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与AUF1相关的富含A+U元件结合活性的黏附依赖性调控。

Adhesion-dependent regulation of an A+U-rich element-binding activity associated with AUF1.

作者信息

Sirenko O I, Lofquist A K, DeMaria C T, Morris J S, Brewer G, Haskill J S

机构信息

Lineberger Comprehensive Cancer Center, University of North Carolina, Chapel Hill 27599-7295, USA.

出版信息

Mol Cell Biol. 1997 Jul;17(7):3898-906. doi: 10.1128/MCB.17.7.3898.

Abstract

Monocyte adherence results in the rapid transcriptional activation and mRNA stabilization of numerous mediators of inflammation and tissue repair. While the enhancer and promoter elements associated with transcriptional activation have been studied, mechanisms linking adhesion, mRNA stabilization, and translation are unknown. GROalpha and interleukin-1beta (IL-1beta) mRNAs are highly labile in nonadhered monocytes but stabilize rapidly after adherence. GROalpha and IL-1beta transcripts both contain A+U-rich elements (AREs) in the 3' untranslated region (UTR) which have been directly associated with rapid mRNA turnover. To determine if the GROalpha ARE region was recognized by factors associated with mRNA degradation, we carried out mobility gel shift analyses using a series of RNA probes encompassing the entire GROalpha transcript. Stable complexes were formed only with the proximal 3' UTR which contained the ARE region. The two slower-moving complexes were rapidly depleted following monocyte adherence but not direct integrin engagement. Deadherence reactivated the two largest ARE-binding complexes and destabilized IL-1beta transcripts. Antibody supershift studies demonstrated that both of these ARE RNA-binding complexes contained AUF1. The formation of these complexes and the accelerated mRNA turnover are phosphorylation-dependent events, as both are induced in adherent monocytes by the tyrosine kinase inhibitor genistein and the p38 MAP kinase inhibitor of IL-1beta translation, SK&F 86002. These results demonstrate that cell adhesion and deadhesion rapidly and reversibly modify both cytokine mRNA stability and the RNA-binding complexes associated with AUF1.

摘要

单核细胞黏附导致众多炎症和组织修复介质的快速转录激活和mRNA稳定。虽然与转录激活相关的增强子和启动子元件已被研究,但连接黏附、mRNA稳定和翻译的机制尚不清楚。GROα和白细胞介素-1β(IL-1β)mRNA在未黏附的单核细胞中高度不稳定,但黏附后迅速稳定。GROα和IL-1β转录本在3'非翻译区(UTR)均含有富含A+U的元件(AREs),这些元件与mRNA的快速周转直接相关。为了确定GROα ARE区域是否被与mRNA降解相关的因子识别,我们使用一系列涵盖整个GROα转录本的RNA探针进行了迁移率凝胶迁移分析。仅与包含ARE区域的近端3'UTR形成稳定复合物。单核细胞黏附后,这两种迁移较慢的复合物迅速减少,但直接整合素结合则不会。脱离黏附重新激活了两个最大的ARE结合复合物,并使IL-1β转录本不稳定。抗体超迁移研究表明,这两种ARE RNA结合复合物均含有AUF1。这些复合物的形成和mRNA周转加速是磷酸化依赖性事件,因为酪氨酸激酶抑制剂染料木黄酮和IL-1β翻译的p38 MAP激酶抑制剂SK&F 86002均可在黏附的单核细胞中诱导这两种事件。这些结果表明,细胞黏附和脱离黏附可快速且可逆地改变细胞因子mRNA稳定性以及与AUF1相关的RNA结合复合物。

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本文引用的文献

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J Biol Chem. 1996 May 24;271(21):12179-84. doi: 10.1074/jbc.271.21.12179.
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