Replacing PCR with COLD-PCR enriches variant DNA sequences and redefines the sensitivity of genetic testing

冷PCR PCR变异 基因分型 生物 聚合酶链反应 遗传学 基因型 PCR的应用 多重位移放大 等位基因 底漆(化妆品) 突变 分子生物学 基因 数字聚合酶链反应 DNA提取 点突变 有机化学 化学
作者
Jin Li,Xin Lin,Harvey J. Mamon,Matthew H. Kulke,Ross Berbeco,G. Mike Makrigiorgos
出处
期刊:Nature Medicine [Springer Nature]
卷期号:14 (5): 579-584 被引量:373
标识
DOI:10.1038/nm1708
摘要

PCR is widely employed as the initial DNA amplification step for genetic testing. However, a key limitation of PCR-based methods is the inability to selectively amplify low levels of mutations in a wild-type background. As a result, downstream assays are limited in their ability to identify subtle genetic changes that can have a profound impact in clinical decision-making and outcome. Here we describe co-amplification at lower denaturation temperature PCR (COLD-PCR), a novel form of PCR that amplifies minority alleles selectively from mixtures of wild-type and mutation-containing sequences irrespective of the mutation type or position on the sequence. We replaced regular PCR with COLD-PCR before sequencing or genotyping assays to improve mutation detection sensitivity by up to 100-fold and identified new mutations in the genes encoding p53, KRAS and epidermal growth factor in heterogeneous cancer samples that had been missed by the currently used methods. For clinically relevant microdeletions, COLD-PCR enabled exclusive amplification and isolation of the mutants. COLD-PCR will transform the capabilities of PCR-based genetic testing, including applications in cancer, infectious diseases and prenatal identification of fetal alleles in maternal blood.
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