4.5 Article

Real-Time Monitoring of Chromophore Isomerization and Deprotonation during the Photoactivation of the Fluorescent Protein Dronpa

Journal

JOURNAL OF PHYSICAL CHEMISTRY B
Volume 119, Issue 6, Pages 2404-2414

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/jp507094f

Keywords

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Funding

  1. P.-G. de Gennes foundation [FPGG 033]
  2. CNRS
  3. Initiative d'Excellence program from French state [ANR-11-LABX-0011-01]

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Dronpa is a photochromic green fluorescent protein (GFP) homologue used as a probe in super-resolution microscopy. It is known that the photochromic reaction involves cis/trans isomerization of the chromophore and protonation/deprotonation of its phenol group, but the sequence in time of the two steps and their characteristic time scales are still the subject of much debate. We report here a comprehensive UVvisible transient absorption spectroscopy study of the photoactivation mechanism of Dronpa, covering all relevant time scales from similar to 100 fs to milliseconds. The Dronpa-2 variant was also studied and showed the same behavior. By carefully controlling the excitation energy to avoid multiphoton processes, we could measure both the spectrum and the anisotropy of the first photoactivation intermediate. We show that the observed few nanometer blue-shift of this intermediate is characteristic for a neutral cis chromophore, and that its anisotropy of similar to 0.2 is in good agreement with the reorientation of the transition dipole moment expected upon isomerization. These data constitute the first clear evidence that trans -> cis isomerization of the chromophore precedes its deprotonation and occurs on the picosecond time scale, concomitantly to the excited-state decay. We found the deprotonation step to follow in similar to 10 mu s and lead directly from the neutral cis intermediate to the final state.

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