or gene-environment interactions that are poorly studied
with current technology (Manolio et al. 2009).
A second challenge relates to understanding the biology and pathways responsible
for the observed associations. For example, the FOXE1 SNP rs965513 that was
106
repeatedly found to be associated with an increased risk of thyroid cancer (Gudmundsson
et al. 2009; Gudmundsson et al. 2012; Jones et al. 2012; Tomaz et al. 2012) and the same
risk allele is associated with low TSH levels in adults and neonates. This risk allele has a
frequency of 37% leading to the fundamental question of why this risk allele was not
influenced by negative selection. There might be underlying beneficial traits that are
associated with this risk allele resulting in the observed high frequency. In this case,
studies have found that high TSH levels within the normal range are a risk factor for adult
thyroid cancer (Kim et al. 2013a) as well as pediatric thyroid cancer (Chiu et al. 2012).
This may explain the persistence of the risk allele resulting in low TSH level, but at the
same time does not explain how the same allele is associated with an increased risk of
thyroid cancer. This leads to the recognized conclusion that the exact mechanisms
involved are yet to be identified.
A third challenge in studying the genetic factors affecting neonatal TSH levels is
the large influence of gestational age, birth weight, and infant sickness on neonatal TSH
levels. This explains the less significant associations that we observed in our preterm
population compared to the term population when we studied genetic factors affecting
TSH levels in neonates (Alul et al. 2013b). There is also a challenge related to the use of
de-identified samples such as the study population that we obtained from the State
Hygienic Lab (SHL). Given that the samples are de-identified, we had no information on
infant sickness to account for when doing the association study with TSH levels.
Furthermore, we did not have diagnostic information on SHL infants with borderline
TSH levels in newborn screening and we could not determine if any of them were later
diagnosed with CH, therefore we had to exclude all SHL infants with borderline TSH
levels from our study although this borderline population may be the best sample to
examine for rare variants with large effect sizes.
107
Future Directions
In iodine sufficient countries, abnormal thyroid gland development is the most
common cause of congenital hypothyroidism (CH) accounting for 80-85% of CH cases
(Hinton et al. 2010; Rastogi and LaFranchi 2010). Thyroid dysgenesis CH is mostly
sporadic; only 2% of cases have a known causing mutation in one of the genes necessary
for thyroid development (NKX2.1, NKX2.5, PAX8, or FOXE1), whereas the remaining
98% of cases have an unknown cause (Rastogi and LaFranchi 2010; Abduljabbar and
Afifi 2012). So, it is evident that we still have much to learn about the genetic etiology of
CH. In thyroid dysgenesis CH cases with a mutation in one of the genes encoding a
transcription factor, CH may be present as part of a syndrome; for example FOXE1
mutations lead to Bamforth-Lazarus Syndrome (Rastogi and LaFranchi 2010). So, it may
be hypothesized that in the remaining sporadic non-syndromic thyroid dysgenesis CH
cases, the presence of a genetic variant within an enhancer element may be the cause of
CH. This hypothesis can be supported by the fact that enhancer elements are often tissue
specific (Epstein 2009). So a genetic variant affecting thyroid specific enhancer activity
may lead to thyroid dysgenesis but not affect gene expression in other tissues therefore
leading to non-syndromic CH. The involvement of genetic variants as the underlying
cause of a sporadic disease may be supported with the argument for gene-gene and geneenvironment interactions. Moreover, sporadic CH is not entirely sporadic, it has been
shown that there is approximately a 2% CH recurrence risk in families of newborns with
thyroid dysgenesis (Rastogi and LaFranchi 2010). Further evidence of genetic
involvement in what is thought to be a sporadic occurrence was shown in a French study
reporting that for patients with thyroid dysgenesis CH, 21.4% of first degree relatives had
asymptomatic thyroid developmental anomalies, compared to 0.9% in controls leading to
the hypothesis of a common genetic component with heterogeneous phenotypes (Leger et
al. 2002). This is not unusual in polygenic or complex disorders and may even be
observed in Mendelian disorders such as the report of a monozygotic twin pair carrying
108
the same mutation for Van der Woude Syndrome, which has an autosomal dominant
inheritance pattern, but are discordant for the phenotype (Jobling et al. 2011). The
authors suggest that this discordance may be explained by genetic and epigenetic factors
as well as the intrauterine environment (Jobling et al. 2011).
To study potential enhancer involvement in CH etiology we recently submitted a
proposal for review by the University of Iowa Institutional Review Board (IRB) to recruit
children diagnosed with CH from the University of Iowa Hospitals and Clinics pediatric
endocrinology clinic. We plan to recruit children diagnosed with CH, their siblings,
parents, and potentially grandparents, uncles, aunts, or cousins if any have thyroid
problems. The aim of this study would be to examine potential enhancer elements for any
genetic variants that may be associated with the disease. Identifying the underlying
genetic cause is of great importance for genetic counseling of the family for future
pregnancies. Although, as mentioned above, the recurrence risk is only about 2% for
“sporadic” thyroid dysgenesis (Rastogi and LaFranchi 2010), there is an increased
prevalence of asymptomatic thyroid developmental anomalies (21.4% versus 0.9% in
controls (Leger et al. 2002)) and these asymptomatic relatives may pass the CH risk to
their offspring.
Additionally, one proof of enhancer activity may be done in vivo through a
transgenic reporter assay. In the work reported in chapter four we selected enhancer
regions for fine mapping based on ENCODE data. One of the SNPs (rs112053411 in
FOXE1 enhancer region 3) identified is especially interesting and worth pursuing; it is a
rare variant that was only identified in neonates with TSH levels above the 95th percentile
of the distribution, one of whom was diagnosed with CH. We believe that this enhancer
element (FOXE1 enhancer region 3) should be studied further in a thyroid cell line to
confirm enhancer activity in thyroid tissue. Studying the effect of the identified SNP
(rs112053411) on enhancer activity and FOXE1 gene expression is also necessary. If it is
proved to be an active enhancer for FOXE1 gene expression in thyroid cell lines, then
109
additional studies of the enhancer activity with the common and rare alleles of SNP
rs112053411 in a mouse model would be necessary to evaluate effect on thyroid
embryogenesis.
The work reported in this thesis explored the contribution of genetic variants to
the wide range of normal variation observed in TSH levels in newborns. As a result, we
estimated this genetic contribution to TSH level variation in newborns for the first time to
be 58%. We identified two genetic variants to be significantly associated with newborn
TSH level variation, replicating previous findings in adults. And finally, the work
reported here sheds light on the importance of fine mapping enhancer elements in
studying the genetic contribution to complex traits. In the future, the use of larger study
cohorts combined with detailed phenotyping especially of relatives of CH patients with
asymptomatic thyroid anomalies will give insights into the true etiology of CH.
Ultimately, this work can have important clinical implications for better screening,
diagnosis, and counseling of CH families for future pregnancies.
110
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