Somatodendritic Depolarization-Activated Potassium Currents in Rat Neostriatal Cholinergic Interneurons Are Predominantly of the A Type and Attributable to Coexpression of Kv4.2 and Kv4.1 Subunits

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The Journal of Neuroscience, May 1, 1998, 18(9):3124-3137

Somatodendritic Depolarization-Activated Potassium Currents in Rat Neostriatal Cholinergic Interneurons Are Predominantly of the A Type and Attributable to Coexpression of Kv4.2 and Kv4.1 Subunits
W.-J. Song, T. Tkatch, G. Baranauskas, N. Ichinohe, S. T. Kitai, and D. J. Surmeier
Department of Anatomy and Neurobiology, College of Medicine, University of Tennessee, Memphis, Memphis, Tennessee 38163

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Unlike other neostriatal neurons, cholinergic interneurons exhibit spontaneous, low-frequency, repetitive firing. To gainan understanding of the K⁺ channels regulating this behavior, acutely isolated adult ratcholinergic interneurons were studied using whole-cell voltage-clampand single-cell reverse transcription-PCR techniques. Cholinergicinterneurons were identified by the presence of choline acetyltransferase(ChAT) mRNA. Depolarization-activated potassium currents in cholinergicinterneurons were dominated by a rapidly inactivating, K⁺-selective A current that became active at subthreshold potentials.Depolarizing prepulses inactivated this component of the current,leaving a delayed, rectifier-like current. Micromolar concentrationsof Cd²⁺ dramatically shifted the voltage dependence of the A currentwithout significantly affecting the delayed rectifier. The A-channelantagonist 4-aminopyridine (4-AP) produced a voltage-dependentblock (IC₅₀, ~1 mM) with a prominent crossover at millimolar concentrations.On the other hand, TEA preferentially blocked the sustained currentcomponent at concentrations <10 mM. Single-cell mRNA profilingof subunits known to give rise to rapidly inactivating K⁺ currents revealed the coexpression of Kv4.1, Kv4.2, and Kv1.4mRNAs but low or undetectable levels of Kv4.3 and Kv3.4 mRNAs.Kv1.1, $beta$ 1, and $beta$ 2 subunit mRNAs, but not $beta$ 3, were also commonlydetected. The inactivation recovery kinetics of the A-type currentwere found to match those of Kv4.2 and 4.1 channels and not thoseof Kv1.4 or Kv1.1 and $beta$ 1 channels. Immunocytochemical analysisconfirmed the presence of Kv4.2 but not Kv1.4 subunits in thesomatodendritic membrane of ChAT-immunoreactive neurons. Theseresults argue that the depolarization-activated somatodendriticK⁺ currents in cholinergic interneurons are dominated by Kv4.2-and Kv4.1-containing channels. The properties of these channelsare consistent with their playing a prominent role in governingthe slow, repetitive discharge of interneurons seen in vivo.

Key words: A current; delayed rectifier; tetraethylammonium; 4-aminopyridine; voltage clamp; single-cell RT-PCR; acutely dissociated neurons; Kv1; Kv2; Kv3

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Although cholinergic interneurons account for only a few percent of all neostriatal neurons (Kemp and Powell, 1971; Phelpset al., 1985), they exert a profound influence on striatal circuitry.For example, it has long been known that disruption of the cholinergicregulation of medium spiny neurons through muscarinic receptorsameliorates movement disorders accompanying striatal dopaminedepletion (Hornykiewcz, 1973). More recently it has been suggestedthat cholinergic interneurons are instrumental in the acquisitionof procedural or associative learning tasks (Aosaki et al., 1994;Graybiel et al., 1994).

Despite their functional importance, cholinergic interneurons have been difficult to study because of their rarity. The firstclear glimpse of interneuronal physiology suggested that theyhad relatively depolarized resting potentials and distinctivespike patterns (Wilson et al., 1990). These studies were extendedby Kawaguchi (1992, 1993) in showing that striatal choline acetyltransferase(ChAT)-immunoreactive neurons in slices exhibited a prolongedspike afterhyperpolarization with slow ramp-like voltage trajectoriespreceding the next spike, enabling these cells to discharge atvery low rates.

Slow ramp-like voltage trajectories of this sort often are governed by inactivating, A-type K⁺ currents (Connor and Stevens, 1971a,b; Rogawski, 1985). However,since their original description, physiological studies have revealedthat A-type currents exhibit a wide range of biophysical and pharmacologicalproperties, sometimes specializing them for other cellular functions(Rogawski, 1985; Rudy, 1988). This functional heterogeneity isreflected in the molecular heterogeneity of A-like K⁺ channels. Depolarization-activated K⁺ channels are thought to be formed by four $alpha$ subunits drawn fromfour $alpha$ subunit gene families (Kv1-4) (Stuhmer et al., 1989; Pongs,1993). Expression studies have shown that homomeric channels arisingfrom Kv1.4, Kv3.4, and Kv4.1, Kv4.2, and Kv4.3 subunits give riseto A-type channels (Stuhmer et al., 1989; Baldwin et al., 1991;Schroter et al., 1991; Serodio et al., 1994, 1996). In addition,inactivating, A-like channels can be formed when ancillary $beta$ 1subunits are coexpressed with subunits of the Kv1 family thatnormally have delayed rectifier properties (Rettig et al., 1994;Heinemann et al., 1996; Sewing et al., 1996). Based on studiesin heterologous cell types, several of these channels (e.g., Kv4.2)have biophysical properties that would enable them to significantlyslow the rate of membrane depolarization at subthreshold potentialsand to promote low-frequency repetitive discharge. However, itis unclear to what extent these subunits are expressed in cholinergicinterneurons and, if so, to what extent they are found withinthe somatodendritic membrane.

Based on these previous studies, it was our working hypothesis that the capacity of cholinergic interneurons to dischargeat low rates was attributable to the expression of A-type K⁺ channels with features similar to those formed from Kv4.2 subunits.To test this hypothesis, whole-cell K⁺ currents in identified cholinergic interneurons were studiedusing voltage-clamp techniques. The molecular identity of thechannel subunits underlying the currents was determined by single-cellreverse transcription-PCR (RT-PCR) analysis (Monyer and Lambolez,1995; Surmeier et al., 1996; Yan and Surmeier, 1996; Yan et al.,1997) and immunohistochemistry (Sheng et al., 1992; Maletic-Savaticet al., 1995). The results described below argue that striatalcholinergic interneurons coexpress several of the $alpha$ and $beta$ subunitsknown to produce A-type channels but, within the somatodendriticmembrane, Kv4.2 and Kv4.1 channels are the predominate channeltypes and possess the biophysical properties necessary to regulaterepetitive discharge.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Acute dissociation procedure. Striatal neurons from young adult (>4 wk) male rats were acutely dissociated using proceduressimilar to those we described previously (Surmeier et al., 1995;Song and Surmeier, 1996). In brief, rats were anesthetized withmethoxyflurane and decapitated; brains were quickly removed, iced,and then blocked for slicing. The blocked tissue was cut in 400µm slices with a Microslicer (Dosaka, Kyoto, Japan) while bathedin a high-sucrose solution (in mM: 250 sucrose, 2.5 KCl, 1 Na₂HPO₄,2 MgSO₄, 2 CaCl₂, 11 glucose, and 15 HEPES, pH 7.4; 300-305 mOsm/l).Slices were then incubated for 1-6 hr at room temperature (20-22°C)in NaHCO₃ buffered saline bubbled with 95% O₂ and 5% CO₂ (in mM:126 NaCl, 2.5 KCl, 2 CaCl₂, 2 MgCl₂, 26 NaHCO₃, 1.25 NaH₂PO₄,1 pyruvic acid, 0.2 ascorbic acid, 0.1 N-nitro-L-arginine, 1 kynurenic acid, and 10 glucose, pH 7.4 withNaOH; 300-305 mOsm/l). All reagents were obtained from Sigma (St.Louis, MO). Slices were then removed into low-Ca²⁺, HEPES-buffered saline (in mM: 140 Na-isethionate, 2 KCl, 4 MgCl₂,0.1 CaCl₂, 23 glucose, and 15 HEPES, pH 7.4; 300-305 mOsm/l),and with the aid of a dissecting microscope, regions of the dorsalstriatum were dissected and placed in an oxygenated Cell-Stirchamber (Wheaton, Inc., Millville, NJ) containing Pronase (1-2mg/ml) in HEPES-buffered HBSS (Sigma) at 35°C. Dissections werelimited to tissue rostral to the anterior commissure to reducethe possibility of contamination from globus pallidus. After 30-40min of enzyme digestion, tissue was rinsed three times in thelow-Ca²⁺, HEPES-buffered saline and mechanically dissociated with a gradedseries of fire-polished Pasteur pipettes. The cell suspensionwas then plated into a 35 mm Lux Petri dish mounted on the stageof an inverted microscope containing HEPES-buffered HBSS. Afterallowing the cells to settle, the solution bathing the cells waschanged to a HEPES-buffered saline.

Whole-cell recordings. Whole-cell recordings used standard techniques (Hamill et al., 1981; Song and Surmeier, 1996). Electrodeswere pulled from Corning (Corning, NY) 7052 glass and fire-polishedbefore use. The internal solution consisted of (in mM): 60 K₂SO₄,60 N-methyl-D-glucamine, 4 MgCl₂, 40 HEPES, 2.5-5 EGTA or 5 BAPTA,12 phosphocreatine, 2 Na₂ATP, 0.2 Na₃GTP, and 0.1 leupeptin, pH7.2 with H₂SO₄ (osmolarity, 265-275 mOsm/l). The pH of N-methylglucaminesolutions was measured with a Corning model 476570 probe. Theexternal solution consisted of (in mM): 140 Na-isethionate, 2-5KCl, 2-4 MgCl₂, 0-2 Ca²⁺, 10 HEPES, 12 glucose, and 0.001 TTX, pH 7.4 with 1N NaOH (~2ml) (osmolarity, 300 ± 5 mOsm/l).

In all the experiments, Na⁺ currents were blocked by TTX. Ca²⁺ currents were eliminated in one of two ways. In almost all ofthe experiments described below, Ca²⁺ in the bathing medium was replaced on an equimolar basis by Mg²⁺. This eliminated measurable currents that were sensitive to inorganicCa²⁺ channel blockers. In some experiments, CdCl₂ (200-400 µM) wasadded to the external solution to block Ca²⁺ currents. These experiments are explicitly described below.

In some experiments, 4-AP (Sigma) or tetraethylammonium chloride (TEA) (Sigma) was applied. When 4-AP was included in theextracellular solutions, the pH was adjusted to 7.4 using H₂SO₄.When 4-AP or TEA was applied at concentrations >1 mM, the osmolaritywas adjusted by reducing the concentration of Na-isethionate.

Solutions were applied with a gravity-fed sewer pipe system. An array of application capillaries (~400 µm inner diameter)was positioned a few hundred micrometers from the cell under study.Solution changes were effected by altering the position of thearray with a DC drive system controlled by a microprocessor-basedcontroller (Newport-Klinger, Inc., Irvine, CA). Solution changeswere complete within <1 sec.

Recordings were obtained with an Axon Instruments 200 patch-clamp amplifier and controlled and monitored with a PC 486 clonerunning pClamp software (version 6.0) with a 125 kHz interface(Axon Instruments Inc., Foster City, CA). Electrode resistanceswere typically 2-6 M $Omega$ in the bath. After seal rupture, seriesresistance (7-15 M $Omega$ ) was compensated (80-90%) and periodicallymonitored. Potentials were not corrected for the liquid junctionpotential, which was estimated to be 1 mV, except when calculatingthe permeability to K⁺ relative to Na⁺. Recordings were made only from large-sized neurons (>14 pF)that had only a few short (<75 µm) proximal dendrites.

Statistical methods. Statistical analyses (including nonlinear curve fitting) were performed with Systat (Evanston, IL; version5.2). Sample statistics are given either as means with SD or asmedians. Box plots were used for graphic presentation of the databecause of the small sample sizes (Tukey, 1977). The box plotrepresents the distribution as a box with the median as a centralline and the hinges as the edges of the box (the hinges dividethe upper and lower halves of the distributions in half). Theinner fences (shown as a line originating from the edges of thebox) run to the limits of the distribution excluding outliers(defined as points that are >1.5× the interquartile range beyondthe interquartiles; Tukey, 1977); outliers are shown as asterisksor circles.

Boltzmann functions were fit to normalized conductance or current plots using previously described formulas (Bargas et al.,1994) with a least squares fitting routine.

Single-neuron RT-PCR analysis. As we have reported previously (Song and Surmeier, 1996; Surmeier et al., 1996; Yan and Surmeier,1996), after recording, cells were lifted up into a stream ofcontrol solution and aspirated into the electrode by applyingnegative pressure. Electrodes contained ~5 µl of sterile recordingsolution (see above). Some cells were harvested without recording,with electrodes filled with water. The capillary glass used formaking electrodes had been heated to 200°C for 4 hr. Sterile gloveswere worn during the procedure to minimize RNase contamination.

After aspiration, the electrode was broken, and contents were ejected into a presiliconized, 0.5 ml Eppendorf tube containing5 µl diethylpyrocarbonate-treated water, 0.5 µl of RNasin (28,000U/ml), and 0.5 µl of dithiothreitol (DTT) (0.1 M). One microliterof either oligo-dT (0.5 µg/µl) or random hexanucleotides (50 ng/µl)was added and mixed before the mixture was heated at 70°C for10 min and incubated on ice for >1 min. Single-strand cDNA wassynthesized from the cellular mRNA by adding SuperScript II reversetranscriptase (1 µl, 200 U/µl), 10× PCR buffer (2 µl, 200 mM TrisCl, pH 8.4, and 500 mM KCl), MgCl₂ (2 µl, 25 mM), RNasin (0.5µl, 28,000 U/ml), DTT (1.5 µl, 0.1 M), and mixed dNTPs (1 µl,10 mM). The reaction mixture (20 µl) was incubated at 42°C for50 min. The reaction was terminated by heating the mixture to70°C for 15 min and then icing. The RNA strand in the RNA-DNAhybrid was then removed by adding 1 µl of RNase H (2 U/µl) andincubating for 20 min at 37°C. All reagents except RNasin (Promega,Madison, WI) were obtained from Life Technologies (Grand Island,NY). The cDNA from the reverse transcriptase of RNA in singlestriatal neurons was subjected to PCR to detect the expressionof mRNAs coding for K⁺ channels, ChAT, and the neuropeptides enkephalin and substanceP.

Conventional PCR was performed with a thermal cycler (MJ Research, Inc., Watertown, MA). Thin-walled plastic tubes (Perkin-Elmer,Norwalk, CT) were used. PCR primers were developed from GenBanksequences with commercially available Oligo software (NationalBiosciences, Plymouth, MN). The primers used in this study areshown in Table 1. Positive controls for primer efficiency wererun using whole-brain cDNA. Primers for ChAT, enkephalin, andsubstance P mRNA were described previously (Surmeier et al., 1996;Yan and Surmeier, 1996). To detect individual mRNAs, 2.5 µl ofthe single-cell cDNA was used as a template for conventional PCRamplification. Reaction mixtures contained 2-2.5 mM MgCl₂, a 0.5mM concentration of each of the dNTPs, 1 µM primers, 2.5 U ofTaq DNA polymerase, and buffer (Promega). The thermal cyclingprogram was 94°C for 1 min, 58°C (or 56°C for some primers) for1 min, and 72°C for 1.5 min for 45 cycles.


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Table 1. PCR primer sets

To identify mRNAs coexpressed in single neurons, a two-step protocol was used. In the first round, 2.5 µl of the single-cellcDNA was used as a template in a multiplex (three or four pairsof primers) PCR reaction. The reaction mixture contained the sameconcentration of reagents as with conventional PCR, except forslightly decreased primer concentration (0.5 µM). Fifteen cycleswere performed. Then, an aliquot () of thisPCR product was used as a template for a second round (35 cycles)of PCR amplification with each pair of specific primers (1 µM).

PCR products were separated by electrophoresis in 1.5-2% agarose gels and visualized by staining with ethidium bromide. Inrepresentative cases, amplicons were purified from the gel (QIAquickgel extraction kit; Qiagen, Hilden, Germany) and sequenced witha dye termination procedure by the University of Tennessee MolecularResource Center or St. Jude Children's Research Hospital MolecularResource Center. These sequences were found to closely match publishedsequences.

PCR reactions were performed following procedures designed to minimize the chances of cross-contamination (Cimino et al.,1990). Negative controls for contamination from extraneous andgenomic DNA were run for every batch of neurons. To ensure thatgenomic DNA did not contribute to the PCR products, neurons wereaspirated and processed in the normal manner, except that thereverse transcriptase was omitted. Contamination from extraneoussources was checked by replacing the cellular template with water.Both controls were consistently negative in these experiments.

Immunohistochemistry. Animals were anesthetized with sodium pentobarbital (40 mg/kg) and chloral hydrate (170 mg/kg) and wereperfused through the ascending aorta with 100 ml of 0.9% sodiumchloride followed by 250 ml of 4% paraformaldehyde in 0.1 M phosphatebuffer (PB), pH 7.4. Brains were removed, cut sagittally at themidline, post-fixed 1 hr in the same fixative, and then immersedovernight in 30% sucrose/PB. The brain was rapidly frozen by immersingin 2-methylbutane cooled by dry ice. The brain was sectioned at15 µm using a cryostat. Sections containing the striatum and theglobus pallidus were mounted on glass slides.

For single-label immunohistochemistry, sections were incubated with 8% bovine serum albumin (BSA) in PBS, pH 7.4, for 1 hrat room temperature, and then, with the primary antibody dilutedin PBS containing 1% BSA (PBSB), were incubated overnight at 4°C.These primary antibodies included mouse monoclonal anti-rat Kv1.4antibody (Upstate Biotechnology, Lake Placid, NY) at a dilutionof 1:100 and rabbit affinity-purified polyclonal anti-Kv4.2C antibody(provided by Dr. James S. Trimmer, State University of New York,Stony Brook, NY) at a dilution of 1:500. This antibody recognizesKv4.2 subunits and at least one form of Kv4.3 subunit. After threewashes in PBS, Kv1.4 sections were incubated with PBSB containingbiotinylated horse anti-mouse IgG antibody (1:200; Vector Laboratories,Burlingame, CA), and Kv4.2C sections were incubated with PBSBcontaining biotinylated goat anti-rabbit IgG antibody (1:200;Vector Laboratories) for 3 hr at room temperature. All the sectionswere washed again in PBS and then incubated for 2 hr at room temperaturewith 1:100 avidin-biotin-horseradish peroxidase complex (ABC Vectastainkit; Vector Laboratories) in PBS. After an additional wash inPBS, sections were incubated in 50 mM Tris buffer, pH 7.6, containing0.02% diaminobenzidine, 0.3% nickel ammonium sulfate, and 0.002%H₂O₂ for 5-15 min. After washing in Tris buffer, sections weredehydrated and coverslipped.

For double-label immunofluorescence, sections were first incubated with 8% BSA in PBS for 1 hr at room temperature and thenwith a mixture of 1:50 rabbit affinity-purified polyclonal anti-Kv4.2Cantibody and 1:250 monoclonal mouse anti-ChAT antibody (Chemicon,Temicula, CA) in PBSB overnight at 4°C. After washing three timesin PBS, sections were incubated with PBSB containing biotinylatedgoat anti-rabbit IgG antibody (1:200; Vector Laboratories) andfluorescein isothiocyanate (FITC)-conjugated horse anti-mouseIgG antibody (1:150; Vector Laboratories) for 3 hr at room temperature,were washed again in PBS, and then were incubated for 2 hr with1:500 avidin-D-Texas Red (Vector Laboratories) in PBS. After additionalwashes in PBS, sections were coverslipped with 1,4-diazabicyclo-[2.2.2]octanein phosphate-buffered glycerol. They were examined under an Olympusepifluorescence microscope with an appropriate filter for FITCor Texas Red.

Controls for nonspecific staining for primary antiserum or cross-reactivity of antiserums were performed. For single-labeledimmunohistochemistry, the control sections were incubated in theabsence of the primary antibody in the first step. For double-labeledimmunofluorescence, the control sections were incubated with PBSBcontaining either antibodies for Kv4.2C or ChAT or with PBSB withoutany antibodies. These control sections were processed througheach remaining step of the protocol in the same manner as theexperimental sections. These control experiments indicated thatthere was no nonspecific labeling of neural soma or processes.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

After dissociation, neurons with large cell bodies were easily recognized (Fig. 1A, inset). One to five of these large neuronswere found per slice. Their whole-cell capacitance ranged from14 to 22 pF in our sample of 88 neurons. In agreement with previousstudies (Yan and Surmeier, 1996; Yan et al., 1997), all largecells tested with single-cell RT-PCR techniques had detectablelevels of choline acetyltransferase mRNA (n = 13) (Fig. 1B). Theselarge neurons did not express enkephalin or substance P mRNA,which are known to be found in striatal medium spiny neurons (Fig.1B,D) (Graybiel, 1990). These results suggest that most, if notall, of the neurons used in this study were cholinergic interneurons.

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Figure 1. Depolarization-activated K⁺ currents in neostriatal cholinergic interneurons are dominated by an A current. A, Whole-cell K⁺ currents recorded from a cholinergic interneuron. Na⁺ and Ca²⁺ currents have been eliminated (see Materials and Methods). Inset, Photomicrograph of an acutely isolated cholinergic interneuron and a medium-sized neuron. Scale bar, 25 µm. B, Photomicrograph of an ethidium bromide-stained gel in which PCR amplicons from the cell recorded from in A were separated by electrophoresis. Note the presence of ChAT amplicon but not enkephalin (Enk) and substance P (SP) amplicons. C, Whole-cell recording from a medium spiny neuron showing currents that inactivate more slowly than in A. D, Photomicrograph of an ethidium bromide-stained gel in which PCR amplicons from the cell recorded from in C were separated by electrophoresis. Note the absence of ChAT amplicon and the presence of enkephalin but not substance P amplicons.

Depolarization-activated outward currents in cholinergic interneurons are dominated by a transient A-type current

With Na⁺ and Ca²⁺ currents eliminated, depolarizing voltage steps from hyperpolarized membrane potentials evoked outward currentsin cholinergic interneurons. The currents were dominated by alarge transient component (Fig. 1A). This current profile wassignificantly different from that seen in recordings from mediumspiny neurons (Fig. 1C,D) (Nisenbaum et al., 1996). In cholinergicinterneurons, peak current amplitude was 6.25 ± 1.72 (mean ± SD;n = 8) times that at the end of a 500 msec test pulse to +35 mV.This ratio was only 1.51 ± 0.16 (n = 5) in the medium spiny cells.An analysis of tail currents evoked by a short depolarizing step(50 msec) in 5 mM extracellular [K⁺] suggested that the evoked currents in interneurons were K⁺-selective, having a p_K/p_Na ratio of 35:1 based on the Goldman-Hodgkin-Katzequation (Hille, 1992) (data not shown).

A-type currents were isolated by taking advantage of their sensitivity to holding potential (Connor and Stevens, 1971a; Neher,1971). From hyperpolarized membrane potentials, depolarizing voltagesteps evoked both rapidly and slowly inactivating currents (Fig.2A). From more positive holding potentials (approximately $-$ 50),depolarizing steps evoked only slowly inactivating currents (Fig.2B). Subtraction of the currents evoked at depolarized potentialsfrom those evoked from more hyperpolarized potentials isolateda rapidly inactivating, A-type current (Fig. 2C). The inset isa graph showing the currents on a faster time scale. A plot ofthe mean normalized peak chord conductances as a function of membranevoltage for a sample of neurons is shown in Figure 2D. These datawere well fit with a Boltzmann function, having a half-activationvoltage of $-$ 27.2 mV and a slope factor of 14.7 mV.

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Figure 2. Interneurons express rapidly inactivating A-type currents that activate at subthreshold potentials. A, Currents evoked by a series of depolarizing steps from $-$ 80 to +40 mV after a hyperpolarizing step to $-$ 100 mV. B, Currents evoked by the same set of depolarizing steps when preceded by a prepulse to $-$ 50 mV. C, Difference currents obtained by subtracting B from A. Inset, Same currents on a slightly faster time scale. D, Plot of mean normalized peak chord conductance as a function of step voltage for difference currents in a sample of four interneurons. Solid line, Boltzmann function with a half-activation voltage of $-$ 27.2 mV and a slope factor of 14.7 mV.

The steady-state voltage dependence of inactivation was studied by applying conditioning steps (1.4 sec) to membrane potentialsbetween $-$ 120 and $-$ 30 mV before a test step to 0 mV. As shown inFigure 3A, depolarizing steps diminished the transient currentsevoked by the test step. A plot of mean normalized peak currentamplitude as a function of conditioning voltage for a sample ofneurons is shown in Figure 3B. These data were well fit with asingle Boltzmann function having a half-inactivation voltage of $-$ 93.5 mV and a slope factor of 7.5 mV (Fig. 3B). Also shown isthe Boltzmann fit of the activation data (Fig. 2D), illustratingthe complementary voltage dependence of the two processes. Itcan also be seen that there is a small window current for thisconductance near the expected resting membrane potential (approximately $-$ 65 mV) (Wilson et al., 1990).

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Figure 3. The A-type current in interneurons inactivated over a relatively negative voltage range. A, K⁺ currents evoked by a depolarizing step to 0 mV after conditioning prepulses (1.4 sec) to membrane potentials between $-$ 120 and $-$ 30 mV. B, Plot of normalized peak current as a function of conditioning voltage for a sample of five neurons. Open circles, Mean values; error bars indicate SEM. Solid line, Boltzmann function with a half-inactivation voltage of $-$ 93.5 mV and a slope factor of 7.5 mV. Also plotted is the activation curve fitted to the data in Figure 2.

Although many of the channels formed from cloned A-type subunits have similar activation and inactivation voltage dependence,the rates at which these channels inactivate or recover from inactivationare frequently quite different (Pongs, 1993; Deal et al., 1996).Inactivation kinetics are also crucial to the functional roleplayed by A-type currents (Rogawski, 1985; Huguenard and McCormick,1992). As a consequence, the development and recovery of A-typeinactivation were characterized. The development of inactivationat depolarized membrane potentials was studied in two complementaryways. First, the inactivating phase of A-type currents (isolatedby a subtraction protocol; Fig. 2) was fit with a decaying exponentialfunction (Fig. 4A). At potentials above $-$ 40 mV, currents werewell fit with a single exponential, having a time constant of20-25 msec. A plot of mean inactivation time constants as a functionof test voltage is shown in Figure 4B. As has been described previouslyfor certain classes of A-type current, the development of inactivationslowed modestly with increasing voltage. A potential complicationof these experiments is that the subtraction procedure may nothave completely isolated the A-type current. An alternative strategythat takes advantage of the rapid activation kinetics of the A-typecurrent is to use a two-step protocol in which the duration ofthe conditioning prepulse is systematically varied (Fig. 4C).Current amplitudes were measured at times expected of the peakA current based on the initial test step. A plot of current amplitudeas a function of prepulse duration was consistently well fit,with a single decreasing exponential having a time constant veryclose to that obtained by fitting the decay of currents duringa single test step (Fig. 4D). The inset is a box plot summaryof the inactivation time constants obtained from a sample of neurons.

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Figure 4. Interneuronal A-type currents inactivated and recovered from inactivation rapidly. A, A-type currents evoked by depolarizing steps from $-$ 40 to 20 mV isolated by subtraction (Fig. 2). Inactivating phase at each voltage is fitted with a single exponential function with a time constant of 23 msec. B, Plot of mean ± SEM inactivation time constant as a function of step voltage for a sample of six neurons. Data were fit with a straight line with an intercept of 26 msec and a slope of 0.062 msec/mV. C, A-type currents were progressively inactivated by lengthening the duration of a step to $-$ 30 mV before a test step to 20 mV. D, Plot of peak current measured isochronously as a function of prepulse duration. Data points were fitted with an exponential with a time constant of 24 msec (solid line). Inset, Box plot of time constants obtained in similar experiments for a sample of five neurons. E, Inactivation recovery was examined by inactivating A-type currents and then stepping to $-$ 80 mV for increasing periods before a test step to 20 mV. F, Plot of peak current as a function of prepulse duration (@ $-$ 80 mV). Data were fit with a sum of exponentials (solid line) with time constants of 19 and 390 msec. Inset, Box plot summarizing the distribution of fast and slow time constants for a sample of eight neurons.

The recovery from inactivation was studied by first inactivating A-type channels by holding at $-$ 40 mV and then stepping tohyperpolarized membrane potentials for increasing durations beforea test step (Fig. 4E). Plots of peak current as a function ofprepulse duration were well fit only with a sum of exponentialfunctions (Fig. 4F). In our sample of interneurons, the smallerrecovery time constant was between 10 and 20 msec, whereas theslower component of recovery was typically between 200 and 400msec (Fig. 4F, inset).

Cd²⁺ dramatically shifts the voltage dependence and kinetics of the A-type current

In all of the experiments described in Figures 2-4, K⁺ currents were isolated by blocking Na⁺ currents with tetrodotoxin and eliminating Ca²⁺ currents by removing extracellular Ca²⁺ and replacing it with Mg²⁺. However, removing extracellular Ca²⁺ typically shortened the duration of recordings. Another commonlyused strategy to eliminate Ca²⁺ currents that does not shorten recording times is to block Ca²⁺ channels with Cd²⁺ (200-400 µM). Although the addition of Cd²⁺ to the extracellular solution effectively blocked Ca²⁺ channel currents, it had dramatic effects on the voltage dependenceand kinetics of the transient K⁺ currents.

A-type currents isolated in Cd²⁺-containing external solutions are shown in Figure 5A. A plot of average peak chord conductancefor a sample of interneurons studied in this way is shown in Figure5B. The data were well fit with a single Boltzmann function, havinga half-activation voltage of 5.5 mV and a slope factor of 11.6mV. This is 32 mV more positive than the fit obtained from dataobtained in the absence of Cd²⁺ (Fig. 2B). The fit of the control data are plotted for the purposeof comparison. The voltage dependence of inactivation was shiftedeven more dramatically. Currents evoked by a two pulse protocolare shown in Figure 5C (note that the abscissa before the testpulse is compressed). A plot of average normalized peak currentas a function of prepulse voltage for our sample of interneuronswas well fit with a single Boltzmann function, having a half-inactivationvoltage of $-$ 35.4 mV and a slope factor of 5.2 mV. Also plottedis the fit of the data obtained in the absence of Cd²⁺ for comparison. The difference in the half-inactivation voltageswas 57 mV.

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Figure 5. Extracellular Cd²⁺ dramatically shifted the voltage dependence of A-channel activation and inactivation gating. A, Difference currents evoked in the presence of Cd²⁺ (400 µM) by a series of depolarizing steps from $-$ 60 to +60 mV after a hyperpolarizing step to $-$ 80 mV. B, Plot of mean normalized peak chord conductance ± SEM as a function of step voltage for difference currents in a sample of six interneurons. Solid line, Boltzmann function with a half-activation voltage of 5.5 mV and a slope factor of 11.6 mV. Also shown is the activation curve fitted to the data obtained in the absence of Cd²⁺. C, K⁺ currents evoked by a depolarizing step to 0 mV after conditioning prepulses to membrane potentials between $-$ 80 and +10 mV. D, Plot of normalized peak current as a function of conditioning voltage for a sample of six neurons. Open circles, Mean values; error bars indicate SEM. Solid line, Boltzmann function with a half-inactivation voltage of $-$ 36.4 mV and a slope factor of 5.2 mV. Also plotted is the activation curve fitted to the data in Figure 3.

In addition to shifting the voltage dependence of activation and inactivation, Cd²⁺ slowed the development of inactivation. At all of the voltagesexamined ( $-$ 30 to +40 mV), the inactivating phase of the currentwas well fit with a single exponential, having a time constantnear 40 msec (data not shown), considerably slower than in theabsence of Cd²⁺ (~20-25 msec) (n = 5; p < 0.05, Mann-Whitney U test). The relativevoltage independence of the time constants argues that the slowingin Cd²⁺ was not caused by the shift in the voltage dependence of inactivation.In contrast, the recovery of the A-type current from inactivationat $-$ 100 mV was not noticeably altered by Cd²⁺ (data not shown) (n = 5; p > 0.05, Mann-Whitney U test).

The A-type current was potently reduced by 4-aminopyridine but not tetraethylammonium

One of the hallmarks of A-type currents is their sensitivity to 4-AP (Rogawski, 1985). In invertebrate neurons, 4-AP blocksA currents in a voltage- and time-dependent manner (Thompson,1982). This aspect of the 4-AP block has been reported much lesscommonly in vertebrate neurons (Gustafsson et al., 1982; Surmeieret al., 1988; Huguenard et al., 1991; Stefani et al., 1992; Wuand Barish, 1992; Foehring and Surmeier, 1993; Nisenbaum et al.,1996). When applied to cholinergic interneurons, 4-AP reducedthe peak current in a dose-dependent manner (Fig. 6A). The IC₅₀of 4-AP was near 1 mM, assessed isochronally at the peak of thecontrol current (Fig. 6B). In addition, 4-AP increased the amplitudeof the current later in the pulse, creating a crossover of thecurrent. This pattern of effects is typical of what has previouslybeen described in invertebrate neurons and in heterologous expressionsystems transfected with Kv4.2 cRNA (Tseng et al., 1996). Thecurrent crossover after 4-AP application also suggests that therewas little or no 4-AP-sensitive delayed rectifier current in theseneurons.

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Figure 6. 4-AP blocked A-type currents in interneurons. A, K⁺ currents evoked by a step to +20 mV in the presence of increasing concentrations of 4-AP. Note the prominent crossover of currents at >1 mM concentrations. B, Plot of average peak current ± SEM (measured isochronously) as a function of 4-AP concentration for a sample of four neurons. The data were fit with a Langmuir isotherm with 1 mM IC₅₀.

In contrast, TEA preferentially blocked the sustained, delayed rectifier component of the current. As shown in Figure 7A,increasing concentrations of TEA reduced both peak and sustainedcurrent components. Difference current estimates of the TEA-sensitivecurrents revealed that at low millimolar concentrations, onlya persistent current was blocked (Fig. 7B). This is consistentwith the well described ability of TEA to block delayed rectifier-typechannels (Rudy, 1988). The IC₅₀ of the TEA block of the persistentcurrent was ~11 mM (Fig. 7C). However, it should be noted thatat TEA concentrations >10 mM a portion of the inactivating currentwas also blocked, suggesting that the transient, A-type currentin interneurons was not as insensitive to TEA as other types ofinactivating K⁺ channel (Stuhmer et al., 1989).

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Figure 7. TEA preferentially blocked delayed rectifier currents. A, K⁺ currents evoked by a step to +20 mV in the presence of increasing concentrations of TEA. B, TEA-sensitive currents isolated by subtraction from the control trace in A. Note that below ~10 mM TEA, the transient component of the current is relatively unaffected. C, Plot of average current amplitude ± SEM measured at the end of the voltage step as a function of TEA concentration for a sample of four neurons. The data were fit with a Langmuir isotherm with 11 mM IC₅₀.

Cholinergic interneurons coexpress K⁺ subunits that form A-like channels

To identify the channel subunits responsible for the A-like current seen in whole-cell recordings, single-cell RT-PCR experimentswere performed. Five K⁺ channel subunits are known to form homomeric channels that haveA-like properties: Kv1.4, Kv3.4, Kv4.1, Kv4.2, and Kv4.3 (Stuhmeret al., 1989; Baldwin et al., 1991; Schroter et al., 1991; Serodioet al., 1994; Serodio et al., 1996). In addition, Kv1 family channelsthat normally yield delayed rectifier type currents inactivaterapidly in the presence of ancillary $beta$ 1 subunits (Rettig et al.,1994; Heinemann et al., 1996; Sewing et al., 1996). To generateas comprehensive a profile as possible of A-type subunit mRNAexpression, individual cholinergic interneurons were simultaneouslyanalyzed for the expression of Kv1.1, Kv1.2, Kv1.4, Kv1.5, Kv3.4,Kv4.1, Kv4.2, Kv4.3, and $beta$ 1-3 mRNAs.

These experiments revealed that several of the subunits capable of forming A-like channels were coexpressed in interneurons.A photograph of an ethidium bromide-stained gel in which PCR ampliconsfrom an individual cell have been separated by electrophoresisis shown in Figure 8A. A summary of the expression patterns ofindividual neurons is shown in Figure 8B. The only transcriptthat was detected in every neuron profiled was Kv4.2. Other subunitsknown to form homomeric channels with A-like properties were detectedin a subset of cells (Kv4.1 and Kv1.4, ~60% of all cells; n =32) or not detected at all (Kv4.3 and Kv3.4; n = 32).

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Figure 8. Interneurons express several $alpha$ subunit mRNAs capable of producing A-type channels. A, Photomicrograph of an ethidium bromide-stained gel in which the PCR products from a single cholinergic interneuron have been separated by electrophoresis. This neuron had detectable levels of $beta$ 1, $beta$ 3, Kv1.4, Kv4.1, and Kv4.2 mRNAs. Lanes at either end of the gel are size markers. B, Summary diagram of the expression profiles in 15 cholinergic interneurons. The percent of the sample in which a particular mRNA was detected is coded by the total length of the bar. C, D, The question of heterogeneity of Kv4.2 and Kv1.4 mRNA expression in ChAT interneurons was addressed by serially diluting the total cellular cDNA from the same cell for PCR. C, Photographs of two representative gels from two different cells show clear presence of Kv4.2 amplicons with 2⁶ () or larger amounts of the total cellular cDNA, whereas only 2² (1/4) or more of the total cell cDNA was enough to see Kv1.4 amplicons clearly. D, Summary of the data from such experiments for Kv1.4 (n = 22) and Kv4.2 (n = 15) mRNAs. The distribution of threshold dilutions for each mRNA is plotted as a normalized density. The smooth lines are Gaussian fits of the distributions. Note unimodal distribution for both mRNAs.

The mRNA for $beta$ subunits was also commonly detected. $beta$ 1 and $beta$ 2 mRNAs were much more commonly detected than $beta$ 3 mRNA. The mRNAsfor some of the Kv1 family subunits known to complex with $beta$ 1 subunitsto yield A-like channels were also found in a subset of interneurons(Kv1.1, ~50%; Kv1.2, ~20%; Kv1.5, 0%; n = 27).

There are several potential reasons why a particular transcript might be detected in only a subset of neurons. One possibilityis that the expression of that transcript varies across the interneuronalpopulation, with some neurons expressing high levels and othersexpressing low or undetectable levels. Another possibility isthat inefficiencies in the RT-PCR reaction are responsible. Thiscould be attributable to inefficient reverse transcription resultingfrom protein and RNA binding to the transcripts or secondary structureof the transcript. It also could be attributable to inefficientPCR amplification.

Distinguishing between biological and technical possibilities is particularly important for the interpretation of the Kv1.4mRNA profiles. Kv1.4 transcripts were the only detectable non-Kv4family subunit mRNAs that could produce A-type K⁺ channels with properties similar to those observed in interneurons.It was our working hypothesis that limitations in the RT-PCR reactionwere responsible for the variation in Kv1.4 detection, not heterogeneitywithin the interneuronal population. To test this hypothesis,serial dilution experiments were performed. The rationale forthese experiments is as follows. First, it is assumed that theRT-PCR efficiency for any one transcript is constant. Next, itis assumed that the fraction of the total cellular cDNA necessaryto detect a particular transcript is inversely related to itsabundance or amplification efficiency. This threshold fractioncan be determined by performing the PCR reaction with serial dilutionsof the original cellular cDNA. If there are two populations ofneurons, one expressing a transcript at high levels and anotherexpressing the same transcript at low levels, the distributionof thresholds across that population should be bimodal.

Serial dilution profiles for Kv4.2 and Kv1.4 mRNAs in two interneurons are shown in Figure 8C. A summary of these experimentsis shown in Figure 8D. It is evident that the threshold densitiesfor both Kv4.2 and Kv1.4 mRNAs were unimodal, suggesting thatthe interneuron population was homogeneous with regard to thesetwo mRNAs.

Somatodendritic A-type currents are attributable to channels with Kv4.2 and Kv4.1 subunits

Based on the RT-PCR analysis, the somatodendritic A-type currents could have arisen from several different channel types.Despite the fact that their mRNA was present, Kv1.1 and $beta$ 1 subunit-containingchannels are unlikely to have made a significant contributionto somatodendritic currents, because their 4-AP affinity is considerablyhigher than the channels responsible for the observed currents(Stuhmer et al., 1989; Rettig et al., 1994). Moreover, their inactivationrates are much faster than those seen in interneurons (Rettiget al., 1994). The potential contribution of Kv1.2 and $beta$ 1 channelscan be discounted on the same grounds. However, Kv4 and Kv1.4channels have more similar pharmacological sensitivities and inactivationkinetics (Stuhmer et al., 1989; Serodio et al., 1994). One biophysicalfeature that distinguishes these channel types in heterologoussystems is recovery from inactivation (Bertoli et al., 1994, 1996;Serodio et al., 1994). Unlike Kv4 family channels, Kv1.4-containingchannels have a slow component of inactivation recovery with atime constant of seconds. As shown in Figure 4, E and F, a veryslow component of inactivation recovery was not present (or verysmall) in this sample of neurons. To provide further confirmationof this result and the inference from the serial dilution experimentsthat the interneuron population was homogeneous, combined patch-clampand RT-PCR experiments were performed. In these experiments, therecovery kinetics of the A-type current were determined, and thenthe neuron was aspirated and profiled for ChAT, Kv4.2, and Kv1.4mRNAs. A typical recovery record is shown in Figure 9A. Normalizedplots of peak current as a function of recovery interval at $-$ 95mV in cells having detectable levels of Kv1.4 (filled symbols;n = 4) and those only having detectable levels of Kv4.2 (opensymbols; n = 7) are shown in Figure 9B. The inset is a scatterplot of the amplitudes of the fast and slow components of recoveryfor each group. There was no obvious relationship between thedetection of Kv1.4 and the properties of inactivation recovery.In none of the cells examined was there a prominent componentof recovery with a time constant of seconds.

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Figure 9. Inactivation recovery kinetics were not correlated with the detection of Kv1.4 mRNA. A, Inactivation recovery was examined by a double-pulse protocol. Current responses to two 200 msec test pulses to $-$ 20 msec separated by increasing the intervals at $-$ 95 mV were recorded while holding the cell at $-$ 95 mV. Note almost complete recovery after 1.5 sec at $-$ 95 mV. B, Plot of peak current as a function of interpulse duration. After recordings the cells were tested by RT-PCR for the presence of Kv4.2 and Kv1.4 mRNA. Kv4.2 mRNA was detected in all, whereas Kv1.4 mRNA was detected only in 4 of 10 cells. Note the almost complete overlap of the traces from the cells in which Kv1.4 mRNA was detected (filled circles) and the cells in which Kv1.4 mRNA was not detected (open circles). Inset, No correlation is shown between the amplitude of slow or fast components of recovery from inactivation and the presence of Kv1.4 mRNA (filled circles). C, D, The presence of a very slow (>1 sec) recovery from inactivation was tested by comparison of current amplitude after 1.5 sec prepulse to $-$ 95 mV (open triangles) and after 25 sec prepulse to $-$ 95 mV. Line, open circles, Current after prepulse to $-$ 60 mV. In the cell of C, no Kv1.4 mRNA was detected as shown in the inset. In contrast, in the cell of D, Kv 1.4 mRNA was detected after recording as shown in the inset. Note that there is almost no difference between the cells in C and D in recovery kinetics.

To ensure that a slow component of recovery was not missed, an additional experiment was performed. First, the A-type currentwas inactivated by holding at $-$ 60 mV. Then, the cell was steppedto $-$ 95 mV for either 1.5 or 25 sec before the delivery of a teststep to $-$ 20 mV. As shown in Figure 9, C and D, the currents evokedby the test step were very similar after holding at $-$ 95 mV for1.5 sec and for 25 sec, arguing against the presence of a significantslow component of inactivation recovery. This was true in neuronsin which only Kv4.2 mRNA (Fig. 9C) was detected as well as incells in which both Kv4.2 and Kv1.4 mRNA was found (Fig. 9D).

Although these results strongly implicate Kv4.2- and Kv4.1-containing channels, they depend on the assumption that the propertiesof heterologously expressed channels are similar to those in nativeexpression systems. To provide an additional test of our hypothesis,immunocytochemical studies were performed using a monoclonal Kv1.4antibody and an affinity-purified polyclonal antibody that recognizesKv4.2 and potentially Kv4.3 subunits. These experiments revealedthat Kv1.4 subunits were localized primarily to fibers withinthe striatum and terminal fields within the globus pallidus (Fig.10A). In contrast, Kv4.2 and Kv4.3 subunits were clearly presentwithin the somata and dendrites of large striatal neurons (Fig.10B, arrowheads); medium-sized neurons were also labeled but toa lesser extent. Double-label immunocytochemistry for Kv4.2 andKv4.3 (Fig. 10C) and ChAT (Fig. 10D) consistently found this K⁺ channel subunit in the dendrites and soma of cholinergic interneurons.Given the apparent absence of Kv4.3 mRNA in ChAT interneurons,the immunoreactivity in the somatodendritic membrane of theseneurons can be attributed to Kv4.2 subunits.

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Figure 10. The somatodendritic membrane of cholinergic interneurons possesses Kv4.2 but not Kv1.4 immunoreactivity. A, Immunohistochemical localization of Kv1.4 in the striatum. Kv1.4-immunoreactive fiber bundles (arrowheads) course through the striatum to the globus pallidus (GP). Neuronal somata within the striatum show no immunoreactivity to Kv1.4. Note a dense Kv1.4 staining in the GP. B, Immunohistochemical localization of Kv4.2C in the striatum. Medium to large somata (arrowheads) were densely labeled with Kv4.2C, whereas small cells were weakly labeled. Note that proximal dendrites of medium to large cells were also labeled. C, D, Examples of striatal neurons double-labeled for Kv4.2C (C) and ChAT (D). C, Two neurons labeled for Kv4.2C with FITC. D, the same two neurons were labeled for ChAT and visualized with Texas Red. Scale bars: A, 50 µm; B, 100 µm; C, D, 50 µm.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Interneuronal somatodendritic K⁺ currents are largely attributable to A-type channels

The results presented show that depolarization-activated, Ca²⁺-independent K⁺ currents in the somatodendritic membrane of striatal interneuronsare dominated by an A-type current. This conductance had manyof the biophysical and pharmacological features of A-type conductancesdescribed previously in invertebrate (Connor and Stevens, 1971a;Neher, 1971; Hagiwara et al., 1981) and vertebrate cells (Rogawski,1985; Rudy, 1988). In particular, the K⁺-selective conductance began to activate at subthreshold potentials,having a half-activation voltage near $-$ 27 mV. On depolarization,the conductance inactivated monoexponentially with a time constantbetween 20-25 msec at all potentials in which evoked currentscould be accurately measured ( $-$ 40 mV or greater). Steady-stateinactivation developed at membrane potentials below the activationthreshold and was accurately described by a Boltzmann functionwith a half-inactivation voltage near $-$ 90 mV.

A notable feature of the A-type current in these neurons was its sensitivity to extracellular Cd²⁺. The addition of 20-400 µM Cd²⁺ to the bath shifted the voltage dependence of activation by 32mV, whereas the voltage dependence of inactivation was shiftedeven more (57 mV). In addition, the kinetics of inactivation atdepolarized potentials were slowed by extracellular Cd²⁺, decaying monoexponentially with a time constant of 40-50 msecrather than 20-25 msec. In contrast, the kinetics of recoveryfrom inactivation were not altered. Qualitatively similar effectsof Cd²⁺ on gating of A-type currents have been described previously (Mayerand Sugiyama, 1988; Agus et al., 1991; Andreasen and Hablitz,1992; Klee et al., 1995), although the magnitude of the shiftsin activation and inactivation were substantially larger in cholinergicinterneurons.

The properties of the A current are consistent with channels composed of Kv4.2 and Kv4.1 subunits

Insights into the molecular architecture of the A-type channels in cholinergic interneurons is of clear value to understandinghow these channels contribute to interneuron physiology and signaling.Molecular cloning and heterologous expression studies have shownthat Kv1.4, Kv3.4, Kv4.1, Kv4.2, and Kv4.3 subunits are capableof forming homomeric channels that rapidly inactivate and aresensitive to 4-AP, the hallmarks of A-type channels (Stuhmer etal., 1989; Baldwin et al., 1991; Schroter et al., 1991; Serodioet al., 1994, 1996). In addition, $beta$ 1 subunits are capable of transformingdelayed rectifier-like channels composed of Kv1 family subunits(Kv1.1, Kv1.2, and Kv1.5) into rapidly inactivating, A-like channels(Rettig et al., 1994; Heinemann et al., 1996; Sewing et al., 1996).To determine which of these subunits contributed to the channelsunderlying the K⁺ currents seen in cholinergic interneurons, single-cell RT-PCRprofiling was performed. These techniques have been used successfullyin the past to identify a wide range of cellular mRNAs, includingthose coding for voltage-dependent K⁺ channels (Gurantz et al., 1996; Baro et al., 1997). The latterstudy also used quantitative techniques to show a linear relationshipbetween mRNA abundance and apparent channel abundance.

Our studies suggested that Kv1.5, Kv3.4, or Kv4.3 subunits are not expressed at significant levels in cholinergic interneurons,despite their ready detection in other cell types and in whole-braincDNA (data not shown). However, these experiments did reveal thepresence of Kv4.2, Kv4.1, Kv1.4, Kv1.1, Kv1.2, and $beta$ 1 mRNAs. Withthe exception of Kv4.2 mRNA, not all of these mRNAs were foundin every interneuron. Does this suggest that there are subsetsof cholinergic interneuron with different complements of K⁺ channels? The unimodal distribution of detection thresholds forKv4.2 and Kv1.4 mRNAs argues against this interpretation. A morelikely interpretation is that the failure to detect Kv1.4, Kv4.1,Kv1.1, and Kv1.2 mRNA in some neurons is a reflection of low mRNAabundance and/or inefficiencies in the RT-PCR procedure.

If we assume that all these subunit mRNAs are present in interneurons, do they all contribute to channels underlying the somatodendriticcurrents? Several observations strongly argue against this scenario.Because subunits from Kv1 and Kv4 gene families do not coassembleto form heteromeric channels (McCormack et al., 1990; Covarrubiaset al., 1991), it is necessary only to consider the propertiesof channels with subunits derived from one or the other family.One of the hallmarks of channels composed of Kv1 family $alpha$ subunitsis the presence of a slow component of inactivation recovery witha time constant in the range of seconds, rather than milliseconds(Bertoli et al., 1994, 1996; Rettig et al., 1994). In contrast,A currents in cholinergic interneurons recovered rapidly withinactivation time constants of near 20 and 300 msec. So, despitethe similarity in voltage dependence and kinetics of inactivationdevelopment, homomeric Kv1.4 channels are unlikely to be significantcontributors. Kv1.1, Kv1.2, and Kv1.4 channels with $beta$ 1 subunitscan also be discarded on the same grounds, as well as their morerapid inactivation development (Rettig et al., 1994; Heinemannet al., 1996).

If channels composed of Kv1 family subunits do not underlie the A current, then do channels containing Kv4.2 and Kv4.1 subunits?The pharmacological properties of the Kv4.2 and Kv4.1 channelsare very similar to interneuronal A-type channels. In heterologousexpression systems, Kv4.2 and Kv4.1 channels are potently blockedby 4-AP, with IC₅₀ values in the low millimolar range (Baldwinet al., 1991; Chabala et al., 1993; Serodio et al., 1994, 1996).Moreover, homomeric Kv4.2 channels exhibit a time- and voltage-dependentblock by 4-AP that is virtually identical to that seen in interneurons(Tseng et al., 1996; Fiset et al., 1997). Kv4.2 channels are alsorelatively insensitive to TEA, as were the A-type channels ininterneurons. Cd²⁺ also dramatically shifts the voltage dependence of Kv4.2 channelstoward more depolarized potentials (Fiset et al., 1997), possiblyreflecting the presence of cysteine residues within a region ofthe pore involved in gating (Yellen et al., 1994). However, thevoltage dependence of activation and inactivation of Kv4 channelsexpressed in Xenopus oocytes is considerably more depolarizedthan the currents seen here (Baldwin et al., 1991; Serodio etal., 1994, 1996). Furthermore, the development and recovery frominactivation is slower. However, when a brain-derived 2-4 kb cRNAfraction is coinjected with Kv4.2 subunit cRNA, the resultingchannels give rise to currents that are very similar in voltagedependence and kinetics to the A currents in interneurons (Chabalaet al., 1993; Serodio et al., 1994).

The inference that Kv4.2 subunits are major constituents of K⁺ channels in the proximal somatodendritic membrane of cholinergicinterneurons and that Kv1.4 subunits are not is in agreement withimmunocytochemical studies of the subcellular localization ofthese subunits shown here and in studies in other cell types (Shenget al., 1992, 1993; Alonso and Widmer, 1997) (cf. Maletic-Savaticet al., 1995). Like previous studies, we found evidence for Kv4.2subunits in the somatodendritic membrane of cholinergic interneuronsand medium spiny neurons, whereas Kv1.4 subunits were restrictedto axons and terminals. A similar subcellular distribution hasbeen inferred for sympathetic ganglion neurons based on RNaseprotection and physiological assays (Dixon and McKinnon, 1996).Although the immunocytochemical and molecular evidence presentedmakes a strong case, this evidence is correlative. Unequivocalproof that somatodendritic A-type K⁺ channels are dominated by Kv4.2 and Kv4.1 subunits will comeonly from a more direct demonstration, such as that afforded byantisense knockdowns of Kv4.2 mRNA.

The properties of A-type channels are consistent with a role in allowing slow repetitive discharge

One of the first cellular functions attributed to A-type currents was the slowing of interspike depolarization (Connor andStevens, 1971b). This slowing enabled neurons to discharge atvery slow rates, a capacity that was absent in early Hodgkin-Huxleymodels based on axonal currents. To accomplish this goal, theA-type conductance needs to open at subthreshold membrane potentialsand then inactivate, allowing spike threshold to be reached. Onrepolarization of the spike, channels must reprime or deinactivatequickly, so that the ensuing depolarization is capable of openingthem once again. These three features, subthreshold activation,rapid inactivation, and rapid recovery from inactivation, wereall features of the A current in cholinergic interneurons. Theyare also characteristics of Kv4.2 and Kv4.1 channels when combinedwith an ancillary protein (Serodio et al., 1994, 1996).

Another feature of these channels that is of potential functional importance was their sensitivity to Cd²⁺. The dramatic effects of Cd²⁺ on the voltage dependence and kinetics of A-channel gating suggestthat these channels may be allosterically regulated by other divalentcations. Zn²⁺ is a particularly intriguing candidate in this regard. Histochemicalstudies have shown a high levels of vesicular Zn²⁺ in the striatum (Vincent and Semba, 1989; Mengual et al., 1995).The distribution of Zn²⁺ is not uniform and is often associated with striosomal compartments,particularly in the rostral striatum. If the vesicular Zn²⁺ is coreleased from glutamatergic terminals as it is in otherregions (Assaf and Chung, 1984), corticostriatal activity couldallosterically modulate the voltage dependence of interneuronalA-type channels. In agreement with previous work (Huang et al.,1993; Erdelyi, 1994; Spires and Begenisich, 1994), preliminarystudies have shown that Zn²⁺ (100 µM) does shift the voltage dependence of A current channelgating, although not as potently as Cd²⁺. This modulation should disenable slow, repetitive activity andpromote higher-frequency, less-regular discharge.

  FOOTNOTES

Received Sept. 15, 1997; revised Feb. 9, 1998; accepted Feb. 10, 1998.

This work was supported by National Institute of Neurological Diseases and Stroke, United States Public Health Service GrantsNS-34696 to D.J.S. and NS-26473 to D.J.S. and S.T.K. and a Parkinson'sDisease Foundation fellowship to W.J.S. We thank Dr. J. Flores-Hernandezfor assisting in some of the physiological experiments, Dr. B.Teng for help in the immunocytochemical experiments, and Dr. L.Dudkin for her technical help. We also thank Dr. James Trimmerfor providing Kv4.2C antisera.
W.-J.S., T.T., and G.B. contributed equally to this work.

Correspondence should be addressed to Dr. D. J. Surmeier, Department of Anatomy and Neurobiology, University of Tennessee,855 Monroe Avenue, Memphis, TN 38163.

Dr. Song's present address: Department of Biophysical Engineering, Faculty of Engineering Science, Osaka University, Toyonaka560, Japan.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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