首页> 外文期刊>Journal of Virological Methods >Development of a TaqMan RT-PCR assay without RNA extraction step for the detection and quantification of African Chikungunya viruses.
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Development of a TaqMan RT-PCR assay without RNA extraction step for the detection and quantification of African Chikungunya viruses.

机译:没有RNA提取步骤的TaqMan RT-PCR检测方法的开发,用于检测和定量非洲基孔肯雅病毒。

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摘要

Chikungunya virus (CHIKV), a member of the alphavirus genus, is of considerable public health concern in Southeast Asian and African countries. However, despite serological evidence, the diagnosis of this arthropod-borne human disease is confirmed infrequently and needs to be improved. In fact, illness caused by CHIKV can be confused with diseases such as dengue or yellow fever, based on the similarity of the symptoms, and laboratory confirmation of suspected cases is required to launch control measures during an epidemic. Moreover, no quantitative molecular tool is described to study CHIKV replication or detection in clinical samples and cell culture supernatants. In this study, a specific and sensitive CHIKV one-step TaqMan RT-PCR assay was developed as a tool for the diagnosis of African CHIKV as well as a rapid indicator of active infection by quantifying viral load. This study also showed that a simple heat viral RNA release during the reverse transcription step constituted an alternative to the conventional RNA extraction method.
机译:基孔肯雅病毒(CHIKV)是alphavirus属的成员,在东南亚和非洲国家引起了广泛的公共卫生关注。然而,尽管有血清学证据,这种节肢动物传播的人类疾病的诊断很少得到确认,需要改进。实际上,基于症状的相似性,CHIKV引起的疾病可以与登革热或黄热病等疾病相混淆,并且在流行期间需要实验室确认可疑病例才能采取控制措施。而且,没有描述用于在临床样品和细胞培养上清液中研究CHIKV复制或检测的定量分子工具。在这项研究中,开发了一种特异性且灵敏的CHIKV一步式TaqMan RT-PCR测定法,作为诊断非洲CHIKV的工具,以及通过量化病毒载量来快速诊断活跃感染的指标。这项研究还表明,在逆转录步骤中简单的热病毒RNA释放是常规RNA提取方法的替代方法。

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