A more sensitive platform for the detection of low-abundance BRAFV600E mutations

被引:1
|
作者
Weiqin Jiang
Weibin Wang
FangFang Fu
Xiaodong Teng
Haohao Wang
Haiyong Wang
Lisong Teng
机构
[1] Zhejiang University School of Medicine,Cancer Center, First Affiliated Hospital
[2] Zhejiang University School of Medicine,Institute of Infectious Diseases, First Affiliated Hospital
[3] Zhejiang University School of Medicine,Department of Pathology, First Affiliated Hospital
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关键词
BRAF; Allele-specific real-time PCR; Sanger sequencing; Pyrosequencing;
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摘要
Identifying low-abundance mutations is important for the therapy and diagnose of cancer. Since the potential for tumor heterogeneity, the efficient detection of cancer-relevant mutations largely depends on the sensitivity of the methods employed. To confirm whether the mutation detection platforms affect the perceived prevalence of the BRAFV600E and its correlation with clinicopathologic features in papillary thyroid carcinomas (PTC), we compared Sanger Sequencing (SS), Pyrosequencing (PS), and a newly built allele-specific real-time PCR (AS-qPCR) apparatus for the detection of BRAFV600E in a Chinese cohort of conventional variant PTC. Accurate plasmid standards were built to assess the limit of detection of the three platforms. In this research, AS-qPCR has been found both the most sensitive and reliable at detecting mutation. The mutations detected by AS-qPCR which were not detected by SS or PS due to low abundance were confirmed by mutation enrichment platform COLD-PCR followed by SS. When analyzed by AS-qPCR, BRAFV600E was associated with a more aggressive phenotype. Our results indicate that the reported prevalence of the BRAFV600E mutations in PTC has been underestimated and more sensitive methods such as AS-qPCR should be applied in clinical settings.
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页码:49 / 58
页数:9
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