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弓形虫蛋白MIC2和M2AP形成细胞内存活所必需的六聚体复合物。

The toxoplasma proteins MIC2 and M2AP form a hexameric complex necessary for intracellular survival.

作者信息

Jewett Travis J, Sibley L David

机构信息

Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, Missouri 63110, USA.

出版信息

J Biol Chem. 2004 Mar 5;279(10):9362-9. doi: 10.1074/jbc.M312590200. Epub 2003 Dec 10.

DOI:10.1074/jbc.M312590200
PMID:14670959
Abstract

Toxoplasma gondii parasites gain entry into host cells through a process that depends on apically stored adhesins that are strategically released during invasion. One of these adhesins, microneme protein 2 (MIC2), is a type one transmembrane protein that binds to an accessory protein known as MIC2-associated protein (M2AP). Together the MIC2 x M2AP complex participates in host cell attachment and invasion. The short cytoplasmic C-domain of MIC2 is implicated in protein trafficking and mediating an association with the parasite cytoskeleton. To define the role of the cytoplasmic domain of MIC2, proteins lacking the C-domain were expressed in transgenic T. gondii. Surprisingly, protein trafficking and secretion were not affected. We hypothesized that mutant mic2 lacking the C-domain might be escorted to the micronemes by association with endogenous wild-type MIC2 possessing functional transmembrane and cytoplasmic domains. To investigate this interaction, native blue gels and gel filtration were employed to identify a stable macromolecular MIC2 x M2AP complex of approximately 450 kDa. Our findings reveal that MIC2 and M2AP proteins form stable hexamers consisting of three alphabeta dimers. Resolution of this complex has implications for how MIC2 x M2AP associates with host cell receptors and the cytoskeleton to facilitate parasite motility and invasion.

摘要

刚地弓形虫寄生虫通过一个依赖于顶端储存的粘附素的过程进入宿主细胞,这些粘附素在入侵过程中被策略性地释放。其中一种粘附素,微线体蛋白2(MIC2),是一种I型跨膜蛋白,它与一种称为MIC2相关蛋白(M2AP)的辅助蛋白结合。MIC2与M2AP复合物共同参与宿主细胞的附着和入侵。MIC2的短细胞质C结构域与蛋白质运输有关,并介导与寄生虫细胞骨架的关联。为了确定MIC2细胞质结构域的作用,在转基因刚地弓形虫中表达了缺乏C结构域的蛋白质。令人惊讶的是,蛋白质运输和分泌并未受到影响。我们推测,缺乏C结构域的突变型mic2可能通过与具有功能性跨膜和细胞质结构域的内源性野生型MIC2结合而被护送至微线体。为了研究这种相互作用,采用天然蓝色凝胶和凝胶过滤来鉴定一个约450 kDa的稳定大分子MIC2与M2AP复合物。我们的研究结果表明,MIC2和M2AP蛋白形成由三个αβ二聚体组成的稳定六聚体。解析这个复合物对于MIC2与M2AP如何与宿主细胞受体和细胞骨架结合以促进寄生虫运动和入侵具有重要意义。

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