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肠杆菌菊欧文氏菌中铁载体控制的铁同化作用:细菌铁蛋白和Suf铁硫簇组装机制参与其中的证据

Siderophore-controlled iron assimilation in the enterobacterium Erwinia chrysanthemi: evidence for the involvement of bacterioferritin and the Suf iron-sulfur cluster assembly machinery.

作者信息

Expert Dominique, Boughammoura Aïda, Franza Thierry

机构信息

Laboratoire Interactions Plantes-Pathogènes, Unité Mixte de Recherche 217, Institut National de la Recherche Agronomique, AgroParisTech, Université Paris 6, 75005 Paris, France.

出版信息

J Biol Chem. 2008 Dec 26;283(52):36564-72. doi: 10.1074/jbc.M807749200. Epub 2008 Nov 6.

DOI:10.1074/jbc.M807749200
PMID:18990691
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2662311/
Abstract

The intracellular fate of iron acquired by bacteria during siderophore-mediated assimilation is poorly understood. We investigated this question in the pathogenic enterobacterium Erwinia chrysanthemi. This bacterium produces two siderophores, chrysobactin and achromobactin, during plant infection. We analyzed the distribution of iron into cytosolic proteins in bacterial cells supplied with 59Fe-chrysobactin using native gel electrophoresis. A parental strain and mutants deficient in bacterioferritin (bfr), miniferritin (dps), ferritin (ftnA), bacterioferredoxin (bfd), or iron-sulfur cluster assembly machinery (sufABCDSE) were studied. In the parental strain, we observed two rapidly 59Fe-labeled protein signals identified as bacterioferritin and an iron pool associated to the protein chain-elongation process. In the presence of increased 59Fe-chrysobactin concentrations, we detected mini-ferritin-bound iron. Iron incorporation into bacterioferritin was severely reduced in nonpolar sufA, sufB, sufD, sufS, and sufE mutants but not in a sufC background. Iron recycling from bacterioferritin did not occur in bfd and sufC mutants. Iron depletion caused a loss of aconitase activity, whereas ferric chrysobactin supplementation stimulated the production of active aconitase in parental cells and in bfr and bfd mutants. Aconitase activity in sufA, sufB, sufD, sufS, and sufE mutant strains was 10 times lower than that in parental cells. In the sufC mutant, it was twice as low as that in the parental strain. Defects observed in the mutants were not caused by altered ferric chrysobactin transport. Our data demonstrate a functional link between bacterioferritin, bacterioferredoxin, and the Suf protein machinery resulting in optimal bacterial growth and a balanced distribution of iron between essential metalloproteins.

摘要

在铁载体介导的同化过程中,细菌获取的铁在细胞内的命运尚不清楚。我们在致病性肠道细菌菊欧文氏菌中研究了这个问题。这种细菌在植物感染期间产生两种铁载体,即金黄色菌素和无色菌素。我们使用天然凝胶电泳分析了在供应59Fe-金黄色菌素的细菌细胞中铁在胞质蛋白中的分布。研究了亲本菌株以及缺乏细菌铁蛋白(bfr)、小型铁蛋白(dps)、铁蛋白(ftnA)、细菌铁氧化还原蛋白(bfd)或铁硫簇组装机制(sufABCDSE)的突变体。在亲本菌株中,我们观察到两个快速被59Fe标记的蛋白质信号,鉴定为细菌铁蛋白和与蛋白质链延伸过程相关的铁池。在59Fe-金黄色菌素浓度增加的情况下,我们检测到与小型铁蛋白结合的铁。在非极性sufA、sufB、sufD、sufS和sufE突变体中,铁掺入细菌铁蛋白的过程严重减少,但在sufC背景下则没有。在bfd和sufC突变体中,细菌铁蛋白中的铁没有发生循环利用。铁缺乏导致乌头酸酶活性丧失,而补充铁离子金黄色菌素刺激亲本细胞以及bfr和bfd突变体中活性乌头酸酶的产生。sufA、sufB、sufD、sufS和sufE突变体菌株中的乌头酸酶活性比亲本细胞低10倍。在sufC突变体中,其活性比亲本菌株低两倍。在突变体中观察到的缺陷不是由铁离子金黄色菌素转运改变引起的。我们的数据表明细菌铁蛋白、细菌铁氧化还原蛋白和Suf蛋白机制之间存在功能联系,从而实现细菌的最佳生长以及必需金属蛋白之间铁的平衡分布。

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