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甲酸还原型大肠杆菌甲酸脱氢酶H:晶体结构的重新诠释提示了一种新的反应机制。

Formate-reduced E. coli formate dehydrogenase H: The reinterpretation of the crystal structure suggests a new reaction mechanism.

作者信息

Raaijmakers Hans C A, Romão Maria João

机构信息

REQUIMTE/CQFB, Departamento de Química, Faculdade de Ciências e Tecnologia, Universidade Nova de Lisboa, 2829-516, Monte de Caparica, Portugal.

出版信息

J Biol Inorg Chem. 2006 Oct;11(7):849-54. doi: 10.1007/s00775-006-0129-2. Epub 2006 Jul 8.

DOI:10.1007/s00775-006-0129-2
PMID:16830149
Abstract

Re-evaluation of the crystallographic data of the molybdenum-containing E. coli formate dehydrogenase H (Boyington et al. Science 275:1305-1308, 1997), reported in two redox states, reveals important structural differences for the formate-reduced form, with large implications for the reaction mechanism proposed in that work. We have re-refined the reduced structure with revised protocols and found substantial rearrangement in some parts of it. The original model is essentially correct but an important loop close to the molybdenum active site was mistraced, and, therefore, catalytic relevant residues were located in wrong positions. In particular selenocysteine-140, a ligand of molybdenum in the original work, and essential for catalysis, is no longer bound to the metal after reduction of the enzyme with formate. These results are incompatible with the originally proposed reaction mechanism. On the basis of our new interpretation, we have revised and proposed a new reaction mechanism, which reconciles the new X-ray model with previous biochemical and extended X-ray absorption fine structure data.

摘要

对含钼的大肠杆菌甲酸脱氢酶H的晶体学数据(Boyington等人,《科学》275:1305 - 1308,1997年)进行重新评估,该数据报告了两种氧化还原状态,结果显示甲酸还原形式存在重要的结构差异,这对该研究中提出的反应机制有重大影响。我们用修订后的方案对还原结构进行了重新精修,发现其中一些部分有大量重排。原始模型基本正确,但靠近钼活性位点的一个重要环被错误追踪,因此,催化相关残基位于错误位置。特别是硒代半胱氨酸-140,在原始研究中是钼的配体且对催化至关重要,在用甲酸还原酶后不再与金属结合。这些结果与最初提出的反应机制不相符。基于我们的新解释,我们修订并提出了一种新的反应机制,该机制使新的X射线模型与先前的生化和扩展X射线吸收精细结构数据相协调。

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