Distinct Contributions of High- and Low-Voltage-Activated Calcium Currents to Afterhyperpolarizations in Cholinergic Nucleus Basalis Neurons of the Guinea Pig

Life science instruments for behavioral neuroscience research

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (29)

Citing Articles via Google Scholar

Google Scholar

Articles by Williams, S.

Articles by Bernheim, L.

Search for Related Content

PubMed

PubMed Citation

Articles by Williams, S.

Articles by Bernheim, L.

Previous Article  |  Next Article

Volume 17, Number 19, Issue of October 1, 1997 pp. 7307-7315
Copyright ©1997 Society for Neuroscience

Distinct Contributions of High- and Low-Voltage-Activated Calcium Currents to Afterhyperpolarizations in Cholinergic Nucleus Basalis Neurons of the Guinea Pig

Sylvain Williams, Mauro Serafin, Michel Mühlethaler, and Laurent Bernheim
Département de Physiologie, Centre Médical Universitaire, 1211 Genève 4, Switzerland

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

The contributions made by low- (LVA) and high-voltage-activated (HVA) calcium currents to afterhyperpolarizations (AHPs) ofnucleus basalis (NB) cholinergic neurons were investigated indissociated cells. Neurons with somata >25 µM were studied because80% of them stained positively for choline acetyltransferase andhad electrophysiological characteristics identical to those ofcholinergic NB neurons previously recorded in basal forebrainslices. Calcium currents of cholinergic NB neurons first weredissected pharmacologically into an amiloride-sensitive LVA andat least five subtypes of HVA currents. Approximately 17% of thetotal HVA current was sensitive to nifedipine (3 µM), 35% to $omega$ -conotoxin-GVIA(200-400 nM), 10% to $omega$ -Agatoxin-IVA (100 nM), and 20% to $omega$ -Agatoxin-IVA(300-500 nM), suggesting the presence of L-, N-, P-, and Q-typechannels, respectively. A remaining current (R-type) resistantto these antagonists was blocked by cadmium (100-200 µM). We thenassessed pharmacologically the role that LVA and HVA currentshad in activating the apamin-insensitive AHP elicited by a longtrain of action potentials (sAHP) and the AHP evoked either bya short burst of action potentials or by a single action potential(mAHP) that is known to be apamin-sensitive. During sAHPs, ~60%of the hyperpolarization was activated by calcium flowing throughN-type channels and ~20% through P-type channels, whereas T-,L-, and Q-type channels were not involved significantly. In contrast,during mAHPs, N- and T-type channels played key roles (~60 and30%, respectively), whereas L-, P-, and Q-type channels were notimplicated significantly. It is concluded that in cholinergicNB neurons various subtypes of calcium channels can differentiallyactivate the apamin-sensitive mAHP and the apamin-insensitivesAHP.
Key words: acetylcholine; afterhyperpolarization; arousal; basal forebrain; calcium currents; low-threshold spike

INTRODUCTION

Cholinergic neurons of the nucleus basalis (NB) represent the principal source of cholinergic fibers that innervate the cerebralcortex (for review, see Jones, 1993; Mesulam, 1995). Because thisarea receives numerous inputs from brainstem nuclei (Jones, 1993)and because acetylcholine has been demonstrated to exert an excitatoryaction on cortical neurons (for review, see McCormick, 1992),the NB is viewed as a major relay of a cortical activating systemimplicated in the control of arousal (Jones, 1994). Cholinergicneurons of the NB differ from those of the medial septum (Markramand Segal, 1990; Gorelova and Reiner, 1996) by their localization,projections, and electrophysiological properties. They are distinguishedin particular by their ability to discharge in rhythmic burstsof action potentials (APs) when they are activated from a hyperpolarizedlevel (Khateb et al., 1992, 1995; Alonso et al., 1996), whereasthey fire tonically when they are depolarized from rest. Theserhythmic bursts are subtended by strong low-threshold calciumspikes resulting from the presence in these cells of an importantlow-voltage-activated (LVA) calcium current (Khateb et al., 1992;Allen et al., 1993; Griffith et al., 1994).

The afterhyperpolarization (AHP) that follows a burst of APs (mAHP) in NB cells is apamin-sensitive (Khateb et al., 1995)and as such is similar to the AHP evoked by a single AP in cholinergicbasal forebrain neurons (Matthews and Lee, 1991; Gorelova andReiner, 1996). In contrast, in the same type of cells, long trainsof APs elicit a long-lasting AHP (sAHP) that is apamin-insensitive(Matthews and Lee, 1991; Gorelova and Reiner, 1996). These twotypes of AHPs (sensitive or insensitive to apamin) are both initiatedby calcium influx through voltage-gated calcium channels, butthe precise contribution of the various calcium current subtypesto the genesis of AHPs is not known in these cells and is, ingeneral, still a matter of debate in central neurons (Sah, 1996).

The major goal of the present study was thus to investigate in dissociated cholinergic NB neurons the involvement of the differentsubtypes of calcium currents in the activation of these two delayedAHPs. The underlying hypothesis was that different firing patterns(tonic vs bursting) could elicit AHPs that depend on contributionsmade by different calcium channels. We were interested in particularto determine whether the T-type current could play a role in themAHP, because this current is a major determinant of the burstpattern of discharge typical of these cells. To our knowledgea contribution of the T-type current to mAHP has never been demonstratedbefore.

A preliminary goal for understanding the respective contribution of the various calcium current subtypes to the AHPs was todissect them pharmacologically by using calcium channel antagonists.In previous studies only T-, L-, and N-type calcium currents weredescribed in cholinergic basal forebrain neurons (Allen et al.,1993; Griffith et al., 1994; Williams et al., 1997). However,because coapplication of nifedipine and $omega$ -conotoxin-GVIA did notblock the total high-voltage-activated (HVA) current completely,additional subtypes must be present in these cells. P-, Q-, andR-type HVA currents now have been identified in various preparations(Mintz et al., 1992; Sather et al., 1993; Stea et al., 1994; Randalland Tsien, 1995). Hence, in addition to T-, L-, and N-type currents,these more recently described subtypes also might be present incholinergic NB neurons and possibly contribute to activate AHPs.

In this report we present evidence that the N-type current plays a key role in activating both apamin-sensitive and apamin-insensitiveAHPs in cholinergic NB neurons. In addition, depending on thefiring pattern, either P- or T-type currents also contribute tothe activation of AHPs and thus could participate in regulatingthe firing properties of these cells.

MATERIALS AND METHODS
Dissociation. Slices from young guinea pigs (80-200 gm) were obtained by standard methods (Khateb et al., 1992, 1993) andwere dissociated with a slightly modified version of the methoddeveloped by Kay and Wong (1986). Briefly, guinea pigs were anesthetizeddeeply with Nembutal and decapitated. The brain was removed andrapidly transferred in cold (4°C) oxygenated (95% O₂/5% CO₂) physiologicalsaline containing (in mM): 130 NaCl, 20 NaHCO₃, 1.25 KH₂PO₄, 1.3MgSO₄, 5 KCl, 10 glucose, and 2.4 CaCl₂, pH 7.35. With a vibratome(Campden Instruments, Berlin, Germany), two to three slices (400µM thick) containing the basal forebrain were cut and left atroom temperature for a period of 1 hr in physiological saline.For dissociations, slices were immersed first in a 100% oxygen-equilibratedPIPES solution containing (in mM): 120 NaCl, 5 KCl, 0.5 CaCl₂,1 MgCl₂, 25 glucose, and 20 PIPES, pH-adjusted to 7.0 with NaOH.Then the region of interest, which included the substantia innominata,the horizontal limb of the diagonal band, and the magnocellularpreoptic nucleus [Paxinos and Watson (1986); see Gritti et al.(1993) for a discussion on basal forebrain cholinergic nuclei],was dissected out (one piece from each hemisphere) with a smallrazor blade. The regions of the medial septum and the verticallimb of the diagonal band containing most of the septohippocampal-projectingneurons were excluded. In this study the term NB neurons willbe used to characterize those cells located within the regionof interest mentioned above. The tissue was placed in small testtubes containing an oxygenated PIPES solution with the enzymetrypsin (Sigma type XII, 0.8 mg/ml; St. Louis, MO) for 120 minat 30°C. The enzymatic reaction was stopped by rinsing the tissuewith 10% goat or horse serum (Life Technologies, Gaithersburg,MD) and left to rest in enzyme-free PIPES for at least anotherhour. Neurons were dispersed by triturating in HEPES (see below)with two different sizes of fire-polished Pasteur pipettes. Thesuspension was transferred to a Cell-tak (Becton Dickinson Labware,Heidelberg, Germany)-coated Petri dish, which was mounted on aninverted microscope (Zeiss, Oberkochen, Germany). Healthy neuronsadhered to the bottom of the dish within 15 min.

Whole-cell recording and solutions. Voltage-clamp recordings from neurons were obtained by using the whole-cell version ofthe patch-clamp technique (Hamill et al., 1981). Patch pipetteswere pulled (Sutter Instruments, Novato, CA) from borosilicateglass (1.5 outer diameter and 0.86 inner diameter; Clark ElectromedicalInstruments, Pangbourne, UK) and had resistances typically of2-4 M $Omega$ in the bath solution. Signals were recorded with an Axopatch200A amplifier (Axon Instruments, Foster City, CA) and monitoredon a 486 PC clone equipped with pClamp software (version 6.0)and a 125 kHz interface (Digidata 1200, Axon Instruments). Recordswere low-pass-filtered at 2 or 5 kHz with a Bessel filter. Typicalaccess resistances ranged from 4-8 M $Omega$ , and compensation of 70-80%was used. Linear leak current and capacitive transients were subtractedby using a P/4 protocol or by subtracting raw traces from thosein the presence of cadmium (100-200 µM). The internal recordingsolution contained the following (in mM): 130 Cs-methylsulfonate,20 CsCl, 5 MgCl₂, 5 HEPES, 3 Na₂ATP, 0.2 GTP-Na, 0.1 BAPTA, and14 phosphocreatine, pH-adjusted to 7.3 with CsOH. Neurons wereperfused continuously (3 ml/min) with a HEPES medium containing(in mM): 150 NaCl, 2.5 KCl, 2 CaCl₂, 1 MgCl₂, 8 glucose, and 10HEPES, pH-adjusted to 7.3 with NaOH. Calcium currents were isolatedby adding tetrodotoxin (1 µM, Latoxan), tetraethylammonium (20mM), and 4-aminopyridine (4 mM) to the HEPES medium. To studymembrane properties and AHPs in current-clamp mode, we perfusedisolated neurons with a HEPES medium (see above) and recordedthem with an internal solution containing (in mM): 121 K-methylsulfate(Pfaltz & Bauer, Waterbury, CT), 4.5 KCl, 5 MgCl₂, 5 HEPES, 3Na₂ATP, 0.1 GTP, 0.1 BAPTA, and 14 phosphocreatine, pH-adjustedto 7.4 with NaOH.

Drugs were applied close to the recorded neuron by a multibarreled pipe system constructed with polyethylene tubing accordingto the method of Bertrand et al. (1997). All drugs were preparedin single-use aliquots and thawed on the day of the experiment.Amiloride (Sigma), $omega$ -conotoxin-GVIA (Alomone Labs, Jerusalem,Israel), and $omega$ -Agatoxin-IVA (gift from Pfizer, New York, NY) wereprepared in distilled water and kept frozen at $-$ 20°C until theday of the experiment. Agatoxin-IVA was aliquoted with cytochromec (0.05%, Sigma) to prevent nonspecific binding to plastic tubing(Mintz et al., 1992). Nifedipine (Sigma) was diluted in dimethylsulfoxide(<0.1%). All experiments were performed at room temperature (20-22°C).

Run-down of calcium currents was greatly minimized by using Cs-methylsulfonate (Zhang et al., 1994) supplemented with ATPand phosphocreatine in the patch pipette (McDonough et al., 1996),by using test pulses that were only 20-40 msec in duration (Murchisonand Griffith, 1996), and, finally, by activating currents no morethan once every 7 sec. In these conditions, run-down of the HVAcalcium current was estimated to be 3.7% per 3 min (n = 3). Accessresistance was checked periodically. The amplitude of the LVAand HVA currents was measured at the peak. The amplitude of theAHP after a burst of APs was determined by taking the differencebetween a point 50 msec before the beginning of the first AP andthe value at the peak of the AHP. For the AHP evoked by a trainof depolarizing current steps (each one eliciting a single AP),measurement of the amplitude was taken at the peak of the AHPfrom the average of two or three traces. All means are expressedas mean ± SE.

Immunocytochemistry. The tissue containing the NB was treated with trypsin as described above. Then the tissue was trituratedin PBS, pH 7.4, and neurons were dispersed onto a Cell-tak-coatedPetri dish. Neurons were rinsed for 45 sec in PBS containing 4%paraformaldehyde (Fluka, Neu-Ulm, Germany) and for 5 min in PBScontaining 0.02% Triton X-100 (Sigma). Afterward, neurons wereincubated for 20 min with a primary rat antibody for choline acetyltransferase(ChAT) Khateb et al., 1992) (dilution 1:250; Jackson ImmunoResearch,West Grove, PA). Nonspecific immunostaining was reduced by rinsingneurons for 20 min with PBS containing 10% normal goat serum.Then the neurons were incubated with a secondary sheep FITC-conjugatedanti-rat antibody (Sigma) for 20 min (dilution 1:320) and finallywere rinsed in PBS for another 20 min. The size of the neuronswas estimated by measuring the longer axis of their soma, excludingthe proximal portion of primary dendrites.

RESULTS

Identification of neurons
Neurons in the NB stain positively for either glutamic acid decarboxylase (GAD), the synthesizing enzyme for GABA, or forChAT, the synthesizing enzyme for acetylcholine (Gritti et al.,1993). It has been suggested from histological analysis that thesetwo populations have similar morphologies (both being bi- or multipolar)but may be distinct with respect to the size of the soma (Nakajimaet al., 1985; Gritti et al., 1993). Hence, ChAT immunostainingwas applied to dissociated NB neurons to characterize the sizeof the soma of both ChAT-positive and ChAT-negative cells (Fig.1A). Neurons that stained positively for ChAT were generally largerin size than those that did not, because 80.9% (n = 93) of neurons>25 µM were ChAT-positive. In contrast, neurons <25 µM compriseda mixed population of neurons. For example, 47.0% (n = 39) ofcells that had a soma between 16 and 25 µM were found to be ChAT-positive.Therefore, to maximize the probability of recordings from neuronswith a cholinergic phenotype, we sampled only neurons >25 µM (29± 3 µm, n = 61) in this study.
Fig. 1. Large dissociated NB neurons are cholinergic. A, Histogram of ChAT-positive and ChAT-negative neurons showing that cells >25µM are mostly cholinergic (>80%). B, In a characteristic cholinergicNB neuron, a hyperpolarizing current step typically elicited onlya weak inward rectifying current (I_h; asterisk), which was followedby an A-type rectification (arrowhead) and burst firing. C, Ata membrane potential of $-$ 62 mV, the same cell responded to a depolarizingcurrent step with regular firing at a low frequency and displayedan AHP at the end of the step. D, In most of the cells, applicationof a depolarizing step from a negative membrane potential ( $-$ 80mV) elicited repetitive bursts of action potentials (enlargedin the inset) that usually were preceded by a delay in firing,presumably because of the A-type current (arrowhead).
[View Larger Version of this Image (20K GIF file)]

Cholinergic NB neurons have been shown in basal forebrain slices to display electrophysiological characteristics distinctfrom those of noncholinergic neurons (Khateb et al., 1992; Alonsoet al., 1994, 1996). Indeed, cholinergic NB neurons show single-spikelow-frequency tonic firing when activated near rest, but theydisplay calcium-dependent low-threshold spikes (LTS) that cantrigger multiple APs when they are activated from a hyperpolarizedlevel. In addition, they exhibit a transient rectification (A-likecurrent) that precedes the LTS and seldom display an inward rectification(Khateb et al., 1992; Alonso et al., 1996). In the present study,dissociated NB neurons >25 µM that were recorded with patch electrodesdisplayed the same electrophysiological properties. Results presentedin Figure 1 show that these cells (57/61) displayed an LTS whenthey were depolarized from a membrane potential more negativethan rest (Fig. 1D), but they responded, in contrast, with a slowtonic firing when they were depolarized from rest (Fig. 1C). Inaddition, whereas they generally displayed a prominent A-likecurrent (56 of 61; arrowhead in Fig. 1B,D), they demonstratedan inward rectification only rarely (4 of 52; asterisk in Fig.1B). Thus, the electrophysiological properties and the ChAT immunostainingboth indicate that neurons with a soma >25 µM are mostly cholinergic.In the present study NB cholinergic neurons had a resting membranepotential more negative than $-$ 60 mV, and, at a depolarized membranepotential of $-$ 52 ± 4 mV (n = 57), APs evoked by small 1-msec-longdepolarizing current steps measured 113 ± 18 mV (from baseline),had a half-width of 1.5 ± 0.4 msec (at 50% amplitude), and hada decay time of 1.7 ± 0.6 msec (from 90% of peak to 10%).

Pharmacology of calcium currents
HVA calcium currents can be separated into distinct components by using pharmacological antagonists (Mintz et al., 1992; Randalland Tsien, 1995; McDonough et al., 1996). In cholinergic basalforebrain neurons, L- and N-type calcium currents have been identifiedin a previous study by using nifedipine and $omega$ -conotoxin-GVIA (cono-GVIA),respectively, but additional subtypes are present because coapplicationof these blockers did not inhibit all of the calcium current (Allenet al., 1993). The effects of these L- and N-type channel blockerswere confirmed in the present study, and the additional presenceof P- and Q-type channels was tested with two different concentrationsof $omega$ -Agatoxin-IVA (Aga-IVA). Indeed, although P-type channelsare known to be inhibited by 100 nM Aga-IVA (Mintz et al., 1992;Mintz and Bean, 1993; McDonough et al., 1996), larger concentrations( $>=$ 200 nM) are necessary to block Q-type channels (Randall andTsien, 1995; Ciranna et al., 1996). Hence to assess for the presenceof Q-type channels, we always added 300-500 nM Aga-IVA after theaddition of 100 nM Aga-IVA.

The effects of cumulative application of antagonists on the peak calcium current from one experiment are plotted as a functionof time in Figure 2A, and current traces are displayed in Figure2B₁. Results for all neurons with the same experimental protocolare shown in Figure 2C₁. These experiments reveal that 3 µM nifedipineblocked 14.6 ± 1.7%, 200-400 nM cono-GVIA blocked 33.0 ± 3.2%,100 nM Aga-IVA inhibited 11.6 ± 2.3%, and 300-500 nM Aga-IVA blocked20.2 ± 3.4% of the total calcium current. The effects of separateapplications of each antagonist on the whole-cell calcium currentwere tested also. Figure 2C₂ shows that 35.2 ± 3.7% of the currentwas blocked by 200-400 nM cono-GVIA, 17.0 ± 2.3% by 3 µM nifedipine,and 10.0 ± 1.8% by 100 nM Aga-IVA. Comparison of the extent ofinhibition obtained with cumulative antagonist applications toseparate antagonist applications revealed that nifedipine didnot interfere with the inhibitory effect of cono-GVIA and thatcoapplication of cono-GVIA with nifedipine did not occlude theeffects of Aga-IVA (compare Fig. 2C₁,C₂). This suggests that theseantagonists were specific for their respective HVA channel subtype.To differentiate further those currents sensitive to low and highconcentrations of Aga-IVA, we measured and compared their timeto peak and decay rates in the same cells in the presence of nifedipine(3 µM) and cono-GVIA (400 nM). It was found that, although thedecay rate of the currents did not differ between the two groupswhen 40-msec-long steps (n = 4) were used, the time to peak ofthe current sensitive to 100 nM Aga-IVA was twice as fast as thatfound for the current sensitive to 400 nM Aga-IVA (7.9 ± 0.4 vs4.1 ± 0.4 msec, n = 4; data not shown). These results furthersupport the idea that low and high concentrations of Aga-IVA reducedistinct components of the HVA calcium current in cholinergicNB neurons, thus indicating the presence of P- and Q-type currents(Sather et al., 1993; Randall and Tsien, 1995) in these cells.A cadmium-sensitive current was left after the addition of allthe antagonists. The threshold of activation of this current alsowas assessed to determine possible similarities with a previouslydescribed R-type (remaining) current (Ellinor et al., 1993) thatis insensitive to all HVA blockers and is known to have an activationthreshold intermediate between LVA and HVA currents. Figure 2Dshows that after the addition of all of the antagonists (filledsymbols), both the threshold of activation and the peak currentof the remaining component appeared unchanged, peaking at 0 mV.Similar results were obtained in three other cells, suggestingthat the remaining current in cholinergic NB neurons displayskinetics that are different from those of the previously describedR-type current. Despite these differences the "R" terminologywas maintained in the present study because it also describeda current resistant to nifedipine, cono-GVIA, and Aga-IVA. Takentogether, these results suggest that cholinergic NB neurons possessat least five distinct types of HVA calcium channels: L-, N-,P-, Q-, and R-types.
Fig. 2. Pharmacological characterization of calcium currents. A, Plot of the peak calcium current versus time during cumulative applicationsof 3 µM nifedipine, 400 nM cono-GVIA, 100 nM Aga-IV, 400 nM Aga-IVA,and 200 µM cadmium. B₁, Whole-cell leak-subtracted current traces(same experiment as in A) elicited by a 40 msec depolarizing stepto 0 mV from a V_h of $-$ 90 mV. In this cell 12% of the total HVAcalcium current was blocked by nifedipine, 37% by cono-GVIA, 7%by Aga-IVA (100 nM), and 12% by Aga-IVA (400 nM), whereas theremaining current (33%) was eliminated by cadmium (200 µM). B₂,Whole-cell leak-subtracted current traces obtained with a depolarizingtest pulse to $-$ 40 mV from a membrane potential of $-$ 90 mV (to activatethe T-type current) showing the reversible block produced by amiloride(300 µM). C, Summary of experiments performed with calcium currentantagonists, expressed in percentage of reduction over the control,for cumulative (C₁) and separate (C₂) applications. D, Peak calciumcurrent as a function of test potential in control conditionsand during cumulative applications of calcium antagonists. A LVAcurrent was evident at potentials greater than $-$ 60 mV and wasfollowed by currents that peaked at 0 mV.
[View Larger Version of this Image (34K GIF file)]

We also investigated the effects of amiloride and HVA blockers on the LVA calcium current (evoked by a test pulse to $-$ 40 mVfrom a holding potential of $-$ 90 mV). Figure 2B₂ shows that amiloridesuppressed the LVA current, as was suggested previously (Tanget al., 1988; Allen et al., 1993). In this cell amiloride reversiblyreduced the LVA current by 64%, whereas the HVA current (evokedby a test pulse to 0 mV) was reduced by only 3% (data not shown).In five cells, 300 µM amiloride reduced the LVA current by 70.8± 1.1% and the HVA current by only 3.0 ± 0.8%. Hence, amilorideshows a high blocking specificity for LVA T-type channels in cholinergicNB neurons. Using separate applications of the HVA blockers, weobserved that cono-GVIA (300 nM; n = 3) had no effect on the LVAcurrent and Aga-IVA (100-400 nM) produced a 9.7 ± 1.8% (n = 4)reduction of this current, whereas 3 µM nifedipine significantlyreduced it by 32.7 ± 4.2% (n = 3). Therefore, whereas cono-GVIAand Aga-IVA were both relatively specific antagonists of differentcomponents of the HVA current, nifedipine also significantly reducedthe T-type LVA current [for review, see Akaike (1991); for cholinergicNB neurons, see Allen et al. (1993)].

Calcium currents and the AHP after a train of APs (sAHP)
Calcium entry through voltage-gated calcium channels is known to be involved in the activation of the AHPs that follow eithera single AP or a train of APs in neurons of the NB (Tatsumi andKatayama, 1993). We (Khateb et al., 1995) and others (Matthewsand Lee, 1991; Gorelova and Reiner, 1996) have shown that theAHP elicited by either a single AP or by bursts of APs in cholinergicbasal forebrain neurons is blocked completely by apamin. On theother hand, the AHP elicited by a train of APs seems to be ofa different kind because it is totally apamin-insensitive (Matthewsand Lee, 1991; Gorelova and Reiner, 1996). In agreement with thesestudies, we found that 100 nM apamin did not affect the sAHP (n= 4; data not shown).

We first assessed the role that each calcium current type played in the apamin-insensitive sAHP. To ensure that the same numberof spikes was elicited in the presence of the various calciumchannel antagonists, we applied trains of short 1-msec-long depolarizations(each event eliciting one AP). The number (10-20 events) and frequency(25-100 Hz) of APs within trains were optimized to always elicitAHPs of maximum amplitude. The applications of either 300 nM cono-GVIAor 100 nM Aga-IVA led to a decrease in the peak AHP amplitude(arrow in Fig. 3A,B); it is, however, noteworthy that the effectof cono-GVIA was clearly more important. In contrast, 300 µM amiloridehad no effect on the AHP (Fig. 3C). The results of separate antagonistsapplications on the sAHP are summarized in Figure 3D. The histogramshows that 59.7 ± 8.3% of the sAHP was reduced by cono-GVIA (200-400nM) and 21.8 ± 1.5% by Aga-IVA (100 nM). On the other hand, nifedipine(3 µM) reduced the sAHP only by 10.5 ± 2.3%, and both the Q-typechannel blocker Aga-IVA at 300-500 nM (added after the additionof 100 nM Aga-IVA) and the T-type channel blocker amiloride (300µM) had only small inhibitory effects on the sAHP. These resultssuggest that N-type channels play a dominant role in activatingthe apamin-insensitive sAHP, whereas P-type channels are alsoinvolved but to a lesser degree. A significant observation isthat the extent of the inhibition by cono-GVIA was similar evenif it was applied (in cumulative experiments) after either nifedipinealone (55.0 ± 7.7%, n = 4) or nifedipine and Aga-IVA together(59.0 ± 3.9%, n = 3). Therefore, the intracellular calcium originatingthrough N-type channels that activated the sAHP could not be substitutedwith that entering through L- or P-type channels. It should bementioned also that a small portion of the sAHP was resistantto all antagonists assayed, but the origin of the calcium couldnot be determined. This resistant component, eliminated by 100µM cadmium, likely would depend on calcium entry through R-typechannels and probably not from ryanodine-sensitive calcium stores,because previous experiments in the BF have shown that cytoplasmiccalcium levels during prolonged membrane depolarization were notaltered by ryanodine (Tatsumi and Katayama, 1993).
Fig. 3. N- and P-type calcium channels are involved in the sAHP. A, An AHP evoked by a 400 msec train of 18 depolarizations (1 mseceach in duration) was greatly reduced (measured at arrow indicatingthe peak amplitude) by the application of 300 nM cono-GVIA. B,In another cell the application of Aga-IVA (100 nM) produced areduction of 20% of the sAHP. C, The T-type calcium current blockeramiloride (300 µM) did not affect the sAHP. D, Histogram summarizingthe percentage of reduction of the sAHP measured at the peak forseparate drug applications. Spike height was truncated in A-C.
[View Larger Version of this Image (23K GIF file)]

Calcium currents and the mAHP either after bursts of APs or after single APs
The respective contribution of LVA and HVA calcium currents in activating the apamin-sensitive mAHP after a burst of APs (Khatebet al., 1995) was assessed also. Bursts (two to three APs) wereelicited by depolarizing current steps from a hyperpolarized levelof membrane potential ( $-$ 80 mV). As shown in Figure 4A, the N-typecurrent again plays a major role in activating the mAHP, becausethe application of 300 nM cono-GVIA reduced it drastically. Asummary of the results obtained with separate applications ofthe various antagonists is shown in Figure 4B. Cono-GVIA (200-400nM) was the dominant blocker, inhibiting 58.7 ± 15.7% of the mAHP,nifedipine (3 µM) inhibited 24.1 ± 5.8% of this AHP, and Aga-IVA(100 nM) blocked 10.0 ± 3.8% of it, whereas Aga-IVA at 300-500nM (added after 100 nM Aga-IVA) blocked only 7.4 ± 3.7% of themAHP. Comparable inhibitory effects on the mAHP were observedduring cumulative application of the HVA antagonists. Indeed,nifedipine (3 µM) reduced the mAHP by 20.2 ± 6.9% (n = 5); addingcono-GVIA (200-400 nM) reduced it by 48.4 ± 6.9% (n = 5), whereasfurther addition of Aga-IVA (100 nM) produced no further inhibition.
Fig. 4. N- and T-type calcium channels are involved in the mAHP. A, An mAHP (peak amplitude indicated by arrow) was elicited by aburst of three APs from a membrane potential of $-$ 80 mV. Applicationof 300 nM cono-GVIA reduced the AHP by ~64%. Note in inset thatthe mAHP was elicited by the same number of APs in control andin the presence of the antagonist cono-GVIA. B, Summary of resultsobtained for separate applications of calcium channel antagonists(cono-GVIA, 200-400 nM; nifedipine, 3 µM). C, D, Amiloride (300µM) reduced the amplitude of the mAHP after a burst but also reducedthe number of APs in the burst to a single AP. E, In mAHP activatedby a single AP (1 msec depolarizing pulse from a potential of $-$ 60 mV), 300 µM amiloride blocked both the DAP (open arrowhead)and a portion of the AHP (arrow), 3 µM nifedipine had no effect(data not shown), and 400 nM cono-GVIA (added with both amilorideand nifedipine) blocked the remaining mAHP (cadmium did not reducethe AHP further). F, Summary of experiments on mAHP elicited aftera single AP. Both amiloride and cono-GVIA significantly reducedthe mAHP, whereas 3 µM nifedipine (added after amiloride) hadno effect on the mAHP.
[View Larger Version of this Image (29K GIF file)]

Amiloride was used next in an attempt to assess the role of T-type channels in the burst-evoked mAHP (Matthews and Lee, 1991;Gorelova and Reiner, 1996). However, because it completely blockedburst firing (Fig. 4C,D) and converted it into tonic firing, amiloridecould not be used for this purpose. Therefore, the effects ofamiloride, and hence the implication of T-type channels, wereinvestigated in the mAHP evoked by one AP. Single APs were elicitedfrom a membrane potential of $-$ 60 mV with 1-msec-long depolarizingcurrent steps. Figure 4E shows in control conditions an AP followedby a depolarizing afterpotential (DAP, open arrowhead) and a consecutivemAHP (arrow), which is reduced by approximately one-half in thepresence of 300 µM amiloride. In addition, it is noteworthy thatamiloride (n = 6) or cadmium (n = 2) completely blocked the DAP,indicating that this depolarization is linked to the activationof a T-type current. Cumulative application of 400 nM cono-GVIAabolished the remaining mAHP (Fig. 4E). Altogether (Fig. 4F),300 µM amiloride reduced the mAHP by 34.1 ± 9.9% and 3 µM nifedipinehad no effect, whereas cono-GVIA inhibited 65.9 ± 9.9% of theremaining AHP. Because no effect of nifedipine was found afteramiloride application, the effect of nifedipine on the mAHP aftera burst (Fig. 3B) thus seems to result from a nonspecific blockingeffect of nifedipine on T-type channels. Taken together, thesedata indicate that calcium entering through N- and T-type channelsis mainly responsible for activating the apamin-sensitive mAHP.

DISCUSSION
The major goal of the present study was to examine the relative contribution of the different calcium current types to thegenesis of AHPs in cholinergic NB neurons. After the demonstrationthat these cells possess at least five types of pharmacologicallydistinguishable HVA currents as well as an amiloride-sensitiveT-type current, we demonstrated that the dominant current contributingto their AHPs is the N-type current although, depending on theirdifferent firing patterns (and different associated AHPs), eitherP- or T-type currents could be involved also.

Identification of neurons
Within the NB, cholinergic and GABAergic neurons have been shown to coexist and together comprise the majority of the largeneurons (Gritti et al., 1993). It is shown here that dissociatedNB neurons also can be classified into two groups on the basisof the size of their soma. Indeed, neurons >25 µM were mostlycholinergic (~80%), whereas those that were <25 µM comprised bothChAT-positive and ChAT-negative neurons. These results indicatethat, in this preparation, a criterion of size represents a reasonablemethod to distinguish cholinergic from noncholinergic neurons,as was proposed initially by Nakajima et al. (1985). The electrophysiologicalproperties of the larger neurons in this study confirmed thiscontention, because they corresponded closely to those of immunohistochemicallyidentified cholinergic NB neurons in basal forebrain slices (Khatebet al., 1992; Alonso et al., 1994, 1996). Indeed, in whole-cellcurrent-clamp recordings, almost all neurons of >25 µM in diameterdisplayed LTS activity, permitting them to discharge in burstsof two to three spikes when they were stimulated from a hyperpolarizedmembrane potential.

NB cholinergic neurons possess at least five types of HVA calcium channels
It has been demonstrated for a wide variety of cell types that the whole-cell HVA calcium current can be separated into severalsubtypes by using different calcium channel antagonists (Mintzet al., 1992; Randall and Tsien, 1995; McDonough et al., 1996).In cholinergic NB neurons the total HVA current was composed of~17% L-type, 35% N-type, 10% P-type, 20% Q-type, and 18% R-type.Although both L- and N-type currents were characterized beforein cholinergic basal forebrain neurons (Allen et al., 1993), P-,Q-, and R-types had not been described before. The demonstrationof the presence of both P- and Q-type currents in these neuronsrelies on the observation that low and high concentrations ofAga-IVA block distinct channels (Sather et al., 1993; Randalland Tsien, 1995; Ciranna et al., 1996). Although an importantnumber of studies has revealed that 100 nM Aga-IVA is saturatingfor the P-type channels in many preparations (Mintz et al., 1992;Mintz and Bean, 1993), more recent studies have shown that thesechannels actually could be blocked by low concentrations of Aga-IVA(IC₅₀ of 1-2 nM; Randall and Tsien, 1995; Ciranna et al., 1996).These latter studies have shown, in addition, that other channels,presumably Q-type channels, could be inhibited (IC₅₀ of ~90-200nM) with higher concentrations of Aga-IVA. Another indicationfor the distinction between a P- and a Q-type current is basedon the different time to peak of the components sensitive to lowand high Aga-IVA concentrations. Indeed, similar to other studiesthat have indicated a faster time to peak for P-type than forQ-type currents (Mintz et al., 1992; Sather et al., 1993; Randalland Tsien, 1995), the present study revealed a faster time topeak of the component sensitive to a lower concentration of Aga-IVA.In addition, we observed a component that was resistant to allHVA antagonists as well as to amiloride but that was blocked bycadmium. This calcium current peaked at 0 mV, a value more positivethan that of the R-type current in cerebellar neurons (Randalland Tsien, 1995) and that of the current flowing through $alpha$ 1E subunitsexpressed in oocytes (Ellinor et al., 1993). Notwithstanding thisdiscrepancy, the usual terminology of R-type current was usedfor the resistant component of the HVA current in cholinergicNB neurons.

Finally, it is worth mentioning that activation and deactivation kinetics of HVA calcium currents may lead to different contributionsof calcium current subtypes during a 40 msec voltage step andduring a brief AP. This issue has been addressed previously insympathetic neurons (Toth and Miller, 1995). In that preparation,APs are long-lasting, having a half-width of ~10 msec, makingAP waveforms a possible tool to voltage-clamp currents. However,APs of cholinergic NB neurons are relatively short (<2 msec athalf-width), making a similar strategy more difficult to use forquantitative assessment of currents in these cells.

Differential contributions of calcium channels to AHPs
In cholinergic NB neurons the N-type current was the one principally involved in the sAHP. Indeed, although only 35% of thetotal HVA current consisted of calcium flowing through N-typechannels, ~60% of this AHP was blocked by cono-GVIA, the selectiveN-type channel blocker. Similarly, although only ~10% of the calciumcurrent was considered to be of the P-type, ~20% of the sAHP wasactivated by calcium flowing through P-type channels. In contrast,current types L and Q contributed little to the sAHP. Also noteworthywas the lack of effect of amiloride on the sAHP. During the mAHP(elicited by one or a burst of APs) the N-type current was againdominant, but the P-type current played a minor role. On the otherhand, contrary to the sAHP, the T-type current was also importantin the activation of the mAHP. To our knowledge this representsthe first demonstration that a LVA calcium current is involvedin the genesis of the mAHP. The fact that the T-type current participatesin the activation of AHPs provides an important mechanism thatwould favor the deinactivation of the LVA current and thus promoteregenerative oscillatory events. The L-type channel blocker nifedipinealso produced a significant reduction of the mAHP elicited bya burst. However, this reduction may be partly attributable toa direct block of the LVA current by nifedipine (Allen et al.,1993; present study) because the addition of nifedipine afterthat of amiloride did not have a significant effect on the mAHP.Dihydropyridines such as nifedipine and nimodipine have been shownpreviously in a variety of cell types (including basal forebraincholinergic neurons) to have nonspecific effects on T-type channelsin addition to their well known antagonization of L-type channels(Akaike, 1991; Allen et al., 1993).

In cholinergic NB neurons the mAHP is mediated by small-conductance apamin-sensitive K_Ca channels, whereas the sAHP is mediatedby the recently described small-conductance apamin-resistant K_Cachannels (Lancaster et al., 1991; Kohler et al., 1996; Sah, 1996).We therefore speculate that apamin-sensitive K_Ca channels preferentiallyinteract with N- and T-type calcium channels, whereas apamin-resistantK_Ca channels interact with N-type and, to a lesser extent, P-typechannels. This preferential interaction may be the result of aspecial colocalization between potassium and calcium channel subtypesand/or characteristics proper to the calcium channels themselves(including in particular their activation and inactivation kinetics).In addition, the kinetics of calcium diffusion and reuptake inthe cell might play a role in this preferential interaction. Thereis earlier evidence in the literature for preferential colocalizationbetween voltage-activated calcium channels and K_Ca channels. Atthe motoneuron terminal N-type channels are located spatiallyclose to large-conductance K_Ca channels (Robitaille et al., 1993).In ciliary ganglion cells L-type, but not N-type, channels specificallycan activate large-conductance K_Ca (Wisgirda and Dryer, 1994).In other cell types N-type channels can activate apamin-sensitiveK_Ca channels, generating the AHP after a single spike (Viana etal., 1993; Umemiya and Berger, 1994; Gorelova and Reiner, 1996).Finally, in vagal neurons (Sah, 1995) L- and N-type calcium currentshave been shown to contribute to the apamin-sensitive mAHP, butnot to the large-conductance charybdotoxin-sensitive AHP. However,to our knowledge a detailed analysis of the precise contributionof all the different calcium channel subtypes to both mAHP andsAHP in the same type of neurons has not been attempted before.

Physiological significance
Although the exact role of this preferential interaction between voltage-gated calcium channel subtypes and K_Ca channels isunknown, this phenomenon may allow neurons to optimize the inhibitorymechanism induced by the AHP. In cholinergic NB neurons one couldspeculate that during tonic slow single-spike firing and shortrhythmic bursting, calcium entering through T- and N-type channelswould play a pivotal role in the activation of the apamin-sensitiveAHP, thereby contributing to regenerative membrane oscillations.However, during prolonged activations an additional (apamin-insensitive)K_Ca current could be recruited that would be activated essentiallythrough N- and P-type channels.

Finally, it is of interest to note that, the delayed AHPs in cholinergic neurons being calcium-dependent, the rhythmicitythat these cells can adopt (in conjunction with the LTS) differsfrom that of thalamic relay cells (Jahnsen and Llinás, 1984;Steriade and Llinás, 1988; McCormick, 1992), which rather dependson a cesium-sensitive I_h (McCormick and Pape, 1990a). Accordingly,in these two neuronal systems implicated in the control of behavioralstates, the modulation by afferents ascending from pontomesencephalicneurons also differs. Indeed, whereas the I_h is an important siteof action of brainstem transmitters on thalamic cells (McCormickand Pape, 1990b; McCormick, 1992), it is the calcium-dependentAHP (by an effect on calcium currents) that often is targetedin NB cholinergic neurons (A. Khateb, unpublished data; Williamset al., 1997).

FOOTNOTES

Received Jan. 21, 1997; revised July 18, 1997; accepted July 22, 1997.

This work was supported by grants from the Swiss Fonds National to L.B. and M.M. S.W. was supported by a postdoctoral fellowshipfrom the Medical Research Council of Canada. We thank Dr. NicholasSaccomano of Pfizer Central Research Laboratories for the generousgift of $omega$ -Agatoxin-IVA, Danièle Machard for her technical assistance,Gilbert von Kaenel for his help with graphics, and Drs. DouglasFraser and Dennis Churchill for critical reading of an earlierversion of this manuscript.

Correspondence should be addressed to Dr. M. Mühlethaler, Département de Physiologie, Centre Médical Universitaire, 1 RueMichel-Servet, 1211 Genève 4, Switzerland.

REFERENCES

Akaike N (1991) T-type calcium channel in mammalian CNS neurones. Comp Biochem Physiol [C] 98:31-40.
Allen TG, Sim JA, Brown DA (1993) The whole-cell calcium current in acutely dissociated magnocellular cholinergic basal forebrain neurones of the rat. J Physiol (Lond) 460:91-116[Abstract/Free Full Text].
Alonso A, Faure MP, Beaudet A (1994) Neurotensin promotes oscillatory bursting behavior and is internalized in basal forebrain cholinergic neurons. J Neurosci 14:5778-5792[Abstract].
Alonso A, Khateb A, Fort P, Jones BE, Mühlethaler M (1996) Differential oscillatory properties of cholinergic and non-cholinergic nucleus basalis neurons in guinea pig brain slice. Eur J Neurosci 8:169-182[Web of Science][Medline].
Bertrand D, Buisson B, Krause RM, Bertrand S (1997) Electrophysiology: a method to investigate the functional properties of ligand-gated channels. J Recept Signal Transduct Res 17:227-242[Web of Science][Medline].
Ciranna L, Feltz P, Schlichter R (1996) Selective inhibition of high-voltage-activated L-type and Q-type Ca²⁺ currents by serotonin in rat melanotrophs. J Physiol (Lond) 490:595-609[Abstract/Free Full Text].
Ellinor PT, Zhang J-F, Randall AD, Zhou M, Schwartz TL, Tsien RW, Horne WA (1993) Functional expression of a rapidly inactivating neuronal calcium channel. Nature 363:455-458[Medline].
Gorelova N, Reiner PB (1996) Role of the afterhyperpolarization in control of discharge properties of septal cholinergic neurons in vitro. J Neurophysiol 75:695-706[Abstract/Free Full Text].
Griffith WH, Taylor L, Davis MJ (1994) Whole-cell and single-channel currents in guinea-pig basal forebrain neurons. J Neurophysiol 71:2359-2376[Abstract/Free Full Text].
Gritti I, Mainville L, Jones BE (1993) Codistribution of GABA- with acetylcholine-synthesizing neurons in the basal forebrain of the rat. J Comp Neurol 329:438-457[Web of Science][Medline].
Hamill OP, Marty A, Neher E, Sakmann B, Sigworth FJ (1981) Improved patch-clamp techniques for high-resolution current recording from cells and cell-free membrane patches. Pflügers Arch 391:85-100[Web of Science][Medline].
Jahnsen H, Llinás R (1984) Ionic basis for the electroresponsiveness and oscillatory properties of guinea-pig thalamic neurones in vitro. J Physiol (Lond) 349:227-247[Abstract/Free Full Text].
Jones BE (1993) The organization of central cholinergic systems and their functional importance in sleep-waking states. Prog Brain Res 98:61-67[Web of Science][Medline].
Jones BE (1994) Reticular formation. Cytoarchitecture, transmitters and projections. In: The nervous system of the rat (Paxinos G, ed), pp 155-171. New South Wales, Australia: Academic.
Kay AR, Wong RKS (1986) Isolation of neurons suitable for patch-clamping from adult mammalian central nervous systems. J Neurosci Methods 16:227-238[Web of Science][Medline].
Khateb A, Mühlethaler M, Alonso A, Serafin M, Jones BE (1992) Cholinergic nucleus basalis neurons display the capacity for rhythmic bursting activity mediated by low-threshold calcium spikes. Neuroscience 51:489-494[Web of Science][Medline].
Khateb A, Fort P, Alonso A, Jones BE, Mühlethaler M (1993) Pharmacological and immunohistochemical evidence for serotonergic modulation of cholinergic nucleus basalis neurons. Eur J Neurosci 5:541-547[Web of Science][Medline].
Khateb A, Fort P, Serafin M, Jones BE, Mühlethaler M (1995) Rhythmical bursts induced by NMDA in guinea-pig cholinergic nucleus basalis neurones in vitro. J Physiol (Lond) 487:623-638[Abstract/Free Full Text].
Kohler M, Hirschberg B, Bond CT, Kinzie JM, Marrion NV, Maylie J, Adelman JP (1996) Small-conductance, calcium-activated potassium channels from mammalian brain. Science 273:1709-1714[Abstract/Free Full Text].
Lancaster B, Nicoll RA, Perkel DJ (1991) Calcium activates two types of potassium channels in rat hippocampal neurons in culture. J Neurosci 11:23-30[Abstract].
Markram H, Segal M (1990) Electrophysiological characteristics of cholinergic and non-cholinergic neurons in the rat medial septum-diagonal band complex. Brain Res 513:171-174[Web of Science][Medline].
Matthews RT, Lee WL (1991) A comparison of extracellular and intracellular recordings from medial septum/diagonal band neurons in vitro. Neuroscience 42:451-462[Web of Science][Medline].
McCormick DA (1992) Neurotransmitter actions in the thalamus and cerebral cortex and their role in neuromodulation of thalamocortical activity. Prog Neurobiol 39:337-388[Web of Science][Medline].
McCormick DA, Pape H-C (1990a) Properties of a hyperpolarization-activated cation current and its role in rhythmic oscillations in thalamic relay neurones. J Physiol (Lond) 431:291-318[Abstract/Free Full Text].
McCormick DA, Pape H-C (1990b) Noradrenergic and serotonergic modulation of a hyperpolarization-activated cation current in thalamic relay neurones. J Physiol (Lond) 431:319-342[Abstract/Free Full Text].
McDonough SI, Swartz KJ, Mintz IM, Boland L, Bean BP (1996) Inhibition of calcium channels in rat central and peripheral neurons by $omega$ -conotoxin MVIIC. J Neurosci 16:2612-2623[Abstract/Free Full Text].
Mesulam MM (1995) Structure and function of cholinergic pathways in the cerebral cortex, limbic system, basal ganglia, and thalamus of the human brain. In: Psychopharmacology: the fourth generation of progress (Bloom FE, Kupfer DJ, eds), pp 135-146. New York: Raven.
Mintz M, Bean BP (1993) GABA_B receptor inhibition of P-type Ca²⁺ channels in central neurons. Neuron 10:889-898[Web of Science][Medline].
Mintz M, Adams ME, Bean BP (1992) P-type calcium channels in rat central and peripheral neurons. Neuron 9:85-95[Web of Science][Medline].
Murchison D, Griffith WH (1996) High-voltage-activated calcium currents in basal forebrain neurons during aging. J Neurophysiol 76:158-174[Abstract/Free Full Text].
Nakajima Y, Nakajima S, Obata K, Carlson GC, Yamaguchi K (1985) Dissociated cell culture of cholinergic neurons from nucleus basalis of Meynert and other basal forebrain nuclei. Proc Natl Acad Sci USA 82:6325-6329[Abstract/Free Full Text].
Nuñez A (1996) Unit activity of rat basal forebrain neurons: relationship to cortical activity. Neuroscience 72:757-766[Web of Science][Medline].
Paxinos G, Watson C (1986) In: The rat brain in stereotaxic coordinates. Sydney: Academic.
Penington NJ, Kelly JS (1993) Ionic dependence of a slow inward tail current in rat dorsal raphe neurones. J Physiol (Lond) 464:33-48[Abstract/Free Full Text].
Randall A, Tsien RW (1995) Pharmacological dissection of multiple types of Ca²⁺ channel currents in rat cerebellar granule neurons. J Neurosci 15:2995-3012[Abstract].
Robitaille R, Garcia ML, Kaczorowski GJ, Charlton MP (1993) Functional colocalization of calcium and calcium-gated potassium channels in control of transmitter release. Neuron 11:645-655[Web of Science][Medline].
Sah P (1995) Different calcium channels are coupled to potassium channels with distinct physiological roles in vagal neurons. Proc R Soc Lond [Biol] 260:105-111[Medline].
Sah P (1996) Ca²⁺-activated K⁺ currents in neurones: types, physiological roles, and modulation. Trends Neurosci 19:150-154[Web of Science][Medline].
Sather WA, Tanabe T, Zhang J-F, Mori Y, Adams ME, Tsien RW (1993) Distinctive biophysical and pharmacological properties of Class A (B1) calcium channels $alpha$ 1 subunits. Neuron 11:291-303[Web of Science][Medline].
Stea A, Tomlinson WJ, Soong TW, Bourinet E, Dubel SJ, Vincent SR, Snutch TP (1994) The localization and functional properties of a rat brain $alpha$ 1A calcium channel reflect similarities to neuronal Q- and P-type channels. Proc Natl Acad Sci USA 91:10576-10580[Abstract/Free Full Text].
Steriade M, Llinás RR (1988) The functional states of the thalamus and the associated neuronal interplay. Physiol Rev 68:649-742[Free Full Text].
Tang C-M, Presser F, Morad M (1988) Amiloride selectively blocks the low-threshold (T) calcium channel. Science 240:213-215[Abstract/Free Full Text].
Tatsumi H, Katayama Y (1993) Regulation of the intracellular free calcium concentration in acutely dissociated neurones from rat nucleus basalis. J Physiol (Lond) 464:165-181[Abstract/Free Full Text].
Tatsumi H, Katayama Y (1995) Na⁺-dependent Ca²⁺ influx induced by depolarization in neurons dissociated from rat nucleus basalis. Neurosci Lett 196:9-12[Web of Science][Medline].
Toth TP, Miller RJ (1995) Calcium and sodium currents evoked by action potential waveform in rat sympathetic neurones. J Physiol (Lond) 485:43-57[Abstract/Free Full Text].
Umemiya M, Berger AJ (1994) Properties and function of low- and high-voltage-activated Ca²⁺ channels in hypoglossal motoneurons. J Neurosci 14:5652-5660[Abstract].
Viana F, Bayliss DA, Berger AJ (1993) The role of multiple potassium conductances in action potential repolarization and repetitive firing behavior of neonatal rat hypoglossal motoneurons. J Neurophysiol 69:2150-2163[Abstract/Free Full Text].
Williams S, Serafin M, Mühlethaler M, Bernheim L (1997) Facilitation of N-type calcium current is dependent on the frequency of action potential-like depolarizations in dissociated cholinergic basal forebrain neurons of the guinea pig. J Neurosci 17:1625-1632[Abstract/Free Full Text].
Wisgirda ME, Dryer SE (1994) Functional dependence of Ca²⁺-activated K⁺ current on L- and N-type Ca²⁺ channels: differences between chicken sympathetic and parasympathetic neurons suggest different regulatory mechanisms. Proc Natl Acad Sci USA 91:2858-2862[Abstract/Free Full Text].
Zhang L, Weiner JL, Valiente TA, Velumian AA, Watson PL, Jahromi SS, Schertzer S, Pennefather P, Carlen P (1994) Whole-cell recording of the Ca²⁺-dependent slow afterhyperpolarization in hippocampal neurones: effects of internally applied anions. Pflügers Arch 426:247-253[Web of Science][Medline].

Copyright ©1997 Society for Neuroscience   0270-6474/1997/177307-09$05.00/0

This article has been cited by other articles:

D. Murchison, A. N. McDermott, C. L. LaSarge, K. A. Peebles, J. L. Bizon, and W. H. Griffith
Enhanced Calcium Buffering in F344 Rat Cholinergic Basal Forebrain Neurons Is Associated With Age-Related Cognitive Impairment
J Neurophysiol, October 1, 2009; 102(4): 2194 - 2207.
[Abstract] [Full Text] [PDF]

S. A. Prescott and T. J. Sejnowski
Spike-Rate Coding and Spike-Time Coding Are Affected Oppositely by Different Adaptation Mechanisms
J. Neurosci., December 10, 2008; 28(50): 13649 - 13661.
[Abstract] [Full Text] [PDF]

X. Li and D. J. Bennett
Apamin-Sensitive Calcium-Activated Potassium Currents (SK) Are Activated by Persistent Calcium Currents in Rat Motoneurons
J Neurophysiol, May 1, 2007; 97(5): 3314 - 3330.
[Abstract] [Full Text] [PDF]

Y. Yaari, C. Yue, and H. Su
Recruitment of apical dendritic T-type Ca2+ channels by backpropagating spikes underlies de novo intrinsic bursting in hippocampal epileptogenesis
J. Physiol., April 15, 2007; 580(2): 435 - 450.
[Abstract] [Full Text] [PDF]

M. Kato, N. Tanaka, S. Usui, and Y. Sakuma
The SK channel blocker apamin inhibits slow afterhyperpolarization currents in rat gonadotropin-releasing hormone neurones
J. Physiol., July 15, 2006; 574(2): 431 - 442.
[Abstract] [Full Text] [PDF]

J. A. Goldberg and C. J. Wilson
Control of Spontaneous Firing Patterns by the Selective Coupling of Calcium Currents to Calcium-Activated Potassium Currents in Striatal Cholinergic Interneurons
J. Neurosci., November 2, 2005; 25(44): 10230 - 10238.
[Abstract] [Full Text] [PDF]

M. Russier, E. Carlier, N. Ankri, L. Fronzaroli, and D. Debanne
A-, T-, and H-type Currents Shape Intrinsic Firing of Developing Rat Abducens Motoneurons
J. Physiol., May 15, 2003; 549(1): 21 - 36.
[Abstract] [Full Text] [PDF]

R. K. Cloues and W. A. Sather
Afterhyperpolarization Regulates Firing Rate in Neurons of the Suprachiasmatic Nucleus
J. Neurosci., March 1, 2003; 23(5): 1593 - 1604.
[Abstract] [Full Text] [PDF]

E. Perez-Reyes
Molecular Physiology of Low-Voltage-Activated T-type Calcium Channels
Physiol Rev, January 1, 2003; 83(1): 117 - 161.
[Abstract] [Full Text] [PDF]

M. R. Smith, A. B. Nelson, and S. du Lac
Regulation of Firing Response Gain by Calcium-Dependent Mechanisms in Vestibular Nucleus Neurons
J Neurophysiol, April 1, 2002; 87(4): 2031 - 2042.
[Abstract] [Full Text] [PDF]

P. Cavelier, F. Pouille, T. Desplantez, H. Beekenkamp, and J.-L. Bossu
Control of the propagation of dendritic low-threshold Ca2+ spikes in Purkinje cells from rat cerebellar slice cultures
J. Physiol., April 1, 2002; 540(1): 57 - 72.
[Abstract] [Full Text] [PDF]

J. Martinez-Pinna, P. J. Davies, and E. M. McLachlan
Diversity of Channels Involved in Ca2+ Activation of K+ Channels During the Prolonged AHP in Guinea-Pig Sympathetic Neurons
J Neurophysiol, September 1, 2000; 84(3): 1346 - 1354.
[Abstract] [Full Text] [PDF]

M. Shah and D. G. Haylett
Ca2+ Channels Involved in the Generation of the Slow Afterhyperpolarization in Cultured Rat Hippocampal Pyramidal Neurons
J Neurophysiol, May 1, 2000; 83(5): 2554 - 2561.
[Abstract] [Full Text] [PDF]

T G J Allen
The role of N-, Q- and R-type Ca2+ channels in feedback inhibition of ACh release from rat basal forebrain neurones
J. Physiol., February 15, 1999; 515(1): 93 - 107.
[Abstract] [Full Text] [PDF]

M. Tanabe, B. H. Gahwiler, and U. Gerber
L-Type Ca2+ Channels Mediate the Slow Ca2+-Dependent Afterhyperpolarization Current in Rat CA3 Pyramidal Cells In Vitro
J Neurophysiol, November 1, 1998; 80(5): 2268 - 2273.
[Abstract] [Full Text] [PDF]

J. C. Pineda, R. S. Waters, and R. C. Foehring
Specificity in the Interaction of HVA Ca2+ Channel Types With Ca2+-Dependent AHPs and Firing Behavior in Neocortical Pyramidal Neurons
J Neurophysiol, May 1, 1998; 79(5): 2522 - 2534.
[Abstract] [Full Text] [PDF]

P. Cavelier, F. Pouille, T. Desplantez, H. Beekenkamp, and J.-L. Bossu
Control of the propagation of dendritic low-threshold Ca2+ spikes in Purkinje cells from rat cerebellar slice cultures
J. Physiol., April 1, 2002; 540(1): 57 - 72.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (29)

Citing Articles via Google Scholar

Google Scholar

Articles by Williams, S.

Articles by Bernheim, L.

Search for Related Content

PubMed

PubMed Citation

Articles by Williams, S.

Articles by Bernheim, L.