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一种用于定量疟原虫子孢子侵袭HepG2细胞的免疫放射分析方法。

An immunoradiometric assay for the quantification of Plasmodium sporozoite invasion of HepG2 cells.

作者信息

Sinnis P

机构信息

Department of Medical and Molecular Parasitology, New York University Medical Center, NY 10016, USA.

出版信息

J Immunol Methods. 1998 Dec 1;221(1-2):17-23. doi: 10.1016/s0022-1759(98)00151-3.

Abstract

Malaria infection in a vertebrate host is initiated when Plasmodium sporozoites invade hepatocytes after injection by an infected mosquito. In vitro, the parasites invade and develop in HepG2 cells and these cells have been used to study target cell invasion by sporozoites. Previously described in vitro invasion assays involve staining and counting of intracellular sporozoites or exoerythrocytic forms of the parasite. Here we describe an immunoradiometric assay that can quantify sporozoite invasion of HepG2 cells in vitro. The assay relies on the differential detection of intracellular and extracellular circumsporozoite protein (CS; the major surface protein of the sporozoite) which can then be used to calculate the efficiency of invasion. Since this assay can be performed more rapidly than the current assays in which parasites must be counted under a microscope, it enables investigators to more rapidly screen inhibitors of sporozoite invasion.

摘要

当被感染的蚊子注射疟原虫子孢子后,疟原虫在脊椎动物宿主体内引发感染,子孢子侵入肝细胞。在体外,这些寄生虫在HepG2细胞中侵入并发育,这些细胞已被用于研究子孢子对靶细胞的侵入。先前描述的体外侵入试验涉及对细胞内子孢子或寄生虫的红细胞外期形式进行染色和计数。在此,我们描述了一种免疫放射分析方法,该方法可在体外定量子孢子对HepG2细胞的侵入。该分析方法依赖于对细胞内和细胞外环子孢子蛋白(CS;子孢子的主要表面蛋白)的差异检测,然后可用于计算侵入效率。由于该分析方法比目前必须在显微镜下对寄生虫进行计数的试验执行速度更快,因此它使研究人员能够更快速地筛选子孢子侵入的抑制剂。

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