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超氧化过氧化物酶 2 与蛋白二硫键异构酶 ERp46 相互作用。

Hyperoxidized peroxiredoxin 2 interacts with the protein disulfide- isomerase ERp46.

机构信息

Centre for Free Radical Research, Department of Pathology, University of Otago, P.O. Box 4345, Christchurch 8140, New Zealand.

出版信息

Biochem J. 2013 Aug 1;453(3):475-85. doi: 10.1042/BJ20130030.

Abstract

Prx (peroxiredoxin) 2 protects cells from deleterious oxidative damage. It catalyses the breakdown of hydroperoxides through a highly reactive cysteine residue and has been linked to chaperone activity that promotes cell survival under conditions of oxidative stress. It may also be involved in redox signalling by binding to other proteins. In the present study we have searched for binding partners of Prx2 in H2O2-treated Jurkat and human umbilical vein endothelial cells and discovered that the hyperoxidized form selectively co-precipitated with the protein disulfide-isomerase ERp46. Mutant analyses revealed that loss of the peroxidative cysteine residue of Prx2 also facilitated complex formation with ERp46, even without H2O2 treatment, whereas the resolving cysteine residue of Prx2 was indispensible for the interaction to occur. The complex involved a stable non-covalent interaction that was disassociated by the reduction of intramolecular disulfides in ERp46, or by disruption of the decameric structure of hyperoxidized Prx2. This is the first example of a protein interaction dependent on the hyperoxidized status of a Prx.

摘要

Prx(过氧化物酶)2 可保护细胞免受有害的氧化损伤。它通过一个高度反应性的半胱氨酸残基催化过氧化物的分解,并与伴侣活性有关,可促进细胞在氧化应激条件下的存活。它还可能通过与其他蛋白质结合参与氧化还原信号转导。在本研究中,我们在 H2O2 处理的 Jurkat 和人脐静脉内皮细胞中搜索 Prx2 的结合伴侣,并发现过氧化物酶活性丧失的 Prx2 形式选择性地与蛋白质二硫键异构酶 ERp46 共沉淀。突变分析表明,即使没有 H2O2 处理,Prx2 的过氧化半胱氨酸残基的丧失也会促进与 ERp46 的复合物形成,而 Prx2 的解析半胱氨酸残基对于发生相互作用是必不可少的。该复合物涉及稳定的非共价相互作用,可通过 ERp46 中分子内二硫键的还原或过氧化物酶 Prx2 的十聚体结构的破坏而解联。这是第一个依赖于 Prx 过氧化物状态的蛋白质相互作用的例子。

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