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弓形虫微小膜泡复合体在蓝氏贾第鞭毛虫中的组装与输出

Assembly and export of a Toxoplasma microneme complex in Giardia lamblia.

作者信息

Gaechter Verena, Hehl Adrian B

机构信息

Institute of Parasitology, University of Zürich, Winterthurerstrasse 266a, CH-8057 Zürich, Switzerland.

出版信息

Int J Parasitol. 2005 Nov;35(13):1359-68. doi: 10.1016/j.ijpara.2005.06.007. Epub 2005 Aug 10.

Abstract

The microneme proteins of Toxoplasma gondii belong to a large family of adhesins of apicomplexan parasites involved in motility and host cell invasion. During secretory transport, soluble micronemes associate with membrane-bound carriers/escorters and become exposed on the parasite surface as complexes with an array of adhesive domains. Previously, we have exploited the intestinal protozoan Giardia lamblia as an expression system to produce correctly folded and unglycosylated monomeric surface proteins of T. gondii. Here, we report assembly and export of a trimeric microneme (MIC1/4/6) adhesin complex from Toxoplasma. Co-expressed, recombinant microneme proteins were used to investigate structural requirements for microneme complex formation. In addition, export of a microneme subunit induced development of novel Golgi-like compartments demonstrating the existence of post endoplasmic reticulum structures involved in constitutive secretion in this 'Golgi-less' cell. Recreation of the trimeric microneme escorter-cargo system in Giardia is a versatile tool to analyse universal requirements for complex assembly, receptor-ligand interactions and Golgi neogenesis in the basal Giardia secretory system.

摘要

刚地弓形虫的微线体蛋白属于顶复门寄生虫粘附素的一个大家族,参与运动和宿主细胞入侵。在分泌运输过程中,可溶性微线体与膜结合载体/护送蛋白结合,并作为具有一系列粘附结构域的复合物暴露在寄生虫表面。此前,我们利用肠道原生动物蓝氏贾第鞭毛虫作为表达系统,来生产正确折叠且未糖基化的刚地弓形虫单体表面蛋白。在此,我们报告了来自弓形虫的三聚体微线体(MIC1/4/6)粘附素复合物的组装和输出。共表达的重组微线体蛋白被用于研究微线体复合物形成的结构要求。此外,微线体亚基的输出诱导了新型高尔基体样区室的形成,这表明在这个“无高尔基体”细胞中存在参与组成型分泌的内质网后结构。在贾第鞭毛虫中重建三聚体微线体护送蛋白-货物系统是一种通用工具,可用于分析基础贾第鞭毛虫分泌系统中复合物组装、受体-配体相互作用和高尔基体新生的普遍要求。

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