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一种针对登革病毒的高通量抗病毒药物筛选检测方法的开发、优化与验证。

The development, optimization and validation of an assay for high throughput antiviral drug screening against Dengue virus.

作者信息

Che Pulin, Wang Lihua, Li Qianjun

出版信息

Int J Clin Exp Med. 2009 Dec 8;2(4):363-73.

Abstract

Dengue virus (DENV) is listed as one of the NIAID Category A priority pathogens. Dengue disease is endemic in most tropical countries, with an estimated 2.5 billion people living in areas at risk of DENV infection. Due to the lack of vaccines and antiviral drugs, it is now a huge public health burden around the world. In order to screen large compound libraries for the identification of novel antivirals targeting DENV, it is essential to develop a high throughput screening (HTS) amenable assay. Here, we present the development, optimization and validation of a cytopathic effect-based assay against Dengue virus serotype-2 (DENV-2). The assay conditions, including cell culturing conditions, DMSO tolerance and the multiplicity of infection, were optimized in both 96- and 384-well plates. Assay robustness and reproducibility were determined under the optimized conditions in 96-well plate, including Z'-value of 0.71, signal-to-background ratio of 6.88, coefficient of variation of 6.3% in mock-infected cells and 12.3% in DENV-2 infected cells. This assay was further miniaturized into a 384-well plate format with similar assay robustness and reproducibility comparing with these in the 96-well plate format. This assay was then validated using the LOPAC(1280) compound library, demonstrating its repeatability with comparable assay robustness and reproducibility. This fully developed and validated HTS amenable assay could be used in future studies to screen large compound libraries for the identification of novel antivirals against dengue disease.

摘要

登革病毒(DENV)被列为美国国立过敏与传染病研究所(NIAID)A类优先病原体之一。登革热在大多数热带国家呈地方性流行,估计有25亿人生活在有感染DENV风险的地区。由于缺乏疫苗和抗病毒药物,它现在是全球巨大的公共卫生负担。为了筛选大型化合物库以鉴定针对DENV的新型抗病毒药物,开发一种适用于高通量筛选(HTS)的检测方法至关重要。在此,我们展示了一种基于细胞病变效应的针对登革病毒2型(DENV-2)的检测方法的开发、优化和验证。在96孔板和384孔板中对包括细胞培养条件、二甲基亚砜(DMSO)耐受性和感染复数在内的检测条件进行了优化。在96孔板的优化条件下确定了检测的稳健性和可重复性,包括Z'值为0.71、信号背景比为6.88、 mock感染细胞的变异系数为6.3%以及DENV-2感染细胞的变异系数为12.3%。该检测方法进一步小型化为384孔板形式,与96孔板形式相比具有相似的检测稳健性和可重复性。然后使用LOPAC(1280)化合物库对该检测方法进行了验证,证明了其具有可重复性以及相当的检测稳健性和可重复性。这种完全开发和验证的适用于HTS的检测方法可用于未来的研究,以筛选大型化合物库来鉴定针对登革热疾病的新型抗病毒药物。

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