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Biotin Synthase Contains Two Distinct Iron-Sulfur Cluster Binding Sites: Chemical and Spectroelectrochemical Analysis of Iron-Sulfur Cluster Interconversions

机译:生物素合酶包含两个不同的铁硫簇结合位点:铁硫簇互变的化学和光谱电化学分析

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摘要

Biotin synthase is an iron-sulfur protein that utilizes AdoMet to catalyze the presumed radical-mediated insertion of a sulfur atom between the saturated C6 and C9 carbons of dethiobiotin. Biotin synthase (BioB) is aerobically purified as a dimer that contains [2Fe-2S]2+ clusters and is inactive in the absence of additional iron and reductants, and anaerobic reduction of BioB with sodium dithionite results in conversion to enzyme containing [4Fe-4S]2+ and/or [4Fe-4S]+ clusters. To establish the predominant cluster forms present in biotin synthase in anaerobic assays, and by inference in Escherichia coli, we have accurately determined the extinction coefficient and cluster content of the enzyme under oxidized and reduced conditions and have examined the equilibrium reduction potentials at which cluster reductions and conversions occur as monitored by UV/visible and EPR spectroscopy. In contrast to previous reports, we find that aerobically purified BioB contains ca. 1.2-1.5 [2Fe-2S]2+ clusters per monomer with ε452 = 8400 M-1 cm-1 per monomer. Upon reduction, the [2Fe-2S]2+ clusters are converted to [4Fe-4S] clusters with two widely separate reduction potentials of -140 and -430 mV. BioB reconstituted with excess iron and sulfide in 60% ethylene glycol was found to contain two [4Fe-4S]2+ clusters per monomer with ε400 = 30 000 M-1 cm-1 per monomer and is reduced with lower midpoint potentials of -440 and -505 mV, respectively. Finally, as predicted by the measured redox potentials, enzyme incubated under typical anaerobic assay conditions is repurified containing one [2Fe-2S]2+ cluster and one [4Fe-4S]2+ cluster per monomer. These results indicate that the dominant stable cluster state for biotin synthase is a dimer containing two [2Fe-2S]2+ and two [4Fe-4S]2+ clusters.
机译:生物素合酶是一种铁硫蛋白,它利用AdoMet催化在硫代生物素的饱和C6和C9碳原子之间推测的自由基介导的硫原子插入。生物素合酶(BioB)被有氧纯化为包含[2Fe-2S] 2 + 簇的二聚体,并且在没有额外的铁和还原剂的情况下是无活性的,并且连二亚硫酸钠对厌氧菌进行了厌氧还原。转化为含有[4Fe-4S] 2 + 和/或[4Fe-4S] + 簇的酶。为了确定在厌氧分析中生物素合酶中存在的主要簇形式,并通过推断大肠杆菌,我们已经准确确定了该酶在氧化和还原条件下的消光系数和簇含量,并研究了簇还原时的平衡还原电位转换发生在紫外/可见光谱和EPR光谱监测下。与以前的报告相反,我们发现需氧纯化的BioB含有ca。每个单体1.2-1.5 [2Fe-2S] 2 + 簇,每个单体的ε452= 8400 M -1 cm -1 。还原后,[2Fe-2S] 2 + 团簇被转换为具有-140和-430 mV的两个大大分开的还原电位的[4Fe-4S]团簇。发现用过量的铁和硫化物在60%的乙二醇中重构的BioB每个单体包含两个[4Fe-4S] 2 + 簇,其ε400= 30 000 M -1 cm每个单体 -1 并分别以-440和-505 mV的较低中点电位降低。最后,根据测得的氧化还原电势预测,在典型的厌氧分析条件下孵育的酶被重新纯化,其中包含一个[2Fe-2S] 2 + 簇和一个[4Fe-4S] 2 + 每个单体簇。这些结果表明,生物素合酶的主要稳定簇状态是包含两个[2Fe-2S] 2 + 和两个[4Fe-4S] 2 + 簇的二聚体。

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