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Structural and mechanistic analysis of the membrane-embedded glycosyltransferase WaaA required for lipopolysaccharide synthesis

机译:脂多糖合成所需的膜嵌入糖基转移酶WaaA的结构和机理分析

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摘要

WaaA is a key enzyme in the biosynthesis of LPS, a critical component of the outer envelope of Gram-negative bacteria. Embedded in the cytoplasmic face of the inner membrane, WaaA catalyzes the transfer of 3-deoxy-d-manno-oct-2-ulosonic acid (Kdo) to the lipid A precursor of LPS. Here we present crystal structures of the free and CMP-bound forms of WaaA from Aquifex aeolicus, an ancient Gram-negative hyperthermophile. These structures reveal details of the CMP-binding site and implicate a unique sequence motif (GGS/TX5GXNXLE) in Kdo binding. In addition, a cluster of highly conserved amino acid residues was identified which represents the potential membrane-attachment and acceptor-substrate binding site of WaaA. A series of site-directed mutagenesis experiments revealed critical roles for glycine 30 and glutamate 31 in Kdo transfer. Our results provide the structural basis of a critical reaction in LPS biosynthesis and allowed the development of a detailed model of the catalytic mechanism of WaaA.
机译:WaaA是LPS生物合成的关键酶,LPS是革兰氏阴性细菌外壳的重要组成部分。 WaaA嵌入内膜的细胞质表面,催化将3-脱氧-d-甘露聚糖-辛基-2-核糖酸(Kdo)转移至LPS的脂质A前体。在这里,我们介绍了来自Aquifex aeolicus(一种古老的革兰氏阴性超嗜热菌)的WaaA的游离和CMP结合形式的晶体结构。这些结构揭示了CMP结合位点的细节,并暗示了Kdo结合中的独特序列基序(GGS / TX5GXNXLE)。另外,鉴定出一组高度保守的氨基酸残基,其代表WaaA的潜在膜附着和受体-底物结合位点。一系列定点诱变实验揭示了甘氨酸30和谷氨酸31在Kdo转移中的关键作用。我们的结果提供了LPS生物合成中关键反应的结构基础,并允许开发WaaA催化机理的详细模型。

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