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Transcript
HIV-1 RNA Viral Load
Carlos E. Martinez
Molecular Diagnostic Student
Austin Community College
08/06/08
Objectives

The HVI-1 RNA PCR viral load is performed
using the COBAS AmpliPrep TagMan HIV-1
Test is an in vitro nucleic acid amplification
test for the quantitation of Human
Immunodeficiency Virus Type 1 (HIV) RNA in
human plasma using this instrument for
automated processing and for automated
amplification and detection.
Objectives…
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The test is intended for use in conjunction
with clinical presentation and other laboratory
markers of disease progress for the clinical
management of HIV-1 infected patient.
The test can be used to assess patient
prognosis by measuring the base line HIV-1
RNA level or to monitor the effects of
antiretroviral therapy by measuring changes
in EDTA plasma HIV-1 RNA levels during the
course of antiretroviral treatment.
Principle of the Procedure
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The COBAS Ampliprep TagMan HIV-1 Test is a nucleic acid
amplification test for the quantitation of Human
Immunodeficiency Virus Type 1 (HIV-1) RNA in human plasma.
Specimen preparation is automated using the Ampliprep
Instrument with amplification and detection automated using the
TagMan 48 analyzer.
The HIV-1 test is based on three major processes:
specimen preparation to isolate HIV-1 RNA;
reverse transcription of the target RNA to generate
complementary DNA (cDNA);
Simultaneous PCR amplification of target cDNA and detection of
cleaved dual-labeled oligonucleotide probe specific to the target.
Store and handling
requirements
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Do not freeze reagents or controls.
Store HIV-1 QC at 2-8 Celsius.
Do no re-use any un-used Quality control,
once is used, discard using safety
procedures as established by laboratory
procedures and guidelines.
Quantitation Standard-QS-RNA
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The instrument TagMan HIV-1 test permits automated specimen preparation
followed by automated reverse transcription, PCR and detection of HIV-1 target
RNA and HIV-1 Quantitation Standard (QS) Armored RNA.
The Master Mix reagent contains primers and probes specific for both HIV-1
RNA and HIV QS RNA. The Master Mix has been developed to ensure
equivalent quantitation of group M subtypes of HIV-1. The detection of amplified
DNA is performed using target-specific and QS-specific dual labeled
oligonucleotide probe that permit independent identification of HIV-1 amplicon
and HIV-1 QS amplicon.
The quantitation of HIV-1 viral RNA is performed using the HIV-1 QS. It
compensates for effects of inhibition and controls the preparation and
amplification process, allowing a more accurate quantitation of HIV-1 RNA in
each specimen. The HIV-1 QS is a non-infectious Armored RNA construct that
contains region that allows HIV-1 QS amplicon to be distinguished from the HIV1 target amplicon.
The HIV-1 QS is added to each specimen at a known copy number and is
carried through the specimen preparation, reverse transcription, PCR
amplification and detection steps of cleaved dual-labeled oligonucleotide RNA
concentration in the test specimen by comparing the HIV-1 signal to the HIV-1
QS signal for each specimen and control
Warning and precautions
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For in vitro diagnostic use.
This test is for use with human plasma collected in EDTA
Do no pipette by mouth.
Wear protective equipments at all times.
Avoid microbial and ribonuclease contamination of reagents
when removing aliquots from control vials.
Do not pool controls from different lots numbers.
Do not mix reagent cassettes or control from different kits.
Specimens and control should be handled as if infectious using
safe laboratory procedures.
Procedural precautions

1. As with any test procedure, good
laboratory technique is essential to
proper performance of this assay.
Procedural limitations
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1.
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2.
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3.
This test has been validated for use with only human
plasma collected in EDTA anticoagulant. Testing of other
specimen types may result in inaccurate results.
The performances of this test using the TagMan only
applies for HIV-1.
Reliable results are dependent on adequate specimen
collection, transport, storage and processing.
Use of this product should be limited to personnel trained
in the techniques of PCR.
Interfering substances

Elevated levels of triglycerides, bilirubin,
albumin, hemoglobin and human DNA in
specimens as well as the presence of
autoimmune diseases such as Systemic
Lupus Erythematosus (SLE), Rheumatoid
Arthritis (RA) and Antinuclear Antibody (ANA)
has been shown NOT to interfere with the
quantitation of HIV-1 RNA or impact the
specificity of the TagMan for HIV-1 Test.
HIV Abstract

HIV infection is a disease caused by the
human immunodeficiency virus (HIV). The
condition gradually destroys the immune
system, which makes it harder for the body to
fight off infections
References

REFERENCES:
Barre-Sinoussi, F., Chermann, J.C., Rey, F., Nugeyre,
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M.T.., Chamaret, S., Gruest, J., Dauguet, C. Isolation of a T-lymphotropic retrovirus from a patient at risk for acquired
immune deficiency syndrome (AIDS). Science 220:868-871.
Popovic, M., Sarngahran, M.G., Read, E., Gallo, R. 1984. Detection, isolation, and continuos production of
cytopathic retroviruses from patients with AIDS and pre- AIDS. Science 224:497-500.
Gaines, H., von Sydow, M.A., von Stedingk, L.V. 1990.
Immunological changes in primary HIV-1 infection. AIDS 4:995-999
Daar, E.S.,Moudgil, T, Meyer.R.D., H. O., D.D.1991
Transient levels of viremia in patient with primary human immunodeficiency virus type 1 infection. New England Journal of
Medecine 324:954 960.
Piatak, M. Jr., Saag, M.S., Yang, L.C., Clark, S.J.,
Kappes, J.C.,Luk, K.C.,1993 High levels of HIV-1 in plasma during all stages of infection determined by competitive PCR.
Science 259:1749-1754.
Mulder, J., Mckinney, N., Christopherson, C., Sninsky,
Greenfield,L.,Kwok, S 1994. Rapid and simple PCR assay for quantitation of human immunodeficiency virus type 1 RNA in
plasma: Application to acute retroviral infection. Journal of Clinical Microbiology 32:292-300.
van Gemen., B., Kievits, T., Schukkink, R., van Strijp,
D., Malek, L.T., Sooknanan, R., Huisman, H.G., Lens,
P. 1993. Quantification of HIV-1 RNA in plasma using
NASBA during HIV-1 primary infection. Journal of Virological Methods 43:177-187.
Holmes, H., Davis, C., C., Heath, A., Hewlett, I and
N. 2001. An international collaborative study to establish the 1st international standard for HIV-1 RNA for use in nucleic acidbased techniques. Journal of Virological Methods 92:141-150.