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产甲烷球菌中节能氢化酶 B 的特性。

Characterization of energy-conserving hydrogenase B in Methanococcus maripaludis.

机构信息

Department of Microbiology, University of Georgia, Athens, Georgia 30602-2605, USA.

出版信息

J Bacteriol. 2010 Aug;192(15):4022-30. doi: 10.1128/JB.01446-09. Epub 2010 May 28.

Abstract

The Methanococcus maripaludis energy-conserving hydrogenase B (Ehb) generates low potential electrons required for autotrophic CO(2) assimilation. To analyze the importance of individual subunits in Ehb structure and function, markerless in-frame deletions were constructed in a number of M. maripaludis ehb genes. These genes encode the large and small hydrogenase subunits (ehbN and ehbM, respectively), a polyferredoxin and ferredoxin (ehbK and ehbL, respectively), and an ion translocator (ehbF). In addition, a gene replacement mutation was constructed for a gene encoding a putative membrane-spanning subunit (ehbO). When grown in minimal medium plus acetate (McA), all ehb mutants had severe growth deficiencies except the DeltaehbO::pac strain. The membrane-spanning ion translocator (DeltaehbF) and the large hydrogenase subunit (DeltaehbN) deletion strains displayed the severest growth defects. Deletion of the ehbN gene was of particular interest because this gene was not contiguous to the ehb operon. In-gel activity assays and Western blots confirmed that EhbN was part of the membrane-bound Ehb hydrogenase complex. The DeltaehbN strain was also sensitive to growth inhibition by aryl acids, indicating that Ehb was coupled to the indolepyruvate oxidoreductase (Ior), further supporting the hypothesis that Ehb provides low potential reductants for the anabolic oxidoreductases in M. maripaludis.

摘要

产甲烷球菌能量保存氢化酶 B(Ehb)产生用于自养 CO2 同化所需的低势能电子。为了分析单个亚基在 Ehb 结构和功能中的重要性,在许多产甲烷球菌 ehb 基因中构建了无标记的框内缺失。这些基因编码大型和小型氢化酶亚基(ehbN 和 ehbM,分别)、多铁氧还蛋白和铁氧还蛋白(ehbK 和 ehbL,分别)以及离子转运蛋白(ehbF)。此外,还构建了一个编码假定膜跨膜亚基(ehbO)的基因替换突变。在含有乙酸盐的最小培养基(McA)中生长时,除了 ehbO::pac 缺失株外,所有 ehb 突变体的生长都严重不足。膜跨离子转运蛋白(ehbF 缺失)和大型氢化酶亚基(ehbN 缺失)缺失菌株显示出最严重的生长缺陷。ehbN 基因的缺失特别有趣,因为该基因与 ehb 操纵子不连续。凝胶内活性测定和 Western blot 证实 EhbN 是膜结合 Ehb 氢化酶复合物的一部分。DeltaehbN 菌株也对芳基酸的生长抑制敏感,表明 Ehb 与吲哚丙酮酸氧化还原酶(Ior)偶联,进一步支持 Ehb 为产甲烷球菌中的合成氧化还原酶提供低势能还原剂的假说。

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