用于常规快速检测BRCA1和BRCA2种系突变的Ion Torrent PGM测序流程评估。
Evaluation of the Ion Torrent PGM sequencing workflow for the routine rapid detection of BRCA1 and BRCA2 germline mutations.
作者信息
Zanella Isabella, Merola Francesca, Biasiotto Giorgio, Archetti Silvana, Spinelli Elide, Di Lorenzo Diego
机构信息
Biotechnology Laboratory and Department of Diagnostics, Civic Hospital of Brescia, Brescia, Italy; Department of Molecular and Translational Medicine, University of Brescia, Brescia, Italy.
Biotechnology Laboratory and Department of Diagnostics, Civic Hospital of Brescia, Brescia, Italy.
出版信息
Exp Mol Pathol. 2017 Apr;102(2):314-320. doi: 10.1016/j.yexmp.2017.03.001. Epub 2017 Mar 2.
PURPOSE
Conventional methods used to identify BRCA1/2 germline mutations in hereditary cancers are time-consuming and expensive, due to the large size of the genes. The recent introduction of next generation sequencing (NGS) benchtop platforms is a great promise, which is rapidly revolutionizing genetic screening in diagnostic and clinical applications. We recently transferred our methodology for routine BRCA1/2 mutation screening (denaturing High Performance Liquid Chromatography plus Sanger sequencing) to the Ion Torrent PGM platform with the Ion Ampliseq BRCA1 and BRCA2 panel and tested the performance of the system.
METHODS
We first validated the NGS approach in a cohort of 33 patients who had previously undergone genetic diagnosis in our laboratory by conventional methods. Then, we tested 29 newly diagnosed and uncharacterized patients by NGS, and Sanger sequencing was used to confirm results from the NGS platform.
RESULTS
In the validation cohort, all previously identified single nucleotide variants, insertions and deletions (also composed of multiple bases and within complex homopolymeric stretches) were identified by NGS in their correct zygosity status except for variants in a complex multinucleotide region within intron 7 of BRCA1 gene. NGS approach was further able to identify previously undetected variants. In the prospective cohort, almost all (99.3%) called variants were confirmed by Sanger. In both cohorts, in addition to the false positive (31) and false negative (110) results in the intron 7 of BRCA1 gene, the NGS method detected 10 false positives, that were solved by Sanger.
CONCLUSIONS
The Ion Torrent PGM NGS approach in BRCA1/2 germline mutation identification is highly sensitive, easy to use, faster and cheaper than traditional approaches. Therefore, according to other recently published works, we highly recommend this system for routine diagnostic testing on BRCA1/2 genes, along with Sanger confirmation of the called variants, and support the usefulness of the approach also in other routine genetic analysis.
目的
由于基因规模庞大,用于识别遗传性癌症中BRCA1/2种系突变的传统方法既耗时又昂贵。新一代测序(NGS)台式平台的近期引入前景广阔,正在迅速革新诊断和临床应用中的基因筛查。我们最近将常规BRCA1/2突变筛查方法(变性高效液相色谱法加桑格测序法)转移至配备Ion Ampliseq BRCA1和BRCA2检测板的Ion Torrent PGM平台,并测试了该系统的性能。
方法
我们首先在一组33例先前已在我们实验室通过传统方法进行基因诊断的患者中验证了NGS方法。然后,我们通过NGS对29例新诊断且未明确特征的患者进行检测,并使用桑格测序法确认NGS平台的结果。
结果
在验证队列中,除了BRCA1基因第7内含子内一个复杂多核苷酸区域中的变异外,所有先前鉴定出的单核苷酸变异、插入和缺失(也由多个碱基组成且在复杂的同聚物延伸区内)均通过NGS以其正确的纯合性状态被鉴定出来。NGS方法还能够鉴定出先前未检测到的变异。在前瞻性队列中,几乎所有(99.3%)检测到的变异都通过桑格测序法得到了确认。在两个队列中,除了BRCA1基因第7内含子中的假阳性(31个)和假阴性(110个)结果外,NGS方法还检测到10例假阳性,这些通过桑格测序法得以解决。
结论
Ion Torrent PGM NGS方法在BRCA1/2种系突变鉴定中高度灵敏,易于使用,比传统方法更快且更便宜。因此,根据其他近期发表的研究成果,我们强烈推荐该系统用于BRCA1/2基因的常规诊断检测,并对检测到的变异进行桑格测序确认,同时支持该方法在其他常规基因分析中的实用性。
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