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ELISA method for detecting Plasmodium falciparum circumsporozoite antibody.

机译:ELISA法检测恶性疟原虫环子孢子抗体。

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摘要

An enzyme-linked immunosorbent assay (ELISA) for circulating IgG mouse antibody to Plasmodium falciparum circumsporozoite (CS) protein was modified for use with human sera collected in an area of northern Zambia that was endemic for malaria and from individuals never exposed to malaria. Optimum sensitivity was achieved using Immulon 2 microtitration plates, boiled casein-Tween 20 blocking buffer, and by adding a solution of boiled casein (4 micrograms/ml) to the capture antigen diluent. The results for the detection of anti-CS IgG correlated well with those of sporozoite immunofluorescence antibody assays. Modification of the ELISA method permitted the simultaneous detection of anti-CS IgG and IgM antibody on a single serum sample in the same well of the microtitration plate and the detection of anti-CS IgG antibody in Kenyan dried whole-blood samples collected on filter-paper. The assay has been used to monitor human antibody levels in a phase-I malaria vaccine trial and in longitudinal studies of malaria transmission in Thailand and Kenya.
机译:酶联免疫吸附测定法(ELISA)用于循环针对恶性疟原虫环子孢子(CS)蛋白的IgG小鼠抗体,经过改良,可与在赞比亚北部流行的疟疾地区和从未接触过疟疾的个体收集的人类血清一起使用。使用Immulon 2微量滴定板,煮沸的酪蛋白-Tween 20封闭缓冲液,以及将煮沸的酪蛋白溶液(4微克/毫升)添加到捕获抗原稀释液中,可获得最佳灵敏度。抗CS IgG的检测结果与子孢子免疫荧光抗体检测的相关性很好。 ELISA方法的修改允许在微量滴定板同一孔中的单个血清样品中同时检测抗CS IgG和IgM抗体,并在通过过滤器收集的肯尼亚干燥全血样品中检测抗CS IgG抗体。纸。该测定法已被用于监测I期疟疾疫苗试验中的人抗体水平以及泰国和肯尼亚的疟疾传播纵向研究。

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