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确定西尼罗河病毒感染细胞培养物和小鼠后分泌的非结构蛋白NS1的水平。

Defining the levels of secreted non-structural protein NS1 after West Nile virus infection in cell culture and mice.

作者信息

Chung Kyung Min, Diamond Michael S

机构信息

Department of Medicine, Washington University School of Medicine, St Louis, Missouri 63110, USA.

出版信息

J Med Virol. 2008 Mar;80(3):547-56. doi: 10.1002/jmv.21091.

Abstract

Infection with West Nile virus (WNV) causes a febrile illness that can progress to meningitis or encephalitis, primarily in humans that are immunocompromised or elderly. For successful treatment of WNV infection, accurate and timely diagnosis is essential. Previous studies have suggested that the flavivirus non-structural protein NS1, a highly conserved and secreted glycoprotein, is a candidate protein for rapid diagnosis. Herein, we developed a capture enzyme-linked immunosorbent assay (ELISA) to detect WNV NS1 using two anti-NS1 monoclonal antibodies (mAbs) that map to distinct sites on the protein. The capture ELISA efficiently detected as little as 0.5 ng/ml of soluble NS1 and exhibited no cross-reactivity for yellow fever, Dengue, and St. Louis encephalitis virus NS1. The capture ELISA reliably detected NS1 in plasma at day 3 after WNV infection, prior to the development of clinical signs of disease. As the time course of infection continued, the levels of detectable NS1 diminished, presumably because of interference by newly generated anti-NS1 antibodies. Indeed, treatment of plasma with a solution that dissociated NS1 immune complexes extended the window of detection. Overall, the NS1-based capture ELISA is a sensitive readout of infection and could be an important tool for diagnosis or screening small molecule inhibitors of WNV infection.

摘要

西尼罗河病毒(WNV)感染会引发一种发热性疾病,主要在免疫功能低下或年长的人群中可能会进展为脑膜炎或脑炎。对于成功治疗WNV感染而言,准确及时的诊断至关重要。先前的研究表明,黄病毒非结构蛋白NS1是一种高度保守的分泌性糖蛋白,是快速诊断的候选蛋白。在此,我们开发了一种捕获酶联免疫吸附测定法(ELISA),使用两种抗NS1单克隆抗体(mAb)来检测WNV NS1,这两种抗体靶向该蛋白上不同的位点。捕获ELISA能够有效检测低至0.5 ng/ml的可溶性NS1,并且对黄热病、登革热和圣路易斯脑炎病毒的NS1没有交叉反应。捕获ELISA能够在WNV感染后第3天,在疾病临床症状出现之前可靠地检测出血浆中的NS1。随着感染时间的推移,可检测到的NS1水平下降,推测是由于新产生的抗NS1抗体的干扰。实际上,用解离NS1免疫复合物的溶液处理血浆可延长检测窗口期。总体而言,基于NS1的捕获ELISA是感染的灵敏检测方法,可能成为诊断或筛选WNV感染小分子抑制剂的重要工具。

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