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基于逆转录定量聚合酶链反应的检测方法的开发,用于广泛检测非洲和亚洲寨卡病毒谱系。

Development of a reverse transcription quantitative polymerase chain reaction-based assay for broad coverage detection of African and Asian Zika virus lineages.

作者信息

Yang Yang, Wong Gary, Ye Baoguo, Li Shihua, Li Shanqin, Zheng Haixia, Wang Qiang, Liang Mifang, Gao George F, Liu Lei, Liu Yingxia, Bi Yuhai

机构信息

Shenzhen Key Laboratory of Pathogen and Immunity, State Key Discipline of Infectious Disease, Shenzhen Third People's Hospital, Shenzhen, 518112, China.

CAS Key Laboratory of Pathogenic Microbiology and Immunology, Collaborative Innovation Center for Diagnosis and Treatment of Infectious Disease, Institute of Microbiology, Center for Influenza Research and Early-warning (CASCIRE), Chinese Academy of Sciences, Beijing, 100101, China.

出版信息

Virol Sin. 2017 Jun;32(3):199-206. doi: 10.1007/s12250-017-3958-y. Epub 2017 May 19.

Abstract

The Zika virus (ZIKV) is an arbovirus that has spread rapidly worldwide within recent times. There is accumulating evidence that associates ZIKV infections with Guillain-Barré Syndrome (GBS) and microcephaly in humans. The ZIKV is genetically diverse and can be separated into Asian and African lineages. A rapid, sensitive, and specific assay is needed for the detection of ZIKV across various pandemic regions. So far, the available primers and probes do not cover the genetic diversity and geographic distribution of all ZIKV strains. To this end, we have developed a one-step quantitative reverse transcription polymerase chain reaction (qRT-PCR) assay based on conserved sequences in the ZIKV envelope (E) gene. The detection limit of the assay was determined to be five RNA transcript copies and 2.94 × 10 50% tissue culture infectious doses (TCID) of live ZIKV per reaction. The assay was highly specific and able to detect five different ZIKV strains covering the Asian and African lineages without nonspecific amplification, when tested against other flaviviruses. The assay was also successful in testing for ZIKV in clinical samples. Our assay represents an improvement over the current methods available for the detection ZIKV and would be valuable as a diagnostic tool in various pandemic regions.

摘要

寨卡病毒(ZIKV)是一种虫媒病毒,近期已在全球迅速传播。越来越多的证据表明,寨卡病毒感染与人类的吉兰-巴雷综合征(GBS)和小头畸形有关。寨卡病毒在基因上具有多样性,可分为亚洲和非洲谱系。需要一种快速、灵敏且特异的检测方法来检测不同疫情地区的寨卡病毒。到目前为止,现有的引物和探针并未涵盖所有寨卡病毒株的基因多样性和地理分布。为此,我们基于寨卡病毒包膜(E)基因中的保守序列,开发了一种一步法定量逆转录聚合酶链反应(qRT-PCR)检测方法。该检测方法的检测限确定为每个反应5个RNA转录本拷贝和2.94×10 50%组织培养感染剂量(TCID)的活寨卡病毒。当与其他黄病毒进行检测时,该检测方法具有高度特异性,能够检测涵盖亚洲和非洲谱系的五种不同寨卡病毒株,且无非特异性扩增。该检测方法在临床样本的寨卡病毒检测中也取得了成功。我们的检测方法是对目前可用的寨卡病毒检测方法的改进,作为一种诊断工具,在不同疫情地区将具有重要价值。

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