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光生氧化剂和长寿命、反应性、过氧化物光产物的细胞效应。

Cellular effects of photogenerated oxidants and long-lived, reactive, hydroperoxide photoproducts.

机构信息

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

出版信息

Free Radic Biol Med. 2010 Nov 30;49(10):1505-15. doi: 10.1016/j.freeradbiomed.2010.08.006. Epub 2010 Aug 12.

DOI:10.1016/j.freeradbiomed.2010.08.006
PMID:20708682
Abstract

Reaction of radicals and singlet oxygen ((1)O(2)) with proteins results in both direct damage and the formation of long-lived reactive hydroperoxides. Elevated levels of protein hydroperoxide-derived products have been detected in multiple human pathologies, suggesting that these secondary oxidants contribute to tissue damage. Previous studies have provided evidence for protein hydroperoxide-mediated inhibition of thiol-dependent enzymes and modulation of signaling processes in isolated systems. In this study (1)O(2) and hydroperoxides have been generated in J774A.1 macrophage-like cells using visible light and the photosensitizer rose bengal, with the consequences of oxidant formation examined both immediately and after subsequent (dark-phase) incubation. Significant losses of GSH (≤50%), total thiols (≤20%), and activity of thiol-dependent proteins (GAPDH, thioredoxin, protein tyrosine phosphatases, creatine kinase, and cathepsins B and L; 10-50% inhibition) were detected after 1 or 2 min photo-oxidation. Non-thiol-dependent enzymes were not affected. In contrast, NADPH levels increased, together with the activity of glutathione reductase, glutathione peroxidase, and thioredoxin reductase; these increases may be components of a rapid global cytoprotective cellular response to stress. Neither oxidized thioredoxin nor radical-mediated protein oxidation products were detected at significant levels. Further decreases in thiol levels and enzyme activity occurred during dark-phase incubation, with this accompanied by decreased cell viability. These secondary events are ascribed to the reactions of long-lived hydroperoxides, generated by (1)O(2)-mediated reactions. Overall, this study provides novel insights into early cellular responses to photo-oxidative damage and indicates that long-lived hydroperoxides can play a significant role in cellular damage.

摘要

自由基和单线态氧(1O2)与蛋白质的反应会导致直接损伤和长寿命的反应性过氧化物的形成。在多种人类病理中都检测到了蛋白质过氧化物衍生产物的水平升高,这表明这些次级氧化剂会导致组织损伤。先前的研究已经为蛋白质过氧化物介导的巯基依赖性酶抑制和信号转导过程的调节提供了证据。在这项研究中,使用可见光和光敏剂玫瑰红孟加拉在 J774A.1 巨噬细胞样细胞中产生 1O2 和过氧化物,检查了氧化剂形成的直接和随后(暗相)孵育后的后果。在 1 或 2 分钟光氧化后,GSH(≤50%)、总巯基(≤20%)和巯基依赖性蛋白(GAPDH、硫氧还蛋白、蛋白酪氨酸磷酸酶、肌酸激酶和组织蛋白酶 B 和 L;10-50%抑制)的活性显著丧失。非巯基依赖性酶不受影响。相比之下,NADPH 水平增加,同时还增加了谷胱甘肽还原酶、谷胱甘肽过氧化物酶和硫氧还蛋白还原酶的活性;这些增加可能是细胞对应激的快速全局细胞保护反应的组成部分。未检测到氧化的硫氧还蛋白或自由基介导的蛋白质氧化产物达到显著水平。在暗相孵育期间,巯基水平和酶活性进一步降低,同时细胞活力降低。这些次要事件归因于(1)O2 介导的反应生成的长寿命过氧化物的反应。总的来说,这项研究为早期细胞对光氧化损伤的反应提供了新的见解,并表明长寿命的过氧化物可以在细胞损伤中发挥重要作用。

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