Potassium Currents during the Action Potential of Hippocampal CA3 Neurons

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The Journal of Neuroscience, December 1, 2002, 22(23):10106-10115

Potassium Currents during the Action Potential of Hippocampal CA3 Neurons
Jörg Mitterdorfer and Bruce P. Bean
Department of Neurobiology, Harvard Medical School, Boston, Massachusetts 02115

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Central neurons have multiple types of voltage-dependent potassium channels, whose activation during action potentials shapesspike width and whose activation and inactivation at subthresholdvoltages modulate firing frequency. We characterized the voltage-dependentpotassium currents flowing during the action potentials of hippocampalCA3 pyramidal neurons and examined the susceptibility of the underlyingchannel types to inactivation at subthreshold voltages. Usingacutely dissociated neurons that permitted rapid voltage clamp,action potentials recorded previously were used as the commandvoltage waveform, and individual components of potassium currentwere identified by pharmacological sensitivity. The overall voltage-dependentpotassium current in the neurons could be split into three majorcomponents based on pharmacology and kinetics during step voltagepulses: I_D (fast activating, slowly inactivating, and sensitiveto 4-aminopyridine at 30 µM), I_A (fast activating, fast inactivating,and sensitive to 4-aminopyridine at 3 mM), and I_K (slowly activating,noninactivating, and sensitive to external TEA at 3-25 mM). Thepotassium current during the action potential was composed ofapproximately equal contributions of I_D and I_A, with a negligiblecontribution of I_K. I_D and I_A had nearly identical trajectoriesof activation and deactivation during the action potential. BothI_A and I_D showed steady-state inactivation at subthreshold voltages,but maximal inactivation at such voltages was incomplete for bothcurrents. Because of the major contribution of both I_D and I_Ato spike repolarization, it is likely that modulation or partialinactivation at subthreshold voltages of either current can influencespike timing with minimal effect on spikewidth.

Key words: action potential; 4-aminopyridine; I_A; I_D; I_K; pyramidal neuron; spike; potassium current

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although action potentials in squid axons are formed by just two types of voltage-dependent channels (Hodgkin and Huxley,1952), vertebrate central neurons each express at least a dozendifferent types of voltage-dependent ion channels (Llinás, 1988;Brown et al., 1990; Hille, 2001). The expression in central neuronsof multiple types of potassium channels in particular confersthe ability to fire with a variety of patterns over a broad rangeof frequencies (Connor and Stevens, 1971a,b; Rudy, 1988; Storm,1990; Hille, 2001; Rudy and McBain, 2001).

How do the many channel types present in a particular neuron work together to determine its firing properties? This issuehas been addressed primarily by computer modeling using Hodgkin-Huxley-likeequations, extended by the addition of many conductances, withequations for each conductance based on experimental analysisof voltage and time dependence (Connor and Stevens, 1971b; Huguenardand McCormick, 1992, 1994; Johnston and Wu, 1995; Locke and Nerbonne,1997b). This approach has been powerful and informative, but ithas limitations. For central neurons, the connection between experimentalmeasurements and modeling is quite indirect. For example, mostvoltage-clamp studies of potassium channels in central neuronsare based on measurements of kinetics using voltage steps farlonger than a typical action potential (0.5-2 msec). Thus, modelingof events during the action potential is typically based on kineticmodels whose behavior is based on extrapolations of kinetics thatare actually measured on a far slower timescale.

Our goal was to directly measure the potassium current flowing during the action potential of hippocampal CA3 pyramidal neuronsand to determine the relative contribution of different channeltypes to the overall current. We performed voltage-clamp experimentsusing experimentally recorded action potentials as the commandwaveform, a procedure that has been used previously in a varietyof cell types to examine the flow of various currents during theaction potential (Llinás et al., 1982; de Haas and Vogel, 1989;Doerr et al., 1989; Zaza et al., 1997; Raman and Bean, 1999).We then used pharmacology to distinguish various components ofthe overall potassium current. Our results fit well with previousstudies in hippocampal pyramidal neurons (Storm, 1987, 1990; Wuand Barish, 1992, 1999) and other excitatory neurons (Locke andNerbonne, 1997a,b; Kang et al., 2000), suggesting that the potassiumcurrents known as I_A and I_D each contribute significantly to therepolarization of the action potential. In addition, we examinedhow the inactivation of I_A and I_D during slow subthreshold depolarizationsaffects their subsequent activation during actionpotentials.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell preparation. Long-Evans rats (postnatal day 5-12) were anesthetized with isoflurane and decapitated, and brains werequickly removed and placed in ice-cold, oxygenated dissociationsolution containing (in mM): 82 Na₂SO₄, 30 K₂SO₄, 5 MgCl₂, 10HEPES, 10 glucose, and 0.001% phenol red, buffered to pH 7.4 withNaOH. Hippocampi were dissected and cut with a McIlwain tissuechopper (Mickle Engineering, Gomshall, UK) into 350-µm-thick slices.The slices were transferred into the dissociation solution with3 mg/ml protease (Sigma type XXIII; Sigma, St. Louis, MO), incubatedat 37°C for 8 min, and then rinsed twice in dissociation solutionwith added 1 mg/ml trypsin inhibitor and 1 mg/ml bovine serumalbumin (at 37°C). After enzyme treatment, the slices were storedin dissociation solution with trypsin inhibitor and bovine serumalbumin at 22°C under a pure oxygen atmosphere. Slices were withdrawnas needed, and the CA3 region was dissected and triturated througha fire-polished Pasteur pipette to release single cells. Hippocampalpyramidal cells were identified morphologically by their largepyramidal shaped cell body (12-16 µM by 20-36 µM) with a thickstump of apicaldendrite.

Recording pipettes. Electrodes were pulled from borosilicate glass micropipettes (VWR Scientific, West Chester, PA) with aSachs-Flaming puller (Sutter Instruments, San Rafael, CA) to yieldresistances between 1 and 1.5 M $Omega$ . To reduce pipette capacitance(and facilitate optimal series resistance compensation), the shanksof the electrodes were wrapped with thin strips of Parafilm (AmericanNational Can, Greenwich, CT) to within several hundreds of micronsof thetip.

Current-clamp recordings. Action potentials were recorded with an Axoclamp 2B amplifier (Axon Instruments, Foster City, CA)in bridge mode. Resting membrane potentials typically ranged from $-$ 45 to $-$ 65 mV. We presume that the less-negative resting potentialsmay reflect depolarization caused by trauma during the isolationor caused by leak around the seal. To elicit full-blown actionpotentials, cells were hyperpolarized to potentials between $-$ 90and $-$ 60 mV with steady injection of DC. Action potentials wereevoked by short (generally 1 msec) current injections so thatthe period of current injection was over before the action potential.Voltage was filtered at 10 kHz (four pole Bessel filter), sampledat an interval of 10-25 µsec using a Digidata 1200A digital-to-analog(D/A) and analog-to-digital (A/D) converter and Clampex7 software(Axon Instruments), and stored on a computer harddisk.

Whole-cell voltage-clamp recordings. Currents were recorded with an Axopatch 200A amplifier (Axon Instruments), filtered witha corner frequency of 10 kHz (four pole Bessel filter), sampledat an interval of 10-50 µsec using a Digidata 1200A D/A and A/Dconverter and Clampex7 software (Axon Instruments), and storedon a computer hard disk. In some cases, currents were later digitallyfiltered with a corner frequency of 1 kHz (boxcar smoothing).Compensation (~80%) for series resistance (typically ~2.5 timeshigher than the pipette resistance) was routinely used. Seal resistanceswere typically 1-4 G $Omega$ , and cells had input resistances between~100 and ~900 M $Omega$ after establishing the whole-cellconfiguration.

Solutions. The standard pipette solution for both current-clamp and voltage-clamp experiments was (in mM): 108 K₂HPO₄, 9 HEPES,9 EGTA, and 4.5 MgCl_2, buffered to pH 7.4 with KOH (Sodicksonand Bean, 1996). To promote the stability of the recordings, 14mM creatine phosphate (Tris salt), 4 mM Mg-ATP, and 0.3 mM Tris-GTPwere included in the pipette solution. Stocks (10×) of the creatinephosphate, ATP and GTP, were stored at $-$ 80°C. Standard externalsolution was Tyrode's solution containing (in mM): 150 NaCl, 4KCl, 2 CaCl₂, 2 MgCl₂, 10 HEPES, and 10 glucose, pH 7.4, withNaOH. Tetrodotoxin (TTX; Calbiochem, La Jolla, CA) was added at0.3-1 µM to block sodium channels. To focus on currents throughvoltage-dependent potassium channels, we blocked calcium entryby replacing external Ca²⁺ with equimolar (2 mM) Co²⁺. We chose Co²⁺ replacement rather than blocking calcium entry with Cd²⁺ or La³⁺, because these both produce dramatic shifts in the voltage dependenceof I_A (Klee et al., 1995). However, even Co²⁺ replacement probably produces a smaller shift of the voltagedependence of I_A in the depolarizing direction compared with Ca²⁺ (Numann et al., 1987); thus, the degree of inactivation of I_Aat subthreshold voltages may be somewhatunderestimated.

After establishing the whole-cell configuration, cells were lifted from the bottom of the recording chamber, and extracellularsolutions were delivered through an array of gravity-fed quartzcapillaries (inner diameter, 145 µm) placed in front of the cell.Stock solutions of TEA (1 M), 4-aminopyridine (4-AP) (1 M), andTTX (0.3 mM) were prepared in deionized water and either storedat 4°C (TEA and 4-AP) or in aliquots at $-$ 20°C (TTX). All reagents,unless noted otherwise, were purchased fromSigma.

Leak subtraction. Correction for linear leak currents was done by subtracting a scaled current elicited by a 10 mV hyperpolarizing(or, at a holding potential of $-$ 110 mV, depolarizing) prepulse.For experiments using action potential waveforms as voltage commands,leak currents were defined by recording the currents in responseto an inverted, scaled-down (by a factor of five) action potentialused as command waveform, delivered from a holding potential of $-$ 80 or $-$ 90mV.

Analysis. Data were analyzed and displayed using ClampFit6 (Axon Instruments), Microcal (Northampton, MA) Origin 5.0, andIgor Pro 3.12 (WaveMetrics, Lake Oswego, OR). All reported voltagesare corrected for a liquid junction potential of $-$ 10 mV betweenthe pipette solution and the Tyrode's solution (in which the pipettecurrent is zeroed before sealing onto a cell), measured as describedby Neher (1992). Statistics are given as mean ±SEM.

All experiments were performed at roomtemperature.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Current-clamp recordings

We began by recording action potentials in the dissociated neurons and examining the effects of various potassium channelblockers on action potential shape. Cells were held at restingpotentials negative to $-$ 60 mV by injecting steady hyperpolarizingcurrent [between 0 and 580 pA, with a mean of 128 (n = 66)], andsingle action potentials were elicited by 1 msec current injections(Fig. 1). The average voltage threshold, measured as the leastdepolarized voltage (just after the current injection) for whichan action potential fired, was $-$ 55 ± 1 mV (66 cells). Analysisof 255 action potentials from 17 cells yielded an average overshootpotential of +31 ± 2 mV, a maximal upstroke of 213 ± 18 mV/msec,a maximal downstroke of $-$ 64 ± 4 mV/msec, and a spike width of1.4 ± 0.1 msec at 0 mV. These are similar to parameters reportedfor intact hippocampal pyramidal cells in brain slices recordedat room temperature (Bergles, 1995).

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Figure 1. Action potentials in an isolated CA3 neuron. The cell was hyperpolarized by steady injection of DC ( $-$ 55 pA), and action potentials were triggered by 1 msec injections of current of increasing amplitude. Bottom panel, The first derivative of the action potentials. External solution was normal Tyrode's solution with 2 mM CaCl₂.

Figure 2 shows the effect of various potassium channel blockers on the action potential. Addition of 4-AP resulted in delayedrepolarization of the action potential (Fig. 2A). With exposureto 30 µM 4-AP, action potentials were 38 ± 10% (n = 7) wider (asmeasured by the area under the curve). At 2.5 mM, 4-AP had a moredramatic effect, increasing the action potential width by 310± 79% (n = 3). Exposure to 25 mM external TEA (Fig. 2B) also producedlarge effects, often leading to a sustained depolarization orplateau near $-$ 40 mV after the action potential. TEA had more pronouncedeffects on the later phases of repolarization than on the earlyphase (from the peak near +40 mV to ~0 mV), whereas 2.5 mM 4-APdramatically affected both phases. Interestingly, the effectson action potential shape of low 4-AP (modest broadening), high4-AP (dramatic broadening, including early phase of repolarization),and TEA (dramatic broadening, but little effect on early phase)in CA3 neurons were very similar to those observed in callosal-projectingrat visual cortical neurons (Locke and Nerbonne, 1997b).

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Figure 2. Effect of potassium channel blockers on action potential shape. A, 4-AP at 30 µM and 2.5 mM produced a dose-dependent delay in repolarization. Hyperpolarizing DC was $-$ 30 pA, and stimulus current (1 msec) was 490 pA. B, TEA at 25 mM had little effect on the initial phase of repolarization but produced a dramatic slowing of late repolarization. Hyperpolarizing DC was $-$ 40 pA, and injected current was 780 pA. C, Replacing external 2 mM calcium with 2 mM cobalt resulted in a delay of firing and little overall change in action potential shape. Action potentials were aligned at the time of maximal upstroke to allow comparison of time course. Hyperpolarizing DC was $-$ 6 pA, and injected current was 850 pA.

In adult hippocampal neurons studied in brain slices, blocking calcium entry or rapidly chelating intracellular calcium significantlyslows the decay of the action potential, suggesting a prominentrole for calcium-activated potassium current in action potentialrepolarization (Storm, 1987; Poolos and Johnston, 1999; Shao etal., 1999). In contrast, in the younger CA3 neurons we studied,removing external calcium (substituting cobalt) had relativelysmall effects on the action potentials (Fig. 2C). Most commonly,the action potential became slightly wider in the initial phaseof repolarization, consistent with a block of a small fractionof calcium-activated potassium current that contributes to initialrepolarization, and slightly narrower in the later phase of repolarization,consistent with removal of a shoulder attributable to net inwardcalcium current. Possibly the role of calcium-activated potassiumchannels would be larger in the absence of the 9 mM EGTA presentin the internal solution, although in adult cells, Storm (1987)found that EGTA was ineffective at disrupting repolarization,in contrast to the faster chelator BAPTA. In subsequent voltage-clampexperiments, we focused on purely voltage-activated potassiumcurrents, using Tyrode's solution in which external Ca²⁺ was replaced by equimolar (2 mM) Co²⁺.

Voltage-dependent potassium currents elicited by step depolarizations

To characterize the components of voltage-dependent potassium currents sensitive to 4-AP and TEA, we began with experimentsusing voltage-clamp protocols using step depolarizations. Figure3 shows a voltage protocol used for one series of experiments,along with representative currents. Currents were elicited inTyrode's solution with 1 µM TTX to block voltage-dependent sodiumcurrents and with external calcium replaced by cobalt to blockvoltage-dependent calcium channels and calcium-activated potassiumcurrents. Voltage steps from $-$ 90 mV to 0 mV activated outwardcurrent consisting of two kinetic components, an early transientpeak, reached within a few milliseconds, and a maintained componentwith little decay for the remainder of a 200 msec test pulse.When a 50 msec prepulse to $-$ 40 mV preceded the test pulse to 0mV, almost all of the initial transient current was removed, leavinga relatively slowly activating, slowly inactivating current (Connorand Stevens, 1971b; Numann et al., 1987; Klee et al., 1995). Subtractionof the current at 0 mV with and without prepulses yielded a currentthat activates quickly (time to peak of 5.2 ± 0.2 msec; n = 33cells) and inactivates completely with a time constant of 15 ±1 msec (n = 33 cells).

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Figure 3. Isolation of I_A by prepulse inactivation. Cells were held at $-$ 90 mV, and the voltage was stepped to 0 mV with or without a prepulse to $-$ 45 mV. There was a 2 msec return to $-$ 90 mV after the prepulse. Subtraction yields fast-activating and fast-inactivating outward current. External solution was 2 mM cobalt Tyrode's solution to block voltage-dependent calcium channels and calcium-activated potassium channels. TTX (1 µM) was included to block voltage-dependent sodium channels. Asterisks indicate records with prepulse. Dotted lines indicate zero current.

Using this protocol to distinguish between these two kinetic components of current, we found that they had different pharmacology.Figure 4A shows the dose-response relationship for inhibitionof these components of current by 4-AP. Application of 4-AP at30 µM had practically no effect on the transient, prepulse-sensitivecomponent of current, and half-block of this component requiredbetween 300 µM and 1 mM 4-AP. Both the kinetic characteristicsof the current and the moderate sensitivity to block by 4-AP ofthe transient current are consistent with identification as A-typepotassium current (I_A). Effects of 4-AP on the maintained, nonprepulse-sensitivecurrent were very different. At 30 µM, 4-AP reduced the sustainedcurrent, measured at the end of a 200 msec test pulse ("late current")by 33 ± 3% (n = 19), and there was only modest additional blockby concentrations $<=$ 3 mM (which blocked by 48 ± 3%; n = 15). Thishigh sensitivity to 4-AP of a slowly inactivating current is consistentwith the potassium current now referred to as I_D described previouslyin hippocampal pyramidal cells (Storm, 1988; Ficker and Heinemann,1992; Wu and Barish, 1992; Bossu et al., 1996; Li and McArdle,1997; Martina et al., 1998) as well as other neurons (McCormick,1991; Surmeier et al., 1991; Locke and Nerbonne, 1997a; Martinaet al., 1998). The additional block of late current at 3 mM 4-APmight reflect the presence of an additional sustained currentcomponent with low 4-AP sensitivity, which most likely representsthe delayed rectifier potassium current I_K (Storm, 1990).

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Figure 4. Differential pharmacological sensitivity of fast-inactivating and slowly inactivating components of potassium current. Currents were elicited by the protocol in Figure 3 using pairs of test pulses to 0 mV with and without prepulses. Filled circles indicate the fast-inactivating component of current obtained by subtraction. Open circles indicate measurement of the current at the end of the step to 0 mV. Inset, top, Superimposed currents with and without prepulse. Bottom, Fast-inactivating component of current obtained by subtraction of these records. Dotted lines indicate zero current.

External TEA at 1 mM had no effect on the transient, prepulse-sensitive current (Fig. 4B). Increasing the concentration ofTEA produced some inhibition, with block of 44 ± 2% at 25 mM TEA(n = 10) of this component of current. The concentration dependenceof TEA sensitivity is consistent with approximately half of thetransient current being sensitive to TEA inhibition, with halfblock of this component by 5 mM TEA. The late current was muchmore sensitive to TEA, with 1 mM TEA producing 39 ± 2% (n = 8)inhibition. Increasing the TEA concentration to 5 mM producedinhibition of 60 ± 5% (n = 6), and there was no additional effectof increasing the concentration to 25 mM (54 ± 6% inhibition;n =10).

The experiment shown in Figure 5 examined in more detail the kinetics of the components of outward current (activated by astep from $-$ 90 to 0 mV) identified by the cumulative applicationof 30 µM 4-AP, 3 mM 4-AP, and 25 mM TEA. The component of currentinhibited by 30 µM 4-AP shows rapid activation kinetics and slowinactivation (~20-30% decay over 200 msec). Both these kineticcharacteristics and the high sensitivity to 4-AP are consistentwith the properties of the current named I_D described in studiesof hippocampal pyramidal cells in brain slices (Storm, 1990).The component of current identified by the further action of 3mM 4-AP shows rapid activation and rapid inactivation. These characteristics,together with the sensitivity of this component to prepulse inactivation(Fig. 3) and its moderate sensitivity to 4-AP, are consistentwith the current component named I_A in hippocampal (Storm, 1990)and other neurons (Rogawski, 1985). The current sensitive to inhibitionby 25 mM TEA (applied in the presence of 3 mM 4-AP) showed slowactivation and no inactivation over 200 msec. These characteristicsare consistent with the delayed rectifier current called I_K (Segaland Barker, 1984; Brown et al., 1990; Locke and Nerbonne, 1997).Our functional definition of I_K was based on applying TEA afterI_A had been blocked by 3 mM 4-AP, because there was some TEA sensitivityof the inactivating, prepulse-sensitive current (which is probablyprimarily I_A). There was a small component of outward currentremaining with 3 mM 4-AP and 25 mM TEA; we did not attempt tofurther characterize this current.

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Figure 5. Strategy for pharmacological separation of I_A, I_D, and I_K. Left panel, Sequentially recorded traces obtained in control solution (2 mM cobalt Tyrode's solution with 1 µM TTX) and in the presence of 30 µM 4-AP, 3 mM 4-AP, and 3 mM 4-AP plus 25 mM TEA. Right panel, Subtracted currents sensitive to 30 µM 4-AP (I_D), 3 mM 4-AP but not 30 µM 4-AP (I_A), and 25 mM TEA but not 3 mM 4-AP (I_K). Horizontal dotted lines indicate zero current.

Together, these results are consistent with three distinct components of voltage-activated potassium current in isolated CA3neurons. One current is rapidly inactivating and prepulse sensitiveand is weakly sensitive to 4-AP. One is very sensitive to 4-AP,slowly inactivating, and not sensitive to a prepulse. A thirdis sensitive to external TEA, slowly inactivating, and not prepulsesensitive. These correspond well to the currents named I_A, I_D,and I_K described previously in studies of hippocampal pyramidalcells in brain slices (Storm, 1990) and cultured neurons (Wu andBarish, 1992, 1999). These three major components of voltage-activatedpotassium current in CA3 neurons seem nearly identical to thecomponents of potassium current distinguished in detailed studieson CA1 pyramidal neurons (Martina et al., 1998) as well as anothercentral excitatory projection neuron, callosal-projecting visualcortical neurons (Locke and Nerbonne, 1997a).

Voltage-dependent potassium currents elicited by action potential waveforms

We subsequently examined currents elicited under voltage clamp using an action potential recorded previously as the commandvoltage. With unmodified Tyrode's solution, the ionic currentelicited by the action potential waveform (Fig. 6A) consistedof a large inward current during the upstroke of the action potentialfollowed by a large outward current during the repolarizationphase of the action potential (Fig. 6B). The relationship betweenthe elicited current and the voltage trajectory during the actionpotential is seen by plotting the elicited current as a functionof the voltage during the action potential (Fig. 6C). The inwardcurrent was completely blocked by TTX, suggesting that the upstrokeof the action potential is entirely caused by TTX-sensitive sodiumcurrent (although calcium channels were not blocked in this experiment).Application of TTX had no effect on the outward current afterthe peak of the action potential, consistent with inactivationof the sodium current being complete before the falling phaseof the action potential. With the outward current isolated afterblock of sodium current, it can be seen that the activation ofthe outward current during the action potential is very abrupt.There is almost no current activated during the upstroke of theaction potential until a voltage of approximately +30 mV is achieved(0.42 msec after the start of the action potential, counting fromthe time the voltage crosses the threshold of $-$ 55 mV). The outwardcurrent increases very rapidly during the time that the actionpotential is near its peak, increasing from ~1 to 6 nA in 0.46msec, during which time the voltage rises from +40 to +55 mV andback to + 40 mV. The outward current then declines smoothly duringthe falling phase of the action potential, reflecting both thedecrease in driving force for potassium ions and also deactivationof potassium channels.

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Figure 6. Ionic current elicited by action potential waveform clamp. A, Command waveform, consisting of a previously recorded action potential (peak, +51 mV; maximal upstroke, +435 mV/msec; maximal downstroke, $-$ 62 mV/msec). B, Ionic currents elicited by the action potential waveform in normal Tyrode's solution (containing 2 mM CaCl₂) and after application of 1 µM TTX. C, Ionic currents plotted as a function of voltage during the action potential.

Experiments examining action potential-elicited currents require good voltage control of large currents with rapid kinetics.Evidence for good voltage control comes from the lack of differencein outward currents when the large inward sodium current is blocked.If there were series resistance errors or other loss of voltagecontrol, the voltage seen by the cell would be artifactually depolarizedduring the flow of sodium current, resulting in larger potassiumcurrents. Such effects were seen if higher resistance pipettesor inadequate series resistance compensation wereused.

Sodium-activated potassium currents have been reported in some neurons (Dryer, 1994). The experiment in Figure 6 shows thatsuch a current does not contribute significantly to repolarizationof the action potential in CA3 neurons, because total potassiumcurrent was unchanged when sodium influx wasblocked.

We used the pharmacological manipulations developed with step depolarizations to determine the contribution of various componentsof potassium current to the overall outward current elicited bythe action potential waveform. An example is shown in Figure 7.Application of 30 µM 4-AP inhibited the peak outward current by38 ± 2% (n = 22), and application of 3 mM 4-AP inhibited the peakcurrent by 84 ± 2% (n = 20). Adding 25 mM TEA (in the continuingpresence of 4-AP) had relatively little effect, producing a detectableamount of additional block in 6 of 11 cells (~2% of the peak controlcurrent). An alternative way to quantify the components of outwardcurrents during the action potential is to examine the total chargecarried by the various components of current, obtained by integratingthe current over the course of the action potential waveform.Based on this analysis, the contributions to the overall chargeby I_D, I_A, and I_K were 39 ± 2% (n = 22), 49 ± 2% (n = 20), and2 ± 1% (n = 11), respectively. A total of 11 ± 2% (n = 11) remainedunblocked by the combination of 3 mM 4-AP and 25 mM TEA.

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Figure 7. Pharmacological dissection of potassium current elicited by action potential waveform. A, Current elicited by action potential waveform in Tyrode's solution with calcium replaced by cobalt to eliminate voltage-activated calcium current and with 1 µM TTX to block sodium current. Action potential (peak, +30 mV; maximal upstroke, +135 mV/msec; maximal downstroke, $-$ 50 mV/msec) was recorded previously in normal Tyrode's solution. To separate I_A, I_D, and I_K, 4-AP and TEA were applied according to the strategy summarized in Figure 5. B, I_A, I_D, and I_K obtained by subtraction. I_D was obtained as the current sensitive to 30 µM 4-AP, I_A as the current sensitive to 3 mM 4-AP but not 30 µM 4-AP, and I_K as the current sensitive to 25 mM TEA but not 3 mM 4-AP.

Figure 7B plots I_D and I_A as a function of the voltage during the action potential. The pattern of flow of I_D and I_A duringthe action potential waveform was very similar. As for total outwardcurrent during the action potential, both showed negligible activationbefore the peak of the action potential was reached (in this case,near +30 mV) and rapid activation immediately after the peak.The similar kinetics of I_D and I_A during the action potentialis consistent with the rapid activation kinetics of both duringstep depolarizations. In addition, both I_D and I_A decayed at approximatelythe same rate during the falling phase of the action potential.Given the difference in inactivation kinetics of the two channels,this suggests that the decrease in the current can be attributedprimarily to deactivation and, to a lesser extent, to a decreasein the driving force on potassium ions (approximately twofoldgreater at 0 mV than $-$ 45mV).

How complete is activation of potassium channels during the action potential? Does activation reach completion before deactivationbegins? We approached this question by testing whether maintainingthe depolarization of an action potential produced larger currents(Fig. 8). The activation of I_D and I_A is particularly interestingin this context, so we isolated total I_D and I_A by block with3 mM 4-AP. The voltage command consisted of a partial action potential,interrupted and extended at a voltage of +10 mV on the fallingphase. This is the point on the action potential at which maximaloutward current is normally reached. Extending the action potentialresulted in a substantial increase in I_D and I_A. Peak currentwas reached after another ~3 msec at +10 mV and was more thantwice that reached on initially reaching +10 mV on the fallingphase of the action potential. Thus, in aggregate, I_A and I_D are<50% fully activated during the action potential. In four experimentsusing this protocol, activation of I_A and I_D during the actionpotential was 46 ± 9% of that achieved with extended step to +10mV.

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Figure 8. Assay of extent of activation of I_A and I_D during an action potential. Total I_A and I_D were isolated as current sensitive to 3 mM 4-AP. Voltage command consisted of a partial action potential interrupted and extended at +10 mV on the falling phase. Current reached at +10 mV during the falling phase was 0.95 nA, compared with a peak of 2.23 nA reached ~3 msec later at the same voltage. The vertical dashed line indicates time at which falling phase of action potential reaches +10 mV; the horizontal dashed line indicates outward current at this time.

The experiment in Figure 8 also suggests that there is little or no inactivation of I_D and I_A during a single action potential,because decay of the combined current is not detectable untilthe action potential has been extended for ~3 msec at +10 mV,approximately three times its normalduration.

Activation of I_A and I_D preceding a spike

Both I_A and I_D are believed to be activated at subthreshold potentials and to contribute to delayed firing of action potentialsduring slow approaches to threshold (Connor and Stevens, 1971a;Segal et al., 1984; Storm, 1988). Because of the slow inactivationof I_D, this effect can last $<=$ 10 sec (Storm, 1988). As in studieson more intact cells, we observed delayed firing when thresholdwas approached slowly in isolated CA3 neurons. Figure 9 showsan example in which action potentials were evoked by long (400msec) injections of current. The delay of the first spike wasdetermined for the least depolarizing current injection that causedaction potential firing. In 42 experiments from 31 cells, thetime to peak for the first spike ranged from 40 to 350 msec witha mean value of 49 msec. This is considerably longer than theaverage membrane time constant of 12 ± 11 msec (mean ± SD), suggestingthat the delay reflects more than the time required to reach threshold.In 20% of the experiments, the time to peak for the first spikewas >86 msec. This cutoff represents three times the mean membranetime constant plus 50 msec (approximately the time for I_A to activateand inactivate). In the example in Figure 9, the membrane wascharged to a subthreshold voltage of $-$ 58 mV after current injection.An ~200 msec delay followed, during which the voltage first hyperpolarizedand then depolarized until threshold was reached, and an actionpotential was fired. This sequence is consistent with a sequenceof activation and inactivation of potassium current, presumablysome combination of I_A and I_D, at subthreshold voltages.

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Figure 9. Delayed firing of an action potential near threshold. An action potential elicited near threshold with stimulation by 400 msec steps of current is shown. Note relaxation from initial depolarization, followed by a second phase of depolarization and then spike firing. Spike occurs 203 msec after start of current step. The dashed line indicates voltage reached during initial depolarizing phase ( $-$ 58 mV).

The experiments like that shown in Figure 9 fit well with previous results in recordings from hippocampal pyramidal neuronsin brain slices, suggesting that delayed firing of action potentialscan result from activation and inactivation of I_A and I_D at subthresholdvoltages. How complete is this inactivation? This is an especiallyinteresting question in light of the fact that I_A and I_D are alsothe major currents contributing to the repolarization of the actionpotential. If inactivation were complete during slow approachto threshold, the repolarization of the resulting action potentialsmight be greatly altered. Therefore, we examined the time courseof inactivation of I_A and I_D at relevant voltages. We used voltage-clampprotocols in which the action potential command waveform was precededby a prepulse of increasing duration. 4-AP and TEA were used topharmacologically separate and quantitatively assess I_A and I_D.As shown in Figure 10, there is substantial but incomplete suppressionof I_A and I_D by rectangular prepulses to $-$ 45 mV (the thresholdpotential) of $<=$ 3 sec duration. As expected from their kinetics,I_A is affected more rapidly and to a greater extent than I_D.

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Figure 10. Partial inactivation of I_A and I_D by prepulses to $-$ 45 mV. A, Currents were elicited by an action potential waveform preceded by a variable length prepulse to $-$ 45 mV, from a steady holding potential of $-$ 70 mV. Arrows indicate variable length of prepulse (0-3000 msec). B, I_D (obtained as fraction of current sensitive to 30 µM 4-AP) elicited by the action potential after prepulses of indicated lengths. C, I_A (obtained as fraction of current sensitive to 3 mM 4-AP but not 30 µM 4-AP) elicited by the action potential after prepulses of indicated lengths. External solution was 2 mM cobalt Tyrode's containing 1 µM TTX. Dashed lines indicate zero current.

Some depolarizing voltage trajectories that were observed to occur preceding a spike do not resemble a rectangular voltagestep but gradually lead up to threshold. Therefore, we also testedthe extent of inactivation of I_A and I_D with a depolarizing rampof increasing duration, up to a threshold voltage of $-$ 45 mV, andcoupled to the action potential command waveform (Fig. 11). Whenpreceded by a depolarizing ramp to threshold, I_A and I_D flowingduring a subsequent action potential were both reduced, with considerablymore effect on I_A than I_D. These data are summarized in Figure12. Both prepulse protocols induced substantial inhibition of eithercurrent, with the square pulse inducing greater attenuation. Inboth cases, the time dependence was faster for I_A than for I_D,and inactivation of both potassium currents was incomplete. Asteady state of I_A peak current amplitude was reached at 31% (squareprepulse) and 45% (ramp) of control. Conversely, inactivationof I_D saturated at 59% (square prepulse) and 75% (ramp) of control.These findings show that even sustained depolarizations to potentialsclose to threshold produce only partial inactivation of I_D andI_A, leaving a substantial fraction of these rapid rectifiers availablefor repolarization of the ensuing action potential.

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Figure 11. Partial inactivation of I_A and I_D by ramps preceding the action potential. Currents were elicited by an action potential waveform preceded by ramps (of variable lengths from 0 to 300 msec) from $-$ 70 mV to $-$ 45 mV (top panel). I_D (middle panel) was obtained as the fraction of current sensitive to 30 µM 4-AP elicited by the waveforms. I_A was obtained as the fraction of current sensitive to 3 mM 4-AP but not 30 µM 4-AP. External solution was 2 mM cobalt Tyrode's containing 1 µM TTX.

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Figure 12. Time course of reduction of I_D and I_A by prepulses or ramps to threshold potentials. A, Normalized peak current of I_D ( $open circle$ ; n = 3) or I_A (; n = 4) elicited by the action potential waveform is plotted against the duration of a step depolarization to $-$ 45 mV. Error bars show mean ± SEM. Fitted curves are single exponential functions. I_D, Time constant of 282 msec; steady-state, 59%. I_A, Time constant of 75 msec; steady-state, 31%. B, Normalized peak current of I_D ( $open circle$ ; n = 7) or I_A (; n = 9) elicited by the action potential waveform is plotted against the duration of a depolarizing ramp as in Figure 11. I_D, Time constant of 183 msec; steady-state, 75%. I_A, Time constant of 94 msec; steady-state, 45%.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previous voltage-clamp studies using brain slices, cultured neurons, and acutely isolated neurons have identified three principalvoltage-activated potassium currents in hippocampal pyramidalneurons: I_A, I_D, and I_K (Gustafsson et al., 1982; Segal and Barker,1984; Zbicz and Weight, 1985; Lancaster and Adams, 1986; Numannet al., 1987; Sah et al., 1988; Storm, 1988; Lancaster et al.,1991; Klee et al., 1995; Bossu et al., 1996). Our results fitwell with these previous studies in finding that most of the voltage-activatedpotassium current can be assigned to these three components, eachidentified with a particular pharmacological and kinetic profile.The component identified as I_D is highly sensitive to 4-AP, fastactivating, and slowly inactivating. I_A is weakly sensitive to4-AP, fast activating, and fast inactivating. I_K is sensitiveto external TEA, slowly activating, and virtuallynoninactivating.

Our results suggest that essentially all of the potassium current underlying repolarization of single action potentials inhippocampal CA3 neurons comes from I_D and I_A, with approximatelyequal contributions of each. The participation of I_D in actionpotential repolarization agrees with previous results showingeffects of low concentrations of 4-AP on action potential widthin hippocampal pyramidal neurons (Storm, 1988; Wu and Barish,1992). Besides contributing nearly equal amounts of current duringthe action potential, I_D and I_A seem interchangeable (at leastduring the spike itself) in that they follow nearly identicaltrajectories of voltage- and time-dependent activation and deactivationduring the action potential (Fig. 7). In both cases, the declineof current during the later phases of the action potential appearsto be primarily attributable to deactivation (along with the decreaseddriving force) rather than inactivation, because there is verylittle inactivation of either current even if the action potentialis artificially prolonged several-fold (Fig. 8). The lack of substantialinactivation of I_A during a single spike is consistent with theobservation of Keros and McBain (1997) that arachidonic acid speedsinactivation of I_A but does not affect spike width. It is alsointeresting that there is a significant surplus capability ofpotassium current from I_D and I_A during a single spike in thatthe combined current reaches only ~40% of maximal activation (Fig.8). However, our experiments were performed at room temperature,and it is possible that at physiological temperature, the degreeof activation of both I_D and I_A during a spike might be higher.Both the participation of two different channel types and thereserve capability can be considered safety factors tending toensure rapidrepolarization.

It is possible to make working hypotheses for the molecular basis of the potassium channel subunits making up the variouscomponents of potassium current in hippocampal pyramidal neurons.Kv2.1 is a likely candidate for I_K, because Murakoshi and Trimmer(1999) found that delayed rectifier current could be inhibitedby intracellular application of antibodies to Kv2.1, and Du etal. (2000) showed that treatment of CA1 neurons with antisenseoligonucleotides directed against Kv2.1 reduced a delayed rectifiersimilar to the I_K component in dissociated neurons. The lack ofeffect on single spike width of antisense treatment (Du et al.,2000) fits well with our finding of negligible activation of I_Kduring an action potential. In agreement with the pharmacologyof I_K, Kv2.1 channels expressed heterologously in mammalian cellsare blocked only weakly by 4-AP, with a half-blocking concentrationof 3 mM (Shi et al., 1994). The kinetic and pharmacological propertiesof I_K as we recorded it in acutely isolated CA3 neurons matchvery well with those of a corresponding component of potassiumcurrent in nucleated patches from CA1 pyramidal neurons in brainslice (Martina et al., 1998) proposed to correspond to Kv2 channels.Because CA1 pyramidal neurons express Kv2.2 as well as Kv2.1 subunits(Martina et al., 1998), it is very possible that the channelsunderlying I_K might be heteromultimers (Du et al., 2000).

Kv4 family subunits are likely candidates for channels contributing to I_A. CA3 pyramidal neurons express both Kv4.2 and Kv4.3subunits (Serodio and Rudy, 1998). In several types of centralneurons that have been examined, the amplitude of I_A is correlatedwith the level of expression of mRNA for Kv4.2 subunits (Songet al., 1998; Tkatch et al., 2000), and in both sympathetic neurons(Malin and Nerbonne, 2000) and cerebellar granule neurons (Shibataet al., 2000), I_A is eliminated or greatly reduced by transfectionwith dominant negative Kv4.3 subunits, expected to eliminate currentsfrom all Kv4 family channels. In CA1 neurons, which, unlike CA3neurons, do not express significant levels of Kv4.3 (Serodio andRudy, 1998), both expression of Kv4.2 immunoreactive protein andI_A are dramatically reduced in regions of heterotopia inducedby prenatal injections of methylazoxymethanol, consistent witha major role for Kv4.2 subunits in the generation of I_A (Castroet al., 2001). As in a subset of sympathetic neurons (Malin andNerbonne, 2001), a component of I_A in CA3 neurons might also originatefrom Kv1 family subunits, which, together with $beta$ 1 subunits, canproduce an I_A-like current (Rettig et al., 1994); this might accountfor the component of I_A blocked weakly byTEA.

The molecular identification of I_D in hippocampal pyramidal neurons is less certain. This current has kinetic properties offast activation and slow inactivation and is blocked by 30 µM4-AP. These properties would fit with channels made by Kv3.1 subunits(Grissmer et al., 1994; Martina et al., 1998), but few hippocampalpyramidal neurons appear to express detectable levels of Kv3.1subunits (Weiser et al., 1995; Martina et al., 1998; Du et al.,2000). Channels formed by Kv1.5 subunits are also candidates forI_D in hippocampal pyramidal neurons. Kv1.5 polypeptides are expressedin the cell bodies of CA3 neurons (Maletic-Savatic et al., 1995)and can underlie rapidly activating, slowly inactivating currentswith high sensitivity to 4-AP (London et al., 2001).

In addition to their role in action potential repolarization, it is believed that both I_A and I_D can undergo a sequence ofpartial activation and inactivation at subthreshold voltages andthus tend to produce a delay in spike firing (Connor and Stevens,1971a; Segal et al., 1984; Storm, 1988; Luthi et al., 1996). Indeed,in our experiments on isolated neurons, such a delay of actionpotential firing was observed when just enough sustained currentwas injected to depolarize the membrane to threshold (Fig. 9).Although the roles of I_A and I_D in spike repolarization appearto be interchangeable, this is unlikely to be true of their rolesat subthreshold voltages, where differences in inactivation ratesand completeness are expected to have more significant functionaleffects. At subthreshold voltages, we found that inactivationof I_A was both faster and more complete than that of I_D. We didnot attempt to resolve activation of I_A and I_D during the lead-upto action potentials. In principle, such currents might be smallif channels can inactivate at subthreshold voltages without firstactivating. This is true for cloned Kv4.2 channels (Bähring etal., 2001), but this important issue has apparently not yet beenexplored for native I_A and I_D in central neurons. The nonmonotonicchange in voltage during the lead up to the action potential withjust-threshold current injections suggests that one or both currentsundergo partial activation followed by inactivation, but the currentsneeded to produce the changes in subthreshold voltage are probablyjust a fewpicoamperes.

One consequence of having two different channel types contributing equally to repolarization is to minimize effects on repolarizationrate when either current is reduced. This may be especially importantbecause both I_D and I_A also play roles in subthreshold phenomena.Thus, one current can undergo a cycle of partial activation andinactivation leading up to the spike without resulting in eliminationof the current available for repolarizing the spike. Because I_Aand I_D contribute approximately equally to the current underlyingrepolarization, we can observe the consequences of reducing thiscurrent by half by examining the effects of 30 µM 4-AP, whichblocks I_D but not I_A. This resulted in a relatively modest broadeningof the action potential. In adult pyramidal neurons, calcium-activatedpotassium current through BK channels also contributes significantlyto repolarization (Storm, 1987; Poolos and Johnston, 1999; Shaoet al., 1999), which would further minimize the effects on spikerepolarization of reducing either I_D and I_Aalone.

Both I_D and I_A are known to be modulated by transmitters and second messenger systems (Nakajima et al., 1986; Deadwyler etal., 1995; Keros and McBain, 1997; Hoffman and Johnston, 1998;Colbert and Pan, 1999; Wu and Barish, 1999; Mu et al., 2000; Lienet al., 2002). The redundancy of their roles in spike repolarizationmeans that modulation of either one may be able to produce significantfunctional effects at subthreshold voltages without compromisingrapid spikerepolarization.

  FOOTNOTES

Received April 11, 2002; revised Sept. 9, 2002; accepted Sept. 10, 2002.

This work was supported by National Institutes of Health Grants NS36855, NS38312, and HL35034 and by Fonds zur Förderungder wissenschaftlichen Forschung Grant J1853-MED. We thank Dr.Marco Martina for comments on thismanuscript.

Correspondence should be addressed to Bruce P. Bean, Department of Neurobiology, Harvard Medical School, 220 Longwood Avenue,Boston, MA 02115. E-mail: Bruce_Bean{at}hms.harvard.edu.

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