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Managing Antiretroviral Therapy in Treatment-Experienced Patients: First Regimen Failure

Managing Antiretroviral Therapy in Treatment-Experienced Patients: First Regimen Failure. MATEC Catherine Creticos, M.D. Medical Director. Objectives. Explain possible causes of drug failure Describe tests used to assess viral resistance

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Managing Antiretroviral Therapy in Treatment-Experienced Patients: First Regimen Failure

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  1. Managing Antiretroviral Therapy in Treatment-Experienced Patients: First Regimen Failure MATEC Catherine Creticos, M.D. Medical Director

  2. Objectives • Explain possible causes of drug failure • Describe tests used to assess viral resistance • Explain how to use resistance test results to select an effective new regimen • Discuss strategies for managing patients with limited treatment options

  3. Case Study 1 • A.D. is a 51 yo male HIV+ since 1989. He started Combivir in 1993, and his viral load remained undetectable until June 2006, with CD4 in the 400-600 range. Since June 2006, his viral load on 2 occasions has been 24,500 and 37,800 respectively. His most recent CD4 count was 378 cells.

  4. First Antiretroviral Treatment Failure • Assessment • What are possible causes of increased viral load? • Is intervention necessary at this point? • Why / Why not? • What intervention(s)?

  5. Reasons for First Antiretroviral Therapy Regimen Failure • Viral load , but patient not failing regimen • recent infection (eg, HSV outbreak, bacterial infection, acute hepatitis) • recent vaccination • Poor adherence – regimen may still be salvagable • Poor absorption (unboosted PIs) • Drug-drug interactions (eg, PPIs and atazanavir) • Incompletely suppressive regimen (eg, dual nucleoside)

  6. First Antiretroviral Failure: Interventions • Review adherence – last month, last few days • Probe for recent events, problems (eg, recent infection or other issues such as running out of medication or not taking medication on a trip) • Repeat viral load (can be done at same time as resistance assay) • Resistance assay – purpose is to identify specific drug resistance that has led to failure and to assist in the selection of the next regimen

  7. Rationale for HIV Resistance Testing • Drug resistance at start of ART is predictor of virologic response • Several prospective studies support use of resistance testing to improve response to ART • Preliminary economic studies suggest resistance testing cost-effective after first HAART failure • Prevalence of resistance in acute/recent HIV infection 10%-26% in recent studies

  8. Current Recommendations forUse of Resistance Testing (DHHS) • Recommended for selection of active drugs when changing therapy if viral suppression is suboptimal w/initial regimen • Recommended for pregnant women initiating therapy or with incomplete virologic suppression • May be useful in cases of acute infection or infection within the last 1-2 years • Not yet recommended at initiation of therapy in all treatment-naïve individuals until more information available on prevalence; however in areas of high prevalence, resistance testing may be useful • Both phenotyping and genotyping may be useful in patients with complex prior treatment history

  9. Evolution of Drug Resistance • Causes of high genetic variability of HIV: • DNA copy of RNA genome for replication • Lack of proofreading by RT during replication • Every possible point mutation occurs ~1,000-10,000 times a day; double mutants common • Genetic recombination between different viruses in the same cell • Acquisition of resistance during tx depends on: • Size and heterogeneity of viral population • Extent of replication during drug therapy • Ease of acquisition of particular mutation • Effect of mutation on drug susceptibility and viral fitness

  10. How Drug Resistance Arises How drug resistance arises. Richman, DD. Scientific American , July 1998

  11. Resistance Testing: Definitions • Mutation (molecular definition): change in nucleic acid sequence compared with consensus or wild-type virus • point mutation: AAA GAC AGT=>AAA AAC AGC • insertion: AAA AAC AGT=> AAA AAC AGT AGT • deletion: AAA AAC AGT=> AAA…AGT • Drug resistant mutation: change in amino acid sequence (vs. reference strain) that affects susceptibility to a drug • Major, primary: can solely affect susceptibility • Minor, secondary, accessory: contributes to reduced susceptibility • Polymorphism: a naturally occurring change in amino acid sequence not shown to directly impact drug susceptibility

  12. Mutational Nomenclature Wild-type amino acid G48V Mutant amino acid  Codon Position • Mixtures are indicated by a slash • K103K/N indicates mixture of wild-type and mutant • T215D/Y/F indicates mixture of 3 mutants

  13. Resistance Assays: Phenotype and Genotype Phenotype: • Direct assay: measures ability of the virus to grow in various concentrations of antiretroviral drugs. Genotype: • Indirect assay: detects drug resistance mutations that are present in the relevant viral genes. • Both assays focus on the reverse transcriptase (RT) and protease (PR) genes of the virus

  14. Phenotyping: Advantages • Provides resistance information on each drug regardless of the presence of multiple mutations • Interpretation may be more intuitive than for genotype assay • Very useful in patients with complex drug history and complicated mutation profile • Very useful for deciphering cross-resistance • May be more useful than genotyping for new drugs until appropriate mutations are established by clinical data

  15. Phenotyping: Disadvantages • If drug resistant population is minor, the phenotypic effect may not be detected • Viral load needs to  1000 copies/ml • Very expensive and time-consuming • Consensus on drug-resistance cut-off values are not yet fully determined - drugs to which a patient is actually still sensitive may be unnecessarily eliminated • initial cut-offs were based on assay variability on repeated testing of known sample • later cut-offs were based on natural variability of wild-type viruses from patients • current cut-offs are being developed based on outcome data from clinical trials

  16. Antivirogramphenotype

  17. PhenoSense HIV Report

  18. Sequence-based Genotyping Assays • HIV circulating in patient’s plasma is isolated; RT and PR genes are copied, amplified & sequenced. • The test sequence is compared to a reference HIV strain and all changes (mutations) are noted. • Software compares changes found to a list of the mutations known to be associated with resistance. • A report documents any mutations and (optimally) the ARV drugs to which the virus is sensitive or resistant based on the presence or absence of particular mutations.

  19. Available Genotypes

  20. Genotyping: Advantages • Identification of all nucleotides, amino acid differences, deletions & insertions • Genotyping has the ability to detect resistant virus that constitutes only a small proportion (~ 20%) of the viral population. • This can provide “predictive” early warning of resistance before full resistance develops • Faster and less expensive than phenotype assay

  21. Genotyping: Disadvantages • Reports may be difficult to interpret unless clinician is very experienced • Labs use different software to predict resistance - a consensus on which mutations are important is needed • There is a lot of variation in the quality of the “product” from different labs, especially in the ability to detect minority species in the population • Significance of many mutations still poorly understood • Lack of understanding of the significance of combinations of mutations • Viral load needs to  1000 copies/ml

  22. Phenotype/Genotype Discordance: • Interpretation Discordance • interpretation is incorrect (especially new drugs) • data base is incomplete or lacking • Test Result Discordance • PT sensitive but GT resistant • mixtures • transitional mutations • antagonistic mutational interactions

  23. Genotype-Phenotype Discordance • Observed differences between phenotype and genotype are not uncommon • Reasons for genotype-phenotype discordance • use of inaccurate genotype interpretation algorithms (not accounting for novel or unknown mutations, or for unrecognized effects of mutations) • Presence of mixtures of wild-type and resistant strains • Variability in phenotypic susceptibility with specific mutations

  24. Virtual Phenotype • Determines genotype of test strain • Computer algorithm matches genotype to strains that have been previously phenotyped • Presents expected phenotype based on the average phenotype of matching isolates

  25. Pros Inexpensive, quick way to generate phenotypic information Clinical studies show good correlation between virtual and real PT and equal efficacy in predicting viral suppression Cons number of matches may be low “union” of limitations of GT and PT techniques clinical studies do not demonstrate benefit of virtual PT added to GT and expert advice Virtual Phenotype: Pros and Cons

  26. NRTIs Major Mutations

  27. NRTIs:Special Considerations • Require triphosphorylation, complicates in vitro assessment & PT testing  discordance b/w in vitro and in vivo potency • NEMs (TAMs) selected primarily in patients treated with AZT or D4T; 10% of patients on DDI monotherapy; rarely during ABC monotherapy • Some NRTI mutations hypersensitize HIV to NNRTIs • K65R confers intermediate resistance to DDI, ABC, TDF, 3TC. Recent study of ABC/3TC/TDF led to high failure rate • Q151M is a 2-base pair change that causes intermediate resistance to AZT, DDI, D4T, and ABC • TDF efficacy reduced by 3 or more TAMs, especially in presence of M41L or L210W

  28. Mutational Interactions: M184V • M184V- causes high-level 3TC resistance and low-level resistance to ddI, ddC, ABC • M184V reverses T215Y-mediated AZT resistance • Resensitization clinically significant; slows AZT resistance in patients on AZT/3TC • M184V appears to reverse effect of NEMs on resistance to d4T, TDF

  29. NNRTIs Major Mutations

  30. NNRTI Mutations:Special Consideration • Y181C/I causes high-level resistance to NVP and DLV, but low-level resistance to EFV. However, isolates only transiently respond to EFV • Y181C and L100I hypersensitize HIV to AZT • G190A/S are resistant to NVP and EFV but hypersensitive to DLV

  31. PIs Major Mutations

  32. PIs:Special Considerations • Cross-resistance problematic; in one study of over 6,000 isolates, 59%-80% of isolates with a 10-fold decrease in susceptibility to one PI also had a 10-fold decrease to at least one other • For LPV/r, at least 4 of 11 mutations may be needed for significant resistance • NFV and ATV when used as first PI may select for mutations with little cross-resistance: • NFV – D30N • ATV – I50L

  33. Stanford HIV Database • http://hivdb.stanford.edu • Can insert mutations and receive an assessment of resistance and a discussion of significance of the mutations

  34. Genotype shows:M184V, D67N, K70K/R, and K219K/Q Reference lab predicted resistance to AZT, ABC, 3TC, FTC, d4T; No resistance to DDI, TDF, all NNRTIs & PIs Stanford database interpretation Nucleoside RTI: 3TC: High-level resistance ABC: Low-level resistance AZT: Intermediate resistance D4T: Low-level resistance DDI: Potential low-level resistance FTC: High-level resistance TDF: Susceptible Non-Nucleoside RTI DLV: Susceptible EFV: Susceptible NVP: Susceptible Case Study 1:A.D.

  35. Stanford Database Comments on Significance of Mutations • D67N contributes some degree of resistance the NRTIs except 3TC and FTC. It usually occurs with mutations at positions 70 or 215. D67E/G occur in heavily treated patients and probably have a similar effect as D67N. • K70R causes low-level AZT and probably D4T resistance but appears to have little effect on the other NRTIs. K70E reduces TDF susceptibility. K70G/N are rare variants of unknown significance.

  36. Stanford Database Comments on Significance of Mutations • M184V/I cause high-level resistance to 3TC and FTC, and low-level in vitro resistance to DDI and ABC. However, it has not been shown to limit the effectiveness of DDI and it has only been shown to limit the effectiveness of ABC when it occurs in combination with multiple TAMs. M184V partially reverses T215Y-mediated resistance to AZT, TDF, and D4T. • K219Q/E increase AZT and probably D4T resistance when present with K70R or T215Y/F but may not have any effect on the remaining NRTIs. K219N/R occur commonly in heavily NRTI-treated patients. • M184V partially reverses AZT, D4T, and TDF resistance caused by other TAMs.

  37. Case Study 1:Treatment Selection and Response • Started Atripla (TDF/3TC/EFV) and Ziagen • What are other reasonable treatment choices? • 6 weeks after initiating therapy, patient’s viral load is undetectable • Continued close f/u is warranted

  38. Case Study 2 • K.L. is a 36 yo male with diabetes and HIV. He has been treated with Combivir and Sustiva as well as glipizide. He presents with decreased vision bilaterally, R>>L eye. An ophtholmologic exam reveals acute retinal necrosis and w/u shows an RPR 1:512. He is treated for syphilitic retinitis with significant improvement in his vision. His viral load = 38,900 and CD4 = 285. He admits to poor adherence over past 2 months. A GT is performed and shows K103N & M184V mutations.

  39. Clinical Decisions and Questions • What antiretroviral combinations would be appropriate to consider? • What type of follow-up should be done if therapy is changed? • What additional concerns need to be addressed?

  40. Case Study 2Treatment Selection and Response • His regimen is changed to: ATV/RTV/TDF/3TC/ZDV. • After 3 months, the viral load is undetectable and CD4 is 354

  41. Case Study 3 • K.C. is a 41 y.o. female with a history of former IVDU and HCV/HIV co-infection. She was treated initially with Viracept and Combivir. She has a long history of non-compliance and her viral load was never undetectable. She was changed to Combivir and Kaletra, but her viral load remained high at 53,000. A GT is done and shows no resistance mutations. A discussion with the patient reveals very poor adherence due to GI side effects and difficulty remembering her pills.

  42. Clinical Decisions and Questions • What is the meaning of the resistance assay and is it believable? • Is it appropriate to start a new antiretroviral regimen in this patient? • If so, what antiretroviral drugs would be appropriate? • What other concerns should be addressed? • What follow-up should be done?

  43. Case Study 3:Treatment Selection and Response • She is changed to ATV/RTV/TDF/ETV and these are given daily with her methadone. • Patient’s viral load after 3 months (and subsequently for the next year) is undetectable

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