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热醋穆尔氏菌中一种可逆的电子分叉依赖铁氧还蛋白和 NAD 的 [FeFe]-氢化酶(HydABC)。

A reversible electron-bifurcating ferredoxin- and NAD-dependent [FeFe]-hydrogenase (HydABC) in Moorella thermoacetica.

机构信息

Max Planck Institute for Terrestrial Microbiology, Marburg, Germany.

出版信息

J Bacteriol. 2013 Mar;195(6):1267-75. doi: 10.1128/JB.02158-12. Epub 2013 Jan 11.

Abstract

Moorella thermoacetica was long the only model organism used to study the biochemistry of acetogenesis from CO(2). Depending on the growth substrate, this Gram-positive bacterium can either form H(2) or consume it. Despite the importance of H(2) in its metabolism, a hydrogenase from the organism has not yet been characterized. We report here the purification and properties of an electron-bifurcating [FeFe]-hydrogenase from M. thermoacetica and show that the cytoplasmic enzyme efficiently catalyzes both H(2) formation and H(2) uptake. The purified heterotrimeric iron-sulfur flavoprotein (HydABC) catalyzed the coupled reduction of ferredoxin (Fd) and NAD(+) with H(2) at 55 °C at pH 7.5 at a specific rate of about 100 μmol min(-1) mg protein(-1) and the reverse reaction, the coupled reduction of protons to H(2) with reduced ferredoxin and NADH, at a specific rate of about 10 μmol min(-1) mg protein(-1) in the stoichiometry Fd(ox) + NAD(+) + 2H(2) Fd(red)(2-) + NADH + 3H(+). When ferredoxin from Clostridium pasteurianum, NAD(+), and the enzyme were incubated at pH 7.0 under 100% H(2) in the gas phase (E(0)' = -414 mV), more than 95% of the ferredoxin (E(0)' = -400 mV) was reduced, which indicated that ferredoxin reduction with H(2) is driven by the exergonic reduction of NAD(+) (E(0)' = -320 mV) with H(2). In the absence of NAD(+), ferredoxin was not reduced. We identified the genes encoding HydABC within the transcriptional unit hydCBAX and mapped the transcription start site.

摘要

高温产乙酰菌长期以来一直是唯一用于研究从 CO(2) 生成乙酰的生物化学的模式生物。根据生长基质的不同,这种革兰氏阳性菌既可以形成 H(2),也可以消耗 H(2)。尽管 H(2)在其新陈代谢中很重要,但该生物的氢化酶尚未得到表征。我们在此报告从高温产乙酰菌中纯化和特性鉴定的电子分叉 [FeFe]-氢化酶,并表明细胞质酶有效地催化 H(2)的形成和 H(2)的摄取。纯化的异三聚体铁-硫黄素蛋白(HydABC)在 55°C、pH7.5 下以约 100 μmol min(-1) mg 蛋白(-1)的比速率,用 H(2)催化还原型铁氧还蛋白(Fd)和 NAD(+)的偶联还原,以及在质子还原为 H(2)的逆反应中,用还原型铁氧还蛋白和 NADH 以约 10 μmol min(-1) mg 蛋白(-1)的比速率在化学计量 Fd(ox) + NAD(+) + 2H(2) Fd(red)(2-) + NADH + 3H(+)下还原质子。当在气相中用 100% H(2)在 pH7.0 下孵育时,来自巴氏梭菌的铁氧还蛋白、NAD(+)和酶(E(0)' = -414 mV),超过 95%的铁氧还蛋白(E(0)' = -400 mV)被还原,这表明铁氧还蛋白的还原与 H(2)是由 NAD(+)(E(0)' = -320 mV)与 H(2)的放能还原驱动的。在没有 NAD(+)的情况下,铁氧还蛋白没有被还原。我们在转录单元 hydCBAX 内鉴定编码 HydABC 的基因,并定位转录起始位点。

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