一项使用454超深度焦磷酸测序技术进行的HIV-1耐药性和嗜性检测多中心协作研究的随访
A Follow-Up of the Multicenter Collaborative Study on HIV-1 Drug Resistance and Tropism Testing Using 454 Ultra Deep Pyrosequencing.
作者信息
St John Elizabeth P, Simen Birgitte B, Turenchalk Gregory S, Braverman Michael S, Abbate Isabella, Aerssens Jeroen, Bouchez Olivier, Gabriel Christian, Izopet Jacques, Meixenberger Karolin, Di Giallonardo Francesca, Schlapbach Ralph, Paredes Roger, Sakwa James, Schmitz-Agheguian Gudrun G, Thielen Alexander, Victor Martin, Metzner Karin J, Däumer Martin P
机构信息
454 Life Sciences, A Roche Company, Branford, CT, United States of America.
National Institute for Infectious Diseases "L. Spallanzani, Rome, Italy.
出版信息
PLoS One. 2016 Jan 12;11(1):e0146687. doi: 10.1371/journal.pone.0146687. eCollection 2016.
BACKGROUND
Ultra deep sequencing is of increasing use not only in research but also in diagnostics. For implementation of ultra deep sequencing assays in clinical laboratories for routine diagnostics, intra- and inter-laboratory testing are of the utmost importance.
METHODS
A multicenter study was conducted to validate an updated assay design for 454 Life Sciences' GS FLX Titanium system targeting protease/reverse transcriptase (RTP) and env (V3) regions to identify HIV-1 drug-resistance mutations and determine co-receptor use with high sensitivity. The study included 30 HIV-1 subtype B and 6 subtype non-B samples with viral titers (VT) of 3,940-447,400 copies/mL, two dilution series (52,129-1,340 and 25,130-734 copies/mL), and triplicate samples. Amplicons spanning PR codons 10-99, RT codons 1-251 and the entire V3 region were generated using barcoded primers. Analysis was performed using the GS Amplicon Variant Analyzer and geno2pheno for tropism. For comparison, population sequencing was performed using the ViroSeq HIV-1 genotyping system.
RESULTS
The median sequencing depth across the 11 sites was 1,829 reads per position for RTP (IQR 592-3,488) and 2,410 for V3 (IQR 786-3,695). 10 preselected drug resistant variants were measured across sites and showed high inter-laboratory correlation across all sites with data (P<0.001). The triplicate samples of a plasmid mixture confirmed the high inter-laboratory consistency (mean% ± stdev: 4.6 ±0.5, 4.8 ±0.4, 4.9 ±0.3) and revealed good intra-laboratory consistency (mean% range ± stdev range: 4.2-5.2 ± 0.04-0.65). In the two dilutions series, no variants >20% were missed, variants 2-10% were detected at most sites (even at low VT), and variants 1-2% were detected by some sites. All mutations detected by population sequencing were also detected by UDS.
CONCLUSIONS
This assay design results in an accurate and reproducible approach to analyze HIV-1 mutant spectra, even at variant frequencies well below those routinely detectable by population sequencing.
背景
超深度测序不仅在研究中,而且在诊断中使用越来越多。为了在临床实验室中实施超深度测序检测用于常规诊断,实验室内和实验室间检测至关重要。
方法
进行了一项多中心研究,以验证针对454生命科学公司的GS FLX Titanium系统的更新检测设计,该设计靶向蛋白酶/逆转录酶(RTP)和env(V3)区域,以高灵敏度鉴定HIV-1耐药突变并确定共受体使用情况。该研究包括30份HIV-1 B亚型和6份非B亚型样本,病毒载量(VT)为3,940 - 447,400拷贝/毫升,两个稀释系列(52,129 - 1,340和25,130 - 734拷贝/毫升),以及一式三份的样本。使用条形码引物生成跨越PR密码子10 - 99、RT密码子1 - 251和整个V3区域的扩增子。使用GS Amplicon Variant Analyzer和geno2pheno进行嗜性分析。为作比较,使用ViroSeq HIV-1基因分型系统进行群体测序。
结果
11个位点的RTP测序深度中位数为每个位置1,829条读数(四分位距592 - 3,488),V3为2,410条读数(四分位距786 - 3,695)。在各位点测量了10个预先选定的耐药变异体,所有位点的数据显示实验室间具有高度相关性(P<0.001)。质粒混合物的一式三份样本证实了实验室间的高度一致性(平均值%±标准差:4.6±0.5、4.8±0.4、4.9±0.3),并显示出良好的实验室内一致性(平均值%范围±标准差范围:4.2 - 5.2±0.04 - 0.65)。在两个稀释系列中,未遗漏任何>20%的变异体,大多数位点检测到2 - 10%的变异体(即使在低病毒载量时),一些位点检测到1 - 2%的变异体。群体测序检测到的所有突变也被超深度测序检测到。
结论
即使在变异频率远低于群体测序常规可检测频率的情况下,这种检测设计也能产生一种准确且可重复的方法来分析HIV-1突变谱。
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