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人类真核生物起始因子的磷酸化化学计量学

Phosphorylation stoichiometries of human eukaryotic initiation factors.

作者信息

Andaya Armann, Villa Nancy, Jia Weitao, Fraser Christopher S, Leary Julie A

机构信息

Department of Molecular and Cellular Biology, University of California at Davis, Davis, CA 95616, USA.

出版信息

Int J Mol Sci. 2014 Jun 27;15(7):11523-38. doi: 10.3390/ijms150711523.

Abstract

Eukaryotic translation initiation factors are the principal molecular effectors regulating the process converting nucleic acid to functional protein. Commonly referred to as eIFs (eukaryotic initiation factors), this suite of proteins is comprised of at least 25 individual subunits that function in a coordinated, regulated, manner during mRNA translation. Multiple facets of eIF regulation have yet to be elucidated; however, many of the necessary protein factors are phosphorylated. Herein, we have isolated, identified and quantified phosphosites from eIF2, eIF3, and eIF4G generated from log phase grown HeLa cell lysates. Our investigation is the first study to globally quantify eIF phosphosites and illustrates differences in abundance of phosphorylation between the residues of each factor. Thus, identification of those phosphosites that exhibit either high or low levels of phosphorylation under log phase growing conditions may aid researchers to concentrate their investigative efforts to specific phosphosites that potentially harbor important regulatory mechanisms germane to mRNA translation.

摘要

真核生物翻译起始因子是调节核酸转化为功能性蛋白质这一过程的主要分子效应物。这一组蛋白质通常被称为eIFs(真核生物起始因子),由至少25个单独的亚基组成,在mRNA翻译过程中以协调、受调控的方式发挥作用。eIF调节的多个方面尚未阐明;然而,许多必需的蛋白质因子会被磷酸化。在此,我们从对数期生长的HeLa细胞裂解物中分离、鉴定并定量了eIF2、eIF3和eIF4G的磷酸化位点。我们的研究是首次对eIF磷酸化位点进行全面定量的研究,并阐明了每个因子残基之间磷酸化丰度的差异。因此,鉴定在对数期生长条件下表现出高磷酸化或低磷酸化水平的那些磷酸化位点,可能有助于研究人员将其研究工作集中于可能具有与mRNA翻译相关的重要调控机制的特定磷酸化位点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d4b6/4139797/a0b484e36bda/ijms-15-11523-g001.jpg

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