Abstract

Tracking vibrational motions during a photochemical or photophysical process has gained momentum, due to its sensitivity to the progression of reaction and change of environment. In this work, we implemented an advanced ultrafast vibrational technique, femtosecond-stimulated Raman spectroscopy (FSRS), to monitor the excited state structural evolution of an engineered green fluorescent protein (GFP) single-site mutant S205V. This mutation alters the original excited state proton transfer (ESPT) chain. By strategically tuning the Raman pump to different wavelengths (i.e., 801, 539, and 504 nm) to achieve pre-resonance with transient excited state electronic bands, the characteristic Raman modes of the excited protonated (A*) chromophore species and intermediate deprotonated (I*) species can be selectively monitored. The inhomogeneous distribution/population of A* species go through ESPT with a similar ~300 ps time constant, confirming that bridging a water molecule to protein residue T203 in the ESPT chain is the rate-limiting step. Some A* species undergo vibrational cooling through high-frequency motions on the ~190 ps time scale. At early times, a portion of the largely protonated A* species could also undergo vibrational cooling or return to the ground state with a ~80 ps time constant. On the photoproduct side, a ~1330 cm−1 delocalized motion is observed, with dispersive line shapes in both the Stokes and anti-Stokes FSRS with a pre-resonance Raman pump, which indicates strong vibronic coupling, as the mode could facilitate the I* species to reach a relatively stable state (e.g., the main fluorescent state) after conversion from A*. Our findings disentangle the contributions of various vibrational motions active during the ESPT reaction, and offer new structural dynamics insights into the fluorescence mechanisms of engineered GFPs and other analogous autofluorescent proteins.

Highlights

  • IntroductionThe accurate measurement and dynamic tracking of characteristic motions can offer valuable “bottom-up” insights into the conformation, structure, and evolution of the functional molecules of interest in the ground and excited state [1,2], and ideally in real time [3,4]

  • Vibrational frequencies of normal modes are the fingerprints of molecules

  • We implemented the femtosecond transient absorption (fs-TA) experiment and the wavelength-tunable femtosecond-stimulated Raman spectroscopy (FSRS) with three strategic Raman pump wavelengths (i.e., 800, 539, and 504 nm) to systematically dissect the excited state structural evolution of a green fluorescent protein (GFP) single-site mutant S205V, which has the same SYG chromophore as wild-type green fluorescent protein (wtGFP)

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Summary

Introduction

The accurate measurement and dynamic tracking of characteristic motions can offer valuable “bottom-up” insights into the conformation, structure, and evolution of the functional molecules of interest in the ground and excited state [1,2], and ideally in real time [3,4]. Among all the advanced molecular vibrational spectroscopic toolsets, femtosecond-stimulated Raman spectroscopy (FSRS) is a relative newcomer since the early 2000s and a promising structural dynamics technique that can simultaneously achieve high time resolution (

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