Next-generation sequencing of dried blood spot specimens: a novel approach to HIV drug-resistance surveillance

被引:30
作者
Ji, Hezhao [1 ]
Li, Yang [1 ]
Graham, Morag [2 ,3 ]
Liang, Ben Binhua
Pilon, Richard [1 ]
Tyson, Shari [2 ]
Peters, Geoff [2 ]
Tyler, Shaun [2 ]
Merks, Harriet [1 ]
Bertagnolio, Silvia [4 ]
Soto-Ramirez, Luis [5 ]
Sandstrom, Paul [1 ]
Brooks, James [1 ]
机构
[1] Publ Hlth Agcy Canada, Natl Microbiol Lab, Natl HIV & Retrovirol Labs, Ottawa, ON, Canada
[2] Publ Hlth Agcy Canada, Natl Microbiol Lab, Genom Core Facil, Winnipeg, MB, Canada
[3] Univ Manitoba, Dept Med Microbiol, Winnipeg, MB, Canada
[4] WHO, CH-1211 Geneva, Switzerland
[5] Inst Nacl Ciencias Med & Nutr Salvador Zubiran, Dept Infect Dis, Mexico City, DF, Mexico
关键词
HUMAN GUT MICROBIOTA; TREATMENT-NAIVE; VARIANTS; THERAPY;
D O I
10.3851/IMP1839
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Background: HIV drug-resistance (DR) surveillance in resource-limited settings can be performed using dried blood spots (DBS) because of ease of collection, transportation and storage. Analysis of pooled specimens on next-generation sequencing (NGS)-based platforms, such as the 454 pyrosequencing, is an efficient sequencing method for determining HIV DR rates. In this study, we conducted HIV DR surveillance on DBS using NGS and identified minority variants in individual patients. Methods: A total of 48 extracts of DBS from an HIV DR surveillance study in Mexico City were re-amplified using primers tagged with multiplex identifiers, pooled and pyrosequenced. Consensus sequences were generated for each specimen with mixtures identified at positions where >20% of the reads contained a variant. Individual consensus sequences were then analysed for DR mutations and compared with those derived from Sanger sequencing. Results: DBS analysed with tagged pooled pyrosequencing (TPP) were highly concordant with Sanger sequencing genotypes from matching plasma and DBS (99.21% and 99.51%, respectively). An exception was an M184I mutation only detected with TPP of DBS at a frequency of 20.4%. Multiple specimens had minority variant reads below the 20% mixture threshold. Conclusions: TPP using DBS is an effective method for HIV DR surveillance. TPP for genotyping results in cost savings of 40% over conventional in-house methods. The effect of low-abundance DR mutations, undetectable by conventional methods, remains to be determined. This technology might be applied to any HIV specimen (plasma/serum) and can also be used for other diagnostic assays where DNA sequencing is required.
引用
收藏
页码:871 / 878
页数:8
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