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来自巴氏甲烷八叠球菌甲醇生长细胞的异二硫还原酶不是黄素酶。

Heterodisulfide reductase from methanol-grown cells of Methanosarcina barkeri is not a flavoenzyme.

作者信息

Künkel A, Vaupel M, Heim S, Thauer R K, Hedderich R

机构信息

Max-Planck-Institut für terrestrische Mikrobiologie, Marburg, Germany.

出版信息

Eur J Biochem. 1997 Feb 15;244(1):226-34. doi: 10.1111/j.1432-1033.1997.00226.x.

DOI:10.1111/j.1432-1033.1997.00226.x
PMID:9063468
Abstract

Heterodisulfide reductase from methanol-grown cells of Methanosarcina barkeri (MbHdrDE) is a membrane-bound enzyme composed of a 46-kDa subunit MbHdrD and a 23-kDa subunit MbHdrE. The enzyme has been shown to contain 0.6 mol heme and 20 mol Fe/S per mol heterodimer. In addition, substoichiometric amounts of FAD, thought to be an essential component of the active enzyme, were detected. We have now obtained preparations of active heterodisulfide reductase in high yields completely devoid of a flavin. Cloning and sequencing of the genes encoding MbHdrD and MbHdrE, which were found to form a transcription unit hdrED, revealed that both subunits also lack an FAD-binding motif. MbHdr thus differs from heterodisulifde reductase from Methanobacterium thermoautotrophicum (MtHdr), which is a flavo iron-sulfur protein composed of the subunits MtHdrA (80 kDa), MtHdrB (36 kDa) and MtHdrC (21 kDa), the subunit HdrA harboring the flavin-binding site. Sequence comparisons revealed that the N-terminal third of MbHdrD, which contained two sequence motifs for [4Fe-4S] clusters, is similar to MtHdrC and that the C-terminal two thirds of MbHdrD are similar to MtHdrB. Thus, MbHdrD and MtHdrC are structurally equivalent subunits. MbHdrE shows sequence similarity to b-type cytochromes, in agreement with the finding that this subunit contains a heme. These and other results indicate that MbHdrD harbors the active site of heterodisulfide reduction and that a flavin is not involved in catalysis. Since MbHdrD contains only iron-sulfur clusters, a mechanism of disulfide reduction involving one electron rather than two electron-transfer reactions has to be considered such as operative in ferredoxin :thioredoxin reductases from chloroplasts and cyanobacteria.

摘要

来自巴氏甲烷八叠球菌甲醇培养细胞的异二硫还原酶(MbHdrDE)是一种膜结合酶,由一个46 kDa的亚基MbHdrD和一个23 kDa的亚基MbHdrE组成。已证明该酶每摩尔异二聚体含有0.6摩尔血红素和20摩尔铁硫簇。此外,还检测到亚化学计量的FAD,其被认为是活性酶的必需成分。我们现在已经获得了高产率的活性异二硫还原酶制剂,且完全不含黄素。对编码MbHdrD和MbHdrE的基因进行克隆和测序,发现它们形成了一个转录单元hdrED,结果表明这两个亚基也缺乏FAD结合基序。因此,MbHdr不同于嗜热自养甲烷杆菌的异二硫还原酶(MtHdr),后者是一种黄素铁硫蛋白,由亚基MtHdrA(80 kDa)、MtHdrB(36 kDa)和MtHdrC(21 kDa)组成,亚基HdrA含有黄素结合位点。序列比较显示,MbHdrD的N端三分之一包含两个[4Fe - 4S]簇的序列基序,与MtHdrC相似,而MbHdrD的C端三分之二与MtHdrB相似。因此,MbHdrD和MtHdrC是结构等效的亚基。MbHdrE与b型细胞色素具有序列相似性,这与该亚基含有血红素的发现一致。这些以及其他结果表明,MbHdrD含有异二硫还原的活性位点,且黄素不参与催化作用。由于MbHdrD仅含有铁硫簇,因此必须考虑一种涉及单电子而非双电子转移反应的二硫还原机制,就像叶绿体和蓝细菌中的铁氧还蛋白:硫氧还蛋白还原酶所起的作用那样。

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