Inhibition of KCa2.2 and KCa2.3 channel currents by protonation of outer pore histidine residues

doi:10.1085/jgp.200910252

Scientifica: Experts in Electrophysiology

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doi:10.1085/jgp.200910252
The Journal of General Physiology, Vol. 134, No. 4, 295-308
The Rockefeller University Press, 0022-1295 $30.00
© Goodchild et al.

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ARTICLE

Inhibition of K_Ca2.2 and K_Ca2.3 channel currents by protonation of outer pore histidine residues

Samuel J. Goodchild¹, Cedric Lamy², Vincent Seutin², and Neil V. Marrion¹

¹ Department of Physiology and Pharmacology, School of Medical Sciences, University of Bristol, Bristol BS8 1TD, England, UK
² Laboratory of Pharmacology, Giga-Neurosciences, University of Liège, 4000 Liège, Belgium

Correspondence to Neil V. Marrion: N.V.Marrion{at}bris.ac.uk

Ion channels are often modulated by changes in extracellularpH, with most examples resulting from shifts in the ionizationstate of histidine residue(s) in the channel pore. The applicationof acidic extracellular solution inhibited expressed K_Ca2.2(SK2) and K_Ca2.3 (SK3) channel currents, with K_Ca2.3 (pIC₅₀of $~$ 6.8) being approximately fourfold more sensitive than K_Ca2.2(pIC₅₀ of $~$ 6.2). Inhibition was found to be voltage dependent,resulting from a shift in the affinity for the rectifying intracellulardivalent cation(s) at the inner mouth of the selectivity filter.The inhibition by extracellular protons resulted from a reductionin the single-channel conductance, without significant changesin open-state kinetics or open probability. K_Ca2.2 and K_Ca2.3subunits both possess a histidine residue in their outer poreregion between the transmembrane S5 segment and the pore helix,with K_Ca2.3 also exhibiting an additional histidine residuebetween the selectivity filter and S6. Mutagenesis revealedthat the outer pore histidine common to both channels was criticalfor inhibition. The greater sensitivity of K_Ca2.3 currents toprotons arose from the additional histidine residue in the pore,which was more proximal to the conduction pathway and in theelectrostatic vicinity of the ion conduction pathway. The decreaseof channel conductance by extracellular protons was mimickedby mutation of the outer pore histidine in K_Ca2.2 to an asparagineresidue. These data suggest that local interactions involvingthe outer turret histidine residues are crucial to enable highconductance openings, with protonation inhibiting current bychanging pore shape.

V. Seutin and N.V. Marrion contributed equally to this paper.

Abbreviations: GHK, Goldman-Hodgkin-Katz

© 2009 Goodchild et al.
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