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髓过氧化物酶衍生的氧化剂迅速氧化并破坏蛋白质中的锌-半胱氨酸/组氨酸簇。

Myeloperoxidase-derived oxidants rapidly oxidize and disrupt zinc-cysteine/histidine clusters in proteins.

机构信息

The Heart Research Institute, Newtown, Sydney, NSW 2042, Australia.

出版信息

Free Radic Biol Med. 2012 Dec 1;53(11):2072-80. doi: 10.1016/j.freeradbiomed.2012.09.033. Epub 2012 Sep 29.

DOI:10.1016/j.freeradbiomed.2012.09.033
PMID:23032100
Abstract

Zinc is an abundant cellular transition metal ion, which binds avidly to protein cysteine (Cys) and histidine (His) residues to form zinc-Cys/His clusters; these play a key role in the function of many proteins (e.g., DNA binding and repair enzymes, transcription factors, nitric oxide synthase). Leukocyte-derived myeloperoxidase generates powerful oxidants including hypochlorous (HOCl), hypobromous (HOBr), and hypothiocyanous (HOSCN) acids from H(2)O(2) and (pseudo)halide ions. Excessive or misplaced formation of these species is associated with cellular dysfunction, apoptosis and necrosis, and multiple inflammatory diseases. HOCl and HOBr react rapidly with sulfur-containing compounds, and HOSCN reacts specifically with thiols. Consequently, we hypothesized that zinc-Cys/His clusters would be targets for these oxidants, and the activity of such enzymes would be perturbed. This hypothesis has been tested using yeast alcohol dehydrogenase (YADH), which contains a well-characterized Zn(1)Cys(2)His(1) cluster. Incubation of YADH with pathologically relevant concentrations of HOSCN, HOCl, and HOBr resulted in rapid oxidation of the protein (rate constants, determined by competition kinetics, for reaction of HOCl and HOSCN with YADH being (3.3±0.9)×10(8) and (2.9±0.4)×10(4) M(-1) s(-1) per YADH monomer, respectively), loss of enzyme activity, Zn(2+) release, changes in protein structure (particularly formation of disulfide cross-links), and oxidation of Cys residues. The loss of enzyme activity correlated with Zn(2+) release, loss of thiols, and changes in protein structure. We conclude that exposure of zinc-Cys/His clusters to inflammatory oxidants can result in impaired protein activity, thiol oxidation, and Zn(2+) release. These reactions may contribute to inflammation-induced tissue damage.

摘要

锌是一种丰富的细胞过渡金属离子,它与蛋白质半胱氨酸(Cys)和组氨酸(His)残基紧密结合,形成锌-Cys/His 簇;这些簇在许多蛋白质的功能中起着关键作用(例如,DNA 结合和修复酶、转录因子、一氧化氮合酶)。白细胞衍生的髓过氧化物酶从 H(2)O(2)和(拟)卤化物离子中生成强大的氧化剂,包括次氯酸(HOCl)、次溴酸(HOBr)和次硫氰酸(HOSCN)。这些物质的过度或错位形成与细胞功能障碍、细胞凋亡和坏死以及多种炎症性疾病有关。HOCl 和 HOBr 与含硫化合物快速反应,而 HOSCN 特异性与硫醇反应。因此,我们假设锌-Cys/His 簇将是这些氧化剂的靶标,并且这些酶的活性将受到干扰。该假设已通过使用酵母醇脱氢酶(YADH)进行了测试,YADH 含有一个特征良好的 Zn(1)Cys(2)His(1)簇。用与病理相关浓度的 HOSCN、HOCl 和 HOBr 孵育 YADH 导致蛋白质的快速氧化(通过竞争动力学确定的反应速率常数,HOCl 和 HOSCN 与 YADH 的反应分别为(3.3±0.9)×10(8)和(2.9±0.4)×10(4) M(-1) s(-1) per YADH 单体),酶活性丧失,Zn(2+)释放,蛋白质结构变化(特别是形成二硫键交联),以及 Cys 残基的氧化。酶活性的丧失与 Zn(2+)释放、硫醇氧化和蛋白质结构变化相关。我们得出结论,锌-Cys/His 簇暴露于炎症性氧化剂可导致蛋白质活性受损、硫醇氧化和 Zn(2+)释放。这些反应可能导致炎症引起的组织损伤。

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