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一种用于鉴定靶向非结构蛋白nsP2的基孔肯雅病毒抑制剂的表型分析。

A phenotypic assay to identify Chikungunya virus inhibitors targeting the nonstructural protein nsP2.

作者信息

Lucas-Hourani Marianne, Lupan Alexandru, Desprès Philippe, Thoret Sylviane, Pamlard Olivier, Dubois Joëlle, Guillou Catherine, Tangy Frédéric, Vidalain Pierre-Olivier, Munier-Lehmann Hélène

机构信息

Institut Pasteur, Unité de Génomique Virale et Vaccination, Paris, France.

出版信息

J Biomol Screen. 2013 Feb;18(2):172-9. doi: 10.1177/1087057112460091. Epub 2012 Sep 14.

DOI:10.1177/1087057112460091
PMID:22983165
Abstract

Chikungunya virus (CHIKV) is a mosquito-transmitted pathogen responsible for an acute infection of abrupt onset, characterized by high fever, polyarthralgia, myalgia, headaches, chills, and rash. In 2006, CHIKV was responsible for an epidemic outbreak of unprecedented magnitude in the Indian Ocean, stressing the need for therapeutic approaches. Since then, we have acquired a better understanding of CHIKV biology, but we are still missing active molecules against this reemerging pathogen. We recently reported that the nonstructural nsP2 protein of CHIKV induces a transcriptional shutoff that allows the virus to block cellular antiviral response. This was demonstrated using various luciferase-based reporter gene assays, including a trans-reporter system where Gal4 DNA binding domain is fused to Fos transcription factor. Here, we turned this assay into a high-throughput screening system to identify small molecules targeting nsP2-mediated shutoff. Among 3040 molecules tested, we identified one natural compound that partially blocks nsP2 activity and inhibits CHIKV replication in vitro. This proof of concept suggests that similar functional assays could be developed to target other viral proteins mediating a cellular shutoff and identify innovative therapeutic molecules.

摘要

基孔肯雅病毒(CHIKV)是一种由蚊子传播的病原体,可引发急性感染,起病急骤,症状包括高热、多关节痛、肌痛、头痛、寒战和皮疹。2006年,CHIKV在印度洋引发了一场规模空前的疫情,凸显了治疗方法的必要性。从那时起,我们对CHIKV生物学有了更深入的了解,但针对这种重新出现的病原体,我们仍缺乏有效的活性分子。我们最近报道,CHIKV的非结构nsP2蛋白会引发转录关闭,使病毒能够阻断细胞的抗病毒反应。这一结论通过各种基于荧光素酶的报告基因检测得以证实,其中包括一个将Gal4 DNA结合域与Fos转录因子融合的反式报告系统。在此,我们将该检测方法转化为高通量筛选系统,以鉴定靶向nsP2介导的转录关闭的小分子。在测试的3040种分子中,我们鉴定出一种天然化合物,它能部分阻断nsP2活性并在体外抑制CHIKV复制。这一概念验证表明,可以开发类似的功能检测方法来靶向其他介导细胞转录关闭的病毒蛋白,并鉴定出创新的治疗分子。

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