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氮酶催化中的电子转移。

Electron transfer in nitrogenase catalysis.

机构信息

Department of Chemistry and Biochemistry, Utah State University, 0300 Old Main Hill, Logan, UT 84322, USA.

出版信息

Curr Opin Chem Biol. 2012 Apr;16(1-2):19-25. doi: 10.1016/j.cbpa.2012.02.012. Epub 2012 Mar 5.

Abstract

Nitrogenase is a two-component enzyme that catalyzes the nucleotide-dependent reduction of N2 to 2NH3. This process involves three redox-active metal-containing cofactors including a [4Fe-4S] cluster, an eight-iron P cluster and a seven-iron plus molybdenum FeMo-cofactor, the site of substrate reduction. A deficit-spending model for electron transfer has recently been proposed that incorporates protein conformational gating that favors uni-directional electron transfer among the metalloclusters for the activation of the substrate-binding site. Also reviewed is a proposal that each of the metal clusters cycles through only two redox states of the metal-sulfur core as the system accumulates the multiple electrons required for substrate binding and reduction. In particular, it was suggested that as FeMo-cofactor acquires the four electrons necessary for optimal binding of N2, each successive pair of electrons is stored as an Fe-H--Fe bridging hydride, with the FeMo-cofactor metal-ion core retaining its resting redox state. We here broaden the discussion of stable intermediates that might form when FeMo-cofactor receives an odd number of electrons.

摘要

固氮酶是一种由两个亚基组成的酶,能够催化核苷酸依赖性的 N2 还原为 2NH3。这个过程涉及三个氧化还原活性的金属配位因子,包括一个[4Fe-4S]簇、一个八铁 P 簇和一个七铁钼 FeMo 配位因子,是底物还原的位点。最近提出了一种赤字支出电子转移模型,其中包含蛋白质构象门控,有利于在金属簇之间单向电子转移,从而激活底物结合位点。还提出了一个建议,即每个金属簇在系统积累结合和还原底物所需的多个电子时,仅经历金属-硫核心的两个氧化还原状态的循环。特别是,有人建议,当 FeMo 配位因子获得最佳结合 N2 所需的四个电子时,每对连续的电子被存储为 Fe-H--Fe 桥接氢化物,而 FeMo 配位因子的金属离子核心保留其静止的氧化还原状态。我们在这里扩展了关于 FeMo 配位因子接收奇数个电子时可能形成的稳定中间产物的讨论。

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