数字聚合酶链反应
多路复用
放大器
肺癌
多重聚合酶链反应
生物
分子生物学
聚合酶链反应
基因
医学
肿瘤科
癌症研究
生物信息学
遗传学
作者
Igor P. Oscorbin,Maria A. Smertina,Ksenia A. Pronyaeva,Mikhail Evgenyevich Voskoboev,U. A. Boyarskikh,Andrey Kechin,Ирина Демидова,М. Л. Филипенко
出处
期刊:Cancers
[Multidisciplinary Digital Publishing Institute]
日期:2022-03-11
卷期号:14 (6): 1458-1458
被引量:10
标识
DOI:10.3390/cancers14061458
摘要
Non-small-cell lung cancer (NSCLC), a subtype of lung cancer, remains one of the most common tumors with a high mortality and morbidity rate. Numerous targeted drugs were implemented or are now developed for the treatment of NSCLC. Two genes, HER2 and MET, are among targets for these specific therapeutic agents. Alterations in HER2 and MET could lead to primary or acquired resistance to commonly used anti-EGFR drugs. Using current methods for detecting HER2 and MET amplifications is time and labor-consuming; alternative methods are required for HER2 and MET testing. We developed the first multiplex droplet digital PCR assay for the simultaneous detection of MET and HER2 amplification in NSCLC samples. The suitability of qPCR was assessed for the optimization of multiplex ddPCR. The optimal elongation temperature, reference genes for DNA quantification, and amplicon length were selected. The developed ddPCR was validated on control samples with various DNA concentrations and ratios of MET and HER2 genes. Using ddPCR, 436 EGFR-negative NSCLC samples were analyzed. Among the tested samples, five specimens (1.15%) showed a higher ratio of MET, and six samples (1.38%) showed a higher ratio of HER2. The reported multiplex ddPCR assay could be used for the routine screening of MET and HER2 amplification in NSCLC samples.
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