Division of Medical Sciences, National Cancer Centre, Singapore, Singapore.
J Mol Diagn. 2012 Nov;14(6):602-12. doi: 10.1016/j.jmoldx.2012.06.003. Epub 2012 Aug 22.
In a clinical setting, next-generation sequencing (NGS) approaches for the enrichment and resequencing of DNA targets may have limitations in throughput, cost, or accuracy. We evaluated an NGS workflow for targeted DNA sequencing for mutation detection. Targeted sequence data of the BRCA1 and BRCA2 genes, generated using a PCR-based, multiplexed NGS approach using the SOLiD 4 (n = 24) and Ion Torrent PGM (n = 20) next-generation sequencers, were evaluated against sequence data obtained by Sanger sequencing. The overall sensitivity for SOLiD and PGM were 97.8% (95% CI = 94.7 to 100.0) and 98.9% (95% CI = 96.8 to 100.0) respectively. The specificity for the SOLiD platform was high, at 100.0% (95% CI = 99.3 to 100.0). PGM correctly identified all 3 indels, but 68 false-positive indels were also called. Equimolar normalization of amplicons was not necessary for successful NGS. Both platforms are highly amenable to scale-up, potentially reducing the reagent cost for BRCA testing to <US$200. Only 325 ng of DNA per patient is required, with similar coverage and accuracy obtained using DNA derived from peripheral blood or buccal wash samples. The strategy described is accurate and easy to incorporate into conventional workflow, and shows potential for mutation screening of clinically important gene targets in genetic disorders.
在临床环境中,下一代测序(NGS)方法在 DNA 目标的富集和重测序方面可能存在通量、成本或准确性方面的限制。我们评估了一种用于突变检测的靶向 DNA 测序的 NGS 工作流程。使用基于 PCR 的多重 NGS 方法生成 BRCA1 和 BRCA2 基因的靶向序列数据,该方法使用 SOLiD 4(n = 24)和 Ion Torrent PGM(n = 20)下一代测序仪,与通过 Sanger 测序获得的序列数据进行了评估。SOLiD 和 PGM 的总体灵敏度分别为 97.8%(95%CI=94.7 至 100.0)和 98.9%(95%CI=96.8 至 100.0)。SOLiD 平台的特异性很高,为 100.0%(95%CI=99.3 至 100.0)。PGM 正确识别了所有 3 个插入缺失,但也有 68 个假阳性插入缺失被检出。扩增子的等摩尔归一化不是成功进行 NGS 的必要条件。两个平台都非常适合扩展,可能将 BRCA 检测的试剂成本降低到<200 美元。每个患者只需要 325ng 的 DNA,使用外周血或口腔洗液样本获得的 DNA 具有相似的覆盖度和准确性。所描述的策略准确且易于纳入常规工作流程,并且具有在遗传疾病中筛选临床重要基因靶标的突变的潜力。
