Measurement of protein synthesis using heavy water labeling and peptide mass spectrometry: Discrimination between major histocompatibility complex allotypes

Riva, Alessandra; Deery, Michael J.; McDonald, Sarah; Lund, Torben; Busch, Robert

doi:10.1016/j.ab.2010.04.018

Cited by 38 publications

(71 citation statements)

References 35 publications

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“…To determine the extent to which the precursor proteogenic amino acid pool is labeled, after an intraperitoneal injection of 2 H 2 O, 2 H labeling of hepatic free amino acids at various time points was assessed by GC-MS (Table I) (12,15,17), alanine, glutamate, glutamine, glycine, and serine were extensively labeled, reflecting their central role in intermediary metabolism. Small, in some cases negligible, amounts of 2 H label were found in most essential amino acids.…”

Section: Animal Experimentsmentioning

confidence: 99%

“…Recently the global metabolic labeling of the entire proteome was achieved using 15 N-labeled medium and diet for cell culture and animal studies, respectively (9,10). Although these techniques allow estimation of global proteome dynamics without the requirement of precursor isotope abundance, these approaches require a long term time course experiment for exponential fitting.…”

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confidence: 99%

“…Although these techniques allow estimation of global proteome dynamics without the requirement of precursor isotope abundance, these approaches require a long term time course experiment for exponential fitting. In addition, these techniques are not suited for human studies because they require the consumption of a fully 15 N-labeled diet. Recently we and others developed the 2 H 2 O metabolic labeling technique to measure protein turnover in free living animals (11)(12)(13)(14)(15).…”

mentioning

confidence: 99%

“…In addition, these techniques are not suited for human studies because they require the consumption of a fully 15 N-labeled diet. Recently we and others developed the 2 H 2 O metabolic labeling technique to measure protein turnover in free living animals (11)(12)(13)(14)(15). In rats that have been given intraperitoneal injection of 2 H 2 O, 2 H equilibrates with total body water and amino acids such as alanine within 10 and 20 min, respectively (16) (Fig.…”

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confidence: 99%

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Plasma Proteome Dynamics: Analysis of Lipoproteins and Acute Phase Response Proteins with 2H2O Metabolic Labeling

Willard

Rachdaoui

et al. 2012

Molecular & Cellular Proteomics

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Understanding the pathologies related to the regulation of protein metabolism requires methods for studying the kinetics of individual proteins. We developed a 2 H 2 O metabolic labeling technique and software for protein kinetic studies in free living organisms. This approach for proteome dynamic studies requires the measurement of total body water enrichments by GC-MS, isotopic distribution of the tryptic peptide by LC-MS/MS, and estimation of the asymptotical number of deuterium incorporated into a peptide by software. We applied this technique to measure the synthesis rates of several plasma lipoproteins and acute phase response proteins in rats. Samples were collected at different time points, and proteins were separated by a gradient gel electrophoresis.2 H labeling of tryptic peptides was analyzed by ion trap tandem mass spectrometry (LTQ MS/MS) for measurement of the fractional synthesis rates of plasma proteins. The high sensitivity of LTQ MS in zoom scan mode in combination with 2 H label amplification in proteolytic peptides allows detection of the changes in plasma protein synthesis related to animal nutritional status. Our results demonstrate that fasting has divergent effects on the rate of synthesis of plasma proteins, increasing synthesis of ApoB 100 but decreasing formation of albumin and fibrinogen. We conclude that this technique can effectively measure the synthesis of plasma proteins and can be used to study the regulation of protein homeostasis under physiological and pathological conditions.

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Section: Animal Experimentsmentioning

confidence: 99%

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confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Plasma Proteome Dynamics: Analysis of Lipoproteins and Acute Phase Response Proteins with 2H2O Metabolic Labeling

Willard

Rachdaoui

et al. 2012

Molecular & Cellular Proteomics

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“…Isotope tracers are particularly useful for tracking such continual renewal of the proteome in living systems, because they allow differentiation between preexisting and newly synthesized proteins (5 (11)(12)(13)(14) and peptide analysis in MALDI-TOF MS (15) and LC-MS (16,17). More recently, Price et al described an approach for measuring protein turnover by calculating the theoretical number of 2 H-labeling sites on a peptide sequence (18) and reported the turnover rates of ϳ100 human plasma proteins.…”

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Metabolic Labeling Reveals Proteome Dynamics of Mouse Mitochondria

Kim

Wang

Kim

et al. 2012

Molecular & Cellular Proteomics

161

187

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Mitochondrial dysfunction is associated with many human diseases. Mitochondrial damage is exacerbated by inadequate protein quality control and often further contributes to pathogenesis. The maintenance of mitochondrial functions requires a delicate balance of continuous protein synthesis and degradation, i.e. protein turnover. To understand mitochondrial protein dynamics in vivo, we designed a metabolic heavy water ( 2 H 2 O) labeling strategy customized to examine individual protein turnover in the mitochondria in a systematic fashion. Mice were fed with 2 H 2 O at a minimal level (<5% body water) without physiological impacts. Mitochondrial proteins were analyzed from 9 mice at each of the 13 time points between 0 and 90 days (d) of labeling. A novel multiparameter fitting approach computationally determined the normalized peak areas of peptide mass isotopomers at initial and steady-state time points and permitted the protein halflife to be determined without plateau-level 2 H incorporation. We characterized the turnover rates of 458 proteins in mouse cardiac and hepatic mitochondria and found median turnover rates of 0.0402 d ؊1 and 0.163 d ؊1 , respectively, corresponding to median half-lives of 17.2 d and 4.26 d. Mitochondria in the heart and those in the liver exhibited distinct turnover kinetics, with limited synchronization within functional clusters. We observed considerable interprotein differences in turnover rates in both organs, with half-lives spanning from hours to months (ϳ60 d). Our proteomics platform demonstrates the first large-scale analysis of mitochondrial protein turnover rates in vivo, with potential applications in translational research. Molecular & Cellular

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Current literature in mass spectrometry

2010

J. Mass Spectrom.

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Measurement of protein synthesis using heavy water labeling and peptide mass spectrometry: Discrimination between major histocompatibility complex allotypes

Cited by 38 publications

References 35 publications

Plasma Proteome Dynamics: Analysis of Lipoproteins and Acute Phase Response Proteins with 2H2O Metabolic Labeling

Plasma Proteome Dynamics: Analysis of Lipoproteins and Acute Phase Response Proteins with 2H2O Metabolic Labeling

Metabolic Labeling Reveals Proteome Dynamics of Mouse Mitochondria

Current literature in mass spectrometry

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