2012
DOI: 10.1074/mcp.o112.022186
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Proteome Dynamics: Revisiting Turnover with a Global Perspective

Abstract: Although bulk protein turnover has been measured with the use of stable isotope labeled tracers for over half a century, it is only recently that the same approach has become applicable to the level of the proteome, permitting analysis of the turnover of many proteins instead of single proteins or an aggregated protein pool. The optimal experimental design for turnover studies is dependent on the nature of the biological system under study, which dictates the choice of precursor label, protein pool sampling st… Show more

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Cited by 115 publications
(169 citation statements)
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“…Protein synthesis is a zero order process and is thus described as a proportional increase of its starting pool (K S /A) per day (Claydon and Beynon, 2012;Li et al, 2012). "A" is the starting abundance for a specific protein at the beginning of the labeling period (T0).…”
Section: Calculation Of K D and K Smentioning
confidence: 99%
“…Protein synthesis is a zero order process and is thus described as a proportional increase of its starting pool (K S /A) per day (Claydon and Beynon, 2012;Li et al, 2012). "A" is the starting abundance for a specific protein at the beginning of the labeling period (T0).…”
Section: Calculation Of K D and K Smentioning
confidence: 99%
“…Malfunctions of protein turnover are increasingly recognized in numerous human disorders, including cystic fibrosis, neurodegenerative diseases, and heart diseases (1, 2). In the normal heart, protein turnover helps maintain the protein pool in homeostasis through continual synthesis and degradation (2,3). The turnover cycle becomes perturbed during cardiac injury and heart failure by factors including hypertrophic signaling (4), calcium regulation (5), and proteolytic stress (6,7), whereas increased oxidative stress compounds the reduced protein degradation capacity of the failing heart (8).…”
Section: Introductionmentioning
confidence: 99%
“…Although disrupted protein homeostasis is a hallmark of the remodeling heart, the technologies to quantify its effects on protein turnover have been lacking until very recently. Quantitative evaluations of protein synthesis and degradation have been well demonstrated in cultured cells using techniques such as stable isotope-labeled amino acid (SILAC) or fluorescence timers (14,15), but the proteome dynamics of freely dividing cells in vitro does not necessarily recapitulate the physical constraints and physiological regulations that occur in animals in vivo (3,16). Measuring protein turnover in vivo entails additional technical challenges including label delivery and tolerance, determination of precursor enrichment, and data interpretation (3,12,16).…”
Section: Introductionmentioning
confidence: 99%
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