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Characterization of the genome of human enteroviruses: Design of generic primers for amplification and sequencing of different regions of the viral genome.

机译:人类肠道病毒基因组的表征:设计通用引物,用于扩增和测序病毒基因组的不同区域。

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摘要

Human enteroviruses are among the most common viruses infecting humans and can cause diverse clinical syndromes ranging from minor febrile illness to severe and potentially fatal diseases. Biodiversity and evolution of human enterovirus genomes are shaped by frequent recombination events. Therefore, identification and characterization of circulating strains of enteroviruses require partial determination of different genomic regions. The development is described of a simple method allowing amplification and partial sequencing of the P1, P2 and P3 genomic regions of field human enterovirus strains isolated in cell cultures, by performing PCR on cDNAs generated through a single RT reaction. A set of generic primers were designed and tested on a panel of 90 field and prototype viruses belonging to the five species of human enteroviruses. This assay was shown to amplify efficiently the targeted regions of all the 90 genomes tested. The generated amplicons were sequenced successfully without the need for gelpurification. This assay could be a valuable tool for laboratories interested in molecular epidemiology and evolution studies implicating a great number of human enterovirus strains isolated from human or environmental samples.
机译:人肠病毒是最常见的人类感染病毒,可引起多种临床综合征,从轻度发热到严重甚至可能致命的疾病。人类肠道病毒基因组的生物多样性和进化受频繁的重组事件影响。因此,鉴定和鉴定肠病毒的循环株需要部分测定不同的基因组区域。描述了一种简单方法的开发,该方法通过对通过单个RT反应生成的cDNA进行PCR,可以扩增和部分测序在细胞培养物中分离的现场人肠病毒株的P1,P2和P3基因组区域。在一组属于人类肠道病毒五种的90种田间和原型病毒中设计并测试了一组通用引物。结果表明,该试验可有效扩增所有90个基因组的靶区域。无需凝胶纯化即可成功测序产生的扩增子。对于那些对分子流行病学和进化研究感兴趣的实验室来说,该分析法可能是一种有价值的工具,其中涉及从人类或环境样品中分离出的许多人类肠道病毒株。

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