HIV-1 Drug Resistance Detected by Next-Generation Sequencing among ART-Naïve Individuals: A Systematic Review and Meta-Analysis

Ouyang, Fei; Yuan, Defu; Zhai, Wenjing; Liu, Shanshan; Zhou, Ying; Yang, Haitao

doi:10.3390/v16020239

Cited by 2 publications

(2 citation statements)

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“…Quality assessment and standardization of NGS methodologies are urgently needed to facilitate data comparison between studies ( 11 , 15 ). There is also a need to define the optimal threshold for LA-RAMs for clinical applications ( 11 , 13 , 14 , 16 , 17 ). Several studies have reported that LA-RAMs detected at levels of 2–9% were linked to virologic failure ( 15 , 18 – 21 ).…”

Section: Discussionmentioning

confidence: 99%

“…Fourth, due to limited sample volumes, we were not able to perform repeat/duplicate testing to evaluate the reproducibility of detection of mutations by NGS. Other approaches, such as the use of unique molecular identifiers during reverse transcription, could be used to assess the frequency of PCR- and sequencing-based errors in NGS data ( 13 , 17 , 26 , 27 ). Finally, parameters required for clinical assay validation were not evaluated in this study since the AB kit is not cleared by the U.S. FDA for clinical use.…”

Section: Discussionmentioning

confidence: 99%

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Performance of the Applied Biosystems HIV-1 Genotyping Kit with Integrase

Moore,

Palumbo,

Notarte

et al. 2024

J Clin Microbiol

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HIV genotyping is used to assess HIV susceptibility to antiretroviral drugs. The Applied Biosystems HIV-1 Genotyping Kit with Integrase (AB kit, Thermo Fisher Scientific) detects resistance-associated mutations (RAMs) in HIV protease (PR), reverse transcriptase (RT), and integrase (IN). We compared results from the AB kit with results obtained previously with the ViroSeq HIV-1 Genotyping System. DNA amplicons from the AB kit were also analyzed using next-generation sequencing (NGS). HIV RNA was extracted using the MagNA Pure 24 instrument (Roche Diagnostics; 96 plasma samples, HIV subtype B, viral load range: 530–737,741 copies/mL). FASTA files were generated from AB kit data using Exatype (Hyrax Biosciences). DNA amplicons from the AB kit were also analyzed by NGS using the Nextera XT kit (Illumina). Drug resistance was predicted using the Stanford HIV Drug Resistance Database. The mean genetic distance for sequences from ViroSeq and the AB kit was 0.02% for PR/RT and 0.04% for IN; 103 major RAMs were detected by both methods. Four additional major RAMs were detected by the AB kit only. These four major RAMs were also detected by NGS (detected in 18.1%–38.2% of NGS reads). NGS detected 27 major RAMs that were not detected with either of the Sanger sequencing-based kits. All major RAMs detected with ViroSeq were detected with the AB kit; additional RAMs were detected with the AB kit only. DNA amplicons from the AB kit can be used for NGS for more sensitive detection of RAMs.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Performance of the Applied Biosystems HIV-1 Genotyping Kit with Integrase

Moore,

Palumbo,

Notarte

et al. 2024

J Clin Microbiol

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The relevance of ultradeep sequencing for low HIV‐1 viral loads and proviruses in the clinical setting

Foury,

Saunier,

Taverniers

et al. 2024

Journal of Medical Virology

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Improving the therapeutic management of HIV‐positive persons is a major public health issue and includes better detection of drug resistance mutations (DRMs). The aim of this study was (i) to explore DRMs in HIV‐1‐positive persons presenting a blood viral load (VL) < 1000 genomes copies (gc)/mL, including the analyze of cerebrospinal fluid (CSF) and HIV‐DNA from peripheral blood mononuclear cells using ultradeep sequencing (UDS) and (ii), to evaluate how these DRMs could influence the clinical practices. For each patient (n = 12), including five low‐VL patients (i.e., <1000 gc/mL), HIV‐1 UDS targeting the protease, reverse transcriptase and integrase genes was performed on plasma, proviral DNA, and CSF when available. Sequencing discordances or failures were mostly found in samples from low‐VL patients. A 5% UDS cut‐off allowed to increase the sensitivity to detect DRMs in different compartments, excepted in CSF. Patients with the highest viral quasispecies heterogeneity were naïve of treatment or presented a medical history suggesting low selection pressure or virological failures. When analyzing compartmentalization and following‐up patients: low‐frequency variants (LFVs) were responsible for 47% (n = 8) and 76% (n = 13) of changes in drug resistance interpretation, respectively. In such cases, we conclude that UDS is a robust technique, which still could be improved by increase the RNA and/or DNA extraction in low‐VL samples to detect LFVs. Further studies are needed to define the impact of LFVs on antiretroviral treatments. At last, when considering a DRM, the use of mutational load would probably be more suitable than frequencies.

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HIV-1 Drug Resistance Detected by Next-Generation Sequencing among ART-Naïve Individuals: A Systematic Review and Meta-Analysis

Cited by 2 publications

References 82 publications

Performance of the Applied Biosystems HIV-1 Genotyping Kit with Integrase

Performance of the Applied Biosystems HIV-1 Genotyping Kit with Integrase

The relevance of ultradeep sequencing for low HIV‐1 viral loads and proviruses in the clinical setting

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