Comparative Profiling of the Mammalian Mitochondrial Proteome:  Multiple Aconitase-2 Isoforms Including <i>N</i>-formylkynurenine Modifications as Part of a Protein Biomarker Signature for Reactive Oxidative Species

Hunzinger, Christian; Woźny, Wojciech; Schwall, Gerhard P.; Poznanović, Slobodan; Stegmann, Werner; Zengerling, Helmut; Schoepf, Rainer; Groebe, Karlfried; Cahill, Michael A.; Osiewacz, Heinz D.; Jägemann, Nora; Bloch, M.; Dencher, Norbert A.; Krause, Frank; Schrattenholz, André

doi:10.1021/pr050377+

Cited by 68 publications

(81 citation statements)

References 67 publications

(163 reference statements)

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“…11 Different isoforms of aconitase have been detected in 2-D protein map 26 and the activity of aconitase has been found be sensitive to oxidative conditions. 27 During oxidative stress and altered metabolic conditions aconitase relocates from the TCA cycle to mtDNA nucleoids, where it stabilizes the genome under these adverse conditions.…”

Section: Discussionmentioning

confidence: 99%

Mitochondrial proteome analysis reveals altered expression of voltage dependent anion channels in pancreatic β-cells exposed to high glucose

Ahmed¹,

Muhammed²,

Kessler³

et al. 2010

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Section: Discussionmentioning

confidence: 99%

Mitochondrial proteome analysis reveals altered expression of voltage dependent anion channels in pancreatic β-cells exposed to high glucose

Ahmed¹,

Muhammed²,

Kessler³

et al. 2010

Islets

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“…Each lane was loaded with the extract from mitochondria containing 150 g (for in-gel activity), 300 g (for 2D SDS-PAGE), or 400 g (for 2D BN-PAGE) of protein before solubilization which was assessed by Bradford assay. For BN-PAGE and CN-PAGE, linear 3 to 13% gradient gels overlaid with a 3% stacking gel were used in a Hoefer SE 600 system (18 by 16 by 0.15 cm 3 ) (40,69,72). CN-PAGE was performed according to the methods of Schägger et al (72), omitting Coomassie blue dye in the cathode buffer and without the addition of detergent in the gel (46,61).…”

Section: Methodsmentioning

confidence: 99%

Supramolecular Organization of the Respiratory Chain in Neurospora crassa Mitochondria

et al. 2007

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The existence of specific respiratory supercomplexes in mitochondria of most organisms has gained much momentum. However, its functional significance is still poorly understood. The availability of many deletion mutants in complex I (NADH:ubiquinone oxidoreductase) of Neurospora crassa, distinctly affected in the assembly process, offers unique opportunities to analyze the biogenesis of respiratory supercomplexes. Herein, we describe the role of complex I in assembly of respiratory complexes and supercomplexes as suggested by blue and colorless native polyacrylamide gel electrophoresis and mass spectrometry analyses of mildly solubilized mitochondria from the wild type and eight deletion mutants.As an important refinement of the fungal respirasome model, we found that the standard respiratory chain of N. crassa comprises putative complex I dimers in addition to I-III-IV and III-IV supercomplexes. Three Neurospora mutants able to assemble a complete complex I, lacking only the disrupted subunit, have respiratory supercomplexes, in particular I-III-IV supercomplexes and complex I dimers, like the wild-type strain. Furthermore, we were able to detect the I-III-IV supercomplexes in the nuo51 mutant with no overall enzymatic activity, representing the first example of inactive respirasomes. In addition, III-IV supercomplexes were also present in strains lacking an assembled complex I, namely, in four membrane arm subunit mutants as well as in the peripheral arm nuo30.4 mutant. In membrane arm mutants, high-molecular-mass species of the 30.4-kDa peripheral arm subunit comigrating with III-IV supercomplexes and/or the prohibitin complex were detected. The data presented herein suggest that the biogenesis of complex I is linked with its assembly into supercomplexes.

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“…The combined application of conventional 2-DE with denaturing/nondenaturing, unconventional 2-DE approaches has been suggested to be sufficient to provide a repertory of all membrane proteins of a given sample [144,164].…”

Section: Membrane Proteomementioning

confidence: 99%

Two‐dimensional gel electrophoresis and mass spectrometry for biomarker discovery

Penque

2009

Proteomics Clinical Apps

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The proteome project, initiated in 1995, was made possible by 2-DE combined with MS. The project main objective was and remains the identification of all proteins expressed by a cell, tissue or organism in a given time and condition. Following this objective, the global profiling of proteins in health versus pathological state by the 2-DE/MS-based proteomic approach has contributed to the elucidation of the basic mechanisms of disease by discovering candidate disease biomarkers and disease targets for new drug development. This review will briefly summarize the historical evolution of 2-DE up to today, and review 2-DE/MS technology and its specific methods of study of immunoresponse (immunoproteomics), PTM of proteins, complex proteinprotein interactions (interactome), the proteome of cell membrane and intracellular proteome turnover in disease biomarker discovery. 2-DE historical evolutionGlobal profiling of proteins in healthy versus pathological states is a strategy to discover biomarkers for early diagnostics, disease progression, treatment response and novel targets for therapeutic drugs development. The idea of making an inventory of all the proteins in a cell, tissue or organism with normal or abnormal physiology, was (re)initiated in the middle of the 1990s with the proteome project [1]. Since then, many technologies to make the analysis of the proteome a reality have been united.The perfect technological 'marriage' that made the proteome project feasible was between high resolution 2-DE for separation of large numbers of proteins and MS for identification and characterization of the proteins displayed on this gel [2]. However, before this happy union occured, science and technology devoted to protein study had a long journey until 2-DE and MS combination was possible (Fig. 1). It started in the last century, in 1937, when Tiselius [3] introduced electrophoresis technique as a modification of Reiner's early concept (1927) [4] to analyse a complex mixture of proteins such as serum proteins. Only 20 years later, in 1959, electrophoresis on a gel support formed by crosslinked polymerization of Cyanogum 41, a commercial name for two organic monomers, acrylamide and the crosslinking agent, N,N1-methylenebisacrylamide, was shown to be useful and was named PAGE by Raymond and Weintraub [5]. The adaptation of polyacrylamide gel to IEF in a stable pH gradient, developed by Svensson in 1962 [6], was possible by the end of the 1960s [7][8][9]. About this time, the 2-D by combining IEF to separate undenatured proteins according to their charge and gradient SDS-PAGE for a second separation, according to their molecular mass, was for the first time introduced by Kenrick and Margolis (1970) [10]. Only in 1975, was IEF in denaturing conditions, as known today, used to follow the 2-D PAGE and it was described in three independent works [11][12][13]. The most powerful demonstraCorrespondence: Dr. Deborah Penque, Laboratório de Proteó-mica, Departamento de Genética, Instituto Nacional de Saúde, Dr. Ricardo Jorge, I.P., A...

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Comparative Profiling of the Mammalian Mitochondrial Proteome: Multiple Aconitase-2 Isoforms Including N-formylkynurenine Modifications as Part of a Protein Biomarker Signature for Reactive Oxidative Species

Cited by 68 publications

References 67 publications

Mitochondrial proteome analysis reveals altered expression of voltage dependent anion channels in pancreatic β-cells exposed to high glucose

Mitochondrial proteome analysis reveals altered expression of voltage dependent anion channels in pancreatic β-cells exposed to high glucose

Supramolecular Organization of the Respiratory Chain in Neurospora crassa Mitochondria

Two‐dimensional gel electrophoresis and mass spectrometry for biomarker discovery

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