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Dis Markers. 2013;34(3):171-7. doi: 10.3233/DMA-120960.
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引用本文的文献

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Molecular Biomarkers for the Evaluation of Colorectal Cancer: Guideline From the American Society for Clinical Pathology, College of American Pathologists, Association for Molecular Pathology, and American Society of Clinical Oncology.用于评估结直肠癌的分子生物标志物:美国临床病理学会、美国病理学家学会、分子病理学协会和美国临床肿瘤学会的指南
J Mol Diagn. 2017 Mar;19(2):187-225. doi: 10.1016/j.jmoldx.2016.11.001. Epub 2017 Feb 6.
2
Molecular Biomarkers for the Evaluation of Colorectal Cancer.结直肠癌的分子生物标志物评估。
Am J Clin Pathol. 2017 Mar;147(3):221-260. doi: 10.1093/ajcp/aqw209. Epub 2017 Feb 3.

用于同时检测结直肠癌标本中 FFPE 提取基因组 DNA 中 KRAS/BRAF 突变的双杂交反向杂交检测。

Duplex reverse-hybridization assay for the simultaneous detection of KRAS/BRAF mutations in FFPE-extracted genomic DNA from colorectal cancer specimens.

机构信息

Second Department of Medicine, Donauspital, Vienna, Austria.

出版信息

Dis Markers. 2013;34(3):171-7. doi: 10.3233/DMA-120960.

DOI:10.3233/DMA-120960
PMID:23324583
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3810114/
Abstract

We report the performance evaluation of a non-quantitative reverse-hybridization assay (KRAS-BRAF StripAssay) designed for the simultaneous detection of 10 mutations in codons 12 and 13 of the KRAS gene and BRAF mutation V600E. Dilution experiments using DNA from tumor cell lines or from formalin-fixed paraffin-embedded (FFPE) colorectal cancer (CRC) tissue were performed to assess assay sensitivity. Using 50 ng of total DNA (mutant and wild-type), the KRAS-BRAF StripAssay demonstrated a detection limit of 1% mutant sequence in a background of wild-type DNA. With respect to BRAF V600E, the KRAS-BRAF StripAssay was evaluated using 60 FFPE CRC samples previously analyzed by high resolution melting (HRM). Test strip hybridization identified 2/60 (3%) samples to carry the BRAF V600E mutation, and results were in agreement with those obtained by HRM analysis. This work demonstrates the KRAS-BRAF StripAssay to be a robust and sensitive method for the detection of common KRAS/BRAF mutations in genomic DNA isolated from FFPE tissue samples.

摘要

我们报告了一种非定量反向杂交检测方法(KRAS-BRAF StripAssay)的性能评估,该方法旨在同时检测 KRAS 基因 12 和 13 密码子中 10 种突变和 BRAF 突变 V600E。使用来自肿瘤细胞系或福尔马林固定石蜡包埋(FFPE)结直肠癌(CRC)组织的 DNA 进行稀释实验,以评估检测方法的灵敏度。使用 50ng 总 DNA(突变型和野生型),KRAS-BRAF StripAssay 显示出在野生型 DNA 背景下检测 1%突变序列的检测限。关于 BRAF V600E,使用先前通过高分辨率熔解(HRM)分析的 60 个 FFPE CRC 样本对 KRAS-BRAF StripAssay 进行了评估。测试条杂交鉴定出 2/60(3%)个样本携带 BRAF V600E 突变,结果与 HRM 分析结果一致。这项工作表明,KRAS-BRAF StripAssay 是一种从 FFPE 组织样本中分离的基因组 DNA 中检测常见 KRAS/BRAF 突变的稳健且敏感的方法。