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使用一种针对核蛋白的新型单克隆抗体通过酶联免疫吸附测定法检测埃博拉病毒抗原。

Detection of Ebola viral antigen by enzyme-linked immunosorbent assay using a novel monoclonal antibody to nucleoprotein.

作者信息

Niikura M, Ikegami T, Saijo M, Kurane I, Miranda M E, Morikawa S

机构信息

Department of Virology 1, National Institute of Infectious Diseases, Tokyo, Japan.

出版信息

J Clin Microbiol. 2001 Sep;39(9):3267-71. doi: 10.1128/JCM.39.9.3267-3271.2001.

Abstract

With the increase in international traffic, the risk of introducing rare but severe infectious diseases like Ebola hemorrhagic fever is increasing all over the world. However, the system for the diagnosis of Ebola virus infection is available in a limited number of countries. In the present study, we developed an Ebola virus antigen-detection enzyme-linked immunosorbent assay (ELISA) system using a novel monoclonal antibody (MAb) to the nucleoprotein (NP). This antibody recognized an epitope defined by a 26-amino-acid stretch near the C terminus of NP. In a sandwich ELISA system with the MAb, as little as 30 ng of purified recombinant NP (rNP) was detected. Although this MAb was prepared by immunization with rNP of subtype Zaire, it also reacted to the corresponding region of NP derived from the Reston and Sudan subtypes. These results suggest that our ELISA system should work with three of four Ebola subtypes. Furthermore, our ELISA system detected the NP in subtype Reston-infected monkey specimens, while the background level in noninfected specimens was very low, suggesting the usefulness of the ELISA for laboratory diagnosis with clinical specimens.

摘要

随着国际交通流量的增加,像埃博拉出血热这样罕见但严重的传染病在全球范围内传播的风险正在上升。然而,能够诊断埃博拉病毒感染的系统仅在少数国家可用。在本研究中,我们利用一种针对核蛋白(NP)的新型单克隆抗体(MAb)开发了一种埃博拉病毒抗原检测酶联免疫吸附测定(ELISA)系统。该抗体识别由NP C末端附近26个氨基酸延伸所定义的一个表位。在使用该MAb的夹心ELISA系统中,可检测到低至30 ng的纯化重组NP(rNP)。尽管该MAb是通过用扎伊尔亚型的rNP免疫制备的,但它也与来自雷斯顿和苏丹亚型的NP相应区域发生反应。这些结果表明,我们的ELISA系统应该对四种埃博拉亚型中的三种有效。此外,我们的ELISA系统在感染雷斯顿亚型的猴标本中检测到了NP,而未感染标本中的背景水平非常低,这表明该ELISA对于临床标本的实验室诊断是有用的。

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