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. 2025 May 1;188(9):2433-2450.e21.
doi: 10.1016/j.cell.2025.03.002. Epub 2025 Mar 31.

Global analysis of protein turnover dynamics in single cells

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Free article

Global analysis of protein turnover dynamics in single cells

Pierre Sabatier et al. Cell. .
Free article

Abstract

Single-cell proteomics (SCPs) has advanced significantly, yet it remains largely unidimensional, focusing primarily on protein abundances. In this study, we employed a pulsed stable isotope labeling by amino acids in cell culture (pSILAC) approach to simultaneously analyze protein abundance and turnover in single cells (SC-pSILAC). Using a state-of-the-art SCP workflow, we demonstrated that two SILAC labels are detectable from ∼4,000 proteins in single HeLa cells recapitulating known biology. We performed a large-scale time-series SC-pSILAC analysis of undirected differentiation of human induced pluripotent stem cells (iPSCs) encompassing 6 sampling times over 2 months and analyzed >1,000 cells. Protein turnover dynamics highlighted differentiation-specific co-regulation of protein complexes with core histone turnover, discriminating dividing and non-dividing cells. Lastly, correlating cell diameter with the abundance of individual proteins showed that histones and some cell-cycle proteins do not scale with cell size. The SC-pSILAC method provides a multidimensional view of protein dynamics in single-cell biology.

Keywords: Chip-Tip; Evosep; Orbitrap Astral; cellenONE; histone; iPSC differentiation; mass spectrometry; protein turnover; pulsed SILAC; single-cell proteomics.

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Conflict of interest statement

Declaration of interests F.I. and A.S. are employees of Cellenion SASU.

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