sensitive detection of braf v600e mutation by amplification refractory mutation system (arms)-pcr敏感的检测braf v600e突变扩增耐火突变系统(武器)pcr.pdfVIP

sensitive detection of braf v600e mutation by amplification refractory mutation system (arms)-pcr敏感的检测braf v600e突变扩增耐火突变系统(武器)pcr.pdf

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sensitive detection of braf v600e mutation by amplification refractory mutation system (arms)-pcr敏感的检测braf v600e突变扩增耐火突变系统(武器)pcr

Huang et al. Biomarker Research 2013, 1:3 /content/1/1/3 METHODOLOGY Open Access Sensitive detection of BRAF V600E mutation by Amplification Refractory Mutation System (ARMS)-PCR Tiangui Huang*†, Jian Zhuge† and Wenyong W Zhang* Abstract Background: BRAF mutations occur in approximately 8% of all human cancers and approach 50% in melanoma and papillary carcinoma of thyroid. These mutations provide potentially valuable diagnostic, prognostic and treatment response prediction markers. A sensitive, specific, low-cost assay to detect these mutations is needed. Results: To detect BRAF V600E mutation in formalin-fixed, paraffin-embedded (FFPE) tissue, we developed a method using Amplification Refractory Mutation System (ARMS)-PCR. This method was designed to amplify three products in a single reaction tube: a 200 bp common product serving as an amplification control, a 144 bp BRAF V600E specific product, and a 97 bp wild-type (wt) specific product. The sensitivity of this method was determined to be as low as 0.5% for the BRAF V600E allele in a wild-type background. This method was successfully validated in 72 thyroid tumors. It detected V600E mutation in 22 out of 33 (67%) of the conventional papillary thyroid carcinoma (PTC), 8 out of 12 (75%) of the tall-cell variant of PTC, whereas none of the 10 follicular variant of PTC showed BRAF V600E mutation. In addition, none of the 14 follicular adenomas and 3 follicular carcinomas had BRAF V600E mutation. As a comparison method, direct dideoxy sequencing found only 27 out of 30 (90%) mutations detected by ARMS-PCR method, suggesting that this ARMS-PCR method has higher sensitivity. Conclusions: Our ARMS-PCR method provides a new tool for rapid detection of BRAF V600E mutation. Our results indicate that ARMS-PCR is more sensitive than automated dideoxy sequencing in d

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