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类Pmp蛋白Pls1和Pls2分泌到沙眼衣原体包涵体的腔内。

Pmp-like proteins Pls1 and Pls2 are secreted into the lumen of the Chlamydia trachomatis inclusion.

作者信息

Jorgensen Ine, Valdivia Raphael H

机构信息

Department of Molecular Genetics and Microbiology, Center for Microbial Pathogenesis, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Infect Immun. 2008 Sep;76(9):3940-50. doi: 10.1128/IAI.00632-08. Epub 2008 Jun 30.

Abstract

The obligate intracellular pathogen Chlamydia trachomatis secretes effector proteins across the membrane of the pathogen-containing vacuole (inclusion) to modulate host cellular functions. In an immunological screen for secreted chlamydial proteins, we identified CT049 and CT050 as potential inclusion membrane-associated proteins. These acidic, nonglobular proteins are paralogously related to the passenger domain of the polymorphic membrane protein PmpC and, like other Pmp proteins, are highly polymorphic among C. trachomatis ocular and urogenital strains. We generated antibodies to these Pmp-like secreted (Pls) proteins and determined by immunofluorescence microscopy that Pls1 (CT049) and Pls2 (CT050) localized to globular structures within the inclusion lumen and at the inclusion membrane. Fractionation of membranes and cytoplasmic components from infected cells by differential and density gradient centrifugation further indicated that Pls1 and Pls2 associated with membranes distinct from the bulk of bacterial and inclusion membranes. The accumulation of Pls1 and, to a lesser extent, Pls2 in the inclusion lumen was insensitive to the type III secretion inhibitor C1, suggesting that this translocation system is not essential for Pls protein secretion. In contrast, Pls secretion and stability were sensitive to low levels of beta-lactam antibiotics, suggesting that a functional cell wall is required for Pls secretion from the bacterial cell. Finally, we tested the requirement for these proteins in Chlamydia infection by microinjecting anti-Pls1 and anti-Pls2 antibodies into infected cells. Coinjection of anti-Pls1 and -Pls2 antibodies partially inhibited expansion of the inclusion. Because Pls proteins lack classical sec-dependent secretion signals, we propose that Pls proteins are secreted into the inclusion lumen by a novel mechanism to regulate events important for chlamydial replication and inclusion expansion.

摘要

专性胞内病原体沙眼衣原体通过含病原体液泡(包涵体)膜分泌效应蛋白,以调节宿主细胞功能。在一项针对沙眼衣原体分泌蛋白的免疫学筛选中,我们鉴定出CT049和CT050为潜在的包涵体膜相关蛋白。这些酸性非球状蛋白与多态膜蛋白PmpC的乘客结构域旁系同源,并且与其他Pmp蛋白一样,在沙眼衣原体眼部和泌尿生殖系统菌株中高度多态。我们制备了针对这些类Pmp分泌(Pls)蛋白的抗体,并通过免疫荧光显微镜确定Pls1(CT049)和Pls2(CT050)定位于包涵体腔内和包涵体膜上的球状结构。通过差速离心和密度梯度离心对感染细胞的膜和细胞质成分进行分级分离,进一步表明Pls1和Pls2与不同于大部分细菌膜和包涵体膜的膜相关。Pls1在包涵体腔内的积累以及在较小程度上Pls2的积累对III型分泌抑制剂C1不敏感,这表明该转运系统对于Pls蛋白分泌并非必不可少。相反,Pls分泌和稳定性对低水平的β-内酰胺抗生素敏感,这表明功能性细胞壁对于细菌细胞分泌Pls是必需的。最后,我们通过向感染细胞中显微注射抗Pls1和抗Pls2抗体,测试了这些蛋白在沙眼衣原体感染中的需求。同时注射抗Pls1和抗Pls2抗体部分抑制了包涵体的扩张。由于Pls蛋白缺乏经典的依赖sec的分泌信号,我们提出Pls蛋白通过一种新机制分泌到包涵体腔内,以调节对沙眼衣原体复制和包涵体扩张重要的事件。

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