Substituent Effects in the Cationic Green Fluorescent Protein Chromophore: Ultrafast Excited‐State Proton Transfer or Twisting?

Author:

Liu Jiawei1ORCID,Chen Cheng1ORCID,Sokolov Anatolii I.23,Baranov Mikhail S.23ORCID,Fang Chong1ORCID

Affiliation:

1. Department of Chemistry Oregon State University 153 Gilbert Hall Corvallis Oregon 97331 USA

2. Institute of Bioorganic Chemistry Russian Academy of Sciences Miklukho-Maklaya 16/10 Moscow 117997 Russia

3. Pirogov Russian National Research Medical University Ostrovitianov 1 Moscow 117997 Russia

Abstract

AbstractUnderstanding the structure‐function relationships of the green fluorescent protein (GFP) chromophore is important in rationally developing new molecular tools for biological imaging and beyond. Herein, we systematically modified the GFP chromophore structure with electron‐withdrawing and ‐donating groups (EWGs and EDGs) to investigate the substituent effects on the excited‐state proton transfer (ESPT) and twisting dynamics of the cationic chromophore in solution. With key insights gained from femtosecond transient absorption and stimulated Raman spectroscopy, we reveal that the EWG substitution by –F increases photoacidity in an additive manner and leads to an ultrafast barrierless ESPT by difluorination, while the EDG substitution by –OCH3 also results in ultrafast ESPT despite the weak photoacidity as estimated by the Förster equation. We ascribe the unusually fast kinetics in methoxylated derivatives to the occurrence of a pre‐existing chromophore‐solvent complex that sets up the acceptor site for ESPT. Furthermore, the kinetic competition between ESPT and twisting pathways is crucial for the observation of ESPT in action, particularly for molecules undergoing efficient nonradiative decay in the excited state through torsional motions. Such flexible and highly engineerable molecules can enable more versatile photoswitches and sensors.

Funder

National Science Foundation

Publisher

Wiley

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