Somatostatin Inhibits Excitatory Transmission at Rat Hippocampal Synapses via Presynaptic Receptors

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Volume 17, Number 11, Issue of June 1, 1997 pp. 4066-4075
Copyright ©1997 Society for Neuroscience

Somatostatin Inhibits Excitatory Transmission at Rat Hippocampal Synapses via Presynaptic Receptors

Stefan Boehm and Heinrich Betz
Max-Planck-Institut für Hirnforschung, Abteilung Neurochemie, D-60528 Frankfurt/Main, Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Somatostatin is one of the major peptides in interneurons of the hippocampus. It is believed to play a role in memory formationand to reduce the susceptibility of the hippocampus to seizure-likeactivity. However, at the cellular level, the actions of somatostatinon hippocampal neurons are still controversial, ranging from inhibitionto excitation. In the present study, we measured autaptic currentsof hippocampal neurons isolated in single-neuron microcultures.Somatostatin and the analogous peptides seglitide and octreotidereduced glutamatergic, but not GABAergic, autaptic currents viapertussis toxin-sensitive G-proteins. This effect was observedwhether autaptic currents were mediated by NMDA or non-NMDA glutamatereceptors. Furthermore, somatostatin did not affect currents evokedby the direct application of glutamate, but reduced the frequencyof spontaneously occurring excitatory autaptic currents. Theseresults show that presynaptic somatostatin receptors of the SRIF₁family inhibit glutamate release at hippocampal synapses. Somatostatin,seglitide, and octreotide also reduced the frequency of miniatureexcitatory postsynaptic currents in mass cultures without affectingtheir amplitudes. In addition, all three agonists inhibited voltage-activatedCa²⁺ currents at neuronal somata, but failed to alter K⁺ currents, effects that were also abolished by pertussis toxin.Thus, presynaptic somatostatin receptors in the hippocampus selectivelyinhibit excitatory transmission via G-proteins of the G_i/G_o familyand through at least two separate mechanisms, the modulation ofCa²⁺ channels and an effect downstream of Ca²⁺ entry. This presynaptic inhibition by somatostatin may providea basis for its reportedly anticonvulsive action.
Key words: autapses; hippocampus; somatostatin; G-proteins; glutamate release; Ca²⁺ current

INTRODUCTION

Somatostatin, a cyclic tetradecapeptide, was initially identified as a hypothalamic peptide that regulates growth hormonesecretion from cells of the anterior pituitary gland (Brazeauet al., 1973). In subsequent years, somatostatin was describedas a neurotransmitter and neuromodulator (for review, see Reichlin,1983). Somatostatin is synthesized in numerous neurons throughoutthe brain (Johansson et al., 1984) and is released in a Ca²⁺-dependent manner (Iversen et al., 1978). The peptide is thoughtto be involved in various complex functions of the CNS, such asthe sensation of pain (Kuriashi et al., 1985) and the formationof memory (Matsuoka et al., 1994). In addition, levels of somatostatinare altered in several human brain dysfunctions, such as seniledementia of the Alzheimer type (Davies et al., 1980) and temporallobe epilepsy (Robbins et al., 1991).

Brain regions that are particularly rich in somatostatin-containing neurons include the neocortex and the hippocampal formation(Johansson et al., 1984). In the hippocampus, somatostatin isa co-transmitter in inhibitory, GABA-containing interneurons (Freundand Buzsaki, 1996). These GABAergic neurons were shown to releasesomatostatin in a Ca²⁺-dependent manner in vitro (Fontana et al., 1996) and in vivo(Mathe et al., 1993). However, it remains controversial whethersomatostatin in the hippocampus is inhibitory, as is GABA, orexcitatory. Inhibitory effects have been reported, for instance,in rat hippocampal slices (Pittman and Siggins, 1981; Moore etal., 1988), but excitatory actions of somatostatin have also beenobserved in the very same preparation (Dodd and Kelly, 1978).Similarly, somatostatin has been found to both excite and inhibitcortical neurons in tissue culture (Delfs and Dichter, 1983).

The reasons for these discrepancies have remained elusive, and several explanations may be considered. (1) Somatostatin mayact via at least five distinct receptors (Hoyer et al., 1995;Reisine and Bell, 1995), and different receptors can mediate opposingactions of somatostatin even in a single neuron (Wang et al.,1990). Transcripts for all five receptors have been detected inrat hippocampus (Thoss et al., 1995). (2) Contrasting effectsof somatostatin may result from a direct and an indirect action,respectively. Such indirect actions of somatostatin might be mediatedby acetylcholine (Araujo et al., 1990) or dopamine (Chesseletand Reisine, 1983), the release of which can be triggered by thisneuropeptide. (3) Opposite effects may arise when a neurotransmitteractivates either pre- or postsynaptic receptors. Presynaptic receptorsfor somatostatin have been described previously in peripheral,sympathetic (Boehm and Huck, 1996), and parasympathetic (Grayet al., 1989), but not central, neurons.

The present study was performed in search of presynaptic somatostatin receptors in hippocampal neurons. To avoid indirecteffects of somatostatin that may arise in neuronal networks, weinvestigated synaptic transmission at autapses formed by neuronsthat grow in isolation on microislands of glial cells. Autapsesof such microculture neurons display functional characteristicssimilar to those of conventional synapses in vitro (Bekkers andStevens, 1991; Tong et al., 1996). Our results indicate that presynapticsomatostatin receptors regulate transmission at excitatory hippocampalsynapses.

MATERIALS AND METHODS
Cell culture. Hippocampi were dissected from neonatal Wistar rats, cut into small pieces, and incubated in papain (Worthington,Freehold, NJ, 1 mg/ml in L-15 Leibovitz medium) for 30 min at36°C. After removal of the enzyme, tissue fragments were washedthree times in 25% fetal calf serum in PBS. Thereafter, a singlecell suspension was obtained by trituration in DMEM (Life Technologies,Berlin, Germany) containing 10% fetal calf serum (Integro, Zaandam,Holland) and 5 µg/ml insulin, 5 µg/ml transferrin, 5 ng/ml Na-selenite(Boehringer Mannheim, Mannheim, Germany), 10 nM progesterone,2 mM MgSO₄, 25,000 IU/l penicillin, and 25 mg/l streptomycin (Sigma,Deisenhofen, Germany). For high-density mass cultures, ~50,000cells were seeded into microchambers created by glass rings (innerdiameter, 10 mm) placed in the center of 35 mm culture dishes(Nunclon #150350) that had been coated with poly-D-lysine (Sigma,1 mg/ml). To obtain microisland cultures, ~100,000 cells wereplated in 35 mm culture dishes prepared as follows. The disheswere first coated with 0.15% agarose and sterilized by UV irradiation.Thereafter, a mixture of poly-D-ornithine (1 mg/ml) and collagen(4 mg/ml) was sprayed onto the dishes under sterile conditionswith a chromatography microatomizer (NeoLab, Heidelberg, Germany).All cultures were kept in a water-saturated 5% CO₂ atmosphereat 37°C.

After 3-5 d, 3 µM cytosine arabinoside (Sigma) was added to the culture medium to reduce the proliferation of non-neural cells.After 6 d in vitro, microislands cultures were treated with 100µM glutamate in recording solution (see below) containing 2 mMCa²⁺, but no Mg²⁺, for 60 min at room temperature; this procedure removed all neuronsto generate pure glial microislands. On day 7, ~40,000 freshlydissociated hippocampal cells were seeded onto these microislands.Cytosine arabinoside (3 µM) was added again after 3-5 d. Mediawere not changed until the cultures were used for experiments.

Electrophysiological recordings of autaptic currents. Single, isolated neurons in microcultures were used for electrophysiologicalexperiments after 8-16 d in vitro. Currents were recorded fromneuronal somata in the whole-cell configuration of the patch-clamptechnique (Hamill et al., 1981) at room temperature (20°-24°C).Unless stated otherwise, neurons were clamped at a holding potentialof $-$ 70 mV and depolarized for 1-2 msec to 0 mV. Autaptic currentswere evoked by this stimulation protocol every 30 sec. Spontaneouslyoccurring excitatory autaptic currents (SEACs) were recorded insweeps of 1-2 sec at a potential of $-$ 70 mV. Stimulation and currentrecordings were obtained with an EPC-9 (HEKA, Lambrecht, Germany)amplifier linked to an Atari Mega STE computer controlled by HEKAsoftware.

Electrodes were pulled from borosilicate glass capillaries (Hilgenberg, Malsfeld, Germany) with a Zeitz DMZ Universal Puller(Zeitz Instruments, Augsburg, Germany) to yield tip resistancesof 1-3 M $Omega$ . Series resistances after whole-cell formation (5-20M $Omega$ ) were monitored regularly throughout recordings and compensatedfor by 60-90%.

Pipettes were filled with a solution containing (in mM): K-glutamate 100, K-gluconate 40, CaCl₂ 1.6, EGTA 10, HEPES 10, Mg-ATP2, and Li-GTP 2, adjusted to pH 7.3 with NaOH. Unless stated otherwise,the bathing solution consisted of (in mM): NaCl 140, KCl 6, CaCl₂3, MgCl₂ 2, glucose 20, and HEPES 10, adjusted to pH 7.4 withNaOH. Neurons under investigation were superfused continuouslywith this solution, containing test drugs if appropriate. Superfusionwas performed with a DAD-12 (Adams and List, Westbury, NY) drugapplication system.

Electrophysiological recordings of miniature excitatory postsynaptic currents (mEPSCs) and glutamate-evoked currents. MEPSCsand glutamate-induced currents in microculture or mass cultureneurons were recorded with the same settings as those used forautaptic currents (see above). As with microcultures, mass cultureswere used for experiments 8-16 d after plating. The bathing solution(see above) contained 1 µM TTX and 1-2 mM kynurenic acid to minimizethe probability of polysynaptic excitations. The neuron from whichmEPSCs were recorded and its surrounding were superfused continuouslywith a solution lacking kynurenic acid to permit the occurrenceof mEPSCs, but containing 1 µM TTX and 30 µM bicuculline methiodide(BMI) to suppress evoked EPSCs and inhibitory postsynaptic currents,respectively.

Currents through glutamate receptors were elicited by the direct application of 100 µM glutamate via the DAD-12 superfusiondevice in either the absence or the continuous presence of somatostatin.

Electrophysiological recordings of voltage-activated Ca²⁺ and K⁺ currents. Voltage-activated Ca²⁺ and K⁺ currents from hippocampal neurons in mass culture were recordedafter 7-14 d in vitro, as described previously for sympatheticneurons (Boehm and Huck, 1996a; Boehm et al., 1996). The internalsolution used to measure Ca²⁺ currents contained (in mM): NMDG 115, tetraethylammonium chloride20, CaCl₂ 1.6, EGTA 10, glucose 10, HEPES 20, Mg-ATP 2, and Li-GTP2, adjusted to pH 7.3 with HCl. For the recording of voltage-dependentK⁺ currents, as well as for the determination of the resting membranepotential, the internal (pipette) solution contained (in mM) KCl140, CaCl₂ 1.59, EGTA 10, HEPES 10, Mg-ATP 2, and Li-GTP 2, adjustedto pH 7.3 with KOH. The bathing solution was the same as aboveand contained 1 µM TTX to block Na⁺ channels and 100 µM Cd²⁺ to block Ca²⁺ channels when K⁺ currents were measured. Unless stated otherwise, K⁺ and Ca²⁺ currents were evoked every 15-20 sec by depolarizations from $-$ 80 mV to 0 mV. For these experiments, we used an EPC-7 amplifier(List Medical, Darmstadt, Germany) linked to an Olivetti personalcomputer under the control of the PClamp (5.0) software (AxonInstruments, Tujunga, CA).

Calculations and statistics. Autaptic currents as well as voltage-activated Ca²⁺ currents occasionally showed considerable rundown. To take thisinto account, current amplitudes in the presence (B) of somatostatinand other test drugs were compared with those obtained beforeapplication (A) and after washout (C); drug effects were evaluatedeither as percent of control [=200 × B/(A + C)] or as percentof inhibition [=100 × (1 $-$ 2B/{A + C})]. MEPSCs or SEACs wereevaluated off-line by the TAC program (Instrutech, Elmont, NY)running on an Atari Mega STE computer. This program automaticallydetects peaks that exceed a certain threshold. Thresholds wereadjusted for each cell by analysis of traces obtained in the presenceof 10 µM CNQX, which entirely blocked all glutamate-mediated synapticcurrents in the presence of Mg²⁺ (Fig. 1A).
Fig. 1. Autaptic currents of hippocampal microisland neurons and their modulation by somatostatin. A and B show EACs and IACs, respectively,recorded from two different neurons by the stimulation protocolshown in C. Currents in the bottom panels were recorded before(control), during, and after (wash) the application of 1 µM TTX(A, B), 10 µM CNQX (A), and 30 µM BMI (B), respectively. The timescale in C applies to the currents shown in A, B, D, and E. D,EACs measured at a holding potential of $-$ 70 mV before (control),during, and after (wash) the application of 1 µM somatostatin.E shows the same sequence of recordings obtained in a neuron displayingIACs measured at a holding potential of $-$ 40 mV. F summarizes theeffects of 1 µM somatostatin on EACs and IACs. The boxes encompassthe median 25th through 75th percentiles and contain a line markingthe median 50th percentile point. The caps of the error bars indicatethe median 10th and 90th percentiles.
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Unless stated otherwise, results are presented as arithmetic means ± SEM; n = number of cells. Differences between data pointswere evaluated by the unpaired Student's t test. Concentration-responsecurves were fitted to experimentally obtained data by the ALLFITprogram (DeLean et al., 1978), which also determines differencesbetween single concentration-response curves by simultaneous fittingwith shared parameters and subsequent calculation of the F statisticon the resulting "extra sum of squares."

Materials. Somatostatin, TTX, BMI, kynurenic acid, and pertussis toxin (PTX) were obtained from Sigma (Deisenhofen, Germany),and CNQX and AP5 from Tocris Cookson (Bristol, UK). Octreotidewas a gift from Sandoz (Basel, Switzerland) and seglitide wasdonated by Merck, Sharp and Dohme (Vienna, Austria).

RESULTS

Effects of somatostatin on autaptic currents in microisland neurons
Conflicting results have been obtained with somatostatin when applied to hippocampal neurons in networks, for example, inslice preparations or conventional primary cell cultures (Doddand Kelly, 1978; Pittman and Siggins, 1981; Moore et al., 1988).Therefore, we used single hippocampal neurons on microislandsof glial cells. Such microisland neurons are isolated from anyother neuron and form only synaptic connections onto themselves,so-called autapses (Bekkers and Stevens, 1991). When such neuronswere shortly (1-2 msec) depolarized to ~0 mV, either excitatory(EAC) or inhibitory (IAC) autaptic currents could be observed.These two types of currents could be easily distinguished by thefollowing criteria. (1) At negative holding potentials, EACs werealways inward directed, whereas IACs reversed at approximately $-$ 60 mV (Fig. 1A-C), as shown previously under similar experimentalconditions (Bekkers and Stevens, 1991). (2) When 2 mM Mg²⁺ was present in the superfusion buffer to block NMDA receptorsat negative potentials, EACs were abolished by 10 µM CNQX, whereasIACs were blocked by 30 µM BMI (Fig. 1A-C). Hence, the currentswere mediated by non-NMDA glutamate receptors and by GABA_A receptors,respectively. (3) EACs decayed rapidly and monoexponentially witha mean time constant of 6.0 ± 0.3 msec (n = 19) when NMDA receptorswere blocked by 2 mM Mg²⁺, whereas IACs had prolonged durations with double exponentialdecay and time constants of 12.4 ± 1.2 and 65.0 ± 6.3 msec (n= 13).

EACs were measured routinely at holding potentials of $-$ 70 mV and had a mean peak current amplitude of $-$ 5.7 ± 0.6 nA (n = 48).The time lag between the end of depolarizations and the peak amplitudeamounted to 7.2 ± 0.3 msec (n = 48). IACs were determined as outwardcurrents at $-$ 40 mV and had peak current amplitudes of 1.8 ± 0.8nA (n = 17). The time between depolarization and peak IACs was6.3 ± 0.4 msec (n = 17). Both EACs and IACs were abolished inthe presence of either 0.3 µM TTX (Fig. 1A,B) or 30 µM Cd²⁺ (data not shown).

Somatostatin (1 µM) reduced EACs (Fig. 1D,F) in an entirely reversible manner. This effect varied considerably between singleneurons, yielding inhibition from down to 32% of control amplitudesto just 93% of control. Conversely, IACs were not affected bysomatostatin (Fig. 1E,F). The inhibitory action of somatostatinon EACs was half-maximal at 12 nM and reached a mean maximum of38% inhibition (Fig. 2A).
Fig. 2. Pharmacological characterization of somatostatin receptors mediating the inhibition of EACs. A, Concentration-response curvesfor the reduction of EACs (measured as shown in Fig. 1D) by somatostatin(circles, n = 7-23, with the exception of 1 nM, for which n =3), seglitide (squares, n = 5-9), and octreotide (triangles, n= 5-9). Data for the three agonists are pooled from differentneurons, but not every neuron could be exposed to all agonistconcentrations. B, Inhibition of EACs by 1 µM somatostatin, seglitide,and octreotide in a common set of neurons (n = 5). C, Effectsof 1 µM somatostatin on EACs in neurons treated with 200 ng/mlPTX for $<=$ 24 hr (PTX), in neurons treated with heat-inactivated(95°C for 5 min) PTX (HI), and in control (untreated) neurons(ctl). Levels of significance for the difference between the resultsobtained in pretreated and in untreated neurons, respectively,are indicated above the bars.
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Native somatostatin receptors can be divided into two subfamilies, SRIF₁ and SRIF₂, which are distinguished by agonist affinitiesand/or potencies; subtype-selective antagonists are currentlynot available (Hoyer et al., 1995; Reisine and Bell, 1995). Twoshort synthetic somatostatin analogs, seglitide (Veber et al.,1981) and octreotide (Tran et al., 1985), have most frequentlybeen used to characterize somatostatin receptors. These two peptideshave nanomolar affinities to receptors of the SRIF₁ family, butless than micromolar affinities for the SRIF₂ family (Hoyer etal., 1994, 1995; Reisine and Bell, 1995). In rat hippocampal microislandneurons, seglitide and octreotide, like somatostatin, reducedEACs. Seglitide caused half-maximal inhibition at 10.2 nM, andoctreotide at 9.4 nM. These values are not different from thoseobtained with somatostatin, indicating equipotency of the threeagonists. From the concentration-response curves in Figure 2A,seglitide and octreotide appeared to yield less maximal inhibitionthan somatostatin. However, when the three agonists were appliedto the same set of neurons, they all produced ~25% inhibition(Fig. 2B) and were thus equieffective.

Somatostatin receptors most commonly exert their cellular effects via PTX-sensitive G-proteins (Rens-Domiano and Reisine,1992), although PTX-insensitive effects of somatostatin have alsobeen reported for central neurons of the rat (Twery et al., 1991).When microisland neurons had been treated with 200 ng/ml PTX forat least 24 hr, somatostatin failed to inhibit EACs (Fig. 2C).Peak amplitudes of EACs ( $-$ 5.3 ± 2.2 nA; n = 6) and the delay betweendepolarization and peak currents (7.2 ± 0.6 msec; n = 6) werenot altered after PTX treatment, compared with untreated neurons.Treatment of neurons with heat-inactivated (95°C for 5 min) PTXdid not alter the inhibitory effect of somatostatin (Fig. 2C).Thus, the inhibition of EACs by somatostatin was mediated by G-proteinsof the G_i/G_o group.

Somatostatin acts at presynaptic receptors
Several mechanisms could underlie the selective inhibition of EACs, but not IACs, by somatostatin. For example, a blockadeof postsynaptic non-NMDA glutamate receptors might have mediatedthese effects. In hypothalamic neurons, somatostatin receptorshave been shown to modulate currents through non-NMDA glutamatereceptors (Gardette et al., 1995). To find out whether effectsof somatostatin arose from a postsynaptic action on a certainglutamate receptor, the following experiments were performed.
Experiment 1 EACs were evoked under conditions that either favor (no Mg²⁺, 10 µM glycine) or prevent (2 mM Mg²⁺, no glycine) the activation of NMDA receptors. When activationof NMDA receptors was permitted, EACs showed a prolonged durationwith biexponential decay kinetics (Fig. 3A); the two time constantsof decay were 6.1 ± 0.5 msec (which is identical to the time constantobtained in the presence of Mg²⁺) and 211.7 ± 7.3 msec (n = 6), respectively. The late phases(>30 msec after the depolarization) of these prolonged EACs werecarried by NMDA receptors, as evidenced by their blockade in thepresence of 50 µM AP5 (Fig. 3A). Somatostatin (1 µM) reduced peakEACs when NMDA receptors were involved (49.5 ± 11.9% of control)to the same extent as when NMDA receptors were blocked (47.7 ±8.9% of control; n = 6). Furthermore, pure NMDA receptor-carriedEACs (measured between 50 and 60 msec after the end of the depolarizingvoltage step) were also inhibited to the same extent (43.2 ± 11.1%of control; n = 6) (Fig. 3B). Hence, EACs were reduced by somatostatinirrespective of the type of glutamate receptor mediating the autapticcurrents.
Fig. 3. Somatostatin acts at presynaptic receptors. A shows EACs recorded at $-$ 70 mV in the presence of 2 mM Mg²⁺, in the presence of 2 mM Mg²⁺ + 10 µM CNQX, after replacement of Mg²⁺ by 10 µM glycine, and after addition of 50 µM AP5. B shows theinhibition of EACs by somatostatin in a different microislandneuron in the presence of 2 mM Mg²⁺ (top traces) and after replacement of Mg²⁺ by 10 µM glycine (bottom traces). Currents were obtained before,during, and after the application of 1 µM somatostatin. C, Currentsevoked by 100 µM glutamate at $-$ 70 mV in a mass culture neuronin the presence of 1 µM somatostatin, as well as before and afterapplication of the peptide.
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Experiment 2 Glutamate (100 µM) was applied directly to hippocampal neurons in mass cultures in either the absence or the presence of somatostatin.The peptide failed to alter glutamate-evoked currents (Fig. 3C).In the presence of 1 µM somatostatin, the rapidly decaying peakcurrents were 94.7 ± 5.8% of control, and the subsequent plateaucurrents were 100.7 ± 1.5% of control (n = 6). These results indicatedthat somatostatin did not interfere with the function of non-NMDAglutamate receptors in rat hippocampal neurons.

The most plausible explanation for these observations is a presynaptic site of action for somatostatin. To corroborate thishypothesis, we recorded evoked and SEACs from single microislandneurons. As shown in Figure 4, 1 µM somatostatin not only reducedthe amplitude of evoked EACs, but also the frequency of SEACs.In three microisland neurons tested, somatostatin increased inter-SEACintervals by 66.5 ± 12.8% (p < 0.05 in each cell) without affectingmean SEAC amplitudes (112.3 ± 2.6% of control; p > 0.1 in eachcell). After washout of the peptide, inter-SEAC intervals returnedto 109.4 ± 12.3% of control, and mean SEAC amplitudes were 117.6± 2.1% of control. These results are entirely compatible witha merely presynaptic site of action for somatostatin (Scanzianiet al., 1992; Scholz and Miller, 1992; Trudeau et al., 1996).
Fig. 4. Somatostatin inhibits evoked as well as spontaneous EACs in microisland neurons. Recordings were obtained at $-$ 70 mV, and evokedEACs were elicited every 30 sec by 1 msec depolarizations to 0mV. SEACs were recorded intermittently in sweeps of 2 sec. Currenttraces were obtained before (control), during, and after (washout)the application of 1 µM somatostatin.
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Somatostatin receptors reduce the probability of spontaneous glutamate release in mass cultures
The results on synaptic currents presented above were all obtained in microisland neurons. To reveal whether presynaptic somatostatinreceptors might also operate in a network of rat hippocampal neurons,mEPSCs were recorded from neurons in mass cultures in the presenceof 30 µM BMI and 1 µM TTX to block GABA_A receptors and evokedEPSCs, respectively. As for the microisland neurons, 1 µM somatostatinshifted the duration of inter-mEPSC intervals to higher values,whereas the distribution of mEPSC amplitudes remained unchanged(Fig. 5A). Seglitide and octreotide, both at 1 µM, increased meaninter-mEPSC intervals to the same extent as somatostatin, withoutcausing changes in mean mEPSC amplitudes (Fig. 5B). These resultscorroborate the pharmacological characteristics obtained withEACs.
Fig. 5. Somatostatin receptors inhibit mEPSCs in hippocampal mass culture neurons. A, MEPSCs were recorded in a mass culture neuronat $-$ 70 mV in 1 sec sweeps in the presence of 1 µM TTX and 30 µMBMI. More than 200 events were evaluated from recordings obtainedbefore (control), during, and after (wash) the application of1 µM somatostatin. The distribution of mEPSC amplitudes (A₁) andinter-mEPSC intervals (A₂) is shown. B, Effects of 1 µM of somatostatin,seglitide, and octreotide on mean mEPSC amplitudes and mean inter-mEPSCintervals of five to six mass culture neurons. Results are shownas percentage of control. Changes in mean intervals (>50 eventsfor each condition) were significant (p < 0.05) in each neuron.C, Effects of somatostatin on mEPSCs recorded as in A and B, butin the presence of 100 µM Cd²⁺ (n = 5). Changes in mean intervals were significant (p < 0.05)in each neuron. D, Effects of somatostatin on mEPSCs recordedas in A-C, but in neurons treated for $>=$ 24 hr with 200 ng/ml PTX(n = 5). Note the loss of somatostatin effects.
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Subsequently, we also measured mEPSCs in the presence of 100 µM Cd²⁺, which entirely blocks voltage-activated Ca²⁺ channels and thereby abolishes EACs (see above). Frequenciesand amplitudes of mEPSCs determined in the presence of both TTXand Cd²⁺ were not different from those in the presence of TTX alone (datanot shown). Somatostatin increased inter-mEPSC intervals in thepresence of Cd²⁺ to about the same extent as in its absence (Fig. 5C). Thus, theseeffects of somatostatin on spontaneous glutamate release wereindependent of transmembrane Ca²⁺ entry. The reduction in the frequency of mEPSCs by somatostatinwas abolished after pretreatment of the cultures with PTX (200ng/ml for $>=$ 24 hr) (Fig. 5D), which per se did not significantlyalter the frequency or the amplitudes of mEPSCs (data not shown).Hence, G_i/G_o-type G-proteins also mediate the effects of presynapticSRIF₁ receptors on glutamate release, which occur downstream ofCa²⁺ entry.

Somatostatin receptors reduce voltage-activated Ca²⁺ currents
In most instances, presynaptic receptors reduce transmitter release via an inhibition of voltage-gated Ca²⁺ channels (Boehm and Huck, 1996b; Scholz and Miller, 1996; Takahashiet al., 1996). Somatostatin has been shown previously to reducevoltage-activated Ca²⁺ currents in various neuronal preparations (for review, see Inoueand Yoshi, 1992). This effect has also been found in pyramidalcells acutely dissociated from the rat hippocampal CA1 region(Ishibashi and Akaike, 1995), but not in the very same neuronswhen investigated in brain slices (Schweitzer et al., 1993). Atpresent, an effect of somatostatin on Ca²⁺ currents in hippocampal neurons in cell culture has not beenreported. Therefore, we investigated whether somatostatin mightmodulate the function of Ca²⁺ channels under our culture conditions. To this end, Ca²⁺ currents were recorded at neuronal somata in the whole-cell patch-clampconfiguration (Hamill et al., 1981). Step depolarizations from $-$ 80 mV to 0 mV elicited rapidly activating currents that reachedpeak amplitudes of $-$ 0.44 ± 0.03 nA within 7.7 ± 0.9 msec afterthe depolarizing voltage step. In several cases, Ca²⁺ current kinetics were distorted, presumably because of spaceclamp problems, and then the recordings were discontinued. In17 of 21 neurons tested, 1 µM somatostatin reduced peak currentamplitudes in an entirely reversible manner. In addition, somatostatindelayed activation kinetics (Fig. 6A) so that the mean time topeak was approximately doubled (15.3 ± 1.5 msec, n = 17; p < 0.001vs control). In current-voltage curves, the inhibitory actionof the peptide decreased as the depolarizing voltage step increased(Fig. 6B,C). Furthermore, facilitation of Ca²⁺ currents by depolarizing prepulses (+100 mV for 50 msec, followedby a 5 msec repolarization to $-$ 80 mV) abolished the slowing ofactivation kinetics by somatostatin and attenuated the reductionof peak current amplitudes (Fig. 6A, inset). Hence, the somatostatin-inducedinhibition displayed the characteristics of a G-protein-mediatedvoltage-dependent modulation of Ca²⁺ channels (Zhang et al., 1996), which has been described for somatostatinin other preparations (Ishibashi and Akaike, 1995; Toth et al.,1996; Zhang et al., 1996).
Fig. 6. Inhibition of voltage-activated Ca²⁺ currents by somatostatin. A, Ca²⁺ currents were evoked in a mass culture neuron by depolarizationsfrom $-$ 80 to 0 mV. Traces were recorded before (control), during,and after (wash) the application of 0.1 and 1 µM somatostatin.The inset shows rising phases of Ca²⁺ currents in the very same neuron under control conditions (a),in the presence of 1 µM somatostatin (b), and in the presenceof somatostatin, but subsequent to a 50 msec predepolarizationto +100 mV, followed by a 5 msec repolarization to $-$ 80 mV (c).Calibration, 50 pA, 10 msec. B, Current-voltage relationship ofthe Ca²⁺ currents in the same neuron as in A before (open circles) andduring (solid circles) the application of 1 µM somatostatin. C,The effect of somatostatin on the current-voltage relationshipin B is shown as percentage of inhibition.
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The inhibition of Ca²⁺ currents by somatostatin was half-maximal at 53 nM and reached a maximum of 26.1 ± 1.6% inhibition at1 µM (n = 7). Seglitide (1 µM) (25.2 ± 4.2% inhibition, n = 6)and octreotide (1 µM) (21.3 ± 4.1% inhibition; n = 8), when testedin neurons showing a somatostatin-induced inhibition of Ca²⁺ currents, reduced peak current amplitudes to the same extentas 1 µM somatostatin (21.1 ± 4.1% inhibition; n = 10). Thus, thesomatostatin receptors that control somatic Ca²⁺ channels belong to the same receptor subfamily as the presynapticreceptors that inhibit glutamate release.

As mentioned above, the function of presynaptic receptors was abolished by PTX. Likewise, somatostatin failed to affect peakCa²⁺ current amplitudes (0.4 ± 1.3% inhibition, n = 11) when neuronshad been treated with 100 ng/ml PTX for $>=$ 24 hr. Peak amplitudesmeasured in the absence of the peptide were not altered with PTXtreatment ( $-$ 0.43 ± 0.06 nA; n = 11). Hence, the effect of somatostatinreceptors on somatic Ca²⁺ channels was also mediated by G-proteins of the G_i/G_o subtype.

The somatostatin-induced inhibition of Ca²⁺ currents occurred at higher concentrations than that of EACs (half-maximal effectsat 53 nM vs 12 nM) and reached a maximum of 26% reduction in Ca²⁺ current amplitudes compared with the 38% reduction of EAC amplitudes.Considering that postsynaptic currents are connected to presynapticCa²⁺ influx via a fourth-power relation (Borst and Sakmann, 1996),these results appear inconsistent. Similar discrepancies havebeen described previously for somatostatin receptors in peripheralneurons and may indicate that the coupling between G-proteinsand voltage-activated Ca²⁺ channels differs between neuronal somata and presynaptic nerveterminals (Boehm and Huck, 1996a).

Lack of evidence for somatostatin-induced alterations in K⁺ currents
Apart from voltage-dependent Ca²⁺ channels, somatostatin receptors are known to modulate neuronal K⁺ channels (Inoue and Yoshi, 1992; Rens-Domiano and Reisine, 1992).In hippocampal CA1 pyramidal neurons in brain slices, somatostatinhas been reported to increase M currents, but no other K⁺ conductances (Moore et al., 1988). To clarify whether somatostatinmight affect transmitter release by an alteration in K⁺ conductance, we also measured K⁺ currents at neuronal somata and used step depolarizations from $-$ 80 to 0 mV, as above. K⁺ currents rapidly (time to peak, 4.4 ± 0.2 msec; n = 8) reachedpeak amplitudes (2.0 ± 0.2 nA; n = 8) and then decreased to approacha level of steady-state current (Fig. 7A). Somatostatin (1 µM)had no effect on these currents (Fig. 7A), and peak current amplitudesin the presence of the peptide were 98.2 ± 0.8% of control (n= 8). To rule out that somatostatin affected K⁺ conductances at other voltages, outward currents were elicitedby ramp depolarizations from $-$ 70 to +50 mV. In these experiments,somatostatin also failed to cause obvious alterations (Fig. 7B).Finally, the resting membrane potential of hippocampal neuronsin the whole-cell patch-clamp configuration ( $-$ 63.1 ± 5.5 mV, n= 5) also was not altered by somatostatin ( $-$ 63.3 ± 6.0 mV; n =5).
Fig. 7. Lack of effect of somatostatin on voltage-dependent K⁺ currents. A, K⁺ currents in a mass culture neuron were evoked by depolarizationsfrom $-$ 80 to 0 mV before (control), during, and after (wash) theapplication of 1 µM somatostatin. B, Outward currents in a massculture neuron were induced by a 0.2 sec ramp depolarization from $-$ 70 to +50 mV before, during, and after the application of 1 µMsomatostatin. Note that three traces are superimposed becauseof the lack of action of somatostatin.
[View Larger Version of this Image (12K GIF file)]

DISCUSSION
Presynaptic receptors for somatostatin have been described previously in peripheral cholinergic (Gray et al., 1989) and noradrenergic(Boehm and Huck, 1996a) neurons. In the present study, we showthat somatostatin also regulates neurotransmission at excitatorycentral synapses via presynaptic receptors.

Presynaptic SRIF₁-type somatostatin receptors at glutamatergic hippocampal synapses
The measurement of autaptic currents in isolated microisland neurons (Bekkers and Stevens, 1991) permits the detection ofeffects at homogenous populations of synapses derived from a singleneuronal soma. Somatostatin reduced EACs only, and not IACs, whichindicated that the peptide did not affect a common step of synaptictransmission in a nonspecific manner. Indeed, all the resultsobtained in the present study support the idea that somatostatinacted via specific receptors. (1) All actions of somatostatinwere abolished when neurons had been pretreated with PTX. Hence,effects were mediated by G_i/G_o-type G-proteins, a class of G-proteinsto which all somatostatin receptors may be linked (Hoyer et al.,1994; Reisine and Bell, 1995). (2) The effects of somatostatinwere concentration-dependent with half-maximal inhibition in therange of 10⁸ M. The five somatostatin receptors characterized by molecularcloning show comparable affinities for the neuropeptide (Hoyeret al., 1994, 1995). (3) The somatostatin-induced inhibition wasmimicked by seglitide and octreotide, short synthetic analog peptidesof somatostatin (Veber et al., 1981; Tran et al., 1985).

Submicromolar concentrations of these peptides activate somatostatin receptors of the SRIF₁ receptor subfamily (Hoyer et al.,1994). This group of receptors currently harbors the cloned receptorssstr-2, $-$ 3, and $-$ 5 (Hoyer et al., 1995; Reisine and Bell, 1995).In our experiments, octreotide and seglitide were equipotent tosomatostatin. At sstr-2 receptors, these peptides display thesame affinities as somatostatin, whereas at sstr-3, they are lesspotent. At sstr-5, seglitide has a lower affinity than somatostatinand octreotide (Hoyer et al., 1994). Thus, our results indicatethat the presynaptic somatostatin receptors of glutamatergic hippocampalneurons belong to the SRIF₁ subfamily and most closely resemblethe cloned sstr-2 receptor. However, additional experiments withhighly selective agonists (Raynor et al., 1993) are required foradditional characterization of these receptors.

Somatostatin receptors have been reported to modulate the function of non-NMDA glutamate receptors (Gardette et al., 1995).Hence, a selective reduction of EACs via somatostatin receptorsmight involve a postsynaptic site of action. However, we foundno evidence for an effect of somatostatin on the function of ionotropicglutamate receptors in rat hippocampal neurons. The observationsthat somatostatin neither altered glutamate-evoked currents noraffected mEPSC amplitudes both indicate that somatostatin actedvia presynaptic receptors.

Signaling mechanisms of presynaptic somatostatin receptors
All presynaptic receptors that have been identified on rat hippocampal neurons belong to the superfamily of G-protein-coupledreceptors, the effects being in many, but not all, cases PTX-sensitive(for review, see Thompson et al., 1993). Most somatostatin receptorsare linked to PTX-sensitive G-proteins (Rens-Domiano and Reisine,1992), and this was also true for the presynaptic receptors investigatedin the present study.

A plethora of signaling mechanisms may mediate the regulation of synaptic transmitter release by heterotrimeric GTP-bindingproteins (for review, see Fang et al., 1994). Intraneuronal effectorsystems for somatostatin receptors include various types of K⁺ channels, which may be activated, and voltage-gated Ca²⁺ channels, which may be inhibited (Inoue and Yoshi, 1992). Eachof these effects could reduce depolarization-evoked transmitterrelease. In our experiments, we were unable to detect any effectof somatostatin on K⁺ currents. Previously, somatostatin has been found to selectivelyincrease one type of K⁺ current, the M current, in rat CA1 pyramidal neurons (Moore etal., 1988). However, it appears unlikely that an increase in Mcurrents contributed to the presynaptic inhibition described here,for the following reasons. (1) Somatostatin receptors and muscarinicacetylcholine receptors modulate M currents of hippocampal neuronsin opposite directions (Inoue and Yoshi, 1992), but both typesof receptors inhibit excitatory synaptic transmission (Scanzianiet al., 1995; present study). (2) Despite the modulation of K_Mchannels by somatostatin, the peptide has almost no effect onaction potentials (Schweitzer et al., 1993) that represent thelink between the depolarization of neuronal somata and Ca²⁺ entry as well as transmitter release at autapses (as evidencedby the inhibitory action of TTX).

In contrast, somatostatin receptors with pharmacological characteristics identical to those of the presynaptic receptors investigatedhere reduced voltage-activated Ca²⁺ currents at the somata of hippocampal neurons. Inhibition ofCa²⁺ entry at presynaptic terminals has been shown to induce inhibitionof glutamatergic transmission (Takahashi et al., 1996). Therefore,we assume that the somatostatin-induced reduction of Ca²⁺ influx also occurred at presynaptic nerve terminals and causedthe inhibition of transmitter release. In peripheral neurons,the inhibition of voltage-gated Ca²⁺ channels appears to represent the only mechanism by which presynapticsomatostatin receptors reduce transmitter release (Gray et al.,1989; Boehm and Huck, 1996a). In hippocampal neurons, the signalingmechanisms of presynaptic somatostatin receptors seem to be morediverse, because agonists reduced the frequency of mEPSCs evenin the presence of Cd²⁺. Hence, like many other presynaptic receptors of hippocampalneurons (Scanziani et al., 1992; Scholz and Miller, 1992; Thompsonet al., 1993; Trudeau et al., 1996), presynaptic somatostatinreceptors may reduce excitatory synaptic transmission via at leasttwo independent signaling mechanisms: an inhibition of Ca²⁺ entry and a reduction of vesicle exocytosis, which arises downstreamof Ca²⁺ entry.

Whether the modulation of Ca²⁺ channels or the action downstream of Ca²⁺ entry mediates the inhibition of action potential-evoked transmitterrelease most likely depends on the organization of synaptic transmission.At hippocampal synapses, N- and Q-type Ca²⁺ channels contribute to synaptic transmission (Wheeler et al.,1994). N-type channels provide ~50% of the Ca²⁺ entry necessary for transmission (Wheeler et al., 1994, 1996),and these channels are preferentially inhibited by somatostatinreceptors (Toth et al., 1996; Zhang et al., 1996). Hence, underphysiological conditions in which postsynaptic responses are proportionalto the fourth power of the presynaptic Ca²⁺ current (Borst and Sakmann, 1996), reduction of currents throughone type of Ca²⁺ channel may be sufficient to cause inhibition of transmitterrelease. If, however, the contribution of one type of Ca²⁺ channel becomes redundant, for example, by broadening of actionpotentials (Wheeler et al., 1996) during neuronal bursting (seeKaczmarek and Levitan, 1987), a modulation of this channel willbe ineffective. Furthermore, the inhibition of all types of neuronalCa²⁺ currents via G-proteins is largely attenuated or abolished whendepolarizations are applied at short intervals (<50msec) (Grassiand Lux, 1989; Toth et al., 1996; Zhang et al., 1996). Hence,high-frequency firing may also hinder the receptor-mediated modulationof Ca²⁺ channels. Taken together, the dual signaling cascade of presynapticsomatostatin receptors may serve to control excitatory transmissionnot only under physiological conditions, but also when transmissionoccurs at higher frequencies, for example, during seizure-likeactivity.

Functional significance of presynaptic somatostatin receptors in the hippocampus
The function of many neuropeptides under physiological conditions is unclear, but it is believed to be important in pathology(Hökfelt, 1991). Somatostatin, in analogy to neuropeptide Y,has been suggested to play a role in hippocampal epilepsy (forReview, see Schwarzer et al., 1996). Neuropeptide y has long beenrecognized to reduce excitatory transmission in the hippocampus(Colmers et al., 1985), an action that forms the basis for theanticonvulsant activity of that peptide (Woldbey et al., 1996).

In the present study, we showed that somatostatin acting at presynaptic SRIF₁ receptors (most probably at sstr-2) reducedsynaptic glutamate release from hippocampal neurons in vitro.Provided this effect also occurs in vivo, activation of presynapticsomatostatin receptors may represent a mechanism to reduce epilepticseizures and subsequent neuronal damage in the hippocampus. Invivo antiepileptic activity of somatostatin (Monno et al., 1993)and sstr-2-preferring agonists (Perez et al., 1995), includingoctreotide (Vezzani et al., 1991), has indeed been reported. Hence,additional investigation of presynaptic somatostatin receptorsin hippocampal neurons under in vivo conditions may have therapeuticpromise for temporal lobe epilepsy.

FOOTNOTES

Received Jan. 27, 1997; revised March 12, 1997; accepted March 17, 1997.

This study was supported by the Fonds der Chemischen Industrie. S.B. is the recipient of a Schrödinger fellowship from theAustrian Science Foundation. We thank R. Harvey, S. Huck, andV. O'Connor for helpful comments on this manuscript and G. Koth,A. Hendricks, and A. Motejlek for perfect technical assistance.

Correspondence should be addressed to Dr. Stefan Boehm, Max-Planck-Institut für Hirnforschung, Abteilung Neurochemie, Deutschordenstrasse46, D-60528 Frankfurt/Main, Germany

REFERENCES

Araujo DM, Lapchak PA, Collier B, Quirion R (1990) Evidence that somatostatin enhances endogenous acetylcholine release in the rat hippocampus. J Neurochem 55:1546-1555[ISI][Medline].
Bekkers JM, Stevens CF (1991) Excitatory and inhibitory autaptic currents in isolated hippocampal neurons maintained in cell culture. Proc Natl Acad Sci USA 88:7834-7838[Abstract/Free Full Text].
Boehm S, Huck S (1996a) A somatostatin receptor inhibits noradrenaline release from chick sympathetic neurons through pertussis toxin-sensitive mechanisms: comparison with the action of alpha2-adrenoceptors. Neuroscience 73:595-604[ISI][Medline].
Boehm S, Huck S (1996b) Inhibition of N-type calcium channels: the only mechanism by which presynaptic $alpha$ ₂-autoreceptors control sympathetic transmitter release. Eur J Neurosci 8:1924-1931[ISI][Medline].
Boehm S, Huck S, Freissmuth M (1996) Involvement of a phorbol ester-insensitive protein kinase C in the alpha₂-adrenergic inhibition of voltage-gated Ca²⁺ current in chick sympathetic neurons. J Neurosci 16:4596-4603[Abstract/Free Full Text].
Borst JGG, Sakmann B (1996) Calcium influx and transmitter release at a fast CNS synapse. Nature 383:431-434[Medline].
Brazeau P, Vale W, Burgus R, Ling N, Butcher M, Rivier J, Guillemin R (1973) Hypothalamic polypeptide that inhibits the secretion of immunoreactive pituitary growth hormone. Science 179:77-79[Abstract/Free Full Text].
Chesselet MF, Reisine T (1983) Somatostatin regulates dopamine release in rat striatal slices and cat caudate nuclei. J Neurosci 3:232-236[Abstract].
Colmers WF, Lukowiak KD, Pittman QJ (1985) Neuropeptide Y reduces orthodromically evoked population spikes in rat hippocampal CA1 by a possibly presynaptic mechanism. Brain Res 346:404-408[ISI][Medline].
Davies P, Katzmann R, Terry RD (1980) Reduced somatostatin-like immunoreactivity in cerebral cortex from cases of Alzheimer disease and Alzheimer senile dementia. Nature 288:279-280[Medline].
Delfs JR, Dichter MA (1983) Effects of somatostatin on mammalian cortical neurons in culture: physiological actions and unusual dose response characteristics. J Neurosci 3:1176-1186[Abstract].
DeLean A, Munson PJ, Rodbard D (1978) Simultaneous analysis of families of sigmoidal curves: application to bioassay, radioligand assay, and physiological dose-response curves. Am J Physiol 235:E97-E102[Abstract/Free Full Text].
Dodd J, Kelly JS (1978) Is somatostatin an excitatory transmitter in the hippocampus? Nature 273:674-675[Medline].
Fang Y, Durgerian S, Basarsky TA, Haydon PG (1994) GTP-binding proteins: necessary components of the presynaptic terminal for synaptic transmission and its modulation. Adv Second Messenger Phosphoprotein Res 29:121-132[ISI][Medline].
Fontana G, De Bernardi R, Ferro F, Gemignani A, Raiteri M (1996) Characterization of the glutamate receptors mediating release of somatostatin from cultured hippocampal neurons. J Neurochem 66:161-168[ISI][Medline].
Freund TF, Buzsaki G (1996) Interneurons of the hippocampus. Hippocampus 6:347-470[ISI][Medline].
Gardette R, Faivre-Baumann A, Loudes C, Kordon C, Epelbaum J (1995) Modulation by somatostatin of glutamate sensitivity during development of mouse hypothalamic neurons in vitro. Dev Brain Res 86:123-133[Medline].
Grassi F, Lux HD (1989) Voltage-dependent GABA-induced modulation of calcium currents in chick sensory neurons. Neurosci Lett 105:113-119[ISI][Medline].
Gray DB, Pilar GR, Ford MJ (1989) Opiate and peptide inhibition of transmitter release in parasympathetic nerve terminals. J Neurosci 9:1683-1692[Abstract].
Hamill OP, Marty A, Neher E, Sakmann B, Sigworth FJ (1981) Improved patch clamp techniques for high-resolution current recording from cells and cell-free membrane patches. Pflügers Arch 391:85-100[ISI][Medline].
Hökfelt T (1991) Neuropeptides in perspective: the last ten years. Neuron 7:867-879[ISI][Medline].
Hoyer D, Lübbert H, Bruns C (1994) Molecular pharmacology of somatostatin receptors. Naunyn Schmiedebergs Arch Pharmacol 350:441-453[ISI][Medline].
Hoyer D, Bell GI, Berelowitz M, Epelbaum J, Feniuk W, Humphrey PPA, O'Carroll AM, Patel YC, Schonbrunn A, Taylor JE, Reisine T (1995) Classification and nomenclature of somatostatin receptors. Trends Pharmacol Sci 16:86-88[Medline].
Inoue M, Yoshi M (1992) Modulation of ion channels by somatostatin and acetylcholine. Prog Neurobiol 38:203-230[ISI][Medline].
Ishibashi H, Akaike N (1995) Somatostatin modulates high-voltage-activated Ca²⁺ channels in freshly dissociated rat hippocampal neurons. J Neurophysiol 74:1028-1036[Abstract/Free Full Text].
Iversen LL, Iversen SD, Bloom F, Douglas C, Brown M, Vale W (1978) Calcium-dependent release of somatostatin and neurotensin from rat brain in vitro. Nature 273:161-163[Medline].
Johansson O, Hökfelt T, Elde RP (1984) Immunohistochemical distribution of somatostatin-like immunoreactivity in the central nervous system of the rat. Neuroscience 13:265-339[ISI][Medline].
Kaczmarek LK, Levitan IB (1987) What is neuromodulation? In: Neuromodulation: the biochemical control of neural excitability (Kaczmarek LK, Levitan IB, eds), pp 3-17. New York: Oxford UP.
Kuriashi Y, Hirota N, Sato Y, Hino Y, Satoh M, Takagi H (1985) Evidence that substance P and somatostatin transmit separate information related to pain in the spinal dorsal horn. Brain Res 325:294-298[ISI][Medline].
Mathe AA, Nomikos GG, Svensson TH (1993) In vivo release of somatostatin from rat hippocampus and striatum. Neurosci Lett 149:201-204[ISI][Medline].
Matsuoka N, Maeda N, Yamaguchi I, Satoh M (1994) Possible involvement of brain somatostatin in the memory formation of rats and the cognitive enhancing action of FR121196 in passive avoidance task. Brain Res 642:11-19[ISI][Medline].
Monno A, Rizzi M, Samanin R, Vezzani A (1993) Anti-somatostatin antibody enhances the rate of hippocampal kindling in rats. Brain Res 602:148-152[ISI][Medline].
Moore SD, Madamba S, Joels M, Siggins GR (1988) Somatostatin augments the M-current in hippocampal neurons. Science 239:278-280[Abstract/Free Full Text].
Pittman QJ, Siggins GR (1981) Somatostatin hyperpolarizes hippocampal pyramidal cells in vitro. Brain Res 221:402-408[ISI][Medline].
Perez J, Vezzani A, Civenni G, Tutka P, Rizzi M, Schüpbach E, Hoyer D (1995) Functional effects of D-Phe-c[Cys-Tyr-D-Trp-Lys-Val-Cys]-Trp-NH₂ and differential changes in somatostatin receptor messenger RNAs, binding sites and somatostatin release in kainic acid-treated rats. Neuroscience 65:1087-1097[ISI][Medline].
Raynor K, Murphy WA, Coy DH, Moreau JP, Yasuda K, Bell GI, Reisine T (1993) Cloned somatostatin receptors: identification of subtype selective peptides and demonstration of high affinity binding of linear peptides. Mol Pharmacol 43:838-844[Abstract].
Reichlin S (1983) Somatostatin. N Engl J Med 309:1495-1501[ISI][Medline], 1556-1563.
Reisine T, Bell GI (1995) Molecular properties of somatostatin receptors. Neuroscience 67:777-790[ISI][Medline].
Rens-Domiano S, Reisine T (1992) Biochemical and functional properties of somatostatin receptors. J Neurochem 58:1987-1996[ISI][Medline].
Robbins RJ, Brines ML, Kim JH, Adrian T, deLannerolle N, Welsh MS, Spencer DD (1991) A selective loss of somatostatin in the hippocampus of patients with temporal lobe epilepsy. Ann Neurol 29:325-332[ISI][Medline].
Scanziani M, Capogna M, Gähwiler BH, Thompson SM (1992) Presynaptic inhibition of miniature excitatory synaptic currents by baclofen and adenosine in the hippocampus. Neuron 9:919-927[ISI][Medline].
Scanziani M, Gähwiler BH, Thompson SM (1995) Presynaptic inhibition of excitatory transmission by muscarinic and metabotropic glutamate receptor activation in the hippocampus: are Ca²⁺ channels involved? Neuropharmacology 34:1549-1557[ISI][Medline].
Scholz KP, Miller RJ (1992) Inhibition of quantal transmitter release in the absence of Ca²⁺ influx by a G protein linked adenosine receptor at hippocampal synapses. Neuron 8:1139-1150[ISI][Medline].
Scholz KP, Miller RJ (1996) Presynaptic inhibition at excitatory hippocampal synapses: development and role of presynaptic Ca²⁺ channels. J Neurophysiol 76:49-46.
Schwarzer C, Sperk G, Samanin R, Rizzi M, Gariboldi M, Vezzani A (1996) Neuropeptides-immunoreactivity and their mRNA expression in kindling: functional implications for limbic epileptogenesis. Brain Res Rev 22:27-50[Medline].
Schweitzer P, Madamba S, Champagnat J, Siggins GR (1993) Somatostatin inhibition of hippocampal CA1 pyramidal neurons: mediation by arachidonic acid and its metabolites. J Neurosci 13:2033-2049[Abstract].
Takahashi T, Forsythe ID, Tsujimoto T, Barnes-Davies M, Onodera K (1996) Presynaptic calcium current modulation by a metanotropic glutamate receptor. Science 274:594-597[Abstract/Free Full Text].
Thompson SM, Capogna M, Scanziani M (1993) Presynaptic inhibition in the hippocampus. Trends Neurosci 16:222-227[ISI][Medline].
Thoss VS, Perez J, Duc D, Hoyer D (1995) Embryonic and postnatal mRNA distribution of five somatostatin receptor subtypes in the rat brain. Neuropharmacology 34:1673-1688[ISI][Medline].
Tong G, Malenka RC, Nicoll RA (1996) Long-term potentiation in cultures of single hippocampal granule cells: a presynaptic form of plasticity. Neuron 16:1147-1157[ISI][Medline].
Toth PT, Shekter LR, Hui Ma G, Philipson LH, Miller RJ (1996) Selective G protein regulation of neuronal calcium channels. J Neurosci 16:4617-4624[Abstract/Free Full Text].
Tran VT, Beal MF, Martin JB (1985) Two types of somatostatin receptors differentiated by cyclic somatostatin analogs. Science 228:492-495[Abstract/Free Full Text].
Trudeau LE, Doyle RT, Emery DG, Haydon PG (1996) Calcium-independent activation of the secretory apparatus by ruthenium red in hippocampal neurons: a new tool to assess modulation of presynaptic function. J Neurosci 16:46-54[Abstract/Free Full Text].
Twery MJ, Wong LA, Gallagher JP (1991) Somatostatin induced hyperpolarization of septal neurons is not blocked by pertussis toxin. Eur J Pharmacol 192:287-291[ISI][Medline].
Veber DF, Freidinger RM, Schwenk Perlow D, Paleveda Jr WJ, Holly FW, Strachan RG, Nutt RF, Arison BH, Homnick C, Randall WC, Glitzer MS, Saperstein R, Hirschmann R (1981) A potent cyclic hexapeptide analogue of somatostatin. Nature 292:55-58[Medline].
Vezzani A, Serafini R, Stasi MA, Vigano G, Rizzi M, Samanin R (1991) A peptidase resistant cyclic octapeptide analogue of somatostatin (SMS 201-995) differently modulates seizures induced by quinolinic and kainic acid in the rat hippocampus. Neuropharmacology 30:345-352[ISI][Medline].
Wang HL, Dichter M, Reisine T (1990) Lack of cross-desensitization of somatostatin-14 and somatostatin-28 receptors coupled to potassium channels in rat neocortical neurons. Mol Pharmacol 38:357-361[Abstract].
Wheeler DB, Randall A, Tsien RW (1994) Roles of N-type and Q-type Ca²⁺ channels in supporting hippocampal synaptic transmission. Science 264:107-111[Abstract/Free Full Text].
Wheeler DB, Randall A, Tsien RW (1996) Changes in action potential duration alter reliance of excitatory transmission on multiple types of Ca²⁺ channels in rat hippocampus. J Neurosci 16:2226-2237[Abstract/Free Full Text].
Woldbey DPD, Madsen TM, Larsen PJ, Mikkelsen JD, Bolwig DG (1996) Neuropeptide Y inhibits hippocampal seizures and wet dog shakes. Brain Res 737:162-168[ISI][Medline].
Zhang JF, Ellinor PT, Aldrich RW, Tsien RW (1996) Multiple structural elements in voltage-dependent Ca²⁺ channels support their inhibition by G proteins. Neuron 17:991-1003[ISI][Medline].

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Somatostatin Inhibits Excitatory Transmission at Rat Hippocampal Synapses via Presynaptic Receptors

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