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The use of real-time PCR methods in DNA sequence variation analysis.

机译:在DNA序列变异分析中使用实时PCR方法。

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摘要

BACKGROUND: Real-time (RT) PCR methods for discovering and genotyping single nucleotide polymorphisms (SNPs) are becoming increasingly important in various fields of biological sciences. SNP genotyping is widely used to perform genetic association studies aimed at characterising the genetic factors underlying inherited traits. The detection and quantification of somatic mutations is an important tool for investigating the genetic causes of tumorigenesis. In infectious disease diagnostics there is an increasing emphasis placed on genotyping variation within the genomes of pathogenic organisms in order to distinguish between strains. METHODS: There are several platforms and methods available to the researcher wishing to undertake SNP analysis using real-time PCR methods. These use fluorescent technologies for discriminating between the alternate alleles of a polymorphism. There are several real-time PCR platforms currently on the market. Two of the key technical challenges are allele discrimination and allele quantification. CONCLUSIONS: Applications of this technology include SNP genotyping, the sensitive detection of somatic mutations and infectious disease subtyping.
机译:背景:在生物科学的各个领域中,用于发现和基因分型单核苷酸多态性(SNP)的实时(RT)PCR方法变得越来越重要。 SNP基因分型被广泛用于进行遗传关联研究,目的是表征遗传特征的遗传因素。体细胞突变的检测和定量是研究肿瘤发生的遗传原因的重要工具。在传染病诊断中,为了区分菌株,越来越强调致病生物基因组内的基因分型变异。方法:有几种平台和方法可供研究人员使用实时PCR方法进行SNP分析。这些使用荧光技术来区分多态性的交替等位基因。当前市场上有几种实时PCR平台。技术上的两个主要挑战是等位基因识别和等位基因定量。结论:该技术的应用包括SNP基因分型,体细胞突变的敏感检测和传染病亚型。

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