Literature DB >> 30146318

Single Live Cell Monitoring of Protein Turnover Reveals Intercellular Variability and Cell-Cycle Dependence of Degradation Rates.

Andrea Brigitta Alber1, Eric Raphael Paquet1, Martina Biserni1, Felix Naef1, David Michael Suter2.   

Abstract

Cells need to reliably control their proteome composition to maintain homeostasis and regulate growth. How protein synthesis and degradation interplay to control protein expression levels remains unclear. Here, we combined a tandem fluorescent timer and pulse-chase protein labeling to disentangle how protein synthesis and degradation control protein homeostasis in single live mouse embryonic stem cells. We discovered substantial cell-cycle dependence in protein synthesis rates and stabilization of a large number of proteins around cytokinesis. Protein degradation rates were highly variable between cells, co-varied within individual cells for different proteins, and were positively correlated with synthesis rates. This suggests variability in proteasome activity as an important source of global extrinsic noise in gene expression. Our approach paves the way toward understanding the complex interplay of synthesis and degradation processes in determining protein levels of individual mammalian cells.
Copyright © 2018 Elsevier Inc. All rights reserved.

Entities:  

Keywords:  fluorescence microscopy; live-cell imaging; mathematical modeling; protein degradation; protein synthesis; single cells; tandem fluorescent timer

Mesh:

Substances:

Year:  2018        PMID: 30146318     DOI: 10.1016/j.molcel.2018.07.023

Source DB:  PubMed          Journal:  Mol Cell        ISSN: 1097-2765            Impact factor:   17.970


  17 in total

Review 1.  Dynamics of protein synthesis and degradation through the cell cycle.

Authors:  Andrea Brigitta Alber; David Michael Suter
Journal:  Cell Cycle       Date:  2019-03-30       Impact factor: 4.534

2.  Tandem Fluorescent Protein Timers for Noninvasive Relative Protein Lifetime Measurement in Plants.

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3.  Indirect Methods To Measure Unfolded Proteins In Living Cells Using Fluorescent Proteins.

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Journal:  Methods Mol Biol       Date:  2022

4.  High-Throughput Analysis of Protein Turnover with Tandem Fluorescent Protein Timers.

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Journal:  Methods Mol Biol       Date:  2022

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Review 6.  In vivo assay and modelling of protein and mitochondrial turnover during aging.

Authors:  Hans S Bell; John Tower
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7.  CALM supports clathrin-coated vesicle completion upon membrane tension increase.

Authors:  Nathan M Willy; Federico Colombo; Scott Huber; Anna C Smith; Erienne G Norton; Comert Kural; Emanuele Cocucci
Journal:  Proc Natl Acad Sci U S A       Date:  2021-06-22       Impact factor: 11.205

8.  Live-cell imaging of circadian clock protein dynamics in CRISPR-generated knock-in cells.

Authors:  Christian H Gabriel; Marta Del Olmo; Amin Zehtabian; Marten Jäger; Silke Reischl; Hannah van Dijk; Carolin Ulbricht; Asylkhan Rakhymzhan; Thomas Korte; Barbara Koller; Astrid Grudziecki; Bert Maier; Andreas Herrmann; Raluca Niesner; Tomasz Zemojtel; Helge Ewers; Adrián E Granada; Hanspeter Herzel; Achim Kramer
Journal:  Nat Commun       Date:  2021-06-18       Impact factor: 14.919

9.  Site-Specific Protein Labeling with Fluorophores as a Tool To Monitor Protein Turnover.

Authors:  Yonatan G Mideksa; Maximilian Fottner; Sebastian Braus; Caroline A M Weiß; Tuan-Anh Nguyen; Susanne Meier; Kathrin Lang; Matthias J Feige
Journal:  Chembiochem       Date:  2020-03-09       Impact factor: 3.164

10.  Mitotic chromosome binding predicts transcription factor properties in interphase.

Authors:  Mahé Raccaud; Elias T Friman; Andrea B Alber; Harsha Agarwal; Cédric Deluz; Timo Kuhn; J Christof M Gebhardt; David M Suter
Journal:  Nat Commun       Date:  2019-01-30       Impact factor: 14.919

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