AI Article Synopsis

  • Non-photochemical quenching (NPQ) is crucial for light tolerance in photosynthetic organisms like cyanobacteria, where it involves light-harvesting complexes and specific proteins like the orange carotenoid protein (OCP).
  • A biophysical model was developed to analyze the interactions between light-harvesting complexes (phycobilisomes), OCP, and fluorescence recovery protein (FRP), allowing for detailed insights into their dynamics and concentrations in cells.
  • The study revealed that while higher OCP levels are needed for effective quenching in vitro, the in vivo balance shifts due to greater phycobilisome concentration, emphasizing the complex regulatory mechanisms of NPQ in cyanobacteria.

Article Abstract

Non-photochemical quenching (NPQ) is a mechanism responsible for high light tolerance in photosynthetic organisms. In cyanobacteria, NPQ is realized by the interplay between light-harvesting complexes, phycobilisomes (PBs), a light sensor and effector of NPQ, the photoactive orange carotenoid protein (OCP), and the fluorescence recovery protein (FRP). Here, we introduced a biophysical model, which takes into account the whole spectrum of interactions between PBs, OCP, and FRP and describes the experimental PBs fluorescence kinetics, unraveling interaction rate constants between the components involved and their relative concentrations in the cell. We took benefit from the possibility to reconstruct the photoprotection mechanism and its parts in vitro, where most of the parameters could be varied, to develop the model and then applied it to describe the NPQ kinetics in the Synechocystis sp. PCC 6803 mutant lacking photosystems. Our analyses revealed  that while an excess of the OCP over PBs is required to obtain substantial PBs fluorescence quenching in vitro, in vivo the OCP/PBs ratio is less than unity, due to higher local concentration of PBs, which was estimated as ~10 M, compared to in vitro experiments. The analysis of PBs fluorescence recovery on the basis of the generalized model of enzymatic catalysis resulted in determination of the FRP concentration in vivo close to 10% of the OCP concentration. Finally, the possible role of the FRP oligomeric state alteration in the kinetics of PBs fluorescence was shown. This paper provides the most comprehensive model of the OCP-induced PBs fluorescence quenching to date and the results are important for better understanding of the regulatory molecular mechanisms underlying NPQ in cyanobacteria.

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http://dx.doi.org/10.1007/s11120-017-0377-8DOI Listing

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