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The role of the clinical laboratory
in diagnosis of HIV infection
By
Dr Ayman A Allam
Prof of Medical Microbiology and Immunology
Faculty of Medicine
Zagazig University
Human Immunodeficiency Virus
•Acquired Immunodeficiency syndrome
first described in 1981
•HIV-1 isolated in 1984 by Luc Montanier
(Pasteur Institute) and HIV-2 in 1986
•Belong to the lentivirus subfamily of the
retroviridae
•Enveloped RNA virus, 120nm in
diameter
Human Immunodeficiency Virus
• RNA retrovirus
• HIV-2 shares 40% nucleotide
homology with HIV-1
• three sub-groups of HIV-1, M (main
or major), N (new) and O (outlier).
• Within Group M: A to J subtypes
HIV
HIV
KEY VIRAL ENZYMES
• Reverse transcriptase
• Integrase
• Protease
6
The Genome of HIVThe Genome of HIV
Three structural genes
LTRs
Extra open reading frames are clue to latency
These ORFs code for small proteins - antibodies in AIDS
patients
HIV
The role of Laboratory
• Initial diagnosis of HIV
1) Screening tests 2) confirmatory tests
• Follow up of patients
1.CD4 count (immune reconstitution )
2.Viral load (viral replication)
3.Virus drug resistance tests
4.HLA-B*5701 testing before use of abacavir in tt
5.viral tropism testing in the case of maraviroc.
6.Other tests to detect the complications of the
disease
Initial diagnosis of HIV
• Screening tests
1.Rapid tests (point of care tests)
2.ELISA
• Confirmatory tests
1.Western blot
2.Nucleic acid amplification tests
Qualitative TMA (FDA approved)
Quantitative tests as Real Time- PCR
The window period
• The time between when a person may have been
exposed to HIV and when a test can tell for sure
whether He has HIV infection
• The window period varies :
(1) the genetics of the virus
(2) the genetics and immunocompetence of the host
(3) The assay (detects antigen, antibodies , RNA)
(4)the specimen type, such as oral fluid, venous or
capillary whole blood and serum/plasma.
• For a period of about 10 days following HIV
infection, no currently available serological or
virological assay can detect any marker of HIV
infection.
The window period
• A nucleic acid test (NAT):10 to 33 days after
an exposure.
• Antibody tests: 23 to 90 days to reliably
detect HIV infection
• Antigen/antibody test: 10 to 45 days after an
exposure
• Rapid Antigen/antibody test : 18 to 90 days
after an exposure
Window period
Screening tests
1- Premarital examination
2- Blood Donors.
3-Antenatal Care
4- Pre-employment screening
5- Before Surgical operations (Medico-legal)
6- Follow up for hemodialysis patients.
7- IV Drug abuse
8-prisoners
9-homosexuals
Rapid HIV-
1/2 antibody-
based tests
performed at the
point of care
(POC) are
becoming the
global standard
for HIV testing,
particularly in
the developing
world
Rapid tests (point of care tests)
• Rapid (point-of-care) give results in less than 20-30
minutes.
• Rapid testing is the method of choice when
immediate information is necessary to determine
the need for prophylaxis:
in the labor/delivery
post-exposure settings
When the person who is being tested is unlikely
to return for a follow-up visit.
Rapid tests
CLIA-waived tests: performed on whole blood
or oral fluid
• The OraQuick Advance
• Uni-Gold Recombigen assays
Moderate complexity: performed on serum or
plasma
• The Reveal G2
• Multispot assays
Rapid tests (point of care tests)
OraQuick rapid test
• OraQuick is a home
HIV test approved by
the United States
Food and Drug Administration
in 2012
• Sample is oral mucosa
transudate
• It can detect reactive
patients after 14 days of
infection
oral fluid sample
Step 1 – Collect sample.
Step 2 - Insert the device
into the buffer.
Step 3 - Read between 20
and 40 minutes.
Non-
Reactive
Preliminary Positive
OraQuick rapid test
Step 1 - Collect
sample.
Step 2- Mix sample
in buffer.
Step 3: Insert the device
into the buffer.
Step 4 - Read between
20 and 40 minutes.
Preliminary Positive
Alere Determine HIV-1/2 Ag/Ab
Combo test
U.S. Food and Drug Administration approved the
Alere Determine HIV-1/2 Ag/Ab Combo test on
August 9, 2013,
• Add sample---buffer---read result in 20 min.
Multispot rapid assays
Rapid tests: False positives
False positives are possible:
• hepatitis A virus (HAV)
• hepatitis B virus (HBV) infections
• rheumatoid factor
• Epstein-Barr virus infection
• in multiparous women.
Rapid tests: False negative
• Before seroconversion
• The adaptive immune response may decline after HIV
acquisition, leading to lower levels of specific gp41 HIV
antibodies.
• false-negative test results may be more common for oral
fluid specimens
• Infection with HIV-1 group O or HIV-2.
• Concurrent acute hepatitis C
• Delayed antibody synthesis in infants and persons receiving
post-exposure prophylaxis
• Diminished immune response in individuals receiving
intensive or long-term immunosuppressive therapy
ELISA
ELISA for HIV antibody
Microplate ELISA for HIV antibody: coloured wells indicate
reactivity
ELISA
ELISA fully automated
• Fully Automated ELISA machines (dilution,
pipetting, washing, incubation and reading)
fourth generation serological
assays
• fourth generation serological assays are the
first-line assay in blood screening.
• Antibody tests are typically positive no sooner
than 2 weeks after exposure, but
seroconversion may take as long as several
months.
• Thus, testing algorithms for exposed patients
include baseline serology with repeat testing at
1, 3, and 6 months post exposure.
ELISA
False positive:
• Epstein-Barr virus
• Influenza vaccination
• Pregnancy
• Receipt of immune globulin
• Autoimmune disease
False negative:
• Before seroconversion
• Using kit not detectiong HIV2 or group O HIV1
Testing algorithm
Confirmatory test
Western blot / line probe assay
Western blot
It detects specific antibodies to specific viral antigens:
1.gp 160 - precursor of ENV glycoprotein
2.gp 120 - outer ENV glycoprotein
3.p66 - reverse transcriptase component of POL
translate
4.p55 - precursor of GAG proteins
5.gp 41 - transmembrane ENV glycoprotein
6.p31 - endonuclease component of POL translate
7.p24 - GAG protein
8.p17 - GAG protein
Western blot
Positive : Any two or more of the bands : p24, gp41 and
gp120/160.
Negative: No bands present
Indeterminate: Any bands present but pattern does not meet
criteria for positive
Indeterminate western blot
Probable True Positive (HIV Infection)
• Sero-converting
• HIV-2 infection
• Technical errors
Probable True Negative (No HIV Infection)
• Recipients of HIV-1 trial vaccine
o Multiparous women
o Polytransfused patients
o Patients receiving chronic hemodialysis
o Patients with autoimmune disease
• Recipients of influenza and hepatitis B virus vaccines
• Persons with non-HIV acute viral infections
• Congenital bleeding disorders
• Alcoholic hepatitis and other chronic liver diseases
• Hematologic malignancies, lymphomas
Nucleic acid amplification tests for
HIV
1) Qualitative
• HIV-1 RNA TMA
• FDA-approved as a confirmation test
• 3-5 days for results
2) Quantitative (viral load test): Not FDA-approved
as a confirmation test
I. HIV-1 RNA, Real-time PCR
II.Quantiplex bDNA or branched DNA test
III.NASBA
• Gen-Probe's (Aptima) HIV-1 RNA qualitative assay is the only
molecular assay that has been approved by the FDA for diagnosis of
acute infection and as a confirmatory test for detection of HIV-1 in
samples that test reactive for HIV-1 antibodies
Real time PCR
•Viral load is a quantitative
measure of viral RNA genomes in
the peripheral circulation.
•Standard assays have a
lower limit of detection of
400 copies/mL
•ultrasensitive assays have
lower limit of detection of 50
copies/mL
•An optimal response to
treatment would be a reduction in
the viral load to undetectable
levels within 6 months
•false-positive quantitative
RNA viral load tests can
occur at counts under
1000/mL.
Nucleic Acid Sequence-Based-
Amplification (NASBA)
Other viral load tests
• ExaVir Load Version 2 : An inexpensive HIV
viral load assay measures viral RT activity
• The test is performed mostly manually
• Was designed primarily for resource-limited
settings.
• The assay has a lower limit of detection of 400
copies/mL
• It is not approved by the FDA for clinical use in
the United States.
Dignosis of HIV infection in the
neonate
• The use of proviral DNA PCR
• Initial testing should be performed as soon as
possible after birth, and because transmission
typically occurs at the time of delivery
• Optimally, exclusion of infection requires at
least 2 further negative DNA PCR tests, one
at 1 month of age and a second at 4 months.
• Serology is done after 18 months of age.
Viral culture
• Viral culture is possible but is labor intensive,
requires specialist laboratory equipment and
training (biosafety level 3 containment
facilities)
• may take several days to weeks to get results.
• It has no place in routine clinical diagnostics.
CD4 count
• CD4+
T cells can be
readily measured by
flow cytometry,
using specific
antibodies that label
CD4 as well as other
T cell markers such
as CD3.
CD4 counts
• A count below 200 cells/mL has been
associated in many studies with an increase in
the relative risk of opportunistic infections
• Many recent studies of treatment initiation at
various CD4+
T-cell counts have shown that
patients who start treatment when their count
drops below 350/mL experience less morbidity
and mortality than those who wait until their
count drops below 200/mL.
Drug Resistance Tests
1. Genotypic methods
2. Phenotypic methods
3. Virtual phenotype
Genotypic resistance assay
• Testing analyzes the genes of the virus to detect
the presence of one or more mutations that are
associated with antiretroviral drug (ART)
resistance.
• Two direct sequencing-based methods have been
approved by the FDA:
The TruGene HIV-1 Genotyping assay (Siemens)
The ViroSeq HIV-1 Genotyping System (Celera
Diagnostics).
Phenotyping resistance assay
• A phenotypic assay provides a direct measure
of drug resistance.
• These assays use recombinant DNA methods
to measure the ability of a patient’s virus to
grow in the presence of a drug.
• The results from a phenotypic test include the
net effect of any and all resistance mutations.
Phenotypic resistance assay
• PhenoSense
HIV can
predict
emergence of
resistance
• It directly
measures the
susceptibility
of a patient's
virus to reverse
transcriptase
inhibitors and
protease
inhibitors
VIRTUAL PHENOTYPE
• This test is really a method of interpreting
genotypic test results.
• First, genotypic testing is done on the sample.
• Phenotypic test results for other virus samples
with a similar genotypic pattern are taken from
a database.
• These matched samples tell you how the virus
is likely to behave.
• The virtual phenotype is faster and less
expensive than a phenotypic test.
Co receptor tropism assay
• It determines types of co-receptor (CCR5 OR
CXCR4) tropism of the virus.
• Maraviroc is active only in CCR5 phenotype
I. Phenotypic Assays : as Trofile assay 2 weeks
II.Genotypic Assays : rapid 2-3d
is based on sequencing of the V3-coding
region of HIV-1 env, the principal determinant
of co-receptor usage.
summary
• The most recommended alogarithm for
diagnosis of HIV is screening by 4th
generation
ELISA followed by confirmation by Western
blot or Transcription Mediated amplification.
• No alogarithm can fit for every scenario.
Physicians should allow for individual
circumstances and unique situations
summary
• Rapid HIV-1/2 antibody-based tests are
becoming the global standard for HIV
testing, particularly in the developing world.
• For a period of about 10 days following HIV
infection, no currently available serological
or virological assay can detect any marker
of HIV infection.
THANK YOU

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The role of the clinical lab in diagnosis of hiv

  • 1. The role of the clinical laboratory in diagnosis of HIV infection By Dr Ayman A Allam Prof of Medical Microbiology and Immunology Faculty of Medicine Zagazig University
  • 2. Human Immunodeficiency Virus •Acquired Immunodeficiency syndrome first described in 1981 •HIV-1 isolated in 1984 by Luc Montanier (Pasteur Institute) and HIV-2 in 1986 •Belong to the lentivirus subfamily of the retroviridae •Enveloped RNA virus, 120nm in diameter
  • 3. Human Immunodeficiency Virus • RNA retrovirus • HIV-2 shares 40% nucleotide homology with HIV-1 • three sub-groups of HIV-1, M (main or major), N (new) and O (outlier). • Within Group M: A to J subtypes
  • 4. HIV
  • 5. HIV KEY VIRAL ENZYMES • Reverse transcriptase • Integrase • Protease
  • 6. 6 The Genome of HIVThe Genome of HIV Three structural genes LTRs Extra open reading frames are clue to latency These ORFs code for small proteins - antibodies in AIDS patients
  • 7. HIV
  • 8. The role of Laboratory • Initial diagnosis of HIV 1) Screening tests 2) confirmatory tests • Follow up of patients 1.CD4 count (immune reconstitution ) 2.Viral load (viral replication) 3.Virus drug resistance tests 4.HLA-B*5701 testing before use of abacavir in tt 5.viral tropism testing in the case of maraviroc. 6.Other tests to detect the complications of the disease
  • 9. Initial diagnosis of HIV • Screening tests 1.Rapid tests (point of care tests) 2.ELISA • Confirmatory tests 1.Western blot 2.Nucleic acid amplification tests Qualitative TMA (FDA approved) Quantitative tests as Real Time- PCR
  • 10. The window period • The time between when a person may have been exposed to HIV and when a test can tell for sure whether He has HIV infection • The window period varies : (1) the genetics of the virus (2) the genetics and immunocompetence of the host (3) The assay (detects antigen, antibodies , RNA) (4)the specimen type, such as oral fluid, venous or capillary whole blood and serum/plasma. • For a period of about 10 days following HIV infection, no currently available serological or virological assay can detect any marker of HIV infection.
  • 11. The window period • A nucleic acid test (NAT):10 to 33 days after an exposure. • Antibody tests: 23 to 90 days to reliably detect HIV infection • Antigen/antibody test: 10 to 45 days after an exposure • Rapid Antigen/antibody test : 18 to 90 days after an exposure
  • 13. Screening tests 1- Premarital examination 2- Blood Donors. 3-Antenatal Care 4- Pre-employment screening 5- Before Surgical operations (Medico-legal) 6- Follow up for hemodialysis patients. 7- IV Drug abuse 8-prisoners 9-homosexuals
  • 14. Rapid HIV- 1/2 antibody- based tests performed at the point of care (POC) are becoming the global standard for HIV testing, particularly in the developing world
  • 15. Rapid tests (point of care tests) • Rapid (point-of-care) give results in less than 20-30 minutes. • Rapid testing is the method of choice when immediate information is necessary to determine the need for prophylaxis: in the labor/delivery post-exposure settings When the person who is being tested is unlikely to return for a follow-up visit.
  • 16. Rapid tests CLIA-waived tests: performed on whole blood or oral fluid • The OraQuick Advance • Uni-Gold Recombigen assays Moderate complexity: performed on serum or plasma • The Reveal G2 • Multispot assays
  • 17. Rapid tests (point of care tests)
  • 18. OraQuick rapid test • OraQuick is a home HIV test approved by the United States Food and Drug Administration in 2012 • Sample is oral mucosa transudate • It can detect reactive patients after 14 days of infection
  • 19. oral fluid sample Step 1 – Collect sample. Step 2 - Insert the device into the buffer. Step 3 - Read between 20 and 40 minutes. Non- Reactive Preliminary Positive
  • 20. OraQuick rapid test Step 1 - Collect sample. Step 2- Mix sample in buffer. Step 3: Insert the device into the buffer. Step 4 - Read between 20 and 40 minutes. Preliminary Positive
  • 21. Alere Determine HIV-1/2 Ag/Ab Combo test U.S. Food and Drug Administration approved the Alere Determine HIV-1/2 Ag/Ab Combo test on August 9, 2013, • Add sample---buffer---read result in 20 min.
  • 23.
  • 24.
  • 25.
  • 26. Rapid tests: False positives False positives are possible: • hepatitis A virus (HAV) • hepatitis B virus (HBV) infections • rheumatoid factor • Epstein-Barr virus infection • in multiparous women.
  • 27. Rapid tests: False negative • Before seroconversion • The adaptive immune response may decline after HIV acquisition, leading to lower levels of specific gp41 HIV antibodies. • false-negative test results may be more common for oral fluid specimens • Infection with HIV-1 group O or HIV-2. • Concurrent acute hepatitis C • Delayed antibody synthesis in infants and persons receiving post-exposure prophylaxis • Diminished immune response in individuals receiving intensive or long-term immunosuppressive therapy
  • 28. ELISA
  • 29. ELISA for HIV antibody Microplate ELISA for HIV antibody: coloured wells indicate reactivity
  • 30. ELISA
  • 31. ELISA fully automated • Fully Automated ELISA machines (dilution, pipetting, washing, incubation and reading)
  • 32. fourth generation serological assays • fourth generation serological assays are the first-line assay in blood screening. • Antibody tests are typically positive no sooner than 2 weeks after exposure, but seroconversion may take as long as several months. • Thus, testing algorithms for exposed patients include baseline serology with repeat testing at 1, 3, and 6 months post exposure.
  • 33. ELISA False positive: • Epstein-Barr virus • Influenza vaccination • Pregnancy • Receipt of immune globulin • Autoimmune disease False negative: • Before seroconversion • Using kit not detectiong HIV2 or group O HIV1
  • 35. Confirmatory test Western blot / line probe assay
  • 36. Western blot It detects specific antibodies to specific viral antigens: 1.gp 160 - precursor of ENV glycoprotein 2.gp 120 - outer ENV glycoprotein 3.p66 - reverse transcriptase component of POL translate 4.p55 - precursor of GAG proteins 5.gp 41 - transmembrane ENV glycoprotein 6.p31 - endonuclease component of POL translate 7.p24 - GAG protein 8.p17 - GAG protein
  • 37. Western blot Positive : Any two or more of the bands : p24, gp41 and gp120/160. Negative: No bands present Indeterminate: Any bands present but pattern does not meet criteria for positive
  • 38. Indeterminate western blot Probable True Positive (HIV Infection) • Sero-converting • HIV-2 infection • Technical errors Probable True Negative (No HIV Infection) • Recipients of HIV-1 trial vaccine o Multiparous women o Polytransfused patients o Patients receiving chronic hemodialysis o Patients with autoimmune disease • Recipients of influenza and hepatitis B virus vaccines • Persons with non-HIV acute viral infections • Congenital bleeding disorders • Alcoholic hepatitis and other chronic liver diseases • Hematologic malignancies, lymphomas
  • 39. Nucleic acid amplification tests for HIV 1) Qualitative • HIV-1 RNA TMA • FDA-approved as a confirmation test • 3-5 days for results 2) Quantitative (viral load test): Not FDA-approved as a confirmation test I. HIV-1 RNA, Real-time PCR II.Quantiplex bDNA or branched DNA test III.NASBA
  • 40. • Gen-Probe's (Aptima) HIV-1 RNA qualitative assay is the only molecular assay that has been approved by the FDA for diagnosis of acute infection and as a confirmatory test for detection of HIV-1 in samples that test reactive for HIV-1 antibodies
  • 41. Real time PCR •Viral load is a quantitative measure of viral RNA genomes in the peripheral circulation. •Standard assays have a lower limit of detection of 400 copies/mL •ultrasensitive assays have lower limit of detection of 50 copies/mL •An optimal response to treatment would be a reduction in the viral load to undetectable levels within 6 months •false-positive quantitative RNA viral load tests can occur at counts under 1000/mL.
  • 43. Other viral load tests • ExaVir Load Version 2 : An inexpensive HIV viral load assay measures viral RT activity • The test is performed mostly manually • Was designed primarily for resource-limited settings. • The assay has a lower limit of detection of 400 copies/mL • It is not approved by the FDA for clinical use in the United States.
  • 44. Dignosis of HIV infection in the neonate • The use of proviral DNA PCR • Initial testing should be performed as soon as possible after birth, and because transmission typically occurs at the time of delivery • Optimally, exclusion of infection requires at least 2 further negative DNA PCR tests, one at 1 month of age and a second at 4 months. • Serology is done after 18 months of age.
  • 45. Viral culture • Viral culture is possible but is labor intensive, requires specialist laboratory equipment and training (biosafety level 3 containment facilities) • may take several days to weeks to get results. • It has no place in routine clinical diagnostics.
  • 46. CD4 count • CD4+ T cells can be readily measured by flow cytometry, using specific antibodies that label CD4 as well as other T cell markers such as CD3.
  • 47. CD4 counts • A count below 200 cells/mL has been associated in many studies with an increase in the relative risk of opportunistic infections • Many recent studies of treatment initiation at various CD4+ T-cell counts have shown that patients who start treatment when their count drops below 350/mL experience less morbidity and mortality than those who wait until their count drops below 200/mL.
  • 48. Drug Resistance Tests 1. Genotypic methods 2. Phenotypic methods 3. Virtual phenotype
  • 49. Genotypic resistance assay • Testing analyzes the genes of the virus to detect the presence of one or more mutations that are associated with antiretroviral drug (ART) resistance. • Two direct sequencing-based methods have been approved by the FDA: The TruGene HIV-1 Genotyping assay (Siemens) The ViroSeq HIV-1 Genotyping System (Celera Diagnostics).
  • 50. Phenotyping resistance assay • A phenotypic assay provides a direct measure of drug resistance. • These assays use recombinant DNA methods to measure the ability of a patient’s virus to grow in the presence of a drug. • The results from a phenotypic test include the net effect of any and all resistance mutations.
  • 51. Phenotypic resistance assay • PhenoSense HIV can predict emergence of resistance • It directly measures the susceptibility of a patient's virus to reverse transcriptase inhibitors and protease inhibitors
  • 52. VIRTUAL PHENOTYPE • This test is really a method of interpreting genotypic test results. • First, genotypic testing is done on the sample. • Phenotypic test results for other virus samples with a similar genotypic pattern are taken from a database. • These matched samples tell you how the virus is likely to behave. • The virtual phenotype is faster and less expensive than a phenotypic test.
  • 53. Co receptor tropism assay • It determines types of co-receptor (CCR5 OR CXCR4) tropism of the virus. • Maraviroc is active only in CCR5 phenotype I. Phenotypic Assays : as Trofile assay 2 weeks II.Genotypic Assays : rapid 2-3d is based on sequencing of the V3-coding region of HIV-1 env, the principal determinant of co-receptor usage.
  • 54. summary • The most recommended alogarithm for diagnosis of HIV is screening by 4th generation ELISA followed by confirmation by Western blot or Transcription Mediated amplification. • No alogarithm can fit for every scenario. Physicians should allow for individual circumstances and unique situations
  • 55. summary • Rapid HIV-1/2 antibody-based tests are becoming the global standard for HIV testing, particularly in the developing world. • For a period of about 10 days following HIV infection, no currently available serological or virological assay can detect any marker of HIV infection.

Notas del editor

  1. The size of the HIV genome is similar to that of other retroviruses but it is more complex. There is no oncogene but there are extra open reading frames which do code for protein. In all 15 proteins are encoded in HIV and they are made because antibodies to them can be found in patients. These extra open reading frames are not typical of retroviruses such as RSV. These extra open reading frames give a clue to the complex lifestyle of HIV. Note that some of them are encoded in two or more exons so there will have to be multiple splice events to make the final RNA. Could these be a site for intervention in the replication of the virus?