Literature DB >> 33238149

Global and Site-Specific Effect of Phosphorylation on Protein Turnover.

Chongde Wu1, Qian Ba1, Dayun Lu2, Wenxue Li1, Barbora Salovska3, Pingfu Hou1, Torsten Mueller4, George Rosenberger5, Erli Gao1, Yi Di1, Hu Zhou2, Eugenio F Fornasiero6, Yansheng Liu7.   

Abstract

To date, the effects of specific modification types and sites on protein lifetime have not been systematically illustrated. Here, we describe a proteomic method, DeltaSILAC, to quantitatively assess the impact of site-specific phosphorylation on the turnover of thousands of proteins in live cells. Based on the accurate and reproducible mass spectrometry-based method, a pulse labeling approach using stable isotope-labeled amino acids in cells (pSILAC), phosphoproteomics, and a unique peptide-level matching strategy, our DeltaSILAC profiling revealed a global, unexpected delaying effect of many phosphosites on protein turnover. We further found that phosphorylated sites accelerating protein turnover are functionally selected for cell fitness, enriched in Cyclin-dependent kinase substrates, and evolutionarily conserved, whereas the glutamic acids surrounding phosphosites significantly delay protein turnover. Our method represents a generalizable approach and provides a rich resource for prioritizing the effects of phosphorylation sites on protein lifetime in the context of cell signaling and disease biology.
Copyright © 2020 Elsevier Inc. All rights reserved.

Entities:  

Keywords:  DeltaSILAC; data-independent acquisition; mass spectrometry; phosphomodiform; phosphorylation; protein lifetime; protein turnover; proteomics; pulse SILAC

Mesh:

Substances:

Year:  2020        PMID: 33238149      PMCID: PMC7855865          DOI: 10.1016/j.devcel.2020.10.025

Source DB:  PubMed          Journal:  Dev Cell        ISSN: 1534-5807            Impact factor:   12.270


  74 in total

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5.  Assessing the Relationship Between Mass Window Width and Retention Time Scheduling on Protein Coverage for Data-Independent Acquisition.

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2.  A peptidoform based proteomic strategy for studying functions of post-translational modifications.

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Journal:  Proteomics       Date:  2021-12-23       Impact factor: 3.984

3.  Linking post-translational modifications and protein turnover by site-resolved protein turnover profiling.

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4.  A novel protein encoded by ZCRB1-induced circHEATR5B suppresses aerobic glycolysis of GBM through phosphorylation of JMJD5.

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5.  Proteotype coevolution and quantitative diversity across 11 mammalian species.

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  9 in total

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