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核糖体蛋白S20的mRNA部分对依赖于寡聚腺苷酸化和RNA二级结构的3'-核酸外切酶的差异敏感性。

Differential sensitivities of portions of the mRNA for ribosomal protein S20 to 3'-exonucleases dependent on oligoadenylation and RNA secondary structure.

作者信息

Coburn G A, Mackie G A

机构信息

Department of Biochemistry and Molecular Biology, University of British Columbia, Vancouver, British Columbia, Canada V6T 1Z3.

出版信息

J Biol Chem. 1996 Jun 28;271(26):15776-81. doi: 10.1074/jbc.271.26.15776.

Abstract

The 3'-exonucleolytic decay of the mRNA for ribosomal protein S20 has been reconstituted in vitro using purified RNase II and crude extracts enriched for polynucleotide phosphorylase (PNPase) activity. We show that RNase II can catalyze the degradation of the 5' two-thirds of the S20 mRNA and that prior oligoadenylation of the 3' termini of truncated S20 mRNA substrates can significantly stimulate the initiation of degradation by RNase II. The intact S20 mRNA is, however, insensitive to attack by RNase II and polyadenylation of its 3'-end cannot overcome the natural resistance of the S20 mRNA to RNase II. Complete degradation of either the entire S20 mRNA without prior endonucleolytic cleavage or the 3'-terminal 147-residue fragment is dependent on both oligoadenylation and PNPase activity. Moreover, this process can take place in the absence of RNase E activity. Our data point to the importance of oligoadenylation in facilitating 3'-exonucleolytic activity and indicate that there are alternative degradative pathways. The implications for mRNA decay are discussed.

摘要

利用纯化的核糖核酸酶II(RNase II)和富含多核苷酸磷酸化酶(PNPase)活性的粗提物,在体外重建了核糖体蛋白S20的信使核糖核酸(mRNA)的3'外切核酸酶降解过程。我们发现,RNase II能够催化S20 mRNA 5'端三分之二的降解,并且截断后的S20 mRNA底物3'末端的寡聚腺苷酸化能够显著刺激RNase II引发降解。然而,完整的S20 mRNA对RNase II的攻击不敏感,其3'端的多聚腺苷酸化也无法克服S20 mRNA对RNase II的天然抗性。无论是未经内切核酸酶切割的完整S20 mRNA,还是3'末端147个残基的片段,其完全降解都依赖于寡聚腺苷酸化和PNPase活性。此外,这一过程可以在没有RNase E活性的情况下发生。我们的数据表明寡聚腺苷酸化在促进3'外切核酸酶活性方面的重要性,并表明存在其他降解途径。文中还讨论了这些结果对mRNA降解的意义。

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