Literature DB >> 25593288

Modeling the contribution of individual proteins to mixed skeletal muscle protein synthetic rates over increasing periods of label incorporation.

Benjamin F Miller1, Christopher A Wolff2, Fredrick F Peelor2, Patrick D Shipman3, Karyn L Hamilton2.   

Abstract

Advances in stable isotope approaches, primarily the use of deuterium oxide ((2)H2O), allow for long-term measurements of protein synthesis, as well as the contribution of individual proteins to tissue measured protein synthesis rates. Here, we determined the influence of individual protein synthetic rates, individual protein content, and time of isotopic labeling on the measured synthesis rate of skeletal muscle proteins. To this end, we developed a mathematical model, applied the model to an established data set collected in vivo, and, to experimentally test the impact of different isotopic labeling periods, used (2)H2O to measure protein synthesis in cultured myotubes over periods of 2, 4, and 7 days. We first demonstrated the influence of both relative protein content and individual protein synthesis rates on measured synthesis rates over time. When expanded to include 286 individual proteins, the model closely approximated protein synthetic rates measured in vivo. The model revealed a 29% difference in measured synthesis rates from the slowest period of measurement (20 min) to the longest period of measurement (6 wk). In support of these findings, culturing of C2C12 myotubes with isotopic labeling periods of 2, 4, or 7 days revealed up to a doubling of the measured synthesis rate in the shorter labeling period compared with the longer period of labeling. From our model, we conclude that a 4-wk period of labeling is ideal for considering all proteins in a mixed-tissue fraction, while minimizing the slowing effect of fully turned-over proteins. In addition, we advocate that careful consideration must be paid to the period of isotopic labeling when comparing mixed protein synthetic rates between studies.
Copyright © 2015 the American Physiological Society.

Entities:  

Keywords:  deuterium oxide; modeling; protein synthesis; stable isotope

Mesh:

Substances:

Year:  2015        PMID: 25593288      PMCID: PMC4360018          DOI: 10.1152/japplphysiol.00987.2014

Source DB:  PubMed          Journal:  J Appl Physiol (1985)        ISSN: 0161-7567


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Journal:  J Physiol       Date:  2005-07-07       Impact factor: 5.182

4.  Comparison of constant infusion and flooding dose techniques to measure muscle protein synthesis rate in dogs.

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6.  Measurement in vivo of proliferation rates of slow turnover cells by 2H2O labeling of the deoxyribose moiety of DNA.

Authors:  R A Neese; L M Misell; S Turner; A Chu; J Kim; D Cesar; R Hoh; F Antelo; A Strawford; J M McCune; M Christiansen; M K Hellerstein
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Authors:  Benjamin F Miller; Joshua C Drake; Bradley Naylor; John C Price; Karyn L Hamilton
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2.  Vitamin supplementation and resistance exercise-induced muscle hypertrophy: shifting the redox balance scale?

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Review 4.  Mitochondrial proteostasis as a shared characteristic of slowed aging: the importance of considering cell proliferation.

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5.  Dietary Methionine Restriction Regulates Liver Protein Synthesis and Gene Expression Independently of Eukaryotic Initiation Factor 2 Phosphorylation in Mice.

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6.  Long-term rates of mitochondrial protein synthesis are increased in mouse skeletal muscle with high-fat feeding regardless of insulin-sensitizing treatment.

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7.  Oxidative stress mediates ethanol-induced skeletal muscle mitochondrial dysfunction and dysregulated protein synthesis and autophagy.

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Review 10.  Mechanisms of protein balance in skeletal muscle.

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