Your search keyword '"Alexandria K. Sahu"' showing total 14 results

1. A framework for installable external tools in Skyline.

Author

Daniel Broudy, Trevor Killeen, Meena Choi, Nicholas Shulman, Deepak R. Mani, Susan E. Abbatiello, Deepak Mani, Rushdy Ahmad, Alexandria K. Sahu, Birgit Schilling, Kaipo Tamura, Yuval Boss, Vagisha Sharma, Bradford W. Gibson, Steven A. Carr, Olga Vitek, Michael J. MacCoss, and Brendan MacLean

Published

2014

2. Protein acetylation dynamics in response to carbon overflow inEscherichia coli

Author

Bozena Zemaitaitis, Linda I. Hu, Alexandria K. Sahu, Arti Walker-Peddakotla, Bradford W. Gibson, Robert Davis, Dylan J. Sorensen, David G. Christensen, Alan J. Wolfe, and Birgit Schilling

Subjects

chemistry.chemical_classification, Lysine, Metabolism, Biology, Proteomics, medicine.disease_cause, Microbiology, Metabolic pathway, Enzyme, Biochemistry, chemistry, Acetylation, medicine, Post-translational regulation, Molecular Biology, Escherichia coli

Abstract

In Escherichia coli, acetylation of proteins at lysines depends largely on a non-enzymatic acetyl phosphate-dependent mechanism. To assess the functional significance of this post-translational modification, we first grew wild-type cells in buffered tryptone broth with glucose and monitored acetylation over time by immunochemistry. Most acetylation occurred in stationary phase and paralleled glucose consumption and acetate excretion, which began upon entry into stationary phase. Transcription of rprA, a stationary phase regulator, exhibited similar behavior. To identify sites and substrates with significant acetylation changes, we used label-free, quantitative proteomics to monitor changes in protein acetylation. During growth, both the number of identified sites and the extent of acetylation increased with considerable variation among lysines from the same protein. As glucose-regulated lysine acetylation was predominant in central metabolic pathways and overlapped with acetyl phosphate-regulated acetylation sites, we deleted the major carbon regulator CRP and observed a dramatic loss of acetylation that could be restored by deleting the enzyme that degrades acetyl phosphate. We propose that acetyl phosphate-dependent acetylation is a response to carbon flux that could regulate central metabolism.

Published

2015

3. MS1 Peptide Ion Intensity Chromatograms in MS2 (SWATH) Data Independent Acquisitions. Improving Post Acquisition Analysis of Proteomic Experiments

Author

Olga Vitek, Alexandria K. Sahu, Matthew J. Rardin, Brendan MacLean, Dylan J. Sorensen, Bradford W. Gibson, Lin-Yang Cheng, Michael J. MacCoss, and Birgit Schilling

Subjects

Special Issue Articles, Proteomics, Analyte, Instrumentation, Medizin, Analytical chemistry, Biochemistry, Analytical Chemistry, Ion, Mice, Software, Animals, Protein Kinase Inhibitors, Molecular Biology, Chemistry, Fragment (computer graphics), business.industry, Reproducibility of Results, Dual Scan, High-Throughput Screening Assays, Intensity (physics), Liver, Peptides, Biological system, business, Quantitative analysis (chemistry)

Abstract

Quantitative analysis of discovery-based proteomic workflows now relies on high-throughput large-scale methods for identification and quantitation of proteins and post-translational modifications. Advancements in label-free quantitative techniques, using either data-dependent or data-independent mass spectrometric acquisitions, have coincided with improved instrumentation featuring greater precision, increased mass accuracy, and faster scan speeds. We recently reported on a new quantitative method called MS1 Filtering (Schilling et al. (2012) Mol. Cell. Proteomics 11, 202-214) for processing data-independent MS1 ion intensity chromatograms from peptide analytes using the Skyline software platform. In contrast, data-independent acquisitions from MS2 scans, or SWATH, can quantify all fragment ion intensities when reference spectra are available. As each SWATH acquisition cycle typically contains an MS1 scan, these two independent label-free quantitative approaches can be acquired in a single experiment. Here, we have expanded the capability of Skyline to extract both MS1 and MS2 ion intensity chromatograms from a single SWATH data-independent acquisition in an Integrated Dual Scan Analysis approach. The performance of both MS1 and MS2 data was examined in simple and complex samples using standard concentration curves. Cases of interferences in MS1 and MS2 ion intensity data were assessed, as were the differentiation and quantitation of phosphopeptide isomers in MS2 scan data. In addition, we demonstrated an approach for optimization of SWATH m/z window sizes to reduce interferences using MS1 scans as a guide. Finally, a correlation analysis was performed on both MS1 and MS2 ion intensity data obtained from SWATH acquisitions on a complex mixture using a linear model that automatically removes signals containing interferences. This work demonstrates the practical advantages of properly acquiring and processing MS1 precursor data in addition to MS2 fragment ion intensity data in a data-independent acquisition (SWATH), and provides an approach to simultaneously obtain independent measurements of relative peptide abundance from a single experiment.

Published

2015

4. TheE. colisirtuin CobB shows no preference for enzymatic and nonenzymatic lysine acetylation substrate sites

Author

Dylan J. Sorensen, Misty L. Kuhn, Alan J. Wolfe, Birgit Schilling, Linda I. Hu, Wayne F. Anderson, Alexandria K. Sahu, Milan Mrksich, Bradford W. Gibson, Dörte Becher, Haike Antelmann, Alaa Abouelfetouh, and Michael D. Scholle

Subjects

Lysine Acetyltransferases, Lysine, Biology, medicine.disease_cause, Microbiology, Substrate Specificity, chemistry.chemical_compound, Escherichia coli, medicine, Sirtuins, bacteria, crystallography, Original Research, mass spectrometry, posttranslational modification, Escherichia coli Proteins, Acetylation, CobB, deacetylase, 3. Good health, chemistry, Biochemistry, Acetyllysine, Sirtuin, biology.protein, NAD+ kinase, Acetyl phosphate

Abstract

N(ε) -lysine acetylation is an abundant posttranslational modification of thousands of proteins involved in diverse cellular processes. In the model bacterium Escherichia coli, the ε-amino group of a lysine residue can be acetylated either catalytically by acetyl-coenzyme A (acCoA) and lysine acetyltransferases, or nonenzymatically by acetyl phosphate (acP). It is well known that catalytic acCoA-dependent N(ε) -lysine acetylation can be reversed by deacetylases. Here, we provide genetic, mass spectrometric, structural and immunological evidence that CobB, a deacetylase of the sirtuin family of NAD(+) -dependent deacetylases, can reverse acetylation regardless of acetyl donor or acetylation mechanism. We analyzed 69 lysines on 51 proteins that we had previously detected as robustly, reproducibly, and significantly more acetylated in a cobB mutant than in its wild-type parent. Functional and pathway enrichment analyses supported the hypothesis that CobB regulates protein function in diverse and often essential cellular processes, most notably translation. Combined mass spectrometry, bioinformatics, and protein structural data provided evidence that the accessibility and three-dimensional microenvironment of the target acetyllysine help determine CobB specificity. Finally, we provide evidence that CobB is the predominate deacetylase in E. coli.

Published

2014

5. Iron promotes protein insolubility and aging in C. elegans

Author

Bradford W. Gibson, Pankaj Kapahi, Alexandria K. Sahu, Gordon J. Lithgow, Dylan J. Sorensen, Birgit Schilling, David W. Killilea, Julie K. Andersen, Ida M. Klang, and Peter Swoboda

Subjects

Proteomics, Aging, Time Factors, Iron, media_common.quotation_subject, chemistry.chemical_element, Calcium, Protein aggregation, protein aggregation, Protein Aggregates, Organelle, Animals, Homeostasis, Caenorhabditis elegans, Caenorhabditis elegans Proteins, Chelating Agents, media_common, Dietary iron, biology, Age Factors, Longevity, Cell Biology, biology.organism_classification, Diet, Cell biology, Solubility, Proteotoxicity, chemistry, C. elegans, metal homeostasis, lifespan, Research Paper

Abstract

Many late-onset proteotoxic diseases are accompanied by a disruption in homeostasis of metals (metallostasis) including iron, copper and zinc. Although aging is the most prominent risk factor for these disorders, the impact of aging on metallostasis and its role in proteotoxic disease remain poorly understood. Moreover, it is not clear whether a loss of metallostasis influences normal aging. We have investigated the role of metallostasis in longevity of Caenorhabditis elegans. We found that calcium, copper, iron, and manganese levels increase as a function of age, while potassium and phosphorus levels tend to decrease. Increased dietary iron significantly accelerated the age-related accumulation of insoluble protein, a molecular pathology of aging. Proteomic analysis revealed widespread effects of dietary iron in multiple organelles and tissues. Pharmacological interventions to block accumulation of specific metals attenuated many models of proteotoxicity and extended normal lifespan. Collectively, these results suggest that a loss of metallostasis with aging contributes to age-related protein aggregation.

Published

2014

6. Variation and quantification among a target set of phosphopeptides in human plasma by multiple reaction monitoring and SWATH-MS2 data-independent acquisition

Author

Anna M. Zawadzka, Bradford W. Gibson, Alexandria K. Sahu, Susan J. Fisher, Birgit Schilling, Jason M. Held, Penelope M. Drake, and Michael P. Cusack

Subjects

Cell signaling, Chromatography, Chemistry, Phosphopeptide, Clinical Biochemistry, Computational biology, Proteomics, Tandem mass spectrometry, Biochemistry, Blood proteins, Analytical Chemistry, Phosphorylation, Data-independent acquisition, Target protein

Abstract

Human plasma contains proteins that reflect overall health and represents a rich source of proteins for identifying and understanding disease pathophysiology. However, few studies have investigated changes in plasma phosphoproteins. In addition, little is known about the normal variations in these phosphoproteins, especially with respect to specific sites of modification. To address these questions, we evaluated variability in plasma protein phosphorylation in healthy individuals using multiple reaction monitoring (MRM) and SWATH-MS2 data-independent acquisition. First, we developed a discovery workflow for phosphopeptide enrichment from plasma and identified targets for MRM assays. Next, we analyzed plasma from healthy donors using an analytical workflow consisting of MRM and SWATH-MS2 that targeted phosphopeptides from 58 and 68 phosphoproteins, respectively. These two methods produced similar results showing low variability in 13 phosphosites from 10 phosphoproteins (CVinter 30%). Moreover, these phosphopeptides originate from phosphoproteins involved in cellular processes governing homeostasis, immune response, cell-extracellular matrix interactions, lipid and sugar metabolism, and cell signaling. This limited assessment of technical and biological variability in phosphopeptides generated from plasma phosphoproteins among healthy volunteers constitutes a reference for future studies that target protein phosphorylation as biomarkers.

Published

2014

7. Phosphoprotein Secretome of Tumor Cells as a Source of Candidates for Breast Cancer Biomarkers in Plasma

Author

Christopher C. Benz, Susan J. Fisher, Alexandria K. Sahu, Anna M. Zawadzka, Birgit Schilling, Penelope M. Drake, Bradford W. Gibson, and Michael P. Cusack

Subjects

Proteomics, Breast Neoplasms, Adenocarcinoma, Bioinformatics, Biochemistry, Analytical Chemistry, Breast cancer, Biomarkers, Tumor, Tumor Cells, Cultured, medicine, Humans, Protein phosphorylation, Phosphorylation, Molecular Biology, biology, Phosphopeptide, Research, Carcinoma, Ductal, Breast, CD44, Cancer, Phosphoproteins, medicine.disease, 3. Good health, Gene Expression Regulation, Neoplastic, Phosphoprotein, MCF-7 Cells, biology.protein, Cancer research, Biomarker (medicine), Female, Signal transduction

Abstract

Breast cancer is a heterogeneous disease whose molecular diversity is not well reflected in clinical and pathological markers used for prognosis and treatment selection. As tumor cells secrete proteins into the extracellular environment, some of these proteins reach circulation and could become suitable biomarkers for improving diagnosis or monitoring response to treatment. As many signaling pathways and interaction networks are altered in cancerous tissues by protein phosphorylation, changes in the secretory phosphoproteome of cancer tissues could reflect both disease progression and subtype. To test this hypothesis, we compared the phosphopeptide-enriched fractions obtained from proteins secreted into conditioned media (CM) derived from five luminal and five basal type breast cancer cell lines using label-free quantitative mass spectrometry. Altogether over 5000 phosphosites derived from 1756 phosphoproteins were identified, several of which have the potential to qualify as phosphopeptide plasma biomarker candidates for the more aggressive basal and also the luminal-type breast cancers. The analysis of phosphopeptides from breast cancer patient plasma and controls allowed us to construct a discovery list of phosphosites under rigorous collection conditions, and second to qualify discovery candidates generated from the CM studies. Indeed, a set of basal-specific phosphorylation CM site candidates derived from IBP3, CD44, OPN, FSTL3, LAMB1, and STC2, and luminal-specific candidates derived from CYTC and IBP5 were selected and, based on their presence in plasma, quantified across all cell line CM samples using Skyline MS1 intensity data. Together, this approach allowed us to assemble a set of novel cancer subtype specific phosphopeptide candidates for subsequent biomarker verification and clinical validation.

Published

2014

8. A framework for installable external tools in Skyline

Author

Alexandria K. Sahu, Nicholas J. Shulman, Deepak R. Mani, Yuval Boss, Kaipo Tamura, Meena Choi, Olga Vitek, Susan E. Abbatiello, Steven A. Carr, Rushdy Ahmad, Vagisha Sharma, Daniel Broudy, Birgit Schilling, Trevor Killeen, Deepak Mani, Bradford W. Gibson, Michael J. MacCoss, and Brendan MacLean

Subjects

Proteomics, Statistics and Probability, Skyline, Downstream (software development), Database, Interface (Java), Computer science, InformationSystems_DATABASEMANAGEMENT, Experimental data, computer.software_genre, Applications Notes, Biochemistry, Mass Spectrometry, Computer Science Applications, Computational Mathematics, Computational Theory and Mathematics, Molecular Biology, computer, Software

Abstract

Summary: Skyline is a Windows client application for targeted proteomics method creation and quantitative data analysis. The Skyline document model contains extensive mass spectrometry data from targeted proteomics experiments performed using selected reaction monitoring, parallel reaction monitoring and data-independent and data-dependent acquisition methods. Researchers have developed software tools that perform statistical analysis of the experimental data contained within Skyline documents. The new external tools framework allows researchers to integrate their tools into Skyline without modifying the Skyline codebase. Installed tools provide point-and-click access to downstream statistical analysis of data processed in Skyline. The framework also specifies a uniform interface to format tools for installation into Skyline. Tool developers can now easily share their tools with proteomics researchers using Skyline. Availability and implementation: Skyline is available as a single-click self-updating web installation at http://skyline.maccosslab.org. This Web site also provides access to installable external tools and documentation. Contact: brendanx@u.washington.edu Supplementary information: Supplementary Data are available at Bioinformatics online.

Published

2014

9. Multiplexed, Scheduled, High-Resolution Parallel Reaction Monitoring on a Full Scan QqTOF Instrument with Integrated Data-Dependent and Targeted Mass Spectrometric Workflows

Author

Michael J. MacCoss, Bradford W. Gibson, Alexandria K. Sahu, Theodore W. Peters, Christie L. Hunter, Jason M. Held, Matthew J. Rardin, Dylan J. Sorensen, Alan J. Wolfe, Birgit Schilling, and Brendan MacLean

Subjects

Chromatography, Time Factors, Chemistry, Selected reaction monitoring, High resolution, Saccharomyces cerevisiae, Mass spectrometry, Mass spectrometric, Multiplexing, Mass Spectrometry, Article, Analytical Chemistry, Triple quadrupole mass spectrometer, Workflow, Escherichia coli, Animals, Caenorhabditis elegans, Peptides, Data dependent, Chromatography, High Pressure Liquid, Software

Abstract

Recent advances in commercial mass spectrometers with higher resolving power and faster scanning capabilities have expanded their functionality beyond traditional data-dependent acquisition (DDA) to targeted proteomics with higher precision and multiplexing. Using an orthogonal quadrupole time-of flight (QqTOF) LC-MS system, we investigated the feasibility of implementing large-scale targeted quantitative assays using scheduled, high resolution multiple reaction monitoring (sMRM-HR), also referred to as parallel reaction monitoring (sPRM). We assessed the selectivity and reproducibility of PRM, also referred to as parallel reaction monitoring, by measuring standard peptide concentration curves and system suitability assays. By evaluating up to 500 peptides in a single assay, the robustness and accuracy of PRM assays were compared to traditional SRM workflows on triple quadrupole instruments. The high resolution and high mass accuracy of the full scan MS/MS spectra resulted in sufficient selectivity to monitor 6-10 MS/MS fragment ions per target precursor, providing flexibility in postacquisition assay refinement and optimization. The general applicability of the sPRM workflow was assessed in complex biological samples by first targeting 532 peptide precursor ions in a yeast lysate, and then 466 peptide precursors from a previously generated candidate list of differentially expressed proteins in whole cell lysates from E. coli. Lastly, we found that sPRM assays could be rapidly and efficiently developed in Skyline from DDA libraries when acquired on the same QqTOF platform, greatly facilitating their successful implementation. These results establish a robust sPRM workflow on a QqTOF platform to rapidly transition from discovery analysis to highly multiplexed, targeted peptide quantitation.

Published

2015

10. Protein acetylation dynamics in response to carbon overflow in Escherichia coli

Author

Birgit, Schilling, David, Christensen, Robert, Davis, Alexandria K, Sahu, Linda I, Hu, Arti, Walker-Peddakotla, Dylan J, Sorensen, Bozena, Zemaitaitis, Bradford W, Gibson, and Alan J, Wolfe

Subjects

Proteomics, Escherichia coli Proteins, Lysine, Acetylation, Gene Expression Regulation, Bacterial, Acetates, Carbon, Article, Carbon Cycle, Glucose, Acetyltransferases, Escherichia coli, Protein Processing, Post-Translational, Metabolic Networks and Pathways

Abstract

In Escherichia coli, acetylation of proteins at lysines depends largely on a non-enzymatic acetyl-phosphate-dependent mechanism. To assess the functional significance of this post-translational modification, we first grew wild-type cells in buffered tryptone broth with glucose, and monitored acetylation over time by immunochemistry. Most acetylation occurred in stationary phase and paralleled glucose consumption and acetate excretion, which began upon entry into stationary phase. Transcription of rprA, a stationary phase regulator, exhibited similar behavior. To identify sites and substrates with significant acetylation changes, we used label-free, quantitative proteomics to monitor changes in protein acetylation. During growth, both the number of identified sites and the extent of acetylation increased with considerable variation among lysines from the same protein. Since glucose-regulated lysine acetylation was predominant in central metabolic pathways and overlapped with acetyl-phosphate-regulated acetylation sites, we deleted the major carbon regulator CRP and observed a dramatic loss of acetylation that could be restored by deleting the enzyme that degrades acetyl phosphate. We propose that acetyl-phosphate-dependent acetylation is a response to carbon flux that could regulate central metabolism.

Published

2015

11. SIRT5 Regulates both Cytosolic and Mitochondrial Protein Malonylation with Glycolysis as a Major Target

Author

Marc K. Hellerstein, Chris Carrico, Matthew J. Rardin, Philipp Gut, Eric Verdin, Wenjuan He, Bradford W. Gibson, Alexandria K. Sahu, Mark Fitch, Yuya Nishida, and Rami Najjar

Subjects

SIRT5, Acylation, Lysine, Dehydrogenase, Article, Mitochondrial Proteins, Succinylation, Protein acylation, Mice, Cytosol, Catalytic Domain, Animals, Humans, Sirtuins, Molecular Biology, Glyceraldehyde 3-phosphate dehydrogenase, Mice, Knockout, biology, Molecular Mimicry, Glyceraldehyde-3-Phosphate Dehydrogenases, Cell Biology, Malonates, HEK293 Cells, Biochemistry, Amino Acid Substitution, Liver, Gene Knockdown Techniques, biology.protein, bacteria, lipids (amino acids, peptides, and proteins), NAD+ kinase, Flux (metabolism), Glycolysis, Metabolic Networks and Pathways

Abstract

Summary Protein acylation links energetic substrate flux with cellular adaptive responses. SIRT5 is a NAD + -dependent lysine deacylase and removes both succinyl and malonyl groups. Using affinity enrichment and label free quantitative proteomics, we characterized the SIRT5-regulated lysine malonylome in wild-type (WT) and Sirt5 −/− mice. 1,137 malonyllysine sites were identified across 430 proteins, with 183 sites (from 120 proteins) significantly increased in Sirt5 −/− animals. Pathway analysis identified glycolysis as the top SIRT5-regulated pathway. Importantly, glycolytic flux was diminished in primary hepatocytes from Sirt5 −/− compared to WT mice. Substitution of malonylated lysine residue 184 in glyceraldehyde 3-phosphate dehydrogenase with glutamic acid, a malonyllysine mimic, suppressed its enzymatic activity. Comparison with our previous reports on acylation reveals that malonylation targets a different set of proteins than acetylation and succinylation. These data demonstrate that SIRT5 is a global regulator of lysine malonylation and provide a mechanism for regulation of energetic flux through glycolysis.

Published

2014

12. Sirtuin regulation of lysine acylation targets diverse metabolic networks in hepatic mitochondria (981.3)

Author

Yuya Nishida, Bradford W. Gibson, Matthew J. Rardin, Wejuan He, Eric Verdin, and Alexandria K. Sahu

Subjects

Acylation, Biochemistry, biology, Chemistry, Sirtuin, Lysine, Genetics, biology.protein, Hepatic mitochondria, Molecular Biology, Biotechnology

Published

2014

13. Structural, kinetic and proteomic characterization of acetyl phosphate-dependent bacterial protein acetylation

Author

Wayne F. Anderson, Linda I. Hu, George Minasov, Alexandria K. Sahu, Bozena Zemaitaitis, Dylan J. Sorensen, Misty L. Kuhn, Milan Mrksich, Michael D. Scholle, Alan J. Wolfe, Birgit Schilling, Bradford W. Gibson, and Bruno P. Lima

Subjects

Proteomics, Lysine Acetyltransferases, Lysine, lcsh:Medicine, Isomerase, Crystallography, X-Ray, Biochemistry, Mass Spectrometry, Triosephosphate isomerase, Microbial Physiology, Bacterial Physiology, lcsh:Science, chemistry.chemical_classification, 0303 health sciences, Spectrometric Identification of Proteins, Crystallography, Multidisciplinary, Physics, Escherichia coli Proteins, Acetylation, Condensed Matter Physics, Organophosphates, Physical Sciences, Carbohydrate Metabolism, Research Article, Protein Structure, Blotting, Western, Molecular Sequence Data, Biology, Microbiology, 03 medical and health sciences, Escherichia coli, Solid State Physics, Amino Acid Sequence, Binding site, Microbial Metabolism, 030304 developmental biology, Cofactor binding, Binding Sites, Staining and Labeling, 030306 microbiology, lcsh:R, Biology and Life Sciences, Proteins, Bacteriology, Kinetics, Metabolism, Glucose, Enzyme, chemistry, bacteria, Mutant Proteins, lcsh:Q

Abstract

The emerging view of Nε-lysine acetylation in eukaryotes is of a relatively abundant post-translational modification (PTM) that has a major impact on the function, structure, stability and/or location of thousands of proteins involved in diverse cellular processes. This PTM is typically considered to arise by the donation of the acetyl group from acetyl-coenzyme A (acCoA) to the ε-amino group of a lysine residue that is reversibly catalyzed by lysine acetyltransferases and deacetylases. Here, we provide genetic, mass spectrometric, biochemical and structural evidence that Nε-lysine acetylation is an equally abundant and important PTM in bacteria. Applying a recently developed, label-free and global mass spectrometric approach to an isogenic set of mutants, we detected acetylation of thousands of lysine residues on hundreds of Escherichia coli proteins that participate in diverse and often essential cellular processes, including translation, transcription and central metabolism. Many of these acetylations were regulated in an acetyl phosphate (acP)-dependent manner, providing compelling evidence for a recently reported mechanism of bacterial Nε-lysine acetylation. These mass spectrometric data, coupled with observations made by crystallography, biochemistry, and additional mass spectrometry showed that this acP-dependent acetylation is both non-enzymatic and specific, with specificity determined by the accessibility, reactivity and three-dimensional microenvironment of the target lysine. Crystallographic evidence shows acP can bind to proteins in active sites and cofactor binding sites, but also potentially anywhere molecules with a phosphate moiety could bind. Finally, we provide evidence that acP-dependent acetylation can impact the function of critical enzymes, including glyceraldehyde-3-phosphate dehydrogenase, triosephosphate isomerase, and RNA polymerase.

Published

2014

14. SIRT5 regulates the mitochondrial lysine succinylome and metabolic networks

Author

Daniel Mulhern, Radha Uppala, Timothy Riiff, John C. Newman, Bradford W. Gibson, Lei Zhu, Robert Stevens, Wenjuan He, Alexandria K. Sahu, Eric Verdin, Philipp Gut, Matthew P. Jacobson, Yuya Nishida, Christopher B. Newgard, Chris Carrico, Steven R. Danielson, Eric S. Goetzman, Mark Fitch, Marc K. Hellerstein, Biao Li, Ailan Guo, Matthew J. Rardin, Jing Zhou, and Olga Ilkayeva

Subjects

Hydroxymethylglutaryl-CoA Synthase, Male, SIRT5, Physiology, Knockout, Lysine, Amino Acid Motifs, Hydroxybutyrates, Mitochondria, Liver, Ketone Bodies, Medical Biochemistry and Metabolomics, Mitochondrion, Article, Cell Line, Mitochondrial Proteins, Endocrinology & Metabolism, 03 medical and health sciences, Protein succinylation, Succinylation, Mice, 0302 clinical medicine, Carnitine, Ketogenesis, Animals, Humans, Sirtuins, Molecular Biology, 030304 developmental biology, Mice, Knockout, 0303 health sciences, ATP synthase, biology, Liver Disease, Succinates, Cell Biology, Mitochondria, Metabolic pathway, Liver, Biochemistry, Mutation, biology.protein, Biochemistry and Cell Biology, Digestive Diseases, Oxidation-Reduction, 030217 neurology & neurosurgery, Metabolic Networks and Pathways, Biotechnology

Abstract

SummaryReversible posttranslational modifications are emerging as critical regulators of mitochondrial proteins and metabolism. Here, we use a label-free quantitative proteomic approach to characterize the lysine succinylome in liver mitochondria and its regulation by the desuccinylase SIRT5. A total of 1,190 unique sites were identified as succinylated, and 386 sites across 140 proteins representing several metabolic pathways including β-oxidation and ketogenesis were significantly hypersuccinylated in Sirt5−/− animals. Loss of SIRT5 leads to accumulation of medium- and long-chain acylcarnitines and decreased β-hydroxybutyrate production in vivo. In addition, we demonstrate that SIRT5 regulates succinylation of the rate-limiting ketogenic enzyme 3-hydroxy-3-methylglutaryl-CoA synthase 2 (HMGCS2) both in vivo and in vitro. Finally, mutation of hypersuccinylated residues K83 and K310 on HMGCS2 to glutamic acid strongly inhibits enzymatic activity. Taken together, these findings establish SIRT5 as a global regulator of lysine succinylation in mitochondria and present a mechanism for inhibition of ketogenesis through HMGCS2.

Published

2013