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Unpaired terminal nucleotides and 5′ monophosphorylation govern 3′ polyadenylation by Escherichia coli poly(A) polymerase I

机译:未配对的末端核苷酸和5单磷酸化控制大肠杆菌poly(A)聚合酶I的3聚腺苷酸化

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摘要

In bacteria, most mRNAs and certain regulatory RNAs are rapidly turned over, whereas mature tRNA and ribosomal RNA are highly stable. The selective susceptibility of unstable Escherichia coli RNAs to 3′ polyadenylation by the pcnB gene product, poly(A) polymerase I (PAP I), in vivo is a key factor in their rapid degradation by 3′ to 5′ exonucleases. Using highly purified His-tagged recombinant PAP I, we show that differential adenylation of RNA substrates by PAP I occurs in vitro and that this capability resides in PAP I itself rather than in any ancillary protein(s). Surprisingly, the efficiency of 3′ polyadenylation is affected by substrate structure at both termini; single-strand segments at either the 5′ or 3′ end of RNA molecules and monophosphorylation at an unpaired 5′ terminus dramatically increase the rate and length of 3′ poly(A) tail additions by PAP I. Our results provide a mechanistic basis for the susceptibility of certain RNAs to 3′ polyadenylation. They also suggest a model of “programmed” RNA decay in which endonucleolytically generated RNA fragments containing single-stranded monophosphorylated 5′ termini are targeted for poly(A) addition and further degradation.
机译:在细菌中,大多数mRNA和某些调节性RNA都可以快速翻转,而成熟的tRNA和核糖体RNA则高度稳定。 pcnB基因产物poly(A)聚合酶I(PAP I)在体内对不稳定的大肠杆菌RNAs对3'聚腺苷酸的选择性敏感性是其在3'至5'核酸外切酶中快速降解的关键因素。使用高度纯化的带有His标签的重组PAP I,我们显示了PAP I在RNA底物上的差异腺苷酸作用在体外发生,并且这种能力存在于PAP I本身,而不是存在于任何辅助蛋白中。令人惊讶的是,3'聚腺苷酸化的效率受两个末端底物结构的影响。 RNA分子5'或3'末端的单链区段和未配对的5'末端的单磷酸化显着提高了PAP I添加3'聚(A)尾巴的速率和长度。我们的结果为某些RNA对3'聚腺苷酸化的敏感性。他们还提出了“程序化” RNA衰变模型,其中包含单链单磷酸化5'末端的核酸内切法产生的RNA片段被靶向添加poly(A)和进一步降解。

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