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RNA 结合蛋白 HuR 和 AUF1 与人类 ATF3 mRNA 3'非翻译区的相互作用调节其氨基酸限制诱导的稳定性。

Interaction of RNA-binding proteins HuR and AUF1 with the human ATF3 mRNA 3'-untranslated region regulates its amino acid limitation-induced stabilization.

作者信息

Pan Yuan-Xiang, Chen Hong, Kilberg Michael S

机构信息

Department of Biochemistry and Molecular Biology, Genetics Institute, and Shands Cancer Center, University of Florida College of Medicine, Gainesville, Florida 32610, USA.

出版信息

J Biol Chem. 2005 Oct 14;280(41):34609-16. doi: 10.1074/jbc.M507802200. Epub 2005 Aug 17.

Abstract

ATF3 expression is induced in cells exposed to a variety of stress conditions, including nutrient limitation. Here we demonstrated that the mechanism by which the ATF3 mRNA content is increased following amino acid limitation of human HepG2 hepatoma cells is mRNA stabilization. Analysis of ATF3 mRNA turnover revealed that the half-life was increased from about 1 h in control cells to greater than 8 h in the histidine-deprived state, demonstrating mRNA stabilization in response to nutrient deprivation. Treatment of HepG2 cells with thapsigargin, which causes endoplasmic reticulum stress, also increased the half-life of ATF3 mRNA. HuR is an RNA-binding protein that regulates both the stability and cytoplasmic/nuclear localization of mRNA species containing AU-rich elements. Another RNA-binding protein, AUF1, regulates target mRNA molecules by enhancing their decay. Amino acid limitation caused a slightly elevated mRNA level for HuR and AUF1 mRNA. The nuclear HuR protein content was unchanged, and AUF1 protein increased slightly after amino acid limitation, whereas the cytoplasmic levels of both HuR and AUF1 protein increased. Immunoprecipitation of HuR-RNA complexes followed by reverse transcriptase-PCR analysis showed that HuR interacted with ATF3 mRNA in vivo and that this interaction increased following amino acid limitation. In contrast, the interaction of AUF1 with the ATF3 mRNA is decreased in histidine-deprived cells relative to control cells. Suppression of HuR expression by RNA interference partially blocked the accumulation of ATF3 mRNA following amino acid deprivation. The results demonstrated that coordinated regulation of mRNA stability by HuR and AUF1 proteins contributes to the observed increase in ATF3 expression following amino acid limitation.

摘要

ATF3表达在暴露于多种应激条件(包括营养限制)的细胞中被诱导。在此我们证明,人类肝癌细胞系HepG2在氨基酸限制后ATF3 mRNA含量增加的机制是mRNA稳定化。对ATF3 mRNA周转的分析显示,其半衰期从对照细胞中的约1小时增加到组氨酸缺乏状态下的超过8小时,表明对营养剥夺有mRNA稳定化反应。用毒胡萝卜素处理HepG2细胞(毒胡萝卜素会引起内质网应激)也增加了ATF3 mRNA的半衰期。HuR是一种RNA结合蛋白,可调节含有富含AU元件的mRNA的稳定性和细胞质/细胞核定位。另一种RNA结合蛋白AUF1通过增强靶mRNA分子的降解来进行调节。氨基酸限制导致HuR和AUF1 mRNA的mRNA水平略有升高。核HuR蛋白含量未变,氨基酸限制后AUF1蛋白略有增加,而HuR和AUF1蛋白的细胞质水平均增加。对HuR-RNA复合物进行免疫沉淀,随后进行逆转录-聚合酶链反应分析表明,HuR在体内与ATF3 mRNA相互作用,并且这种相互作用在氨基酸限制后增加。相比之下,相对于对照细胞,在组氨酸缺乏的细胞中AUF1与ATF3 mRNA的相互作用减少。通过RNA干扰抑制HuR表达可部分阻断氨基酸剥夺后ATF3 mRNA的积累。结果表明,HuR和AUF1蛋白对mRNA稳定性的协同调节有助于在氨基酸限制后观察到的ATF3表达增加。

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