Redox Proteomics of Protein-bound Methionine Oxidation

Bart Ghesquière; Veronique Jonckheere; Niklaas Colaert; Joost Van Durme; Evy Timmerman; Marc Goethals; Joost Schymkowitz; Frédéric Rousseau; Joël Vandekerckhove; Kris Gevaert

doi:10.1074/mcp.m110.006866

Redox Proteomics of Protein-bound Methionine Oxidation

Bart Ghesquière(Ghent University), Veronique Jonckheere(VIB-UGent Center for Medical Biotechnology), Niklaas Colaert(Ghent University), Joost Van Durme(Vrije Universiteit Brussel), Evy Timmerman(Ghent University), Marc Goethals(VIB-UGent Center for Medical Biotechnology), Joost Schymkowitz(Vrije Universiteit Brussel), Frédéric Rousseau(Vrije Universiteit Brussel), Joël Vandekerckhove(VIB-UGent Center for Medical Biotechnology), Kris Gevaert(VIB-UGent Center for Medical Biotechnology)

Molecular & Cellular Proteomics

March 15, 2011

10.1074/mcp.m110.006866

Cited by 134Open Access

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Abstract

We here present a new method to measure the degree of protein-bound methionine sulfoxide formation at a proteome-wide scale. In human Jurkat cells that were stressed with hydrogen peroxide, over 2000 oxidation-sensitive methionines in more than 1600 different proteins were mapped and their extent of oxidation was quantified. Meta-analysis of the sequences surrounding the oxidized methionine residues revealed a high preference for neighboring polar residues. Using synthetic methionine sulfoxide containing peptides designed according to the observed sequence preferences in the oxidized Jurkat proteome, we discovered that the substrate specificity of the cellular methionine sulfoxide reductases is a major determinant for the steady-state of methionine oxidation. This was supported by a structural modeling of the MsrA catalytic center. Finally, we applied our method onto a serum proteome from a mouse sepsis model and identified 35 in vivo methionine oxidation events in 27 different proteins.

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