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基于细胞的 ELISA 的验证作为一种筛选工具,可识别抗甲病毒小分子抑制剂。

Validation of a cell-based ELISA as a screening tool identifying anti-alphavirus small-molecule inhibitors.

机构信息

US Army Medical Research Institute of Infectious Diseases, Frederick, MD 21702, United States.

出版信息

J Virol Methods. 2013 Oct;193(1):226-31. doi: 10.1016/j.jviromet.2013.06.007. Epub 2013 Jun 10.

Abstract

Venezuelan (VEEV), eastern, and western equine encephalitis viruses, members of the genus Alphavirus, are causative agents of debilitative and sometimes fatal encephalitis. Although human cases are rare, these viruses pose a threat to military personnel, and to public health, due to their potential use as bioweapons. Currently, there are no licensed therapeutics for treating alphavirus infections. To address this need, small-molecules with potential anti-alphavirus activity, provided by collaborators, are tested routinely in live alphavirus assays utilizing time-consuming virus yield-reduction assays. To expedite the screening/hit-confirmation process, a cell-based enzyme-linked immunosorbent assay (ELISA) was developed and validated for the measurement of VEEV infection. A signal-to-background ratio of >900, and a z-factor of >0.8 indicated the robustness of this assay. For validation, the cell-based ELISA was compared directly to results from virus yield reduction assays in a single dose screen of 21 compounds. Using stringent criteria for anti-VEEV activity there was 90% agreement between the two assays (compounds displaying either antiviral activity, or no effect, in both assays). A concurrent compound-induced cell toxicity assay effectively filtered out false-positive hits. The cell-based ELISA also reproduced successfully compound dose-response virus inhibition data observed using the virus yield reduction assay. With available antibodies, this assay can be adapted readily to other viruses of interest to the biodefense community. Additionally, it is cost-effective, rapid, and amenable to automation and scale-up. Therefore, this assay could expedite greatly screening efforts and the identification of effective anti-alphavirus inhibitors.

摘要

委内瑞拉(VEEV)、东部和西部马脑炎病毒,属于黄病毒属,是导致衰弱甚至致命脑炎的病原体。尽管人类感染病例罕见,但由于这些病毒可能被用作生物武器,因此对军事人员和公共卫生构成了威胁。目前,尚无治疗黄病毒感染的许可疗法。为了满足这一需求,合作伙伴提供了具有潜在抗黄病毒活性的小分子,这些小分子在利用耗时的病毒产量减少测定法进行的活黄病毒测定中进行了常规测试。为了加快筛选/确认过程,开发并验证了一种基于细胞的酶联免疫吸附测定(ELISA),用于测量 VEEV 感染。>900 的信号与背景比和>0.8 的 z 因子表明该测定法具有稳健性。在验证中,在对 21 种化合物进行单次剂量筛选中,将基于细胞的 ELISA 与病毒产量减少测定的结果直接进行了比较。使用严格的抗 VEEV 活性标准,两种测定方法之间有 90%的一致性(在两种测定中均显示抗病毒活性或无作用的化合物)。同时进行的化合物诱导细胞毒性测定有效地筛选出了假阳性命中。基于细胞的 ELISA 还成功地再现了使用病毒产量减少测定观察到的化合物剂量反应病毒抑制数据。通过使用可用的抗体,该测定法可以很容易地适应生物防御界感兴趣的其他病毒。此外,它具有成本效益,快速,并且易于自动化和扩展。因此,该测定法可以大大加快筛选工作,并鉴定有效的抗黄病毒抑制剂。

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