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一氧化二氮结合在亚硝基还原酶的一个[4Cu:2S]铜-硫簇中。

N2O binding at a [4Cu:2S] copper-sulphur cluster in nitrous oxide reductase.

机构信息

Lehrstuhl für Biochemie, Institut für organische Chemie und Biochemie, Albert-Ludwigs-Universität Freiburg, Albertstr. 21, 79104 Freiburg, Germany.

出版信息

Nature. 2011 Aug 14;477(7363):234-7. doi: 10.1038/nature10332.

DOI:10.1038/nature10332
PMID:21841804
Abstract

Nitrous oxide (N(2)O) is generated by natural and anthropogenic processes and has a critical role in environmental chemistry. It has an ozone-depleting potential similar to that of hydrochlorofluorocarbons as well as a global warming potential exceeding that of CO(2) 300-fold. In bacterial denitrification, N(2)O is reduced to N(2) by the copper-dependent nitrous oxide reductase (N(2)OR). This enzyme carries the mixed-valent Cu(A) centre and the unique, tetranuclear Cu(Z) site. Previous structural data were obtained with enzyme isolated in the presence of air that is catalytically inactive without prior reduction. Its Cu(Z) site was described as a [4Cu:S] centre, and the substrate-binding mode and reduction mechanism remained elusive. Here we report the structure of purple N(2)OR from Pseudomonas stutzeri, handled under the exclusion of dioxygen, and locate the substrate in N(2)O-pressurized crystals. The active Cu(Z) cluster contains two sulphur atoms, yielding a [4Cu:2S] stoichiometry; and N(2)O bound side-on at Cu(Z), in close proximity to Cu(A). With the substrate located between the two clusters, electrons are transferred directly from Cu(A) to N(2)O, which is activated by side-on binding in a specific binding pocket on the face of the [4Cu:2S] centre. These results reconcile a multitude of available biochemical data on N(2)OR that could not be explained by earlier structures, and outline a mechanistic pathway in which both metal centres and the intervening protein act in concert to achieve catalysis. This structure represents the first direct observation, to our knowledge, of N(2)O bound to its reductase, and sheds light on the functionality of metalloenzymes that activate inert small-molecule substrates. The principle of using distinct clusters for substrate activation and for reduction may be relevant for similar systems, in particular nitrogen-fixing nitrogenase.

摘要

一氧化二氮(N2O)是由自然和人为过程产生的,在环境化学中具有重要作用。它的臭氧消耗潜能类似于氢氯氟烃,全球变暖潜能是二氧化碳的 300 多倍。在细菌反硝化过程中,N2O 通过依赖铜的一氧化二氮还原酶(N2OR)还原为 N2。该酶携带混合价态的 Cu(A)中心和独特的四核 Cu(Z)位点。以前的结构数据是在有氧存在的情况下从酶中获得的,而没有预先还原,这种酶是无催化活性的。它的 Cu(Z)位点被描述为一个[4Cu:S]中心,而底物结合模式和还原机制仍然难以捉摸。在这里,我们报告了来自假单胞菌的紫色 N2OR 的结构,在排除氧气的情况下进行处理,并在 N2O 加压晶体中定位了底物。活性 Cu(Z)簇含有两个硫原子,产生[4Cu:2S]化学计量;N2O 侧接结合在 Cu(Z)上,靠近 Cu(A)。随着底物位于两个簇之间,电子直接从 Cu(A)转移到 N2O,N2O 通过侧接结合在[4Cu:2S]中心的特定结合口袋中被激活。这些结果调和了大量无法用早期结构解释的关于 N2OR 的可用生化数据,并概述了一种机制途径,其中两个金属中心和中间蛋白协同作用以实现催化。该结构代表了我们所知的第一个直接观察到的 N2O 与它的还原酶结合的结构,并阐明了激活惰性小分子底物的金属酶的功能。使用不同簇来激活底物和还原的原理可能与类似的系统有关,特别是固氮氮酶。

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