![Author ORCID: We display the ORCID iD icon alongside authors names on our website to acknowledge that the ORCiD has been authenticated when entered by the user. To view the users ORCiD record click the icon. [opens in a new tab]](https://chemrxiv.org/engage/assets/public/chemrxiv/images/logos/orcid.png)
Abstract
Protein motion is central to enzymatic catalysis but the influence of femtosecond – picosecond timescale fluctuations on chemical reaction steps remains poorly understood. One barrier to uniting experiment and theory is difficulty in resolving the dynamics of configurational sub-populations in an ensemble. Here we use ultrafast two-dimensional infrared (2D IR) spectroscopy to examine the fluctuations about a vibrationally labeled substrate analog linked to the active site of Pyrococcus horikoshii ene-reductase (PhENR) in two orientations mimicking proposed reactive and inactive reactant states. Frequency fluctuation correlation functions (FFCFs) derived from 2D IR experiments show a near-quantitative tradeoff between fast (<1 ps) and slow (>5 ps) motions upon rotation of the analog. Increased dynamical heterogeneity and a unique ~10 cm-1 oscillation are also observed in the putative reactive configuration. These observations suggest divergent dynamics among distinct reactant state sub-populations and establish PhENR as a useful model system for continued studies.
Supplementary materials
Title
Supporting information.
Description
Detailed description of experimental methods and data processing. Inhibitor binding analysis using UV-vis spectroscopy. FTIR and 2D IR spectra of the free 4CN-M label. C≡N vibrational lifetimes of PhENR varaints. Simulated linear responses from FFCF parameters.
Actions
