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采用针对病毒核蛋白基因的引物组,通过逆转录聚合酶链反应检测所有已知丝状病毒物种。

Detection of all known filovirus species by reverse transcription-polymerase chain reaction using a primer set specific for the viral nucleoprotein gene.

机构信息

Hokudai Center for Zoonosis Control in Zambia, School of Veterinary Medicine, The University of Zambia, Lusaka, Zambia.

出版信息

J Virol Methods. 2011 Jan;171(1):310-3. doi: 10.1016/j.jviromet.2010.11.010. Epub 2010 Nov 17.

Abstract

The filoviruses, Marburg virus (MARV) and Ebola virus (EBOV), are causative agents of severe hemorrhagic fever with high mortality rates in humans and non-human primates. Sporadic outbreaks of filovirus infection have occurred in Central Africa and parts of Asia. Identification of the natural reservoir animals that are unknown yet and epidemiological investigations are current challenges to forestall outbreaks of filovirus diseases. The filovirus species identified currently include one in the MARV group and five in the EBOV group, with large genetic variations found among the species. Therefore, it has been difficult to develop a single sensitive assay to detect all filovirus species, which would advance laboratory diagnosis greatly in endemic areas. In this study, a highly sensitive universal RT-PCR assay targeting the nucleoprotein (NP) gene of filoviruses was developed. The genomic RNAs of all known MARV and EBOV species were detected by using an NP-specific primer set. In addition, this RT-PCR procedure was verified further for its application to detect viral RNAs in tissue samples of animals infected experimentally and blood specimens of infected patients. This assay will be a useful method for diagnostics and epidemiological studies of filovirus infections.

摘要

丝状病毒,马尔堡病毒(MARV)和埃博拉病毒(EBOV),是引起人类和非人灵长类动物严重出血热的病原体,死亡率很高。丝状病毒感染的散发性暴发发生在中非和亚洲部分地区。确定目前未知的自然储主动物以及进行流行病学调查是预防丝状病毒病暴发的当前挑战。目前鉴定的丝状病毒种类包括 MARV 组中的一种和 EBOV 组中的五种,在这些种类中发现了很大的遗传变异。因此,很难开发出一种单一的敏感检测方法来检测所有丝状病毒种类,这将极大地促进在流行地区的实验室诊断。在这项研究中,开发了一种针对丝状病毒核蛋白(NP)基因的高度敏感的通用 RT-PCR 检测方法。使用 NP 特异性引物组检测所有已知的 MARV 和 EBOV 物种的基因组 RNA。此外,进一步验证了该 RT-PCR 程序在检测实验感染动物的组织样本和感染患者的血液样本中的病毒 RNA 方面的应用。该检测方法将是诊断和丝状病毒感染的流行病学研究的有用方法。

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