Somatostatin Depresses Long-Term Potentiation and Ca2+ Signaling in Mouse Dentate Gyrus

doi:10.1152/jn.00398.2002

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Somatostatin Depresses Long-Term Potentiation and Ca²⁺ Signaling in Mouse Dentate Gyrus

Michael V. Baratta, Tyra Lamp, and Melanie K. Tallent

Department of Neuropharmacology, The Scripps Research Institute La Jolla, California 92037

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Baratta, Michael V., Tyra Lamp, and Melanie K. Tallent. Somatostatin Depresses Long-Term Potentiation and Ca²⁺ Signaling in Mouse Dentate Gyrus. J. Neurophysiol. 88: 3078-3086, 2002. The selective loss of somatostatin (SST)-containing interneurons from the hilus of the dentate gyrus is a hallmark of epileptichippocampus. The functional consequence of this loss, includingits contribution to postseizure hyperexcitability, remains unclear.We address this issue by characterizing the actions of SST inmouse dentate gyrus using electrophysiological techniques. Althoughthe majority of dentate SST receptors are located in the outermolecular layer adjacent to lateral perforant path (LPP) synapses,we found no consistent action of SST on standard synaptic responsesgenerated at these synapses. However, when SST was present duringapplication of high-frequency trains that normally generate long-termpotentiation (LTP), the induction of LTP was impaired. SST didnot alter the maintenance of LTP when applied after its induction.To examine the mechanism by which SST inhibits LTP, we recordedfrom dentate granule cells and examined the actions of this neuropeptideon synaptic transmission and postsynaptic currents. Unlike findingsin the CA1 hippocampus, we observed no postsynaptic actions onK⁺ currents. Instead, SST inhibited Ca²⁺/Ba²⁺ spikes evoked by depolarization. This inhibition was dependenton N-type Ca²⁺currents. Blocking these currents also blocked LTP, suggestinga mechanism through which SST may inhibit LTP. Our results indicatethat SST reduction of dendritic Ca²⁺ through N-type Ca²⁺ channels may contribute to modulation of synaptic plasticityat LPP synapses. Therefore the loss of SST function postseizurecould result in abnormal synaptic potentiation that contributestoepileptogenesis.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

A consistent finding in postseizure hippocampus, in both tissue removed from humans with epilepsy and in animal models, isthe highly selective loss of somatostatin (SST)-containing interneuronsin the hilus of the dentate gyrus (de Lanerolle et al. 1989; Robbinset al. 1991; Sloviter 1987). These are GABAergic neurons withprojections and inputs that have been characterized in detail.These neurons receive input from both mossy fiber collateralsof dentate granule cells and from perforant path (Leranth et al.1990) and project in a highly defined pattern to distal dendritesof granule cells in the outer molecular layer (Milner and Bacon1989). The SST-containing interneurons appear to form synapseson spines adjacent to perforant path synapses, thus they are criticallylocalized to regulate the major input into the dentate from entorhinalcortex. SST terminals are found in the hilus as well (Leranthet al. 1990; Milner and Bacon 1989). Based on these anatomicalconsiderations, it has been speculated that SSTergic interneuronsmediate feedback inhibition in the dentate. However, the deathof these neurons failed to be correlated with any deficit in feedbackinhibition in animal models of epilepsy (Buckmaster and Dudek1997). Thus it remains unclear how loss of somatostatinergic neuronscontributes to the pathophysiology of seizure-induced hyperexcitabilityin thedentate.

Intracerebroventricular and intrahippocampal injections of SST and SST analogs have been shown to modulate seizure activityin animal models. Although some early studies suggested that SSThad augmenting actions on seizures (Higuchi et al. 1983; Perlinet al. 1987), more recent studies, including those in which SSTwas directly injected into hippocampus, have revealed robust inhibitoryactions on behavioral and electrical seizures recorded in vivo(Perez et al. 1995; Vezzani et al. 1991, 2000). At the cellularlevel, SST also has inhibitory effects in CA1 and CA3 regionsof the hippocampus in vitro. In CA1, SST activates postsynapticK⁺ currents in pyramidal neurons (Moore et al. 1988; Schweitzeret al. 1998) to hyperpolarize neurons away from their thresholdfor firing. SST inhibits glutamatergic excitatory postsynapticcurrents (EPSCs) at CA1 Schaeffer collateral synapses, while notaffecting GABAergic inhibitory postsynaptic currents (Boehm andBetz 1997; Tallent and Siggins 1997). In CA3, SST inhibits EPSCsgenerated at associational/commissural synapses while not affectingmossy fiber EPSCs (Tallent and Siggins 1999). Using in vitro seizuremodels, we showed that SST inhibits epileptiform bursting andevoked afterdischarges in both CA1 and CA3 (Tallent and Siggins1999).

Thus, although the actions of SST have been characterized in CA1 and CA3 hippocampus, its actions in dentate remain unknown.We therefore chose to examine the actions of SST in the dentateof the mouse using electrophysiological methods, with the goalof addressing the functional consequence of the loss of SST functionin epileptic hippocampus. Although much of the previous work onSST actions in hippocampus was done in rat, we chose to use themouse as a model, with the future goal of studying SST actionsin transgenic/knockout mice. Some of the data presented here havebeen published in abstract form (Tallent et al. 1999, 2000).

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

All mouse experiments were performed in accordance with institute and National Institutes of Health guidelines on the careand use of laboratory animals. We similarly prepared hippocampalslices to our previous description for rat (Pittman and Siggins1981; Schweitzer et al. 1993), with some modifications. Briefly,male mice (5-10 wk) were anesthetized with halothane (4%) anddecapitated, and the brains rapidly removed and placed in ice-coldartificial cerebrospinal fluid (ACSF), gassed with 95% O₂-5% CO₂(carbogen), of the following composition (in mM): 130 NaCl, 3.5KCl, 1.25 NaH₂PO₄, 1.5 MgSO₄ · 7H₂O, 2 CaCl₂ · 2H₂O, 24 NaHCO₃,and 10 glucose. We cut horizontal brain slices (400 µM) usinga Campden vibraslicer or a Vibratome Series 3000 (Technical ProductsInternational, St. Louis, MO). Hippocampal formations and adjacententorhinal cortex were dissected from the slices and incubatedin the recording chamber for 20 min with their upper surfacesexposed to warmed, humidified carbogen. The slices were submergedand continuously superfused with warm (31°C), gassed ACSF at aconstant rate (2-3 ml/min) for the remainder of the experiment.The inner chamber had a total volume of 1 ml; at the superfusionrates used, 90% replacement of the chamber solution could be obtainedwithin 1-1.5 min. Drugs and peptides were added to the bath fromstock solutions at known concentrations. We obtained SST fromBachem (Torrance, CA) or Anaspec (San Jose, CA). D-2-amino-phosphonovalericacid (APV) and 6-cyano-7-nitroquinoxaline-2,3-dione disodium (CNQX)were purchased from Tocris (St. Louis, MO) and $omega$ -conotoxin GVIAfrom Anaspec. All other chemicals were from Sigma (St. Louis,MO).

Extracellular recording

We acquired data with an Axoclamp 2A or 2B amplifier (Axon Instruments) by D/A sampling using pCLAMP acquisition software(Axon Instruments). Extracellular field EPSPs (fEPSPs) were recordedin the outer one-third of the molecular layer (OML) of the innerblade of the dentate using a glass micropipette filled with 3M NaCl. We evoked lateral perforant path (LPP) synaptic responsesat 0.033 Hz with a bipolar tungsten stimulating electrode placednear the apex of the dentate in the OML. To confirm that we wererecording LPP EPSPs, we examined paired-pulse modulation of fEPSPsusing an interstimulus interval of 15-30 ms. Only responses thatshowed facilitation were considered LPP mediated and used in thisstudy (McNaughton 1980). Stability of baseline fEPSPs was establishedby stimulating at 30-50% maximal field amplitude for 20-30 minprior to beginning experiments. We generated input-output curvesby stimulating at three different stimulus intensities (thresholdfor generating a fEPSP, half-maximal, and maximal). Stimulus intensityranged between 50 and 500 µA.

We generated LTP with two high-frequency trains (HFTs) of 1 s each at 100 Hz, 20 s apart, using the maximal stimulus intensity.Test responses at 30-50% of maximal amplitudes were recorded for10-15 min prior to and 60 min following trains. The mean initialslopes (between the 0 and 50% points on the rising phase) of twoto four averaged fEPSPs were compared between the slice groupsover the 60 min following LTP generation. To study effect on LTPinduction, SST (0.2 or 1 µM) was added to the bath 7 min priorto, and washed out 1 min following, HFTs. For studies of LTP maintenance,SST was applied 30-45 min following HFTs. To control for variabilityin amount of potentiation between electrophysiological setupsand over time, control experiments were always performed on thesame setup and during the same week as thedrug.

Pharmacologically isolated N-methyl-D-aspartate (NMDA) receptor-mediated fEPSPs were generated as above, except in the presenceof 20 µM CNQX and with Mg²⁺ removed from the ACSF. The stimulus intensity required for generatingthese fEPSPs was generally around 10 times that required for generatingnormal fEPSPs (0.5-5 mA). Under these recording conditions, hyperexcitableevoked afterdischarges or "bursts" are generated that can be difficultto analyze using measures of slope, amplitude, or area. Therefore,to quantify the SST effect, we used a measure of burst intensitycalled coastline burst index (CBI). This is a measure of the "outline"of the burst waveform that is determined by summing the distancebetween successive points in the digitized burst (Korn et al.1987; Tallent and Siggins 1999).

Intracellular recording

We used discontinuous single-electrode voltage-clamp (switching frequency 3-4 kHz) or current-clamp techniques with sharpintracellular micropipettes (3 M KCl, 60-80 M $Omega$ ) as described previously(Madamba et al. 1999; Tallent and Siggins 1997). Sustained postsynapticcurrents were measured in TTX from a holding potential near $-$ 70mV by 1-s voltage steps from $-$ 120 to $-$ 40 in 10-mVincrements.

To measure Ca²⁺ spikes, we recorded intracellularly in current-clamp in the presence of 1-2 µM TTX, 300-600 µM Ba²⁺ and 1 mM tetraethlyammonium. Ca²⁺ spikes were elicited with a series of 1-s depolarizing currentsteps (50- to 100-pA increments) from a holding potential near $-$ 60 mV and were sensitive to 500 µM Cd²⁺ (Fig. 5).

Whole-cell patch clamp

We performed the "blind" version of whole-cell patch-clamp technique as previously described (Tallent et al. 2001). Patchsolution contained (in mM) 130 K-gluconate, 7 KCl, 10 HEPES, 2MgCl₂, 0.5 EGTA, 5 ATP, 1 GTP (the latter two were added freshon the day of the recording). We pulled patch electrodes on aFlaming/Brown puller from borosilicate glass (input resistanceof 2-3 M $Omega$ when filled). The junction potential was nulled withamplifier circuitry (Axopatch 200B, AxonInstruments).

Statistics

We used ANOVA with or without repeated measures using CRUNCH software (CRUNCH Software Corporation) or EXCEL (Microsoft) todetermine statistical significance at P < 0.05. For LTP, we measureddifferences across the last 15 min of trials (45-60 min post HFTs).For posttetanic potentiation, we analyzed 1-5 min following thetrains.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

SST does not inhibit LPP fEPSPs

When LPP EPSPs were evoked by a single test stimulus, 1 µM SST did not consistently alter the amplitude or area of the event.In three of seven slices we saw a moderate inhibition of <15%.The overall effect of SST on fEPSPs recorded at different stimulusstrengths was not statistically significant (P > 0.1; n = 7),although there is a trend toward a decrease at the lowest stimulusintensity (Fig. 1A). Application of SST did not alter paired-pulsefacilitation of fEPSPs tested at interstimulus intervals rangingfrom 15 to 100 ms. Shown in Fig. 1B, left, are representativepairs of fEPSPs generated at 50-ms intervals using a half-maximalstimulus intensity. SST (1 µM) superfusion did not alter the degreeof facilitation. Mean data from seven slices is shown in Fig.1B, right. No significant effect on facilitation of fEPSP initialslope is observed at any of the interstimulus intervals (P > 0.5).A lower concentration of SST (0.2 µM) also did not significantlyaffect fEPSP slope or amplitude (n = 12, see Fig. 2A baseline).

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Fig. 1. Somatostatin (SST) does not affect field excitatory postsynaptic potentials (fEPSPs) recorded at LPP synapses. A: Left: representative fEPSPs recorded in the outer molecular layer generated with a half-maximal stimulus intensity. Addition of 1 µM SST does not change the fEPSP amplitude or shape. Stimulus artifacts in this and subsequent figures are blanked by amplifier circuitry. Right: mean data showing no effect of SST on fEPSPs generated at three different stimulus intensities. B: Left: voltage records showing response to pairs of half-maximal stimuli with a 50-ms interstimulus interval. SST (1 µM) does not affect the first fEPSP nor does it alter paired-pulse facilitation. Right: mean data from 7 cells showing no effect of SST on paired-pulse facilitation of fEPSPs generated at half-maximal intensity using various interstimulus intervals. Data plotted as ratio of initial slope of the 2^nd fEPSP/1^st fEPSP (S2/S1).

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Fig. 2. SST depresses induction but not maintenance of long-term potentiation at lateral perforant path synapses. Left: initial fEPSP slope is plotted over time. When applied for 8 min beginning 7 min prior to high-frequency trains, SST (200 nM) blocks the stabilization of long-term potentiation (LTP) (n = 15 and 12 for control and SST, respectively). Trains consist of two 100-Hz stimuli for 1 s, given 20 s apart. Closed bar indicates time of SST application. Inset: representative fEPSPs for control experiment show potentiation 60 min following trains. When SST was present during induction phase, no potentiation is seen 60 min following the trains. Right: after LTP is induced, superfusion of 200 nM SST for 15 min does not alter the maintenance phase (n = 7). Inset: fEPSPs from a representative experiment showing LTP is preserved following superfusion of SST 30-45 min following trains.

SST inhibits induction/stabilization but not maintenance of LTP

When 200 nM SST was applied 7-8 min prior to application of LTP-generating trains of stimuli, posttetanic potentiation inthe first 5 min following the trains was unchanged (P > 0.05)but LTP was depressed (P < 0.001; n = 12). Instead of the normaldecay to a plateau level within the first 15 min seen in controlslices (Fig. 2, left; n = 15), when SST was applied during theinduction phase, the fEPSPs never attained a stable potentiatedlevel and instead slowly decayed back to baseline levels. By 32min following HFTs, the fEPSPslope was 104 ± 7.9% of baseline.By 8 min following HFTs, the fEPSP slope from slices where SSThad been applied and washed out was significantly less than incontrol slices. A higher concentration of SST produced less consistentresponses. LTP was blocked (<110% of baseline 60 min followingHFTs) in 6 of 12 slices exposed to 1 µM SST prior to HFTs. However,in all 12 slices there was not a significant effect overall (notshown). In the 6 slices in which LTP was reduced, this concentrationof SST also significantly reduced posttetanic potentiation inthe first 5 min following the train (notshown).

To examine the action of SST on maintenance of LTP, we established LTP in control ACSF and superfused 200 nM SST from 30 to45 min following HFTs. After LTP was established, superfusionof SST did not affect its maintenance (Fig. 2, right; n = 7).Prior to beginning SST application 30 min following HFTs, fEPSPslopes were 146 ± 4% of baseline. At the end of the SST superfusion(45 min post-HFTs), fEPSP slopes were 143 ± 9% of baseline, and,at 60 min post-HFTs, fEPSP slope was 147 ± 8% of baseline. ThusSST did not cause a decrement of the fEPSP slope after LTP hadstabilized.

Since SST did not appear to inhibit LPP fEPSPs, we further examined the mechanism by which SST blocked stabilization of LTP.Since LTP at this pathway is NMDA receptor dependent, we examinedwhether SST could block isolated NMDA receptor-mediated fEPSPs.To isolate NMDA receptor-mediated responses, we superfused 30µM CNQX to block AMPA/kainate glutamate receptors and removedMg²⁺ from the ACSF to unmask NMDA receptor responses. We evoked fEPSPsas described above by stimulating the LPP. Since under these recordingconditions hyperexcited fEPSPs were generated, we analyzed SSTeffects on evoked burst intensity using CBI (see METHODS). SSTsignificantly reduced burst intensity (Fig. 3A). However, whenwe recorded pharmacologically isolated NMDA EPSCs using whole-cellpatch-clamp, we found no effect of SST (Fig. 3B, n = 4). Theseresults suggest that SST may not be acting directly on NMDA receptor-mediatedresponses and could instead be acting on underlying voltage-sensitiveconductances activated during NMDA receptor-mediated depolarizations.

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Fig. 3. SST moderately depresses pharmacologically isolated N-methyl-D-aspartate (NMDA) fEPSPs but not voltage-clamped NMDA EPSCs. A: Left: NMDA fEPSPs recorded in outer molecular layer in 6-cyano-7-nitroquinoxaline-2,3-dione disodium (CNQX, 30 µM) and Mg²⁺-free artificial cerebrospinal fluid at threshold, half-maximal, and maximal stimulus intensities. SST (1 µM) moderately depresses the fEPSPs in a reversible manner. Right: mean effect of SST on NMDA fEPSP quantified using coastline burst index (CBI). Addition of 250 nM $omega$ -conotoxin 25-30 min prior to SST effectively blocks the effect of the peptide. B: Left: representative NMDA EPSCs recorded from dentate granule cells using whole-cell voltage-clamp. SST does not affect the EPSCs. Right: mean data showing no significant effect of SST on NMDA EPSC amplitude at three different stimulus intensities (n = 4).

SST does not act on sustained postsynaptic currents in dentate granule cells

To determine whether SST could reduce postsynaptic excitability by augmenting noninactivating K⁺ currents, as in CA1 hippocampus, we used intracellular voltage-clamptechniques to analyze SST actions on postsynaptic currents. Inthe presence of TTX, we evoked currents by stepping the membranepotential from about $-$ 70 mV to a range of voltages from $-$ 120 to $-$ 40 mV. We found that SST (1 µM) had no significant action oncurrents active in this voltage range (Fig. 4; n = 5). In threeneurons voltage clamped using whole-cell patch-clamp, SST alsodid not affect postsynaptic currents (not shown).

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Fig. 4. SST does not alter postsynaptic conductances recorded in dentate granule cells. A: current responses to voltage steps recorded using intracellular discontinuous voltage-clamp. SST (1 µM) does not affect the sustained currents. Some current and voltage steps were removed for clarity. B: mean current-voltage curves for 5 neurons before, during, and after bath superfusion of 1 µM SST. C: current-clamp recording from a dentate granule cell. SST (1 µM) does not alter the voltage response to current injections or the firing properties of this dentate granule cell.

SST depresses Ca²⁺ spikes in dentate granule cells

Because of difficulty in recording Ca²⁺ currents in the slice preparation and the unsuitability of our studies to use of acutelyisolated neurons (see DISCUSSION) to determine possible actionsof SST on Ca²⁺ conductances we examined Ca²⁺/Ba²⁺ spikes evoked by depolarizing current steps and recorded in current-clampin 1-2 µM TTX, 300-600 µM Ba²⁺, and 1 mM TEA. These spikes were sensitive to superfusion of500 µM Cd²⁺ (Fig. 5C). We found that Ca²⁺ spikes were inhibited by 0.2 to 1 µM SST. In seven neurons tested,1 µM SST reduced the number of spikes generated at a given membranepotential. SST inhibited the number of spikes evoked by depolarizingthe neuron to between $-$ 45 and $-$ 40 mV from 2.1 ± 0.4 to 0.9 ± 0.3(P < 0.05), representing a reduction of 57%. This action was reversibleon washout in five neurons. In most neurons, SST blocked spikingat current injection amplitudes just above threshold and reducedthe number of spikes per step with increasing depolarization.Unlike its effect on LTP, 1 µM SST was more potent than 200 nMin reducing the number of spikes (n = 5), with only a 35 ± 18%reduction in firing rate during a depolarization between $-$ 45 and $-$ 40 mV with the lower concentration. To determine whether SSTwas acting directly on a Ca²⁺ current, we tested whether subtype-selective Ca²⁺ channel antagonists could block SST inhibition of spikes. Ca²⁺ spikes could still be generated in the presence of L-, T-, andN-type channel blockers (Fig. 5A). SST (1 µM) inhibited Ca²⁺ spikes in the presence of 10 µM nifedipine (L-type blocker; n= 6; Fig 5A) and 50 µM nickel (T-type blocker; n = 6; Fig. 5B).Multiple spikes could not be evoked in the presence of nifedipine(Fig. 5A). When SST was added 20-25 min after addition of 250nM $omega$ -conotoxin GVIA to block N-type Ca²⁺ channels, no inhibition by SST was observed (Fig. 5C; n = 6).These data suggest that SST is acting on N-type Ca²⁺ channels to depress Ca²⁺ spikes.

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Fig. 5. Ca²⁺ spikes recorded from dentate granule cells. A: when slices were previously treated with the L-type channel blocker nifedipine (10 µM) for 20 min, SST (1 µM) still depressed Ca²⁺ spikes. B: in the presence of 50 µM nickel, SST (1 µM) was able to inhibit Ca²⁺ spikes. C: no inhibition of Ca²⁺ spikes by SST was seen in the presence of 250 nM $omega$ -conotoxin. D: LTP expression is reduced when 250 nM $omega$ -conotoxin is applied beginning 20 min prior to trains (n = 7). When 20 µM D-2-amino-phosphonovaleric acid (APV) is applied beginning 20 min prior to trains, no LTP is generated (n = 3).

We next examined whether N-type Ca²⁺ channels contributed to the generation of LPP LTP. $omega$ -Conotoxin (250 nM) significantly reducedthe size of the fEPSP, consistent with the presynaptic role ofN-type Ca²⁺ channels in mediating neurotransmitter release (Luebke et al.1993; Takahashi and Momiyama 1993). When $omega$ -conotoxin was applied20 min prior to HFS, LTP was significantly reduced, even whenstimulus strengths were normalized to generate 30-50% of maximalresponses (Fig. 5D; n = 7). These results suggest that influxof Ca²⁺ through N-type Ca²⁺ channels contributes to LTP at LPP synapses. To verify that ourstimulus paradigm evoked an LTP that was dependent on activationof NMDA receptors, as has previously been reported for this synapse(Colino and Malenka 1993; Xie and Lewis 1995), we superfused 30µM APV prior to application of trains. No LTP was generated inthese three slices (Fig. 5D), confirming our protocol inducesNMDA receptor-dependent LTP. We also tested whether $omega$ -conotoxincould block the SST inhibition of the NMDA fEPSP, since this didnot appear to be a direct effect on NMDA receptors (see DISCUSSION).The SST effect was largely blocked when 250 nM $omega$ -conotoxin wasapplied 25-30 min prior to superfusion of SST (Fig. 3A; n = 6,P < 0.005).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We show here that SST blocks induction of LPP LTP when applied prior to and during LTP-generating HFTs. SST does not affectLTP after its establishment and does not have apparent directeffects on standard synaptic responses recorded extracellularlyor intracellularly. These results suggest that SST is not likelyacting presynaptically to inhibit glutamate release. SST bindingis dense in the outer molecular layer, and SST receptors appearto be expressed on distal dendrites of dentate granule cells andnot presynaptically on LPP terminals (Schindler et al. 1997).Therefore SST is likely acting at a postsynaptic site to affectsynapticpotentiation.

Previous studies have suggested that SST facilitates LTP at some synapses in the hippocampus. An in vitro study in guineapig demonstrated that SST augmented mossy fiber LTP in CA3 neurons(Matsuoka et al. 1991). In dentate, a previous in vivo study inrat suggested facilitation by SST of medial perforant path LTP(Nakata et al. 1996). Thus SST may have different effects at differenthippocampal synapses; however, species differences cannot be ruledout. Our previous studies in rat have demonstrated only inhibitoryactions of SST in CA1 and CA3 at the cellular and network level(Tallent and Siggins 1997, 1999). Likewise, most in vivo studiesin rat suggest that SST reduces hyperexcitability in hippocampus(Perez et al. 1995; Vezzani et al. 1991, 2000).

The localization of SST receptors on distal dendrites of dentate granule cells makes it technically difficult to determinethe action of SST in these neurons using intracellular recordingtechniques. It is possible that changes in cellular propertiesinduced by SST in distal dendrites would not be reflected at thecell soma, where recording electrodes are located. Likewise, voltageclamping in the soma is unlikely to extend to distal dendrites(Spruston et al. 1993), thus it is difficult to determine current-voltageproperties in these regions. Techniques typically used to minimizesuch space-clamp problems, such as studying acutely dissociateddentate granule cells, are not appropriate in our studies, becauseof the localization of SST receptors in distal dendrites, whichare not preserved in this preparation. Future studies will addressthese issues by directly recording from distaldendrites.

We found no postsynaptic action of SST on K⁺ currents nor did we detect any hyperpolarizing action of SST on dentate granulecells. This is in contrast to previously reported actions of SSTin CA1 and CA3 hippocampus (Moore et al. 1988; Pittman and Siggins1981; Schweitzer et al. 1998; Tallent and Siggins 1999). We alsopreviously showed that SST inhibits excitatory neurotransmissionin CA1 and CA3 pyramidal neurons. NMDA and AMPA/KA-mediated EPSCsrecorded at both Schaeffer collatoral/CA1 synapses and associational/commissuralCA3 synapses are inhibited by SST (Tallent and Siggins 1997, 1999).These actions of SST are likely presynaptic, as corroborated bya study in cultured hippocampal pyramidal neurons showing SSTinhibited glutamate but not GABA release (Boehm and Betz 1997).In contrast, we detected no presynaptic action of SST at LPP/dentategranulesynapses.

It is possible that differences between hippocampal regions are due to distinct localization of SST receptors in each region.In CA1 and CA3, SST receptors are located in stratum radiatumand to a lesser extent in the stratum pyramidale (Leroux et al.1993). Thus SST actions recorded at the soma are likely to beless "filtered" by the cable properties of the dendrites thanresponses recorded in dentate granule cells, where SST receptorexpression occurs mostly in the distal dendrites. Also, the patternof expression of SST receptor subtypes may be different betweenthese regions. Immunohistochemistry studies in rat indicate thatSST₁ density is greater in dentate than CA1 (Hervieu and Emson1998), whereas SST₄ expression is similar in both regions (Schreffet al. 2000). SST₂ expression was shown by one group to be greaterin CA1 than dentate (Dournaud et al. 1996), whereas another groupusing a different antibody reported a higher density in dentate(Schindler et al. 1997). SST₃ immunohistochemistry has not yetbeen reported, although in rat its mRNA is expressed in both CA1and dentate (Kaupmann et al. 1993; Thoss et al. 1995). Each ofthese receptors may couple to a distinct repertoire of effectors(Schonbrunn 1999); however, the actions of these different receptorsubtypes in central neurons are not well characterized (Csabaand Dournaud 2001).

Immunohistochemical localization of SST receptors has not been reported for mouse, although in situ hybridization demonstratedhigh levels of mRNA expression for SST_1-4 in mouse dentategranule cells (Jinno and Kosaka 2000). In rat, most immunohistochemistrystudies have confirmed postsynaptic expression of receptors indentate, especially on dentate granule cell dendrites. SST₁ proteinis localized largely in the granule cell layers on cell somas(Hervieu and Emson 1998). For SST_2a one group reported dense expressionon granule cell dendrites (Schindler et al. 1997), while anothergroup using a different antibody reported presynaptic localization(Dournaud et al. 1996). SST_2b is localized postsynaptically ondendrites of dentate granule cells (Schindler et al. 1999). SST₄is also expressed on dendrites of dentate granule cells, as wellas on processes of SSTergic interneurons in the hilus (Schreffet al. 2000). These anatomical observations therefore supportour findings of a postsynaptic action for SST in dentate, althoughthe current study does not address receptor subtypespecificity.

Interestingly, in rats but not mice (Buckmaster et al. 1994; Jinno and Kosaka 2000), the outer molecular layer is denselyinnervated by terminals of SSTergic interneurons. Thus in micethere may be a mismatch between the location of peptide and receptors.Such a mismatch is not uncommon for peptides and their receptors(see for example Schindler et al. 1999) and suggests that peptidesmay diffuse away from their site of release and exert effectson distal targets (Elde et al. 1995). Also, there is increasingevidence that peptides are released extrasynaptically; for example,dendritic release of dynorphin has been reported in dentate gyrus(Simmons et al. 1995).

SST effects on LTP were more consistent at 0.2 than 1 µM, although in slices in which the higher concentration was effectiveits action was more robust, reducing both posttetanic potentiationas well as LTP. This difference could be due to desensitizationof SST receptors at the higher concentration. However, in CA1and CA3, 1 µM SST produces maximal effects on regulating bothpostsynaptic K⁺ currents and EPSCs (Tallent and Siggins 1997, 1999). Also, indentate, SST has a greater action on Ca²⁺ spikes at 1 than at 0.2 µM, and this action of SST did not rapidlydesensitize during a single application of the higher concentration.Another possibility is that the higher concentration interactswith multiple receptor subtypes that have different effects. Forexample, SST₁ and SST₂ have opposing effects in hypothalamus (Lanneauet al. 1998), and both these subtypes are present in dentategyrus.

We found that SST modestly depressed pharmacologically isolated NMDA fEPSPs recorded in Mg²⁺-free ACSF. However, when we recorded NMDA receptor-mediated EPSCsin voltage-clamp, we observed no effect of SST. These resultssuggest that SST is not likely directly acting on NMDA responses.Instead, SST may be acting on voltage-sensitive conductances (i.e.,Ca²⁺) activated during the depolarizing fEPSP. Accordingly, when SSTwas applied in the presence of $omega$ -conotoxin, little inhibitionwas observed. In any case, this modest effect on the NMDA-mediatedfEPSP is unlikely to account for SST inhibition of LTP, sincea much greater reduction of the NMDA response is necessary toblock LTP (Blake et al. 1988; Grunze et al. 1996; Rosenblum etal. 1999).

SST may regulate LTP by inhibiting N-type Ca²⁺ currents, an action that has been demonstrated for SST in acutely dissociatedand cultured hippocampal pyramidal neurons (Boehm and Betz 1997;Ishibashi and Akaike 1995). LPP LTP induced by high-frequencytrains is an NMDA receptor-dependent event, similar to LTP inCA1 but not CA3. Dendritic L-type Ca²⁺ channels are thought to be involved in an NMDA-independent typeof LTP in CA1 (Huang and Malenka 1993). The involvement of Ca²⁺ channels in LPP LTP has not previously been demonstrated. Ourdata suggest that LPP LTP evoked by a relatively moderate, nonsaturatingstimulus paradigm involves entry of Ca²⁺ through both N-type Ca²⁺ channels and NMDA receptors. However, since N-type channels areinvolved in glutamate release, a presynaptic site of action for $omega$ -conotoxin cannot be ruled out. Blockade of N-type channels doesnot, however, influence presynaptically generated LTP at mossyfiber/CA3 synapses (Castillo et al. 1994), nor does it block CA1LTP (Schulz 1997; Szinyei et al. 1999). Therefore a synapse-specificeffect is indicated in dentate that could be postsynaptic. PostsynapticN-type Ca²⁺ channels have similarly been implicated in the induction of long-termdepression in CA1 (Normann et al. 2000).

Multiple inhibitory neuropeptides depress dentate gyrus LTP. An in vivo study showed neuropeptide Y (NPY)-mediated inhibitionof dentate LTP (Whittaker et al. 1999), whereas in vitro studieshave shown nociceptin (Yu and Xie 1998), dynorphin (Terman etal. 1994), galanin, and cortistatin (unpublished observations)to depress LTP at LPP synapses. Some of these peptides robustlydepress baseline perforant-path fEPSPs (i.e., dynorphin, nociceptin);these peptides likely have a presynaptic site of action in inhibitingglutamate releases, although they could also act postsynaptically(Yu and Xie 1998). Galanin (unpublished observations) and NPY(Klapstein and Colmers 1993; McQuiston et al. 1996), like SST,do not consistently inhibit baseline EPSPs at this synapse. NPYinhibits N-type Ca²⁺ currents and Ca²⁺ transients in dentate granule cells (McQuiston et al. 1996);thus, like SST, this is a possible mechanism through which thispeptide could attenuate LTP. In contrast, opiate peptides actingon delta and mu receptors have facilitory actions on dentate LTP,through inhibition of GABAergic interneurons (Bramham et al. 1988,1991; Xie and Lewis 1991). Interestingly, the excitatory neuropeptidecorticotropin-releasing factor (CRF) has direct LTP-like actionson dentate granule cells in vivo (Wang et al. 2000). These resultssuggest a role for neuropeptides as important regulators of synapticplasticity in dentate gyrus. Inhibition of synaptic potentiationat this synapse could be one mechanism through which some peptidesdiminish seizure events in models of temporal lobe epilepsy, sinceLTP at this synapse may contribute to invasion of seizures intohippocampus (Sutula and Steward 1986, 1987; Wasterlain et al.1999).

Our results suggest SST is released during high-frequency activation of SST containing interneurons and acts to prevent LTPof LPP synapses. Seizure events have been shown to cause intenseactivation of SST/GABAergic hilar interneurons (Vezzani et al.1996). Thus the seizure-induced death of these neurons would leadto the loss of an important regulatory mechanism in the dentatethat could contribute to the increased susceptibility of the dentateto invasion by subsequentseizures.

	ACKNOWLEDGMENTS

We thank Dr. George Siggins for support (National Institute of Mental Health Grant MH-44346) and Dr. Marisa Roberto for readingthemanuscript.

This work was supported by National Institute of Neurological Disorders and Stroke Grant NS-38633.

Present address of M. K. Tallent: Drexel University College of Medicine, Department of Pharmacology and Physiology MS 488,245 N. 15^th St., Philadelphia, PA19102.

	FOOTNOTES

Address for reprint requests: M. K. Tallent, Dept. of Pharmacology and Physiology, Drexel University College of Medicine,MS 488, 245 N. 15th St, Philadelphia, PA 19104 (E-mail: tallent{at}drexel.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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