Iberiotoxin

Cerebellar Purkinje cells (PCs) are the sole output neurons of the cerebellar cortex. Mature PCs discharge either tonically Na+ spikes or bursts of Na+ spikes ending to a Ca2+ spike. These cells express inactivating and non-inactivating large conductance Ca2+ -dependent K+ (BK) channels in their soma and dendrites. Somatic intracellular recording of acutely prepared brain slices was performed to examine the role of BK channels-mediated current in the tonic and burst firing of PCs. Continuous injection of a negative DC current was used to both suppress the spontaneous activity and stabilize the resting membrane potential around -70 mV. Then, the short depolarizing current injection was used to evoke spike discharge. For establishing of the burst firing, 4-aminopyridine (4-AP) was bath applied to the bath solution. Blockade of BK channels with iberiotoxin (IbTx); a specific blocker of BK channels, did not affect the Na+ spike configuration in the tonic firing but caused a remarkable change in the shape of Na+ and Ca2+ spikes in 4-AP-induced burst. Our results showed that during the burst firing, strong activation of IbTx-sensitive BK channels enhances the amplitude of fast afterhyperpolarization while decreases the duration of both Na+ and Ca2+ spikes. The current from these channels contributes to both the repolarizing of Na+ spike in the burst and setting of the amplitude of post-pulse AHP that occurs immediately after a depolarizing pulse. These data reveal an important role of IbTx-sensitive BK current in regulating of the spike configuration during the burst firing of PCs.

The role which Ca(2+)-activated K(+) (K(Ca)) channels play in regulating acetylcholine (ACh) release was examined at mouse motor nerve terminals. In particular, the ability of the antagonist iberiotoxin to recruit normally silent L-type Ca(2+) channels to participate in nerve-evoked release was examined using conventional intracellular electrophysiological techniques. Incubation of cut hemidiaphragm preparations with 10 microM nimodipine, a dihydropyridine L-type Ca(2+) channel antagonist, had no significant effect on quantal content of end-plate potentials. Nevertheless, 1 microM S-(-)-1,4-dihydro-2,6-dimethyl-5-nitro-4-(2-[trifluoromethyl]phenyl)-3-pyridine carboxylic acid methyl ester (Bay K 8644) enhanced quantal content to 134.7 +/- 3.5% of control. Iberiotoxin (150 nM) increased quantal content to 177.5 +/- 9.9% of control, whereas iberiotoxin plus nimodipine increased quantal content to only 145.7 +/- 10.4% of control. Coapplication of 1 microM Bay K 8644 with iberiotoxin did not significantly increase quantal content further than did treatment with iberiotoxin alone. The effects of iberiotoxin and nimodipine alone or in combination on the miniature end-plate potential (MEPP) frequency following KCl-induced depolarization were examined using uncut hemidiaphragm preparations. Nimodipine alone had no effect on MEPP frequency from preparations incubated in physiological saline containing 5 to 20 mM KCl. Moreover, iberiotoxin alone or combined with nimodipine also had no effect on MEPP frequency in physiological salines containing 5 to 15 mM KCl. At 20 mM KCl, however, iberiotoxin significantly increased MEPP frequency to 125.6% of iberiotoxin-free values; combined treatment with nimodipine and iberiotoxin prevented this increase in MEPP frequency. Thus, loss of functional K(Ca) channels unmasks normally silent L-type Ca(2+) channels to participate in ACh release from motor nerve terminals, particularly under conditions of intense nerve terminal depolarization.

Iberiotoxin (IbTX or alpha-KTx 1.3), a selective, high-affinity blocker of the large-conductance, calcium-activated (maxi-K) channel, exhibits a unique, asymmetric distribution of charge. To test how these charges control kinetics of IbTX binding, we generated five mutants at two positions, K27 and R34, that are highly conserved among other isotoxins. The dissociation and association rate constants, koff and kon, were determined from toxin-blocked and -unblocked durations of single maxi-K channels incorporated into planar lipid bilayers. Equilibrium dissociation constant (Kd) values were calculated from koff/kon. The IbTX mutants K27N, K27Q, and R34N caused large increases in Kd values compared to wild-type, suggesting that the IbTX interaction surface encompasses these residues. A well-established pore-blocking mechanism for IbTX predicts a voltage dependence of toxin-blocked times following occupancy of a potassium binding site in the channel pore. Time constants for block by K27R were approximately 5-fold slower at -20 mV versus +40 mV, while neutralization of K27 relieved the voltage dependence of block. This suggests that K27 in IbTX interacts with a potassium binding site in the pore. Neutralized mutants of K27 and R34, with zero net charge, displayed toxin association rate constants approximately 10-fold slower than wild-type. Association rates for R34N diminished approximately 19-fold when external potassium was increased from 30 to 300 mM. These findings suggest that simple net charge and diffusional processes do not control ingress of IbTX into the channel vestibule.