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使用碘酰苯和磺基琥珀酰亚胺生物素鉴定和分离马来丝虫的表皮蛋白。

Use of Iodogen and sulfosuccinimidobiotin to identify and isolate cuticular proteins of the filarial parasite Brugia malayi.

作者信息

Alvarez R M, Henry R W, Weil G J

机构信息

Division of Infectious Diseases, Jewish Hospital, Washington University Medical Center, St. Louis, MO 63110.

出版信息

Mol Biochem Parasitol. 1989 Mar 1;33(2):183-9. doi: 10.1016/0166-6851(89)90032-7.

Abstract

The cuticle of filarial nematodes is a dynamic structure which may be an important target for protective host immune responses. Prior studies have employed radioiodination of intact parasites to demonstrate that the collagenous cuticle of filariids contains relatively few exposed proteins, some of which are stage and/or species-specific. In the present study, we have used sulfo-NHS-biotin to label and affinity purify cuticular components of living adult Brugia malayi. Results obtained by this method were compared with the widely used Iodogen method of surface radioiodination by SDS-PAGE analysis of detergent-solubilized worms and by ultrastructural analysis. Both labeling methods produced very similar electrophoretic patterns with major doublets at 70 and 100 kDa, a major band at 25 kDa, and minor bands between 60-200 kDa. Ultrastructural analysis showed that both methods labeled components throughout all levels of the parasite cuticle; underlying somatic tissues were not labeled. The biotinylated components were isolated from the total parasite extract by affinity chromatography on an avidin matrix. Further characterization of these surface-associated proteins may lead to improved methods for the control of filariasis.

摘要

丝虫线虫的角质层是一种动态结构,可能是宿主保护性免疫反应的重要靶点。先前的研究利用完整寄生虫的放射性碘化来证明丝虫的胶原质角质层所含的暴露蛋白相对较少,其中一些蛋白具有阶段和/或物种特异性。在本研究中,我们使用磺基-NHS-生物素标记并亲和纯化成年马来布鲁线虫的角质层成分。通过对去污剂溶解的虫体进行SDS-PAGE分析以及超微结构分析,将该方法获得的结果与广泛使用的表面放射性碘化碘原方法进行了比较。两种标记方法产生的电泳图谱非常相似,主要双峰位于70和100 kDa,一条主要条带位于25 kDa,以及60 - 200 kDa之间的次要条带。超微结构分析表明,两种方法都标记了寄生虫角质层各个层面的成分;其下方的体细胞组织未被标记。通过在抗生物素蛋白基质上进行亲和色谱,从总寄生虫提取物中分离出生物素化成分。对这些表面相关蛋白的进一步表征可能会带来控制丝虫病的改进方法。

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