Kinetics of the Terminal Electron Transfer Step in Cytochrome c Oxidase

Cytochrome c oxidase (cco) catalyzes the oxygen reduction reaction in most aerobically respiring organisms. Decades of research have uncovered many aspects relating to structure and function of this enzyme. However, the origin of the unusually fast terminal electron transfer step from heme a to heme...

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Bibliographic Details
Published inThe journal of physical chemistry. B Vol. 116; no. 6; pp. 1876 - 1883
Main Authors Tipmanee, Varomyalin, Blumberger, Jochen
Format Journal Article
LanguageEnglish
Published United States American Chemical Society 16.02.2012
Subjects
cytochrome-c oxidase
Cytochromes
Electron transfer
Electron Transport
Electron Transport Complex IV - chemistry
Electron Transport Complex IV - metabolism
Electronics
Electrons
equations
Free energy
Gibbs free energy
heme
Heme - chemistry
Kinetics
Mathematical analysis
molecular dynamics
Molecular Dynamics Simulation
Oxidase
Oxidation-Reduction
oxygen
Protein Structure, Tertiary
Proteins
temperature
Terminals
Thermodynamics
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Summary:Cytochrome c oxidase (cco) catalyzes the oxygen reduction reaction in most aerobically respiring organisms. Decades of research have uncovered many aspects relating to structure and function of this enzyme. However, the origin of the unusually fast terminal electron transfer step from heme a to heme a3 in cco has been the subject of intense discussions over recent years. Yet, no satisfactory consensus has been achieved. Carrying out large-scale molecular dynamics simulation of the protein embedded in a solvated membrane, we obtain a reorganization free energy λ = 0.57 eV. Evaluation of the quantized single-mode rate equation using the experimental rate and the computed reorganization free energy gives a value of 1.5 meV for the average electronic coupling (H ab) between heme a and heme a3. Thus, according to our calculations, the nanosecond electron transfer (ET) is due to a small but significant activation barrier (ΔG ‡ = 0.12 eV) in combination with effective electronic coupling between the two cofactors. The activation free energy is caused predominantly by collective reorganization of protein residues. We show that our results are consistent with the weak temperature dependence observed in experiment if one allows for very minor variations in the donor–acceptor distance as the temperature changes.
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ISSN:1520-6106
1520-5207
1520-5207
DOI:10.1021/jp209175j