Localization of the K+ lock-in and the Ba2+ binding sites in a voltage-gated calcium-modulated channel: Implications for survival of K+ permeability

Abstract

Using Ba2 1 as a probe, we performed a detailed characterization of an external K 1 binding site located in the pore of a large conductance Ca2 1-activated K 1 (BKCa) channel from skeletal muscle incorporated into planar lipid bilayers. Internal Ba2 1 blocks BKCa channels and decreasing external K 1 using a K 1 chelator, ( 1)-18- Crown-6-tetracarboxylic acid, dramatically reduces the duration of the Ba2 1-blocked events. Average Ba2 1 dwell time changes from 10 s at 10 mM external K 1 to 100 ms in the limit of very low [K 1]. Using a model where external K 1 binds to a site hindering the exit of Ba2 1 toward the external side (Neyton, J., and C. Miller. 1988. J. Gen. Physiol. 92:549–568), we calculated a dissociation constant of 2.7 mM for K 1 at this lock-in site. We also found that BKCa channels enter into a long-lasting nonconductive state when the external [K 1] is reduced below 4 mM using the crown ether. Channel activity can be recovered by adding K 1, Rb 1, Cs 1, or NH4 1 to the external solution. These results suggest that the BKCa channel stability in solutions of very low [K 1] is due to K 1 binding to a site having a very high affinity. Occupancy of this site by K 1 avoids the channel conductance collapse and the exit of Ba2 1 toward the external side. External tetraethylammonium also reduced the Ba2 1 off rate and impeded the channel from entering into the long-lasting nonconductive state. This effect requires the presence of external K 1. It is explained in terms of a model in which the conduction pore contains Ba2 1, K 1, and tetraethylammonium simultaneously, with the K 1 binding site located internal to the tetraethylammonium site. Altogether, these results and the known potassium channel structure (Doyle, D.A., J.M. Cabral, R.A. Pfuetzner, A. Kuo, J.M. Gulbis, S.L. Cohen, B.T. Chait, and R. MacKinnon. 1998. Science. 280:69–77) imply that the lock-in site and the Ba2 1 sites are the external and internal ion sites of the selectivity filter, respectively.