Giant Depolarizing Potentials: the Septal Pole of the Hippocampus Paces the Activity of the Developing Intact Septohippocampal Complex In Vitro

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The Journal of Neuroscience, August 15, 1998, 18(16):6349-6357

Giant Depolarizing Potentials: the Septal Pole of the Hippocampus Paces the Activity of the Developing Intact Septohippocampal Complex In Vitro
Xavier Leinekugel, Ilgam Khalilov, Yehezkel Ben-Ari, and Roustem Khazipov
Institut National de la Santé et de la Recherche Médicale, 75014 Paris, France

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In neonatal hippocampal slices, recurrent spontaneous giant depolarizing potentials (GDPs) provide neuronal synchronized firingand Ca²⁺ oscillations. To investigate the possible role of GDPs in thesynchronization of neuronal activity in intact neonatal limbicstructures, we used multiple simultaneous electrophysiologicalrecordings in the recently described preparation of intact neonatalseptohippocampal complex in vitro. Combined whole-cell (in singleor pairs of cells) and extracellular field recordings (one tofive simultaneous recording sites) from the CA3 hippocampal regionand various parts of the septum indicated that spontaneous GDPs,which can be initiated anywhere along the longitudinal hippocampalaxis, are most often initiated in the septal poles of hippocampusand propagate to medial septum and temporal poles of both hippocampisimultaneously. GDPs were abolished in the medial septum but notin the hippocampus after surgical separation of both structures,suggesting hippocampal origin of GDPs. The preferential septotemporalorientation of GDP propagation observed in the intact hippocampuswas associated with a corresponding gradient of GDP frequencyin isolated portions of hippocampus. Accordingly, most GDPs propagatedin the septotemporal direction in both septal and temporal hippocampalisolated halves, and whereas GDP frequency remained similar inthe septal part of hippocampus after its surgical isolation, itprogressively decreased in more temporally isolated portions ofthe hippocampus. Because GDPs provide most of the synaptic driveof neonatal neurons, they may modulate the development of neuronalconnections in the immature limbic system.

Key words: giant depolarizing potentials (GDPs); GABAergic network; synchronized neuronal activity; oscillations in neonates; rat; development; intact neonatal hippocampus and septum in vitro; electrophysiology

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Synchronized and propagating neuronal activities shape neuronal pathways during the early stages of development. Neuronalsynchronization during development can be provided by sensoryexperience, as well as by endogenous patterns of activity (O'Donovanet al., 1992; Yuste et al., 1992, 1995; Gu and Spitzer, 1995;Kandler and Katz, 1995; Feller et al., 1996; Ben-Ari et al., 1997),and participate in network formation by activity-dependent mechanisms(Constantine-Paton et al., 1990; Goodman and Shatz, 1993; Katzand Shatz, 1996). It is therefore of primary importance to describewhether and how spontaneous patterns coordinate the activity ofneurons inside and across intact developing neuronal structures.

Limbic structures form a functional complex in the adult and are implicated in memory processes and pathological disorders.Although physiological interactions and associated patterns ofactivity (theta rhythm, sharp waves) between septum and hippocampushave been extensively studied in the adult (for review, see Buzsakiand Chrobak, 1995; Freund and Buzsaki, 1996), little is knownabout the spontaneous patterns of activity present in these structuresat the early stages of development. Previous works in the rathippocampal slice preparations have shown that during the firstpostnatal week [postnatal days 0-5 (P0-P5)], the spontaneous neuronalactivity is characterized by network-driven giant depolarizingpotentials (GDPs) (Ben-Ari et al., 1989). In slices, GDPs providesynchronous neuronal activation and Ca²⁺ oscillations attributable to the cooperation of excitatory GABAergicand glutamatergic synaptic transmissions (Corradetti et al., 1988;Gaïarsa et al., 1990; Leinekugel et al., 1995, 1997a, 1998; Ben-Ariet al., 1997; Khazipov et al., 1997). Understanding the coordinationof neuronal activity in the intact neonatal septohippocampal systemis a major requirement for the study of activity-dependent processesimplicated in the formation of functional neuronal ensembles inthe limbic system. We presently investigated whether and how GDPscoordinate neuronal activity in the intact neonatal septohippocampalcomplex in vitro.

A major obstacle for the study of generation and propagation of organized neuronal activities in the brain is that they mayrequire intact neuronal networks. In vivo recordings, which preserveneuronal networks intact, do not offer the technical facilitiesof in vitro experiments, can hardly be made in neonates becauseof intrinsic difficulties, and the use of anesthetics may affectsynaptic transmission (Mooney et al., 1996). On the other hand,more complex in vitro preparation than slices in which the neuronalnetwork is damaged are clearly required to study the generationand propagation of synchronized neuronal activities. A successfuldevelopment was recently realized in the study of neuronal activitypropagation in the visual system: using a preparation includingthe intact retina and visual pathway to LGN slices from neonatalmice in vitro, Mooney et al. (1996) observed that spontaneouswaves of activity in the retina before the onset of vision propagatedto LGN, which could play a crucial role in the formation of functionaltransmission of subsequent visual information. We have shown recentlythat neuronal activity in neonatal rat intact limbic structures(including both hippocampi and septum functionally connected)could also be studied in vitro (Khalilov et al., 1997a,b; Leinekugelet al., 1997b). The use of multiple simultaneous patch-clamp andextracellular field recordings in this novel in vitro preparationenabled us to observe that GDPs provide synchronized neuronalactivity in the intact neonatal septohippocampal complex and supporta septotemporal orientation of hippocampal activity. Because GDPsprovide most of the synaptic drive of neonatal neurons, they maymodulate the development of neuronal connections in the immaturelimbic system.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Preparation of acute intact hippocampi. The intact septohippocampal complexes or intact hippocampal formations (IHFs) wereprepared as described previously (Khalilov et al., 1997a). Neonatalmale Wistar rats (age, P0-P6) were anesthetized by hypothermiaand decapitated. After decapitation, the brains were quickly removedand immersed for dissection in ice-cold (2-4°C) oxygenated standardartificial CSF (ACSF) composed of (in mM): 126 NaCl, 3.5 KCl,2.0 CaCl₂, 1.3 MgCl₂, 25 NaHCO₃, 1.2 NaH₂PO₄, and 11 glucose).After removing the cerebellum and the most frontal part of theneocortex by coronal sectioning, the complex including the twohippocampi and septum was gently isolated from surrounding structureswith two plastic spatulas. Great care was given to avoid damageof connections between structures. For a number of experiments,single IHFs were then isolated from the septohippocampal complex.The septohippocampal complex or the IHFs were then gently transferredto a beaker containing oxygenated ACSF and kept at room temperature(20-22°C) for at least 1-2 hr before use. They were then transferredto a fully submerged chamber, laid on a nylon mesh, fixed withentomological needles inserted to Sylgard, and superfused at arate of 10-12 ml/min with oxygenated ACSF (30-32°C). The preparationwas laid down on its internal side to allow direct access to theCA1 and CA3 regions.

Electrophysiological recordings. Electrophysiological recordings were performed using the patch-clamp technique in the whole-cellconfiguration (Blanton et al., 1989) with Axopatch 200 (Axon Instruments)patch-clamp amplifiers. Cells were patched blindly with 7-10 M $Omega$ microelectrodes containing one of the following (in mM): (1) 120Cs gluconate, 10 CsCl, 1 CaCl₂, 10 EGTA, 2 MgATP, and 10 HEPES;(2) 135 K gluconate, 2 MgCl₂, 0.1 CaCl₂, 2 Na2ATP, 1 EGTA, and10 HEPES; or (3) 140 CsCl, 1 CaCl₂, 10 EGTA, 10 HEPES, and 2 MgATP,pH 7.25; osmolarity, 270-280 mOsm. Lucifer yellow (0.2-0.4%) wasroutinely added to the pipette solution for post hoc morphologicalidentification.

Extracellular field potentials were recorded conventionally using glass micropipettes filled with ACSF (1-5 M $Omega$ ) and DAM80amplifiers (low filter, 1 Hz; high filter, 0.1 KHz; WPI). Electricalstimulations (0-80 V, 10-30 µsec) were provided by a bipolar electrodeplaced in the CA3 hippocampal region.

Data analysis. Spontaneous neuronal activity and stimulation-evoked responses were acquired on a digital audio tape recorder(Biologic) and loaded into an 80486 personal computer using ananalog-to-digital converter (TL1 DMA; Labmaster). Acquis (samplingrate, 1.3 KHz; Axon) and Axotape (sampling rate, 0.5 KHz; Axon)programs were used for the acquisition and analysis of evokedand spontaneous events, respectively.

Group measures were expressed as mean ± SEM. Statistical significance of differences between means was assessed with the Student'st test with the aid of the statistical software StatView SE+ Graphics(Abacus Concepts, Calabases, CA). The level of significance wasset at p < 0.05.

Drugs. Tetrodotoxin was purchased from Sigma (St. Louis, MO); bicuculline, CNQX, and APV were purchased from Tocris Neuramin;and Lucifer yellow was purchased from Molecular Probes (Eugene,OR).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Spontaneous synaptic activity in the limbic system of newborn rats was investigated using electrophysiological techniquescombining patch-clamp and extracellular field-potential recordingsin the in vitro preparation containing septum and both hippocampidissected from P0-P6 animals.

Synaptic activity of individual neurons in the intact septum and hippocampus is characterized by network-driven GDPs

Patch-clamp whole-cell recordings were performed blindly in the CA3 region of hippocampus and medial septum from 19 animals.The addition of Lucifer yellow in the internal solution allowedfor post hoc identification of the recorded neurons.

As in age-matched hippocampal slices, the spontaneous activity of hippocampal neurons (n = 104 cells from 22 hippocampi) wascharacterized by recurrent GDPs (Ben-Ari et al., 1989). GDPs arenetwork-driven events: (1) their amplitude, but not frequency,was modified by changing the membrane potential (Fig. 1A); (2)they were reversibly blocked by perfusion with high-Mg²⁺ (9 mM) external solution (data not shown); and (3) they wereevoked by electrical stimulation in an all-or-none manner, increasingstimulation intensity above threshold decreasing their latencywithout modifying their amplitude (Fig. 1B). GDPs in the intacthippocampus had features similar to those described in slices:(1) they were reversibly blocked by bath application of TTX (1µM) or the GABA_A and glutamate receptor antagonists bicuculline(10 µM), APV (50 µM), and CNQX (10 µM), respectively (data notshown), confirming that they are mediated by synaptic transmissionvia the activation of GABA_A and glutamate receptors (Ben-Ari etal., 1997; Khazipov et al., 1997; Leinekugel et al., 1997a); and(2) the reversal potential of the GDPs was highly dependent oninternal Cl (4.2 mM Cl, E_inv = $-$ 57 ± 2 mV; n = 17; 12 mM Cl, E_inv = $-$ 47 ± 2 mV; n = 4; and 142 mM Cl, E_inv = $-$ 2 ± 5 mV; n = 8), indicating that they were primarilymediated by GABA_A receptors (Fig. 1C).

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Figure 1. Spontaneous and evoked GDPs are present in neonatal hippocampal and medioseptal neurons of the intact septohippocampal complex in vitro. A, Whole-cell recording (voltage clamp) at two different membrane potentials (left, $-$ 40 mV; right, +20 mV) from a CA3 pyramidal cell. Note the presence of recurrent GDPs which amplitude, but not frequency, changed with membrane potential. B, GDPs evoked by electrical stimulations (arrow) in a CA3 pyramidal cell. Note that above threshold, increasing stimulation decreases GDP latency without affecting its amplitude. C-D, Whole-cell recordings with different internal Cl concentrations (top traces: left, Cl_i = 142 mM; right, Cl_i = 12 mM) and extracellular field recordings (bottom traces) of spontaneous GDPs in the CA3 region of hippocampus (C) and in the medial septum (D). GDPs were synchronized in individual neurons (w/c, whole cell) and in the local neuronal population (field, field recordings very close to whole-cell pipette). Note also that GDP amplitude strongly depends on internal Cl in neurons from both hippocampus and medial septum.

Interestingly, GDPs were present also in neurons from the medial septum with similar properties (n = 15) (Fig. 1D), suggestingthat they represent a common pattern of neuronal activity in developinginterconnected limbic structures. Because GDPs in hippocampaltransverse slices were shown to provide synchronous neuronal activity(Khazipov et al., 1997; Leinekugel et al., 1997a), we investigatedwhether neuronal activity among these developing limbic structureswas synchronized.

GDPs are locally synchronized events that propagate

As a first approach to study GDP synchronization, we combined whole-cell and extracellular field potential recordings at differentlocations in the intact hippocamposeptal complex. An extracellularelectrode was placed in the CA3 pyramidal region of hippocampusor in medial septum, and a nearby individual neuron was simultaneouslyrecorded in the whole-cell mode. As illustrated in Figure 1, Cand D, GDPs in individual cells were highly synchronized withlocal extracellular field potentials, suggesting that GDPs arelocally synchronized events (n = 6 whole-cell-field pairs in hippocampus;n = 8 whole-cell-field pairs in septum). Moreover, as illustratedin Figure 2, double patch-clamp recordings (n = 12 pairs) indicatedthat GDPs propagate from one hippocampus to the other: (1) GDPs,which are typically associated with a burst of one to five actionpotentials (Khazipov et al., 1997; Leinekugel et al., 1997a),were synchronous in CA3 neurons from both hippocampi (Fig. 2B-D);and (2) electrical stimulation in one hippocampus evoked the generationof ipsilateral and contralateral GDPs (Fig. 2E,F).

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Figure 2. GDPs are synchronous in neurons from ipsilateral and contralateral hippocampi. Spontaneous (B-D) and evoked (E-F) GDPs recorded in the whole-cell configuration from two CA3 pyramidal cells (A, one from each hippocampus). B-C, Simultaneous recording of two pyramidal cells in the cell-attached (cell 2) and whole-cell (cell 1) configurations. Note that bursts of action potentials occur in cell 2 during GDP in cell 1 (the first GDP of B is presented in an expanded time scale in C). D, Entry into whole-cell mode in cell 2 shows that GDPs are synchronous in both cells. E-F, GDPs evoked in the same two cells as in B-D by electrical stimulation (E: cell 1, whole-cell mode; cell 2, cell-attached mode; F: both cells in whole-cell mode). Note that electrical stimulation in the temporal extremity of one hippocampus generated GDP in both ipsilateral (cell 1) and contralateral (cell 2) hippocampi, whereas when spontaneous GDPs appeared simultaneously in both cells, the GDP evoked in the ipsilateral side preceded the contralateral GDP.

In keeping with these results, both spontaneous and evoked GDPs were highly synchronous in simultaneous whole-cell recordingsfrom pairs of individual neurons close to each other (n = 32 pairs).Spontaneous GDPs also appeared synchronously in pairs of neuronscomprising one neuron in each hippocampus at similar distancesfrom their respective septal poles (n = 12 pairs) (Fig. 2B-D).However, with recordings from distant cells along the septotemporalaxis, significant delays of up to 1 sec were systematically observed.In fact, whereas evoked GDPs appeared first in the cell closestto the stimulus location (in both single and bilateral hippocampi)(Fig. 2F), spontaneous GDPs appeared most often first in the cellclosest to the septal pole of hippocampus. These results suggestthat locally synchronized spontaneous GDPs initiate in the septalpoles of the hippocampus and then propagate toward the temporalpoles.

To directly address this question, simultaneous multiple field-potential recordings were used, allowing us to study the originand propagation of GDPs in the neonatal septohippocampal complex.

Spontaneous GDPs originate in the septal poles of hippocampus and propagate to temporal poles

Three to five extracellular electrodes for field recordings were placed in the CA3 region at various locations along the septotemporalaxis of one or both hippocampi. Each experiment consisted in therecording of 50-200 consecutive GDPs. As illustrated in Figure3, GDPs appeared synchronously in both hippocampi and propagatedfrom septal to temporal poles. In average of 28 experiments, 82± 3% of GDPs appeared in the most septal recording site and propagatedin the septotemporal direction, whereas 3 ± 2% appeared in themiddle of hippocampus and propagated in both septal and temporaldirections, 5 ± 2% appeared in the temporal pole and propagatedtoward the septal pole, 5 ± 1% appeared simultaneously in allrecording sites, and 5 ± 1% appeared in only one recording siteand did not propagate. These features were very similar when recordingswere obtained from two interconnected hippocampi (n = 13) (Fig.3) or in the isolated hippocampus (n = 15) (Fig. 4A). Most GDPsrecorded in one hippocampus also appeared in the contralateralone (84 ± 9%; n = 8). Although GDPs tended to appear first inthe left hippocampus, no significant leading behavior betweenleft versus right septal hippocampal poles was evidenced; 18 ±4% of GDPs appeared synchronously in both septal poles, 54 ± 9%appeared first in the left hippocampus, and 28 ± 9% appeared firstin the right hippocampus (n = 8; p = 0.2).

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Figure 3. Spontaneous GDPs propagate synchronously in both hippocampi from septal to temporal poles. Multiple extracellular field recordings from the CA3 region of the intact bilateral septohippocampal complex. A, Simultaneous extracellular field recordings at the four recording sites indicated in the top scheme. RH, right hippocampus; LH, left hippocampus. Note that most GDPs (field deflections, arrow) appeared quite simultaneously in the four recording sites, with few exceptions of GDPs that appeared in septal poles but not in temporal poles (asterisk a) or appeared locally in one hippocampal site but did not propagate (asterisk b). B-D, Simultaneous extracellular field recordings at the four recording sites indicated in the scheme (B). Corresponding electrophysiological traces (1-4) showing propagation of a GDP at a large time scale. Note that GDPs appeared first in the most septal recording site (1, dashed arrow) and propagated toward the most temporal recording site (4, dashed arrow). As illustrated in A, not all GDPs propagated to the temporal extremity or to the contralateral hippocampus. D, Summary of the percentage of GDP propagation from one hippocampus to its contralateral counterpart (H-H) and from the septal pole to the other recording sites in the same hippocampus (x-axis values correspond to normalized septotemporal distances as represented in B). Numbers above each bar indicate the corresponding number of averaged experiments. Note that a significant percentage of GDPs initiated in the septal pole faded away before reaching the temporal extremity.

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Figure 4. GDPs propagate in the septotemporal direction in isolated portions of hippocampus. Simultaneous recording of GDPs at different recording sites (1-4) in the intact (A), isolated septal (B), or temporal (C) halves of the hippocampus. Cross-correlograms for GDPs (y-axis, number of GDPs; x-axis, time, 100 msec bin) of different recording sites (septal pole, filled bars; temporal pole, open bars) are plotted below the corresponding traces. A, Cross-correlogram of GDPs in sites 1 (septal pole, filled bars), 3 (reference event, GDP in site 3), and 4 (temporal pole, open bars) in the intact hippocampus. B, Cross-correlogram of GDPs in sites 1 (septal pole) and 4 (reference event, GDP in site 4) in the septal half of hippocampus. C, Cross-correlogram of GDPs in sites 1 (reference event, GDP in site 1) and 4 (temporal pole) in the temporal half of hippocampus. Note the septotemporal propagation of GDPs in the intact hippocampus, as well as in the septal and temporal halves of the same hippocampus after they were surgically transsected.

Interestingly, a limited proportion of GDPs appeared in both septal poles but did not propagate until temporal extremities.Precise analysis indeed revealed that although almost all GDPs(97 ± 1%; n = 24 hippocampi) recorded in the most 10-25% septalpart propagated to the first half of hippocampus, an increasingnumber of them faded with distance along the temporal half. Asillustrated in Figure 3D, among GDPs recorded in the 10-25% mostseptal part of hippocampus, 85 ± 4% propagated to the rest 50-65%of hippocampus (n = 22 hippocampi), 77 ± 7% to the rest 65-80%of hippocampus (n=17), and 60 ± 8% reached the rest 80-90% ofhippocampus (n=12). Analysis of the delays of appearance of GDPsat these different locations indicated that this septotemporalpropagation occurred at a speed of 7.55 ± 2 mm/sec (n = 11 hippocampi).Although GDP propagation tended to slow down in the temporal part,no significant difference in speeds was observed as a functionof the portion of hippocampus (9.2 ± 2, 9.4 ± 2, 7.7 ± 1, and5 ± 2 mm/sec in the first 10-50, 50-65, 65-75, and 75-90% of hippocampusrespectively; n = 11 hippocampi; p > 0.7).

Therefore, in the intact septohippocampal complex in vitro, most of hippocampal GDPs appear in the septal poles and propagatebilaterally toward temporal extremities.

Septotemporal orientation of hippocampal activity

Taking advantage of the in vitro preparation, we investigated the behavior of surgically isolated parts of hippocampus toexamine whether the septotemporal pattern of GDP propagation isdetermined by particular differences between septal and temporalhippocampal poles or by a septotemporal gradient of activity alongthe longitudinal hippocampal axis. Removal of the septum (n =18 with hippocampus and septum together; n = 14 with hippocampusalone), separation of each hippocampus (n = 13 with both hippocampitogether; n = 12 with only one isolated intact hippocampus), andmore surprisingly, isolation of septal and temporal halves ofhippocampus (n = 11 experiments with recording from the same hippocampusbefore and after separation of septal from temporal halves) didnot affect the septotemporal pattern of propagation of GDPs (Fig.4), suggesting that it does not require the integrity of the septohippocampalcomplex. In the temporal half of hippocampus, 80 ± 9% of GDPsappeared in the most septal recording site and propagated in theseptotemporal direction, whereas 7 ± 7% appeared in the middleof the preparation and propagated in both septal and temporaldirections, 1 ± 1% appeared in the most temporal recording siteand propagated toward the septal pole, 2 ± 2% appeared simultaneouslyin all recording sites, and 9 ± 5% appeared in only one recordingsite and did not propagate. For the septal half, the correspondingvalues were 72 ± 12, 1 ± 2, 15 ± 8,12 ± 5, and 0%, respectively.

To test the hypothesis that the septal pole could drive the intact hippocampal network because of higher spontaneous activity,we compared the frequency of spontaneous GDPs in isolated portionsof hippocampus. In the experiment illustrated in Figure 5, measuringspontaneous activity before and after the cutting of hippocampusinto one-thirds revealed a real septotemporal gradient of GDPfrequency, the most septal third having similar GDP frequencyas the intact hippocampus, whereas this frequency decreased by30% and 80% in the middle and temporal thirds, respectively. Innine experiments in which GDP frequency was compared in septalversus temporal hippocampal halves, GDPs had a frequency of 10.9± 1 min¹ in the septal half and 8.9 ± 2 min¹ in the temporal half of intact hippocampus. After a knife cutwas made to isolate septal from temporal halves (n = 9), GDP frequencyremained unchanged in the septal part (11.4 ± 2 min¹) but decreased by two to four times in the temporal half (5.3± 1 min¹; p < 0.05) (Fig. 5D).

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Figure 5. Septotemporal gradient of GDP frequency in the hippocampus. GDP frequency in different portions of hippocampus (top, recording sites 1-3) was measured before (A) and after (B) their surgical transsection (top, dashed lines). Note that in addition to being desynchronized after surgical transsection (compare A, B), GDP frequency gradually decreased toward the temporal pole (compare traces 1-3 in B). C, Quantification of GDP frequency before (H) and after (1/3 S, most septal third; 1/3 m, middle third: 1/3 T, most temporal third) surgical transsection. D, Average GDP frequency (n = 9 hippocampi) in the septal and temporal halves before (1/2 S and 1/2 T, respectively) and after (1/2 S alone and 1/2 T alone, respectively) surgical transsection. Note that whereas surgical hemisection did not affect GDP frequency in the septal half, it decreased GDP frequency by two times in the temporal half.

A possible additional factor for the preferential septotemporal orientation of GDP propagation is derived from the observationthat spontaneous GDPs initiated in the septal poles had a higherrate of propagation to the rest of the hippocampus than spontaneousGDPs initiated in the temporal poles. From 17 experiments in whichboth types of GDPs were present, we observed that 75 ± 6% of GDPsinitiated in the septal pole propagated to the temporal pole,whereas 41 ± 9% of GDPs initiated in the temporal pole propagatedto the septal pole (data not shown; p < 0.01).

Therefore, septotemporal initiation and propagation of GDPs is supported by at least two factors: (1) GDPs occur more frequentlyin the septal than in the temporal pole; and (2) GDPs initiatedin the septal pole have a higher rate of propagation than GDPsinitiated in the temporal pole. It remains to be elucidated whetherthis septotemporal gradient is attributable to differences incell properties or to network organization, possibly in relationwith maturational differences.

GDPs in septum are driven by the activity of extrinsic hippocamposeptal projections

To examine the relationship between septal and hippocampal GDPs, we recorded simultaneously the synaptic activity from septaland hippocampal neurons. As illustrated in Figure 6A, most GDPs(92.5 ± 4%; n = 4) appearing in the septal pole of the hippocampusappeared also in the medial septum. In addition, GDPs typicallyappeared first in the hippocampus before appearing in the septum(Fig. 6A).

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Figure 6. GDPs in medial septum originate in the hippocampus. Extracellular field potentials were recorded simultaneously from the medial septum (top scheme, S) and from the CA3 hippocampal region (top scheme, H1, H2) before (A) and after (B) cutting the connections between hippocampus and septum (B, dashed line). In the septohippocampal complex (A), GDPs (arrows) were synchronized in the hippocampus and the medial septum. The GDP indicated by an asterisk in A is presented in the right top corner at expended time scale, showing that GDPs typically appeared first in the septal pole of hippocampus (H1) and propagated to the septum (S) and temporal pole of hippocampus (H2). After surgical separation of hippocampus and septum (B), GDPs (arrows) were still present in hippocampus (H2) but not in septum (S).

To know whether GDPs could be generated in septum independently from hippocampus, we recorded synaptic activity from septalneurons before and after section of hippocamposeptal connections(Fig. 6). Although GDPs were present in septum when functionallyconnected to hippocampus, surgical isolation by a knife cut betweenhippocampus and septum abolished GDPs in septum but not in hippocampus(n = 12) (Fig. 6B). These results suggest that septal GDPs originatein hippocampus and propagate to septum via hippocamposeptal-projectingneurons.

Together, these results suggest that the septal pole of the hippocampus paces the activity of the developing intact septohippocampalcomplex in vitro.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Spontaneous neuronal activity of the intact neonatal septohippocampal complex in vitro was studied using simultaneous multiplewhole-cell and extracellular field recordings. We found that spontaneousGDPs, initially described in hippocampal transverse slices (Ben-Ariet al., 1989), have particular spatiotemporal characteristicsof generation and propagation in the intact septohippocampal complex.Three principal conclusions can be drawn from the present results:(1) the neonatal hippocampal network is characterized by a septotemporalgradient of automaticity; spontaneous GDPs are present in isolatedtransverse portions of hippocampus, but the septal pole has thehighest rhythm of activity and drives the entire hippocampal network;(2) GDPs are synchronized in both hippocampi via commissural connections;and (3) in contrast to hippocampus, the septal network itselfdoes not generate GDPs. However, septal neurons undergo GDPs originatingin and propagating from hippocampus. Therefore, the spontaneousneuronal activity of the intact septohippocampal complex is tightlysynchronized during the first postnatal week of life, which mayhave major implications for the coordinated development of theneuronal ensembles in immature limbic structures.

Septotemporal orientation of hippocampal activity

Synchronized patterns of activity at the early stages of development were observed, primarily in the slice preparation, invarious structures (O'Donovan et al., 1992; Yuste et al., 1992,1995; Gu and Spitzer, 1995; Kandler and Katz, 1995; Feller etal., 1996; Mooney et al., 1996; Ben-Ari et al., 1997). The useof novel in vitro preparations such as the intact septohippocampalcomplex allows the study of the generation and propagation ofnetwork activities with similar technical facilities as in slices(Khalilov et al., 1997a,b; Leinekugel et al., 1997b). We recentlyshowed that this preparation was fully viable and actually allowedbetter tissue preservation than age-matched slices (Khalilov etal., 1997a). Patch-clamp whole-cell recordings allow us to drawthe conclusion that GDPs in the intact hippocampus have the sameprincipal features as in hippocampal slices: (1) they are mainlyGABAergic, because their reversal potential was primarily dependenton Cl gradient; and (2) they are locally synchronous, because theyappeared synchronously in pairs of nearby individual cells.

However, recording from pairs of distant cells along the septotemporal axis, we observed systematic delays of GDP occurrence.Combining simultaneous whole-cell and multiple extracellular field-potentialrecordings clearly indicated that in the intact hippocampus, andmore surprisingly also in isolated transverse portions of hippocampus,GDPs propagate in the septotemporal direction. These results suggestthat the neonatal hippocampus has a septotemporal gradient ofneuronal activity and/or a septotemporal orientation of neuronalprojections.

Although most GDPs are initiated in the septal pole, a significant number of them are initiated in the temporal pole and areable to propagate toward the septal pole. Moreover, GDPs beinginitiated in the middle of hippocampus propagate toward both poles.These observations suggest that the hypothesis of asymmetric longitudinalorientation of projections is unlikely to fully explain the preferentialseptotemporal orientation of GDP propagation.

Because GDPs are present in isolated portions of hippocampus at various septotemporal locations, including 500-µm-thick transversehippocampal slices and even minislices of CA3 subfield or fasciadentata (Khazipov et al., 1997), the neuronal elements requiredfor their generation are present already in local neuronal circuits.However, the present results indicate a higher frequency of GDPsin isolated septal parts of hippocampus compared with more temporalparts. Therefore, the neonatal hippocampal network has a septotemporalgradient of autorhythmicity, and the septal pole, being the mostactive, paces the rhythm of the entire structure. Further investigationsare required to examine whether this gradient is attributableto differences in cellular properties or in synaptic connectivityalong the septotemporal axis of hippocampus. Because GABAergicinterneurons play a major role in the generation of GDPs, an additionalpossibility is that an asymmetric longitudinal distribution ofsubclasses of GABAergic interneurons, as suggested in previousmorphological studies (Buzsaki et al., 1990), could be implicatedin the observed septotemporal gradient of GDPs frequency.

Synchronization of hippocamposeptal activity

Our present results indicate that in the intact septohippocampal complex in vitro, GDPs are synchronous in both hippocampiand medial septum. However, they were absent in the isolated septum.Therefore, only the use of a preparation that preserves hippocamposeptalconnections intact could allow the observation that GDPs representa common pattern of activity for hippocampal and septal neurons,which is one of the major findings of this work.

Septal GDPs have some similarities with hippocampal GDPs, including their synchronous occurrence in neurons and the main contributionof GABA_A receptors. However, the mechanisms of generation of GDPsin septum are different from in hippocampus. Although hippocampalGDPs can be generated in isolated portions of the hippocampalnetwork, the local septal neuronal network does not seem ableto generate GDPs. This may be attributable to the absence of glutamatergicrecurrent collaterals in the septum (Jakab and Leranth, 1995),which play an important role in synergy with GABAergic excitatoryconnections in the generation of hippocampal GDPs (Ben-Ari etal., 1997; Khazipov et al., 1997; Leinekugel et al., 1997a). Instead,septal GDPs result from the propagation of hippocampal GDPs viahippocamposeptal projections.

From previous morphological and electrophysiological studies (Freund and Antal, 1988; Buzsaki et al., 1992; Toth et al., 1993;Lee et al., 1994; Bragin et al., 1995; Buzsaki and Chrobak, 1995;Ylinen et al., 1995; Freund and Buzsaki, 1996; Toth et al., 1997),extensive GABAergic networks were proposed to play a key rolein the synchronization of limbic neurons in the adult hippocampus,septum, and entorhinal cortex, giving rise to spontaneous patternsof synchronized activities (theta rhythm, sharp waves). Severalmorphological studies using retrograde and anterograde labelingof hippocamposeptal and interhippocampal (commissural) neuronalprojections have already reported the presence of early GABAergicconnections (Crutcher, 1982; Milner et al., 1983; Linke and Frotscher,1993; Super and Soriano, 1994). The present results suggest thathippocamposeptal and commissural projections are already functionalat birth and support the view of a major role of the GABAergicnetwork in synchronizing activity of large neuronal ensembles,inside and across developing limbic structures.

Possible physiological implications of GDPs propagation

Previous works on hippocampal slices showed that GDPs were associated with synchronous Ca²⁺ oscillations mediated by voltage-dependent Ca²⁺ channels and NMDA receptors (Leinekugel et al., 1996, 1997a).Although the consequences of the Ca²⁺ influx during GDPs via voltage-gated Ca²⁺ channels and NMDA channels are presently unknown, activationof voltage-gated Ca²⁺ channels promotes neuronal differentiation in several preparations(Desarmenien and Spitzer, 1991; Gu and Spitzer, 1995; LoTurcoet al., 1995; Rusanescu et al., 1995), and localized Ca²⁺ influx through NMDA receptors can provide a hebbian modulationof developing synapses (Komatsu and Iwakiri, 1993; Crair and Malenka,1995; Fox, 1995; Kirkwood et al., 1995; Durand et al., 1996; Liaoand Manilow, 1996; McLean et al., 1996; Wu et al., 1996). It isnow generally accepted that the establishment and modulation ofsynaptic connections during development is at least partly dependenton the coordination between presynaptic and postsynaptic neuronalelements (Constantine-Paton et al., 1990; Goodman and Shatz, 1993;Katz and Shatz, 1996). It was shown recently that depending onthe precise timing of presynaptic and postsynaptic firing, eitherlong-term potentiation or long-term depression of synaptic transmissioncould be induced (Markram et al., 1997). Interestingly, GDPs providedhigh synchronization locally, but because of their slow speedof propagation, distant cells in the septotemporal hippocampalaxis have very significant delays of activation (up to 1 sec).According to the hebbian hypothesis "neurons that fire together,wire together" (Stent, 1973), local synchrony could serve as abasis for the formation of functional units inside large neuronalensembles. Existence of functional units in the septohippocampalsystem was recently suggested from morphological studies indicatingthat distinct groups of cells, depending on their positions alongthe longitudinal axis of hippocampus, project to distinct specificareas of septum (Risold and Swanson, 1996). One may thereforeassume that GDPs, by differentially regulating synaptic efficacybetween neurons depending on their septotemporal distance, maydrive the formation of functional units in the septohippocampalcomplex.

Although the intact septohippocampal preparation in vitro allows us to characterize the neuronal activity in intact structures,further studies are needed to examine whether similar spatiotemporalcharacteristics of spontaneous activity are present in the neonatallimbic system in vivo.

  FOOTNOTES

Received March 3, 1998; revised June 8, 1998; accepted June 9, 1998.

This work was funded by Institut National de la Santé et de la Recherche Médicale (I.K.), Ministere de l'Education Nationale,and Foundation pour la Recherche Medicale (X.L.). We thank Dr.V. Dzhala for useful comments and discussions, Dr. M. Esclapezfor help in morphological analysis, and S. Weiller for technicalassistance.
Correspondence should be addressed to Xavier Leinekugel, Institut National de la Santé et de la Recherche Médicale U.29,23, Boulevard de Port Royal, 75014 Paris, France. E-mail: leinekugel{at}cochin.inserm.fr

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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