Detection of archived lamivudine-associated resistance mutations in virologically suppressed, lamivudine-experienced HIV-infected adults by different genotyping techniques (GEN-PRO study)

Author:

Montejano Rocio1ORCID,Dominguez-Dominguez Lourdes2,de Miguel Rosa1,Rial-Crestelo David2,Esteban-Cantos Andrés3,Aranguren-Rivas Paula4,García-Álvarez Mónica4,Alejos Belén5,Bisbal Otilia2,Santacreu-Guerrero Mireia2,Hernando Asunción2,Bermejo-Plaza Laura2,Cadiñanos Julen1,Mayoral Mario6,Castro Juan Miguel6,Moreno Victoria6,Martin-Carbonero Luz6,Rodés Berta3,Delgado Rafael4ORCID,Rubio Rafael2,Pulido Federico2,Arribas José Ramón1ORCID

Affiliation:

1. Infectious Diseases Unit, Internal Medicine Department, Hospital Universitario La Paz—IdiPAZ, Paseo de la Castellana 261, 28046 Madrid, Spain

2. HIV Unit, Internal Medicine Department, Hospital Universitario 12 de Octubre—Imas12, Av. de Córdoba, s/n, 28041 Madrid, Spain

3. Hospital Universitario La Paz—IdiPAZ, Paseo de la Castellana 261, 28046 Madrid, Spain

4. Microbiology Department, Hospital Universitario 12 de Octubre—Imas12, Av. de Córdoba, s/n, 28041 Madrid, Spain

5. Instituto de Salud Carlos III, Av. de Monforte de Lemos, 5, 28029 Madrid, Spain

6. HIV Unit, Internal Medicine Department, Hospital Universitario La Paz—IdiPAZ, Paseo de la Castellana 261 28046, Madrid, Spain

Abstract

Abstract Background Previously selected lamivudine resistance-associated mutations (RAMs) may remain archived within the proviral HIV-DNA. Objectives To evaluate the ability of proviral DNA genotyping to detect lamivudine RAMs in HIV-1 virologically suppressed participants; the correlation between Sanger and next generation sequencing (NGS); and predictive factors for detection of lamivudine RAMs in proviral DNA. Methods Cross-sectional study of participants on stable antiretroviral therapy and suppressed for ≥1 year. Analysis of proviral DNA was performed by Sanger sequencing in whole blood and by NGS in PBMCs. Results We analysed samples from 102 subjects (52 with and 50 without lamivudine RAMs in historical plasma RNA-genotypes). Among participants with previous lamivudine resistance, Sanger sequencing detected RAMs in 26.9%. Detection rates significantly increased using NGS: 47.9%, 64.6%, 75% and 87.5% with the 20%, 10%, 5% and 1% thresholds, respectively. As for participants without historical lamivudine resistance, Sanger detected the RAMs in 1/49 (2%), and NGS (5% threshold) in 8/45 (17.8%). Multivariate models fitted to the whole population revealed that having a history of lamivudine resistance was a risk factor for detection of lamivudine RAMs by NGS. Among participants with historical lamivudine resistance, multivariate analysis showed that a longer time since HIV diagnosis was associated with persistence of archived mutations by NGS at thresholds of >10% [OR 1.10 (95% CI: 1.00–1.24)] and >5% [OR 1.16 (95% CI: 1.02–1.32)]. Conclusions Proviral DNA Sanger sequencing does not detect the majority of historical lamivudine RAMs. NGS increases the sensitivity of detection at lower thresholds, although the relevance of these minority populations with lamivudine RAMs needs further evaluation.

Funder

Fondo de Investigaciones Sanitarias, Instituto de Salud Carlos III

Publisher

Oxford University Press (OUP)

Subject

Infectious Diseases,Pharmacology (medical),Pharmacology,Microbiology (medical)

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