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在Rotor-Gene 2000上使用荧光共振能量转移杂交探针通过多重实时聚合酶链反应对凝血因子V Leiden(G1691A)和凝血酶原(G20210A)进行联合基因分型。

Combined factor V leiden (G1691A) and prothrombin (G20210A) genotyping by multiplex real-time polymerase chain reaction using fluorescent resonance energy transfer hybridization probes on the Rotor-Gene 2000.

作者信息

Ameziane Nejma, Lamotte Maryse, Lamoril Jérôme, Lebret Dominique, Deybach Jean-Charles, Kaiser Thomas, de Prost Dominique

机构信息

Service d'Hématologie Biologique et d'lmmunologie, Hôpital Louis Mourier, AP-HP, Colombes, France.

出版信息

Blood Coagul Fibrinolysis. 2003 Jun;14(4):421-4. doi: 10.1097/00001721-200306000-00016.

Abstract

Several methods have been developed to detect common single point mutations in the factor V and prothrobin genes that are risk factors for thrombophilia. Most are based on PCR followed by restriction enzyme digestion and electrophoresis (RFLP), but gel analysis has certain limitations, and alternative detection methods, including real-time PCR, have therefore been developed. In this study we developed and evaluated a combined factor V Leiden and prothrombin (G20210A) genotyping method based on multiplex real-time PCR with fluorescent resonance energy transfer (FRET) hybridization probes on the Rotor-Gene 2000. Two hundred subjects were screened for the two mutations. The FRET assay clearly discriminated among wild-type, homozygous and heterozygous status for the two mutations, and the results were in full agreement with those of the RFLP assay. This robust FRET probe-based assay also has a higher throughput capacity than conventional methods, handling up to 72 samples in 90 min.

摘要

已经开发出几种方法来检测凝血因子V和凝血酶原基因中的常见单点突变,这些突变是血栓形成倾向的危险因素。大多数方法基于聚合酶链反应(PCR),随后进行限制性内切酶消化和电泳(RFLP),但凝胶分析有一定局限性,因此已开发出包括实时PCR在内的替代检测方法。在本研究中,我们基于Rotor-Gene 2000上的荧光共振能量转移(FRET)杂交探针的多重实时PCR,开发并评估了一种联合检测凝血因子V莱顿突变和凝血酶原(G20210A)突变的基因分型方法。对200名受试者进行了这两种突变的筛查。FRET分析能够清晰地区分两种突变的野生型、纯合子和杂合子状态,结果与RFLP分析完全一致。这种基于FRET探针的可靠检测方法还具有比传统方法更高的通量,在90分钟内可处理多达72个样本。

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