Comparison of HIV-1 DNA load measurements in blood and in relation to successful proviral sequencing

IF 2.9 4区 医学 Q2 INFECTIOUS DISEASES Infectious diseases now Pub Date : 2023-12-14 DOI:10.1016/j.idnow.2023.104845
Anne Fuchs , Antoine Wasser , Clayton Faua , Stéphanie Caspar , Frédéric Jegou , Aurélie Velay , Elodie Laugel , Axel Ursenbach , David Rey , Samira Fafi-Kremer , Pierre Gantner
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Abstract

Objective

HIV DNA sequencing is now routinely used for HIV-infected individuals on antiretroviral therapy (ART) with or without partial genotypic history. Successful amplification of HIV pol gene has yet to be correlated with HIV DNA levels. Here, we assessed the relationship between HIV DNA load and sequencing results.

Methods

We analyzed three different qPCR measurements of total (LTR and LTR-gag) and integrated (Alu-LTR) HIV DNA in blood samples collected from viremic as well as virally suppressed HIV-infected individuals on ART. HIV DNA levels were compared to HIV DNA Sanger sequencing and clinical and therapeutic parameters.

Results

Among the 135 individuals analyzed for HIV DNA measurements and sequencing, all three HIV DNA measurements were associated with HIV DNA Sanger sequencing results. A threshold of around 2 and 1.5 log copies/million leukocytes of total HIV DNA was identified for LTR and LTR-gag qPCRs, respectively. Integrated HIV DNA positivity was also associated with successful sequencing. We further compared HIV DNA measurement techniques in an extended cohort of 312 individuals and showed that all measurements correlated between the different techniques, regardless of the HIV-1 subtypes analyzed. However, higher detection rates were observed with LTR (96%) compared to LTR-gag (86%) and Alu-LTR (59%) qPCRs. Duration of virological control on ART and CD4 nadir were the main determinants of HIV reservoir size.

Conclusions

HIV DNA measurement is associated with Sanger sequencing success, regardless of the technique used. In a clinical setting, Application of HIV DNA quantification before sequencing should be further evaluated.

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血液中 HIV-1 DNA 负载测量结果与成功前病毒测序结果的比较
目前,HIV DNA 测序已成为接受抗逆转录病毒疗法(ART)的 HIV 感染者(无论是否有部分基因型史)的常规检测方法。HIV pol 基因的成功扩增与 HIV DNA 水平之间尚无关联。在此,我们评估了 HIV DNA 负载与测序结果之间的关系。方法我们分析了从病毒感染者和接受抗逆转录病毒疗法的病毒抑制型 HIV 感染者血液样本中采集的总 HIV DNA(LTR 和 LTR-gag)和整合 HIV DNA(Alu-LTR)的三种不同 qPCR 测量结果。将 HIV DNA 水平与 HIV DNA Sanger 测序结果以及临床和治疗参数进行了比较。结果在 135 名进行了 HIV DNA 测定和测序分析的个体中,所有三种 HIV DNA 测定结果都与 HIV DNA Sanger 测序结果相关。LTR 和 LTR-gag qPCR 的阈值分别为约 2 和 1.5 log copies/百万白细胞总 HIV DNA。整合 HIV DNA 阳性也与成功测序有关。我们在 312 人的扩展队列中进一步比较了 HIV DNA 测量技术,结果表明,无论分析的是哪种 HIV-1 亚型,不同技术之间的所有测量结果都是相关的。然而,与 LTR-gag(86%)和 Alu-LTR (59%)qPCR 相比,LTR(96%)的检出率更高。抗逆转录病毒疗法的病毒学控制持续时间和 CD4 nadir 是 HIV 储库规模的主要决定因素。在临床环境中,应进一步评估测序前对 HIV DNA 定量的应用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Infectious diseases now
Infectious diseases now Medicine-Infectious Diseases
CiteScore
7.10
自引率
2.90%
发文量
116
审稿时长
40 days
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