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用于检测与活化蛋白C抵抗相关的因子V突变的序列特异性引物聚合酶链反应。

The polymerase chain reaction with sequence specific primers for the detection of the factor V mutation associated with activated protein C resistance.

作者信息

Kirschbaum N E, Foster P A

机构信息

Hemostasis Reference Laboratory, Blood Center of Southeastern Wisconsin, Milwaukee 53201-2178, USA.

出版信息

Thromb Haemost. 1995 Sep;74(3):874-8.

PMID:8571314
Abstract

The prevalence of the Factor V (FV) mutation associated with activated protein C resistance (FV Leiden) and its significance as a genetic risk factor for venous thrombosis have necessitated the development of a simple, rapid, and accurate assay for its detection. The polymerase chain reaction with sequence specific primers (PCR-SSP) provides a powerful technique for the discrimination of alleles resulting from single base substitutions. PCR amplification was performed using a sense primer complementary to both FV alleles coupled with either of two antisense allele specific primers, one complementary to the normal FV allele and one complementary to the FV Leiden allele. PCR conditions were developed that favored amplification only in the case of perfect complementation between template DNA and allele specific primer. The FV genotype was assigned based on whether or not each allele specific primer set produced an amplified product. Assignment of genotypes correlated 100% with those determined by the method of PCR amplification followed by Mn1I digestion. PCR-SSP allows the rapid and accurate identification of carriers of the Factor V Leiden mutation by a simple PCR reaction without the need for the usual post-amplification specificity step.

摘要

与活化蛋白C抵抗相关的因子V(FV)突变(FV莱顿突变)的患病率及其作为静脉血栓形成遗传风险因素的重要性,使得开发一种简单、快速且准确的检测方法成为必要。序列特异性引物聚合酶链反应(PCR-SSP)为鉴别单碱基取代产生的等位基因提供了一种强大的技术。使用与两种FV等位基因均互补的正义引物以及两种反义等位基因特异性引物之一进行PCR扩增,其中一种反义引物与正常FV等位基因互补,另一种与FV莱顿等位基因互补。开发了PCR条件,该条件仅在模板DNA与等位基因特异性引物完全互补的情况下才有利于扩增。根据每个等位基因特异性引物组是否产生扩增产物来确定FV基因型。基因型的判定与通过PCR扩增后用Mn1I消化的方法所确定的基因型100%相关。PCR-SSP通过简单的PCR反应就能快速、准确地鉴定FV莱顿突变的携带者,而无需通常的扩增后特异性步骤。

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