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鉴定VceA和VceC,它们是VjbR调控子的两个成员,可通过布鲁氏菌IV型分泌系统转运至巨噬细胞内。

Identification of VceA and VceC, two members of the VjbR regulon that are translocated into macrophages by the Brucella type IV secretion system.

作者信息

de Jong Maarten F, Sun Yao-Hui, den Hartigh Andreas B, van Dijl Jan Maarten, Tsolis Renée M

机构信息

Department of Medical Microbiology and Immunology, School of Medicine, University of California at Davis, One Shields Ave., Davis, CA 95616-8645, USA.

出版信息

Mol Microbiol. 2008 Dec;70(6):1378-96. doi: 10.1111/j.1365-2958.2008.06487.x. Epub 2008 Oct 24.

Abstract

Survival and replication inside host cells by Brucella spp. requires a type IV secretion system (T4SS), encoded by the virB locus. However, the identity of the molecules secreted by the T4SS has remained elusive. We hypothesized that proteins translocated by the T4SS would be co-regulated with the virB operon. The LuxR family regulator VjbR, known to regulate virB, bound a fragment of the virB promoter containing an 18 bp palindromic motif (virB promoter box), showing that VjbR regulated the virB operon directly. To identify virB co-regulated genes, we searched the Brucella suis 1330 and B. abortus 2308 genomes for genes with an upstream virB promoter box. One hundred and forty-four promoters in the two genomes contained the virB promoter box, including those of fliC encoding flagellin and cgs encoding cyclic beta-glucan synthetase. Thirteen of these proteins were tested for VirB-dependent translocation into macrophages using a beta-lactamase reporter assay. This analysis resulted in the identification of the proteins encoded by BAB1_1652 (VceA) and BR1038/BAB1_1058 (VceC) as novel protein substrates of the Brucella T4SS. VceC could also be translocated by the Legionella pneumophila Dot/Icm T4SS into host cells. Our results suggest that VjbR co-ordinates expression of the T4SS and at least two of its secreted substrates.

摘要

布鲁氏菌属在宿主细胞内的存活和复制需要由virB基因座编码的IV型分泌系统(T4SS)。然而,T4SS分泌的分子身份一直难以确定。我们推测,由T4SS转运的蛋白质将与virB操纵子共同调控。已知调节virB的LuxR家族调节因子VjbR结合了包含18 bp回文基序(virB启动子框)的virB启动子片段,表明VjbR直接调节virB操纵子。为了鉴定与virB共同调控的基因,我们在猪布鲁氏菌1330和流产布鲁氏菌2308基因组中搜索具有上游virB启动子框的基因。两个基因组中的144个启动子包含virB启动子框,包括编码鞭毛蛋白的fliC和编码环状β-葡聚糖合成酶的cgs的启动子。使用β-内酰胺酶报告分析测试了其中13种蛋白质是否依赖VirB转运到巨噬细胞中。该分析鉴定出由BAB1_1652(VceA)和BR1038/BAB1_1058(VceC)编码的蛋白质是布鲁氏菌T4SS的新型蛋白质底物。VceC也可以被嗜肺军团菌Dot/Icm T4SS转运到宿主细胞中。我们的结果表明,VjbR协调T4SS及其至少两种分泌底物的表达。

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