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ROP13 的加工和分泌:一种独特的弓形虫效应蛋白。

Processing and secretion of ROP13: A unique Toxoplasma effector protein.

机构信息

Department of Microbiology, Immunology and Molecular Genetics, University of California, Los Angeles, Los Angeles, CA 90095-1489, USA.

出版信息

Int J Parasitol. 2010 Aug 1;40(9):1037-44. doi: 10.1016/j.ijpara.2010.02.014. Epub 2010 Mar 30.

Abstract

Like most intracellular pathogens, Toxoplasma synthesizes and secretes an arsenal of proteins to successfully invade its host cell and hijack host functions for intracellular survival. The rhoptries are key secretory organelles that inject proteins into the host cell where they are positioned to co-opt host processes, although little is known regarding how these proteins exert their functions. We show here that the rhoptry protein ROP13 is synthesized as a pre-pro-protein that is processed in the parasite. Processing occurs at a conserved SphiXE cleavage site as mutagenesis of glutamic acid to alanine at the P1 position disrupts ROP13 maturation. We also demonstrate that processing of the prodomain is not necessary for rhoptry targeting and secretion. While gene disruption reveals that ROP13 is not essential for growth in fibroblasts in vitro or for virulence in vivo, we find that ROP13 is a soluble effector protein that can access the cytoplasm of host cells. Exogenously expressed ROP13 in human cells remains cytosolic but also appears toxic, suggesting that over-expression of this effector protein is disrupting some function within the host cell.

摘要

像大多数细胞内病原体一样,弓形虫合成并分泌了一整套蛋白质,成功入侵宿主细胞并劫持宿主功能以实现细胞内生存。 微线体是关键的分泌细胞器,可将蛋白质注入宿主细胞,使其能够利用宿主过程,尽管对于这些蛋白质如何发挥作用知之甚少。 我们在这里表明,微线体蛋白 ROP13 作为前原蛋白合成,在寄生虫中进行加工。 加工发生在保守的 SphiXE 切割位点,因为在 P1 位置将谷氨酸突变为丙氨酸会破坏 ROP13 的成熟。 我们还证明,前导肽的加工对于微线体的靶向和分泌不是必需的。 虽然基因敲除表明 ROP13 对于体外成纤维细胞中的生长或体内毒力不是必需的,但我们发现 ROP13 是一种可溶性效应蛋白,可以进入宿主细胞的细胞质。 在人类细胞中外源表达的 ROP13 仍留在细胞质中,但也表现出毒性,这表明这种效应蛋白的过表达正在破坏宿主细胞中的某些功能。

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