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通过高分辨率DNA熔解分析进行同步突变扫描和基因分型

Simultaneous mutation scanning and genotyping by high-resolution DNA melting analysis.

作者信息

Montgomery Jesse, Wittwer Carl T, Palais Robert, Zhou Luming

机构信息

Department of Pathology, UUMC, 5B418, 50 N. Medical Drive, Salt Lake City, Utah 84105, USA.

出版信息

Nat Protoc. 2007;2(1):59-66. doi: 10.1038/nprot.2007.10.

Abstract

This protocol permits the simultaneous mutation scanning and genotyping of PCR products by high-resolution DNA melting analysis. This is achieved using asymmetric PCR performed in the presence of a saturating fluorescent DNA dye and unlabeled oligonucleotide probes. Fluorescent melting curves of both PCR amplicons and amplicon-probe duplexes are analyzed. The shape of the PCR amplicon melting transition reveals the presence of heterozygotes, whereas specific genotyping is enabled by melting of the unlabeled probe-amplicon duplex. Unbiased hierarchal clustering of melting transitions automatically groups different sequence variants; this allows common variants to be easily recognized and genotyped. This technique may be used in both laboratory research and clinical settings to study single-nucleotide polymorphisms and small insertions and deletions, and to diagnose associated genetic disorders. High-resolution melting analysis accomplishes simultaneous gene scanning and mutation genotyping in a fraction of the time required when using traditional methods, while maintaining a closed-tube environment. The PCR requires <30 min (capillaries) or 1.5 h (96- or 384-well plates) and melting acquisition takes 1-2 min per capillary or 5 min per plate.

摘要

本方案允许通过高分辨率DNA熔解分析对PCR产物进行同步突变扫描和基因分型。这是通过在饱和荧光DNA染料和未标记的寡核苷酸探针存在下进行不对称PCR来实现的。分析PCR扩增子和扩增子-探针双链体的荧光熔解曲线。PCR扩增子熔解转变的形状揭示了杂合子的存在,而未标记的探针-扩增子双链体的熔解则实现了特定的基因分型。熔解转变的无偏层次聚类自动将不同的序列变异分组;这使得常见变异易于识别和基因分型。该技术可用于实验室研究和临床环境,以研究单核苷酸多态性以及小的插入和缺失,并诊断相关的遗传疾病。高分辨率熔解分析在使用传统方法所需时间的一小部分内完成同步基因扫描和突变基因分型,同时保持封闭管环境。PCR需要<30分钟(毛细管)或1.5小时(96或384孔板),熔解采集每个毛细管需要1-2分钟,每个板需要5分钟。

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