Palanché Tania, Blanc Sylvie, Hennard Christophe, Abdallah Mohamed A, Albrecht-Gary Anne-Marie
Laboratoire de Physico-Chimie Bioinorganique, CNRS UMR 7509, ECPM, 25, Rue Becquerel, 67200 Strasbourg, France.
Inorg Chem. 2004 Feb 9;43(3):1137-52. doi: 10.1021/ic034862n.
Azotobacter vinelandii, a nitrogen-fixing soil bacterium, secretes in iron deficiency azotobactin delta, a highly fluorescent pyoverdin-like chromopeptidic hexadentate siderophore. The chromophore, derived from 2,3-diamino-6,7 dihydroxyquinoline, is bound to a peptide chain of 10 amino acids: (L)-Asp-(D)-Ser-(L)-Hse-Gly-(D)-beta-threo-HOAsp-(L)-Ser-(D)-Cit-(L)-Hse-(L)-Hse lactone-(D)-N(delta)-Acetyl, N(delta)-HOOrn. Azotobactin delta has three different iron(III) binding sites which are one hydroxamate group at the C-terminal end of the peptidic chain (N(delta)-Acetyl, N(delta)-HOOrn), one alpha-hydroxycarboxylic function in the middle of the chain (beta-threo-hydroxyaspartic acid), and one catechol group on the chromophore. The coordination properties of its iron(III) and iron(II) complexes were measured by spectrophotometry, potentiometry, and voltammetry after the determination of the acid-base functions of the uncomplexed free siderophore. Strongly negatively charged ferric species were observed at neutral p[H]'s corresponding to a predominant absolute configuration Lambda of the ferric complex in solution as deduced from CD measurements. The presence of an alpha-hydroxycarboxylic chelating group does not decrease the stability of the iron(III) complex when compared to the main trishydroxamate siderophores or to pyoverdins. The value of the redox potential of ferric azotobactin is highly consistent with a reductive step by physiological reductants for the iron release. Formation and dissociation kinetics of the azotobactin delta ferric complex point out that both ends of this long siderophore chain get coordinated to Fe(III) before the middle. The most striking result provided by fluorescence measurements is the lasting quenching of the fluorophore in the course of the protonation of the ferric azotobactin delta complex. Despite the release of the hydroxyacid and of the catechol, the fluorescence remains indeed quenched, when iron(III) is bound only to the hydroxamic acid, suggesting a folded conformation at this stage, around the metal ion, in contrast to the unfolded species observed for other siderophores such as ferrioxamine or pyoverdin PaA.
棕色固氮菌是一种能固氮的土壤细菌,在缺铁情况下会分泌阿佐菌素δ,它是一种具有高荧光性的类绿脓菌素的发色肽六齿铁载体。发色团源自2,3 - 二氨基 - 6,7 - 二羟基喹啉,与一条由10个氨基酸组成的肽链相连:(L)-天冬氨酸-(D)-丝氨酸-(L)-羟丝氨酸-甘氨酸-(D)-β-苏式-羟基天冬氨酸-(L)-丝氨酸-(D)-瓜氨酸-(L)-羟丝氨酸-(L)-羟丝氨酸内酯-(D)-N(δ)-乙酰基,N(δ)-羟基鸟氨酸。阿佐菌素δ有三个不同的铁(III)结合位点,分别是肽链C末端的一个异羟肟酸基团(N(δ)-乙酰基,N(δ)-羟基鸟氨酸)、链中间的一个α-羟基羧酸官能团(β-苏式-羟基天冬氨酸)以及发色团上的一个儿茶酚基团。在测定未络合的游离铁载体的酸碱官能团之后,通过分光光度法、电位滴定法和伏安法测量了其铁(III)和铁(II)配合物的配位性质。从中性pH值下观察到带强负电荷的铁物种,根据圆二色性测量推断,溶液中铁(III)配合物的主要绝对构型为Λ。与主要的三异羟肟酸铁载体或绿脓菌素相比,α-羟基羧酸螯合基团的存在并不会降低铁(III)配合物的稳定性。阿佐菌素铁的氧化还原电位值与铁释放过程中生理还原剂的还原步骤高度一致。阿佐菌素δ铁(III)配合物的形成和解离动力学表明,这条长铁载体链的两端在中间之前就与Fe(III)配位。荧光测量提供的最显著结果是,在阿佐菌素δ铁(III)配合物质子化过程中,荧光团持续猝灭。尽管释放了羟基酸和儿茶酚,但当铁(III)仅与异羟肟酸结合时,荧光确实仍然猝灭,这表明在此阶段围绕金属离子存在一种折叠构象,这与其他铁载体如去铁胺或绿脓菌素PaA所观察到的未折叠物种形成对比。
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