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Nucleoside modifications in the regulation of gene expression: focus on tRNA

期刊

CELLULAR AND MOLECULAR LIFE SCIENCES
卷 73, 期 16, 页码 3075-3095

出版社

SPRINGER BASEL AG
DOI: 10.1007/s00018-016-2217-y

关键词

Regulation of gene expression; Modified nucleosides; Stress signaling; tRNA; Translation rate

资金

  1. National Science Centre in Poland [UMO-2011/03/B/ST5/02669, 2014/13/B/ST5/03979]
  2. Centre of Molecular and Macromolecular Studies of the Polish Academy of Sciences
  3. Lodz University of Technology, Poland

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Both, DNA and RNA nucleoside modifications contribute to the complex multi-level regulation of gene expression. Modified bases in tRNAs modulate protein translation rates in a highly dynamic manner. Synonymous codons, which differ by the third nucleoside in the triplet but code for the same amino acid, may be utilized at different rates according to codon-anticodon affinity. Nucleoside modifications in the tRNA anticodon loop can favor the interaction with selected codons by stabilizing specific base pairs. Similarly, weakening of base pairing can discriminate against binding to near-cognate codons. mRNAs enriched in favored codons are translated in higher rates constituting a fine-tuning mechanism for protein synthesis. This so-called codon bias establishes a basic protein level, but sometimes it is necessary to further adjust the production rate of a particular protein to actual requirements, brought by, e.g., stages in circadian rhythms, cell cycle progression or exposure to stress. Such an adjustment is realized by the dynamic change of tRNA modifications resulting in the preferential translation of mRNAs coding for example for stress proteins to facilitate cell survival. Furthermore, tRNAs contribute in an entirely different way to another, less specific stress response consisting in modification-dependent tRNA cleavage that contributes to the general down-regulation of protein synthesis. In this review, we summarize control functions of nucleoside modifications in gene regulation with a focus on recent findings on protein synthesis control by tRNA base modifications.

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