4.8 Article

Dual Photoisomerization on Distinct Potential Energy Surfaces in a UV-Absorbing Rhodopsin

Journal

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
Volume 142, Issue 26, Pages 11464-11473

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/jacs.0c03229

Keywords

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Funding

  1. Chemical Sciences Council of The Netherlands Organization for Scientific Research (NWO)
  2. German Research Foundation (DFG) [SFB1078]
  3. Hertie Foundation

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UV-absorbing rhodopsins are essential for UV vision and sensing in all kingdoms of life. Unlike the well-known visible-absorbing rhodopsins, which bind a protonated retinal Schiff base for light absorption, UV-absorbing rhodopsins bind an unprotonated retinal Schiff base. Thus far, the photoreaction dynamics and mechanisms of UV-absorbing rhodopsins have remained essentially unknown. Here, we report the complete excited- and ground-state dynamics of the UV form of histidine kinase rhodopsin 1 (HKR1) from eukaryotic algae, using femtosecond stimulated Raman spectroscopy (FSRS) and transient absorption spectroscopy, covering time scales from femtoseconds to milliseconds. We found that energy-level ordering is inverted with respect to visible-absorbing rhodopsins, with an optically forbidden low-lying S-1 excited state that has Ag- symmetry and a higher-lying UV-absorbing S-2 state of Bu+ symmetry. UV-photoexcitation to the S-2 state elicits a unique dual-isomerization reaction: first, C13=C14 cis-trans isomerization occurs during S-2-S-1 evolution in <100 fs. This very fast reaction features the remarkable property that the newly formed isomer appears in the excited state rather than in the ground state. Second, C15=N16 anti-syn isomerization occurs on the S-1-S-0 evolution to the ground state in 4.8 ps. We detected two ground-state unprotonated retinal photoproducts, 13-trans/15-anti (all-trans) and 13-cis/15-syn, after relaxation to the ground state. These isomers become protonated in 58 mu s and 3.2 ms, respectively, resulting in formation of the blue-absorbing form of HKR1. Our results constitute a benchmark of UV-induced photochemistry of animal and microbial rhodopsins.

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