Molecular basis of proton uptake in single and double mutants of cytochromec oxidase

Rowan M Henry; David Caplan; Elisa Fadda; Régis Pomès

doi:10.1088/0953-8984/23/23/234102

Journal of Physics: Condensed Matter

Molecular basis of proton uptake in single and double mutants of cytochrome c oxidase

Rowan M Henry^1,2, David Caplan^1,2, Elisa Fadda³ and Régis Pomès^1,2

Published 25 May 2011 • IOP Publishing Ltd
Journal of Physics: Condensed Matter, Volume 23, Number 23 Citation Rowan M Henry et al 2011 J. Phys.: Condens. Matter 23 234102 DOI 10.1088/0953-8984/23/23/234102

Download Article PDF

Article metrics

311 Total downloads

Submit

Submit to this Journal

Permissions

Get permission to re-use this article

Author affiliations

¹ Molecular Structure and Function, Hospital for Sick Children, Toronto, ON, M5G 1X8, Canada

² Department of Biochemistry, University of Toronto, Toronto, ON, M5S 1A8, Canada

³ Department of Chemistry, University of Galway, Ireland

⁴ Address for correspondence: Molecular Structure and Function, Hospital for Sick Children, 555 University Avenue, Toronto, ON, M5G 1X8, Canada

Dates

Received 10 December 2010
Published 25 May 2011

Buy this article in print

Journal RSS

Abstract

Cytochrome c oxidase, the terminal enzyme of the respiratory chain, utilizes the reduction of dioxygen into water to pump protons across the mitochondrial inner membrane. The principal pathway of proton uptake into the enzyme, the D channel, is a 2.5 nm long channel-like cavity named after a conserved, negatively charged aspartic acid (D) residue thought to help recruiting protons to its entrance (D132 in the first subunit of the S. sphaeroides enzyme). The single-point mutation of D132 to asparagine (N), a neutral residue, abolishes enzyme activity. Conversely, replacing conserved N139, one-third into the D channel, by D, induces a decoupled phenotype, whereby oxygen reduction proceeds but not proton pumping. Intriguingly, the double mutant D132N/N139D, which conserves the charge of the D channel, restores the wild-type phenotype. We use molecular dynamics simulations and electrostatic calculations to examine the structural and physical basis for the coupling of proton pumping and oxygen chemistry in single and double N139D mutants. The potential of mean force for the conformational isomerization of N139 and N139D side chains reveals the presence of three rotamers, one of which faces the channel entrance. This out-facing conformer is metastable in the wild-type and in the N139D single mutant, but predominant in the double mutant thanks to the loss of electrostatic repulsion with the carboxylate group of D132. The effects of mutations and conformational isomerization on the pKa of E286, an essential proton-shuttling residue located at the top of the D channel, are shown to be consistent with the electrostatic control of proton pumping proposed recently (Fadda et al 2008 Biochim. Biophys. Acta 1777 277–84). Taken together, these results suggest that preserving the spatial distribution of charges at the entrance of the D channel is necessary to guarantee both the uptake and the relay of protons to the active site of the enzyme. These findings highlight the interplay of long-range electrostatic forces and local structural fluctuations in the control of proton movement and provide a physical explanation for the restoration of proton pumping activity in the double mutant.

Export citation and abstract BibTeX RIS

Previous article in issue

Next article in issue

Please wait… references are loading.