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In vitro alkylation methods for assessing the protein redox state
Faculté des Sciences et Technologies, UMR 1136 Interactions Arbres/Microorganismes, Université de Lorraine/INRA, Vandoeuvre-lès-Nancy, France.
Faculté des Sciences et Technologies, UMR 1136 Interactions Arbres/Microorganismes, Université de Lorraine/INRA, Vandoeuvre-lès-Nancy, France.
Umeå universitet, Teknisk-naturvetenskapliga fakulteten, Institutionen för fysiologisk botanik. Umeå universitet, Teknisk-naturvetenskapliga fakulteten, Umeå Plant Science Centre (UPSC).ORCID-id: 0000-0002-0546-7721
Faculté des Sciences et Technologies, UMR 1136 Interactions Arbres/Microorganismes, Université de Lorraine/INRA, Vandoeuvre-lès-Nancy, France.
2017 (Engelska)Ingår i: Photorespiration: methods and protocols / [ed] Alisdair R. Fernie; Hermann Bauwe; Andreas P.M. Weber, New York: Humana Press, 2017, 1, , s. 14s. 51-64Kapitel i bok, del av antologi (Refereegranskat)
Abstract [en]

Cysteines are important residues for protein structure, function, and regulation. Owing to their modified reactivity, some cysteines can undergo very diverse redox posttranslational modifications, including the reversible formation of disulfide bonds, a widespread protein regulatory process as well exemplified in plant chloroplasts for Calvin-Benson cycle enzymes. Both core- and peripheral-photorespiratory enzymes possess conserved cysteines, some of which have been identified as being subject to oxidative modifications. This is not surprising considering their presence in subcellular compartments where the production of reactive species can be important. However, in most cases, the types of modifications and their biochemical effect on protein activity have not been validated, meaning that the possible impact of these modifications in a complex physiological context, such as photorespiration, remains obscure. We here describe a detailed set of protocols for alkylation methods that have been used so far to (1) study the protein cysteine redox state either in vitro by submitting purified recombinant proteins to reducing/oxidation treatments or in vivo by western blots on protein extracts from plants subject to environmental constraints, and its dependency on the two major reducing systems in the cell, i.e., the thioredoxin and glutathione/glutaredoxin systems, and (2) determine two key redox parameters, i.e., the cysteine pKa and the redox midpoint potential.

Ort, förlag, år, upplaga, sidor
New York: Humana Press, 2017, 1. , s. 14s. 51-64
Serie
Methods in Molecular Biology, ISSN 1064-3745, E-ISSN 1940-6029 ; 1653
Nyckelord [en]
Alkylation, Cysteine, Oxidative modification, pKa, Redox potential
Nationell ämneskategori
Biokemi Molekylärbiologi Botanik
Identifikatorer
URN: urn:nbn:se:umu:diva-208655DOI: 10.1007/978-1-4939-7225-8_4PubMedID: 28822125Scopus ID: 2-s2.0-85028022254ISBN: 9781493972241 (tryckt)ISBN: 9781493972258 (digital)OAI: oai:DiVA.org:umu-208655DiVA, id: diva2:1764957
Tillgänglig från: 2023-06-09 Skapad: 2023-06-09 Senast uppdaterad: 2025-02-20Bibliografiskt granskad

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Keech, Olivier

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Institutionen för fysiologisk botanikUmeå Plant Science Centre (UPSC)
BiokemiMolekylärbiologiBotanik

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