![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
Horseradish peroxidase (HRP) is an important enzyme for industrial purposes due to its ability to oxidize pollutants from wastewater. A previous report indicated that peroxidases can have up to a 20% increase in the initial enzymatic activity in an aqueous solution of 0.26 M 1-Ethyl-3-methylimidazolium ethyl sulfate ([EMIm][EtSO4]) at neutral pH. However, the atomistic details of how the solution affects peroxidase activity remain elusive. In the enzymatic landscape of HRP, an intermediate termed Compound II (Cpd II) plays a key role and involves a histidine (H42) residue that may take different protonation states. Cpd II displays structural versatility, existing as oxo-ferryl (2a) or hydroxo-ferryl (2b(FeIV)) forms, where 2a is the predominantly observed form in experimental studies. Intriguingly, the ferric 2b(FeIII) form seen in synthetic complexes, has not been observed in HRP. Here, we have investigated the structure and dynamics of HRP in pure water and aq. [EM-Im][EtSO4] (0.26 M), as well as the reaction mechanism of Cpd II catalyzed conversion of 2a to 2b using polarizable molecular dynamics (MD) and quantum mechanics/molecular mechanics (QM/MM) calculations. When HRP is solvated in aq. [EMIm][EtSO4] a significant reduction in the fluctuation of residues 70, 71 and 74 is observed. This reduction is due to the migration of EtSO4– ions close to this region, which results in structural changes in the active site; including the displacement of the catalytic water, and orientation of H42 directly over the ferryl moiety. This configuration of the active site leads to a direct proton transfer (PT) with a significant energy reduction in the reaction barrier. Conversely, in neat water, the reaction for 2a to 2b follows the previously reported mechanism where H42+ transfers a proton to the ferryl moiety via an ordered water in the active site. We further investigated an alternative path with the deprotonated form of H42, where the mechanism shifts to hydrogen atom transfer (HAT), with similar reaction barrier differences between the aqueous and aqueous/IL mixture, albeit with significantly higher relative barriers. Analysis of the electric fields at the active site indicate that the aq. [EMIm][EtSO4] medium facilitate the reaction by providing a more favorable environment compared with the system solvated in neat water. Overall, our calculations provide atomic-level insights that help explain the observed improvement in activity for peroxidases in IL solution, and underscore the importance of favorable electric fields in the active site to promote catalysis.
Supplementary materials
Title
Supporting Information for Impact of an Ionic Liquid Solution on Horseradish Peroxidase Activity
Description
RMSF by residues for Water(H42) and Water/IL(H42), root
mean squared fluctuation difference (ΔRMSF) analysis, radial distribution function in Water/IL(H42) system, non-covalent interactions in the active site at the critical points in Water(H42) and Water/IL(H42) systems, elbow plot for k-means clustering, QM/MM energies for singlet and triplet states of the reactant and products, relative energies corresponding to reaction paths, spin density and ESP charges analysis, LOBA, ELF analysis, distance analysis for the Water(H42) and Water/IL systems. (PDF)
Actions
Title
Electronic Supporting Information for Impact of an Ionic Liquid Solution on Horseradish Peroxidase Activity
Description
Newly generated parameters, input coordinates for MD simulations, QM/MM input files, and QM/MM reaction paths, movies of MEPs.
Actions
