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Lgt 的失活使得对单核细胞增生李斯特菌的脂蛋白进行系统表征成为可能。

Inactivation of Lgt allows systematic characterization of lipoproteins from Listeria monocytogenes.

作者信息

Baumgärtner Maja, Kärst Uwe, Gerstel Birgit, Loessner Martin, Wehland Jürgen, Jänsch Lothar

机构信息

Department of Cell Biology, Helmholtz Centre for Infection Research (HZI), D-38124 Braunschweig, Germany.

出版信息

J Bacteriol. 2007 Jan;189(2):313-24. doi: 10.1128/JB.00976-06. Epub 2006 Oct 13.

Abstract

Lipoprotein anchoring in bacteria is mediated by the prolipoprotein diacylglyceryl transferase (Lgt), which catalyzes the transfer of a diacylglyceryl moiety to the prospective N-terminal cysteine of the mature lipoprotein. Deletion of the lgt gene in the gram-positive pathogen Listeria monocytogenes (i) impairs intracellular growth of the bacterium in different eukaryotic cell lines and (ii) leads to increased release of lipoproteins into the culture supernatant. Comparative extracellular proteome analyses of the EGDe wild-type strain and the Delta lgt mutant provided systematic insight into the relative expression of lipoproteins. Twenty-six of the 68 predicted lipoproteins were specifically released into the extracellular proteome of the Delta lgt strain, and this proved that deletion of lgt is an excellent approach for experimental verification of listerial lipoproteins. Consequently, we generated Delta lgt Delta prfA double mutants to detect lipoproteins belonging to the main virulence regulon that is controlled by PrfA. Overall, we identified three lipoproteins whose extracellular levels are regulated and one lipoprotein that is posttranslationally modified depending on PrfA. It is noteworthy that in contrast to previous studies of Escherichia coli, we unambiguously demonstrated that lipidation by Lgt is not a prerequisite for activity of the lipoprotein-specific signal peptidase II (Lsp) in Listeria.

摘要

脂蛋白在细菌中的锚定由前脂蛋白二酰甘油转移酶(Lgt)介导,该酶催化二酰甘油部分转移至成熟脂蛋白预期的N端半胱氨酸。革兰氏阳性病原体单核细胞增生李斯特菌中lgt基因的缺失,(i)损害了该细菌在不同真核细胞系中的细胞内生长,(ii)导致脂蛋白释放到培养上清液中的量增加。对EGDe野生型菌株和Delta lgt突变体进行的细胞外蛋白质组比较分析,为脂蛋白的相对表达提供了系统的见解。68种预测的脂蛋白中有26种特异性释放到Delta lgt菌株的细胞外蛋白质组中,这证明lgt基因的缺失是实验验证李斯特菌脂蛋白的一种极佳方法。因此,我们构建了Delta lgt Delta prfA双突变体,以检测属于由PrfA控制的主要毒力调节子的脂蛋白。总体而言,我们鉴定出三种细胞外水平受调控的脂蛋白,以及一种根据PrfA进行翻译后修饰的脂蛋白。值得注意的是,与先前对大肠杆菌的研究不同,我们明确证明了Lgt进行的脂化并非李斯特菌中脂蛋白特异性信号肽酶II(Lsp)活性的先决条件。

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