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编码酵母ARE结合蛋白Cth2的信使核糖核酸是通过一种全新的3'加工途径产生的。

The mRNA encoding the yeast ARE-binding protein Cth2 is generated by a novel 3' processing pathway.

作者信息

Ciais Delphine, Bohnsack Markus T, Tollervey David

机构信息

Wellcome Trust Centre for Cell Biology, University of Edinburgh, EH9 3JR, UK.

出版信息

Nucleic Acids Res. 2008 May;36(9):3075-84. doi: 10.1093/nar/gkn160. Epub 2008 Apr 8.

Abstract

Microarray analyses of mRNAs over-expressed in strains lacking the nuclear exosome component Rrp6 identified the transcript encoding the ARE-binding protein Cth2, which functions in cytoplasmic mRNA stability. Subsequent northern analyses revealed that exosome mutants accumulate a 3'-extended transcript at the expense of the mature CTH2 mRNA. The 3' ends of the CTH2 mRNA were mapped to a GU(3-5) repeat, unlike any previously characterized polyadenylation site. CTH2 mRNA accumulation was not inhibited by mutations in 3'-cleavage and polyadenylation factors, Rna14, Rna15 and Pap1, which block accumulation of other mRNAs. The 3'-extended CTH2 pre-mRNA strongly accumulated in strains with mutations in the TRAMP4 polyadenylation complex or the Nrd1/Nab3/Sen1 complex, and contains multiple Nrd1 and Nab3 binding sites. CTH2 carries a consensus ARE element and levels of the pre-mRNA and mRNA were elevated by mutation of the ARE or inactivation of the nuclear 5'-exonuclease Rat1. We propose that CTH2 mRNA is processed from a 3'-extended primary transcript by the exosome, TRAMP and Nrd1/Nab3/Sen1 complexes. This unusual pathway may allow time for nuclear, ARE-mediated regulation of CTH2 levels involving Rat1.

摘要

对缺乏核外切体组分Rrp6的菌株中过表达的mRNA进行微阵列分析,鉴定出编码ARE结合蛋白Cth2的转录本,该蛋白在细胞质mRNA稳定性中发挥作用。随后的Northern分析表明,外切体突变体积累了一种3'端延长的转录本,而成熟的CTH2 mRNA减少。CTH2 mRNA的3'端定位于一个GU(3 - 5)重复序列,这与任何先前鉴定的聚腺苷酸化位点不同。3'切割和聚腺苷酸化因子Rna14、Rna15和Pap1的突变可阻断其他mRNA的积累,但不抑制CTH2 mRNA的积累。3'端延长的CTH2前体mRNA在TRAMP4聚腺苷酸化复合体或Nrd1/Nab3/Sen1复合体发生突变的菌株中强烈积累,并且包含多个Nrd1和Nab3结合位点。CTH2带有一个共有ARE元件,前体mRNA和mRNA的水平通过ARE的突变或核5'外切核酸酶Rat1的失活而升高。我们提出,CTH2 mRNA是由外切体、TRAMP和Nrd1/Nab3/Sen1复合体从3'端延长的初级转录本加工而来的。这种不寻常的途径可能为涉及Rat1的核内、ARE介导的CTH2水平调控留出时间。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cc85/2396412/31a592c01ef8/gkn160f1.jpg

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