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炭疽芽孢杆菌(BA1797)的尿苷一磷酸激酶晶体结构揭示了一个变构核苷酸结合位点。

The crystal structure of UMP kinase from Bacillus anthracis (BA1797) reveals an allosteric nucleotide-binding site.

作者信息

Meier Christoph, Carter Lester G, Sainsbury Sarah, Mancini Erika J, Owens Raymond J, Stuart David I, Esnouf Robert M

机构信息

Oxford Protein Production Facility, University of Oxford, The Henry Wellcome Building for Genomic Medicine, Roosevelt Drive, Oxford OX3 7BN, UK.

出版信息

J Mol Biol. 2008 Sep 19;381(5):1098-105. doi: 10.1016/j.jmb.2008.06.078. Epub 2008 Jul 3.

Abstract

Uridine monophosphate (UMP) kinase is a conserved enzyme that catalyzes the ATP-driven conversion of uridylate monophosphate into uridylate diphosphate, an essential metabolic step. In prokaryotes, the enzyme exists as a homohexamer that is regulated by various metabolites. Whereas the enzymatic mechanism of UMP kinase (UK) is well-characterized, the molecular basis of its regulation remains poorly understood. Here we report the crystal structure of UK from Bacillus anthracis (BA1797) in complex with ATP at 2.82 A resolution. It reveals that the cofactor, in addition to binding in the active sites, also interacts with separate binding pockets located near the center of the hexameric structure. The existence of such an allosteric binding site had been predicted by biochemical studies, but it was not identified in previous crystal structures of prokaryotic UKs. We show that this putative allosteric pocket is conserved across different bacterial species, suggesting that it is a feature common to bacterial UKs, and we present a structural model for the allosteric regulation of this enzyme.

摘要

尿苷单磷酸激酶(UMP激酶)是一种保守的酶,它催化由ATP驱动的单磷酸尿苷向二磷酸尿苷的转化,这是一个必不可少的代谢步骤。在原核生物中,该酶以同六聚体形式存在,受多种代谢物调节。虽然UMP激酶(UK)的酶促机制已得到充分表征,但其调节的分子基础仍知之甚少。在此,我们报道了炭疽芽孢杆菌(BA1797)的UK与ATP复合物的晶体结构,分辨率为2.82 Å。结果表明,辅因子除了结合在活性位点外,还与位于六聚体结构中心附近的独立结合口袋相互作用。生化研究曾预测存在这样一个别构结合位点,但在先前原核生物UK的晶体结构中未被发现。我们表明,这个假定的别构口袋在不同细菌物种中是保守的,这表明它是细菌UK的一个共同特征,并且我们提出了该酶别构调节的结构模型。

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