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富含A+U的不稳定元件差异激活5'-3'和3'-5'mRNA衰变。

A+U-rich instability elements differentially activate 5'-3' and 3'-5' mRNA decay.

作者信息

Murray Elizabeth L, Schoenberg Daniel R

机构信息

Department of Molecular and Cellular Biochemistry, The Ohio State University, 1645 Neil Ave., Columbus, OH 43210-1218, USA.

出版信息

Mol Cell Biol. 2007 Apr;27(8):2791-9. doi: 10.1128/MCB.01445-06. Epub 2007 Feb 12.

Abstract

The A+U-rich elements (or AREs) are cis-acting sequences that activate rapid mRNA decay, yet the overall polarity of this process is unknown. The current study describes an unbiased approach to this using the Invader RNA assay (Third Wave Technologies, Inc.) to quantify the decay of each of the three exons of human beta-globin mRNA without added instability elements or with the AREs from c-fos or granulocyte-macrophage colony-stimulating factor (GM-CSF) mRNA in the 3' untranslated region. Each of these genes under tetracycline operator control was stably transfected into cells, and beta-globin mRNA was quantified with exon-specific probes following transcription termination. There was little overall evidence for polarity in stable mRNA decay. Adding the c-fos ARE activated rapid and simultaneous decay from both ends of the mRNA. In contrast, the GM-CSF ARE activated decay primarily from the mRNA 5' end. These data were supported by reciprocal RNA interference knockdowns, and we present evidence that the 5'-3' and 3'-5' decay pathways are functionally linked.

摘要

富含AU元件(或AREs)是激活mRNA快速降解的顺式作用序列,但该过程的整体极性尚不清楚。当前研究描述了一种无偏倚的方法,即使用入侵RNA检测法(Third Wave Technologies公司)来量化人β-珠蛋白mRNA三个外显子中每个外显子的降解情况,其中未添加不稳定元件,或在3'非翻译区带有来自c-fos或粒细胞-巨噬细胞集落刺激因子(GM-CSF)mRNA的AREs。这些在四环素操纵子控制下的每个基因都被稳定转染到细胞中,转录终止后用外显子特异性探针定量β-珠蛋白mRNA。在稳定的mRNA降解中几乎没有整体极性的证据。添加c-fos ARE会激活mRNA两端快速且同时的降解。相比之下,GM-CSF ARE主要从mRNA 5'端激活降解。这些数据得到了相互RNA干扰敲低实验的支持,并且我们提供证据表明5'-3'和3'-5'降解途径在功能上是相关联的。

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