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

机译:编码酵母ARE结合蛋白Cth2的mRNA通过新颖的3加工途径产生

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摘要

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 [GU3–5]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.
机译:对缺乏核外泌体成分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,该转录本在细胞质mRNA稳定性中起作用。随后的Northern分析显示,外泌体突变体以成熟的CTH2 mRNA为代价积累了3'延伸的转录本。 CTH2 mRNA的3'端定位于[GU3-5] 5重复序列,这与以前表征的多聚腺苷酸化位点不同。 CTH2 mRNA的积累不受3'裂解和多腺苷酸化因子Rna14,Rna15和Pap1突变的抑制,这些突变阻断了其他mRNA的积累。 3'延伸的CTH2 pre-mRNA在TRAMP4聚腺苷酸复合物或Nrd1 / Nab3 / Sen1复合物中具有突变的菌株中强烈积累,并包含多个Nrd1和Nab3结合位点。 CTH2携带一个共有的ARE元件,并且通过ARE突变或5'核酸外切酶Rat1的失活提高了前mRNA和mRNA的水平。我们建议,CTH2 mRNA是由外来体,TRAMP和Nrd1 / Nab3 / Sen1复合体从3'延伸的初级转录本加工而成。这种不寻常的途径可能会为涉及Rat1的CTH2水平的核,ARE介导调控提供时间。

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