4.6 Article

Interplay between Flavodiiron Proteins and Photorespiration in Synechocystis sp. PCC 6803

Journal

JOURNAL OF BIOLOGICAL CHEMISTRY
Volume 286, Issue 27, Pages 24007-24014

Publisher

AMER SOC BIOCHEMISTRY MOLECULAR BIOLOGY INC
DOI: 10.1074/jbc.M111.223289

Keywords

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Funding

  1. Academy of Finland Center of Excellence [118637]
  2. European Union [212508]
  3. CNRS/Japan Science and Technology Agency
  4. Nordic Energy Research Program
  5. European Union
  6. Region Provence Alpes Cote d'Azur
  7. French Ministry of Research
  8. Commissariat a l'Energie Atomique

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Flavodiiron (Flv) proteins are involved in detoxification of O-2 and NO in anaerobic bacteria and archaea. Cyanobacterial Flv proteins, on the contrary, function in oxygenic environment and possess an extra NAD(P) H: flavin oxidoreductase module. Synechocystis sp. PCC 6803 has four genes (sll1521, sll0219, sll0550, and sll0217) encoding Flv proteins (Flv1, Flv2, Flv3, and Flv4). Previous in vitro studies with recombinant Flv3 protein from Synechocystis provided evidence that it functions as a NAD(P) H: oxygen oxidoreductase, and subsequent in vivo studies with Synechocystis confirmed the role of Flv1 and Flv3 proteins in the Mehler reaction (photoreduction of O-2 to H2O). Interestingly, homologous proteins to Flv1 and Flv3 can be found also in green algae, mosses, and Selaginella. Here, we addressed the function of Flv1 and Flv3 in Synechocystis using the Delta flv1, Delta flv3, and Delta flv1/Delta flv3 mutants and applying inorganic carbon (C-i)-deprivation conditions. We propose that only the Flv1/Flv3 heterodimer form is functional in the Mehler reaction in vivo. O-18(2) labeling was used to discriminate between O-2 evolution in photosynthetic water splitting and O-2 consumption. In wild type, similar to 20% of electrons originated from water was targeted to O-2 under air level CO2 conditions but increased up to 60% in severe limitation of C-i. Gas exchange experiments with Delta flv1, Delta flv3, and Delta flv1/Delta flv3 mutants demonstrated that a considerable amount of electrons in these mutants is directed to photorespiration under C-i deprivation. This assumption is in line with increased transcript abundance of photorespiratory genes and accumulation of photorespiratory intermediates in the WT and to a higher extent in mutant cells under C-i deprivation.

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