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本文引用的文献

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Dual myxovirus screen identifies a small-molecule agonist of the host antiviral response.双流感病毒筛选鉴定出一种宿主抗病毒反应的小分子激动剂。
J Virol. 2013 Oct;87(20):11076-87. doi: 10.1128/JVI.01425-13. Epub 2013 Aug 7.
2
The pandemic potential of Nipah virus.尼帕病毒的大流行潜力。
Antiviral Res. 2013 Oct;100(1):38-43. doi: 10.1016/j.antiviral.2013.07.011. Epub 2013 Jul 30.
3
A treatment for and vaccine against the deadly Hendra and Nipah viruses.亨德拉和尼帕病毒的治疗方法和疫苗。
Antiviral Res. 2013 Oct;100(1):8-13. doi: 10.1016/j.antiviral.2013.06.012. Epub 2013 Jul 6.
4
Recombinant Hendra viruses expressing a reporter gene retain pathogenicity in ferrets.表达报告基因的重组亨德拉病毒在雪貂中保持致病性。
Virol J. 2013 Mar 25;10:95. doi: 10.1186/1743-422X-10-95.
5
Henipavirus pathogenesis in human respiratory epithelial cells.亨德拉尼帕病毒在人呼吸道上皮细胞中的发病机制。
J Virol. 2013 Mar;87(6):3284-94. doi: 10.1128/JVI.02576-12. Epub 2013 Jan 9.
6
Distinct and overlapping roles of Nipah virus P gene products in modulating the human endothelial cell antiviral response.在调节人类内皮细胞抗病毒反应方面,寨卡病毒 P 基因产物具有独特和重叠的作用。
PLoS One. 2012;7(10):e47790. doi: 10.1371/journal.pone.0047790. Epub 2012 Oct 19.
7
Type I interferon signaling protects mice from lethal henipavirus infection.I 型干扰素信号通路保护小鼠免受亨德拉病毒致死性感染。
J Infect Dis. 2013 Jan 1;207(1):142-51. doi: 10.1093/infdis/jis653. Epub 2012 Oct 22.
8
Piloting the use of indigenous methods to prevent Nipah virus infection by interrupting bats' access to date palm sap in Bangladesh.在孟加拉国,利用本土方法防止尼帕病毒感染,通过阻止蝙蝠接触椰枣树汁液来进行试点。
Health Promot Int. 2013 Sep;28(3):378-86. doi: 10.1093/heapro/das020. Epub 2012 Jun 4.
9
Molecular virology of the henipaviruses.亨德拉尼帕病毒的分子病毒学。
Curr Top Microbiol Immunol. 2012;359:41-58. doi: 10.1007/82_2012_211.
10
Rapid screening for entry inhibitors of highly pathogenic viruses under low-level biocontainment.在低水平生物防护下,对高致病性病毒进入抑制剂进行快速筛选。
PLoS One. 2012;7(3):e30538. doi: 10.1371/journal.pone.0030538. Epub 2012 Mar 2.

用于快速定量抗病毒筛选的表达荧光素酶和绿色荧光蛋白的尼帕病毒的评估。

Evaluation of luciferase and GFP-expressing Nipah viruses for rapid quantitative antiviral screening.

作者信息

Lo Michael K, Nichol Stuart T, Spiropoulou Christina F

机构信息

Viral Special Pathogens Branch, Centers for Disease Control and Prevention, Atlanta, GA, United States.

Viral Special Pathogens Branch, Centers for Disease Control and Prevention, Atlanta, GA, United States.

出版信息

Antiviral Res. 2014 Jun;106:53-60. doi: 10.1016/j.antiviral.2014.03.011. Epub 2014 Mar 27.

DOI:10.1016/j.antiviral.2014.03.011
PMID:24680955
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5100748/
Abstract

Nipah virus (NiV) outbreaks have occurred in Malaysia, India, and Bangladesh, and the virus continues to cause annual outbreaks of fatal human encephalitis in Bangladesh due to spillover from its bat host reservoir. Due to its high pathogenicity, its potential use for bio/agro-terrorism, and to the current lack of approved therapeutics, NiV is designated as an overlap select agent requiring biosafety level-4 containment. Although the development of therapeutic monoclonal antibodies and soluble protein subunit vaccines have shown great promise, the paucity of effective antiviral drugs against NiV merits further exploration of compound libraries using rapid quantitative antiviral assays. As a proof-of-concept study, we evaluated the use of fluorescent and luminescent reporter NiVs for antiviral screening. We constructed and rescued NiVs expressing either Renilla luciferase or green fluorescent protein, and characterized their reporter signal kinetics in different cell types as well as in the presence of several inhibitors. The 50% effective concentrations (EC50s) derived for inhibitors against both reporter viruses are within range of EC50s derived from virus yield-based dose-response assays against wild-type NiV (within 1Log10), thus demonstrating that both reporter NiVs can serve as robust antiviral screening tools. Utilizing these live NiV-based reporter assays requires modest instrumentation, and circumvents the time and labor-intensive steps associated with cytopathic effect or viral antigen-based assays. These reporter NiVs will not only facilitate antiviral screening, but also the study of host cell components that influence the virus life cycle.

摘要

尼帕病毒(NiV)疫情已在马来西亚、印度和孟加拉国爆发,由于该病毒从其蝙蝠宿主库外溢,在孟加拉国它继续每年引发致命的人类脑炎疫情。由于其高致病性、可能被用于生物/农业恐怖主义,以及目前缺乏经批准的治疗方法,尼帕病毒被指定为需要在生物安全4级实验室进行防护的重叠选择病原体。尽管治疗性单克隆抗体和可溶性蛋白亚单位疫苗的研发已显示出巨大前景,但针对尼帕病毒的有效抗病毒药物匮乏,这值得利用快速定量抗病毒试验对化合物文库进行进一步探索。作为一项概念验证研究,我们评估了使用荧光和发光报告基因尼帕病毒进行抗病毒筛选的情况。我们构建并拯救了表达海肾荧光素酶或绿色荧光蛋白的尼帕病毒,并在不同细胞类型以及存在几种抑制剂的情况下对其报告信号动力学进行了表征。针对这两种报告基因病毒的抑制剂的50%有效浓度(EC50)与基于病毒产量的剂量反应试验针对野生型尼帕病毒得出的EC50在同一范围内(相差1个对数单位以内),因此表明这两种报告基因尼帕病毒均可作为强大的抗病毒筛选工具。利用这些基于活尼帕病毒的报告试验所需仪器设备简单,并且规避了与细胞病变效应或基于病毒抗原的试验相关的耗时且费力的步骤。这些报告基因尼帕病毒不仅将促进抗病毒筛选,还将有助于研究影响病毒生命周期的宿主细胞成分。