PT - JOURNAL ARTICLE AU - Sophie A. Meredith AU - Takuro Yoneda AU - Ashley M. Hancock AU - Simon D. Connell AU - Stephen D. Evans AU - Kenichi Morigaki AU - Peter G. Adams TI - Understanding the photophysics and structural organization of photosynthetic proteins using model lipid membranes assembled from natural plant thylakoids AID - 10.1101/2020.09.15.296665 DP - 2020 Jan 01 TA - bioRxiv PG - 2020.09.15.296665 4099 - http://biorxiv.org/content/early/2020/09/16/2020.09.15.296665.short 4100 - http://biorxiv.org/content/early/2020/09/16/2020.09.15.296665.full AB - The light-harvesting (LH) biomembranes from photosynthetic organisms perform solar energy absorption and transfer with high efficiency. There is great interest in the nanoscale biophysics of photosynthesis, however, natural membranes are complex and highly curved so can be challenging to study. Here we present model photosynthetic “hybrid membranes” assembled from a combination of natural LH membranes and synthetic lipids deposited into a patterned polymerized lipid template on glass. This arrangement offers many advantages over previous model systems including: a sufficiently complex mixture of natural proteins to mimic the biological processes, a modular self-assembly mechanism, and a stabilizing template promoting the formation of supported lipid bilayers from complex natural membranes with high protein content (that would not otherwise form). These hybrid membranes can be used as a platform to delineate the complex relationship between LH energy pathways and membrane organization. Atomic force microscopy and fluorescence lifetime microscopy revealed that hybrid membranes have an elongated fluorescence lifetime (∼4 ns) compared to native membranes (∼0.5 ns), a direct consequence of reduced protein density and an uncoupling of protein-protein interactions. We observed the real time self-assembly and migration of LH proteins from natural membrane extracts into the hybrid membranes and monitored the photophysical state of the membranes at each stage. Finally, experiments utilizing our hybrid membranes suggest that assays currently used in the photosynthesis community to test the electron transfer activity of Photosystem II may have non-specific interactions with other proteins, implying that new methods are needed for reliable quantification of electron transfers in photosynthesis.Competing Interest StatementThe authors have declared no competing interest.