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在聚合酶链反应中使用通用引物可检测多种人类乳头瘤病毒基因型。

The use of general primers in the polymerase chain reaction permits the detection of a broad spectrum of human papillomavirus genotypes.

作者信息

Snijders P J, van den Brule A J, Schrijnemakers H F, Snow G, Meijer C J, Walboomers J M

机构信息

Department of Pathology, Free University Hospital, Amsterdam, The Netherlands.

出版信息

J Gen Virol. 1990 Jan;71 ( Pt 1):173-81. doi: 10.1099/0022-1317-71-1-173.

Abstract

A novel polymerase chain reaction (PCR) method was developed that permits the detection of 11 different human papillomavirus (HPV) genotypes using two general primer sets. By computer-assisted sequence analysis, two pairs of general primers were selected from the conserved L1 open reading frame and tested in the PCR on a set of cloned HPV genotypes. Experimental analysis showed that up to three mismatches between primers and target DNA did not influence the efficiency of the assay. The use of these primers in the PCR enabled the detection of HPV genotypes HPV-1a, -6, -8, -11, -13, -16, -18, -30, -31, -32 and -33, and was also successfully applied to well characterized cervical carcinoma cell lines and clinical samples. For the HPV types tested sub-picogram amounts of cloned DNA could be detected after general primer-mediated PCR and subsequent hybridization. The specificity of the amplification products was confirmed by blot hybridization procedures and RsaI restriction enzyme digestion. The results indicate that this PCR method can be a powerful tool for identifying novel HPV genotypes in dysplasias and squamous cell carcinomas suspected of having an HPV aetiology.

摘要

开发了一种新型聚合酶链反应(PCR)方法,该方法使用两组通用引物可检测11种不同的人乳头瘤病毒(HPV)基因型。通过计算机辅助序列分析,从保守的L1开放阅读框中选择了两对通用引物,并在PCR中对一组克隆的HPV基因型进行了测试。实验分析表明,引物与靶DNA之间最多三个错配不会影响检测效率。在PCR中使用这些引物能够检测HPV基因型HPV-1a、-6、-8、-11、-13、-16、-18、-30、-31、-32和-33,并且也成功应用于特征明确的宫颈癌细胞系和临床样本。对于所测试的HPV类型,通用引物介导的PCR及随后的杂交后可检测到亚皮克级量的克隆DNA。通过印迹杂交程序和RsaI限制性酶切确认了扩增产物的特异性。结果表明,这种PCR方法可能是一种强大的工具,用于在怀疑由HPV病因引起的发育异常和鳞状细胞癌中鉴定新型HPV基因型。

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