聚合酶链反应与对抗双对引物多态性基因分型。

N Hamajima, T Saito, K Matsuo, K Kozaki, T Takahashi, K Tajima
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引用次数: 246

摘要

引入了一种新的PCR方法,使用对抗性的两对引物,称为PCR- ctpp,用于检测单核苷酸多态性(碱基X或Y)。X等位基因的一个引物被设置为在3'端包含X'(反义),其中X'是X的反义,对应的义引物在上游。对于Y等位基因,在3'端设置一个包含Y的义引物,在下游设置反义引物。每个等位基因的一个共同带和一个特定带被扩增,这允许直接通过电泳进行基因分型。这种方法被应用于β -肾上腺素能受体2和白细胞介素1B的多态性。它比PCR-RFLP(限制性内切片段长度多态性)更简单,需要用限制性内切酶孵育,适用于涉及数百个样本的遗传流行病学研究。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Polymerase chain reaction with confronting two-pair primers for polymorphism genotyping.

A novel PCR method using confronting two-pair primers, named PCR-CTPP, is introduced to detect a single nucleotide polymorphism (base X or Y). One primer for the X allele is set to include X' at the 3' end (antisense), where X' is the antisense of X, with the counterpart sense primer upstream. For the Y allele, a sense primer including Y at the 3' end is set, with the antisense primer downstream. One common band and one specific band for each allele are amplified, which allows genotyping directly by electrophoresis. This method is exemplified by application to the polymorphisms of beta-adrenoceptor 2 and interleukin 1B. It is simpler than PCR-RFLP (restriction fragment length polymorphism), which requires incubation with a restriction enzyme, and is suitable for genotyping in studies of genetic epidemiology involving hundreds of samples.

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