2. Disclosure of Financial Relationships This speaker has the following financial relationships with commercial entities to disclose:
Speaker’s Bureau - Pfizer Use this slide if you have no significant financial relationships with any commercial entities.
If you use this slide, please delete slide 3.Use this slide if you have no significant financial relationships with any commercial entities.
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3. Course Objectives At the conclusion of this conference, the participant will be able to:
Understand basic principles of virus growth and evolution
Appreciate advantages and limitations of different types of resistance tests
Recognize the effect of specific mutation patterns on drug susceptibility
Interpret reports from various resistance tests
4. Course Objectives, cont.
Evaluate the possible uses for resistance testing in patient management
Compare the advantages and disadvantages of each type of test
Understand supporting clinical data relevant to RT usage
5. Resistance Definition Resistance refers to the reduced susceptibility of a patient’s viral isolate to suppression by an antiviral drug
This is a relative phenomenon, dependent on the levels of drug that are achieved and host factors
6. Increase in HIV Drug Resistance Mutations
7. Viral Resistance is the Outcome of Viral Replication, Mutations and Selection Pressure
9. Guidelines: Treatment-Naive Patients
10. HIV Drug Resistance Broadly defined as any change that improves viral replication in the presence of an antiretroviral (ARV) drug
Measured by
Genotype
Phenotype
VircoTYPE
Clinical/Virologic response HIV resistance is broadly defined as any change that improves viral replication in the presence of an antiretroviral drug
Changes are due to an altered phenotype resulting from a change in the genotype, or in other words, a change in the sequence of the virus. Such changes occur primarily in the reverse transcriptase and protease genes. Changes in the virus are usually compared against a wild-type virus, a virus that does not have any drug-associated mutations. HIV resistance is rarely absolute; rather, the susceptibility of the virus for a particular drug or combination of drugs is reduced but not complete
Resistance can be measured in a test tube (in vitro) using laboratory virus strains with or without HIV drug-associated mutations, or it can be measured in a subject (in vivo) by obtaining a blood sample containing virus and doing a resistance testHIV resistance is broadly defined as any change that improves viral replication in the presence of an antiretroviral drug
Changes are due to an altered phenotype resulting from a change in the genotype, or in other words, a change in the sequence of the virus. Such changes occur primarily in the reverse transcriptase and protease genes. Changes in the virus are usually compared against a wild-type virus, a virus that does not have any drug-associated mutations. HIV resistance is rarely absolute; rather, the susceptibility of the virus for a particular drug or combination of drugs is reduced but not complete
Resistance can be measured in a test tube (in vitro) using laboratory virus strains with or without HIV drug-associated mutations, or it can be measured in a subject (in vivo) by obtaining a blood sample containing virus and doing a resistance test
11. Genotype Refers to the sequence of bases (A,C,T,G) coding for amino acids that comprise viral proteins
Typically expressed as the coded amino acid and position (eg, M184)
If mutated, the change is indicated after the position (eg, M184V)
12. HIV Resistance and Mutation Definitions Primary mutations are selected early and usually decrease drug susceptibility
Secondary mutations are selected after primary mutations and may have a limited effect on drug susceptibility
Multidrug resistance mutations can contribute to resistance or decreased susceptibility to many or all drugs in a single class
Changes are due to a change in the sequence of the virus
Resistance can be measured either in vitro or in vivo
After primary mutations are detected, they are studied in vitro to determine if they confer drug resistance
If secondary mutations alone are studied in the laboratory, drug resistance will not be observed
A few known mutations confer drug resistance to the entire class of reverse transcriptase inhibitors or protease inhibitors
Changes are due to a change in the sequence of the virus
Resistance can be measured either in vitro or in vivo
After primary mutations are detected, they are studied in vitro to determine if they confer drug resistance
If secondary mutations alone are studied in the laboratory, drug resistance will not be observed
A few known mutations confer drug resistance to the entire class of reverse transcriptase inhibitors or protease inhibitors
13. Anonymous questionnaire at a meeting in 2001 128/421 providers, 100 had used resistance testing�List of 16 resistance associated point mutations
14. Knowledge of Specific Mutations
15. Overview of Current HIV Resistance Testing Technologies Genotypic testing
Capillary sequencing (ABI) or other dideoxy method
High level of concordance between two commercial assay kits when performed by the same laboratory
Results interpreted by individual judgment or computerized rules-based algorithms
Variation can be seen between algorithms in classification of expected drug activity
Requires regular updating
Still must interpret meaning of report with regard to regimen selection
16. Interpretation of Genotypic Assays Expert advice (common in Europe)
May not be available
Experts’ views may be inconsistent
Rules-based algorithms (Bayer/VGI, others)
Provided by most labs, third-party sites
Need regular updating
vircoTYPE HIV-1 (Virco)
Database of matched genotypes and phenotypes
17. Genotypic Assays More rapid results (days)
Less technically complex
Proven value in predicting�short-term virologic outcome
Mutations may precede phenotypic resistance
Less expensive than phenotype
Genotypic correlates of resistance increasingly well-defined Indirect measure of resistance
May not correlate with phenotype
Requires viral load > 1000 copies/mL
May not detect minor species
Interpretation required
Cannot assess interactions between mutations
18. Genotype Examples
21. Defining Genotypic Determinants of Amprenavir Resistance
22. Overview of Current HIV Resistance Testing Technologies Standard phenotypic testing
Results usually expressed as fold-change in susceptibility compared to a laboratory control isolate
Interpretation of drug activity dependent on methodology used to define cutoffs (technical, biologic, clinical)
Virtual phenotype testing
Matches genotypic data against database of virus samples with paired GT and PT data
Confidence level based on number of matching genotypes within the database
23. Phenotype Phenotype refers to the growth characteristics of the virus in vitro, which is largely determined by genotype
Analogous to tube dilution bacterial sensitivity testing.
Remember, cellular factors may modify the effect of phenotype in vivo.
24. Phenotypic Susceptibility: Relationship�Between Drug Concentration and Viral Inhibition
25. Phenotypic Susceptibility: Relationship�Between Drug Concentration and Viral Inhibition
26. Interpretation of Phenotypic Assays Results reported as
IC50 of patient virus vs IC50 of wild-type virus
Fold-change (FC) from IC50 of wild-type virus
Individual results provided for each drug
Thresholds to define reduced susceptibility
Biologic cut-off
Based on biologic variations
in treatment-naive patients
Usually 2 SD above median
Clinical cut-off
Based on patient virologic
response, compared with
suboptimal or non-response
27. Phenotypic Assays Direct measure of resistance
Results simple to understand (eg, IC50)
Can be used for any drug without requiring knowledge of genotypic correlates of resistance
Assesses impact of interactions between mutations Less rapid results (weeks)
Results too simple to understand?
Thresholds for resistance not fully defined for all drugs
Does not take into account activity of drugs in combination
Require HIV RNA > 500-1000
May not reflect minor species
More expensive than genotype
28. Viral Fitness NRTI-resistant viruses may display impaired viral fitness
Impaired fitness = ? replication efficiency, ? growth
Impairment can be caused by single mutations
Particularly M184V, L74V and K65R
Specific combinations of NRTI-resistance mutations can have additive effects on viral fitness
Virus containing both M184V and K65R is “less fit” than virus with either mutation alone
Secondary PI resistance mutations and cleavage site mutations may improve viral fitness in viruses with primary PI mutations Ed: The text refers to a figure 2. Do we have this?
Also, wasn’t sure where to fit this in the order of the slides.
Ed: The text refers to a figure 2. Do we have this?
Also, wasn’t sure where to fit this in the order of the slides.
29. Phenotype Examples
30. Drug Susceptibility Reports
31. HIV phenotype from >1000 drug naďve patients
Samples from N America, Europe & S Africa
Mean & standard deviation values were derived for each data set
For each drug, the cut-off was set at 2 standard deviations above the mean
97.5% samples Within normal susceptible range
2.5% samples Above normal susceptible range Re-defining Phenotypic Cut-Offs Based on Biological Variation
32. Fold-change IC50 associated with treatment-dependent viral load change, more relevant
Difficult to ascertain since treatment with 3-5 drugs, effect of single drugs not measured
Probably will be able to modify cutoff values determined by biologic variability based on virologic change with therapy of resistant virus strains
Re-defining Phenotypic Cut-Offs Based on Clinical Response
33. Phenotype/Genotype Discordance
34. Genotypic Resistance Interpretation Concordance: ANRS, HIVDB, Rega, VGI
35. Which resistance test and when?
38. NRTI Drug Resistance Pathways TAMs – 215, 41, 210, 67, 70, 219
Decrease susceptibility to all NRTIs, unblocking mechanism
Alternate pathway – 65, 74
Abacavir, tenofovir, didanosine, (3TC)
Hypersusceptibility to ZDV, sensitive to d4T
M184V – mixed effects
High level 3TC resistance, can affect abacavir
Increased susceptibility to AZT, d4T, TDF
Diminishes viral fitness
39. Multinucleoside and Nucleotide Resistance Multinucleoside resistance is typically associated with high level resistance to most nucleosides:
Q151M complex (TDF susceptibility preserved)
serine insertions - 69S(S,S)
multiple NAMS, especially with 184V
K65R – only ZDV reliably active; some d4T/TDF/ABC activity possible, but reduced
Tenofovir resistance: K65R, 41/210/215Y, but may retain phenotypic (and clinical) activity
40. Non-Nucleoside RTI Resistance Mutations 2 clusters around
K103
Y181
98/101/106/108/188/190 also important
K103N is dominant, associated with class cross-resistance by itself
Y181C may be seen without 103N although some efavirenz in vitro activity, not clinically durable
Non-clade B, 106 mutations may be primary
41. Protease Inhibitor Resistance Mutations
42. Mutations Selected by PIs Many mutations in the protease gene, as shown in this recent representation,1 confer significant cross-resistance across the entire class. The mutations highlighted in yellow generally develop in patients who receive the individual PIs for the first time with or without nucleosides.
Indinavir—46 and 82
Ritonavir—84 and 82
Saquinavir—48 and 90
Nelfinavir—30 and 90, occasionally 88
Amprenavir—50, 54, and 84
Lopinavir/ritonavir—It is unclear which mutation develops first in patients, but the mutations shown all contribute to lopinavir resistance, based on phenotypic and genotypic analyses of clinical isolates. It has been suggested that as few as 4 mutations may be associated with high-level resistance to lopinavir/ritonavir. Although L63P causes no appreciable increase in IC50, it is shown for only lopinavir/ritonavir because, along with other mutations, it predicts a lack of viral load response to regimens containing this agent.Many mutations in the protease gene, as shown in this recent representation,1 confer significant cross-resistance across the entire class. The mutations highlighted in yellow generally develop in patients who receive the individual PIs for the first time with or without nucleosides.
Indinavir—46 and 82
Ritonavir—84 and 82
Saquinavir—48 and 90
Nelfinavir—30 and 90, occasionally 88
Amprenavir—50, 54, and 84
Lopinavir/ritonavir—It is unclear which mutation develops first in patients, but the mutations shown all contribute to lopinavir resistance, based on phenotypic and genotypic analyses of clinical isolates. It has been suggested that as few as 4 mutations may be associated with high-level resistance to lopinavir/ritonavir. Although L63P causes no appreciable increase in IC50, it is shown for only lopinavir/ritonavir because, along with other mutations, it predicts a lack of viral load response to regimens containing this agent.
43. Mutations Selected by PIs (cont) Many mutations in the protease gene, as shown in this recent representation,1 confer significant cross-resistance across the entire class. The mutations highlighted in yellow generally develop in patients who receive the individual PIs for the first time with or without nucleosides.
Indinavir—46 and 82
Ritonavir—84 and 82
Saquinavir—48 and 90
Nelfinavir—30 and 90, occasionally 88
Amprenavir—50, 54, and 84
Lopinavir/ritonavir—It is unclear which mutation develops first in patients, but the mutations shown all contribute to lopinavir resistance, based on phenotypic and genotypic analyses of clinical isolates. It has been suggested that as few as 4 mutations may be associated with high-level resistance to lopinavir/ritonavir. Although L63P causes no appreciable increase in IC50, it is shown for only lopinavir/ritonavir because, along with other mutations, it predicts a lack of viral load response to regimens containing this agent.Many mutations in the protease gene, as shown in this recent representation,1 confer significant cross-resistance across the entire class. The mutations highlighted in yellow generally develop in patients who receive the individual PIs for the first time with or without nucleosides.
Indinavir—46 and 82
Ritonavir—84 and 82
Saquinavir—48 and 90
Nelfinavir—30 and 90, occasionally 88
Amprenavir—50, 54, and 84
Lopinavir/ritonavir—It is unclear which mutation develops first in patients, but the mutations shown all contribute to lopinavir resistance, based on phenotypic and genotypic analyses of clinical isolates. It has been suggested that as few as 4 mutations may be associated with high-level resistance to lopinavir/ritonavir. Although L63P causes no appreciable increase in IC50, it is shown for only lopinavir/ritonavir because, along with other mutations, it predicts a lack of viral load response to regimens containing this agent.
44. Mutations in the gp41 env associated with Resistance to enfuvirtide This slide summarizes NNRTI resistance patterns. There is a clustering of mutations between codons 100 and 106 and codons 181 and 190, with several others occurring in the low 200s. There is broad cross-resistance in these patterns, although subtle differences can be seen.1
This slide summarizes NNRTI resistance patterns. There is a clustering of mutations between codons 100 and 106 and codons 181 and 190, with several others occurring in the low 200s. There is broad cross-resistance in these patterns, although subtle differences can be seen.1
45. HIV Drug Resistance Testing
All Approaches have Strengths and Limitations:
Strong positive correlation with resistance or decreased virologic response when present
All commercial assays relatively insensitive
Lack of detection does not mean resistance is not present; resistance from previous regimens or exposure may not be detected Moving on to some additional definitions, primary mutations are those that are selected early and usually result in decreased drug susceptibility. For the most part, primary mutations are either discovered in vitro or discovered after the drug has been given to patients and virologic failure has ensued. After primary mutations are discovered in a patient, they are studied in vitro in order to determine if they do confer drug resistance
Secondary mutations are those that are selected after primary mutations have occurred. Secondary mutations likely have a very limited effect on drug susceptibility. In other words, if secondary mutations alone are studied in the laboratory, drug resistance will not be observed
Multi-drug resistance mutations often confer resistance or decreased susceptibility to many or all drugs in a single class. A few known mutations confer drug resistance to the entire reverse transcriptase inhibitor or protease inhibitor classMoving on to some additional definitions, primary mutations are those that are selected early and usually result in decreased drug susceptibility. For the most part, primary mutations are either discovered in vitro or discovered after the drug has been given to patients and virologic failure has ensued. After primary mutations are discovered in a patient, they are studied in vitro in order to determine if they do confer drug resistance
Secondary mutations are those that are selected after primary mutations have occurred. Secondary mutations likely have a very limited effect on drug susceptibility. In other words, if secondary mutations alone are studied in the laboratory, drug resistance will not be observed
Multi-drug resistance mutations often confer resistance or decreased susceptibility to many or all drugs in a single class. A few known mutations confer drug resistance to the entire reverse transcriptase inhibitor or protease inhibitor class
46. HIV Drug Resistance Testing
All Approaches have Strengths and Limitations:
Complex mutation patterns should be more readily interpreted by phenotype, but this has not been demonstrated in clinical trials
VirtualPhenotype offers sequence analysis and interpretation based on viral growth properties related to patient RT and protease Moving on to some additional definitions, primary mutations are those that are selected early and usually result in decreased drug susceptibility. For the most part, primary mutations are either discovered in vitro or discovered after the drug has been given to patients and virologic failure has ensued. After primary mutations are discovered in a patient, they are studied in vitro in order to determine if they do confer drug resistance
Secondary mutations are those that are selected after primary mutations have occurred. Secondary mutations likely have a very limited effect on drug susceptibility. In other words, if secondary mutations alone are studied in the laboratory, drug resistance will not be observed
Multi-drug resistance mutations often confer resistance or decreased susceptibility to many or all drugs in a single class. A few known mutations confer drug resistance to the entire reverse transcriptase inhibitor or protease inhibitor classMoving on to some additional definitions, primary mutations are those that are selected early and usually result in decreased drug susceptibility. For the most part, primary mutations are either discovered in vitro or discovered after the drug has been given to patients and virologic failure has ensued. After primary mutations are discovered in a patient, they are studied in vitro in order to determine if they do confer drug resistance
Secondary mutations are those that are selected after primary mutations have occurred. Secondary mutations likely have a very limited effect on drug susceptibility. In other words, if secondary mutations alone are studied in the laboratory, drug resistance will not be observed
Multi-drug resistance mutations often confer resistance or decreased susceptibility to many or all drugs in a single class. A few known mutations confer drug resistance to the entire reverse transcriptase inhibitor or protease inhibitor class
47. Part II��Resistance Testing�Clinical Applications
48. What is Treatment Failure?* True definition encompasses virologic, immunologic, and/or clinical status
Different types
First or second regimen:
Initial goal is an “undetectable” viral load
“Failure” therefore defined as
Inability to achieve a viral load below the limit of quantification
Any sustained return of virus to above the target level
49. Treatment Failure II* Multiple regimen failures:
Achieving an undetectable viral load may not be realistic
Goal is to prevent clinical progression
Deterioration of the CD4 count or
Occurrence of an OI
Lack of viable options suggest continuing the regimen in the face of on-going viral replication and presence of resistance
50. Causes of HIV Treatment Failure
51. Why Do We Need Antiretroviral Resistance Testing? To help clinicians make better treatment decisions
Before beginning antiretroviral therapy
Naive patients infected with resistant HIV
When to change a regimen
To help determine which drug(s) are not working
To decrease use of ineffective and/or potentially toxic drugs
In the setting of transmission
Vertical
After “accidental” exposure
To aid in the development of better treatment guidelines
To help pharmaceutical companies make better drugs
52. Antiretroviral Resistance Testing Is Part
of the Recommended STANDARD of CARE
in the Management of the
HIV-Infected Individual!1,2 References:
Panel on Clinical Practices for Treatment of HIV Infection for the Department of Health and Human Services and the Henry J Kaiser Family Foundation. Guidelines for the Use of Antiretroviral Agents in HIV-Infected Adults and Adolescents. Washington, DC: Department of Health and Human Services; February 4, 2002. Available at: http://www.aidsinfo.nih.gov/guidelines/adult/html_adult_02-04-02.html. Accessed February 23, 2002.
Yeni PG, Hammer SM, Carpenter CCJ, Cooper DA, Fischl MA, Gattell JM, et al. Antiretroviral Treatment for Adult HIV Infection in 2002: Updated Recommendations of the International AIDS Society-USA Panel. JAMA. July 10, 2002;288:222-252.References:
Panel on Clinical Practices for Treatment of HIV Infection for the Department of Health and Human Services and the Henry J Kaiser Family Foundation. Guidelines for the Use of Antiretroviral Agents in HIV-Infected Adults and Adolescents. Washington, DC: Department of Health and Human Services; February 4, 2002. Available at: http://www.aidsinfo.nih.gov/guidelines/adult/html_adult_02-04-02.html. Accessed February 23, 2002.
Yeni PG, Hammer SM, Carpenter CCJ, Cooper DA, Fischl MA, Gattell JM, et al. Antiretroviral Treatment for Adult HIV Infection in 2002: Updated Recommendations of the International AIDS Society-USA Panel. JAMA. July 10, 2002;288:222-252.
53. General Limitations and Caveats of Resistance Testing Current assays requires 500*–1000 viral copies to isolate sufficient nucleic acid to amplify
Insensitive to minor viral species
If drug-resistant viruses <10-20% of the circulating viral population, may not be detected by the assay
In the absence of drug pressure
Wild type virus will typically be preferentially expressed
Resistant clones will be “overgrown” and fade to undetectable
However, resistance is a genetic characteristic.
It is “archived” and can be re-expressed rapidly
* ViroLogic assays are validated at 500 copies/mL
54. Therefore, the absence of resistance does not necessarily indicate susceptibility!
55. Genotyping
56. Genotyping
57. Genotyping
58. Genotyping Advantages
Specifies the mutations in the HIV genome associated with resistance
Sensitive for detection of emerging resistance (mixtures)
May provide early warning signals to development of full resistance
More rapid and less expensive than a phenotype
Offered by many commercial laboratories
Limitations
Not a direct measure of viral resistance
Increasingly complex mutational patterns
Cannot predict interactions of mutations
Presupposes knowledge of critical mutations
Requires interpretation for prediction of resistance or susceptibility to drugs
Variations in available sequencing methodologies
No Clinical Cutoffs for genotype
59. Phenotyping
60. Phenotyping
61. Phenotyping Advantages
Direct measure of resistance—measures the ability of the patient’s virus to grow in different concentrations of drug in vitro: the gold standard
Accounts for net effect of any and all resistance mutations
Prediction of resistance or susceptibility already built-in and does not require external interpretation Limitations
Technically more complex than genotyping
More expensive
May longer turnaround time
Establishment of accurate fold-resistance cut-off values critical for prediction of response
Need for true “clinical cut-offs”
Only looks at individual drugs and not PK-enhanced PIs
63. VirtualPhenotype™ Advantages
Report provides both sequence data (GENOTYPE) and prediction of phenotype: “2-for-1” test
Assessment of drug resistance based on actual data from a growing set of samples with paired genotype/phenotype
Updated in real-time Limitations
Not a real phenotype
Strength of correlation depends on number of matches
Number of matches for new drugs may be limited
64. Combination Genotype/Phenotype Report
65. HIV-1 Drug Resistance Testing�Items To Consider Genotyping
Does the test cover all known mutations?
Are there any ‘gaps’ in the sequencing?
How often is the library/database updated?
What does the genotype tell the healthcare provider?
Can healthcare providers make a clinical judgment based on the report?
Phenotyping
Are drug-specific clinical cut-offs available for each drug?
Is the report easy to read?
66. Clinical Trials of �Antiretroviral Resistance Testing
67. Published Prospective Clinical Trials I* References:
Durant J, Clevenbergh P, Halfon P, et al. Drug-resistance genotyping in HIV-1 therapy: the VIRADAPT randomised controlled trial. Lancet. June 26, 1999;353(9171):2195-2199.
Baxter JD, Mayers DL, Wentworth DN, et al. A randomized study of antiretroviral management based on plasma genotypic antiretroviral resistance testing in patients failing therapy. AIDS. June 16, 2000;14(9):F83-F93.
Tural C, Ruiz L, Holtzer C, et al, and the Havana Study Group. Clinical utility of HIV-1 genotyping and expert advice: the Havana trial. AIDS. January 25, 2002;16(2):209-218.
Cingolani A, Antinori A, Rizzo MG, et al. Usefulness of monitoring HIV drug resistance and adherence in individuals failing highly active antiretroviral therapy: a randomized study (ARGENTA). AIDS. February 15, 2002;16(3):369-379.
Cohen CJ, Hunt S, Sension M, et al, and the VIRA3001 Study Team. A randomized trial assessing the impact of phenotypic resistance testing on antiretroviral therapy. AIDS. March 8, 2002;16(4):579-588.
Meynard JL, Vray M, Morand-Joubert L, et al, and the Narval Trial Group. Phenotypic or genotypic resistance testing for choosing antiretroviral therapy after treatment failure: a randomized trial. AIDS. March 29, 2002;16(5):727-736.
References:
Durant J, Clevenbergh P, Halfon P, et al. Drug-resistance genotyping in HIV-1 therapy: the VIRADAPT randomised controlled trial. Lancet. June 26, 1999;353(9171):2195-2199.
Baxter JD, Mayers DL, Wentworth DN, et al. A randomized study of antiretroviral management based on plasma genotypic antiretroviral resistance testing in patients failing therapy. AIDS. June 16, 2000;14(9):F83-F93.
Tural C, Ruiz L, Holtzer C, et al, and the Havana Study Group. Clinical utility of HIV-1 genotyping and expert advice: the Havana trial. AIDS. January 25, 2002;16(2):209-218.
Cingolani A, Antinori A, Rizzo MG, et al. Usefulness of monitoring HIV drug resistance and adherence in individuals failing highly active antiretroviral therapy: a randomized study (ARGENTA). AIDS. February 15, 2002;16(3):369-379.
Cohen CJ, Hunt S, Sension M, et al, and the VIRA3001 Study Team. A randomized trial assessing the impact of phenotypic resistance testing on antiretroviral therapy. AIDS. March 8, 2002;16(4):579-588.
Meynard JL, Vray M, Morand-Joubert L, et al, and the Narval Trial Group. Phenotypic or genotypic resistance testing for choosing antiretroviral therapy after treatment failure: a randomized trial. AIDS. March 29, 2002;16(5):727-736.
68. References:
Durant J, Clevenbergh P, Halfon P, et al. Drug-resistance genotyping in HIV-1 therapy: the VIRADAPT randomised controlled trial. Lancet. June 26, 1999;353(9171):2195-2199.
Baxter JD, Mayers DL, Wentworth DN, et al. A randomized study of antiretroviral management based on plasma genotypic antiretroviral resistance testing in patients failing therapy. AIDS. June 16, 2000;14(9):F83-F93.
Tural C, Ruiz L, Holtzer C, et al, and the Havana Study Group. Clinical utility of HIV-1 genotyping and expert advice: the Havana trial. AIDS. January 25, 2002;16(2):209-218.
Cingolani A, Antinori A, Rizzo MG, et al. Usefulness of monitoring HIV drug resistance and adherence in individuals failing highly active antiretroviral therapy: a randomized study (ARGENTA). AIDS. February 15, 2002;16(3):369-379.
Cohen CJ, Hunt S, Sension M, et al, and the VIRA3001 Study Team. A randomized trial assessing the impact of phenotypic resistance testing on antiretroviral therapy. AIDS. March 8, 2002;16(4):579-588.
Meynard JL, Vray M, Morand-Joubert L, et al, and the Narval Trial Group. Phenotypic or genotypic resistance testing for choosing antiretroviral therapy after treatment failure: a randomized trial. AIDS. March 29, 2002;16(5):727-736.
References:
Durant J, Clevenbergh P, Halfon P, et al. Drug-resistance genotyping in HIV-1 therapy: the VIRADAPT randomised controlled trial. Lancet. June 26, 1999;353(9171):2195-2199.
Baxter JD, Mayers DL, Wentworth DN, et al. A randomized study of antiretroviral management based on plasma genotypic antiretroviral resistance testing in patients failing therapy. AIDS. June 16, 2000;14(9):F83-F93.
Tural C, Ruiz L, Holtzer C, et al, and the Havana Study Group. Clinical utility of HIV-1 genotyping and expert advice: the Havana trial. AIDS. January 25, 2002;16(2):209-218.
Cingolani A, Antinori A, Rizzo MG, et al. Usefulness of monitoring HIV drug resistance and adherence in individuals failing highly active antiretroviral therapy: a randomized study (ARGENTA). AIDS. February 15, 2002;16(3):369-379.
Cohen CJ, Hunt S, Sension M, et al, and the VIRA3001 Study Team. A randomized trial assessing the impact of phenotypic resistance testing on antiretroviral therapy. AIDS. March 8, 2002;16(4):579-588.
Meynard JL, Vray M, Morand-Joubert L, et al, and the Narval Trial Group. Phenotypic or genotypic resistance testing for choosing antiretroviral therapy after treatment failure: a randomized trial. AIDS. March 29, 2002;16(5):727-736.
69. Clinical Trials�Summary and Conclusions* Many abstracts, but few published studies
Difficult to compare
Interpretations are complicated
Short term benefits demonstrated for both assays
Evidence strongest for genotyping
Insufficient evidence favoring 1 test type over another
Complex situations: genotyping and phenotyping provide complementary information
70. Recent Applications of Antiretroviral Resistance Testing
71. Transmitted HIV Drug Resistance New York City MDR / Rapid Disease Progression Case
72. Follow-Up on the New York City MDR Case Blick et al performed an analysis on 135,000 HIV strains in the database
Matched the NYC strain with a strain from a 52 yo Conn. man who began AZT in 1995 & HAART in 1997
This “Pt Zero” reported having unprotected sex with the NYC pt while on crystal methamphetamine in 10/04
Phylogenetic analysis confirmed that the 2 strains were identical ; both dual tropic with identical resistance patterns
Pt Zero currently has CD4 of 180-262 & VL < 400; and he is clinically stable
Refutes the concept of a “new virulent strain” & suggests that host factors might explain the rapid decline of the NYC pt (CD4 of 60 four to twenty months into infection)
73. Patient Zero? �Transmission of MDR Resistant Virus
74. US surveillance of HIV drug resistance Drug resistance in 787 newly diagnosed ART-naďve subjects from 89 sites in 6 states (2003–2004) Background/Methods:
CDC re-analysis newly diagnosed but chronically infected between 2002–2004.
First analysis of new data set; 2003–4.
Rise in resistance across all classes with a 3.1% rise in >2 class resistance.
Methods:
In 2003–4, drug resistance surveillance began in 65 sites in 6 states (Illinois, Colorado, Washington, Virginia, Maryland, and Michigan). A total of 595 residual HIV diagnostic sera from drug-naďve persons newly diagnosed with HIV were processed in the public health laboratories where routine HIV testing takes place. Sequencing was performed at Stanford University, Maryland State, and University of Washington laboratories. Results were available to providers within 30 days.
Conclusions:
In participating surveillance sites, as in other recent US studies, resistance to NNRTI was more prevalent than resistance to NRTI, although overall HIV drug resistance prevalence was lower than prevalence reported in other studies.
Persons diagnosed in publicly funded sites may have a lower prevalence of drug resistance than those in specialists’ care, possibly because persons who transmit HIV to persons diagnosed in specialist centers may, as a group, have more access to HIV treatment and therefore to ARV drugs.
Representative drug resistance surveillance methods and sufficiently large numbers are needed to obtain accurate national estimates. The use of residual HIV diagnostic sera from counseling and testing sites as well as clinical sites can provide a representative sample of persons newly diagnosed with HIV for surveillance purposes.
Limitations:
Not all newly diagnosed in 2003–4 in participating sites included; specimens not available from all persons and unable to GT in 5% of specimens.
Analysis of associated risk factors was limited for patients for whom demographic data are currently available; numbers may be too small to show differences among groups.
Patients in private practice or non–public-funded centers may have a higher risk for HIV drug resistance than those included in this analysis (possibly due to better access to care and access to ARVs?).
Background/Methods:
CDC re-analysis newly diagnosed but chronically infected between 2002–2004.
First analysis of new data set; 2003–4.
Rise in resistance across all classes with a 3.1% rise in >2 class resistance.
Methods:
In 2003–4, drug resistance surveillance began in 65 sites in 6 states (Illinois, Colorado, Washington, Virginia, Maryland, and Michigan). A total of 595 residual HIV diagnostic sera from drug-naďve persons newly diagnosed with HIV were processed in the public health laboratories where routine HIV testing takes place. Sequencing was performed at Stanford University, Maryland State, and University of Washington laboratories. Results were available to providers within 30 days.
Conclusions:
In participating surveillance sites, as in other recent US studies, resistance to NNRTI was more prevalent than resistance to NRTI, although overall HIV drug resistance prevalence was lower than prevalence reported in other studies.
Persons diagnosed in publicly funded sites may have a lower prevalence of drug resistance than those in specialists’ care, possibly because persons who transmit HIV to persons diagnosed in specialist centers may, as a group, have more access to HIV treatment and therefore to ARV drugs.
Representative drug resistance surveillance methods and sufficiently large numbers are needed to obtain accurate national estimates. The use of residual HIV diagnostic sera from counseling and testing sites as well as clinical sites can provide a representative sample of persons newly diagnosed with HIV for surveillance purposes.
Limitations:
Not all newly diagnosed in 2003–4 in participating sites included; specimens not available from all persons and unable to GT in 5% of specimens.
Analysis of associated risk factors was limited for patients for whom demographic data are currently available; numbers may be too small to show differences among groups.
Patients in private practice or non–public-funded centers may have a higher risk for HIV drug resistance than those included in this analysis (possibly due to better access to care and access to ARVs?).
75. Drug resistance and its association with increased risk of death in pts on 1st HAART 1388 ART-naďve Canadian pts
Initiated HAART Aug 96–July 00
Primary endpoint: all-cause mortality
238 deaths observed (17.2%)
Increased risk of death
Increased age
Decreased adherence
Lower baseline CD4+
Higher baseline HIV RNA
Decreased physician experience
Emergence of ART resistance ABSTRACT:
Resistance to any class of drug was 28.3% (n=393).
COMMENTS:
Manuscript in review; this is first data looking at resistance as related to risk of mortality. Dr Hogg is not a physician but a “demographer” and doing great work at describing patient cohorts.
One of two things might be going on for NNRTI:
NNRTI-resistant virus thought to be more pathogenic relative to other viruses; generally see full viral rebound when there is resistance alluding to relatively fit viruses; often see CD4+ decline in these patients.
Low levels of adherence puts patients at risk for resistance; pharmacy refill data used for this cohort and in other studies; not as precise as could be, might be some uncontrolled confounding adherence-related factors; nonadherent group probably in ballpark of <50%, ie, NNRTI-resistant virus “picks out” nonadherent patients.
FOR PI: both theories above possibly true in opposite direction…
With PI-resistant virus: generally see partial viral rebound; sustained elevations in CD4+ suggests PI-resistant virus not “fully” pathogenic; does not explain protective effect, but probably not as pathogenic; a lot of single PIs in this study; early data.
PI resistance is a marker of high levels of adherence among patients who are on single PIs (Bangsberg et al); some uncontrolled confounding; this group probably taking a lot of their meds (>90%). ABSTRACT:
Resistance to any class of drug was 28.3% (n=393).
COMMENTS:
Manuscript in review; this is first data looking at resistance as related to risk of mortality. Dr Hogg is not a physician but a “demographer” and doing great work at describing patient cohorts.
One of two things might be going on for NNRTI:
NNRTI-resistant virus thought to be more pathogenic relative to other viruses; generally see full viral rebound when there is resistance alluding to relatively fit viruses; often see CD4+ decline in these patients.
Low levels of adherence puts patients at risk for resistance; pharmacy refill data used for this cohort and in other studies; not as precise as could be, might be some uncontrolled confounding adherence-related factors; nonadherent group probably in ballpark of <50%, ie, NNRTI-resistant virus “picks out” nonadherent patients.
FOR PI: both theories above possibly true in opposite direction…
With PI-resistant virus: generally see partial viral rebound; sustained elevations in CD4+ suggests PI-resistant virus not “fully” pathogenic; does not explain protective effect, but probably not as pathogenic; a lot of single PIs in this study; early data.
PI resistance is a marker of high levels of adherence among patients who are on single PIs (Bangsberg et al); some uncontrolled confounding; this group probably taking a lot of their meds (>90%).
76. Reduced Transmission of Drug-Resistant Strains Containing M184V & PI Mutations Compared genotypes among pts with primary HIV infection (PHI) and chronically infected patients (CIP)
Found that the RR of transmitting HIV harboring M184V was less than the RR of transmitting HIV with TAMS or NNRTI mutations (P < 0.05)
RR of transmitting strains harboring PI mutations was less than the RR of those without PI mutations (P<0.01)
77. Reduced Transmission of Drug-Resistant Strains Containing M184V & PI Mutations In chronic pts with TAMS or NNRTI mutations, the median VL was 35,000; while pts with M184V, median VL was 4252
In chronic pts, median VL of pts with no PI mutations was 24,104; while pts with PI mutations had a median VL of 11,800
Hypothesis: M184V & PI mutations ?’s RC, which ?’s VL, which reduces the likelihood of transmission during sex
78. Future Directions for Resistance Testing Importance of Secondary Protease Resistance Mutations
79. Reduced Susceptibility to PI’s in the Absence of Primary PI Resistance Mutations Parkin et al defined primary PI mutations as the following: any change from wt in 23,24,30,32,46,47,48,50,54,82,84,88 & 90
Excluded I54V & N88D (which are not reported without other primary mutations) and V82I (known polymorphism in PI naives)
Determined PR genotype and PI susceptibility (FC in IC 50); also determined gag genotypes
Found 125 pts with no primary mutations but at least one PI with FC >5
80. Reduced Susceptibility to PI’s in the Absence of Primary PI Resistance Mutations Compared the 125 pts to 3,956 samples with no PI mutations & all PI FC’s < 5; described PR mutations over-represented in samples with PI FC>5: L10IV, I13V, L19V, K20IMT, A22V, M36IV, N37D, I54V, H69R, A71TV, G73S, T74KS, V82I, N83D, N88D, & I93L
In gag, found that K418ER, A431V, I437V, L449IP, P453L & E482G were also associated with PI FC > 5 in pts without primary PR mutations
Concluded that accumulation of secondary mutations in PR and also in gag contribute to PI susceptibility
81. NNRTI Hypersusceptibility:��Nucleoside mutations (TAMS) create HIV strains uniquely sensitive to NNRTI therapy� 215Y, 41L, 210W, 118I and 208Y
82. NNRTI hypersusceptibility – a review If you do phenotypic resistance testing, you may have noticed in some of your patients that sometimes, instead of seeing a 10-fold reduction in susceptibility, the fold change reported is 0.3 or 0.2, suggesting that the virus is hypersusceptible to the drug. Does that really matter? Here is a pooled analysis of 444 samples from 5 ACTG studies that was presented by Nancy Shulman at Stanford and they were able to look at this phenomenon of hypersusceptibility and link it to specific mutations in reverse transcriptase that are associated with thymidine analogs. The 5 mutations listed, all of which seem to have some linkage to NNRTI hypersusceptibility, are induced by thymidines and may actually have a favorable outcome in terms of the efficacy of NNRTI-based regimens and persons who are NNRTI-naďve.
Lisa Demeter also examined response to a regimen of efavirenz, indinavir and abacavir in nucleoside-experienced patients. The genotypic score for efavirenz hypersusceptibility from ACTG368 was predictive of outcome in these patients. The specific mutations that were associated with hypersusceptibility are shown. The more of these mutations present, the lower likelihood of virologic failure.
Previous studies show improved response associated with HS to EFV1, 2 and APV3.
References
Haubrich R, et al. AIDS 2002;16:33–40
2. Shulman N, et al. AIDS 2001; 15:1125–1132
3. Schooley R, et al. 10th CROI, Boston 2003, #143)If you do phenotypic resistance testing, you may have noticed in some of your patients that sometimes, instead of seeing a 10-fold reduction in susceptibility, the fold change reported is 0.3 or 0.2, suggesting that the virus is hypersusceptible to the drug. Does that really matter? Here is a pooled analysis of 444 samples from 5 ACTG studies that was presented by Nancy Shulman at Stanford and they were able to look at this phenomenon of hypersusceptibility and link it to specific mutations in reverse transcriptase that are associated with thymidine analogs. The 5 mutations listed, all of which seem to have some linkage to NNRTI hypersusceptibility, are induced by thymidines and may actually have a favorable outcome in terms of the efficacy of NNRTI-based regimens and persons who are NNRTI-naďve.
Lisa Demeter also examined response to a regimen of efavirenz, indinavir and abacavir in nucleoside-experienced patients. The genotypic score for efavirenz hypersusceptibility from ACTG368 was predictive of outcome in these patients. The specific mutations that were associated with hypersusceptibility are shown. The more of these mutations present, the lower likelihood of virologic failure.
Previous studies show improved response associated with HS to EFV1, 2 and APV3.
References
Haubrich R, et al. AIDS 2002;16:33–40
2. Shulman N, et al. AIDS 2001; 15:1125–1132
3. Schooley R, et al. 10th CROI, Boston 2003, #143)
83. K65R Leads to NNRTI Hypersusceptibility Not only TAM’s lead to NNRTI HS, but also K65R & L74V
Landman et al evaluated salvage tx for 22 pts with K65R from the TONUS & GS903 trials
Median baseline VL was 6336
At 48 wks, 86% were < 50 copies; mean RC was 54%
The K65R and M184V double mutants were HS to EFV, NVP & ZDV
Concluded that NNRTI hypersusceptibility & impaired RC associated with K65R contributed to successful salvage with EFV & ZDV
84.
Guidelines for the Use of
Antiretroviral Agents in HIV-1-Infected
Adults and Adolescents
July 14, 2003
86. Recommendations for Resistance Testing References:
Panel on Clinical Practices for Treatment of HIV Infection for the Department of Health and Human Services and the Henry J Kaiser Family Foundation. Guidelines for the Use of Antiretroviral Agents in HIV-Infected Adults and Adolescents. Washington, DC: Department of Health and Human Services; February 4, 2002. Available at: http://www.aidsinfo.nih.gov/guidelines/adult/html_adult_02-04-02.html. Accessed February 23, 2002.
Hirsch MS, Brun-Vezinet F, D’Aquila RT, et al. Antiretroviral drug resistance testing in adult HIV-1 infection: recommendations of an International AIDS Society-USA Panel. JAMA. May 10, 2000;283(18):2417-2426.
Yeni PG, Hammer SM, Carpenter CCJ, Cooper DA, Fischl MA, Gattell JM, et al. Antiretroviral Treatment for Adult HIV Infection in 2002: Updated Recommendations of the International AIDS Society-USA Panel. JAMA. July 10, 2002;288:222-252.
References:
Panel on Clinical Practices for Treatment of HIV Infection for the Department of Health and Human Services and the Henry J Kaiser Family Foundation. Guidelines for the Use of Antiretroviral Agents in HIV-Infected Adults and Adolescents. Washington, DC: Department of Health and Human Services; February 4, 2002. Available at: http://www.aidsinfo.nih.gov/guidelines/adult/html_adult_02-04-02.html. Accessed February 23, 2002.
Hirsch MS, Brun-Vezinet F, D’Aquila RT, et al. Antiretroviral drug resistance testing in adult HIV-1 infection: recommendations of an International AIDS Society-USA Panel. JAMA. May 10, 2000;283(18):2417-2426.
Yeni PG, Hammer SM, Carpenter CCJ, Cooper DA, Fischl MA, Gattell JM, et al. Antiretroviral Treatment for Adult HIV Infection in 2002: Updated Recommendations of the International AIDS Society-USA Panel. JAMA. July 10, 2002;288:222-252.
87. Guidelines Vary by State��General Recommendations
88. Antiretroviral Resistance Testing�Standards for Medicaid Reimbursement Most state Medicaid guidelines agree with the current DHHS Guidelines and recommend RT in the following clinical settings:
Virologic failure while on recommended Antiretroviral Therapy (ART)
Suboptimal virologic response after beginning ART
Acute HIV infection (ie, those strongly documented to have been infected within the previous 6 months)
Consider in ARV-naďve patients if the rate of resistance in the community is substantial
89. Resistance Testing in Pregnancy DOH recommends RT for:
All HIV + pregnant women with viral loads >1000/mm3 or greater than the documented statement of threshold accuracy by the laboratory
Recommended independent of whether or not they are already being treated with combination therapy
Testing should be done as near to the first prenatal visit as possible
Antiretroviral therapy should be continued or begun empirically pending results, with treatment becoming more urgent the higher the viral load
90. Pediatric Resistance Testing�Recommendations Resistance testing is recommended for newly infected infants, children, and adolescents
When the HIV RNA does not decrease as expected within 4 to 6 months of initiating HAART, or
When there is viral rebound
91. When NOT to Use �Antiretroviral Resistance Testing After discontinuation of antiretroviral treatment for more than 2 weeks
If plasma HIV RNA <1000 co/ml or less than the documented statement of threshold accuracy by the laboratory
To document lack of adherence and in situations other than above
92. Which antiretroviral resistance tests should be used?� Studies in patients failing a first antiretroviral regimen: genotypic ~ phenotypic resistance testing
In patients with multiple ART failures
May be advantageous to use phenotypic resistance testing
Or concurrent use of both tests, to optimize therapy
93. Cost-Effectiveness�and Pharmacoeconomics
Genotyping
ARV-experienced patients
VIRADAPT: 1st study to suggest cost-effectiveness of resistance testing
Weinstein et al. (Ann Intern Med. 2001;134(6):440-450)
Model based on 2 prospective short term trials
Suggests genotyping is as cost effective as HAART
ARV-naďve patients
Sax et al. (XIV IAC. Barcelona, July 7-12, 2002. Ab#MoPeB3129)
Simulation model based upon prospective clinical trials
Depends upon prevalence of resistant virus in a particular area
Phenotyping: studies underway
94. VIRADAPT Study Mean 12-Month Cost per Patient Clinical Care*
ART Drugs
Genotyping†
Total Cost Reference:
Chaix C, Grenier-Sennelier C, Clevenbergh P, et al. Economic evaluation of drug resistance genotyping for the adaptation of treatment in HIV-infected patients in the VIRADAPT study. J Acquir Immune Defic Syndr. July 1, 2000;24(3):227-231.Reference:
Chaix C, Grenier-Sennelier C, Clevenbergh P, et al. Economic evaluation of drug resistance genotyping for the adaptation of treatment in HIV-infected patients in the VIRADAPT study. J Acquir Immune Defic Syndr. July 1, 2000;24(3):227-231.
95. Cost-Effectiveness of Genotypic Resistance Testing After�HAART Failure1,2 Models derived from 2 prospective clinical trials
QALY used to determine cost-benefit
<$25,000/QALY “very cost-efficient”
PCPP: $16,000/QALY
MACP: $35,000-58,000/QALY
Others References:
Weinstein MC, Goldie SJ, Losina E, et al. Use of genotypic resistance testing to guide HIV therapy: clinical impact and cost-effectiveness. Ann Intern Med. March 20, 2001;134(6):440-450.
Saag MS. HIV resistance testing in clinical practice: a QALY-fied success. Ann Intern Med. March 20, 2001;134(6):475-477.References:
Weinstein MC, Goldie SJ, Losina E, et al. Use of genotypic resistance testing to guide HIV therapy: clinical impact and cost-effectiveness. Ann Intern Med. March 20, 2001;134(6):440-450.
Saag MS. HIV resistance testing in clinical practice: a QALY-fied success. Ann Intern Med. March 20, 2001;134(6):475-477.
96. How frequently should �resistance testing be ordered? Currently, there are no guidelines regarding the frequency of resistance testing
However, based on the accepted time frames defining virologic failure as outlined in the DHHS guidelines, reimbursement in most states will be limited to no more than 2-3 tests in a 12-month period
Exceptions to the 2-test limit may be requested
97. Thank you for your time and attention
