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大肠杆菌细菌铁蛋白中铁氧化酶中心的鉴定。

Identification of the ferroxidase centre of Escherichia coli bacterioferritin.

作者信息

Le Brun N E, Andrews S C, Guest J R, Harrison P M, Moore G R, Thomson A J

机构信息

Centre for Metalloprotein Spectroscopy and Biology, School of Chemical Sciences, University of East Anglia, Norwich, U.K.

出版信息

Biochem J. 1995 Dec 1;312 ( Pt 2)(Pt 2):385-92.

PMID:8526846
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1136274/
Abstract

The bacterioferritin (BFR) of Escherichia coli takes up iron in the ferrous form and stores it within its central cavity as a hydrated ferric oxide mineral. The mechanism by which oxidation of iron (II) occurs in BFR is largely unknown, but previous studies indicated that there is ferroxidase activity associated with a site capable of forming a dinuclear-iron centre within each subunit [Le Brun, Wilson, Andrews, Harrison, Guest, Thomson and Moore (1993) FEBS Lett. 333, 197-202]. We now report site-directed mutagenesis experiments based on a putative dinuclear-metal-ion-binding site located within the BFR subunit. The data reveal that this dinuclear-iron centre is located at a site within the four-alpha-helical bundle of each subunit of BFR, thus identified as the ferroxidase centre of BFR. The metal-bound form of the centre bears a remarkable similarity to the dinuclear-iron sites of the hydroxylase subunit of methane mono-oxygenase and the R2 subunit of ribonucleotide reductase. Details of how the dinuclear centre of BFR is involved in the oxidation mechanism were investigated by studying the inhibition of iron (II) oxidation by zinc (II) ions. Data indicate that zinc (II) ions bind at the ferroxidase centre of apo-BFR in preference to iron (II), resulting in a dramatic reduction in the rate of oxidation. The mechanism of iron (II) oxidation is discussed in the light of this and previous work.

摘要

大肠杆菌的细菌铁蛋白(BFR)以亚铁形式摄取铁,并将其作为水合氧化铁矿物储存在其中心腔内。BFR中铁(II)氧化发生的机制在很大程度上尚不清楚,但先前的研究表明,在每个亚基内能够形成双核铁中心的位点存在亚铁氧化酶活性[勒·布伦、威尔逊、安德鲁斯、哈里森、格斯特、汤姆森和摩尔(1993年)《欧洲生物化学学会联合会快报》333卷,197 - 202页]。我们现在报告基于位于BFR亚基内的一个假定的双核金属离子结合位点进行的定点诱变实验。数据显示,这个双核铁中心位于BFR每个亚基的四螺旋束内的一个位点,因此被确定为BFR的亚铁氧化酶中心。该中心的金属结合形式与甲烷单加氧酶羟化酶亚基和核糖核苷酸还原酶R2亚基的双核铁位点有显著相似性。通过研究锌(II)离子对铁(II)氧化的抑制作用,对BFR双核中心如何参与氧化机制的细节进行了研究。数据表明,锌(II)离子优先于铁(II)结合在脱辅基BFR的亚铁氧化酶中心,导致氧化速率急剧降低。结合这项工作和先前的研究讨论了铁(II)氧化的机制。

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