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自身抗原介导氧化应激诱导的 Nrf2 蛋白翻译从头合成。

La autoantigen mediates oxidant induced de novo Nrf2 protein translation.

机构信息

Department of Pharmacology, University of Arizona, College of Medicine, 1501 N Campbell Ave, Tucson, Arizona 85724, USA.

出版信息

Mol Cell Proteomics. 2012 Jun;11(6):M111.015032. doi: 10.1074/mcp.M111.015032. Epub 2011 Dec 29.

DOI:10.1074/mcp.M111.015032
PMID:22207702
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3433904/
Abstract

Nrf2 gene encodes a transcription factor that regulates the expression of a cluster of antioxidant and detoxification genes. Recent works from our laboratory indicate that oxidative stress causes rapid de novo synthesis of Nrf2 protein. We have found that 5' Untranslated Region (5'UTR) of Nrf2 allows the mRNA to undergo an Internal Ribosomal Entry Site (IRES) mediated protein translation. Using liquid chromatography tandem MS, we have discovered that La/SSB protein bound to Nrf2 5'UTR in response to oxidative stress. In vitro RNA binding and in vivo ribonucleoprotein immunoprecipitation showed H(2)O(2) dose and time dependent increases of La/SSB binding to Nrf2 5'UTR. La/SSB protein translocated from the nuclei to cytoplasm and distributed in the perinuclear space in cells treated with H(2)O(2). Isolation of ribosomal fractions indicated that oxidants caused an association of La/SSB with ribosomes. Physical interaction of La/SSB with representative proteins from the small or large subunits of ribosomes was found to increase in cells responding to H(2)O(2) treatment. Knocking down La/SSB gene with siRNA prevented Nrf2 protein elevation or Nrf2 5'UTR activation by oxidants. In contrast, overexpression of La/SSB gene was able to enhance Nrf2 5'UTR activation and Nrf2 protein increase. Our data suggest that oxidants cause nuclear export of La/SSB protein and subsequent association of La/SSB with Nrf2 5'UTR and ribosomes. These events contribute to de novo Nrf2 protein translation because of oxidative stress.

摘要

Nrf2 基因编码一种转录因子,可调节抗氧化和解毒基因簇的表达。我们实验室的最新研究表明,氧化应激会导致 Nrf2 蛋白的快速从头合成。我们发现 Nrf2 的 5'非翻译区(5'UTR)允许 mRNA 通过内部核糖体进入位点(IRES)介导的蛋白质翻译。通过液相色谱串联质谱,我们发现 La/SSB 蛋白在氧化应激时与 Nrf2 5'UTR 结合。体外 RNA 结合和体内核糖核蛋白免疫沉淀显示 H2O2 剂量和时间依赖性增加 La/SSB 与 Nrf2 5'UTR 的结合。La/SSB 蛋白从细胞核易位到细胞质,并在 H2O2 处理的细胞中分布在核周空间。核糖体部分的分离表明氧化剂引起 La/SSB 与核糖体的关联。在响应 H2O2 处理的细胞中,发现 La/SSB 与核糖体小或大亚基的代表性蛋白之间的物理相互作用增加。用 siRNA 敲低 La/SSB 基因可防止氧化剂引起的 Nrf2 蛋白升高或 Nrf2 5'UTR 激活。相反,La/SSB 基因的过表达能够增强 Nrf2 5'UTR 激活和 Nrf2 蛋白增加。我们的数据表明,氧化剂导致 La/SSB 蛋白的核输出,随后与 Nrf2 5'UTR 和核糖体结合。这些事件导致应激氧化引起的 Nrf2 蛋白的从头翻译。

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