Probing Energy Landscapes of Cytochrome b 6 f with Spectral Hole Burning: Effects of Deuterated Solvent and Detergent

• Published in: The journal of physical chemistry. B Vol. 121; no. 42; pp. 9848 - 9858
• Main Authors: Levenberg, Alexander, Shafiei, Golia, Lujan, Maria A, Giannacopoulos, Steven, Picorel, Rafael, Zazubovich, Valter
• Format: Journal Article
• Language: English
• Published: United States American Chemical Society 26.10.2017
• ISSN: 1520-6106; 1520-5207
• DOI: 10.1021/acs.jpcb.7b07686

In non-photochemical spectral hole burning (NPHB) and spectral hole recovery experiments, cytochrome b 6 f protein exhibits behavior that is almost independent of the deuteration of the buffer/glycerol glassy matrix containing the protein, apart from some differences in heat dissipation. On the other hand, strong dependence of the hole burning properties on sample preparation procedures was observed and attributed to a large increase of the electron–phonon coupling and shortening of the excited-state lifetime occurring when n-dodecyl β-d-maltoside (DM) is used as a detergent instead of n-octyl β-d-glucopyranoside (OGP). The data was analyzed assuming that the tunneling parameter distribution or barrier distribution probed by NPHB and encoded into the spectral holes contains contributions from two nonidentical components with accidentally degenerate excited state λ-distributions. Both components likely reflect protein dynamics, although with some small probability one of them (with larger md 2) may still represent the dynamics involving specifically the −OH groups of the water/glycerol solvent. Single proton tunneling in the water/glycerol solvent environment or in the protein can be safely excluded as the origin of observed NPHB and hole recovery dynamics. The intensity dependence of the hole growth kinetics in deuterated samples likely reflects differences in heat dissipation between protonated and deuterated samples. These differences are most probably due to the higher interface thermal resistivity between (still protonated) protein and deuterated water/glycerol outside environment.