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通过特异性掺入硒对非硒谷胱甘肽过氧化物酶进行翻译后激活。

Post-translational activation of non-selenium glutathione peroxidase of by specific incorporation of selenium.

作者信息

Takeda Toru

机构信息

Department of Advanced Bioscience, Faculty of Agriculture, Kinki University 3327-204 Nakamachi, Nara 631-8505, Japan.

出版信息

Biochem Biophys Rep. 2015 Aug 28;4:39-43. doi: 10.1016/j.bbrep.2015.08.018. eCollection 2015 Dec.

DOI:10.1016/j.bbrep.2015.08.018
PMID:29124185
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5668893/
Abstract

Glutathione peroxidase (GPX) plays a pivotal role in the protection of cells against oxidative damage. The green alga expresses both selenocysteine-containing GPX and the non-selenium GPX homolog (GPXH). We previously reported that supplementation of selenium to algal culture induces GPXH to exhibit GPX activity. Here we investigated the incorporation of selenium into GPXH and its causal relationship with the upregulation of the enzymatic activity. GPXH was purified from algal cells grown with selenium and proteolytically digested into four fragments. Selenium content analysis for these proteolytic fragments confirmed that GPXH-incorporated selenium is predominantly enriched in a fragment that carries the putative catalytic residue Cys-38. We next constructed three kinds of engineered GPXH proteins by substituting Ser for one of three Cys residues in native GPXH, Cys-38, -66, and -84, using a bacterial overexpression system, resulting in Cys38Ser, Cys66Ser, and Cys84Ser derivatives, respectively. Of these, the Cys66Ser and Cys84Ser derivatives exhibited the same level of selenium-dependent GPX activity as the normal recombinant GPXH, whereas the Cys38Ser mutant GPXH not only lost its activity completely but also demonstrated severely impaired incorporation of selenium. These findings strongly suggest that selenium is post-translationally assimilated into the Cys-38 of the GPXH protein, thereby enhancing its enzymatic activity.

摘要

谷胱甘肽过氧化物酶(GPX)在保护细胞免受氧化损伤方面起着关键作用。绿藻同时表达含硒代半胱氨酸的GPX和非硒GPX同源物(GPXH)。我们之前报道过,向藻类培养物中添加硒会诱导GPXH表现出GPX活性。在此,我们研究了硒在GPXH中的掺入情况及其与酶活性上调的因果关系。从用硒培养的藻类细胞中纯化出GPXH,并将其用蛋白酶消化成四个片段。对这些蛋白水解片段的硒含量分析证实,掺入GPXH的硒主要富集在一个携带假定催化残基Cys - 38的片段中。接下来,我们使用细菌过表达系统,通过将天然GPXH中三个半胱氨酸残基之一(Cys - 38、- 66和- 84)替换为丝氨酸,构建了三种工程化的GPXH蛋白,分别得到Cys38Ser、Cys66Ser和Cys84Ser衍生物。其中,Cys66Ser和Cys84Ser衍生物表现出与正常重组GPXH相同水平的硒依赖性GPX活性,而Cys38Ser突变型GPXH不仅完全丧失了活性,而且硒的掺入也严重受损。这些发现有力地表明,硒在翻译后被同化到GPXH蛋白的Cys - 38中,从而增强其酶活性。

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