Next generation sequencing based in-house HIV genotyping method: validation report

Alisen Ayitewala; Isaac Ssewanyana; Charles Kiyaga

doi:10.1186/s12981-021-00390-8

Next generation sequencing based in-house HIV genotyping method: validation report

AIDS Res Ther. 2021 Oct 2;18(1):64. doi: 10.1186/s12981-021-00390-8.

Authors

Alisen Ayitewala¹, Isaac Ssewanyana², Charles Kiyaga²

Affiliations

¹ National Health Laboratories and Diagnostic Services, Central Public Health Laboratories, Ministry of Health, P.O Box 7272, Kampala, Uganda. ayitewala@gmail.com.
² National Health Laboratories and Diagnostic Services, Central Public Health Laboratories, Ministry of Health, P.O Box 7272, Kampala, Uganda.

Abstract

Background: HIV genotyping has had a significant impact on the care and treatment of HIV/AIDS. At a clinical level, the test guides physicians on the choice of treatment regimens. At the surveillance level, it informs policy on consolidated treatment guidelines and microbial resistance control strategies. Until recently, the conventional test has utilized the Sanger sequencing (SS) method. Unlike Next Generation Sequencing (NGS), SS is limited by low data throughput and the inability of detecting low abundant drug-resistant variants. NGS can improve sensitivity and quantitatively identify low-abundance variants; in addition, it has the potential to improve efficiency as well as lowering costs when samples are batched. Despite the NGS benefits, its utilization in clinical drug resistance profiling is faced with mixed reactions. These are largely based on a lack of a consensus regarding the quality control strategy. Nonetheless, transitional views suggest validating the method against the gold-standard SS. Therefore, we present a validation report of an NGS-based in-house HIV genotyping method against the SS method in Uganda.

Results: Since there were no established proficiency test panels for NGS-based HIV genotyping, 15 clinical plasma samples for routine care were utilized. The use of clinical samples allowed for accuracy and precision studies. The workflow involved four main steps; viral RNA extraction, targeted amplicon generation, amplicon sequencing and data analysis. Accuracy of 98% with an average percentage error of 3% was reported for the NGS based assay against the SS platform demonstrating similar performance. The coefficient of variation (CV) findings for both the inter-run and inter-personnel precision showed no variability (CV ≤ 0%) at the relative abundance of ≥ 20%. For both inter-run and inter-personnel, a variation that affected the precision was observed at 1% frequency. Overall, for all the frequencies, CV registered a small range of (0-2%).

Conclusion: The NGS-based in-house HIV genotyping method fulfilled the minimum requirements that support its utilization for drug resistance profiling in a clinical setting of a low-income country. For more inclusive quality control studies, well-characterized wet panels need to be established.

Keywords: HIV Genotyping; Next Generation Sequencing; Sanger Sequencing; Uganda.

MeSH terms

Drug Resistance, Viral / genetics
Genotype
HIV Infections* / diagnosis
HIV Infections* / drug therapy
HIV-1* / genetics
High-Throughput Nucleotide Sequencing
Humans
Mutation