通过 V3 基因分型提高对 CXCR4 使用的 HIV 的检测:基于人群的和“深度”测序在血浆 RNA 和前病毒 DNA 中的应用。
Improved detection of CXCR4-using HIV by V3 genotyping: application of population-based and "deep" sequencing to plasma RNA and proviral DNA.
机构信息
British Columbia Centre for Excellence in HIV/AIDS, Vancouver, Canada.
出版信息
J Acquir Immune Defic Syndr. 2010 Aug;54(5):506-10. doi: 10.1097/QAI.0b013e3181d0558f.
BACKGROUND
Tropism testing should rule out CXCR4-using HIV before treatment with CCR5 antagonists. Currently, the recombinant phenotypic Trofile assay (Monogram) is most widely utilized; however, genotypic tests may represent alternative methods.
METHODS
Independent triplicate amplifications of the HIV gp120 V3 region were made from either plasma HIV RNA or proviral DNA. These underwent standard, population-based sequencing with an ABI3730 (RNA n = 63; DNA n = 40), or "deep" sequencing with a Roche/454 Genome Sequencer-FLX (RNA n = 12; DNA n = 12). Position-specific scoring matrices (PSSMX4/R5) (-6.96 cutoff) and geno2pheno[coreceptor] (5% false-positive rate) inferred tropism from V3 sequence. These methods were then independently validated with a separate, blinded dataset (n = 278) of screening samples from the maraviroc MOTIVATE trials.
RESULTS
Standard sequencing of HIV RNA with PSSM yielded 69% sensitivity and 91% specificity, relative to Trofile. The validation dataset gave 75% sensitivity and 83% specificity. Proviral DNA plus PSSM gave 77% sensitivity and 71% specificity. "Deep" sequencing of HIV RNA detected >2% inferred-CXCR4-using virus in 8/8 samples called non-R5 by Trofile, and <2% in 4/4 samples called R5.
CONCLUSIONS
Triplicate analyses of V3 standard sequence data detect greater proportions of CXCR4-using samples than previously achieved. Sequencing proviral DNA and "deep" V3 sequencing may also be useful tools for assessing tropism.
背景
在使用 CCR5 拮抗剂进行治疗之前,应当通过嗜性测试排除使用 CXCR4 的 HIV。目前,最广泛应用的是重组表型 Trofile 检测(Monogram);然而,基因型检测可能是另一种方法。
方法
从血浆 HIV RNA 或前病毒 DNA 中独立地进行 HIV gp120 V3 区的重复扩增。这些扩增产物接受标准的、基于群体的测序,采用 ABI3730(RNA n = 63;DNA n = 40),或 Roche/454 Genome Sequencer-FLX(RNA n = 12;DNA n = 12)的“深度”测序。位置特异性评分矩阵(PSSMX4/R5)(-6.96 截断值)和 geno2pheno[核心受体](5%假阳性率)根据 V3 序列推断嗜性。然后,通过来自 maraviroc MOTIVATE 试验的独立、盲法数据集(n = 278)对这些方法进行独立验证。
结果
与 Trofile 相比,用 PSSM 对 HIV RNA 进行标准测序,敏感性为 69%,特异性为 91%。验证数据集的敏感性为 75%,特异性为 83%。前病毒 DNA 加 PSSM 的敏感性为 77%,特异性为 71%。在 8/8 个 Trofile 鉴定为非 R5 的样本中,用 HIV RNA 的“深度”测序检测到 >2%推断的 CXCR4 使用病毒,而在 4/4 个鉴定为 R5 的样本中检测到 <2%。
结论
V3 标准序列数据的三重分析比以前的方法检测到更多比例的 CXCR4 使用样本。测序前病毒 DNA 和“深度”V3 测序也可能是评估嗜性的有用工具。
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