The role of phosphorylation in redox regulation of photosynthesis genes psaA and psbA during photosynthetic acclimation of mustard

verfasst von: Sebastian Steiner, Lars Dietzel, Yvonne Schröter, Vidal Fey, Raik Wagner, Thomas Pfannschmidt
Abstract: The long-term response (LTR) to light-quality gradients improves performance and survival of plants in dense stands. It involves redox-controlled transcriptional regulation of the plastome-encoded genes psaAB (encoding the P700 apoproteins of photosystem I) and psbA (encoding the D1 protein of photosystem II) and requires the action of plastid-localized kinases. To study the potential impact of phosphorylation events on plastid gene expression during the LTR, we analyzed mustard seedlings acclimated to light sources favoring either photosystem I or photosystem II. Primer extension analyses of psaA transcripts indicate that the redox regulation occurs at the principal bacterial promoters, suggesting that the plastid encoded RNA polymerase (PEP) is the target for redox signals. Chloroplast protein fractions containing PEP and other DNA-binding proteins were purified from mustard via heparin-Sepharose chromatography. The biochemical properties of these fractions were analyzed with special emphasis on promoter recognition and specificity, phosphorylation state, and kinase activity. The results demonstrate that the LTR involves the action of small DNA-binding proteins; three of them exhibit specific changes in the phosphorylation state. Auto-phosphorylation assays, in addition, exhibit large differences in the activity of endogenous kinase activities. Chloroplast run-on transcription experiments with the kinase inhibitor H7 and the reductant DTT indicate that phosphorylation events are essential for the mediation of redox signals toward psaA and psbA transcription initiation, but require the synergistic action of a thiol redox signal. The data support the idea that redox signals from the thylakoid membrane are linked to gene expression via phosphorylation events; however, this mediation appears to require a complex network of interacting proteins rather than a simple phosphorelay.
Organisationseinheit(en): Institut für Botanik
Externe Organisation(en): Friedrich-Schiller-Universität Jena
Typ: Artikel
Journal: Molecular plant
Band: 2
Seiten: 416-29
Anzahl der Seiten: 14
ISSN: 1674-2052
Publikationsdatum: 05.2009
Publikationsstatus: Veröffentlicht
Peer-reviewed: Ja
Elektronische Version(en): https://doi.org/10.1093/mp/ssp007 (Zugang: Unbekannt)

BibTeX

@article{2e6c0316e2e44d3ea3e8c6a6a5504d5a,
title = "The role of phosphorylation in redox regulation of photosynthesis genes psaA and psbA during photosynthetic acclimation of mustard",
abstract = "The long-term response (LTR) to light-quality gradients improves performance and survival of plants in dense stands. It involves redox-controlled transcriptional regulation of the plastome-encoded genes psaAB (encoding the P700 apoproteins of photosystem I) and psbA (encoding the D1 protein of photosystem II) and requires the action of plastid-localized kinases. To study the potential impact of phosphorylation events on plastid gene expression during the LTR, we analyzed mustard seedlings acclimated to light sources favoring either photosystem I or photosystem II. Primer extension analyses of psaA transcripts indicate that the redox regulation occurs at the principal bacterial promoters, suggesting that the plastid encoded RNA polymerase (PEP) is the target for redox signals. Chloroplast protein fractions containing PEP and other DNA-binding proteins were purified from mustard via heparin-Sepharose chromatography. The biochemical properties of these fractions were analyzed with special emphasis on promoter recognition and specificity, phosphorylation state, and kinase activity. The results demonstrate that the LTR involves the action of small DNA-binding proteins; three of them exhibit specific changes in the phosphorylation state. Auto-phosphorylation assays, in addition, exhibit large differences in the activity of endogenous kinase activities. Chloroplast run-on transcription experiments with the kinase inhibitor H7 and the reductant DTT indicate that phosphorylation events are essential for the mediation of redox signals toward psaA and psbA transcription initiation, but require the synergistic action of a thiol redox signal. The data support the idea that redox signals from the thylakoid membrane are linked to gene expression via phosphorylation events; however, this mediation appears to require a complex network of interacting proteins rather than a simple phosphorelay.",
keywords = "Acclimatization, DNA-Binding Proteins/metabolism, Light, Oxidation-Reduction, Phosphorylation, Photosynthesis/physiology, Photosystem I Protein Complex/metabolism, Transcription, Genetic",
author = "Sebastian Steiner and Lars Dietzel and Yvonne Schr{\"o}ter and Vidal Fey and Raik Wagner and Thomas Pfannschmidt",
note = "Funding information: This work was supported by grants from the Deutsche Forschungsgemeinschaft to T.P. ( PF323/4 ), the DFG Research groups 387 and 804 , and by the NWP program of Thuringia.",
year = "2009",
month = may,
doi = "10.1093/mp/ssp007",
language = "English",
volume = "2",
pages = "416--29",
journal = "Molecular plant",
issn = "1674-2052",
publisher = "Cell Press",
number = "3",
}