Muscarinic Receptor Activity Induces an Afterdepolarization in a Subpopulation of Hippocampal CA1 Interneurons

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The Journal of Neuroscience, July 15, 1999, 19(14):5703-5710

Muscarinic Receptor Activity Induces an Afterdepolarization in a Subpopulation of Hippocampal CA1 Interneurons
A. Rory McQuiston and Daniel V. Madison
Department of Molecular and Cellular Physiology, Stanford University School of Medicine, Stanford, California 94305

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cholinergic input to the hippocampus may be involved in important behavioral functions and the pathophysiology of neurodegenerativediseases. Muscarinic receptor activity in interneurons of thehippocampus may play a role in these actions. In this study, weinvestigated the effects of muscarinic receptor activity on theexcitability of different subtypes of interneurons in rat hippocampalCA1. Most interneurons displayed an afterhyperpolarizing potential(AHP) after depolarization by injected current or synaptic stimulation.In the presence of a muscarinic agonist, the AHP of a subset ofthese interneurons was replaced by an afterdepolarization (ADP),often of sufficient magnitude to evoke action potentials in theabsence of further stimulation. The ADP was insensitive to cadmiumand low extracellular calcium. It was blocked by low extracellularsodium but not by tetrodotoxin or low concentrations of amiloride.Muscarinic ADPs were sometimes observed in isolation but wereoften accompanied by depolarizing, hyperpolarizing, or biphasicchanges in the membrane potential. Interneurons with muscarinicADPs were found in all strata of CA1 and did not fall into a singlemorphological classification. The potential functions of the prolongedaction potential output of interneurons produced by the ADP couldinclude changes in hippocampal circuit properties and facilitationof the release of peptide cotransmitters in theseinterneurons.

Key words: muscarinic receptor; acetylcholine; hippocampus; CA1; interneuron; afterdepolarization

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acetylcholine (ACh) has an important role in normal hippocampal function and has been shown to have a variety of actions onboth principal pyramidal neurons as well as interneurons. However,compared with its actions on principal cells, relatively littleis known about the detailed effects of muscarinic receptor activityon interneurons. In hippocampal pyramidal cells, muscarinic receptoractivity consistently produces a depolarization of the membranepotential and a blockade of a calcium-activated potassium conductancewith a concomitant decrease in spike frequency accommodation (Benardoand Prince, 1982; Cole and Nicoll, 1983). It also generates afterdepolarizationsor plateau potentials (Benardo and Prince, 1982; Frazer and MacVicar,1996). Although some of the complex effects of muscarinic activityon interneuronal membrane potential are beginning to be understood(Benardo and Prince, 1982; Reece and Schwartzkroin, 1991; McQuistonand Madison, 1996; Parra et al., 1998), little is known aboutthe effect of muscarinic receptor activity on the firing propertiesof interneurons in thehippocampus.

Hippocampal interneurons show a high degree of diversity in dendritic arborization, axonal termination regions, and probablefunction (for review, see Freund and Buzsaki, 1996). Evidenceis beginning to accumulate that there is also a diversity of responsivenessto afferent neurotransmitters across hippocampal interneuronalpopulations (cf. Parra et al., 1998) that, at least in some cases,correlates with interneuronal morphology [accompanying article(McQuiston and Madison, 1999)]. Here, we investigate the effectsof muscarinic receptor activity on the excitability of interneuronsin all layers of rat hippocampal CA1. Effects of muscarinic agonistswere tested across many different types of interneurons and assessedfor correlation with their anatomical structures. We show thata subset of interneurons generate an afterdepolarizing potential(ADP) when stimulated in the presence of a muscarinic agonistand that this effect is distributed across a wide range of interneuronalmorphologies.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Young male rats (16- to 54-d-old) were anesthetized with halothane and killed by decapitation. Brains were rapidly removedand placed in cold (4°C) oxygenated saline [(in mM): NaCl 119,KCl 2.5, CaCl₂ 1.0, MgCl₂ 3, NaHPO₄ 1, NaHCO₃ 26.2, glucose 11,and kynurenic acid 1, pH 7.4]. Brains were hemisected; coronalslices (300- to 400-µm-thick) were cut on a Vibratome (Ted PellaInc., St. Louis, MO) and submerged in an incubation chamber (30°C,30 min). Slices were then cooled to room temperature (~23°C) andrecorded from over the next 2-4hr.

Whole-cell patch-clamp recordings were made from visualized interneurons in all layers of area CA1 (MacVicar, 1984; Dodt andZieglgansberger, 1990). Slices, on cover glass, were placed ina recording chamber mounted on the stage of a modified Nikon Optiphot2 microscope (Technical Instruments, San Francisco, CA) and superfusedwith oxygenated saline [(in mM): NaCl 119, KCl 2.5, CaCl₂ 2.5,MgSO₄ 1.3, NaHPO₄ 1, NaHCO₃ 26.2, and glucose 11, pH 7.4; 22-24°C].Neurons were visualized using near-infrared light (40× magnification).Images were collected by a Hamamatsu C2400 intensified CCD camera(Hamamatsu Corporation, Bridgewater, NJ) with contrast enhancement.The images were displayed on a video monitor, and glass patchpipettes were visually advanced through the slice to the surfaceof the cell from which to berecorded.

Patch pipettes were fabricated from borosilicate glass (KG33; 1.5 mm outer diameter, 1.0 mm inner diamter; Garner Glass Co.,Claremont, CA) and filled with a HEPES-gluconate or methylsulfatebuffer [(in mM): K gluconate or K methlysulfate 130, NaCl 8, HEPES10, MgATP 2, Na₃GTP 0.3, and BAPTAK₄ 0.1, pH 7.25]. When neurobiotin(0.5%) was included in the internal solution to label cells, Kgluconate-methylsulfate was reduced to 120 mM to maintain osmolarity.Methylsulfate was preferred because, anecdotically, we felt thatthere was less rundown of ADPs when methylsulfate was used insteadof gluconate. This is consistent with previous findings that methylsulfatebetter preserves the firing patterns of an individual neuron duringwhole-cell recording (Velumian et al., 1997).

Membrane potentials were monitored with an Axoclamp 2A amplifier (Axon Instruments, Foster City, CA), acquired through anMIO-16-E2 analog-to-digital interface (National Instruments, Austin,TX) onto a Pentium personal computer using software written inLabview (National Instruments) by members of our laboratory (Stanford,CA) (Eric Schaible and Paul Pavlidis). Data were analyzed usingprograms written in Labview and Axum (Mathsoft Inc., Cambridge,MA). ADPs were quantified by calculating the area under the ADP.Area was calculated by summing the amplitudes of all individualdata samples over time, relative to the baseline of prestimulusmembrane potential. Samples were summed from the end of the evokingdepolarizing pulse to the point at which the membrane potentialreturned to the prestimulus level (indicated by a dashed linein the figures). Thus, an ADP had a positive value for area, whereasan afterhyperpolarizing potential (AHP) had a negative value.Statistical significance was determined by two-tailed unpairedStudent's t test for data of unequal variance. Values are reportedas mean ± SEM. Because muscarinic receptor activity often causeda change in the resting membrane potential, cells were alwaysreturned to the control resting potential by current injectedthrough the recording electrode. This ensured that ADPs were alwaysevoked from a consistent membrane potential within each cell,thus ensuring that any effect, drug, or treatment on an ADP wasnot secondary to a change in membranepotential.

All drugs were applied by bath superfusion. Muscarinic responses were produced by bath application of muscarine, carbachol,or ACh. Carbachol and acetylcholine were used in combination withthe nicotinic antagonists $alpha$ -bungarotoxin ( $alpha$ -BgTx) (100 nM) andmecamylamine (MEC) (10 µM) to prevent the activation of nicotinicreceptors. Antagonists were applied to the tissue and equilibratedbefore the agonist wasapplied.

Neuronal morphology was visualized using neurobiotin or biocytin (Bolam, 1992). For histology, slices were fixed overnightin buffered 4% paraformaldehyde (containing 0.05% glutaraldehydeand 0.2% picric acid), embedded in gelatin, and sectioned (100µm). Sections were permeabilized (0.5% Triton X-100), treatedwith 0.3% hydrogen peroxide to reduce background peroxidase activity,and incubated overnight in avidin-biotin-peroxidase complex (EliteVectastain ABC kit; Vector Laboratories, Burlingame, CA). Sectionswere stained with diaminobenzidine, intensified with nickel, mountedon slides, cleared, andcoverslipped.

All chemicals were purchased from Fluka (Milwaukee, WI) except for the following: (±)-muscarine, acetylcholine, $alpha$ -bungarotoxin,mecamylamine, and methyllycaconitine (Research Biochemicals, Natick,MA); tetrodotoxin (TTX) (Calbiochem, La Jolla, CA); and paraformaldehyde(Electron Microscopy Sciences, Fort Washington,PA).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We investigated the effect of muscarinic receptor activity on the firing properties of hippocampal CA1 interneurons usingwhole-cell patch clamping. We applied 600 msec depolarizing currentinjections to evoke a train of action potentials (typically 120pA).

Muscarinic receptor activity produces an afterdepolarizing potential in some CA1 interneurons

A subset of interneurons in all layers of CA1 exhibited increased excitability when treated with muscarinic agonists. Trainsof action potentials induced by injecting depolarizing currentthrough the recording electrode were generally followed by smallAHPs (Fig. 1A,B, left). In some (~15%) interneurons, muscarine(10 µM) caused the replacement of the AHP with a large and long-lastingADP. This ADP was usually sufficiently large to itself elicita prolonged burst of action potentials from an interneuron (Fig.1A,B, middle). These ADPs varied considerably in duration fromseveral hundred milliseconds (Fig. 1A) to several seconds (Fig.1B). The effects of muscarinic agonist in producing an ADP werereversible (Fig. 1A,B, right). ADPs were seen in a total of 97(of ~650) interneurons located in all layers of CA1 (Table 1).

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Figure 1. An ADP is produced in some interneurons during muscarinic receptor activity in CA1 interneurons. A, Injection of depolarizing current (600 msec, 120 pA) into an interneuron in SR evoked an accommodating train of action potentials followed by a small AHP (left). Application of muscarine (10 µM) resulted in an ADP after current injection of several hundred milliseconds duration that supported a burst of action potentials (middle). The effect of muscarine was reversible after removal of the agonist (right). B, In an SLM interneuron, depolarizing current (600 msec, 120 pA) resulted in a train of action potentials followed by a small AHP (left). Addition of muscarine (10 µM) resulted in an ADP lasting several seconds (middle). These effects of muscarine were reversible (right). C, Summary plot of ADPs in response to muscarine from 85 interneurons in CA1. Plotted are the means of the area under the afterpotentials relative to the resting membrane potential before, during, and after muscarine application. Positive values indicate an ADP; negative values indicate an AHP.


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Table 1. Distribution of interneurons displaying an ADP

The mean values for the area of the afterpotentials are plotted in Figure 1C. In 85 interneurons, muscarinic receptor activitychanged the AHP (area $-$ 102 ± 45 mV · sec) to ADP (area 395 ± 144mV · sec; p < 0.005); when the drug was removed, the sign of theafterpotential area recovered (area $-$ 16 ± 4 mV · sec; p < 0.001).

Production of an ADP by application of muscarine was prevented by previous treatment with atropine. In the example shown inFigure 2A, application of muscarine (10 µM) transformed an AHP(Fig. 2A, left) into an ADP (Fig. 2A, middle). Atropine (1 µM)prevented this transformation (Fig. 2A, right). The results ofthese experiments are summarized in the plot of afterpotentialareas shown in Figure 2B. Significant changes in afterpotentialarea were induced by muscarine (control area $-$ 47 ± 32 mV · secvs muscarine 118 ± 44 mV · sec; p < 0.05). Previous applicationof atropine (1 µM) prevented any significant changes in area (atropine $-$ 57 ± 12 mV · sec vs atropine plus muscarinic agonist $-$ 67 ± 16mV · sec; p > 0.63; n = 3).

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Figure 2. Inhibition of ADP production by atropine. A, Injection of depolarizing current into an interneuron in SR resulted in an accommodating train of action potentials followed by an AHP (left). In the presence of muscarine (10 µM), action potential accommodation was reduced and the AHP was replaced by an ADP (middle). When atropine was also present (1 µM), muscarine (10 µM) did not produce an ADP (right). B, Summary plot of the area of the afterpotential in interneurons before and during the application of muscarinic agonist, in the absence (left) and presence (right) of atropine (1-5 µM). ADPs were not observed in atropine (n = 3).

We observed that consecutive applications of muscarinic agonists did not produce ADPs of consistent magnitude. With repeatedapplication of muscarinic agonists, the area of the ADP progressivelydecreased. An example is shown in Figure 3. The first applicationof muscarine (10 µM) produced an ADP (Fig. 3A, middle) in an interneuronthat had previously responded to a depolarizing pulse with anAHP (Fig. 3A, left). After recovery from the first applicationof muscarine (Fig. 3, A, right, B, left), a second applicationof muscarine produced an ADP of smaller amplitude (Fig. 3B, middle).This reduction in amplitude was a consistent finding (Fig. 3C).The area of the ADPs from initial muscarinic applications (161± 39 mV · sec; n = 15) were significantly greater than the ADPsmeasured after subsequent muscarinic applications (47 ± 9 mV ·sec; n = 15; p < 0.02). We did not investigate the reason forthe instability of the ADPs any further. The rundown of ADPs fromone application of muscarine to the next made experiments investigatingthe ionic mechanism of the ADP difficult, because muscarine neededto be applied two or more times in different ionic conditions.To avoid this potential problem, we only analyzed those experimentsin which there was clear recovery of the ADP after an inhibitorymanipulation.

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Figure 3. Effect of repeated applications of muscarine on the size of the ADPs. A, Initial application of muscarine (10 µM) resulted in an ADP in response to an injection of depolarizing current (600 msec, 120 pA) (middle), whereas an AHP was observed in response to the same current injection in the absence of muscarine (Control, Wash). B, A second application of muscarine (10 µM) produced a smaller ADP (compare with A) in response to the same current injection (middle). C, Summary of the effects of consecutive applications of muscarinic agonists on the ADP. During a second application of muscarine, the area of the ADP is reduced (n = 15).

Calcium influx is not required for stimulating a muscarinic ADP

Previous studies on CA1 pyramidal cells (Fraser and MacVicar, 1996) and neocortical pyramidal cells (Schwindt et al., 1988;Andrade, 1991) showed that the muscarinic ADP in these cells resultedfrom activation of a calcium-activated nonselective cation currentsecondary to the influx of calcium through voltage-dependent calciumchannels (VDCCs) (Fraser and MacVicar, 1996). We tested whetherthe muscarinic ADP we observed in CA1 interneurons was causedby the activation of a similar current. Interneurons displayingmuscarinic ADPs were treated with cadmium (200 µM) to inhibitcalcium influx through VDCCs. In control conditions, an interneuronthat normally produced an AHP after a depolarizing pulse (Fig.4A, Control) produced a large ADP after activation of muscarinicreceptors [Fig. 4A, ACh (300 µM). After removal of ACh, applicationof cadmium produced a small plateau during the depolarizationpulse; this was followed by a small AHP (Fig. 4A, Cd²⁺). However, an ADP was still produced when ACh was applied subsequentlyin the continued presence of cadmium (Fig. 4A, ACh + Cd²⁺).

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Figure 4. Calcium influx is not required for an ADP to occur. A, Left to right, injection of a depolarizing current injection (600 msec, 100 pA) into an interneuron in SR resulted in a train of accommodating action potentials followed by an AHP. ACh (300 µM), in the presence of nicotinic receptor antagonists ( $alpha$ -BgTx 100 nM; MEC 10 mM) resulted in an ADP after the depolarizing current injection. Blockade of voltage-dependent calcium channels by Cd²⁺ (200 µM) produced a train of accommodating action potentials in response to an injection of depolarizing current. ACh (300 µM), in the presence of Cd²⁺ (200 µM), still promoted an ADP after the current injection. B, Left to right, Injection of depolarizing current (600 msec, 120 pA) into an interneuron in SR resulted in a train of accommodating action potentials followed by an AHP. Bath application of muscarine (10 µM) resulted in an ADP after the current injection. Low extracellular Ca²⁺ (0.1 mM Ca²⁺-4 mM Mg²⁺) reduced action potential accommodation and the AHP but did not prevent the muscarinic ADP. C, Summary of the effects of low Ca²⁺ and Cd²⁺ on the area of the ADPs. Muscarine did not block the activation of ADPs in the presence of Cd²⁺ or low extracellular Ca²⁺ in interneurons in all layers of CA1 (n = 11).

Similar results were seen with low extracellular calcium. The interneuron in Figure 4B produced an AHP after a depolarizingpulse (Control); addition of muscarine (10 µM) resulted in anADP (Fig. 4B, Muscarine). The neuron responded to low extracellularcalcium (0.1 mM Ca²⁺-4 mM Mg²⁺) with an increased firing rate and decreased amplitude of theAHP (Fig. 4B, Low Ca²⁺), but addition of muscarine still resulted in an ADP after adepolarizing pulse (Fig. 4B, +Muscarine). The survival of themuscarinic ADP in both cadmium and low calcium indicates thatcalcium influx is not required to activate theADP.

The results of the experiments with cadmium and low calcium are summarized in Figure 4C. In the absence of calcium influx,muscarinic receptor activity significantly changed the area ofthe afterpotential (before muscarine, $-$ 15 ± 8 mV · sec; aftermuscarine, 69 ± 14 mV · sec; p < 0.0001; n = 11). Although themuscarinic ADP produced in low Ca²⁺ or cadmium was somewhat smaller relative to the first applicationof muscarine (125 ± 26 mV · sec vs low Ca²⁺-cadmium 69 ± 14 mV · sec; n = 11), this reduction was not significant(p > 0.08). This decrease in the area of the ADP is likely causedby the rundown of theADP.

Sodium influx is required for ADP production

Calcium-activated currents are only one of several mechanisms that have been identified as underlying ADPs. Short durationADPs in CA1 pyramidal cells have been reported to be inhibitedby TTX and are thought to arise from the activation of a persistentvoltage-dependent sodium channel (VDSC) (Azouz et al., 1996).There is also evidence that the sodium-calcium exchanger in neocorticalpyramidal cells may be responsible for plateau potentials observedin neocortical neurons when potassium channels are inhibited (Friedmanet al., 1992). Therefore, we investigated the possibility thatthe ADP in interneurons was the result of opening of sodium channelsor of sodiumtransport.

We first examined the possibility that muscarine was promoting the appearance of ADPs by potentiating a persistent TTX-sensitiveVDSC in CA1 interneurons (Crill, 1996). TTX (5 µM) was appliedto interneurons having muscarinic ADPs to block persistent VDSCs(Fig. 5A). This was done in the presence of cadmium (500 µM) toblock any calcium activated currents as well. Because TTX inhibitedaction potential generation (Fig. 5A, TTX/Cd²⁺), we increased the current amplitude to depolarize the membranepotential to the same voltage as the peak of the action potential.Under these conditions, application of muscarine continued toproduce an ADP after the depolarizing pulse. Similar observationswere seen in seven other cells exposed to TTX (TTX $-$ 4 ± 3 mV ·sec vs muscarine plus TTX 69 ± 16 mV · sec; p < 0.003; n = 8)(Fig. 5B). In this set of experiments, the area of the ADP inthe presence of TTX was somewhat smaller than in the presenceof muscarine alone but not significantly (muscarine 146 ± 33 mV· sec vs muscarine plus TTX 69 ± 16 mV· sec; n = 8; p > 0.06).This decrease could be caused by depolarization in the absenceof action potentials being less effective in evoking an ADP orto the rundown of the ADP with repeated application of muscarine(Fig. 3). Rundown did still occur in the presence of TTX.

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Figure 5. Activation of TTX-sensitive sodium channels is not required for ADPs. A, Left to right, Injection of depolarizing current (600 msec, 120 pA) into an interneuron in SR produced a train of action potentials. Muscarine (10 µM) resulted in a large ADP that lasted for several seconds. Bath application of TTX (5 µM) and Cd²⁺ (200 µM) blocked action potentials but not the muscarine-induced ADP after depolarizing current injection, to give a depolarization equal to the action potential peak (600 msec, 410 pA). B, Summary of the effects of TTX and muscarine on the area of ADPs (n = 8).

We next examined the possibility that the muscarinic ADP was the result of the activation of a TTX-insensitive sodium channelor the sodium-calcium exchanger. In these studies, extracellularNaCl was replaced with choline chloride. In normal saline, muscarine(10 µM) induced an ADP after injection of a depolarizing current(Fig. 6A, compare Control, Muscarine). After removal of muscarinefrom the bath, replacement of extracellular NaCl with cholinechloride usually abolished action potentials (Fig. 6A, Low Sodium).The amplitude of the current injection was increased so that theamplitude of the depolarization was equivalent to the action potentialamplitude. There was a small AHP after this depolarization. Additionof muscarine (10 µM) in low sodium solution did not result inthe production of an ADP (Fig. 6A, +Muscarine). A summary of allsuch experiments is plotted in Figure 6C. The area of the afterpotentialafter a depolarizing current pulse in the presence of muscarineand low sodium was not significantly different from the area ofthe afterpotential in low sodium alone ( $-$ 14 ± 10 mV · sec vs lowsodium plus muscarine $-$ 8 ± 10 mV · sec; p > 0.63) (Fig. 6C, LowSodium). However, the muscarinic ADP in normal saline was significantlydifferent from the muscarinic afterpotential in low sodium (normalsaline 236 ± 56 mV · sec vs low sodium $-$ 8 ± 10 mV · sec; p < 0.002).We concluded, therefore, that the muscarinic ADP is dependenton extracellular sodium.

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Figure 6. Sodium influx is required for ADPs. A, Left to right, In an SR interneuron, the AHP after a current injection (600 msec, 120 pA) was transformed into an ADP after application of muscarine (10 µM). Replacement of NaCl by choline chloride blocks action potentials; however, the depolarizing current (600 msec, 520 pA) was still followed by an AHP. In low sodium, current depolarizing the cell to the same voltage as the peak of the action potential did not result in a muscarinic ADP. B, Left to right, Depolarizing current injection (600 msec, 100 pA) into an interneuron in SR resulted in an accommodating train of action potentials followed by an AHP. ACh (300 µM), in the presence of nicotinic antagonists ( $alpha$ -BgTx 100 nM; MEC 10 µM), promoted an ADP after the current injection. Amiloride (100 µM) did not significantly affect the train of action potentials in response to depolarizing current and did not block the response to ACh. C, Plot of the area of the ADP with depolarizing current. Substitution of sodium by choline blocked the ADP (n = 10).

Both sodium transport and slow sodium channels are sensitive to amiloride. We tested whether amiloride inhibited the muscarinicADP in interneurons. In interneurons in which application of muscarineor ACh (300 µM) normally produced an ADP (Fig. 6B), this afterpotentialwas not inhibited by amiloride (area 5255 mV · sec in normal salinevs 6688 mV · sec in 100 µM amiloride; n = 2) (Fig. 6B, +ACh).Figure 6C summarizes the effects of low sodium on the muscarinicADP.

Muscarinic ADPs can be elicited by synaptic potentials

All ADPs studied to this point were elicited by depolarizations induced by injection of current into the cell through therecording electrode. We next determined whether a more physiologicalsignal could induce a muscarinic ADP. Excitatory afferents ontointerneurons were stimulated with an electrode placed in stratumoriens (SO), resulting in EPSPs that evoked a short burst of actionpotentials (Fig. 7, Control). After activation of muscarinic receptors,the EPSP was inhibited (data not shown). When the stimulus wasincreased to bring the amplitude of the EPSP back up to controllevels, an ADP was produced. ADPs evoked by synaptic stimulationwere of sufficient amplitude and duration to support long barragesof action potentials in the absence of any further stimulation(n = 3) (Fig. 7, middle).

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Figure 7. Muscarinic receptor activity produces ADPs after stimulus-evoked excitatory postsynaptic potentials. Suprathreshold synaptic stimulation (arrows; 100 µsec duration, 200 µA amplitude) via a tungsten bipolar stimulating electrode placed in SO evoked an EPSP and a burst of action potentials (left). Synaptic stimulation in the presence of muscarine (10 µM) produced a long-lasting (several seconds) burst of action potentials (ADP) after the EPSP (n = 3). Removal of muscarine eliminated the ADP response.

Distribution of interneurons expressing a muscarinic ADP

Muscarinic ADPs were observed in subsets of interneurons in all layers of CA1 (Table 1). The majority of cells demonstratingmuscarinic ADPs were recorded in stratum radiatum (SR), althoughinterneurons displaying ADPs were found in all layers of areaCA1.

Muscarinic receptor activity is known to cause changes in the resting potentials in most CA1 interneurons (McQuiston and Madison,1996; Parra et al., 1998). These can include depolarization, hyperpolarization,or biphasic responses (depolarization followed by a hyperpolarization).Interneurons having ADPs are no different in this regard, oftenshowing changes in resting membrane potential in response to muscarinicreceptor activity. There was no clearly dominant membrane potentialresponse that accompanied ADPs: 34% of ADP-producing cells alsodepolarized, 26% hyperpolarized, 14% had an initial hyperpolarizationfollowed by a slower depolarization (biphasic), and 26% showedan ADP with no effect on the resting membrane potential. Thisis similar to the distribution of membrane potential changes seenwith muscarinic receptor activity in the entire population ofCA1 interneurons (i.e., those with and without ADPs) (McQuistonand Madison, 1999).

Although the location of the neuronal cell body sometimes provides information on potential interneuron anatomical subtypes,it alone is not sufficient to infer the function of interneurons(Freund and Buzsaki, 1996). To attempt a clearer definition ofthe types of interneurons that displayed muscarinic afterpotentials,interneurons having ADPs were filled with biocytin and identifiedby their dendritic and axonal arborizations. Four examples areshown in Figure 8. These interneurons displayed a variety of morphologies,and no layer lacked their axonal or dendritic arborizations. Forexample, a bilaminar interneuron had dendrites that extended fromSO to SR and stratum lacunosum moleculare (SLM) and axons in theareas of SO and SR nearest the pyramidal cell body layer [stratumpyramidale (SP)] (Fig. 8A). The interneuron in Figure 8B had asimilar morphology; however, a significant portion of its axonwas found in SP, and its dendrites were restricted to SO. Twoother cells had axonal projections similar to the neurons in Figure8, A and B. The interneuron in Figure 8C had dendrites in alllayers of CA1; its axon arborized in the layers containing theproximal apical dendrites and cell bodies of CA1 pyramidal cells.The neuron in Figure 8D also had its dendrites in all layers,but its axon arborized throughout the entire extent of SR andparts of SO as well. In all, there were eight interneurons whoseaxons arborized predominantly in SR and/or SLM; six of these hadcell bodies in SR/SLM, and two had cell bodies in SO. In addition,the axons of two interneurons arborized exclusively in SO. Therefore,interneurons displaying muscarinic ADPs do not appear to be confinedto a single well defined anatomical subtype.

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Figure 8. Neurolucida reconstructions of CA1 interneurons displaying muscarinic ADPs after injections of depolarizing current injections. Neurons in A and B responded to muscarine with membrane potential depolarizations and ADPs. C, D, These interneuron did not show a change in membrane potential to muscarine. Axons are shown in thin lines and dendrites in thick lines.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we have described an ADP that occurs in a subpopulation of interneurons in hippocampal area CA1. This ADP arisesafter a train of action potentials only in the presence of muscarinicagonists.

Ionic mechanism of the muscarinic ADP

The ionic mechanisms producing the muscarinic ADP in CA1 interneurons are unlike any others that have been described for corticalneurons, including those in the hippocampus (Benardo and Prince,1982; Gahwiler, 1984). In our study, the ADP was inhibited onlyby low extracellular sodium. Thus, we believe that muscarinicreceptor activity produces an ADP by a novel ionic mechanism thatinvolves sodium influx ortransport.

In some types of neurons, an ADP is supported by calcium influx and is sensitive to inhibitors of VDCCs. This mechanism hasbeen suggested to be the result of activation of a calcium-dependentnonselective cation current (Schwindt et al., 1988; Andrade, 1991;Caeser et al., 1993; Fraser and MacVicar, 1996). A study of olfactorycortex pyramidal cells reported an ADP that was most likely causedby the inhibition of a calcium-activated potassium conductancethat is thought to be responsible for repolarization after a burstof action potentials (Constanti and Bagetta, 1991; Constanti etal., 1993). In neocortical cells, the ADP is probably caused byactivation of a sodium-calcium exchanger (Friedman et al., 1992).None of these mechanisms are likely to underlie the ADP describedhere because inhibition of calcium influx did not inhibit theADP.

A persistent voltage-dependent sodium channel (French et al., 1990) was described to be the mechanism generating a small ADPin bursting CA1 pyramidal neurons. A similar mechanism does notappear to be responsible for the muscarinic ADP in this subsetof interneurons, because it was not inhibited by TTX. However,the muscarinic ADP in interneurons does appear to depend on sodiuminflux or transport because the ADP was blocked by removal ofextracellular sodium but not by amiloride at low concentrationsthat block some types of sodium channels (Garty and Palmer, 1997).

Anatomical structure of interneurons with muscarinic ADPs

Studies to date have suggested that interneurons with similar morphological structure do not necessarily subserve similarfunctions (Freund and Buzsaki, 1996). For example, interneuronswith similar regions of axonal arborization may have differentsynaptic targets; some innervate principal cell dendrites (Gulyásand Freund, 1996), whereas others are specialized to innervateother interneurons (Acsady et al., 1996; Gulyás et al., 1996;Hájos et al., 1996; Blasco-Ibanez et al., 1998). Interneuronswith overlapping axonal distributions can also contain differenttypes of peptide cotransmitters, a factor that may indicate differentfunctions (Freund and Buzsaki, 1996). Finally, interneurons withsimilar anatomical structure often show different firing properties;this may suggest different physiological functions in the hippocampalcircuit (Buhl et al., 1994; Mott et al., 1997; Ali et al., 1998;Ali and Thomson, 1998; Vida et al., 1998). It is also the casethat interneurons with different morphologies may perform similarfunctions. Given this heterogeneity, it is not surprising thatour morphological reconstruction of interneurons with muscarinicADPs showed no distinct structural uniformity. The cell bodiesof these neurons were found in all layers of CA1, albeit withgreater frequency in SR and SLM. In addition, the dendritic andaxonal distribution patterns of these interneurons did not permitcoherent classification. Therefore, although our anatomical resultsappear to describe multiple types of interneurons displaying ADPs,these interneurons with varying morphological features may stillbelong to specific class(es) with similar or overlappingfunctions.

Physiological function of muscarinic ADPs

Muscarinic ADPs often occurred in conjunction with a change in the resting membrane potential, thereby increasing the complexityof possible neuronal outcomes during muscarinic agonist exposure.Some cells depolarized and had an ADP; in these cells, the ADPcould act to augment the increased excitability of the cell. Cellsthat were hyperpolarized by muscarinic receptor activity wouldgenerally be inhibited. A combination of this inhibitory hyperpolarizationand an excitatory ADP might serve to increase the signal-to-noiseratio of the interneuron to excitatory input. Relatively weakinputs would not bring the interneuron to action potential thresholdduring muscarinic hyperpolarization, but inputs strong enoughto evoke an ADP would still result in enhanced action potentialoutput from that same interneuron. Alternatively, the hyperpolarizationcould simply be limiting the barrage of output arising from theADP. In cells that show a biphasic response accompanied by anADP, a combination of these mechanisms might come into play. Forbiphasic responses in the absence of an ADP, the initial hyperpolarizingphase could be responsible for creating a time delay (phase shift)to the excitatory depolarizing phase of the muscarinic response.In biphasic cells that have an ADP, the ADP could reduce the timedelay by either potentiating an excitatory input during the initialhyperpolarizing phase or by augmenting the depolarizing phaseso that it generates action potentials earlier during the biphasicresponse. In cells that showed no membrane potential responseto a muscarinic agonist, the ADP would serve as the sole mechanismfor potentiating the response to excitatoryinput.

During elevated activity of septal cholinergic input, muscarinic activity changes the response to excitatory synaptic inputof ADP-producing interneurons, from brief bursts of a few actionpotentials to long barrages of action potentials produced by thegeneration of the ADP. Given the complexity of muscarinic actionsthroughout the hippocampal circuitry, it is difficult to speculateabout the circuit outcomes of a muscarinic ADP. Nonetheless, cholinergicpromotion of a synaptically activated ADP could have a numberof potential consequences for the function of the hippocampalcircuitry. Perhaps the simplest proposal on the function of theADP is it might cause prolonged inhibition of all or part of theentire hippocampal circuit. Because the ADP is found across differentinterneuronal morphologies, the inhibition it generates mightbe distributed throughout all elements of thecircuitry.

Prolonged inhibition supported by muscarinic ADPs could also conceivably participate in the competitive processes that arehypothesized to underlie many models of synaptic plasticity anddevelopment. These models often invoke a competition whereby "strong"inputs are enhanced and "weak" inputs are further weakened oreven eliminated. An excitatory input that evoked an ADP mightgain an advantage over other subsequent excitatory inputs, becauseit would act to inhibit the ability of those later inputs to firetheir postsynaptic targets over a prolonged period of time. Anexcitatory input strong enough to evoke an ADP in interneuronswould arrive at the principal cells before the ADP-supported inhibitionand thus would be more likely to cause the principal cell to discharge.Inputs arriving later, during the ADP-supported inhibitory period,would be less likely to discharge the principal cells and, undersome models of plasticity and competition, would beweakened.

Another possible function for the ADP could be to switch the interneuron from a predominantly GABA-releasing cell to one whichreleases increased levels of a peptide transmitter. Differenttypes of interneurons contain a variety of neuropeptide cotransmitters,including peptides such as cholecystokinin, vasoactive intestinalpeptide, neuropeptide Y, somatostatin, and opioids (Freund andBuzsaki, 1996). Peptide release requires higher frequencies ofpresynaptic action potentials than classical transmitters (Miller,1990). Thus, peptide release would be more likely to occur asthe result of the action potential barrage stimulated by muscarinicADPs.

  FOOTNOTES

Received Nov. 30, 1998; revised April 9, 1999; accepted April 19, 1999.

This work was supported by National Institutes of Health Grants MH48874 and MH56454 to D.V.M. We thank Brie Linkenhoker forher helpful comments on this manuscript, Eric Schaible and PaulPavlidis for writing the acquisition and analysis software, andDavid Prince and John Huguenard for allowing us use of the Neurolucidafor neuronalreconstructions.
Correspondence should be addressed to Daniel V. Madison, Department of Molecular and Cellular Physiology, Beckman Center,Room 111b, Stanford University School of Medicine, Stanford, CA94305-5345.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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