片段长度差异等位基因特异性PCR—一种改良的SNP分型新方法

法医学杂志 ›› 2005, Vol. 0 ›› Issue (1): 11-14.

片段长度差异等位基因特异性PCR—一种改良的SNP分型新方法

黄代新,杨庆恩,赵贵森

华中科技大学同济医学院法医学系,华中科技大学同济医学院法医学系,华中科技大学同济医学院法医学系湖北武汉430030 ,湖北武汉430030 ,湖北武汉430030

发布日期:2005-02-25 出版日期:2005-02-28

A Simple and Rapid Modified -New Method for SNP Typing by Fragment Length Discrepant Allele Specific PCR

HUANG DAI-XIN, YANG QING-EN, ZHAO GUI-SEN (FACULTY OF FORENSIC MEDICINE, TONGJI MEDICAL COLLEGE, HUAZHONG UNIVERSITY OF SCIENCE AND TECHNOLOGY, WUHAN 430030, CHINA)

Online:2005-02-25 Published:2005-02-28

摘要/Abstract

摘要： 目的建立一种基于等位基因特异性PCR原理的改良SNP分型新方法:片段长度差异等位基因特异性PCR,并考察特异性引物的3'端第3位、第4位碱基错配对特异性延伸的影响。方法以SNP位点rs759117和rs760887为例,设计两条长度不同、3'末端分别与SNP两个等位基因碱基配对的上游引物,同时在两个等位基因特异性引物3'端第3或第4位碱基引入错配以增加特异性,下游为公用引物。PCR产物经聚丙烯酰胺凝胶电泳、银染显带后确定样本的基因型。结果不同SNP纯合子为长度不同的单一谱带,杂合子则为两条带,其结果与直接测序完全一致。两条特异性上游引物3'端第3或第4位碱基引入错配后非特异性延伸显著减少,且对PCR反应条件的严格性要求明显降低。结论片段长度差异等位基因特异性PCR是一种简单快速而有效的SNP分型新方法;两条特异性引物3'端第3、第4位碱基引入错配可使特异性显著增加

关键词: 单核苷酸多态性, 片段长度差异等位基因特异性PCR, 碱基错配

Abstract: Objective To establish a new method for single nucleotide polymorphism (SNP) typing based on allele specific PCR: fragment length discrepant allele specific PCR (FLDAS-PCR), and study the influence on specific extension by introducing a mismatch at the third or fourth 3′-terminal base of allele specific primers. Methods For SNP loci rs759117 and rs760887, two allele specific forward primers, with different length and a mismatch introduced at the third or fourth 3′-terminal base, and a public reverse primer were designed for SNP typing. The genotyping of SNP was determined by the two allele specific fragments different in size after polyacrylamide gel and silver staining. Results The different homozygote genotypes comprised a single band with different size respectively, and the heterozygote genotypes comprised two bands. Typing results were completely consistent with those by direct sequencing. Non-specific primer extension was decreased remarkably after introducing a mismatch at the third or fourth 3′-terminal base of allele specific primers, and the stringency of PCR reaction was cut down. Conclusion FLDAS-PCR is a simple, rapid and efficient new method for SNP typing. During FLDAS-PCR, specific primers with a mismatch at the third or fourth 3′-terminal base have more power to identify two alleles.

Key words: single nucleotide polymorphism, fragment length discrepant allele specific PCR, base mismatch

黄代新;杨庆恩;赵贵森. 片段长度差异等位基因特异性PCR—一种改良的SNP分型新方法[J]. 法医学杂志, 2005, 0(1): 11-14.

HUANG DAI-XIN;YANG QING-EN;ZHAO GUI-SEN (FACULTY OF FORENSIC MEDICINE;TONGJI MEDICAL COLLEGE;HUAZHONG UNIVERSITY OF SCIENCE AND TECHNOLOGY;WUHAN 000;CHINA). A Simple and Rapid Modified -New Method for SNP Typing by Fragment Length Discrepant Allele Specific PCR[J]. , 2005, 0(1): 11-14.

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