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非洲爪蟾内含子编码的U16小核仁RNA加工的体外研究。

In vitro study of processing of the intron-encoded U16 small nucleolar RNA in Xenopus laevis.

作者信息

Caffarelli E, Arese M, Santoro B, Fragapane P, Bozzoni I

机构信息

Centro Acidi Nucleici, Consiglio Nazionale delle Ricerche, Rome, Italy.

出版信息

Mol Cell Biol. 1994 May;14(5):2966-74. doi: 10.1128/mcb.14.5.2966-2974.1994.

Abstract

It was recently shown that a new class of small nuclear RNAs is encoded in introns of protein-coding genes and that they originate by processing of the pre-mRNA in which they are contained. Little is known about the mechanism and the factors involved in this new type of processing. The L1 ribosomal protein gene of Xenopus laevis is a well-suited system for studying this phenomenon: several different introns encode for two small nucleolar RNAs (snoRNAs; U16 and U18). In this paper, we analyzed the in vitro processing of these snoRNAs and showed that both are released from the pre-mRNA by a common mechanism: endonucleolytic cleavages convert the pre-mRNA into a precursor snoRNA with 5' and 3' trailer sequences. Subsequently, trimming converts the pre-snoRNAs into mature molecules. Oocyte and HeLa nuclear extracts are able to process X. laevis and human substrates in a similar manner, indicating that the processing of this class of snoRNAs relies on a common and evolutionarily conserved mechanism. In addition, we found that the cleavage activity is strongly enhanced in the presence of Mn2+ ions.

摘要

最近的研究表明,一类新的小核RNA编码于蛋白质编码基因的内含子中,且它们是通过对其所包含的前体mRNA进行加工而产生的。对于这种新型加工过程所涉及的机制和因素,我们知之甚少。非洲爪蟾的L1核糖体蛋白基因是研究这一现象的理想系统:几个不同的内含子编码两种小核仁RNA(snoRNA;U16和U18)。在本文中,我们分析了这些snoRNA的体外加工过程,并表明两者都是通过一种共同机制从前体mRNA中释放出来的:内切核酸酶切割将前体mRNA转化为带有5'和3'拖尾序列的前体snoRNA。随后,修剪将前体snoRNA转化为成熟分子。卵母细胞和HeLa细胞核提取物能够以类似的方式加工非洲爪蟾和人类的底物,这表明这类snoRNA的加工依赖于一种共同且进化保守的机制。此外,我们发现,在Mn2+离子存在的情况下,切割活性会显著增强。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f7de/358664/65a6f66417d0/molcellb00005-0140-a.jpg

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