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A Streamlined Mutation Detection System: Multicolor Post-PCR Fluorescence Labeling and Single-Strand Conformational Polymorphism Analysis by Capillary Electrophoresis

机译:简化的突变检测系统:多色后PCR荧光标记和毛细管电泳分析单链构象多态性

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摘要

Effective use of knowledge of human genome sequences in studies of hereditary diseases or cancer heavily depends on efficient methods for detection of mutations in individual samples. We describe here a simple and efficient mutation scanning system in which PCR products are post-labeled with two different fluorescent dyes in one tube, and analyzed by an automated capillary electrophoresis system using single-strand conformation polymorphism (SSCP) conditions (PLACE–SSCP). With the appropriate use of an internal control DNA, differences in electrophoretic mobilities between a reference and samples are precisely evaluated, then the presence of mutations is statistically judged. Thirty-three of 34 known mutations in fragments of three unrelated sequence contexts up to 741 bp were detected using one electrophoresis condition at the confidence level of <0.3% false positive. All the mutations were detected by analyzing at two temperatures. The described system has the advantage of little human intervention, short analysis time, high sensitivity, and objectivity of data interpretation.
机译:在遗传性疾病或癌症研究中有效利用人类基因组序列的知识在很大程度上取决于检测单个样本中突变的有效方法。我们在这里描述一个简单而有效的突变扫描系统,在该系统中,PCR产品在一根试管中用两种不同的荧光染料进行后标记,然后通过使用单链构象多态性(SSCP)条件(PLACE–SSCP)的自动毛细管电泳系统进行分析。通过适当使用内部对照DNA,可以精确评估参比样品与样品之间电泳迁移率的差异,然后从统计学上判断突变的存在。使用一种电泳条件,在<0.3%假阳性的置信水平下,检测到三个最长741 bp的无关序列上下文片段中的34个已知突变中的33个。通过在两个温度下分析来检测所有突变。所描述的系统具有人工干预少,分析时间短,灵敏度高和数据解释的客观性的优点。

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