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首页> 外文期刊>Journal of Clinical Microbiology >Detection of rubella virus gene sequences by enzymatic amplification and direct sequencing of amplified DNA.
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Detection of rubella virus gene sequences by enzymatic amplification and direct sequencing of amplified DNA.

机译:通过酶促扩增和直接测序扩增的DNA来检测风疹病毒基因序列。

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We developed a rapid and sensitive polymerase chain reaction (PCR) assay for detecting and identifying rubella virus (RV). A segment of the RV gene which encodes the E1 membrane glycoprotein of RV was selected as a target for PCR amplification. Single-stranded viral RNA, extracted from infected cells or released from virions, was used as a template for reverse transcription followed by PCR amplification with two different sets of primer pairs, one nested within the other. The amplified E1 gene sequences were detected in ethidium bromide-stained agarose minigels, and their identities were verified by restriction enzyme digestion and hybridization to a probe directed at a site within the PCR target. Single-stranded DNA generated by asymmetric amplification of the target was directly sequenced by using fluorescent dideoxy-terminators and an automated procedure in order to confirm the target sequence. This PCR assay provides a rapid confirmatory test for the detection of RV by cell culture and appears to have considerable potential for the direct detection of RV in clinical specimens. The strategy used in the development of this PCR assay should be useful for developing other diagnostic PCR assays for viruses.
机译:我们开发了一种快速灵敏的聚合酶链反应(PCR)分析法,用于检测和鉴定风疹病毒(RV)。选择编码RV的E1膜糖蛋白的RV基因的片段作为PCR扩增的靶。从感染细胞中提取或从病毒体中释放出的单链病毒RNA被用作反转录的模板,然后用两组不同的引物对进行PCR扩增,其中一组嵌套在另一对中。在溴化乙锭染色的琼脂糖微凝胶中检测到扩增的E1基因序列,并通过限制性内切酶消化和与PCR靶位点上的探针杂交来验证其身份。通过使用荧光双脱氧终止子和自动化程序直接对由靶标的不对称扩增产生的单链DNA进行测序,以确认靶标序列。该PCR测定法为通过细胞培养检测RV提供了快速的验证性测试,并且在临床样品中直接检测RV似乎具有相当大的潜力。该PCR检测方法的开发中使用的策略对于开发病毒的其他诊断PCR检测方法应该是有用的。

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