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Puf1p与其他酵母Puf蛋白共同作用来控制mRNA的稳定性。

Puf1p acts in combination with other yeast Puf proteins to control mRNA stability.

作者信息

Ulbricht Randi J, Olivas Wendy M

机构信息

Department of Biology, University of Missouri-St. Louis, St. Louis, Missouri 63121, USA.

出版信息

RNA. 2008 Feb;14(2):246-62. doi: 10.1261/rna.847408. Epub 2007 Dec 19.

Abstract

The eukaryotic Puf proteins bind 3' untranslated region (UTR) sequence elements to regulate the stability and translation of their target transcripts, and such regulatory events are critical for cell growth and development. Several global genome analyses have identified hundreds of potential mRNA targets of the Saccharomyces cerevisiae Puf proteins; however, only three mRNA targets for these proteins have been characterized thus far. After direct testing of nearly 40 candidate mRNAs, we established two of these as true mRNA targets of Puf-mediated decay in yeast, HXK1 and TIF1. In a novel finding, multiple Puf proteins, including Puf1p, regulate both of these mRNAs in combination. TIF1 mRNA decay can be stimulated individually by Puf1p and Puf5p, but the combination of both proteins is required for full regulation. This Puf-mediated decay requires the presence of two UGUA binding sites within the TIF1 3' UTR, with one site regulated by Puf5p and the other by both Puf1p and Puf5p. Alteration of the UGUA site in the tif1 3' UTR to more closely resemble the Puf3p binding site broadens the specificity to include regulation by Puf3p. The stability of the endogenously transcribed HXK1 mRNA, cellular levels of Hxk1 protein activity, and HXK1 3' UTR-directed decay are affected by Puf1p and Puf5p as well as Puf4p. Together these results identify the first mRNA targets of Puf1p-mediated decay, describe similar yet distinct combinatorial control of two new target mRNAs by the yeast Puf proteins, and suggest the importance of direct testing to evaluate RNA-regulatory mechanisms.

摘要

真核生物的Puf蛋白结合3'非翻译区(UTR)序列元件,以调节其靶转录本的稳定性和翻译,而这种调节事件对细胞生长和发育至关重要。多项全基因组分析已鉴定出酿酒酵母Puf蛋白数百个潜在的mRNA靶标;然而,迄今为止,仅对其中三个mRNA靶标进行了表征。在对近40个候选mRNA进行直接测试后,我们确定其中两个是酵母中Puf介导的降解的真正mRNA靶标,即HXK1和TIF1。一项新发现表明,多种Puf蛋白,包括Puf1p,共同调节这两个mRNA。Puf1p和Puf5p可分别刺激TIF1 mRNA的降解,但两种蛋白共同作用才能实现完全调节。这种Puf介导的降解需要TIF1 3'UTR内存在两个UGUA结合位点,其中一个位点由Puf5p调节,另一个位点由Puf1p和Puf5p共同调节。将tif1 3'UTR中的UGUA位点改变为更类似于Puf3p结合位点,可拓宽特异性,使其包括Puf3p的调节作用。内源性转录的HXK1 mRNA的稳定性、Hxk1蛋白活性的细胞水平以及HXK1 3'UTR介导的降解均受Puf1p、Puf5p以及Puf4p的影响。这些结果共同确定了Puf1p介导的降解的首批mRNA靶标,描述了酵母Puf蛋白对两个新靶标mRNA的相似但又不同的组合控制,并表明直接测试对评估RNA调节机制的重要性。

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