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BRCA1 和 BRCA2 基因突变检测下一代测序检测方法的评估。

Evaluation of a Next-Generation Sequencing Assay for BRCA1 and BRCA2 Mutation Detection.

机构信息

Department of Experimental and Clinical Biomedical Sciences Mario Serio, Medical Genetics Unit, University of Florence, Florence, Italy.

Department of Experimental and Clinical Biomedical Sciences Mario Serio, Medical Genetics Unit, University of Florence, Florence, Italy.

出版信息

J Mol Diagn. 2018 Jan;20(1):87-94. doi: 10.1016/j.jmoldx.2017.09.005. Epub 2017 Oct 20.

Abstract

The efficiency of a novel targeted next-generation sequencing (NGS) test, the Devyser BRCA kit, for a comprehensive analysis of all 48 coding exons of the high-risk breast/ovarian cancer susceptibility genes BRCA1 and BRCA2 has been assessed. The new assay intended to detect nucleotide substitutions, small deletions/insertions, and large deletions/duplications. To document the false-negative and false-positive rates of the NGS assay in the hands of end users, 48 samples with previously identified 444 small variants and seven gross rearrangements were analyzed, showing 100% concordance with gold standards. Furthermore, all other 43 variants (42 single-nucleotide variation or insertion/deletion variation and one copy number variation, whose significance is or may be of clinical value), which were called by the NGS assay in a prospectively analyzed 179-sample set, were confirmed by Sanger sequencing or multiplex ligation probe amplification, according to their nature. We conclude that the Devyser BRCA kit performed satisfactorily for use in a clinical laboratory.

摘要

一种新型靶向下一代测序(NGS)检测方法——Devyser BRCA 试剂盒,用于对高风险乳腺癌/卵巢癌易感基因 BRCA1 和 BRCA2 的所有 48 个编码外显子进行全面分析。该新检测方法旨在检测核苷酸取代、小缺失/插入和大片段缺失/重复。为了记录终端用户使用 NGS 检测方法的假阴性和假阳性率,对 48 个先前已鉴定出 444 个小变异体和 7 个大片段重排的样本进行了分析,结果与金标准完全一致。此外,在对一个前瞻性分析的 179 个样本组进行的 NGS 检测中发现的所有其他 43 个变异体(42 个单核苷酸变异或插入/缺失变异体和 1 个拷贝数变异体,其临床意义或可能具有临床价值),均根据其性质通过 Sanger 测序或多重连接探针扩增得到了确认。我们得出结论,Devyser BRCA 试剂盒在临床实验室中表现良好。

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