Differential Expression of K4-AP Currents and Kv3.1 Potassium Channel Transcripts in Cortical Neurons that Develop Distinct Firing Phenotypes

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Volume 17, Number 9, Issue of May 1, 1997 pp. 3136-3147
Copyright ©1997 Society for Neuroscience

Differential Expression of K_4-AP Currents and Kv3.1 Potassium Channel Transcripts in Cortical Neurons that Develop Distinct Firing Phenotypes

Jennifer L. Massengill, Martin A. Smith, Dong Ik Son, and Diane K. O'Dowd
Departments of Anatomy and Neurobiology and Developmental and Cell Biology, University of California, Irvine, California 92697-1280

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Maturation of electrical excitability during early postnatal development is critical to formation of functional neural circuitryin the mammalian neocortex. Little is known, however, about thechanges in gene expression underlying the development of firingproperties that characterize different classes of cortical neurons.Here we describe the development of cortical neurons with twodistinct firing phenotypes, regular-spiking (RS) and fast-spiking(FS), that appear to emerge from a population of immature multiple-spiking(IMS) neurons during the first two postnatal weeks, both in vivo(within layer IV) and in vitro. We report the expression of aslowly inactivating, 4-AP-sensitive potassium current (K_4-AP)at significantly higher density in FS compared with RS neurons.The same current is expressed at intermediate levels in IMS neurons.The kinetic, voltage-dependent, and pharmacological propertiesof the K_4-AP current are similar to those observed by heterologousexpression of Kv3.1 potassium channel mRNA. Single-cell RT-PCRanalysis demonstrates that PCR products representing Kv3.1 transcriptsare amplified more frequently from FS than RS neurons, with anintermediate frequency of Kv3.1 detection in neurons with immaturefiring properties. Taken together, these data suggest that theKv3.1 gene encodes the K_4-AP current and that expression of thisgene is regulated in a cell-specific manner during development.Analysis of the effects of 4-AP on firing properties suggeststhat the K_4-AP current is important for rapid action potentialrepolarization, fast after-hyperpolarization, brief refractoryperiod, and high firing frequency characteristic of FS GABAergicinterneurons.
Key words: Kv3.1 mRNA; potassium currents; cortical neurons; development; single cell RT-PCR; fast spiking; regular spiking; mouse somatosensory cortex; firing properties

INTRODUCTION

The adult mammalian neocortex is a complex neural network in which regular-spiking (RS) glutamatergic neurons and fast-spiking(FS) GABAergic neurons are principal components (Connors and Gutnick,1990). Therefore, a determination of the mechanisms that underliematuration of the characteristic firing properties of these neuronsis critical for understanding the development of normal brainfunction. Previous studies in rodents have reported the appearanceof neurons with RS and FS firing properties during the first twopostnatal weeks (McCormick and Prince, 1987; Lorenzon and Foehring,1993; Zhou and Hablitz, 1996); however, the questions of whendistinct firing phenotypes are first seen and what cell-specificpatterns of neuronal ion channel gene expression are responsiblefor the appearance of these distinct firing patterns are stilllargely unanswered.

As a first step toward answering these questions we have characterized the changes in firing properties of neurons in layerIV of the mouse somatosensory cortex during early postnatal development.Previous studies have demonstrated both GABA (Keller and White,1987; Del Rio et al., 1992) and glutamate (Conti et al., 1987)immunoreactivity within this layer, predicting the presence ofneurons with FS and RS firing phenotypes. In this study we demonstratethat layer IV neurons with FS and RS phenotypes emerge from apopulation of immature multiple-spiking (IMS) neurons during thefirst two postnatal weeks. In a parallel series of experiments,we observed a similar pattern of electrophysiological maturationin a more heterogenous population of cortical neurons developingin dissociated cell culture. These data are consistent with thepossibility that differentiation of neurons with FS and RS firingproperties are mediated by similar mechanisms in all corticallayers.

A second series of experiments was performed to identify cell-specific changes in ion channel expression underlying maturationof FS and RS firing phenotypes in cortical neurons. Previous studieshave shown that developmental regulation of voltage-gated potassiumcurrents plays an important role in the maturation of neuronalfiring properties in a number of systems (Ribera and Spitzer,1992). Therefore, electrophysiological and pharmacological techniqueswere used to identify potassium currents that were differentiallyexpressed in cultured neurons with specific firing properties.We were also interested in determining which genes encoded differentiallyexpressed ion channels. Recent studies using single-cell RT-PCRin cortical neurons showed that firing properties can be correlatedwith specific patterns of ion channel gene expression in neuronsfrom the adult rodent neocortex (Jonas et al., 1994; Lambolezet al., 1996). Using a similar strategy we examined the frequencyof expression of the voltage-gated potassium channel gene Kv3.1in developing cortical neurons. Our results suggest that upregulationin the expression of a 4-AP-sensitive potassium (K_4-AP) currentencoded by Kv3.1 mRNA plays a role in the development of a numberof electrophysiological properties unique to FS GABAergic neurons.

MATERIALS AND METHODS
Acute slice preparation. Neonatal ICR mice between the day of birth (PO) and postnatal day 14 (P14) were used for electrophysiologicalrecordings in acute slice preparations. Pups were anesthetizedon ice (<P5) or with halothane ( $>=$ P5) before decapitation. Brainswere removed in ice-cold artificial cerebral spinal fluid (ACSF)containing (in mM): 126 NaCl, 3 KCl, 1.25 NaH₂PO₄, 1.3 MgSO₄,26 NaHCO₃, 10 D-glucose, 2.5 CaCl₂. Coronal sections (400 µM)were cut through the somatosensory cortex in ACSF using a vibraslicer(Campden Instruments), transferred to a recording chamber, andperfused with oxygenated ACSF at room temperature until recordingswere made.

Preparation of cultures. Neuronal cultures were prepared using a procedure modified from Baughman and colleagues (Baughmanet al., 1991). P0 pups were anesthetized for ~1 min on ice beforedecapitation. Brains were removed in ice-cold balanced salt solution(BSS) containing (in mM): 137 NaCl, 5.3 KCl, 0.15 Na₂HPO₄, 0.2KH₂PO₄, 9.8 HEPES, 33.3 glucose, 43.8 sucrose. Coronal sections(600 µM) were cut through the somatosensory cortex using a vibraslicer.Small pieces of somatosensory cortex (1 mm) from a single mousewere incubated in BSS containing 10 U/ml papain (LS03126, WorthingtonBiochemical, Freehold, NJ) activated by L-cysteine (1.32 mM) (C-7755,Sigma, St. Louis, MO) along with 5 mM D( $-$ )-2-amino-5-phosphonopentanoicacid (APV), and maintained at 37°C in a humidified incubator for30 min. The tissue was washed briefly in 5 ml of BSS, twice in1.5 ml of BSS containing 5 mM APV, 1.0% BSA, 1.0% trypsin inhibitor(1.5 min/wash), and three times in 2.5 ml of BSS containing 5mM APV, 0.1% BSA, 0.1% trypsin inhibitor (1.5 min/wash). Tissuewas rinsed two times in 5 ml of neurobasal medium with B27 supplements(NBM+B27) (Life Technologies, Gaithersburg, MD), mechanicallytriturated through glass micropipettes, dispersed onto poly-D-lysine-coatedglass coverslips, and maintained at 37°C in a humidified 5.0%CO₂ incubator overnight. On the following day the coverslips weretransferred, cell side up, to dishes containing confluent non-neuronalfeeder layers in NBM+B27. Coverslips were subsequently transferredto new feeder cultures every 3-5 d. Neurons preferentially surviveand differentiate in NBM+B27, and in all cases the majority ofcells on coverslips prepared in this fashion was neuronal, onthe basis of morphological and electrophysiological criteria.A small number of non-neuronal cells, however, were present inthe older cultures.

Non-neuronal feeder cultures were prepared from whole cortices obtained from mice at P0-P3. Cortices were removed and placedin ice-cold BSS, manually chopped into 2-3 mm pieces with a razorblade, and dissociated in enzyme solution as described for theneuronal cultures. Tissue was washed three times in 5 ml BSS,two times in 5 ml minimal essential medium (MEM) + 10% fetal calfserum (1 min/wash), mechanically dissociated, and plated ontopoly-D-lysine-coated plastic tissue-culture dishes. Non-neuronalcultures were fed by replacing the MEM + 10% fetal calf serumevery 4 d. In preparation for the neuronal transfers, the MEM+ 10% fetal calf serum medium in confluent dishes was replacedwith NBM+B27 24 hr before transfer.

Electrophysiological recordings. Electrophysiological recordings were obtained using the whole-cell configuration of the patch-clamptechnique (Hamill et al., 1981) in either current-clamp or voltage-clampmode. Recording pipettes were unpolished, with open pipette resistancesof 2-5 mOhm. The internal pipette solution contained (in mM):0.1 CaCl₂, 2 MgCl₂, 1.1 EGTA, 10 HEPES, 120 K⁺-gluconate, 20 NaCl, pH 7.2. The external solution contained (inmM): 140 NaCl, 4 MgCl₂, 5 HEPES, 1 CaCl₂, 3 KCl, pH 7.2. The followingdrugs were added to the external solutions to block specific voltage-gatedcurrents: Na⁺ currents: 1 µM tetrodotoxin (TTX) (RBI); K_4-AP currents: 10-100µM 4-AP (RBI) or 100-200 µM tetraethylammonium (TEA) (RBI); Ca²⁺ and K_Ca²⁺ currents: 2 mM cobalt. To examine recording stability, leak currentswere monitored after each solution change. Voltage-gated currentswere analyzed only if leak currents remained unchanged. Data werecollected and analyzed using a List EPC-7 patch-clamp amplifier,Dell 386/486 computers, and pCLAMP software (Axon Instruments,v 5.5.1). All recordings were performed at room temperature.

Lucifer yellow fills. To intracellularly label neurons recorded from slices, 0.5% Lucifer yellow/K⁺-salt was added to the recording pipette. Dye was allowed to fillthe cell by passive diffusion. After electrophysiological recording,slices were fixed with 4% paraformaldehyde (in 0.1 M PB) and clearedin methylsalicylate. Filled neurons were imaged using a confocalmicroscope.

RT-PCR. The presence of Kv3.1 mRNA in RNA isolated from adult mouse brain or cultured somatosensory cortical neurons was determinedby RT-PCR. Total RNA was isolated from brain or cultured neuronsby the single-step method of Chomczynski and Sacchi (1987). First-strandcDNA was synthesized by random-primed RT of 100-200 ng of totalRNA as described previously (O'Dowd et al., 1995), followed bytwo rounds of amplification using nested primers. Oligonucleotideprimer pairs F1/B1 and F2/B2 corresponding to 1422-1445/1647-1626bp and 1447-1467/1581-1559 bp of the published sequence (Yokoyamaet al., 1989) were used to specifically amplify Kv3.1 mRNA. PCRproducts, labeled by inclusion of ~5 × 10⁵ cpm of ³²P-labeled forward primer F2 in the second PCR were separated byelectrophoresis on 8% nondenaturing polyacrylamide gels and visualizedby film autoradiography or phosphor-imager analysis (MolecularDynamics, Sunnyvale, CA).

RT-PCR analysis of Kv3.1 mRNA expression was also performed on RNA harvested from single cells as described previously (Smithand O'Dowd, 1994; O'Dowd et al., 1995). Briefly, after acquisitionof electrophysiological records using the whole-cell patch-clamptechnique, mild suction was used to aspirate the contents of thecell into the tip of the recording electrode that were then expelledinto first-strand cDNA synthesis buffer. First-strand cDNA wasinitiated by the addition of 100 U of Moloney's murine leukemiavirus reverse transcriptase, and the reaction was allowed to proceedfor 1 hr at 37°C. After termination of the first-strand reaction,the resulting cDNA was subjected to two rounds of amplificationusing the nested primers F1/B1 and F2/B2, and the products wereanalyzed by gel electrophoresis and autoradiography, as describedabove, for the analysis of Kv3.1 transcripts in RNA isolated frombrain or cultured cells. The sequence of the PCR product amplifiedfrom RNA harvested from cultured neurons at 6 d in vitro (DIV)was determined using an fmol sequencing kit (Promega, Madison,WI) with an end-labeled primer protocol.

RESULTS

Development of layer IV cortical neurons with FS and RS phenotypes
Our initial experiments focused on a developmental analysis of the firing properties of layer IV neurons in the somatosensorycortex of mouse during the first two postnatal weeks. Whole-cellrecordings were obtained, using the blind-patch technique (Blantonet al., 1989), from 95 layer IV neurons in coronal slices throughsomatosensory cortices prepared from 35 mice, ages P4-P14. Neuronswithin layer IV were targeted by positioning the pipette overthe barrel structures visualized by transillumination of the livingslice (Fig. 1A). To confirm that this method resulted in recordingsfrom cells in layer IV, Lucifer yellow was included in the intracellularrecording solution in some experiments. Subsequent confocal analysisrevealed that 16/17 neurons labeled in this manner were locatedin layer IV, two of which are illustrated in Figure 1B. Althoughthe majority of recordings was from neurons with their cell bodieswithin layer IV, current clamp recordings from ~10% of the cellswere characterized by small spikes riding on a slow depolarizingwave, consistent with the recording electrode being located onthe dendrites (Kim and Connors, 1993). Because it was possiblethat these were recordings from neurons whose cell bodies werelocated in other layers, these records were not analyzed further.
Fig. 1. A, Layer IV is identified by the presence of barrels visualized by transillumination of a 400-µm-thick living slice throughP7 mouse somatosensory cortex. Large arrowheads delineate dorsaland lateral extents of the barrel cortex in this slice. Scalebar, 1 mm. B, Morphology of two stellate neurons located in thesame barrel of a P11 slice, visualized with confocal microscopy.The two cells were independently filled with separate whole-cellrecording pipettes that contained 0.5% Lucifer yellow in the internalsolutions. Pial surface is toward the top of this collapsed compositephotograph (individual images were taken at 3 µm increments throughouta total depth of 78 µm). Scale bar, 25 µm. C, Representative whole-cellrecordings illustrating three layer IV neurons with distinct firingphenotypes. The immature multiple-spiking phenotype (IMS) froma neuron in a P5 slice is characteristic of the majority of neuronsthat can be recorded during the first postnatal week. During thesecond and third postnatal weeks, both FS neurons (FS) and RSneurons (RS) are observed. Shown here are representative tracesfrom an FS and an RS neuron from a P8 and a P11 slice, respectively.Characteristic fAHP and action potential doublet (AP doublet)are indicated in the traces from the FS and RS neurons, respectively.APs were elicited by a 600 msec depolarizing current pulse.
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In the first postnatal week, the majority of neurons fired low-frequency trains of action potentials (APs) at constant interspikeintervals, with no evidence of a fast after-hyperpolarization(fAHP) between spikes in the train. These neurons were classifiedas IMS cells. On the basis of previously established criteria(Connors and Gutnick, 1990), RS and FS phenotypes appeared inthe first postnatal week, but the frequency of encountering neuronswith these firing patterns increased throughout the second postnatalweek. FS neurons fired trains of APs at constant interspike intervalsand exhibited a prominent fAHP between spikes in the train (Fig.1C). RS neurons were characterized by an AP doublet at the beginningof the spike train followed by additional spikes throughout thedepolarizing current step at either constant interspike intervalor with increasing interspike intervals (Fig. 1C). Thus, two classesof neurons with distinct firing properties (FS and RS) developwithin layer IV of the somatosensory cortex during the first twopostnatal weeks. During the first week and throughout the secondweek, neurons that fired only a single AP in response to sustaineddepolarizing stimuli were encountered, but they were not analyzedfurther in these studies.

Cortical neurons in cell culture develop FS and RS phenotypes
To examine the developmental changes in voltage-gated currents and in underlying gene expression that give rise to cells withdistinct firing properties, we used a primary dissociated cellculture system. Although electrophysiological recordings in theslice were obtained exclusively from layer IV neurons, cultureswere prepared from coronal slices spanning the pial-to-white matterboundary and were therefore assumed to contain neurons that wouldnormally reside in all of the cortical laminae, including layerIV. Immediately after dissociation, neurons could be identifiedas round-phase bright cells with processes of varying lengths(Fig. 2A). As early as 3-5 DIV, individual neurons extended longbranching neurites, many of which overlapped extensively (Fig.2B). During the next 2 weeks in culture, neurites continued togrow in length, often forming thick fascicles. At the later timesin culture, neurites formed an intricate mat throughout the culturedish (Fig. 2C,D). Functional synaptic connections that formedbetween neurons were seen as early as 4-5 DIV (Li et al., 1996)and at all stages in vitro thereafter. At all times throughoutdevelopment in vitro, individual cell bodies could be visualizedfor whole-cell patch-clamp recordings and single-cell RT-PCR experiments.
Fig. 2. Morphological development of cortical neurons in dissociated cell cultures. Neurons dissociated from somatosensory cortexharvested from newborn mice were plated on poly-D-lysine-coatedcoverslips in NBM+B27 supplements. Coverslips were transferredinto fresh non-neuronal feeder plates on day 1 and every 3-4 dthereafter. A, Immediately after dissociation (0 DIV), the somataof the majority of the cells were spherical or ovoid in shape.Some of the neurons had processes that remained intact throughoutthe dissociation procedure. B, By 5 DIV the majority of neuronshave extended neurites that connect individuals and groups ofneurons. C, D, The web of interconnecting processes continuesto elaborate throughout the first 3 weeks in vitro. At the platingdensity used in these cultures, the cell bodies of some of theneurons are physically isolated from each other even at the oldestages. Scale bar, 20 µm.
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Whole-cell recordings were made from 152 neurons in 25 cultures between 3 and 23 DIV. As seen in the slice preparation, neuronsthat could fire only a single AP in response to sustained depolarizingcurrent injection were encountered at all ages but were not analyzedfurther; however, the majority of cultured neurons examined exhibitedfiring properties that could be classified initially as IMS, FS,or RS, on the basis of the same criteria used in the slice preparation.Within each of these groups, firing properties showed considerablevariation, as illustrated by the range in firing frequencies observedamong IMS, FS, and RS neurons (Fig. 3A). A similar variabilitywas observed in the layer IV neurons recorded in slice (data notshown). Therefore, to test the validity of our classificationscheme, a number of electrophysiological measures were examinedto determine which, if any, might correlate with firing groupassignment. A scatter plot of the maximal firing frequency versusfAHP amplitude reveals that FS and RS neurons fall naturally intotwo distinct groups, although considerable overlap was evidentbetween IMS and RS cells (Fig. 3B). Better discrimination amongthe three groups was observed in a plot of firing frequency versusthe ratio of the first to second interspike interval, althoughsome overlap occurred between the IMS and both FS and RS groups(Fig. 3B). Table 1 shows the mean values for each of these electrophysiologicalparameters for the three groups. Consistent with the clusteringseen in the scatter plots, significant differences were apparentin all five properties shown between FS and RS neurons. Thesedata demonstrate that cortical neurons in dissociated cell culturefall into two distinct firing phenotypes (FS and RS) and that,to some extent, IMS neurons overlap both of these categories dependingon compared parameters.
Fig. 3. Maturation of firing phenotypes in cultured neurons parallels the development of layer IV neurons in vivo. A, Voltage recordingsfrom two IMS, two FS, and two RS neurons in dissociated cell cultureafter injection of a 600 msec depolarizing current pulse. Thevariation in the maximal firing frequencies within each classis illustrated by the top and bottom traces. B, Quantitative analysisdemonstrates that when maximal firing frequency and fAHP are plottedfor all neurons examined, FS neurons form a distinct group (squares,n = 41), whereas RS (circles, n = 56) and IMS neurons (triangles,n = 47) are not well segregated by this analysis. A scatter plotof firing frequency and the ratio of first to second interspikeinterval (ISI-1/ISI-2) reveal a better separation among the threegroups, although there is still some overlap between the IMS groupwith both the FS and RS groups. C, A box plot illustrates theage range over which the three firing phenotypes were observed.The 10th and 90th percentiles are indicated by the whiskers, andthe 25th, 50th, and 75th percentile boundaries are indicated bythe box for each group. Solid squares denote the means.
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Table 1. Electrophysiological properties of IMS, FS, and RS neurons

Firing frequency (Hz) fAHP (mV) AP duration (msec) Refractory period (msec) ISI1/ISI2

IMS 7.4 ± 0.5 0.2 ± 0.7 3.5 ± 0.1 13.7 ± 1.3 0.8 ± 0.02

n = 57        n = 54 n = 56    n = 26   n = 47

FS 24 ± 1.0 $-$ 9.1 ± 0.4 1.9 ± 0.1 5.9 ± 0.5 0.9 ± 0.01

n = 41 n = 40 n = 41 n = 23 n = 40

RS 12.1 ± 0.5 0.7 ± 0.6 2.6 ± 0.1 15.0 ± 1.3 0.6 ± 0.02

n = 58 n = 57 n = 58 n = 24 n = 56

The mean firing frequency, fAHP, action potential duration, refractory period, and ratio of first to second interspike interval(ISI1/ISI2) were determined for neurons in each of the three firingcategories. The firing frequency was determined from the maximalnumber of spikes evoked by a suprathreshold 600 msec depolarizingcurrent step. The fAHP was measured from threshold to maximalhyperpolarization, after the first spike in the train. Actionpotential duration was measured at half amplitude. The refractoryperiod was defined as the interstimulus interval between two identicaldepolarizing stimuli necessary for a neuron to fire an actionpotential, during the second pulse, with an amplitude at least90% of that elicited during the first pulse. To calculate theISI1/ISI2, the time between the first and second spikes in a trainis expressed as a percentage of the time between the second andthird spikes in the train. Values presented are mean ± SEM; nindicates total number of neurons examined. All five propertiesare significantly different between RS and FS neurons (p < 0.01;Student's t test).

The box plot in Figure 3C illustrates the wide range of ages over which neurons within each of the firing groups were observed.During the first week in culture, however, the majority of theneurons had an IMS phenotype, whereas RS and FS neurons were rarelyseen. FS and RS neurons were found predominantly in the secondand third week in vitro, with a median age of 12 d for both groups(Fig. 3C). These findings suggest that RS and FS neurons emergefrom a population of IMS neurons, both in vivo and in vitro, overa similar time course.

A K_4-AP current is positively correlated with a FS phenotype
As a first step toward understanding how developmental changes in voltage-gated currents influence the appearance of FS andRS phenotypes, we examined the properties of voltage-gated potassiumcurrents in cultured neurons with identified firing patterns.For each neuron, we initially measured the whole-cell capacitance,resting membrane potential, input resistance, and firing propertiesusing a potassium gluconate-based internal solution and a standardphysiological external solution. Subsequently we examined isolatedpotassium currents using voltage protocols and pharmacologicalblocking agents similar to those described previously (Storm,1988; Andreasen and Hablitz, 1992; Wu and Barish, 1992; Foehringand Surmeier, 1993). A family of outward potassium currents evokedin a single cell by a series of depolarizing voltage steps ina normal external solution containing TTX, to block sodium current,and cobalt, to block calcium and calcium-activated potassium currents,is illustrated in Figure 4A. Transient A-currents were obtainedby digital subtraction of traces in which the A-current was inactivated( $-$ 40 mV prepulse) from the total outward potassium current (Fig.4A,B). The K_4-AP current was obtained by digital subtraction oftraces in which the A-current was inactivated and 4-AP-sensitivecurrent was blocked by 100 µM 4-AP, from traces in which justthe A-current was inactivated (Fig. 4B,C). The I_K was definedas the current activated after a prepulse to $-$ 40 mV in the presenceof 100 µM 4-AP (Fig. 4C).
Fig. 4. Isolation of voltage-gated potassium currents in developing cortical neurons. Voltage-gated potassium currents evoked by aseries of 400 msec voltage steps to $-$ 30, $-$ 10, 10, and +30 mV ina single cultured neuron. The whole-cell recording electrode wasfilled with a potassium gluconate-based internal solution, andin each case the bathing solution contained 1 µM TTX and 2 mMcobalt to block the voltage-gated sodium, calcium, and calcium-activatedpotassium currents, respectively. A, Total outward current (I_A+I_K4-AP+I_K)is activated from a holding potential of $-$ 80 mV. B, The fast transientpotassium current (I_A) is inactivated by prepulsing the neuronto $-$ 40 mV for 1 sec, resulting in isolation of I_K+I_K4-AP. C, I_Kis isolated by prepulsing to $-$ 40 mV, thus inactivating I_A, andaddition of 100 µM 4-AP to the bathing medium to pharmacologicallyblock I_K4-AP. A - B, I_A is isolated by digitally subtracting tracesin B from traces in A. B - C, I_K4-AP is isolated by digitallysubtracting traces in C from traces in B.
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All three potassium currents, I_A, I_K, and I_K4-AP, could be detected in neurons within each of the firing groups (Fig. 5).Although there were differences in the average peak current amplitudesand kinetic properties of the isolated potassium currents amongindividual neurons, the most notable difference among cells inthe three groups was amplitude of the K_4-AP current. The amplitudesof the K_4-AP currents in the IMS and RS neurons, at each voltage,were smaller than those in the FS cells (Fig. 5). To control forvariation in cell size, we calculated the K_4-AP current densityin each cell by normalizing the peak current amplitude evokedby a voltage step to +40 mV to the whole-cell capacitance. TheK_4-AP current density in the population of IMS neurons is intermediatebetween the RS and FS groups, whereas the density of this currentin FS neurons is significantly greater (threefold) than in RSneurons (Fig. 6A). This positive correlation between the K_4-APcurrent density and neurons with an FS phenotype suggests thatthis current contributes to firing properties that are uniqueto FS neurons.
Fig. 5. The three voltage-gated potassium currents, I_A, I_K4-AP, and I_K, could be detected in neurons with each of the identified firingphenotypes. Isolated currents were recorded from cultured neuronsusing the protocols illustrated in Figure 4. IMS records wereobtained from three different neurons, 7-8 DIV. FS records wereobtained from two different neurons, 8 DIV. RS records were obtainedfrom two different neurons, 10 and 14 DIV. Scale bar for the I_Acurrent is 1 nA for the IMS and RS neurons and 1.5 nA for theFS neuron.
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Fig. 6. Differential expression of K_4-AP currents among IMS, FS, and RS neurons. A, Because the size of the individual neurons varieswith age and firing properties, the K_4-AP current density in thethree populations of cells, developing in vitro, was examinedby normalizing the peak current amplitude (pA) elicited by a voltagestep to +40 mV, to the whole-cell capacitance (pF). The K_4-APcurrent density of IMS cells (n = 17) is intermediate betweenthe RS (n = 15) and FS (n = 10) groups. The K_4-AP current densityof the FS group is significantly greater than that of the RS group(**p < 0.01; Student's t test). B, Normalized conductance versusvoltage curves were generated for the IMS (squares, n = 15), RS(circles, n = 16), and FS (cross, n = 12) groups. Each of thesecurves was fit with a Boltzmann's distribution indicating similarV_1/2 values (12-16 mV). SEMs were in all cases smaller than thesymbols and therefore were excluded from the graph.
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The K_4-AP currents are characterized by relatively rapid activation kinetics and a slowly inactivating component at the moredepolarized voltages (Fig. 5). Mean conductance-voltage curvesfor each of the three groups were well fit by Boltzmann's distributionsthat indicated a positive (12-16 mV) voltage dependence of activation(Fig. 6B). To investigate further the pharmacological propertiesof the K_4-AP current in FS neurons, a dose-response curve to 4-APwas generated from four FS neurons. These data demonstrate anincrease in percentage current blocked with increasing concentrationof 4-AP, with a predicted half-maximal blocking concentrationof 21 µM (Fig. 7A). Currents with a similar voltage dependence,although lacking the slow inactivation at the more depolarizedpotentials, were also isolated by application of 100 µM TEA (Fig.7B). The lack of slow inactivation in the TEA-isolated currentscould in theory be attributable to 4-AP and TEA blocking the samechannels in a kinetically distinct manner; however, currents isolatedby combined application of 100 µM 4-AP and 100-200 µM TEA in eightneurons were all similar in time course but consistently slightlylarger than those isolated by 4-AP alone (Fig. 7C). These twofindings suggest that whereas the K_4-AP current is sensitive toTEA, it seems likely that TEA also affects one or more additionalcurrents at this concentration.
Fig. 7. Pharmacological properties of I_K4-AP. A, Average dose-response curve for 4-AP, generated from FS neurons (n = 4) developingin vitro. K_4-AP current amplitude was measured after sequentialapplication of 10, 20, 50, and 100 µM 4-AP, and the percentagecurrent (with 100% defined as the current blocked by 100 µM 4-AP)was determined at each 4-AP concentration. The average current(% maximal) from the four cells is plotted as a function of drugconcentration, and these data are fit by the decreasing logisticequation [y = 1/((xⁿ/EC₅₀ⁿ)+1); n = Hill coefficient], with a calculated EC₅₀ of 21 µM.B, Waveforms and current density versus voltage relationship ofcurrents isolated by 100 µM 4-AP in one FS cell and by 100 µMTEA in a second FS cell. C, Current isolated by application of100 µM 4-AP is compared with the current subsequently isolatedfrom the same cell with 100 µM 4-AP and 150 µM TEA. Currents wereevoked by voltage steps between $-$ 20 and +40 in steps of 20 mV,from a holding potential of $-$ 40 mV.
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The K_4-AP current contributes to firing properties characteristic of FS neurons
To establish candidate functions for the K_4-AP current in developing cortical neurons, we looked for firing properties thatwere differentially affected by 100 µM 4-AP in the three firinggroups. Initial studies were performed in the presence of cobaltto rule out the possibility that the effects of 4-AP were mediatedeither directly or indirectly by Ca²⁺ and/or K_Ca²⁺ currents. In the presence of cobalt, exposure of FS neurons to4-AP caused an increase in AP duration, a dramatic reduction inthe large fAHP amplitude, an increase in refractory period, anda decline in the maximal firing frequency (Fig. 8A). Quantitativeanalyses of the effects of 4-AP in FS and RS neurons are illustratedin Figure 8B. Significant changes in AP duration (1.5-fold increase),fAHP amplitude (10-fold decrease), refractory period (threefoldslower), and firing frequency (30% decrease) were observed inthe FS neurons (Fig. 8B). In contrast, 4-AP treatment did notseem to alter AP duration, refractory period, or firing frequencyin RS neurons. The fAHP amplitude of RS neurons was small, bothbefore and after 4-AP, and therefore was not included in the analysis.As is clearly illustrated in Figure 8A, however, the applicationof 4-AP does not result in repetitive firing properties that arereminiscent of RS neurons (no doublet is present) or IMS neurons(firing frequency is too high). Similar experiments were performedin the absence of cobalt, allowing activation of Ca²⁺ and/or K_Ca²⁺ currents. Under these conditions, similar changes in AP duration,fAHP amplitude, refractory period, and firing frequency were alsoapparent in FS neurons after treatment with 4-AP. Consistent withthe data obtained in the presence of cobalt, 4-AP did not significantlyalter the AP duration or firing frequency of RS neurons, althougha small increase in the refractory period was noted.
Fig. 8. Role of the K_4-AP current in firing properties characteristic of FS neurons. All of the electrophysiological recordings wereobtained from cultured cortical neurons in a standard externalsolution that included 2 mM cobalt to block both the calcium andcalcium-activated potassium currents. A, Exposure of an FS neuronto 100 µM 4-AP results in an increase in AP duration from 1.4to 2.6 msec. A decrease in the fAHP, from $-$ 13.7 to $-$ 1.7 mV, isalso observed after exposure to 100 µM 4-AP. Examination of therefractory period reveals an increase from 6 msec (top traces)to 15 msec (bottom traces) after exposure of an FS neuron to 4-AP.Exposure to 4-AP also reduces firing frequency, from 23 to 15Hz in an FS neuron. B, The bar graphs illustrate the mean valuesfor each of these four properties in seven FS and three RS neurons,before and after 4-AP. Drug treatment caused significant changesin all of the parameters in the FS group (**p < 0.01, *p < 0.02;paired Student's t test). No significant changes were noted inthe RS neurons. Error bars on histogram indicate SEMs.
[View Larger Version of this Image (47K GIF file)]

These data suggest that the K_4-AP current makes a critical contribution to the short AP duration, the large fAHP, the briefrefractory period, and the high firing frequency characteristicof neurons that develop an FS phenotype. Because blockade of thiscurrent in FS neurons, however, does not result in repetitivefiring properties that would be classified clearly as RS or IMS,and the K_4-AP current is present in IMS cells and some RS neurons,differences in the numbers, types, or localization of other voltage-gatedchannels must also contribute to the distinct firing patternsamong the three groups.

Kv3.1 mRNA expression is correlated with firing phenotype
Comparison of the electrophysiological and pharmacological properties of the K_4-AP currents with those generated by clonedrat potassium channel genes in heterologous expression systems(Chandy and Gutman, 1995) suggested that Kv3.1 was an excellentcandidate gene for encoding the K_4-AP channels. In rat, the Kv3.1gene gives rise to two alternatively spliced transcripts, designatedKv3.1a and Kv3.1b (Luneau et al., 1991; Grissmer et al., 1992).Although Kv3.1b has not been described in mouse, sequence datafor Kv3.1a, formerly known as NGK2, has been published (Yokoyamaet al., 1989). Therefore, to examine Kv3.1 gene expression indeveloping mouse cortical neurons, primers for RT-PCR were targetedto the 3 $'$ region of the mouse Kv3.1a cDNA in which the sequencediverges from that of other closely related potassium channelgenes. Initial studies demonstrated that these primers amplifieda single product from RNA extracted from both mouse brain andcortical cultures, which based on its electrophoretic mobilityand sequence analysis represents the mouse Kv3.1a transcript.

Given the differential expression of the K_4-AP current, we hypothesized that FS neurons should have the highest levels ofKv3.1 mRNA. Therefore, in an RT-PCR analysis of RNA harvestedfrom single cultured cortical neurons after characterization oftheir firing properties, we predicted that the probability ofobtaining PCR products in FS neurons, given identical PCR conditions,should be higher than in either IMS or RS neurons. In a typicalsingle-cell RT-PCR experiment, PCR products representing the Kv3.1gene were obtained in 3/4 FS neurons and 0/3 RS neurons (Fig.9A,B). The frequency of the Kv3.1 mRNA expression was determinedfor the distinct firing phenotypes in each of four similar experiments(Fig. 9C). The average frequency of amplifying a Kv3.1 productwas approximately four times greater in FS versus RS neurons,with an intermediate frequency of expression observed in the IMScells. The strong positive correlation between the expressionof Kv3.1 transcripts and FS neurons supports the hypothesis thatthis gene encodes the K_4-AP current and that levels of expressionof this gene are regulated during development in a cell-specificmanner.
Fig. 9. Differential amplification of Kv3.1 transcripts in neurons with distinct firing properties. A, Autoradiogram from a singleexperiment showing PCR products representing Kv3.1 transcriptsamplified from RNA harvested from three of the four identifiedFS neurons at 12 DIV. In contrast, no PCR products were amplifiedfrom the three RS neurons examined. Kv3.1 transcripts amplifiedfrom total RNA from adult whole brain (B) and cortical cultureat 6 DIV (C) are shown for comparison. Interleaved control lanesin which medium from the recording chamber (M) or water (W) wasaspirated into the patch pipette and processed in parallel withother samples are all negative. B, Representative traces froman FS and an RS cell (firing properties corresponding to PCR profilein lanes 4 and 6, respectively). C, To determine the average frequencyof expression in the different firing classes, we calculated thefrequency with which PCR products representing Kv3.1 transcriptswere amplified from cultured neurons in the three firing groupsas a function of the total number of neurons in each group, infour individual experiments similar to the one illustrated above.A total of 5, 13, and 18 neurons in the IMS, FS, and RS groups,respectively, were examined. The frequency of expression of Kv3.1was significantly higher in the FS group when compared with theRS group (p < 0.02; Student's t test; n = 4 experiments).
[View Larger Version of this Image (28K GIF file)]

DISCUSSION

Development of FS and RS phenotypes
Our data demonstrate rapid maturation of firing properties of neurons within layer IV during early postnatal development.Neurons that fire low-frequency trains of long-duration APs (IMS)predominate during the first postnatal week, with RS and FS phenotypesseen with increasing frequency throughout the second postnatalweek. A similar maturation profile is observed in a more heterogenouspopulation of neurons developing in dissociated cell culture duringthe first 2 weeks in vitro. As previously demonstrated in corticalneurons from adult rodents (Lambolez et al., 1996), developingneurons with FS and RS phenotypes can also be separated into twodistinct groups on the basis of firing frequency and fAHP amplitude;however, the IMS neurons show considerable overlap with the RSneurons in this analysis. The IMS neurons also show overlap withFS neurons when firing frequency and the ratio of the first andsecond interspike interval are considered. In addition, withinall three firing groups there is variation in a number of electrophysiologicalproperties, including firing frequency, that is likely to reflectdifferences in maturity among neurons within these broad groups.Together these data suggest that cortical neurons, within layerIV and developing in culture, undergo a cell-specific maturationin membrane properties during the first two postnatal weeks suchthat the RS and FS phenotypes emerge from a population of neuronswith an IMS phenotype. In addition, at least within layer IV,specification of distinct firing phenotype seems to occur afterlaminar differentiation. Although the early firing phenotype ofthese neurons may be similar, this does not imply that RS andFS neurons necessarily arise from a common progenitor. For example,immunocytochemical studies have indicated the presence of GABA-immunoreactiveneurons (Del Rio et al., 1992) within layer IV during early postnataldevelopment, when the IMS phenotype predominates. Thus, othercharacteristics may distinguish between neurons that will becomeeither FS or RS before differentiation of the firing properties.

Differential expression of the K_4-AP current
The similarity in the development of firing phenotypes in vivo and in vitro suggests that there are characteristic developmentalchanges in ion channel expression that underlie the basic differentiationof cortical neurons from an IMS phenotype to either FS or RS phenotypes.Previous studies have demonstrated changes in sodium, calcium,and potassium currents during early postnatal development of corticalneurons (Huguenard et al., 1988; Hamill et al., 1991; Lorenzonand Foehring, 1995), but the relationship between these changesand maturation of specific firing properties is not well understood.Using a voltage-dependent and pharmacological isolation strategy,we identified three macroscopic currents in the developing corticalneurons similar to those described as A, K, and D in embryonichippocampal neurons (Wu and Barish, 1992). Consistent with theirnomenclature, we classify two of the currents as A and K; however,because the term D-current was first used in an earlier study(Storm, 1988) to describe a 4-AP-sensitive current with voltage-dependentgating properties different from those of the 4-AP-sensitive currentdescribed here, we refer to the current as K_4-AP.

Our data demonstrate that I_A, I_K, and I_K4-AP were present in neurons within each of the firing classes. This is in contrastto an earlier study that reported the absence of I_A currents inFS neurons (Hamill et al., 1991). Although all of the currentswere observed in each class, there were a number of propertiessuch as activation and inactivation kinetics of I_A that variedboth among classes (Fig. 5) and within a class. The most strikingdifference among the three firing phenotypes, however, was thedensity of the K_4-AP current. FS neurons had a significantly higherK_4-AP current density than RS neurons. Consistent with the suggestionthat both RS and FS neurons arise from neurons that express asimilar complement of voltage-gated ion channels that underliethe common firing phenotype, IMS neurons had intermediate K_4-APcurrent density. Although the maturation of firing propertiesis clearly a product of the coordinate regulation of a numberof different ion channels, the differential expression of K_4-APcurrent suggests that developmental upregulation of this currentis important in the maturation of firing properties that are uniqueto FS neurons.

Evidence that the Kv3.1 gene encodes the K_4-AP current
Several lines of evidence support the hypothesis that the K_4-AP current is encoded by Kv3.1 mRNA. First, currents expressedin mammalian cell lines (Grissmer et al., 1994) and Xenopus oocytes(Yokoyama et al., 1989; Luneau et al., 1991) injected with Kv3.1mRNA exhibit electrophysiological and pharmacological propertiesthat are similar to those of the K_4-AP currents described in thisstudy. Second, our single-cell RT-PCR data demonstrate that thefrequency of detecting PCR products representing Kv3.1 mRNA issignificantly higher in FS neurons that exhibit a high K_4-AP currentdensity compared with RS neurons, whereas an intermediate expressionfrequency is seen in the IMS neurons that express intermediatelevels of K_4-AP current. Because expression of mRNA for severalother genes, including agrin and a type II sodium channel, wassimilar between FS and RS neurons (data not shown), we believethat the low probability of obtaining a Kv3.1 PCR product in RSneurons reflects relatively low levels of Kv3.1 mRNA. Finally,consistent with our finding that the K_4-AP current is preferentiallyexpressed in FS neurons, previous studies demonstrate that theKv3.1 mRNA (Weiser et al., 1994) and protein (Du et al., 1996)are localized in GABAergic neurons in the rodent cortex.

Previous studies in rat have shown that the Kv3.1 gene gives rise to two alternatively spliced variants, Kv3.1a and Kv3.1b,that encode potassium channels with similar biophysical and pharmacologicalproperties (Yokoyama et al., 1989; Luneau et al., 1991; Grissmeret al., 1994). In situ hybridization and other studies have demonstratedfurther that although both transcripts are present in rat corticalneurons, Kv3.1a is the most abundant of the two isoforms duringembryonic and early postnatal development (Perney et al., 1992).The primers used in the present study were specific for the mouseKv3.1a. Given the pattern of Kv3.1a expression in rat, it is temptingto speculate that many of the developmental changes seen in theK_4-AP current are a consequence of changes in Kv3.1a expression;however, although our data are consistent with the Kv3.1 geneencoding 4-AP sensitive channels, we cannot determine the contributionof specific splice variants.

Functional role of the K_4-AP current in firing properties
Recent studies have demonstrated that expression of the Kv3.1 protein is localized in GABAergic interneurons in the hippocampusand that exposure of GABAergic neurons to low concentrations of4-AP affect AP duration, suggesting that a Kv3.1-encoded currentinfluences AP waveform (Du et al., 1996). Our results demonstratingthat application of 4-AP differentially altered a number of electrophysiologicalproperties of FS neurons with relatively little effect on neuronswith RS phenotypes (does not abolish AP doublet at beginning ofspike train) are consistent with this suggestion and also implicatea role for this current in the repetitive firing properties ofdeveloping FS neurons. We found that 4-AP significantly increasedthe AP duration in the cultured neurons, although the averageincrease in our study was less than that seen in parvalbumin-containinginterneurons in the rat hippocampus (Du et al., 1996), which mayreflect differences in the relative density of this current. Exposureto 4-AP also significantly decreased the firing frequency in theFS neurons. This is in contrast to the increase in firing frequencyreported in embryonic hippocampal neurons under similar conditions(Wu and Barish, 1992). Cell-specific differences in relative numbersand localization of channels mediating K_4-AP currents or the expressionof other currents that influence firing frequency may underliethese differences. Similar results were obtained in the presenceand absence of cobalt, demonstrating that the primary mechanismof 4-AP action is likely to be through specific blockade of theK_4-AP current and not mediated through calcium or calcium-activatedpotassium currents. Interestingly, the prominent fAHP in the FSneurons, also altered by 4-AP, was calcium independent. Althoughthe fAHP reported in hippocampal pyramidal cells seems to be calciumdependent (Storm, 1987), calcium-independent fAHPs have been describedpreviously in motoneurons (Barrett and Barrett, 1976; Yarom etal., 1985) .

These data suggest that upregulation of the K_4-AP current, either through increased transcription or stability of Kv3.1 mRNA,is important in the development of a number of firing propertiescharacteristic of FS neurons. Blockade of this current in FS neurons,however, does not result in repetitive firing properties thatwould be clearly classified as RS or IMS. Therefore, additionalchanges in the numbers, types, or localization of other channeltypes are clearly important in the development of the mature FSphenotype.

Future studies
Molecular genetic manipulations will be important to test the hypothesis that the Kv3.1 gene encodes the developmentally regulatedK_4-AP current expressed in developing cortical neurons. This shouldbe possible using a strain of Kv3.1-deficient mice that were generatedby homologous recombination (Ho et al., 1997) or with antisenseoligonucleotides targeted specifically to Kv3.1 transcripts. Wepredict that cortical neurons lacking Kv3.1 transcripts will alsolack the K_4-AP current and that the FS GABAergic neurons shouldhave longer than normal AP durations, little or no fAHP, and longerthan normal refractory periods. Changes in the firing propertiesof FS neurons, resulting from changes in the levels of expressionof Kv3.1-encoded currents, may also influence the overall activityof FS GABAergic neurons in developing cortical circuits both invivo and in vitro.

FOOTNOTES

Received Nov. 26, 1996; revised Feb. 12, 1997; accepted Feb. 14, 1997.

This study was supported by National Institutes of Health Grants NS30109 and NS27501 and a Research Career Development AwardNS01854 to D.K.O. Additional support was provided by NationalInstitutes of Health Grant NS33213 and National Science FoundationGrant IBN9319355 to M.A.S. We thank Dr. F. Ehlert for helpfuldiscussions and Dr. Ariel Agmon for critical comments on a previousversion of this manuscript.

Correspondence should be addressed to Diane K. O'Dowd, Department of Anatomy and Neurobiology, University of California, Irvine,CA 92697-1280.

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Volume 17, Number 9, Issue of May 1, 1997 pp. 3136-3147 Copyright ©1997 Society for Neuroscience

Differential Expression of K4-AP Currents and Kv3.1 Potassium Channel Transcripts in Cortical Neurons that Develop Distinct Firing Phenotypes

Copyright ©1997 Society for Neuroscience 0270-6474/1997/173136-12$05.00/0

Volume 17, Number 9, Issue of May 1, 1997 pp. 3136-3147
Copyright ©1997 Society for Neuroscience

Differential Expression of K_4-AP Currents and Kv3.1 Potassium Channel Transcripts in Cortical Neurons that Develop Distinct Firing Phenotypes