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Major improvement in the detection of microsatellite instability in colorectal cancer using HSP110 T17 E‐ ice ice ‐COLD‐PCR

机译:使用HSP110 T17 E-冰冰在结肠直肠癌中检测微卫星不稳定性的重大改进-Cold-PCR

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摘要

Abstract Every colorectal cancer (CRC) patient should be tested for microsatellite instability (MSI) to screen for Lynch syndrome. Evaluation of MSI status involves screening tumor DNA for the presence of somatic deletions in DNA repeats using PCR followed by fragment analysis. While this method may lack sensitivity due to the presence of a high level of germline DNA, which frequently contaminates the core of primary colon tumors, no other method developed to date is capable of modifying the standard PCR protocol to achieve improvement of MSI detection. Here, we describe a new approach developed for the ultra‐sensitive detection of MSI in CRC based on E‐ ice ‐COLD‐PCR, using HSP110 T17, a mononucleotide DNA repeat previously proposed as an optimal marker to detect MSI in tumor DNA, and an oligo(dT) 16 LNA blocker probe complementary to wild‐type genotypes. The HT17 E‐ ice ‐COLD‐PCR assay improved MSI detection by 20–200‐fold compared with standard PCR using HT17 alone. It presents an analytical sensitivity of 0.1%–0.05% of mutant alleles in wild‐type background, thus greatly improving MSI detection in CRC samples highly contaminated with normal DNA. HT17 E‐ ice ‐COLD‐PCR is a rapid, cost‐effective, easy‐to‐implement, and highly sensitive method, which could significantly improve the detection of MSI in routine clinical testing.
机译:摘要应对每种结肠直肠癌(CRC)患者进行用于晶体综合征的微卫星不稳定性(MSI)进行测试。 MSI状态的评估涉及筛选肿瘤DNA在使用PCR的DNA重复中存在体细胞缺失,然后进行片段分析。虽然这种方法可能由于存在高水平的种系DNA而缺乏敏感性,但是经常污染原色子结肠肿瘤的核心,迄今为止没有发育的其他方法能够改变标准PCR方案以实现MSI检测的改善。在这里,我们描述了一种新的方法,用于基于E-Ice-COLD-PCR,使用HSP110 T17,先前提出的作为最佳标记物以检测肿瘤DNA中MSI的单核苷酸DNA,并且寡核苷酸(DT)16 LNA阻滞剂探针与野生型基因型互补。与单独使用HT17的标准PCR相比,HT17 e-冰-Cold -Cold -Cold -CCR测定改善MSI检测20-200倍。它呈现出野生型背景中突变等位基因0.1%-0.05%的分析敏感性,从而大大改善了具有正常DNA的CRC样品中的MSI检测。 HT17 E-ICOL-COLD-PCR是一种快速,经济效益,易于实施和高度敏感的方法,可显着改善常规临床测试中MSI的检测。

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