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GDP介导的细菌酰基辅酶A硫酯酶调控的结构见解

Structural insights into GDP-mediated regulation of a bacterial acyl-CoA thioesterase.

作者信息

Khandokar Yogesh B, Srivastava Parul, Cowieson Nathan, Sarker Subir, Aragao David, Das Shubagata, Smith Kate M, Raidal Shane R, Forwood Jade K

机构信息

From the School of Biomedical Sciences and.

the Life Sciences Division, Diamond Light Source, Didcot OX11 0DE, United Kingdom.

出版信息

J Biol Chem. 2017 Dec 15;292(50):20461-20471. doi: 10.1074/jbc.M117.800227. Epub 2017 Oct 2.

DOI:10.1074/jbc.M117.800227
PMID:28972175
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5733585/
Abstract

Thioesterases catalyze the cleavage of thioester bonds within many activated fatty acids and acyl-CoA substrates. They are expressed ubiquitously in both prokaryotes and eukaryotes and are subdivided into 25 thioesterase families according to their catalytic active site, protein oligomerization, and substrate specificity. Although many of these enzyme families are well-characterized in terms of function and substrate specificity, regulation across most thioesterase families is poorly understood. Here, we characterized a TE6 thioesterase from the bacterium Structural analysis with X-ray crystallographic diffraction data to 2.0-Å revealed that each protein subunit harbors a hot dog-fold and that the TE6 enzyme forms a hexamer with D3 symmetry. An assessment of thioesterase activity against a range of acyl-CoA substrates revealed the greatest activity against acetyl-CoA, and structure-guided mutagenesis of putative active site residues identified Asn and Asp as being essential for activity. Our structural analysis revealed that six GDP nucleotides bound the enzyme in close proximity to an intersubunit disulfide bond interactions that covalently link thioesterase domains in a double hot dog dimer. Structure-guided mutagenesis of residues within the GDP-binding pocket identified Arg as playing a key role in the nucleotide interaction and revealed that GDP is required for activity. All mutations were confirmed to be specific and not to have resulted from structural perturbations by X-ray crystallography. This is the first report of a bacterial GDP-regulated thioesterase and of covalent linkage of thioesterase domains through a disulfide bond, revealing structural similarities with ADP regulation in the human ACOT12 thioesterase.

摘要

硫酯酶催化许多活化脂肪酸和酰基辅酶A底物中硫酯键的裂解。它们在原核生物和真核生物中均普遍表达,并根据其催化活性位点、蛋白质寡聚化和底物特异性细分为25个硫酯酶家族。尽管这些酶家族中的许多在功能和底物特异性方面已得到充分表征,但对大多数硫酯酶家族的调控了解甚少。在此,我们对来自细菌的一种TE6硫酯酶进行了表征。利用X射线晶体学衍射数据进行的结构分析显示,每个蛋白质亚基都具有一个热狗折叠结构,并且TE6酶形成具有D3对称性的六聚体。对一系列酰基辅酶A底物的硫酯酶活性评估显示,对乙酰辅酶A的活性最高,对假定活性位点残基的结构导向诱变确定天冬酰胺和天冬氨酸是活性所必需的。我们的结构分析表明,六个GDP核苷酸与该酶结合,紧邻亚基间二硫键相互作用,该相互作用在双热狗二聚体中以共价方式连接硫酯酶结构域。对GDP结合口袋内残基的结构导向诱变确定精氨酸在核苷酸相互作用中起关键作用,并表明活性需要GDP。所有突变均经证实具有特异性,并非由X射线晶体学引起的结构扰动导致。这是关于细菌GDP调节硫酯酶以及通过二硫键实现硫酯酶结构域共价连接的首次报道,揭示了与人类ACOT12硫酯酶中ADP调节的结构相似性。

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