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肺炎军团菌糖基转移酶抑制延伸因子 1A 的分子机制。

Molecular mechanism of elongation factor 1A inhibition by a Legionella pneumophila glycosyltransferase.

机构信息

Division of Molecular Microbiology, College of Life Sciences, University of Dundee, Dundee DD1 5EH, Scotland, UK.

出版信息

Biochem J. 2010 Feb 24;426(3):281-92. doi: 10.1042/BJ20091351.

Abstract

Legionnaires' disease is caused by a lethal colonization of alveolar macrophages with the Gram-negative bacterium Legionella pneumophila. LpGT (L. pneumophila glucosyltransferase; also known as Lgt1) has recently been identified as a virulence factor, shutting down protein synthesis in the human cell by specific glucosylation of EF1A (elongation factor 1A), using an unknown mode of substrate recognition and a retaining mechanism for glycosyl transfer. We have determined the crystal structure of LpGT in complex with substrates, revealing a GT-A fold with two unusual protruding domains. Through structure-guided mutagenesis of LpGT, several residues essential for binding of the UDP-glucose-donor and EF1A-acceptor substrates were identified, which also affected L. pneumophila virulence as demonstrated by microinjection studies. Together, these results suggested that a positively charged EF1A loop binds to a negatively charged conserved groove on the LpGT structure, and that two asparagine residues are essential for catalysis. Furthermore, we showed that two further L. pneumophila glycosyltransferases possessed the conserved UDP-glucose-binding sites and EF1A-binding grooves, and are, like LpGT, translocated into the macrophage through the Icm/Dot (intracellular multiplication/defect in organelle trafficking) system.

摘要

军团病是由革兰氏阴性菌嗜肺军团菌对肺泡巨噬细胞的致命定植引起的。最近,LpGT(嗜肺军团菌葡萄糖基转移酶;也称为 Lgt1)已被确定为一种毒力因子,通过 EF1A(延伸因子 1A)的特异性葡萄糖基化,特异性地抑制人细胞中的蛋白质合成,其使用未知的底物识别模式和保留机制进行糖基转移。我们已经确定了与底物结合的 LpGT 的晶体结构,揭示了具有两个不寻常突出结构域的 GT-A 折叠。通过对 LpGT 的结构引导突变,确定了几个对于结合 UDP-葡萄糖供体和 EF1A-受体底物至关重要的残基,这些残基也通过微注射研究影响了嗜肺军团菌的毒力。总之,这些结果表明,带正电荷的 EF1A 环与 LpGT 结构上的带负电荷的保守凹槽结合,并且两个天冬酰胺残基对于催化至关重要。此外,我们表明,另外两种嗜肺军团菌糖基转移酶具有保守的 UDP-葡萄糖结合位点和 EF1A 结合凹槽,并且像 LpGT 一样,通过 Icm/Dot(细胞内繁殖/细胞器运输缺陷)系统易位进入巨噬细胞。

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