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Production of superoxide radicals by soluble hydrogenase from Alcaligenes eutrophus H16.

机译:可溶性加氢酶从拟南芥H16中产生超氧自由基。

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摘要

The soluble hydrogenase (hydrogen-NAD+ oxidoreductase, EC 1.12.1.2) of Alcaligenes eutrophus H16 was shown to be stabilized by oxidation with oxygen and ferricyanide as long as electron donors and reducing compounds were absent. The simultaneous presence of H2, NADH and O2 in the enzyme solution, however, caused an irreversible inactivation of hydrogenase that was dependent on the O2 concentration. The half-life periods of 4 degrees C under partial pressures of 0.1, 5, 20 and 50% O2 were 11, 5, 2.5 and 1.5 h respectively. Evidence has been obtained that hydrogenase produces superoxide free radical anions (O2-.), which were detected by their ability to oxidize hydroxylamine to nitrite. The correlation between O2 concentration, nitrite formation and inactivation rates and the stabilization of hydrogenase by addition of superoxide dismutase indicated that superoxide radicals are responsible for enzyme inactivation. During short-term activity measurements (NAD+ reduction, H2 evolution from NADH), hydrogenase activity was inhibited by O2 only very slightly. In the presence of 0.7 mM-O2 an inhibition of about 20% was observed.
机译:研究表明,只要不存在电子供体和还原性化合物,Alcaligenes eutrophus H16的可溶性氢化酶(氢-NAD +氧化还原酶,EC 1.12.1.2)就可以通过用氧气和亚铁氰化物氧化而稳定。但是,在酶溶液中同时存在H2,NADH和O2会导致不可逆的氢化酶失活,这取决于O2的浓度。在0.1、5、20和50%O2的分压下4摄氏度的半衰期分别为11、5、2.5和1.5 h。已经获得的证据表明,氢化酶会产生超氧自由基阴离子(O2-。),可以通过将羟胺氧化为亚硝酸盐的能力进行检测。 O2浓度,亚硝酸盐形成和失活速率与通过添加超氧化物歧化酶而稳定氢化酶之间的相关性表明,超氧化物自由基是导致酶失活的原因。在短期活性测量中(NAD +还原,NADH释放出H2),O2仅轻微抑制了氢化酶活性。在0.7mM-O 2存在下,观察到约20%的抑制。

著录项

  • 作者

    Schneider, K; Schlegel, H G;

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  • 年度 1981
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  • 原文格式 PDF
  • 正文语种 en
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