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首页> 外文期刊>Journal of biological inorganic chemistry: JBIC: a publication of the Society of Biological Inorganic Chemistry >Interaction of the active site of the Ni-Fe-Se hydrogenase from Desulfovibrio vulgaris Hildenborough with carbon monoxide and oxygen inhibitors
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Interaction of the active site of the Ni-Fe-Se hydrogenase from Desulfovibrio vulgaris Hildenborough with carbon monoxide and oxygen inhibitors

机译:寻常脱硫弧菌希尔登堡的镍铁硒氢化酶活性位点与一氧化碳和氧气抑制剂的相互作用

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摘要

The study of Ni-Fe-Se hydrogenases is interesting from the basic research point of view because their active site is a clear example of how nature regulates the catalytic function of an enzyme by the change of a single residue, in this case a cysteine, which is replaced by a selenocysteine. Most hydrogenases are inhibited by CO and O_2. In this work we studied these inhibition processes for the Ni-Fe-Se hydrogenase from Desulfovibrio vulgaris Hildenborough by combining catalytic activity measurements, followed by mass spectrometry or chronoamperometry, with Fourier transform IR spectroscopy experiments. The results show that the CO inhibitor binds to Ni in both conformations of the active site of this hydrogenase in a way similar to that in standard Ni-Fe hydrogenases, although in one of the CO-inhibited conformations the active site of the Ni-Fe-Se hydrogenase is more protected against the attack by O_2. The inhibition of the Ni-Fe-Se hydrogenase activity by O _2 could be explained by oxidation of the terminal cysteine ligand of the active-site Ni, instead of the direct attack of O_2 on the bridging site between Ni and Fe.
机译:从基础研究的角度出发,对Ni-Fe-Se氢化酶的研究很有趣,因为它们的活性位点是自然界如何通过改变单个残基(在这种情况下为半胱氨酸)来调节酶的催化功能的明确实例。被硒代半胱氨酸代替。大多数氢化酶均受CO和O_2抑制。在这项工作中,我们通过结合催化活性测量,质谱或计时安培与傅里叶变换红外光谱实验相结合,研究了对脱硫弧菌希尔登堡的镍铁硒化氢酶的这些抑制过程。结果表明,CO抑制剂以与标准Ni-Fe氢化酶相似的方式在该氢化酶活性位点的两个构象中结合Ni,尽管在一种CO抑制构象中Ni-Fe的活性位点-Se氢化酶更能抵抗O_2的攻击。 O _2对Ni-Fe-Se氢化酶活性的抑制作用可以用活性位点Ni的末端半胱氨酸配体的氧化来解释,而不是O_2直接攻击Ni和Fe之间的桥接位点。

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