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Published online Feb 28 2005. doi:10.1085/jgp.200409239
The Rockefeller University Press, 0022-1295 $8.00
JGP, Volume 125, Number 3, 273-286
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Divalent Cation Sensitivity of BK Channel Activation Supports the Existence of Three Distinct Binding Sites

Xu-Hui Zeng1, Xiao-Ming Xia1, and Christopher J. Lingle1,2

1 Department of Anesthesiology, Washington University School of Medicine, St. Louis, Missouri 63110
2 Department of Anatomy and Neurobiology, Washington University School of Medicine, St. Louis, Missouri 63110

Correspondence to Chris Lingle: clingle{at}morpheus.wustl.edu

Mutational analyses have suggested that BK channels are regulated by three distinct divalent cation-dependent regulatory mechanisms arising from the cytosolic COOH terminus of the pore-forming {alpha} subunit. Two mechanisms account for physiological regulation of BK channels by µM Ca2+. The third may mediate physiological regulation by mM Mg2+. Mutation of five aspartate residues (5D5N) within the so-called Ca2+ bowl removes a portion of a higher affinity Ca2+ dependence, while mutation of D362A/D367A in the first RCK domain also removes some higher affinity Ca2+ dependence. Together, 5D5N and D362A/D367A remove all effects of Ca2+ up through 1 mM while E399A removes a portion of low affinity regulation by Ca2+/Mg2+. If each proposed regulatory effect involves a distinct divalent cation binding site, the divalent cation selectivity of the actual site that defines each mechanism might differ. By examination of the ability of various divalent cations to activate currents in constructs with mutationally altered regulatory mechanisms, here we show that each putative regulatory mechanism exhibits a unique sensitivity to divalent cations. Regulation mediated by the Ca2+ bowl can be activated by Ca2+ and Sr2+, while regulation defined by D362/D367 can be activated by Ca2+, Sr2+, and Cd2+. Mn2+, Co2+, and Ni2+ produce little observable effect through the high affinity regulatory mechanisms, while all six divalent cations enhance activation through the low affinity mechanism defined by residue E399. Furthermore, each type of mutation affects kinetic properties of BK channels in distinct ways. The Ca2+ bowl mainly accelerates activation of BK channels at low [Ca2+], while the D362/D367-related high affinity site influences both activation and deactivation over the range of 10–300 µM Ca2+. The major kinetic effect of the E399-related low affinity mechanism is to slow deactivation at mM Mg2+ or Ca2+. The results support the view that three distinct divalent-cation binding sites mediate regulation of BK channels.

Key Words: BK channels • Ca2+ regulatory sites • divalent cations • Slo • activation


Abbreviation used in this paper: RCK, regulatory of conductance for K+.


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