4.5 Article

Toward a hypothesis-free understanding of how phosphorylation dynamically impacts protein turnover

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PROTEOMICS
卷 23, 期 3-4, 页码 -

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WILEY
DOI: 10.1002/pmic.202100387

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clustering; data analysis; DeltaSILAC; DIA-MS; peptidoform; phosphorylation; protein turnover; pulse SILAC; time course

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Recent studies have integrated post-translational modifications (PTMs) measurement with protein turnover exploration in steady state systems. However, the biological interpretation of these complex datasets remains unclear.
The turnover measurement of proteins and proteoforms has been largely facilitated by workflows coupling metabolic labeling with mass spectrometry (MS), including dynamic stable isotope labeling by amino acids in cell culture (dynamic SILAC) or pulsed SILAC (pSILAC). Very recent studies including ours have integrated themeasurement of post-translational modifications (PTMs) at the proteome level (i.e., phosphoproteomics) with pSILAC experiments in steady state systems, exploring the link between PTMs and turnover at the proteome-scale. An open question in the field is how to exactly interpret these complex datasets in a biological perspective. Here, we present a novel pSILAC phosphoproteomic dataset which was obtained during a dynamic process of cell starvation using data-independent acquisition MS (DIA-MS). To provide an unbiased hypothesis-free analysis framework, we developed a strategy to interrogate how phosphorylation dynamically impacts protein turnover across the time series data. With this strategy, we discovered a complex relationship between phosphorylation and protein turnover that was previously underexplored. Our results further revealed a link between phosphorylation stoichiometry with the turnover of phosphorylated peptidoforms. Moreover, our results suggested that phosphoproteomic turnover diversity cannot directly explain the abundance regulation of phosphorylation during cell starvation, underscoring the importance of future studies addressing PTM site-resolved protein turnover.

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