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黄素-二铁蛋白的组氨酸配体变体:对结构和活性的影响。

Histidine ligand variants of a flavo-diiron protein: effects on structure and activities.

机构信息

Department of Chemistry, University of Texas at San Antonio, San Antonio, TX 78249, USA.

出版信息

J Biol Inorg Chem. 2012 Dec;17(8):1231-9. doi: 10.1007/s00775-012-0938-4. Epub 2012 Sep 19.

DOI:10.1007/s00775-012-0938-4
PMID:22990880
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3508297/
Abstract

Flavo-diiron proteins (FDPs) contain non-heme diiron and proximal flavin mononucleotide (FMN) active sites and function as terminal components of a nitric oxide reductase (NOR) and/or a four-electron dioxygen reductase (O(2)R). While most FDPs show similar structural, spectroscopic, and redox properties, O(2)R and NOR activities vary significantly among FDPs. A potential source of this variability is the iron ligation status of a conserved His residue that provides an iron ligand in all known FDP structures but one, where this His residue is rotated away from iron and replaced by a solvent ligand. In order to test the effect of this His ligation status, we changed this ligating His residue (H90) in Thermotoga maritima (Tm) FDP to either Asn or Ala. The wild-type Tm FDP shows significantly higher O(2)R than NOR activity. Single crystal X-ray crystallography revealed a remarkably conserved diiron site structure in the H90N and -A variants, differing mainly by either Asn or solvent coordination, respectively, in place of H90. The steady-state activities were minimally affected by the H90 substitutions, remaining significantly higher for O(2)R versus NOR. The pre-steady-state kinetics of the fully reduced FDP with O(2) were also minimally affected by the H90 substitutions. The results indicate that the coordination status of this His ligand does not significantly modulate the O(2)R or NOR activities, and that FDPs can retain these activities when the individual iron centers are differentiated by His ligand substitution. This differentiation may have implications for the O(2)R and NOR mechanisms of FDPs.

摘要

黄素双铁蛋白(FDPs)含有非血红素双铁和近位黄素单核苷酸(FMN)活性位点,作为一氧化氮还原酶(NOR)和/或四电子氧还原酶(O(2)R)的末端组件发挥作用。虽然大多数 FDPs 表现出相似的结构、光谱和氧化还原性质,但 O(2)R 和 NOR 活性在 FDPs 之间差异很大。这种可变性的一个潜在来源是保守的 His 残基的铁配位状态,该残基在所有已知的 FDP 结构中提供一个铁配体,但有一种结构中,该 His 残基从铁上旋转并被溶剂配体取代。为了测试这种 His 配位状态的影响,我们将嗜热栖热菌(Tm)FDP 中的保守 His 残基(H90)改变为 Asn 或 Ala。野生型 Tm FDP 表现出显著更高的 O(2)R 比 NOR 活性。单晶 X 射线晶体学揭示了 H90N 和 -A 变体中非常保守的双铁位点结构,主要区别在于 H90 分别由 Asn 或溶剂配位取代。稳态活性受 H90 取代的影响最小,O(2)R 对 NOR 的活性仍然显著更高。与 O(2)的完全还原 FDP 的预稳态动力学也受 H90 取代的最小影响。结果表明,该 His 配体的配位状态不会显著调节 O(2)R 或 NOR 活性,并且当单个铁中心通过 His 配体取代区分时,FDP 可以保留这些活性。这种分化可能对 FDP 的 O(2)R 和 NOR 机制有影响。

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