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来自大肠杆菌的[NiFe]氢化酶成熟蛋白HypE的结构及其与HypF的相互作用。

Structure of [NiFe] hydrogenase maturation protein HypE from Escherichia coli and its interaction with HypF.

作者信息

Rangarajan Erumbi S, Asinas Abdalin, Proteau Ariane, Munger Christine, Baardsnes Jason, Iannuzzi Pietro, Matte Allan, Cygler Miroslaw

机构信息

Department of Biochemistry, McGill University, Montréal, Québec, Canada.

出版信息

J Bacteriol. 2008 Feb;190(4):1447-58. doi: 10.1128/JB.01610-07. Epub 2007 Dec 7.

Abstract

Hydrogenases are enzymes involved in hydrogen metabolism, utilizing H2 as an electron source. [NiFe] hydrogenases are heterodimeric Fe-S proteins, with a large subunit containing the reaction center involving Fe and Ni metal ions and a small subunit containing one or more Fe-S clusters. Maturation of the [NiFe] hydrogenase involves assembly of nonproteinaceous ligands on the large subunit by accessory proteins encoded by the hyp operon. HypE is an essential accessory protein and participates in the synthesis of two cyano groups found in the large subunit. We report the crystal structure of Escherichia coli HypE at 2.0-A resolution. HypE exhibits a fold similar to that of PurM and ThiL and forms dimers. The C-terminal catalytically essential Cys336 is internalized at the dimer interface between the N- and C-terminal domains. A mechanism for dehydration of the thiocarbamate to the thiocyanate is proposed, involving Asp83 and Glu272. The interactions of HypE and HypF were characterized in detail by surface plasmon resonance and isothermal titration calorimetry, revealing a Kd (dissociation constant) of approximately 400 nM. The stoichiometry and molecular weights of the complex were verified by size exclusion chromatography and gel scanning densitometry. These experiments reveal that HypE and HypF associate to form a stoichiometric, hetero-oligomeric complex predominantly consisting of a [EF]2 heterotetramer which exists in a dynamic equilibrium with the EF heterodimer. The surface plasmon resonance results indicate that a conformational change occurs upon heterodimerization which facilitates formation of a productive complex as part of the carbamate transfer reaction.

摘要

氢化酶是参与氢代谢的酶,利用H2作为电子源。[NiFe]氢化酶是异二聚体铁硫蛋白,大亚基包含涉及铁和镍金属离子的反应中心,小亚基包含一个或多个铁硫簇。[NiFe]氢化酶的成熟涉及由hyp操纵子编码的辅助蛋白在大亚基上组装非蛋白质配体。HypE是一种必需的辅助蛋白,参与大亚基中发现的两个氰基的合成。我们报告了大肠杆菌HypE在2.0埃分辨率下的晶体结构。HypE呈现出与PurM和ThiL相似的折叠并形成二聚体。C末端催化必需的Cys336在N末端和C末端结构域之间的二聚体界面处内化。提出了硫代氨基甲酸盐脱水形成硫氰酸盐的机制,涉及Asp83和Glu272。通过表面等离子体共振和等温滴定量热法详细表征了HypE和HypF的相互作用,揭示解离常数(Kd)约为400 nM。通过尺寸排阻色谱法和凝胶扫描密度测定法验证了复合物的化学计量和分子量。这些实验表明,HypE和HypF缔合形成化学计量的异源寡聚复合物,主要由[EF]2异源四聚体组成,其与EF异二聚体处于动态平衡。表面等离子体共振结果表明,异二聚化时发生构象变化,这有助于形成作为氨基甲酸盐转移反应一部分的有活性的复合物。

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