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HIV-1C in-House RNA-Based Genotyping Assay for Detection of Drug Resistance Mutations in Samples with Low-Level Viral Loads

基因分型 病毒学 抗药性 病毒载量 抗性突变 艾滋病毒耐药性 人类免疫缺陷病毒(HIV) 生物 人口 病毒血症 基因型 遗传学 医学 聚合酶链反应 抗逆转录病毒疗法 逆转录酶 基因 环境卫生
作者
Ontlametse T. Bareng,Wonderful T. Choga,Segomotso T Maphorisa,Sekgabo Seselamarumo,Kaelo K Seatla,Patrick Mokgethi,Dorcas Maruapula,Mompati Mogwele,Doreen Ditshwanelo,Natasha O. Moraka,Irene Gobe,Modisa S. Motswaledi,Joseph Makhema,Rosemary Musonda,Roger Shapiro,Max Essex,Vlad Novitsky,Sikhulile Moyo,Simani Gaseitsiwe
出处
期刊:Infection and Drug Resistance [Dove Medical Press]
卷期号:Volume 15: 7565-7576
标识
DOI:10.2147/idr.s388816
摘要

Monitoring HIV-1 drug resistance mutations (DRM) in treated patients on combination antiretroviral therapy (cART) with a detectable HIV-1 viral load (VL) is important for the selection of appropriate cART. Currently, there is limited data on HIV DRM at low-level viremia (LLV) (VL 401-999 copies/mL) due to the use of a threshold of VL ≥1000 copies/mL for HIV DRM testing. We here assess the performance of an in-house HIV drug resistance genotyping assay using plasma for the detection of DRM at LLV.We used a total of 96 HIV plasma samples from the population-based Botswana Combination Prevention Project (BCPP). The samples were stratified by VL groups: 50 samples had LLV, defined as 401-999 copies/mL, and 46 had ≥1000 copies/mL. HIV pol (PR and RT) region was amplified and sequenced using an in-house genotyping assay with BigDye sequencing chemistry. Known HIV DRMs were identified using the Stanford HIV Drug Resistance Database. Genotyping success rate between the two groups was estimated and compared using the comparison of proportions test.The overall genotyping success rate was 79% (76/96). For VL groups, the genotyping success was 72% (36/50) at LLV and 87% (40/46) at VL ≥1000 copies/mL. Among generated sequences, the overall prevalence of individuals with at least 1 major or intermediate-associated DRM was 24% (18/76). The proportions of NNRTI-, NRTI- and PI-associated resistance mutations were 28%, 24%, and 0%, respectively. The most predominant mutations detected were K103N (18%) and M184V (12%) in NNRTI- and NRTI-associated mutations, respectively. The prevalence of DRM was 17% (6/36) at LLV and 30% (12/40) at VL ≥1000 copies/mL.The in-house HIV genotyping assay successfully genotyped 72% of LLV samples and was able to detect 17% of DRM amongst them. Our results highlight the possibility and clinical significance of genotyping HIV among individuals with LLV.
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