Calcium Influx via L- and N-Type Calcium Channels Activates a Transient Large-Conductance Ca2+-Activated K+ Current in Mouse Neocortical Pyramidal Neurons

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The Journal of Neuroscience, May 1, 2003, 23(9):3639

Calcium Influx via L- and N-Type Calcium Channels Activates a Transient Large-Conductance Ca²⁺-Activated K⁺ Current in Mouse Neocortical Pyramidal Neurons
Xiaolu Sun¹^,³, Xiang Q. Gu¹^,³, and Gabriel G. Haddad¹^,²^,³^,⁴
Departments of ¹ Pediatrics (Section of Respiratory Medicine) and ² Cellular and Molecular Physiology, Yale University School of Medicine, New Haven, Connecticut 06520, and Departments of ³ Pediatrics (Section of Respiratory Medicine) and ⁴ Neuroscience, Albert Einstein College of Medicine, Bronx, New York 10461

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Ca²⁺-activated K⁺ currents and their Ca²⁺ sources through high-threshold voltage-activated Ca²⁺ channels were studied using whole-cell patch-clamp recordingsfrom freshly dissociated mouse neocortical pyramidal neurons.In the presence of 4-aminopyridine, depolarizing pulses evokedtransient outward currents and several components of sustainedcurrents in a subgroup of cells. The fast transient current anda component of the sustained currents were Ca²⁺ dependent and sensitive to charybdotoxin and iberiotoxin butnot to apamin, suggesting that they were mediated by large-conductanceCa²⁺-activated K⁺ (BK) channels. Thus, mouse neocortical neurons contain both inactivatingand noninactivating populations of BK channels. Blockade of eitherL-type Ca²⁺ channels by nifedipine or N-type Ca²⁺ channels by $omega$ -conotoxin GVIA reduced the fast transient BK current.These data suggest that the transient BK current is activatedby Ca²⁺ entry through both N- and L-type Ca²⁺ channels. The physiological role of the fast transient BK currentwas also examined using current-clamp techniques. Iberiotoxinbroadened action potentials (APs), indicating a role of BK currentin AP repolarization. Similarly, both the extracellular Ca²⁺ channel blocker Cd²⁺ and the intracellular Ca²⁺ chelator BAPTA blocked the transient component of the outwardcurrent and broadened APs in a subgroup of cells. Our resultsindicate that the outward current in pyramidal mouse neurons iscomposed of multiple components. A fast transient BK current isactivated by Ca²⁺ entry through high-threshold voltage-activated Ca²⁺ channels (L- and N-type), and together with other voltage-gatedK⁺ currents, this transient BK current plays a role in APrepolarization.

Key words: Ca²⁺ channels; Ca²⁺-activated K⁺ channels; BK channels; neocortical pyramidal neurons; iberiotoxin; charybdotoxin; nifedipine; $omega$ -conotoxin GVIA; BAPTA

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Acute hypoxia causes various biological responses in many types of organs or cells. The specific intracellular signaling pathwaysinvolved in the cellular responses and adaptation to hypoxia arenot yet well defined. Our interest has been focused on the factorsthat initially trigger these processes. For example, we have shownpreviously that hypoxia inhibited single large-conductance Ca²⁺-activated K⁺ (BK) channel activities in mouse neocortical neurons (Liu etal., 1999). The signaling pathways involved in this inhibitionhave not been clear. Indeed, the reduction in BK channel activitiescould have resulted from a hypoxia-evoked decline in Ca²⁺ influx or a direct effect of cytosolic factors on the channelsthemselves. Although there is some evidence that hypoxia can reducethe voltage-dependent Ca²⁺ currents in carotid glomus cells (Lopez-Barneo et al., 1997),other studies have shown either an increase (Summers et al., 2000)or no significant changes in such currents (Keating et al., 2001).

An elevation in intracellular Ca²⁺ level has been identified, however, as one of the early responses to exposure to hypoxiain dissociated central neurons, including hippocampal neurons(Friedman and Haddad, 1993) and cultured neocortical neurons (Chowand Haddad, 1998). A high cytosolic concentration of Ca²⁺ may result in the activation of many physiological or pathophysiologicalprocesses, including the activation of Ca²⁺-dependent K⁺ channels, such as BK channels. In many neurons, calcium influxvia voltage-gated calcium channels activates a variety of calcium-dependentK⁺ currents with different functional roles. In hippocampal neurons,N-type Ca²⁺ channels activate BK channels selectively, whereas L-type channelsprovide Ca²⁺ for small-conductance Ca²⁺-activated K⁺ (SK) channel activation (Marrion and Tavalin, 1998). In the presentstudy, we sought to (1) identify the Ca²⁺-dependent components of the outward currents and (2) characterizeBK currents and their Ca²⁺ sources through Ca²⁺ channels using whole-cell patch-clamp recordings in neocorticalpyramidal neurons. Understanding the relationship of BK channelsand their Ca²⁺ sources would be helpful for a better understanding of the pathophysiologicalroles they play under conditions of hypoxia andischemia.

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Preparation of neocortical neurons. In accordance with the guidelines of the Yale Animal Care and Use Committee, mice [postnatalday 9(P9)-P15] were deeply anesthetized with halothane and killedby decapitation. The brain was removed rapidly, chilled in 0-4°Coxygenated isolation buffer containing (in mM): 120 NaCl, 5 KCl,1 CaCl₂, 10 HEPES, and 25 glucose, pH adjusted to 7.0 with NaOH,and sectioned transversely into <800 µm slices. The neocorticalslices were dissected from these slices with the aid of a dissectingmicroscope. Neocortical slices were then incubated for 20 minwith oxygenated isolation buffer containing protease (type XIVfrom Streptomyces griseus, Sigma P-5147, 0.5 mg/ml, at 32°C).Thick slices and low concentrations of protease were used to minimizeenzyme exposure. Slices were then washed in oxygenated bufferand maintained for up to 4 hr. Immediately before recording, acortical slice was dissociated by gentle trituration with fire-polishedPasteur pipettes. The cells were collected and placed into a plasticPetri dish and were allowed several minutes to settle and adhereto the Petri dish before perfusion was initiated. Recordings wereobtained only from pyramidal-shaped neurons that had a singlethick proximal dendrite and did not show any visible evidenceofinjury.

Application of drugs and perfusion. Solutions were applied by a single-pass, gravity-fed perfusion system that delivered mediumto the recording chamber (chamber volume, <0.5 ml) at a rate of2 ml/min. To record Ca²⁺ channel currents, the chamber was perfused with a bathing solutioncontaining (in mM): 110 NaCl, 3 KCl, 5 CsCl, 15 TEACl, 3 CaCl₂,1 MgCl₂, 10 HEPES, 0.0005 TTX, and 10 glucose, with pH adjustedto 7.4 with NaOH. To record calcium-activated potassium channelcurrents, cells were superfused with a HEPES solution contained(in mM): 140 NaCl, 3 KCl, 1 CaCl₂, 1 MgCl₂, 10 HEPES, 0.0005 TTX,1 4-aminopyridine (4-AP), 0.005 glybenclamide, and 10 glucose,pH adjusted to 7.4 with NaOH. TTX, 4-AP, and glybenclamide wereincluded routinely in the K⁺ recording solution unless otherwise indicated. 4-AP (1 mM) wasused to reduce voltage-gated K⁺ currents and unmask Ca²⁺ dependence of K⁺ currents. A low concentration of 4-AP was chosen to minimizepossible nonspecific blockade on other K⁺ currents, such as SK currents. Experiments were conducted atroom temperature (22-25°C).

Whole-cell patch-clamp recording. Calcium and potassium currents were recorded from mouse neocortical neurons by use of thewhole-cell patch-clamp technique. Recording pipettes were madefrom filament borosilicate capillary glass (1.2 mm outer diameter,0.69 mm inner diameter) (Warner Instruments, Hamden, CT), usinga Flaming/Brown micropipette puller (model P-87; Sutter Instrument,Novato, CA). The pipettes were fire-polished and had resistancesof 2-5 M $Omega$ when filled with the solutions listed below. To recordcalcium current, pipettes were filled with intracellular solutioncontaining (in mM): 120 CsCl, 5 NaCl, 0.5 CaCl₂, 2 MgCl₂, 10 HEPES,10 EGTA, 1 ATP, 0.2 GTP, and 0.1 leupeptin, with pH adjusted to7.4 with CsOH. Patch solutions for potassium current recordingcontained (in mM): 110 K-gluconate, 10 KCl, 5 NaCl, 2 MgCl₂, 10HEPES, 0.5 EGTA, 1 ATP, 0.2 GTP, and 0.1 leupeptin, with pH adjustedto 7.4 with KOH. BAPTA (10 mM) was included in intracellular solutionsin some experiments. Osmolarity was measured and adjusted to between290 and 310 mOsm (Wescor osmometer; Wescor Inc., Logan, UT). Membranepotential and membrane currents were recorded with an Axopatch200A amplifier (Axon Instruments, Foster City, CA). Signals wereobtained at sampling rates of 5 and 50 kHz for voltage- and current-clamprecordings, respectively, and stored on the hard disk of a personalcomputer. Stimulus generation and data acquisition were controlledwith the ClampEx program in the pClamp6 software package (AxonInstruments). Before seals were made on cells, offset potentialswere nulled. Capacitance subtraction was used in all recordings.Recordings were accepted when resting membrane potentials (measuredimmediately after membrane rupture) were more negative than $-$ 40mV or holding currents at $-$ 70 mV were <100 pA. The series resistanceswere primarily 10-20 M $Omega$ . Leak currents were not subtractedonline.

Drugs and solutions. All the channel blockers used in the present study were purchased from Sigma. Charybdotoxin (ChTX) andapamin were first dissolved in water at concentrations of 0.1and 2 mg/ml, respectively; Bay K 8644 stock solution was preparedin methanol at 10 mM; glybenclamide and nifedipine were dissolvedin dimethyl sulfoxide (DMSO) at 20 and 50 mM, respectively; $omega$ -conotoxinGVIA was dissolved in medium at 0.1 mM. TTX stock solution concentrationwas 1 mM. Aliquots of stock solutions were kept at $-$ 80°C and werelater diluted with external solution before use. The final concentrationof either methanol or DMSO was <1:5000, a concentration that wasfound to have no effect on Ca²⁺ current (Sun et al., 2002)

Data analysis. Calcium channel currents were elicited from a holding potential of $-$ 70 mV. Single steps to $-$ 10 mV or a seriesof 10 mV steps between $-$ 60 and +50 mV for 100 msec were used.Mean values measured at 60 msec in a 100 msec voltage step wereused to evaluate calcium channel current amplitude. K⁺ currents were evoked by depolarizing steps ( $-$ 70 to +50 mV) froma holding potential of $-$ 70 mV for 190 msec, with a 5 sec interval.Current-voltage (I-V) relationships were generated by measuringvalues at the first peak for the transient outward current andat 100 msec for the sustained current. Percentage block of thesecurrents was defined as [1 $-$ (I_test)/(I_control)] × 100, and valuesfrom depolarizing steps to $-$ 10 and +30 mV were used to evaluateCa²⁺ and K⁺ current percentage changes respectively. Raw data were comparedfor statistical significance using ANOVA for between-group comparisonand paired t test for within-group comparison. Data are presentedas mean ±SEM.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

General properties of outward currents

Using whole-cell patch-clamp techniques, inward Ca²⁺ currents, outward K⁺ currents, and membrane potential were studied in a total of 124neocortical pyramidal neurons. Figure 1A shows the morphologyof the somata and the apical dendrite of a typical cell studied.

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Figure 1. Outward currents in neocortical pyramidal neurons. A, Morphology of freshly dissociated neocortical pyramidal neurons. Bright-field image showing typical shape of the soma and at least one apical dendrite. The arrow indicates a pyramidal cell. Scale bar, 30 µm. B, Superimposed outward current traces in response to a voltage step to $-$ 10 mV from a holding potential of $-$ 70 mV before and during application of recording solution containing 1 mM 4-AP, 0.5 µM TTX, and 5 µM glybenclamide. Transient sodium currents were blocked by TTX. In the presence of 4-AP, a transient outward current was revealed. C, Currents were elicited by depolarizing voltage steps ( $-$ 70 to +50 mV) from a holding potential of $-$ 70 mV (for 160 msec, in 10 mV steps, every 5 sec) during superfusion. Representative examples of cells expressing an early transient outward current (C1) and cells showing only a sustained current (C2). D, Expanded current traces taken from C1, showing an early transient outward current at depolarizing voltages from $-$ 40 to 10 mV.

Whole-cell voltage-clamp experiments were performed using K⁺-filled pipettes to characterize the K⁺ currents evoked by depolarization. Extracellular recording solutioncontained a mixture of channel blockers: 4-AP, 1 mM, for transientvoltage-gated K⁺ current; TTX, 0.5 µM, for Na⁺ current; and glybenclamide, 5 µM, for ATP-sensitive K⁺ current. These agents were added routinely to the recording perfusateunless otherwise stated. The effects of these blockers were evaluatedin five cells. Figure 1 shows an example of inward Na⁺ and outward K⁺ currents, evoked by a depolarizing pulse to $-$ 10 mV from a holdingpotential of $-$ 70 mV before (control) and after application ofchannel blockers. The inward Na⁺ currents were blocked by TTX. The outward K⁺ currents could be separated into a rapidly activating transientcomponent and a more slowly activating sustained component. Thetransient component could be partially blocked by 4-AP, revealingthe presence of a rapidly activating, partially inactivating,4-AP-insensitive outward current. The sustained component wasnot greatlyaffected.

In a total of 100 control cells using the solutions described above, 64 cells expressed a transient outward current. Figure1C shows families of currents evoked by holding at $-$ 70 mV andstepping to potentials ranging from $-$ 70 to +50 mV for 160 msecduring superfusion. In the example shown in Figure 1C1, this paradigmresulted in transient outward currents at potentials positiveto $-$ 40 mV. In another cell shown in Figure 1C2, however, thesedepolarizing steps evoked only slowly activating, sustained outwardcurrents. The expanded traces shown in Figure 1D are from currenttraces in Figure 1C1. The transient outward current showed a thresholdat $-$ 40 mV and became both larger and faster between $-$ 40 and $-$ 10mV (Fig. 1D). At membrane potentials >0 mV, however, the peakamplitude of the transient K⁺ currents did not increase further and even fell slightly at moredepolarized potentials, despite an increased driving force onK⁺. Such a decrease at much depolarized potentials is expected forCa²⁺-dependent currents because of the suppression of Ca²⁺ influx as the membrane potential approaches the equilibrium potentialfor Ca²⁺.

Ca²⁺-dependent component of outward currents

To further test the Ca²⁺ dependence of the transient outward currents, we examined the effects of blocking Ca²⁺ influx on this current by applying Cd²⁺, a nonspecific Ca²⁺ channel blocker. In the presence of 1 mM 4-AP, eight cells showeda transient outward current with varied amplitude, and the transientcomponent was completely and reversibly blocked by 100 µM Cd²⁺. An example is shown in Figure 2A. Outward currents were evokedby stepping from $-$ 70 mV to potentials ranging from $-$ 70 to +50mV in control (Fig. 2A1) and with 100 µM Cd²⁺ (Fig. 2A2). Control currents resembled those described in Figure1 in having an early transient component followed by a sustainedcurrent. The transient component was abolished by Cd²⁺. On average, Cd²⁺ significantly reduced the transient peak (evoked by single depolarizingsteps from $-$ 70 to +30 mV) from 1527 ± 179 to 972 ± 124 pA (n =10; p < 0.05). The voltage dependence of the Cd²⁺-sensitive current correlates well with that of Ca²⁺ currents (Fig. 2A3,A4) (see also Fig. 8).

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Figure 2. Ca²⁺ dependence of the transient outward current. Membrane potential was held at $-$ 70 mV and stepped from $-$ 70 to +50 mV for 160 msec in 10 mV steps every 5 sec. A and B show currents activated by these voltage steps in superfusing medium containing 4-AP (1 mM) before (A1, B1) and during application of 100 µM Cd²⁺- (A2) or Ca²⁺-free (B2) solution. A3, B3, Ca²⁺-sensitive currents (subtraction A1 $-$ A2 or B1 $-$ B2). A4, B4, I-V plots obtained from outward currents in A1-3 and B1-3 measured at the time point of first peak of control transient currents. $black-square$ , Control; , in the presence of Cd²⁺- (A4) or Ca²⁺-free solution (B4); $black-triangle$ , Cd²⁺ (A4) or Ca²⁺ (B4)-sensitive currents. Insets, Superimposed current traces in response to a voltage step to $-$ 10 from $-$ 70 mV showing a reversible effect of 100 µM Cd²⁺- and Ca²⁺-free medium on outward currents.

The effect of free Ca²⁺ on the outward currents was also examined. Application of Ca²⁺-free medium, in which Ca²⁺ was replaced by Mg²⁺, virtually eliminated the transient outward current. The peakamplitude of this transient outward current (evoked by depolarizingsteps from $-$ 70 to +30 mV) was reduced from 1339 ± 148 to 989 ±139 pA (n = 6; p < 0.05). An example is shown in Figure 2B. ACa²⁺-sensitive current, which was obtained by subtraction of currentsevoked in Ca²⁺-free medium from currents evoked in control medium, consistedof both transient and sustained components (Fig. 2B3). The sensitivityof the transient outward current to treatments that block Ca²⁺ influx indicates that this current is Ca²⁺dependent.

Effects of block of BK channel blockers on the transient outward current

Because the transient outward current is Ca²⁺-dependent, we also used specific Ca²⁺-activated potassium channel blockers to determine which channelsmediate this current. Evidence that a major part of this currentwas mediated by BK channels is presented by the experiments shownin Figure 3, in which the effects of two potent BK channel blockerswere examined in 14 cells. Figure 3A shows an example of outwardcurrents evoked by stepping from $-$ 70 mV to depolarized potentials( $-$ 70 to +50 mV) in control (Fig. 3A1) and in the presence of 50nM ChTX, a BK channel blocker (Fig. 3A2). Application of ChTXeliminated most of the transient currents (Fig. 3A). Block ofChTX was irreversible during the time course of these experiments(Fig. 3A4, inset), and the amplitude of the early peak (evokedby depolarizing step to +30 from $-$ 70 mV) was reduced from 1370± 163 to 1025 ± 165 pA (n = 9; p < 0.05).

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Figure 3. ChTX and IBTX block the transient outward currents. Membrane potential was held at $-$ 70 mV and stepped from $-$ 70 to +50 mV for 160 msec in 10 mV steps every 5 sec. A and B show currents activated by these voltage steps in superfusing medium containing 4-AP before (A1, B1) and during application of 50 nM ChTX (A2) and 100 nM IBTX (B2). A3, B3, ChTX-sensitive currents (subtraction A1 $-$ A2) and IBTX-sensitive currents (B1 $-$ B2). A4, B4, I-V plots obtained from outward currents in A1-A3 and B1-B3 measured at the time point of early peak of control transient currents. $black-square$ , Control; , in the presence of ChTX (A4) or IBTX (B4); $black-triangle$ , ChTX (A4) or IBTX (B4)-sensitive currents. Insets, Superimposed current traces evoked by depolarizing steps to $-$ 10 from $-$ 70 mV, showing an irreversible effect of ChTX and IBTX on outward currents during the time course of experiment.

The effect of another selective blocker for the BK type of Ca²⁺-activated K⁺ current, iberiotoxin (IBTX), was also examined. Figure 3B showsthat this peptide similarly blocked the transient current in allcells tested (Fig. 3B). On average, the early peak current was1492 ± 105 pA before and 998 ± 96 pA after 100 nM IBTX (n = 5;p < 0.05). These toxins also reduced a component of the sustainedcurrents. The BK current activated fully within 5 msec and thendecayed within 20 msec to a steady level (Fig. 3A3,B3). Inactivationcould be fit by a single exponential equation. The inactivationtime constant of the transient BK current evoked by a depolarizingstep to +30 mV from $-$ 70 mV was 3.5 ± 0.2 msec, and time to peakwas 4.9 ± 0.4 msec (n = 4), which is not significantly differentfrom the time to peak for calcium current (4.5 ± 0.3 msec; n =13; one-way ANOVA; p < 0.05) (see also Fig. 5A).

Voltage dependence of the transient BK current (Fig. 3) and Ca²⁺ current (Fig. 5) match well in the voltage range of $-$ 40 to +20mV, where the Ca²⁺ current is obvious. The observation that the transient K currentsshow little or no decline at positive membrane potentials is consistentwith a series resistance error. The I-V relationships of ChTX-and IBTX-sensitive currents differed slightly from those of Cd²⁺- and Ca²⁺-sensitive currents shown in Figures 2 and 3. The ChTX- or IBTX-sensitivecurrents presumably represented the effects of blocking BK currentsonly, whereas the Cd²⁺- or Ca²⁺-sensitive currents reflected the combined effects of blockinginward Ca²⁺ currents and outward Ca²⁺-dependent K⁺ currents (BK andSK).

These results indicate that BK channels mediate a major part of the transient outward current in mouse neocortical pyramidalneurons.

Effect of block of SK channels on the transient component

To test whether SK channels were involved, we examined the effect of apamin, which blocks SK channels. In contrast to ChTXand IBTX, application of 500 nM apamin had no obvious effect onthe fast transient outward current, suggesting that the transientcurrent is apamin insensitive. In seven of the cells tested, however,apamin affected only the slower current in six cells and did nothave an obvious effect in another (data not shown). An exampleis shown in Figure 4. The fast transient outward current persistedafter application of apamin (Fig. 4A,B), and addition of ChTXto the solution resulted in complete blockade of the fast transientoutward currents (Fig. 4C). A sustained component of the outwardcurrent is sensitive to apamin (Fig. 4D), whereas ChTX-sensitivecurrent is fast activating and rapidly inactivating (Fig. 4E).Thus, the fast transient outward current is sensitive to a toxinspecific for BK channels but not to a toxin that blocks SK channels.

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Figure 4. Charybdotoxin but not apamin blocks the transient outward current. Membrane potential was held at $-$ 70 mV and stepped from $-$ 70 to +50 mV for 160 msec in 10 mV steps every 5 sec. A-C, Currents activated by these voltage steps in superfusing medium containing 4-AP before (A, Control) and during additive application of 500 nM apamin (B) and 50 nM ChTX (C). ChTX but not apamin resulted in complete blockade of the transient outward current. D1 shows the apamin-sensitive currents obtained by subtracting B from A. D2, I-V plots obtained from outward currents in A, B, and D1 measured at the time point of peak transient currents in the control. E1, ChTX-sensitive current obtained by subtracting C from B. E2, I-V plots measured from B, C, and E1.

Characterization of the inward calcium currents

Rat neocortical neurons have been shown previously to express pharmacologically distinct types of calcium channels, includingN-type and L-type channels (Lorenzon and Foehring, 1995). We usedthe selective Ca²⁺ channel blockers $omega$ -conotoxin-GVIA ( $omega$ -CgTX, N-type) and nifedipine(L-type) and have confirmed previous observations that neocorticalpyramidal neurons express multiple subtypes of high-thresholdCa²⁺ currents. Figure 5 shows Ca²⁺ currents evoked by depolarizing voltage steps from a holdingpotential of $-$ 70 mV. Figure 5A,B illustrates the effects of sequentialapplication of $omega$ -CgTX (1 µM), nifedipine (5 µM), and Cd²⁺ (100 µM) on the calcium current evoked at $-$ 10 mV. Nifedipineproduced a rapid and reversible block of Ca²⁺ current in all cells tested, indicating the presence of L-typeCa²⁺ channels. Nifedipine alone blocked calcium channel current byapproximately one-third (29.8 ± 9.1%; n = 7; p < 0.05) (Fig. 5A-C). $omega$ -CgTX produced irreversible inhibition of Ca²⁺ current by an average of 26 ± 2.9% (n = 4; p < 0.05) (Fig. 5A-C).A substantial fraction (50%) of the total Ca²⁺ current was unaffected by the combined actions of nifedipineand $omega$ -CgTX, indicating the presence of other HVA currents. Cd²⁺ completely and reversibly blocked all inward calcium currentin all cells tested (n = 6; p < 0.05). Figure 5D shows the Ca²⁺ current I-V relationships obtained in the absence (control) andpresence of Ca²⁺ channel blockers. When elicited by step depolarization from aholding potential of $-$ 70 mV, Ca²⁺ currents were normally activated at approximately $-$ 40 mV, peakedat $-$ 10 mV, and reversed between +30 and +40 mV. Nifedipine and $omega$ -CgTX exerted an inhibitory effect at all potentials at whichcurrents were activated; this inhibition was not accompanied bya shift in the peak voltage of Ca²⁺ current.

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Figure 5. Analysis of contribution of L- and N-type Ca²⁺ channel in total Ca²⁺ currents in mouse neocortical pyramidal neurons. A, A representative experiment illustrating the effect of the L-type Ca²⁺ channel blocker nifedipine (5 µM), N-type Ca²⁺ channel blocker $omega$ -CgTx GVIA (1 µM), and Cd²⁺ (100 µM) on the inward Ca²⁺ current. B, Time course of the experiment shown in A illustrating the sequential blocking actions of $omega$ -CgTx GVIA, nifedipine, and Cd²⁺. C, Group data of percentage block of nifedipine (n = 6), and $omega$ -CgTx GVIA (n = 4). D, I-V plots of Ca²⁺ currents in the absence (control, n = 6) and presence of nifedipine and $omega$ -CgTx GVIA.

Contribution of L- and N-type Ca²⁺ channels in activating transient BK current

The role of L-type Ca²⁺ channels in the fast transient BK current activation was examined next with 5 µM nifedipine (antagonist)and 1 µM Bay K8644 (agonist). Figure 6 shows an example of theeffects of nifedipine on BK currents. Nifedipine caused a reductionin the magnitude of the fast transient BK current (Fig. 6). Nifedipine-sensitivecurrent, which was obtained by subtracting B (nifedipine) fromA (control), had an early transient component followed by a sustainedcomponent (Fig. 6D). Six cells tested expressed the transientBK current, and nifedipine reduced the early peak current to amean of 1180 ± 186 pA from a mean of 1343 ± 157 pA (n = 6; p <0.05). An L-type Ca²⁺ agonist, Bay K8644, enhanced a transient outward current (n =3; data not shown).

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Figure 6. L-type Ca²⁺ channels contribute to activation of the transient BK currents. Currents were evoked by depolarizing steps ( $-$ 70 to +50 mV) for 160 msec from a holding potential of $-$ 70 mV in control (A), in the presence of nifedipine (5 µM) (B), and after washout (C). Nifedipine inhibits the transient BK current and a sustained outward current. D, Nifedipine-sensitive current was obtained by subtracting B from A. E, I-V plots, which were measured at the early peak time point, showing a slightly N-shaped nifedipine-sensitive transient current. Inset, Superimposed current traces evoked by depolarizing steps to $-$ 10 from $-$ 70 mV.

We also examined the contribution of N-type channels toward BK current activation. Five cells expressed, to various extents,a transient outward current, and 1 µM $omega$ -CgTX partially blockedthe early peak current (average of 1711 ± 254 pA before and 1540± 239 pA after $omega$ -CgTX; n = 5; p < 0.05). As shown in Figure 7,in the presence of 500 nM apamin, which removed apamin-sensitiveSK current, $omega$ -CgTX resulted in partial reduction in the transientBK current, yielding a small $omega$ -CgTX-sensitive current (Fig. 7B,D).Another addition of nifedipine (5 µM) eliminated most of the transientBK current (Fig. 7C,E). After pretreatment with ChTX, $omega$ -CgTX reducedonly the slow component of outward currents, whereas in cellspretreated with apamin, $omega$ -CgTX inhibited the fast transient BKcurrent (data not shown). Thus, these results indicate that N-typeCa²⁺ channels contributed to the transient BK current activation.

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Figure 7. Both L- and N-type Ca²⁺ channels contribute to activation of the transient BK currents. Membrane potential was held at $-$ 70 mV and stepped from $-$ 70 to +50 mV for 160 msec in 10 mV steps every 5 sec. Currents were recorded in the presence of apamin (500 nM) to eliminate SK current contribution. A-C, Currents recorded in superfusing medium containing apamin (A, control) and during additive application of 1 µM CgTX (B) and 5 µM nifedipine (C). Subtracting B from A and C from B reveals a small transient CgTX-sensitive current (D1) and a nifedipine-sensitive current with both transient and sustained components (E1), respectively. D2, E2, I-V plots obtained from A-E.

Sustained component of outward currents

As described above, both BK and SK channel blockers and Ca²⁺ channel blockers (L- and N-type) blocked part of the sustainedoutward currents. The extent of blockade varied greatly from cellto cell. Figure 8 summarizes the effects of all the above-mentionedagents for both the early peak and sustained outward currents.These data suggested that the sustained outward current was composedof multiple components, including both BK and SK currents, andmost of all, voltage-gated potassium currents. Ca²⁺ entry through both L- and N-type Ca²⁺ channels activated these Ca²⁺-activated BK and SK currents.

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Figure 8. Effects of various blocking agents on components of transient and sustained outward currents. A, Summary of effects of various agents on the early peak outward current. Values are measured at the first peak of outward current evoked by a depolarizing step from $-$ 70 to +30 mV before each agent (control). Numbers included only cells expressing transient outward current. B, Group data of effects of various agents on sustained outward current. Values are measured at 100 msec of outward current evoked by a depolarizing step from $-$ 70 to +30 mV. Numbers included cells with and without transient outward currents. Data are expressed as mean ± SE. The asterisk indicates a significant difference (p < 0.05) between control and treatments (Student's paired t test).

Role of transient BK current in membrane and action potentials

The functional role of the transient BK current has not been determined in neocortical neurons. To examine the role of theBK current, we performed current-clamp experiments. The extracellularsolutions used were the same as those for voltage-clamp recordingsfor K⁺ currents, except that TTX was omitted. In the presence of 1 mM4-AP, action potentials were elicited by suprathreshold depolarizingcurrent injection. Because blockade of Ca²⁺ currents by Ca²⁺ channel blockers can produce effects unrelated to the reductionof BK current activation, we attempted to selectively remove thecontribution of BK currents to action potential repolarizationusing IBTX. Application of 100 nM IBTX blocked the transient BKcurrent (Fig. 9A) and resulted in a slowing of the action potentialrepolarization recorded in the same cell with current-clamp recording(Fig. 9B). We found no significant differences in action potentialamplitude, with a mean of 91.3 ± 6.2 mV before and 90.5 ± 5.9mV after IBTX (p > 0.05; n = 6). The action potential half-width(width of the spike measured at half-maximal amplitude) was significantlyincreased by IBTX, from 2.9 ± 0.2 to 3.3 ± 0.3 msec, whereas thethreshold duration (width of the spike measured at threshold)was increased to 8.9 ± 1.0 msec from 6.9 ± 0.6 msec (p < 0.05;n = 6). This experiment clearly shows that the transient BK currentis normally activated during repolarization.

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Figure 9. Effects of IBTX on outward currents and action potentials of neocortical pyramidal neurons. A, Voltage-clamp recordings showing superimposed current traces before (control) and after 100 nM IBTX during superfusion with 4-AP. Currents were evoked by a depolarizing step to $-$ 10 from $-$ 70 mV. B, Current-clamp recordings from the same cell as in A, showing superimposed voltage traces taken in these treatments. Action potentials were elicited by suprathreshold current injections. IBTX blocked the transient BK current and broadened action potentials.

Ca²⁺ dependence of action potential and membrane currents

Several previous studies of neocortical pyramidal cells in rats, cats, and guinea pigs have failed to show evidence for Ca²⁺ dependence of action potential repolarization. We therefore testedthis in mice in this work. As shown in Figure 1, cells vary inthe expression of total outward currents, and only a subgroupof cells studied showed obvious transient outward currents. Wethen compared Cd²⁺-sensitive currents (current obtained by subtracting the currentremaining in the presence of 100 µM Cd²⁺ from control current) during depolarization in different cells.We found that during the first 10 msec depolarization steps from $-$ 70 to +10 mV, depolarization evoked varied amounts of Ca²⁺ (the small inward current that precedes outward currents) andK⁺ currents (Fig. 10A1-3). Ca²⁺ dependence of action potential repolarization would then be expectedto vary in these different cells.

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Figure 10. Variations in Cd²⁺-sensitive currents activated by membrane depolarization in different cells. Currents are activated by 160 msec voltage steps from $-$ 70 to +10 mV. A1-A3, Cd²⁺-sensitive currents from three different cells. Currents are obtained by subtracting remaining currents in the presence of Cd²⁺ (100 µM) from currents before Cd²⁺ application (control). A small inward Ca²⁺ current precedes outward currents in A2 and A3. The relative amount of Ca²⁺ and transient outward currents varies among these cells in the initial 10 msec depolarization period. B, A transient BK current in another cell. ChTX-sensitive current is obtained by subtracting the remaining current in the presence of ChTX (50 nM) from control current.

We next examined Ca²⁺ dependence of action potential repolarization using extracellularly applied Cd²⁺ (100 µM) and internal BAPTA (10 mM). In the presence of 1 mM4-AP, membrane currents and action potentials were measured usingvoltage- and current-clamp recordings, respectively. Again, Cd²⁺ and BAPTA blocked all the transient outward currents (Fig. 11A1,B1),and we found that in a majority of cells (8 of 11), action potentialhalf-width was increased, from 2.6 ± 0.2 msec in control to 3.1± 0.5 msec; action potential threshold duration from 6.9 ± 0.6to 9.7 ± 0.5 msec in the presence of Cd²⁺ (p < 0.05). In all the cells tested, the afterhyperpolarization(AHP) was consistently attenuated markedly by Cd²⁺. Examples of the effects of Cd²⁺ and BAPTA on outward currents and action potential repolarizationare illustrated in Fig. 11.

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Figure 11. Effects of Cd²⁺ and intracellular BAPTA on outward currents and action potentials of neocortical pyramidal neurons. A1, Voltage-clamp recordings showing superimposed current traces before (control) and after 100 nM IBTX during superfusion with 4-AP. Currents were evoked by a depolarizing step to $-$ 10 from $-$ 70 mV. A2, Current-clamp recordings from the same cell as in A1, showing superimposed voltage traces taken in these treatments. Action potentials were elicited by suprathreshold current injections. B1, Superimposed current traces from another cell taken with 10 mM intracellular BAPTA in the pipette immediately after rupture (control) and 2 min later (BAPTA). B2, Current-clamp recordings from the same cell as in B1. Both Cd²⁺ and BAPTA blocked transient outward currents and broadened action potentials.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In the present study, we have made several interesting observations. For example, we have identified a fast transient BK currentin mouse neocortical pyramidal neurons. In the presence of 4-AP,the fast transient outward current is Ca²⁺ dependent and sensitive to the specific BK channel blockers ChTXand IBTX but not to the SK channel blocker apamin. Furthermore,the transient BK current is activated by Ca²⁺ influx from L- and N-type Ca²⁺ channels during depolarization. Finally, this BK current playsan important role in action potentialrepolarization.

Variations in the transient BK current

In the present study, the magnitude of the transient and sustained BK currents varied from cell to cell. This may result fromvaried levels of expression of inactivating and noninactivatingBK channels or varied regulation of the current itself. Variationsin Ca²⁺ inward currents would also be a source of variations in the BKcurrents. Neocortical pyramidal cells are different in size, projections,laminar distribution, and firing pattern. Individual neocorticalpyramidal cells vary greatly in the percentage contribution ofeach Ca²⁺ channel type to the whole-cell Ca²⁺ current (Stewart and Foehring, 2000). Thus, Ca²⁺ channel subtypes contribute differently to specific cellularevents, such as neurotransmitter release, action potential repolarizations(BK channel activation), and AHPs (SK channel activation). Moreover,it is possible that some of the variability may also arise fromthe technique used by us and others to dissociate cells with differentamounts of dendrites still attached to the soma, because thereis a subcellular compartmentalization of channeltypes.

Inactivation of BK channel

In this study, we have shown that a transient outward current is sensitive to the BK channel blockers ChTX and IBTX (Fig.3) but not to the SK channel blocker apamin (Fig. 4), indicatingthat the current is mediated by BK channels. In these neocorticalneurons, the rapidly activating transient BK current decays rapidlyto a steady level within ~20 msec, with an inactivating time constantof ~4 msec. In the present study, Ca²⁺ was used as current carrier. I_Ca reached its peak rapidly andstarted to inactivate slowly (Fig. 5). The transient BK currentpeaked at approximately the same time as Ca²⁺ current and started to inactivate when Ca²⁺ current also declined. Thus, it is unlikely that some of theapparent decline in outward current was actually a manifestationof the activation kinetics of the Ca²⁺current.

Although BK channels are clearly found in many organisms and cell types, only a few of them exhibit inactivation, includinghippocampal neurons (Hicks and Marrion, 1998), Drosophila muscle(Salkoff, 1983), chromaffin cells (Solaro and Lingle, 1992), RINm5fcells (Li et al., 1999), and frog hair cells (Armstrong and Roberts,2001). The only known mechanism of BK channel inactivation isthat conferred by auxiliary ( $beta$ ) subunits, which mediate inactivationthrough an intracellular "ball and chain" mechanism (Wallner etal., 1999; Xia et al., 1999, 2000). $beta$ -Subunit expression was detectedin rat brain tissue and human cerebral cortex (Xia et al., 1999).However, to the best of our knowledge, our study is the firstto report on inactivating BK currents in cortical pyramidal neurons.From the fast inactivation of this transient BK current in ourstudy, it is possible that inactivation could be the result ofinteraction between $alpha$ - and $beta$ 3-subunits (Xia et al., 2000).

Role of L- and N-type Ca²⁺ channels in activating BK currents

Although intracellular recording studies have shown that various Ca²⁺ channel subtypes are involved in the generation of AHPs (SK)in neocortical pyramidal neurons (Pineda et al., 1998, 1999),an association of Ca²⁺ channels with BK channels has not been well delineated. We foundthat both N- and L-type Ca²⁺ channel blockers partially eliminated the transient BK current(Figs. 6, 7), indicating that both subtypes provided Ca²⁺ for the activation of the current. In the present study, we cannotrule out the combination of other Ca²⁺ sources for the activation of the BK current; however, our dataindicate that N- and L-type Ca²⁺ channels seem to be the major Ca²⁺ sources for thiscurrent.

The relationship between Ca²⁺ currents and Ca²⁺-dependent K⁺ currents depends on the subcellular localization of these channelsand on intracellular Ca²⁺ accumulation during neural activity. Large and localized Ca²⁺ elevations are thought to occur only in the immediate vicinityof Ca²⁺ channels because of intracellular buffering. In the present study,intracellular solutions contained low concentrations of EGTA (0.5mM). The presence of low intracellular concentrations of Ca²⁺ buffers could result in a smaller peak value of [Ca²⁺]_i transient after a fixed influx of Ca²⁺ and a prolonged decay (Schwindt et al., 1992; Sah and Clements,1999). Ca²⁺ buffers have different roles in the control of different Ca²⁺-activated K⁺ currents in neurons. It has been shown that in hippocampal neurons,the action potential repolarization and the fast AHP, which ismediated by BK channels, were unaffected by 100 µM to 3 mM ofinternally applied BAPTA, whereas the slow AHP, which is presumedto be generated by SK-type Ca²⁺-activated K⁺ channels, was potentiated (Velumian and Carlen, 1999). Similarly,in cat neocortical neurons, a small reduction of intracellularCa²⁺, resulting from low internal Ca²⁺ chelator concentration, preferentially enhanced a slow, Ca²⁺-dependent K⁺ current but did not significantly affect action potential timeto half amplitude (Schwindt et al., 1992). Close proximity ofBK channels to Ca²⁺ channels has been shown in hippocampal neurons (Marrion and Tavalin,1998; Velumian and Carlen, 1999). The fast-rising phase of thetransient BK current in our study in neocortical neurons (Fig.3) suggests that a fast increase in [Ca²⁺]_i delivered close to the BK channels activates them rapidly.Thus, it seems likely that the low EGTA in the intracellular solutionwould not significantly affect the transient BK current (whichconstitutes our main interest in this study), although the possibleenhancing effect on SK current cannot be excluded. In this study,we found that 10 mM internal BAPTA eliminated the transient outwardcurrents (Fig. 11), suggesting that the distance between the transientBK current and its Ca²⁺ sources is larger than the buffering length constant forBAPTA.

Physiological roles of transient BK current in neocortical pyramidal neurons

In neurons, Ca²⁺-activated K⁺ channels have been reported to play an important role in regulating resting and action potentials(Lancaster and Nicoll, 1987; Storm, 1987; Sah and McLachlan, 1992).Because BK channels require simultaneous depolarization and elevatedcytosolic calcium to become activated, this necessitates thatelectrical activity be coupled to changes in intracellular calcium.Furthermore, the large conductance of neuronal BK channels allowsthem to play an important role in hyperpolarizing the membranepotential when they areactivated.

Although a number of K⁺ currents have been described previously in neocortical neurons, a major part of the action potentialrepolarization has not been found to be significantly Ca²⁺ dependent (Spain et al., 1991; Foehring and Surmeier, 1993; Kanget al., 2000). The physiological roles of BK channels in neocorticalpyramidal neurons were relatively unclear from previous studies.The effect of Ca²⁺ entry blockade (Cd²⁺, BAPTA) on the repolarization phase of action potentials wasvariable in mouse neocortical neurons in our study, with a majorityof cells increasing action potential half-width (Fig. 11). We believethat the difference between cells reflects the relative numberof Ca²⁺ and BK channels activated during the action potential in differentcells, with the two types of channels affecting action potentialrepolarization in opposite directions. The amount of Ca²⁺ current and BK current activated during depolarization indeedvaries among cells (Fig. 10). A transient K⁺ current was found previously to be sensitive to TEA but not to4-AP and to be involved in action potential repolarization; however,a BK channel blocker was not tested on these currents (Spain etal., 1991; Kang et al., 2000). Furthermore, it has been shownthat a calcium-activated outward current was involved in the laterepolarization in a subgroup of pyramidal cells of cat motor cortex(Chen et al., 1996), although the nature of this current was notcharacterized in that study. In rat neocortical pyramidal neurons,the final phase of repolarization was sensitive to block of N-typeCa²⁺ current (Pineda et al., 1998). In our present work, the specificBK channel blockers ChTX and IBTX are used, and we demonstratethat a transient BK current is present in these cells in mice.Hence, we have extended previous observations in helix neurons(Crest and Gola, 1993), hippocampal pyramidal neurons (Storm,1987), and bullfrog sympathetic neurons (MacDermott and Weight,1982) to demonstrate that a fast inactivating BK current operatesduring action potential and is involved in action potential repolarizationin mouse neocortical pyramidalneurons.

The role of this transient outward current is now made clearer in neocortical pyramidal neurons, because we found that thiscurrent is eliminated by Cd²⁺ and Ca²⁺ removal from extracellular solutions. It is also sensitive tothe BK channel blockers ChTX and IBTX but not to the SK channelblocker apamin. Blocking this transient BK current results inbroadening of action potentials, indicating that it is involvedin action potential repolarization. Pathophysiological roles ofthis current, in relation to changes in its Ca²⁺ sources from voltage-gated Ca²⁺ channels, under conditions such as hypoxia and ischemia wouldbe of interest for futurestudies.

  FOOTNOTES

Received Dec. 16, 2002; revised Jan. 29, 2003; accepted Feb. 11, 2003.

This work was supported by National Institutes of Health Grant 1P01NS42202. We appreciate the help of Cate Muenker and HillarySunamoto for animal handling. Parts of this paper have been publishedpreviously in abstract form (Sun and Haddad, 2002).

Correspondence should be addressed to Dr. Gabriel G. Haddad, Department of Pediatrics, Albert Einstein College of Medicine,Rose Kennedy Center, Room 846, 1410 South Pelham Parkway, Bronx,NY 10461. E-mail: ghaddad{at}aecom.yu.edu.

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Materials and Methods
Results
Discussion
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