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通过核糖核酸酶III切割和核酸外切酶降解对酵母酸式还原酮双加氧酶mRNA的正常形式和3'延伸形式进行调控与监测。

Regulation and surveillance of normal and 3'-extended forms of the yeast aci-reductone dioxygenase mRNA by RNase III cleavage and exonucleolytic degradation.

作者信息

Zer Cindy, Chanfreau Guillaume

机构信息

Department of Chemistry and Biochemistry and the Molecular Biology Institute, University of California, Los Angeles, CA 90095, USA.

出版信息

J Biol Chem. 2005 Aug 12;280(32):28997-9003. doi: 10.1074/jbc.M505913200. Epub 2005 Jun 20.

DOI:10.1074/jbc.M505913200
PMID:15967792
Abstract

Aci-reductone dioxygenases are key enzymes in the methionine salvage pathway. The mechanisms by which the expression of this important class of enzymes is regulated are poorly understood. Here we show that the expression of the mRNA encoding the yeast aci-reductone dioxygenase ADI1 is controlled post-transcriptionally by RNase III cleavage. Cleavage occurs in a large bipartite stem loop structure present in the open reading frame region of the ADI1 mRNA. The ADI1 mRNA is up-regulated in the absence of the yeast orthologue of RNase III Rnt1p or of the 5' --> 3' exonucleases Xrn1p and Rat1p. 3'-Extended forms of this mRNA, including a polycistronic mRNA ADI1-YMR010W mRNA, also accumulate in cells lacking Rnt1p, Xrn1p, and Rat1p or the nuclear exosome component Rrp6p, suggesting that these 3'-extended forms are subject to nuclear surveillance. We show that the ADI1 mRNA is up-regulated under heat shock conditions in a Rnt1p-independent manner. We propose that Rnt1p cleavage targets degradation of the ADI1 mRNA to prevent its expression prior to heat shock conditions and that RNA surveillance by multiple ribonucleases helps prevent accumulation of aberrant 3'-extended forms of this mRNA that arise from intrinsically inefficient 3'-processing signals.

摘要

乙醛酸还原酶是甲硫氨酸补救途径中的关键酶。这类重要酶的表达调控机制目前还知之甚少。在此我们表明,编码酵母乙醛酸还原酶ADI1的mRNA的表达在转录后受核糖核酸酶III切割的控制。切割发生在ADI1 mRNA开放阅读框区域中存在的一个大的二分茎环结构内。在缺乏核糖核酸酶III的酵母同源物Rnt1p或5'→3'核酸外切酶Xrn1p和Rat1p时,ADI1 mRNA上调。这种mRNA的3'延伸形式,包括多顺反子mRNA ADI1 - YMR010W mRNA,也在缺乏Rnt1p、Xrn1p和Rat1p或核外切体组分Rrp6p的细胞中积累,这表明这些3'延伸形式受到核监测。我们表明,在热休克条件下,ADI1 mRNA以不依赖Rnt1p的方式上调。我们提出,Rnt1p切割靶向ADI1 mRNA的降解,以防止其在热休克条件之前表达,并且多种核糖核酸酶的RNA监测有助于防止这种mRNA的异常3'延伸形式的积累,这些异常形式源于本质上低效的3'加工信号。

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