Muscarinic Induction of Synchronous Population Activity in the Entorhinal Cortex

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Volume 17, Number 17, Issue of September 1, 1997 pp. 6729-6744
Copyright ©1997 Society for Neuroscience

Muscarinic Induction of Synchronous Population Activity in the Entorhinal Cortex

Clayton T. Dickson and Angel Alonso
Department of Neurology and Neurosurgery, Montreal Neurological Institute and McGill University, Montreal, Quebec, Canada H3A 2B4

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Oscillation and synchronization of neural activity is important in normal brain function but is also relevant to epileptogenesis.One of the most frequent forms of epilepsy originates in temporallobe circuitry of which the entorhinal cortex (EC) is crucial.Because muscarinic receptor activation promotes oscillatory dynamicsin EC neurons, we investigated in a brain slice preparation theeffects of carbachol (CCh) on oscillatory population activityin the EC. We found that CCh produced epileptiform activity inEC, which according to field profile and current source densityanalysis was usually driven by layer V. In addition, localizedCCh application and surgical isolation experiments demonstratedthat EC layer II, but not layer III, can also independently generatesynchronous population activity.
Intracellular recordings from EC principal cells during epileptiform activity demonstrated large-amplitude, synaptically drivendepolarizing events and bursts of action potentials synchronizedto the field spikes. In layer II neurons, the depolarizing eventshad a multiphasic reversal potential that suggested concurrentglutamatergic and GABAergic synaptic input. Interestingly, althoughthe epileptiform activity required activation of AMPA but notNMDA receptors, small-amplitude field spikes persisted duringblock of fast excitatory neurotransmission. These field spikeswere correlated to large-amplitude IPSPs in layer II neurons,and both activities were abolished by GABA_A-receptor antagonism.Thus, in response to muscarinic activation, pools of EC interneuronsdischarge synchronously by a mechanism not necessarily involvingprincipal cell activation.
Given the differential projection pattern of EC layers V and II toward the neocortex and hippocampus, respectively, theirrobust epileptogenic character may be of major importance in temporallobe epilepsy.
Key words: temporal lobe epilepsy; parahippocampal gyrus; cholinergic; oscillation; pacemaker; inhibition

INTRODUCTION

The majority of intractable epilepsy cases involve foci located in the mesial aspect of the temporal lobes (Lothman et al.,1991). To understand the basic mechanisms of temporal lobe epilepsyand to suggest more efficacious pharmacological and/or surgicaltreatments (Engel, 1987), it is important to define a preciselocus for the generation of ictal activity in the temporal lobe.In general, most research approaches concerning this disorderhave focused on the contribution of the hippocampal formation(Lothman et al., 1991; Schwartzkroin, 1994). Recent experimentaland clinical studies, however, have suggested that the entorhinalcortex (EC) may play a similar or more important role in temporallobe epilepsy (Dasheiff and McNarmara, 1982; Walther et al., 1986;Wilson et al., 1988; Rutecki et al., 1989; Deutch et al., 1991;Goldring et al., 1992; Jones et al., 1992; Paré et al., 1992;Stringer and Lothman, 1992; Spencer and Spencer, 1994; Braginet al., 1997).

The EC is known to be a "gateway" for the bi-directional passage of information in the neocortical-hippocampal-neocorticalcircuit (Van Hoesen, 1982; Witter et al., 1989; Lopes da Silvaet al., 1990). Via a cascade of cortico-cortical projections,the superficial layers of the EC (II and III) receive an extensiveinput from polymodal sensory cortices (Jones and Powell, 1970;Van Hoesen and Pandya, 1975; Amaral et al., 1983; Deacon et al.,1983; Room and Groenewegen, 1986; Insausti et al., 1987; Reepet al., 1987) that is then conveyed to the hippocampal formationvia the perforant path (Steward and Scoville, 1976). In turn,the hippocampal formation projects back on the deep layers ofthe EC (V-VI) (Swanson and Cowan, 1977), which provide outputpaths that reciprocate the input channels (Swanson and Kohler,1986; Insausti et al., 1997). In addition, the deep layers ofthe EC also project massively on the EC superficial layers (Kohler,1986b; Dolorfo and Amaral, 1997), thereby closing an EC-hippocampalloop. Thus, by virtue of its extensive projection systems, theEC network may act powerfully in the generalization of temporallobe seizures.

The EC is also known to receive a profuse cholinergic input from the basal forebrain that terminates primarily in layers IIand V (Lewis and Shute, 1967; Mellgren and Srebro, 1973; Milneret al., 1983; Alonso and Köhler, 1984; Lysakowski et al., 1989;Gaykema et al., 1990), precisely those layers that gate the mainhippocampal input and output. It is well known that the cholinergicsystem promotes cortical activation and the expression of normalpopulation oscillatory dynamics. In the EC, in vivo electrophysiologicalstudies have shown that the cholinergic theta rhythm is generatedprimarily by cells in layer II (Mitchell and Ranck, 1980; Alonsoand García-Austt, 1987a,b; Dickson et al., 1995). In addition,in vitro studies have also shown that muscarinic receptor activationpromotes the development of intrinsic oscillations in EC layerII neurons (Klink and Alonso, 1997a,b).

On the other hand, some evidence indicates that altered activity of the cholinergic system is relevant to epileptogenesis.Pharmacological activation of cholinergic receptors may promoteand maintain epileptiform discharge (for review, see Turski etal., 1989), and cholinergic neurotransmission seems necessaryfor the normal progression of kindling (Cain, 1989). Upregulationin the levels and activity of both acetylcholine and its metabolicenzymes has also been reported in human epilepsy (Pope et al.,1947; Tower and McEarchern, 1949; Tower and Elliot, 1952; Coutinho-Nettoet al., 1981; Kish et al., 1988). In the EC, expression of muscarinicreceptor protein is increased in kindling-induced epileptic animals(Beldhuis et al., 1993), and the EC also shows a lower thresholdfor carbachol (CCh)-induced electrographic seizure activity thanthe hippocampus (Dickson, 1994).

Given the above information, and that CCh is known to induce rhythmic population activity in the hippocampus in vitro (Konopackiet al., 1987; MacVicar and Tse, 1989; Traub et al., 1992; Huertaand Lisman, 1993; Bianchi and Wong, 1994), we considered it importantto test whether moderate muscarinic receptor activation wouldalso trigger oscillatory population activity in the EC slice andto explore the relation of this activity to an epileptogenic state.Our study demonstrates that CCh induces, in the EC slice, large-amplituderhythmic field activity correlated to the development of paroxysmaldepolarizations in all EC principal neurons. We further demonstratethat muscarinic-induced epileptiform activity can be generatedindependently by both superficial (layer II) and deep laminae(layers V-VI). Moreover, CCh was found to synchronize not onlyprincipal cells but also inhibitory interneurons, and this evenin the absence of fast excitatory neurotransmission (Michelsonand Wong, 1994).

Some of these data have been published previously in abstract form (Dickson and Alonso, 1995a,b; Klink et al., 1995).

MATERIALS AND METHODS
General. Brain slices were prepared from male Long-Evans rats (100-250 gm) using standard procedures (Alonso and Klink, 1993).Animals were decapitated, and the brain was rapidly removed, blocked,and placed in a cold (4-6°C) oxygenated Ringer's solution containing(in mM): 124 NaCl, 5 KCl, 1.2 NaH₂PO₄, 2.4 CaCl₂, 1.3-2.6 MgSO₄,26 NaHCO₃, and 10 glucose, pH 7.4, by saturation with 95% O₂/5%CO₂. Horizontal slices from the retrohippocampal region were cutat a thickness of 400 µm using a Vibratome (Pelco, Redding, CA)and typically did not include the hippocampal formation, becauseour focus was on oscillatory mechanisms within the EC. After atleast a 1 hr recovery period during which they were submergedat room temperature, individual slices were transferred to aninterface chamber maintained at 34 ± 1° and superfused at a rateof 1-2 ml/min. The borders and the cellular layers of the EC werediscerned with a dissecting microscope and a transilluminatorylight source.

Drugs were mixed fresh weekly and stored and refrigerated in stock solutions at 100- to 1000-fold concentrations. They weremixed to their final concentrations in graduated cylinders filledwith Ringer's solution that were attached to the superfusion tubing.Carbamylcholine (CCh), atropine sulfate, bicuculline methiodide,and picrotoxin (PTX) were purchased from Sigma (St. Louis, MO),and 6-cyano-7-nitroxaline-2,3-dione (CNQX), and DL( $-$ )-2-amino-5-phosphonopentanoicacid (AP-5) were purchased from Tocris Cookson (Langford, UK).Salts used in the making of Ringer's solution were all purchasedfrom BDH (Toronto, Ontario, Canada).

Recording and stimulation. Recording electrodes were pulled from micropipette glass (World Precision Instruments, Sarasota,FL) on a Sutter Instruments puller (Novato, CA). Extracellularfield electrodes were filled with Ringer's solution (tip resistance5-10 M $Omega$ ), and intracellular electrodes were filled with 2.5 Mpotassium acetate (tip resistance 60-120 M $Omega$ ).

Field and intracellular signals were amplified using both channels of an Axoclamp 2A amplifier (Axon Instruments, Foster City,CA). Field signals were further amplified by a CyberAmp amplifier(Axon Instruments) to a final gain of 1000 and filtered at a bandpassof 0.1-1.0 kHz (some signals were recorded with the DC componentand later filtered). Signals were visualized on-line using twodigital storage oscilloscopes at slow and fast screen sweep speeds,and stored on VHS tape (Neuro-Corder, New York, NY) for off-lineanalysis using a 386-based computer.

Bipolar stimulation electrodes were constructed from two strips of fine tungsten wire glued along their length and insulatedexcept at their tips. The two poles were positioned straddlingthe angular bundle obliquely (tip separation ~300 µm) above themedial portion of the EC. Electrical stimulation was deliveredusing a square wave generator (MNI technical services) coupledto a constant current/stimulus isolation unit (World PrecisionInstruments), and stimuli consisted of 1 msec square waves ofamplitude 2-5 V. Field potentials effects of stimulation weremeasured in layer II.

Field and intracellular activities were digitized from tape at sampling rates ranging from 1 to 50 kHz and plotted using asoftware acquisition package (Acqui, SICMU, Geneva, Switzerland).The amplitude of field spikes was calculated as the differencefrom peak to trough of the field waveform. Duration of field spikeswas measured from the onset of negativity to the crossing pointat the same potential level. In addition, field activity filteredat a bandpass of 1-40 Hz and sampled at 1 kHz was subjected toFast Fourier Transform using a software package (Origin, MicrocalSoftware, Northampton, MA) for analysis in the frequency domain.The predominant frequency of the signal was taken from the fundamentalpeak of the resulting spectra.

Field profiles. A stationary (reference) electrode was positioned in layer V while a roving electrode was moved along a planeorthogonal to the laminations of the EC in 50 µm stepwise increments.The reference and roving electrodes were separated in the medialaxis by <50 µm, and care was taken to ensure that the trajectoryof the roving electrode remained in the same column along thedepth of the profile. Up to 16 field events were sampled at eachlevel, and typically 10 events were averaged for each using thereference waveform for temporal alignment. The averaged fieldpotential values were then stored in two-dimensional (space vstime) matrices and plotted as a three-dimensional contour plot(Origin).

Current source density (CSD) analysis (Mitzdorf, 1985) was conducted by direct computation of the second spatial derivativeof the extracellular voltage potentials. Briefly, the potentialvalues corresponding to all spatial depths at each time pointwere fitted with a seventh order polynomial. The second derivativeof this function was then computed. Derivative functions for eachtime point were then stored in matrix form and plotted in thesame fashion as for the extracellular potentials.

Horizontal field profiles were constructed in much the same manner as laminar profiles. A stationary (reference) electrodewas positioned in either layer II or V, and the roving electrodewas moved in 50-100 µm stepwise increments along the same medial-to-lateralaxis within the confines of the same cellular layer. When averagingwas conducted, traces were averaged as described above.

Laminar CCh application profiles. Laminar localized application of CCh was conducted during simultaneous field recordingsmade in both layers II and V by fast (10-50 msec) pressure pulses(Picospritzer, General Valve, Fairfield, NJ) to the back of apatch pipette containing 10 mM CCh in a 1% solution of Luxol FastBlue in Ringer's solution. The dye was added to visualize thearea of the slice inundated to ensure that the area of applicationwas highly localized and lamina specific. Only those applicationsthat were confined to the lamina of interest were subsequentlyanalyzed. In some experiments, 1 µM atropine sulfate was addedto the superfusing Ringer's solution during the applications toensure that the recorded field effects were specific to the muscarinicactions of CCh.

Laminar isolation experiments. Cellular layers were separated physically by scalpel cuts that were made in a clear petri dishfilled with oxygenated Ringer's solution after the removal ofthe slice from the recording chamber. Slices were quickly replacedin the chamber after successful completion of the cuts and reperfusedwith CCh. In some cases, a broken pipette was used to separatecellular layers without removal from the recording chamber. Inadditional experiments, the isolation cuts were made before incubationwith CCh.

Intracellular recordings. Intracellular impalements were made in layers II, III, and V. Only neurons fulfilling the followingcriteria were reported in the following study: resting membranepotential negative to $-$ 55mV, input resistance >30 M $Omega$ , and overshootingspikes of amplitude >60 mV. Superficial EC neurons were identifiedelectrophysiologically according to criteria outlined previously(Alonso and Klink, 1993; Dickson et al., 1997). Briefly, layerII stellate cells (SCs) showed profound time-dependent inwardrectification in the hyperpolarizing direction and prominent subthresholdmembrane potential oscillations and cluster spiking on DC depolarization.Layer II pyramidal-like cells showed less robust time-dependentinward rectification with hyperpolarizing pulses and no rhythmicsubthreshold oscillations. In addition to their location in distinctlyobservable lamina, layer III pyramids showed high input resistance(<70 M $Omega$ ) and no, or only minor, time-dependent inward rectificationwith hyperpolarizing current pulses, and went easily into tonicfiring with DC depolarization (Dickson et al., 1997).

RESULTS

General characteristics of CCh-induced population activity
Bath application of moderate concentrations of CCh (10-30 µM) induced rhythmic large-amplitude (>500 µV) field activity in55% (67 of 122) of EC slices tested without previous control forfield responses to angular bundle stimulation. The success rateof rhythmic population activity induction was much higher (20of 21; ~95%), however, when CCh was applied to EC slices selectedfor responding to angular bundle electrical stimulation, withan evoked field potential in layer II of at least 500 µV.

The induction and maintenance of rhythmic field activity by CCh was dependent on muscarinic receptor activation because itwas blocked by atropine (300 nM-1 µM; n = 9). As illustrated inFigure 1, the CCh-induced field activity had an epileptiform morphology.It was typically initiated by a long-duration ictiform event (LDE:5-40 sec in duration) (Fig. 1A,B) and was usually followed bya slow periodic occurrence of short-duration ictiform events (SDEs:0.1-4,0 sec in duration) (Fig. 1A,C). Occasionally, however, LDEswould show a similar periodicity, although at slower frequencies(<0.05 Hz) (see Figs. 6, 9). Aside from their differences in durationand interevent frequency, both LDEs and SDEs were similar in theirinitial waveform pattern (Fig. 1D).
Fig. 1. Population (field) activity elicited in entorhinal slices perfused with CCh (20 µM). A, After 6 min of perfusion with CCh,large-amplitude rhythmic field events typically develop. The insetdemonstrates the experimental setup. B, An AC recording of theinitial LDE in A at an expanded time scale. C, An AC recordingof an SDE in A shown at an expanded time scale. D, A superimpositionof the first five field spikes in B and C. Note the very goodcorrespondence between the two. E, An AC recording of an LDE elicitedin another experiment. Multiple phases can be seen correspondingto the lines underneath the analog recording. Fast Fourier Transformscorresponding to the three phases are shown below, with the fundamentalpeak frequency noted. In this and in all subsequent figures, negativityis down.
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Fig. 6. Activation of an electrophysiologically identified EC layer II SC during rhythmic epileptiform events evoked by CCh (20 µM).The field recording location was in layer II, 150 µm lateral tothe intracellular electrode. A, Long trace showing the cell becomingstrongly activated during epileptiform events. This cell was depolarizedby 6 mV in response to CCh before the initiation of field events.During the last field event shown, DC hyperpolarization unveiledlarge-amplitude depolarizing synaptic potentials synchronizedwith the negative field spikes. B, Fast sweep speed trace of thefirst and last epileptiform events shown in A. C, Higher sweepspeed traces for the indicated periods of the epileptiform eventshown in B.
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Fig. 9. Field events elicited by CCh are not abolished by pharmacological blockade of NMDA receptors. A, Local field and correspondingintracellular activity in a layer II non-SC elicited by 20 µMCCh. SDEs are elicited at a frequency of 0.8 Hz and have an averageduration of 2.9 ± 1.1 sec. B, A single field event from A shownat expanded time scale. Individual field spikes averaged 134 ±49 msec for three events taken from this sample and occurred ata frequency of 5.5 Hz. C, Bath perfusion of AP-5 (30 µM) did notabolish the field activity or the paroxysms in the neuron; however,the duration of the field events increased slightly to 4.0 ± 0.1sec. D, An expanded trace from C. Individual field spikes averaged98 ± 25 msec and occurred at a frequency of 11.3 Hz.
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As recorded in layer V, LDEs consisted of a train of negative-going population spikes superimposed on a large-amplitude (0.5-1.4mV) negative DC potential (Fig. 1A). As in the cases illustratedin Figure 1B,E, LDEs were consistently multiphasic, having atleast two and sometimes three phases of population spike activitywith different spectral peak frequencies, which resembled thetonic and clonic phases characteristic of an electrographic seizurewith a "transition" phase occasionally interposed between. Thefeatures of LDEs are summarized in Table 1. Essentially, thetonic phase was characterized by a train of high frequency populationspikes (14.4 Hz), whereas the transitional and clonic phases showedprogressively slower frequencies of field spikes (7.5 and 4.0Hz, respectively) (Fig. 1E). Similarly, the duration of individualpopulation spikes tended to increase as the event progressed.The average amplitude of population spikes, however, was relativelyconstant over the three phases when summed over all cases butcould show systematic variations in individual cases, such asthe increase-decrease-increase sequence shown in Figure 1E.

Table 1. Summary of features of long-duration ictiform events

Duration(s) Frequency (Hz)
Field spike duration (msec)
Field spike amplitude (µV)

InterLDE IntraLDE Tonic Trans Clonic Overall Tonic Trans Clonic Overall Tonic Trans Clonic

10.6 ± 7.4 0.010 ± 0.006 7.9 ± 4.1 14.4 ± 4.5 7.5 ± 3.3 4.0 ± 1.0 162 ± 121 108 ± 53 128 ± 65 226 ± 157 446 ± 267 450 ± 319 463 ± 270 432 ± 233

Values reported are means ± SD for at least five separate occurrences of long-duration ictiform events (LDEs) in seven differentexperiments. InterLDE frequency, The frequency of the periodicitiesof occurrence of LDEs; IntraLDE frequency, the frequency of populationspike occurrence as computed by FFTs within LDEs across all phases;Tonic, Trans, and Clonic frequency, the frequency of populationspike occurrence within the first (tonic), second (transitional),and third (clonic) phase of an LDE, respectively. Overall fieldspike duration, The duration of population spikes (measured acrossthe baseline width) averaged across all phases of an LDE; Tonic,Trans, and Clonic field spike duration, the duration of populationspikes averaged across the first (tonic), second (transitional),and third (clonic) phase of an LDE, respectively. Overall fieldspike amplitude, The amplitude of population spikes (measuredfrom baseline to peak) averaged across all phases of an LDE; Tonic,Trans, and Clonic field spike amplitude, the amplitude of populationspikes averaged across the first (tonic), second (transitional),and third (clonic) phase of an LDE, respectively.

SDEs consisted of large-amplitude negative-going field potentials typically associated with a repetitive sequence of fieldspikes (Fig. 1A,C), often resembling those seen during the LDEs(Fig. 1D). In fact, the average frequency of these field spikes(7.7 Hz) (Table 2) was virtually identical to the average populationspike frequency summed over all phases of the LDEs (7.9 Hz) (Table1). SDEs typically repeated with a clock-like rhythmicity (Fig.1A) at a frequency that ranged from 0.05 to 0.6 Hz for differentcases. The quantified features of SDEs are summarized in Table2.

Table 2. Summary of features of short-duration ictiform events

Duration(s) Frequency (Hz)
Field spike

InterSDE IntraSDE Duration (msec) Amplitude (µV)

1.06 ± 0.85 0.30 ± 0.31 7.7 ± 5.0 147 ± 50 767 ± 438

Values reported are means ± SD for nine different experiments. InterSDE frequency, The frequency of the periodicities of occurrenceof short-duration ictiform events (SDEs); IntraSDE frequency,the frequency of population spike occurrence within SDEs; fieldspike duration and amplitude, the duration (across baseline) andamplitude (baseline to peak) of population spikes within an SDE.

Field profile and CSD analysis
In an attempt to clarify which EC layer acts as the generator of CCh-induced epileptiform activity, we examined the laminardistribution of field events to construct laminar field potentialprofiles and perform CSD analysis for the localization of themain sinks and sources of current (n = 6). A typical case is illustratedin Figure 2. As shown in Figure 2A, a stationary electrode (red)was positioned in layer V while a moving electrode (blue) wasadvanced in 50 µm steps from the pial surface (layer I) to theangular bundle in a direction normal to the cortical layers. Figure2B illustrates the laminar field potential profile correspondingto the initial 60 msec of averaged SDEs recorded at distinct locations(indicated to the left). The corresponding reference recordingsused to construct the profile have been superimposed at the top(red). It can be observed that a robust field negativity (correspondingto a population spike) appeared first in layers V-VI and thensuccessively at later times in layer III and then in layer II.Using the latency values corresponding to the peak negativitiesin the respective lamina, the speed of propagation was calculatedto be 110 ± 14 mm/sec. Although appearing first in layers V-VI,the field negativity in layer III showed both a greater amplitudeand longer duration. The laminar field profile in Figure 2B hasbeen represented as a contour plot in the right panel of Figure2C. Field negativity has been coded in the hot (red) end of thespectrum and was initiated in the deep layers and propagated superficiallyto layer III and finally to layer II.
Fig. 2. Laminar field potential profile and CSD analysis of epileptiform events. A, A representation of the experimental scheme. Astationary (reference) electrode was located in layers V-VI whileanother electrode (moving) was advanced from the pial surface(layer I) to the deep layers [angular bundle (AB)] in 50 µm increments.B, Field potential profile of the first 60 msec of an SDE recordedat the layers noted. The superimposed traces at the top representthe field potentials recorded at the level of the reference electrodeat all levels shown and were used to align the traces recordedfrom the moving electrode. The latency from the onset of the peaknegativity in layers V-VI to layers III and II was 3.0 and 5.9msec, respectively. C, Pseudocolor surface contour plot of thefield potential (left panel) and CSD (right panel) profile. Thefield negativity is observed first in layers V-VI from where itpropagates to layers III and II. It is largest and shows the longestduration in layer III. Associated with the initial field negativitiesare spatially distinct current sinks lasting for ~2 msec, seenfirst in layers V-VI and subsequently in layers III and II. Afterthe initial sink there is a rhythmic reappearance of sinks inlayers V-VI (approximate frequency 200 Hz), whereas a more tonicsink of elongated duration (12 msec) appears in layer III, faroutlasting those in either layers V-VI or II.
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The left panel of Figure 2C represents the contour plot for the CSD analysis of the field potential profile in B and C. Currentsinks have been coded in the hot (red) end of the spectrum. Notethat a distinct short-lasting (2-3 msec) current sink appearedfirst in layers V-VI. A second but much larger current sink developednext in layer III, where it extended over the full extent of thelayer progressing from its deepest border with layer IV (laminadessicans) to the transition with layer II, where it stopped.A third distinct and final current sink then developed in layerII. The sequential development of current sinks first in layersV-VI, then in layer III, and finally in layer II suggests thatthese epileptiform discharges are typically generated in the deeplayers of EC and then propagated actively toward layers III andII after the known ascending pathways (Kohler, 1986a). As is thecase in the CSD profile of Figure 2, it was a consistent observationthat in layer V the initial current sink was always followed bytwo other sinks at a fixed interval of ~5 msec, thus indicatingthat the population activity in layer V occurred as a high frequency(~200 Hz) population oscillation. In contrast, in layer III theinitial short-lasting current sink was followed at ~5 msec bya second, maintained sink of very long duration (~20 msec). Onthe other hand, in layer II, only the initial short-lasting currentsink was typically observed.

We also wanted to examine whether the activity generated in layers V-VI occurred synchronously over the full horizontal extentof the layer or whether there was some specific focal zone fromwhich the activity was propagated. With this in mind we constructedfield potential profiles along the mediolateral axis of layerV (horizontal profiles, n = 6). A typical experiment is illustratedin Figure 3. The diagram in Figure 3A summarizes the experimentalprotocol. The reference electrode was positioned in the most medialportion of layer V, and a moving electrode was advanced at fixedsteps (100 µm) along layer V. Representative recordings of SDEsrecorded at increasing distances from the reference electrodeare plotted in Figure 3B. The top traces in this panel are a superimpositionof all averaged reference recordings during the track. Note thatSDEs recorded at increasing lateral distances from the referencerecording occur at increasing latencies, thus indicating thatin this case the epileptiform activity propagated in the mediolateraldirection along layer V at a speed of ~100 mm/sec (Fig. 3D, opencircles). Occasionally (such as the case illustrated in Fig. 3),SDEs could appear at the same recording site with two differentwaveforms (Fig. 3C). Although the events corresponding to oneof the waveforms showed positive latencies at increasing lateraldistances from the reference (B, C, D; open circles), the othershowed negative latencies (C, D; filled circles) that indicatedindependent focal events showing opposing propagation directionsin the mediolateral axis. Although independent, the speed of propagationof epileptiform activity in either the mediolateral (open circles)or lateromedial direction (filled circles) was almost identical(D). These results suggest the existence of multiple focal generatorsof epileptiform activity within layer V that can be propagatedin either the lateral or medial direction in the horizontal axisof the slice.
Fig. 3. Horizontal propagation of epileptiform events in the entorhinal slice. A, Representation of the experimental protocol. A referenceelectrode was placed in the medial aspect of layers V-VI whilea moving electrode was advanced in 100 µm increments along themedial-lateral axis of layers V-VI. B, Horizontal profile of thefirst 60 msec of an SDE. The traces at the top represent the superimpositionof the potentials recorded at the reference electrode site foreach of the horizontal levels shown below. As the moving electrodewas moved further in a lateral direction the latency differenceincreased, indicating a medial to lateral propagation of the event.C, Combined horizontal profile for two distinct SDEs as distinguishedby their different waveforms as recorded at the level of the stationaryreference electrode (A). The events alternated in their occurrenceand appeared to propagate in opposite directions. One event isthe same as in B ( $open circle$ ) and propagated in the medial-to-lateral directionas indicated by the increasing latency from the reference at increasingrecording distances. The second ( $bullet$ ) propagated in the lateral-to-medialdirection as suggested by the opposite temporal relation. D, Aregression plot of the relationship between the latency differencesbetween the activity at the stationary and the moving electrodefor both SDEs shown in C. Both events appear to travel at similarspeeds across the horizontal aspect of the slice. The averagepropagation speed of the event shown in B ( $open circle$ ) was 111 mm/sec,whereas the second event shown in C ( $bullet$ ) propagated at 100 mm/sec.
[View Larger Version of this Image (26K GIF file)]

Surgical isolations and pressure pulse application
Although the above data indicate that layers V-VI play a leading role in the generation of epileptiform activity in the EC,our laboratory has shown that CCh has a robust facilitatory actionon the intrinsic oscillatory and bursting properties of EC layerII neurons (Klink and Alonso, 1997a,b). Also, projection neuronsfrom layer II display a profuse net of recurrent collaterals thatare likely to excite neighboring cells (R. Klink and A. Alonso,unpublished observations). Thus, the electrophysiology and anatomyof EC layer II suggests that this layer could act as an independentpacemaker for oscillatory dynamics. Indeed, in those cases (n= 10) in which we monitored the induction of epileptiform activityusing CCh by making dual simultaneous recordings in both layerII and layer V, low-amplitude short-duration field events wereobserved occasionally (n = 2) in layer II before any field activityin layer V.

To examine the issue of whether EC layer II could independently generate synchronous population activity, we initially performedfocal CCh applications in layers II, III, and V while we simultaneouslyrecorded field activity in layers II and V (Fig. 4A) (n = 17).As illustrated in Figure 4B, in 30% of the cases (n = 17), pressurepulse applications of CCh in layer II evoked synchronous populationactivity localized exclusively to layer II. On the other hand,when CCh was focally applied to layer V, a prolonged series ofepileptiform events was consistently recorded (100%; n = 17) byboth layer V and layer II electrodes (Fig. 4D). This activitymimicked the onset of epileptiform discharges seen with bath perfusionof CCh in that the first event triggered by CCh was an LDE andwas followed by short ictiform discharges. Focal CCh applicationsto layer III never resulted in the elicitation of epileptiformevents, whereas applications to deep layer VI/angular bundle typicallyresulted in no activity or the onset of a small number of SDEsat long delays (Fig. 4E). In all cases tested (n = 3), it wasfound that atropine blocked the activity elicited by focal CChapplications at both layer II and layer V sites (not shown). Thus,these results suggest that both EC layers II and V, but not layerIII, contain the appropriate neuronal and circuit machinery toindependently generate synchronous population activity.
Fig. 4. Field effects of laminar-localized pressure pulse applications of CCh (10 mM) in the entorhinal slice. A, A diagrammatic representationof the recording and application arrangement. Two stationary recordingelectrodes were located in layers II and V. A pressure pipettewas placed consecutively in layers I, II, III, V, and VI and inthe angular bundle (AB), and a 10 msec pulse was administeredat each point. B, Layer II application (denoted by the verticalline). After only a short delay, small-amplitude epileptiformactivity was recorded in layer II. Note the absence of activityin layer V. C, Layer III application. No activity was elicited.D, Layer V application. A long-lasting series of large-amplitudeepileptiform events of both long and short duration were elicitedin layer V and propagated to layer II. These events are remarkablysimilar to those engendered by bath perfusion of CCh (see Fig.1). E, Layer VI application. One short-duration field spike waselicited at a long delay from the onset of the pressure pulse.
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To further clarify whether EC layer II could independently generate rhythmic population activity, we undertook surgical isolationexperiments. In the intact EC slice, we first induced epileptiformactivity with CCh to be ensured of the viability of the slice,and then under continuous CCh superfusion we cut the slice toseparate the internal and external principal laminae. As shownin Figure 5, preserved epileptiform activity resembling that seenprevious to the cut could be observed in most cases, in both thepiece of slice containing the deep layers V-VI (Fig. 5A) (90%;n = 19) or the superficial layers I-III (Fig. 5B) (32%; n = 19)laminae. In additional cases, with surgical cuts that selectivelyisolated layer II, epileptiform activity was maintained over thislayer (Fig. 5C) (3 of 12 cases). In no case, however, was activitymaintained in a piece of slice containing only layer III (n =10). In addition, field potential profiles conducted after surgicalisolation of the superficial principal lamina (layers I-III; n= 3) indicated that the remaining field activity was generatedby layer II only and volume conducted to the remaining layer III.
Fig. 5. Effect of knife cuts separating the external and internal principal lamina on the maintenance of CCh-induced epileptiformactivity. A, Maintenance of LDEs and SDEs in the internal principallamina after surgical separation of the superficial principallamina. Left, A diagrammatic representation of the experimentis shown. The recording both pre- and post-cut was at the levelof layer V in the internal (deep) principal lamina. The levelof the cut is shown by the dotted line. Middle, Activity elicitedby CCh before the surgical removal of the superficial laminae.Both SDEs and LDEs are shown. Right, Activity maintained in thedeep laminae after the cut. Again, both LDEs and SDEs can be seenwith a similar pattern of expression. B, Maintenance of LDEs andSDEs in the external principal lamina after surgical separationof the deep principal lamina. Left, A representation of the experimentis shown. The recording both pre- and post-cut was at the levelof layer II in the superficial principal lamina. The level ofthe cut is shown by the dotted line. Before (middle) and after(right) the removal of the deep laminae, both SDEs and LDEs canbe observed. The frequency of expression of SDEs appeared to quickenafter the cut, but the overall pattern appears similar. C, Inanother experiment, recording pre- and post-cut was performedin both layers II and V. Activity is coincident in both layersprevious to but not after the cut.
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To further substantiate the above results, surgical cuts separating the deep and superficial laminae were also performed beforeperfusion with CCh was undertaken (n = 21). In most of these cases(n = 19), the piece of slice containing the deep laminae showedpatterns of epileptiform activity similar to those of intact sliceswhen perfused with CCh. Also, in several cases (n = 6) CCh applicationto the piece of slice containing layer II induced epileptiformactivity (not shown). The above surgical isolation experimentsindicate that both layers V-VI and layer II can act as independentpacemakers of synchronous population activity.

Intracellular correlates
We also investigated the intracellular correlates of the CCh-induced epileptiform activity, particularly in neurons from layerII (n = 47), because they have been the most extensively characterizedelectrophysiologically, but also in neurons from layers III (n= 12) and V (n = 9). During both LDEs and SDEs, principal cellsin all layers fired bursts of action potentials synchronized withthe local negative-going field spikes (Figs. 6, 7). As in thespecific layer II cell illustrated in Figure 6, in neurons fromall layers, membrane voltage manipulation always revealed thatthe field-associated bursts of action potentials were driven bydepolarizing events of synaptic nature. It was also apparent thatin neurons from all layers the epileptiform discharges were typicallyassociated with a plateau depolarization (Fig. 7; note dottedline in A-D). This plateau depolarization was particularly prominentand considerably outlasted the field discharges in neurons fromlayers III and V in comparison to neurons from layer II (Fig.7).
Fig. 7. Typical recordings from entorhinal neurons during epileptiform events induced by 10 mM CCh. A, A layer II SC; B, a layer IInon-SC; C, a layer III pyramidal cell; D, a layer V cell. Allfour types of cells show activity synchronized to the local fieldnegativity. In addition, all cell types demonstrate the generationof a plateau potential during the production of field activity;however, the depolarization evoked in cells of both layers III(C) and V (D) show a markedly greater depolarization than thatdemonstrated in either layer II subtypes.
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In layer II projections neurons, we explored the reversal potential of the synaptic events underlying the epileptiform dischargesby means of DC current injection (n = 6). As in the case illustratedin Figure 8, the depolarizing synaptic events were always fullyreversed at potentials positive to approximately $-$ 40mV; however,we could always detect at least two components that reversed atdifferent potentials. There was an early phase that reversed atapproximately $-$ 50mV (Fig. 8A, arrow) and a later phase that reversedat membrane potentials ~5-10 mV more positive (Fig. 8A, asterisk)than the early phase. Among other factors, this multiphasic reversalpotential may have resulted from the rather synchronous inputonto projection cells of both glutamatergic- and GABAergic-mediatedsynaptic potentials. Consistent with this interpretation, threefast-spiking cells (presumably interneurons) that were briefly(1-3 min) recorded during CCh-induced population activity alsofired in bursts synchronized to the negative-going populationspikes of the epileptiform events (not shown).
Fig. 8. Reversal of synaptic events induced by CCh in a layer II SC. A, A long trace of activity induced by 30 µM CCh. B, Alterationsin amplitude and direction of potential changes induced by depolarizingand hyperpolarizing current injection. At potentials near andjust above the firing threshold of the cell, the intracellulartrace appears biphasic, with an initial component reversing atapproximately $-$ 50 mV (arrow) and another reversing approximately5-10 mV more positive (asterisk).
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Pharmacology
Given the excitatory nature of the intracellular correlate of field epileptiform events, we sought to characterize their dependenceon glutamatergic neurotransmission. Antagonism of NMDA receptor-mediatedneurotransmission with AP-5 (30 µM) did not abolish the epileptiformdischarges in any of the cases tested (n = 6) (Fig. 9); however,it did produce some consistent effects. First, block of NMDA neurotransmissiondecreased the duration of individual population spikes from 179± 40 to 105 ± 36 msec and increased their frequency from 7.0 ±1.7 to 14.2 ± 4.1 Hz. Second, NMDA receptor block also producedan increase in the duration of the epileptiform events from anaverage of 4.3 ± 2.3 to 6.1 ± 1.5 sec (Fig. 9).

The excitatory component of the field activity was dependent, however, on AMPA receptor-mediated glutamatergic transmission.It could be blocked by CNQX alone (n = 5) or in combination withAP-5 (n = 10) (Fig. 10). To our surprise, however, small-amplitudefield activity always persisted in layer II after blockade offast excitatory amino acid (EAA) neurotransmission (Fig. 10A,B).This activity was also present in surgically isolated layer IIas well (n = 3), and typically consisted of positive-going fieldevents (Figs. 10, 11). The intracellular correlate of this activityin layer II projection cells were large-amplitude IPSPs (8 ± 2mV at 61 ± 2 mV; n = 8) [for simplicity hereafter referred toas giant IPSPs (gIPSPs)] of a rather fast rate of rise (43 ± 21msec) and slow decay (total duration, 903 ± 116 msec) (Fig. 10A-C).After peaking, these gIPSPs continuously decreased toward theresting level (Fig. 10B,C); however, we could typically distinguish,particularly at hyperpolarized levels, a decrease in the rateof decay at ~100 msec from the gIPSP onset (Fig. 10C). Membranehyperpolarization revealed that gIPSP peak reversed at approximately $-$ 75 mV and the late phase at ~10 mV more negative (Fig. 10C) (n= 3).
Fig. 10. During CCh superfusion, blockade of EAA neurotransmission reveals synchronized firing of inhibitory interneurons. A, Duringperfusion with 10 µM CNQX and 30 µM AP-5, excitatory paroxysmsin a layer II stellate were abolished; however, small-amplitudepositive-directed field events (top trace) persist that correspondto giant IPSPs in the intracellular recording (bottom trace).B, Superimposition of field events in A shown at a faster sweepspeed demonstrates a relative degree of discordance between thefield and intracellular recordings. Although the field eventsappear roughly similar, there is not a perfect synchrony of thecorresponding IPSPs, some of which occur at a slightly differentphase of the field event. In addition, field events could be unaccompaniedby a gIPSP ( $bullet$ ), and conversely gIPSP could be unaccompanied bya field event (*). C, Membrane hyperpolarization reveals thatthe fast component of the gIPSP reverses at approximately $-$ 75mV,whereas a slower component reverses at more negative potentials.D, Blockade of fast GABAergic neurotransmission with picrotoxin(PTX) (100 µM) abolished both the field and the intracellularevents.
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Fig. 11. Horizontal and laminar profiles of GABAergic field potentials in layer II. A, Experimental setup. Small-amplitude positivefield events were elicited by 20 µM CCh in the presence of 10µM CNQX and 30 µM AP-5. A stationary electrode was centered inlayer II, and a moving electrode was used to construct both ahorizontal and a laminar profile. B, Results of the horizontalprofile (shown in A as sites numbered 1-6). The amplitude of positivefield events appears to decay monotonically as the roving electrodeis moved further lateral. In addition, independent field eventswere apparent at lateral distances as close as 100 µm, which showedlittle to no correspondence at the reference site (traces 3 and4). C, Results of the laminar profile conducted in the same slice(shown in A as sites lettered a-f). The amplitude of the signalrapidly decays as the electrode is displaced from layer II; however,a measurable reversal appears in upper layer III (trace 1e). D,Results of a horizontal profile in another slice in which thetrajectory of the roving electrode passed sites both medial andlateral to the reference electrode. Similar to the results shownin B, the waveform decays monotonically at distant sites in boththe medial and lateral directions.
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Interestingly, we observed that when the extracellular and intracellular electrodes were separated by distances greater than~200 µm, there was a lack of synchrony between the field eventsand the intracellular gIPSPs. In addition, as in the case illustratedin Figure 10, even within this critical range there tended to bea lack of absolute consistency between the intracellular and extracellularrecordings in terms of waveform and synchrony. To illustrate thispoint, all individual field events and gIPSPs from Figure 10A havebeen superimposed in Figure 10B at an expanded time scale. Notethat gIPSPs could occur in the absence of a field event (Fig.10A,B, asterisk), or conversely field events could occur in theabsence of gIPSP (Fig. 10A, filled circle). In addition, the shapeof the field waveform could occasionally vary, and although mostgIPSPs were associated with a field event, they could occur atclose but different time relations to the field event (Fig. 10B,right). Finally, we examined the effect of GABA_A receptor antagonismwith PTX (100 µM) or bicuculline (10 µM) on the field events andgIPSPs. As shown in Figure 10D, in all cases (n = 5) GABA_A receptorantagonism always abolished all field events and IPSPs that persistedduring glutamatergic transmission block.

The above data suggest that gIPSPs may result from the synchronous firing of interneurons, the positive-going field eventsin layer II arising from the associated inhibitory currents inprincipal neurons. The lack of perfect synchrony between the gIPSPsand field events suggest, however, that there might be multiplepools of interneurons impinging on distinct (and perhaps overlapping)pools of principal cells. To further examine this possibility,we performed mediolateral and depth profiles of the layer II positive-goingfield events (Fig. 11A-D) (n = 5). Typically, a reference electrodewas centered in layer II, and a second moving electrode recordedactivity at increasing fixed 50 µm steps in the mediolateral orlaminar axis (Fig. 11A). Figure 11, B and D, demonstrates that asthe distance from the reference electrode increased, the amplitudeof the reference field event decreased and became practicallyundetectable at a distance of ~200-300 µm. Despite large-amplitudechanges at these distances, no measurable latency changes wereapparent in the waveform recorded at the moveable electrode. Atthe same time, as the distance from the reference electrode increased,other field events not detected by the reference electrode appearedin the moving electrode (Fig. 11B, traces 4 and 5). Profiles conductedin both the medial and lateral directions with respect to thestationary electrode (Fig. 11D) demonstrated similar findings.Laminar profile analysis also indicated that the layer II positiveevents reversed in the upper layer III to become quickly undetectableas the test electrode was advanced further toward layer IV (Fig.11B).

DISCUSSION
This report focused on the ability of muscarinic receptor activation with CCh to trigger rhythmic population activity in theEC slice. CCh, in moderate concentrations (10-30 µM), indeed triggeredpopulation activity in EC, which had an epileptiform character.Similar to that of the neocortex, epileptiform activity in ECwas typically driven by layer V; however, an isolated layer IIwas also able to generate epileptiform events. Because EC layersII and V gate the cortical input and output, respectively, ofthe hippocampal formation (Sorensen and Shipley, 1979; Van Hoesen,1982; Swanson and Kohler, 1986; Witter et al., 1986; Witter, 1989),our data suggest that they may act as powerful distributors ofepileptiform activity throughout the temporal lobe. In addition,we also found that CCh synchronized firing of inhibitory interneuronsby a mechanism not necessarily dependent on principal cell activation(Michelson and Wong, 1994).

The epileptiform activity induced by CCh in EC showed similarities to that observed in the combined entorhinal-hippocampalslice using several proconvulsive manipulations such as low Mg²⁺ (Walther et al., 1986), high K⁺ (Bear and Lothman, 1993), GABA_A receptor block (Jones and Heinemann,1988), 4-aminopyridine (4-AP) (Avoli et al., 1996), and pilocarpine(Nagao et al., 1996). In all cases, LDEs appeared to be generatedby the EC and were maintained exclusively in that region afterits surgical isolation.

Recent clinical data have also highlighted the importance of EC in epilepsy. Sclerotic lesions, long thought to be limitedto the hippocampus in temporal lobe epilepsy (Babb, 1991; Meenchkeand Veith, 1991; Swanson, 1995), have recently been demonstratedto include cortex further lateral in the temporal lobe, includingthe EC (Gloor, 1991; Levesque et al., 1991; Du et al., 1993).Furthermore, EC stimulation generates field potentials in thehippocampus that resemble spontaneous interictal discharge (Ruteckiet al., 1989), and limbic seizures recorded with depth or subduralstrip electrodes demonstrate focal seizure generation in EC (Spencerand Spencer, 1994). Moreover, recent surgical evidence has pointedto the role of entorhinal removal in controlling intractable temporallobe seizures (Goldring et al., 1992, 1993; Fried, 1993; Feindelet al., 1996).

Our laminar field potential profile and CSD analysis clearly indicated that the CCh-induced epileptiform discharges were initiatedin layer V from where they propagated actively toward layers IIIand II at a speed of ~0.1 m/sec. In addition, horizontal fieldpotential profiles also demonstrated that layer V could containseveral foci from where epileptiform events propagated horizontallyin either the medial or lateral direction, also at a speed of~0.1 m/sec (Miles et al., 1988; Chagnac-Amitai and Connors, 1989a;Traub et al., 1993). It thus appears that once the activity isinitiated by a small pool of layer V neurons, it spreads rapidlythroughout the EC. That layer V neurons are primarily responsiblefor the generation of CCh-induced epileptiform activity is consistentwith previous studies in the neocortical slice (Chagnac-Amitaiand Connors, 1989b; Silva et al., 1991; Prince, 1993). A roleof EC layer V neurons in the generation of epileptiform activityin the Mg²⁺-free model has also been suggested recently (Jones and Heinemann,1988).

A leading role of EC layer V in the generation of epileptiform events was definitively established by focal CCh applicationsand surgical isolation experiments. Focal CCh applications inlayer V always resulted in robust synchronous activity that wasactively propagated toward superficial layers. In addition, asurgically isolated layer V continued to robustly generate epileptiformactivity. The spread of epileptiform activity from layer V tolayers III and II is consistent with the known unidirectionalorganization of the EC layer connections in which each EC layerinnervates every layer situated superficially to it (Kohler, 1986b).

Interestingly, our experiments also pointed out that EC layer II, but not layer III, also has the capacity to independentlygenerate hypersynchronous rhythmic population activity. Indeed,focal CCh applications to layer II frequently resulted in locallygenerated long trains of rhythmic population activity that didnot actively spread to deeper layers, and a surgically isolatedlayer II was often found to sustain short or long ictiform discharges.Thus, in the EC, both layers V and II seem to have the adequateneuronal and circuit machinery for the generation of hypersynchronouspopulation activity. In the neocortex, an isolated layer II/IIIhas recently been shown to generate population events at a slowfrequency in response to kainic acid application (Flint and Connors,1996).

EC layer II contains two morphologically and electrophysiologically distinct principal cell types: the SCs and pyramidal-likecells (Alonso and Klink, 1993). The SCs generate rhythmic subthresholdmembrane potential oscillations, the manifestation of which isfacilitated by muscarinic receptor activation (Klink and Alonso,1997b). The pyramidal-like cells behave more similarly to regularlyspiking neocortical neurons, and muscarinic receptor activationfacilitates in them the generation of intrinsic bursting activity(Klink and Alonso, 1997b). Both neuronal types display a profusenet of recurrent axonal collaterals that distribute extensivelyover layer II (Kohler, 1986b) (R. Klink and A. Alonso, unpublishedobservations). EC layer II thus appears to contain the appropriateneuronal and circuit mechanisms for the local promotion of oscillatorydynamics, and it is thus not surprising that CCh triggers synchronizedpopulation oscillations locally in layer II.

The inability of EC layer III to independently generate synchronized population oscillations in response to CCh was particularlyevidenced by the inability of focal layer III CCh applicationsto induce population oscillations, in spite of the fact that focalCCh applications do cause direct depolarizing responses in theseneurons (R. Klink and A. Alonso, unpublished observations). Thisfinding is somewhat consistent with the absence of intrinsic oscillatoryneurons in layer III (Dickson et al., 1997) and the more restrictedhorizontal projections of layer III as compared with those oflayer II (Kohler, 1986b). Our CSD and intracellular recordinganalysis indicate, however, that during the epileptiform eventslayer III neurons are subjected to very strong excitatory synapticbombardment (presumably from layer V neurons) (Scharfman, 1996;Gloveli et al., 1997). It might be that a massive NMDA receptoractivation in layer III cells, caused by hyperactivation of layerV neurons, is at the basis of the robust layer III neuronal degenerationobserved in temporal lobe epilepsy (Du et al., 1993, 1995). Itis tempting to speculate that during chronic epilepsy the lossof the layer III input onto layer II (Kohler, 1986b) may leadto sprouting of the recurrent collaterals of layer II cells, therebyenhancing feedback excitation and thus the epileptiform tendencyof layer II.

Our intracellular analysis demonstrated that principal neurons in all EC layers discharged bursts of action potentials synchronizedwith the local negative-going field spikes. In all cases, membranehyperpolarization revealed that these bursts were driven by large-amplitudesynaptic events. In layer II neurons, these synaptic events werealways fully reversed at approximately $-$ 40 mV, and we could alwaysdetect an early component that reversed at slightly more hyperpolarizedlevels. This suggests that the epileptogenic synaptic events areprobably the compound action of both glutamatergic-mediated EPSPsand GABAergic-mediated IPSPs. Similar data have been reportedduring perfusion of hippocampal slices with 4-AP (Rutecki et al.,1987), and simultaneous firing of interneurons and principal cellshas been described in the high potassium model of epilepsy inthe hippocampus in vitro (McBain, 1994), as well as during paroxysmalevents in vivo (Steriade et al., 1994; Bragin et al., 1995, 1997;Steriade and Contreras, 1995). Moreover, in epileptic human mesialtemporal lobe tissue, the observation of synchronized synapticpotentials with similar reversal properties as observed in thepresent study has also led to the suggestion of concomitant activationof inhibitory and excitatory synaptic input (Schwartzkroin andKnowles, 1984).

The maintenance of the ictiform activity induced by CCh appeared selectively dependent on fast EAA neurotransmission, becauseit was only modulated by NMDA receptor antagonism but blockedby AMPA-receptor antagonism. This pharmacological profile is similarto that reported for CCh-induced rhythmic population oscillationsin the hippocampus (MacVicar and Tse, 1989). In the EC, however,small-amplitude, positive-going field events persisted in layerII during combined block of both AMPA and NMDA receptors. Theseevents occurred periodically and were correlated with gIPSPs inlayer II principal cells and abolished by GABA_A receptor antagonism.Recurrent gIPSPs in principal cells during EAA neurotransmissionblock have also been observed in the neocortical and hippocampalslice in the presence of 4-AP (Aram et al., 1991; Perrault andAvoli, 1992; Michelson and Wong, 1994). Also, recently, 4-AP applicationto EC slices has been shown to induce long-lasting depolarizationsin principal neurons that persisted during EAA neurotransmissionblock and were markedly depressed by GABA_A receptor antagonism(Lopantsev and Avoli, 1996). Furthermore, synchronized synapticpotentials observed in epileptic human mesial temporal lobe tissuewere also found to be dependent on fast GABAergic neurotransmission(Schwartzkroin and Haglund, 1986).

The mechanism of 4-AP-induced synchronization of inhibitory neurons in the hippocampus has been studied in detail by Michelsonand Wong (1994). These authors reported that in the presence of4-AP and during blockade of EAA neurotransmission, gIPSPs occurrhythmically in hippocampal principal cells. These gIPSPs wereinvariably triphasic in appearance, and PTX blocked the fast initialevent (GABA_A mediated) and left in isolation a slower monophasicevent (GABA_B mediated). These authors also concluded that hippocampalGABAergic interneurons may become synchronized via (1) recurrentinterneuron collaterals and the depolarizing action of synapticallyactivated GABA_A receptors and (2) electrotonic coupling. Similarmechanisms may also operate in EC (Buhl and Jones, 1993; Wouterloodet al., 1995). Even though the gIPSPs in EC layer II neurons werenot triphasic in appearance, they did demonstrate a fast risetime (~43 msec) compatible with GABA_A receptor activation (Michelsonand Wong, 1991) and a slow decay compatible with GABA_B receptoractivation. In addition, the early phase reversed at approximately $-$ 75 mV, whereas the slow late phase reversed ~10 mV more negative.

The fact that the gIPSPs in layer II neurons were correlated with the locally generated positive field events suggests thatthese events result from inhibitory synaptic currents in projectioncells. Because there was not always a perfect synchrony betweenthe field events and the gIPSPs (Fig. 10), and because field eventsrecorded at sites separated by distances greater than ~200 µmtended to be uncorrelated (Fig. 11), this suggests that these eventsarise from the synchronous activation of discrete, localized poolsof interneurons that innervate discrete, localized pools of principalcells (Freund and Buzsaki, 1996). Thus, inhibitory networks mayplay a fundamental role in the organization of population dynamics(Llinas et al., 1991; Cobb et al., 1995; Jefferys et al., 1996;Wang and Buzsaki, 1996) and functional domains within the EC.

FOOTNOTES

Received April 16, 1997; revised June 4, 1997; accepted June 10, 1997.

This work was supported by a grant from the Canadian Medical Research Council. Dr. Dickson was supported by a fellowship fromthe Natural Sciences and Engineering Council of Canada. Dr. Alonsois a Montreal Neurological Institute Killam Scholar

Correspondence should be addressed to Dr. A. Alonso, Department of Neurology and Neurosurgery, Montreal Neurological Instituteand McGill University, Montreal, Quebec, Canada H3A 2B4.

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Volume 17, Number 17, Issue of September 1, 1997 pp. 6729-6744 Copyright ©1997 Society for Neuroscience

Muscarinic Induction of Synchronous Population Activity in the Entorhinal Cortex

Volume 17, Number 17, Issue of September 1, 1997 pp. 6729-6744
Copyright ©1997 Society for Neuroscience