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脑膜炎奈瑟菌唾液酸合酶NeuB与Mn2+、磷酸烯醇丙酮酸和N-乙酰甘露糖胺醇复合物的结构和机制分析

Structural and mechanistic analysis of sialic acid synthase NeuB from Neisseria meningitidis in complex with Mn2+, phosphoenolpyruvate, and N-acetylmannosaminitol.

作者信息

Gunawan Jason, Simard Dave, Gilbert Michel, Lovering Andrew L, Wakarchuk Warren W, Tanner Martin E, Strynadka Natalie C J

机构信息

Department of Biochemistry and Molecular Biology, University of British Columbia, Vancouver, British Columbia V6T 1Z3.

出版信息

J Biol Chem. 2005 Feb 4;280(5):3555-63. doi: 10.1074/jbc.M411942200. Epub 2004 Oct 29.

DOI:10.1074/jbc.M411942200
PMID:15516336
Abstract

In Neisseria meningitidis and related bacterial pathogens, sialic acids play critical roles in mammalian cell immunity evasion and are synthesized by a conserved enzymatic pathway that includes sialic acid synthase (NeuB, SiaC, or SynC). NeuB catalyzes the condensation of phosphoenolpyruvate (PEP) and N-acetylmannosamine, directly forming N-acetylneuraminic acid (or sialic acid). In this paper we report the development of a coupled assay to monitor NeuB reaction kinetics and an 18O-labeling study that demonstrates the synthase operates via a C-O bond cleavage mechanism. We also report the first structure of a sialic acid synthase, that of NeuB, revealing a unique domain-swapped homodimer architecture consisting of a (beta/alpha)8 barrel (TIM barrel)-type fold at the N-terminal end and a domain with high sequence identity and structural similarity to the ice binding type III antifreeze proteins at the C-terminal end of the enzyme. We have determined the structures of NeuB in the malate-bound form and with bound PEP and the substrate analog N-acetylmannosaminitol to 1.9 and 2.2 A resolution, respectively. Typical of other TIM barrel proteins, the active site of NeuB is located in a cavity at the C-terminal end of the barrel; however, the positioning of the swapped antifreeze-like domain from the adjacent monomer provides key residues for hydrogen bonding with substrates in the active site of NeuB, a structural feature that leads to distinct modes of substrate binding from other PEP-utilizing enzymes that lack an analogous antifreeze-like domain. Our observation of a direct interaction between a highly ordered manganese and the N-acetylmannosaminitol in the NeuB active site also suggests an essential role for the ion as an electrophilic catalyst that activates the N-acetylmannosamine carbonyl to the addition of PEP.

摘要

在脑膜炎奈瑟菌及相关细菌病原体中,唾液酸在逃避哺乳动物细胞免疫方面发挥着关键作用,且由一条保守的酶促途径合成,该途径包括唾液酸合酶(NeuB、SiaC或SynC)。NeuB催化磷酸烯醇丙酮酸(PEP)与N - 乙酰甘露糖胺的缩合反应,直接形成N - 乙酰神经氨酸(即唾液酸)。在本文中,我们报告了一种用于监测NeuB反应动力学的偶联测定法的开发以及一项18O标记研究,该研究表明该合酶通过C - O键裂解机制起作用。我们还报告了唾液酸合酶NeuB的首个结构,其呈现出独特的结构域交换同型二聚体架构,在N端由一个(β/α)8桶状结构(TIM桶状结构)组成,在酶的C端有一个与冰结合III型抗冻蛋白具有高度序列同一性和结构相似性的结构域。我们分别测定了结合苹果酸以及结合PEP和底物类似物N - 乙酰甘露糖胺醇的NeuB结构,分辨率分别为1.9 Å和2.2 Å。与其他TIM桶状蛋白一样,NeuB的活性位点位于桶状结构C端的一个腔内;然而,来自相邻单体的交换抗冻样结构域的定位为与NeuB活性位点中的底物形成氢键提供了关键残基,这一结构特征导致其底物结合模式与其他缺乏类似抗冻样结构域的利用PEP的酶不同。我们观察到在NeuB活性位点中高度有序的锰与N - 乙酰甘露糖胺醇之间存在直接相互作用,这也表明该离子作为亲电催化剂激活N - 乙酰甘露糖胺羰基以促进PEP的加成起着至关重要的作用。

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