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J Gen Physiol
1997 Nov 01;1105:579-89. doi: 10.1085/jgp.110.5.579.
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Correlation between charge movement and ionic current during slow inactivation in Shaker K+ channels.
Olcese R
,
Latorre R
,
Toro L
,
Bezanilla F
,
Stefani E
.
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Prolonged depolarization induces a slow inactivation process in some K+ channels. We have studied ionic and gating currents during long depolarizations in the mutant Shaker H4-Delta(6-46) K+ channel and in the nonconducting mutant (Shaker H4-Delta(6-46)-W434F). These channels lack the amino terminus that confers the fast (N-type) inactivation (Hoshi, T., W.N. Zagotta, and R.W. Aldrich. 1991. Neuron. 7:547-556). Channels were expressed in oocytes and currents were measured with the cut-open-oocyte and patch-clamp techniques. In both clones, the curves describing the voltage dependence of the charge movement were shifted toward more negative potentials when the holding potential was maintained at depolarized potentials. The evidences that this new voltage dependence of the charge movement in the depolarized condition is associated with the process of slow inactivation are the following: (a) the installation of both the slow inactivation of the ionic current and the inactivation of the charge in response to a sustained 1-min depolarization to 0 mV followed the same time course; and (b) the recovery from inactivation of both ionic and gating currents (induced by repolarizations to -90 mV after a 1-min inactivating pulse at 0 mV) also followed a similar time course. Although prolonged depolarizations induce inactivation of the majority of the channels, a small fraction remains non-slow inactivated. The voltage dependence of this fraction of channels remained unaltered, suggesting that their activation pathway was unmodified by prolonged depolarization. The data could be fitted to a sequential model for Shaker K+ channels (Bezanilla, F., E. Perozo, and E. Stefani. 1994. Biophys. J. 66:1011-1021), with the addition of a series of parallel nonconducting (inactivated) states that become populated during prolonged depolarization. The data suggest that prolonged depolarization modifies the conformation of the voltage sensor and that this change can be associated with the process of slow inactivation.
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9348329
???displayArticle.pmcLink???PMC2229383 ???displayArticle.link???J Gen Physiol ???displayArticle.grants???[+]
Figure 1. N- and C-type inactivation in Shaker channels. (A) Shaker H4: pulses from â60 to 10 mV in 10-mV steps. Note the fast decay of the K+ current due to the N-type inactivation. (B) Shaker H4-Î: pulses from â80 to 30 mV in 10-mV steps. The deletion of the amino acids 6â46 (Shaker H4-Î) completely removes the fast inactivating properties of the channel. (C) Shaker H4-Î: long pulses (18 s) from â40 to 20 mV in 10-mV steps. Long depolarizing pulses make evident the presence of a slow inactivation process. COVG technique, external isotonic Na-MES.
Figure 2. Steady state inactivation properties of Shaker H4-Î. (A) Effect of the HP (â70 and â30 mV) on K+ currents recorded with the COVG technique in isotonic K-MES. Pulses between â70 and 17 mV in 3-mV steps from the tested HP were applied. Tail currents were measured at the end of these pulses at a repolarization potential to â50 mV. The oocyte was maintained at each holding potential for 1 min before running the stimulating protocol with low frequency stimulating pulses to prevent their effect on the inactivation (e.g., a pulse every 1 s at â70 mV and every 5 s at 0 mV HPs). Linear components were subtracted after the stimulating run with P/1 from a subtracting holding potential 70 mV more negative than the tested HP and were between â140 and â53 mV with 3-mV increments. (B) G-V curves with the protocol shown in A from the same oocyte at different HPs: â¦, â90; â¡, â70; âª, â60; âµ, â50; â´, â40; â, â30 mV. (C) Normalized G-V curves. (D) Steady state inactivation curve obtained from tail current amplitude at â50 mV after a depolarizing pulse to â1 mV. Experimental points were fitted to Gm = Gmin + Gmax/{1 + exp[âz(V1/2 â Vm)F/RT]}. The fitted values were: Gmax = 0.17 mS, Gmin = 0.007 mS, V1/2 = â38.5 mV and z = 7.2.
Figure 3. Gating currents from â90 and 0 mV HPs in the conducting Shaker Î. The oocyte interior was perfused with isotonic NMG-MES up to the complete elimination of K+ currents. The external solution was isotonic NMG-MES Ca-(MES)2. Unsubtracted gating currents; linear components were analogically compensated with the amplifier transient cancellation at 20 mV HP. (A and B) Current traces from â90 and 0 mV HP, respectively. The cell was maintained at 0 mV HP for 1 min; pulse stimulation was every 1 s at 0 mV and every 0.5 s at â90 mV HP. (C) Q-V curves obtained by integrating the ON gating currents to different test potentials from â90 (âª) and 0 (â¢) mV HP. (D) Q-V curves from C replotted defining Q = 0 at the extreme negative potential for both HPs. The total charge moved is the same at both HPs, but holding the membrane potential at 0 mV induces an â¼50-mV shift to more negative potentials of the Q-V curve.
Figure 4. Gating currents from â90 and 0 mV HP in the nonconducting mutant Shaker Î-W434F. Same protocol and ionic conditions as in Fig. 3, A and B. Unsubtracted gating currents from â90 and 0 mV HP, respectively. (C) Q-V curve with the absolute charge values. The total charge moved is the same at both HPs. Holding the membrane potential at 0 mV induces an â¼25-mV shift to the more negative potential of the Q-V curve.
Figure 5. Correlation between the time course of installation of C-type inactivation and time course of changes in charge movement. (A) Shaker H4-Î-W434F upper trace is the pulse protocol, remaining traces are unsubtracted gating currents. Linear components were analogically compensated with the amplifier transient cancellation at 20 mV HP. Numbers preceding the traces are the duration of the conditioning pulse to 0 mV. The â90 mV HP was held for 1 min between each stimulating pulse to fully recover from the inactivation. Note that increasing the duration of the conditioning pulse to 0 mV induces a reduction in the charge movement measured for a pulse from 0 to â60 mV. (B) Shaker H4-Î. Time course of the ionic current during 1-min depolarizing pulse to 0 mV. (C, symbols) Normalized charge movement (from 0 to â60 mV, from records of the type shown in A as a function of the inactivating prepulse. (wide trace) Time course of ionic current during a pulse to 0 mV (as shown in B). Data are normalized to their minima and maxima and fitted to the sum of two exponential functions (narrow trace) constraining the two time constants to be the same for ionic and gating current data: Ïfast = 4.1 s, Ïslow = 24 s. The ratios between the fast and slow components for charge movement and ionic current were 2.15 and 3.7, respectively. COVG technique in external isotonic Na-MES. Error bars are SEM (n = 6).
Figure 6. Correlation between the time course of recovery of slow inactivation and of changes in charge movement. (A) Shaker H4-Î-W434F. Upper trace is the pulse protocol, remaining traces are unsubtracted gating currents. Linear components were analogically compensated with the amplifier transient cancellation at 20 mV HP. Numbers preceding the traces are the duration of the conditioning pulse to â90 mV. The 0 mV HP was held for 1 min between each stimulating pulse to fully slow inactivate the channels. Note that increasing the duration of the conditioning pulse to â90 mV induces an increase of the charge movement measured for a pulse from â90 to â20 mV. (B) Shaker H4-Î. Similar protocol as in A to investigate the recovery of the ionic current from slow inactivation. Upper trace is the pulse protocol, remaining traces are unsubtracted K+ currents for a test pulse from â90 to â20 mV. The durations of the conditioning pulses to â90 mV are shown next to the traces. (C) Simultaneous fit to normalized charge movement (from â90 to â20 mV as in A) and ionic current during the same voltage step as shown in B. Averaged data (â¢, charge, n = 3; and â´, ionic current, n = 3) were fitted to the sum of two exponential functions with the same two time constants but with different amplitudes: Ïfast = 0.01 s, Ïslow = 1.1 s. The ratios between the fast and slow components for charge movement and ionic current were 0.46 and 0.43, respectively. Data points are normalized to their minima and maxima. COVG technique in external isotonic Na-MES.
Figure 7. Cs+ currents in Shaker H4-Î. (A) Membrane currents in cell-attached mode from an oocyte in which the internal medium was equilibrated with isotonic Cs-MES. The pipette was filled with isotonic 2 mM Cs-MES CaCl2, â90 mV HP. Pulse protocol (top): pulses were from â80 to 60 mV in 20-mV increments. Linear components were subtracted with P/â4 protocol from â90 mV subtracting HP. (B) I-V relationship from the experiment in A. The reversal potential for Cs+ is 0 mV.
Figure 8. Ionic and gating current of Shaker H4-Î recover from slow inactivation with the same course. Same conditions as in Fig. 7. (A) Current traces in isotonic Cs-MES obtained pulsing to the reversal potential for Cs+ (0 mV). The channels were inactivated at 0 mV for 1 min and recovered with different pulse duration to â90 mV. Note that increasing the duration of the conditioning pulse to â90 mV produces an increase of the charge movement measured for a pulse from â90 to 0 mV, and a parallel increase in the tail current at the repolarizing potential (â90 mV). (B) Time course of the recovery of ionic current and gating charge. Simultaneous fit to normalized charge movement (from â90 to 0 mV as in A) and peak tail current during the repolarization to â90 mV. Data (ionic current ⢠and charge â´, normalized to their minima and maxima) were fitted to the sum of two exponential functions (continuous line) with the same time constants and different amplitudes: Ïfast = 0.28 s, Ïslow = 6.47 s. The ratios between the fast and slow components for charge movement and ionic current were 2.33 and 1.35, respectively.
Figure 9. Effect of intermediate holding potentials on the charge movement. COVG technique in isotonic Na-MES. (A) Normalized Q(V) curves from the same oocyte obtained from HPs ranging from â90 to 0 mV as indicated. Continuous lines are the fits to a sum of two Boltzmann distributions in the form of: Qon/Qâmax = Qâ1/Qmax/{1 + exp[z1(V1half â Vm)F/RT]} + Qâ2/Qmax/{1 + exp[z2(V2half â Vm)F/RT]} where Qâmax is the maximum charge movement, Qâ1 and Qâ2 are the amplitudes of the charge components, z1 and zâ2 are the effective valences and V1half and V2half, the respective half activation potentials; F, R, and T are the usual thermodynamic constants. The fitting was performed to obtain the same effective valences (z1 and zâ2) for all the Q-V curves and different amplitude and half activation potentials. The effective valences (z) were 2.9 for the first, more negative component, and 4.4 for the second component of the Q-Vs. The half activation potentials (V1half and V2half) and the amplitudes Qâ1 and Qâ2 for all the Q-V curves are plotted as a function of the holding potential in B and C, respectively. *Data points are from a different oocyte.
Armstrong,
Inactivation of the sodium channel. II. Gating current experiments.
1977, Pubmed
Armstrong,
Inactivation of the sodium channel. II. Gating current experiments.
1977,
Pubmed
Bezanilla,
Distribution and kinetics of membrane dielectric polarization. 1. Long-term inactivation of gating currents.
1982,
Pubmed
Bezanilla,
Gating of Shaker K+ channels: II. The components of gating currents and a model of channel activation.
1994,
Pubmed
,
Xenbase
Bezanilla,
Molecular basis of gating charge immobilization in Shaker potassium channels.
1991,
Pubmed
,
Xenbase
Choi,
Tetraethylammonium blockade distinguishes two inactivation mechanisms in voltage-activated K+ channels.
1991,
Pubmed
De Biasi,
Inactivation determined by a single site in K+ pores.
1993,
Pubmed
Ehrenstein,
Slow changes of potassium permeability in the squid giant axon.
1966,
Pubmed
Fedida,
Slow gating charge immobilization in the human potassium channel Kv1.5 and its prevention by 4-aminopyridine.
1996,
Pubmed
HODGKIN,
A quantitative description of membrane current and its application to conduction and excitation in nerve.
1952,
Pubmed
Hoshi,
Two types of inactivation in Shaker K+ channels: effects of alterations in the carboxy-terminal region.
1991,
Pubmed
,
Xenbase
Hoshi,
Biophysical and molecular mechanisms of Shaker potassium channel inactivation.
1990,
Pubmed
,
Xenbase
Kamb,
Molecular characterization of Shaker, a Drosophila gene that encodes a potassium channel.
1987,
Pubmed
Liu,
Dynamic rearrangement of the outer mouth of a K+ channel during gating.
1996,
Pubmed
López-Barneo,
Effects of external cations and mutations in the pore region on C-type inactivation of Shaker potassium channels.
1993,
Pubmed
,
Xenbase
Noceti,
Effective gating charges per channel in voltage-dependent K+ and Ca2+ channels.
1996,
Pubmed
,
Xenbase
Ogielska,
Cooperative subunit interactions in C-type inactivation of K channels.
1995,
Pubmed
,
Xenbase
Olcese,
Correlation between charge movement and ionic current during slow inactivation in Shaker K+ channels.
1997,
Pubmed
,
Xenbase
Panyi,
C-type inactivation of a voltage-gated K+ channel occurs by a cooperative mechanism.
1995,
Pubmed
Perozo,
Gating currents from a nonconducting mutant reveal open-closed conformations in Shaker K+ channels.
1993,
Pubmed
Stefani,
Gating of Shaker K+ channels: I. Ionic and gating currents.
1994,
Pubmed
,
Xenbase
Yellen,
An engineered cysteine in the external mouth of a K+ channel allows inactivation to be modulated by metal binding.
1994,
Pubmed
Zagotta,
Restoration of inactivation in mutants of Shaker potassium channels by a peptide derived from ShB.
1990,
Pubmed
,
Xenbase
Zagotta,
Gating of single Shaker potassium channels in Drosophila muscle and in Xenopus oocytes injected with Shaker mRNA.
1989,
Pubmed
,
Xenbase
