Opioid Enhancement of Calcium Oscillations and Burst Events Involving NMDA Receptors and L-Type Calcium Channels in Cultured Hippocampal Neurons

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The Journal of Neuroscience, November 15, 1999, 19(22):9705-9715

Opioid Enhancement of Calcium Oscillations and Burst Events Involving NMDA Receptors and L-Type Calcium Channels in Cultured Hippocampal Neurons
Rysard Przewlocki, Kathy L. Parsons, Dan D. Sweeney, Carol Trotter, Jeffrey G. Netzeband, George R. Siggins, and Donna L. Gruol
Department of Neuropharmacology, The Scripps Research Institute, La Jolla, California 92037

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Opioid receptor agonists are known to alter the activity of membrane ionic conductances and receptor-activated channels inCNS neurons and, via these mechanisms, to modulate neuronal excitabilityand synaptic transmission. In neuronal-like cell lines opioidsalso have been reported to induce intracellular Ca²⁺ signals and to alter Ca²⁺ signals evoked by membrane depolarization; these effects on intracellularCa²⁺ may provide an additional mechanism through which opioids modulateneuronal activity. However, opioid effects on resting or stimulatedintracellular Ca²⁺ levels have not been demonstrated in native CNS neurons. Thus,we investigated opioid effects on intracellular Ca²⁺ in cultured rat hippocampal neurons by using fura-2-based microscopicCa²⁺ imaging. The opioid receptor agonist D-Ala²-N-Me-Phe⁴,Gly-ol⁵-enkephalin (DAMGO; 1 µM) dramatically increased the amplitudeof spontaneous intracellular Ca²⁺ oscillations in the hippocampal neurons, with synchronizationof the Ca²⁺ oscillations across neurons in a given field. The effects ofDAMGO were blocked by the opioid receptor antagonist naloxone(1 µM) and were dependent on functional NMDA receptors and L-typeCa²⁺ channels. In parallel whole-cell recordings, DAMGO enhanced spontaneous,synaptically driven NMDA receptor-mediated burst events, depolarizingresponses to exogenous NMDA and current-evoked Ca²⁺ spikes. These results show that the activation of opioid receptorscan augment several components of neuronal Ca²⁺ signaling pathways significantly and, as a consequence, enhanceintracellular Ca²⁺ signals. These results provide evidence of a novel neuronal mechanismof opioid action on CNS neuronal networks that may contributeto both short- and long-term effects ofopioids.

Key words: glutamate receptors; synaptic transmission; calcium channels; NMDA receptors; intracellular calcium; opioid receptors

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pharmacological studies demonstrate that opiates and opioid peptides regulate neuronal activity in a variety of ways, dictatedin part by the opioid receptor subtypes that are involved. Themost widespread effect of opioids in the mammalian CNS is thereduction of excitatory and inhibitory synaptic transmission viathe presynaptic inhibition of transmitter release (North and Lovinger,1993). In addition, opioids can act postsynaptically to inhibitneuronal activity by opening K⁺ channels (North et al., 1987; Madison and Nicoll, 1988; Wimpeyand Chavkin, 1991; Moore et al., 1994) and thereby hyperpolarizingneurons or by inhibiting voltage-sensitive Ca²⁺ channels (Gross and MacDonald, 1987; Seward et al., 1991; Schroederand McCleskey, 1993; Moises et al., 1994) and thereby reducingdepolarizing drive. Opioids also can excite neurons directly byclosing K⁺ channels (Shen and Crain, 1990; Moore et al., 1994; Baraban etal., 1995) or by augmenting NMDA receptor-mediated responses (Chenand Huang, 1991; Martin et al., 1997) or indirectly by disinhibition(Zieglgansberger et al., 1979; Nicoll et al., 1980; Cohen et al.,1992).

Many of the effects of opioids on neuronal excitability occur via the direct actions of opioid receptor-coupled G-proteinsor via the regulation of cAMP levels (Childers, 1993; North, 1993).In addition, recent studies indicate that opioids can influencethe levels of other second messengers, including intracellularCa²⁺ (Tomura et al., 1992; Jin et al., 1994; Kaneko et al., 1994;Tang et al., 1994, 1995; Fields et al., 1995; Wandless et al.,1996; Connor et al., 1997) and inositol 1,4,5-trisphosphate (IP₃)(Johnson et al., 1994; Smart et al., 1994); these second messengersmay provide additional pathways for opioid control of neuronalactivity. Opioid effects on intracellular Ca²⁺ are of particular interest because of the wide-ranging role ofintracellular Ca²⁺ in a variety of cellular processes such as protein phosphorylation,membrane excitability, synaptic transmission, synaptic plasticity,genomic expression, cell growth and differentiation, and neurotoxicity(Siesjo, 1994; Petersen and Kasai, 1996; Ghosh and Greenberg,1998).

Although results from studies of opioid regulation of intracellular Ca²⁺ in neuronal-like cell lines could have profound implicationsfor CNS neuronal function and viability, little is known aboutopioid effects on the pathways that regulate intracellular Ca²⁺ levels in native CNS neurons. Therefore, we have examined theeffect of the opioid receptor agonist D-Ala²-N-Me-Phe⁴,Gly-ol⁵-enkephalin (DAMGO; 1 µM) on baseline Ca²⁺ levels and on physiological events known to increase intracellularCa²⁺ in primary cultures of rat hippocampal neurons. Neurons in thehippocampus are known to contain opioids, to express opioid receptors,and to show altered function when they are exposed to exogenouslyapplied opioids (Simmons and Chavkin, 1996).

We find that the activation of opioid receptors by DAMGO potentiates and synchronizes intracellular Ca²⁺ oscillations generated by the network synaptic activity in thehippocampal cultures and that these effects of DAMGO involve theNMDA subtype of glutamate receptors and L-type voltage-sensitiveCa²⁺ channels. DAMGO produced only small changes in baseline intracellularCa²⁺ levels when synaptic transmission was blocked pharmacologically.The intracellular Ca²⁺ oscillations generated by opioids could serve as important regulatorsof a variety of neuronalfunctions.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell culture. Modified organotypic cultures were prepared from 20 d embryonic rat hippocampi according to methods reportedpreviously (Gruol, 1983; Urrutia and Gruol, 1992). Briefly, hippocampiwere isolated from the brain, minced, gently triturated, and platedon Matrigel-coated (Collaborative Biochemicals, Bedford, MA) coverglassesin tissue culture dishes containing Minimal Essential Medium (MEM)with Earle's salts and L-glutamine (Life Technologies, Gaithersburg,MD), D-glucose (5 gm/l), 10% fetal calf serum, and 10% horse serum.The cultures were maintained at 37°C in a 5% CO₂ humidified atmospherefor up to 1 month. Medium was changed twice weekly by using MEMwith 10% horse serum. Brief treatment with 5-fluorodeoxyuridine(20 µg/ml; 3 d) added at the first medium change retarded thegrowth of non-neuronalcells.

Immunohistochemistry. Cultures were immunostained with antibodies to microtubular-associated protein-2 (MAP-2; BoehringerMannheim, Indianapolis, IN), glial fibrillary acidic protein (GFAP;Boehringer Mannheim), $gamma$ -aminobutyric acid (GABA; Incstar, Stillwater,MN), or glutamate (Chemicon, Temecula, CA). The immunohistochemistryprotocol followed methods published previously (Gruol and Crimi,1988). Briefly, the cells were fixed for 30 min at room temperaturein buffered fixative, were permeabilized with 0.25% Triton X-100(Sigma, St. Louis, MO) in PBS, pH 7.4, and were incubated overnightin primary antibody at 4°C. Immunoreactivity was detected thenext day via an immunoperoxidase reaction by using the materialsand procedures provided in the Vectastain Elite kit (Vector Laboratories,Burlingame,CA).

Intracellular Ca²⁺ measurement. Intracellular Ca²⁺ levels were determined for individual hippocampal neurons in selected microscopicfields by using standard fura-2 digital imaging methods describedpreviously (Qiu et al., 1995). Hippocampal neurons were loadedwith 3 µM fura-2 AM in physiological saline containing 0.02% pluronicF-127 (Molecular Probes, Eugene, OR) for 30 min, followed by incubationin physiological saline to allow for de-esterification of thefura-2 AM. For experiments the coverglass containing the neuronswas mounted in a chamber attached to the stage of an invertedfluorescent microscope used for fura-2 imaging. The chamber containedphysiological saline with reduced Mg²⁺ to enable activation of the NMDA receptors at normal restingmembrane potentials and with glycine (5 µM), a coagonist at theNMDA receptor. The composition of the saline was (in mM): 140NaCl, 3.5 KCl, 0.4 KH₂PO₄, 1.25 Na₂HPO₄, 2.2 CaCl₂, 0.030 MgCl₂,10 glucose, and 10 HEPES-NaOH, pH 7.3. In some studies ion channelblockers or transmitter receptor agonists were included in therecording saline. Dye loading and experiments were performed atroom temperature (21-23°C).

Live video images of microscopic fields illuminated at 340 and 380 nm wavelengths were recorded with a SIT-66 video camera(DAGE-MTI, Michigan City, IN) and digitized by computer. Datapoints were collected at 3-5 sec intervals, depending on the experiment.For each data point eight frames were averaged per wavelength.Ratio images of individual neurons in each field were formed bya pixel-by-pixel division of the averaged images collected at340 and 380 nm (340/380 nm). Real time digitized display, imageacquisition, and the calculation of intracellular Ca²⁺ levels were made with MCID imaging software (Imaging Research,St. Catharine's, Ontario). Intracellular Ca²⁺ levels were estimated from the following formula:

(1)

where R is the ratio value, R_min is the ratio for a Ca²⁺ free solution, R_max is the ratio for a saturated Ca²⁺ solution, K_d is 135 (the dissociation constant for fura-2), F_ois the intensity of a Ca²⁺ free solution at 380 nm, and F_s is the intensity of a saturatedCa²⁺ solution at 380 nm. The low level of background fluorescenceeliminated the need for background subtraction. Calibration wasdone by using fura salt (100 µM) in solutions of known Ca²⁺ concentration (Molecular Probes kit C-3009). In vitro calibrationproduced inconsistent results and thus was not used. Typical R_max,R_min, and F_o/F_s values were 0.61, 2.85, and 2.5,respectively.

Measurements were made of resting Ca²⁺ levels, the amplitude of spontaneous Ca²⁺ oscillations, and the amplitude of Ca²⁺ signals produced by the application of NMDA. For the spontaneousCa²⁺ oscillations the amplitude of individual oscillations (peak totrough) was measured with Axograph software (Axon Instruments,Foster City, CA). Approximately eight oscillations were measuredper cell. In some studies the data from control and drug conditionswere obtained from the same field of neurons. However, in mostcases different fields were used for each condition to avoid thepossibility of UV damage to the neurons. For intracellular Ca²⁺ signals elicited by exogenously applied NMDA, measurements weremade of the peak amplitude of the Ca²⁺ signal, defined as the difference between resting Ca²⁺ levels and the maximum increase in Ca²⁺ after stimulation withNMDA.

Intracellular Ca²⁺ measurements (amplitude of the Ca²⁺ oscillation or peak amplitude of the Ca²⁺ signal to NMDA) from individual neurons were normalized to themean value for the respective measurement under control conditionsin neurons in the same culture dish. Data from several cultureswere pooled and analyzed for statistical significance (p < 0.05)by one-way ANOVA, followed by the Fisher post hoc test for multiplecomparisons. In general, results were obtained from at least threeculture sets for each treatment group. For each culture set oneto three culture dishes were analyzed for each treatment group,with three to five microscopic fields (5-15 neurons per field)examined per culture dish. Compiled data are expressed as mean± SEM, with n denoting the number of neurons that werestudied.

Electrophysiological studies. To identify the effects of opioid receptor agonists on electrophysiological measurements, wemade whole-cell recordings in the somatic region of pyramidal-likeneurons by using the nystatin/perforated-patch method. Beforerecording, the culture medium was replaced with reduced Mg²⁺ saline (with 5 µM glycine) to parallel the recording conditionsused in the Ca²⁺ imaging experiments (see above). In some studies ion channelblockers or transmitter receptor agonists were included in therecording saline. The tips of the patch pipettes (4-6 M $Omega$ resistances)were filled with recording solution containing (in mM): 6 NaCl,154 K⁺-gluconate, 2 MgCl₂, 10 glucose, 1 BAPTA, 0.5 CaCl₂, and 10 HEPES-KOH,pH 7.3. The patch pipettes were backfilled with the same solutionbut containing nystatin (200 µg/ml; stock, 50 mg/ml DMSO; Sigma).Recordings were made with the Axopatch-1C amplifier (Axon Instruments)and monitored on a polygraph, computer, and oscilloscope. Forhigher resolution of fast events, selected data were recordedon FM tape (Racal, Irvine, CA) for playback at reduced tape speedonto a polygraph recorder. Recordings were made at room temperature(21-23°C).

Measurements were made of resting membrane potential, input resistance, current-evoked spiking, spontaneous burst activity,and the amplitude and duration of the membrane responses to NMDAor AMPA. Typically, one neuron was studied per culture dish, firstunder baseline conditions and then in the presence of an opioidreceptor agonist. Data from several cultures were pooled and analyzedfor statistically significant differences (p < 0.05) by usingthe paired Student's ttest.

Drug application. Opioid receptor agonists were added to the recording saline by bath addition or bath exchange. The studiesfocused on the opioid receptor agonist DAMGO (Sigma), which wastested at a standard dose of 1 µM in most experiments. The neuronswere exposed to the opioid receptor agonists for 5-20 min beforemeasurements weremade.

Several receptor antagonists and ion channel blockers were tested by bath addition or bath exchange; these included naloxone,tetrodotoxin (TTX), picrotoxin (all from Sigma), (S)- $alpha$ -methyl-4-carboxyphenylglycine(MCPG), 6,7-dinitroquinoxaline-2,3-dione (DNQX), 6-nitro-7-sulfamoylbenzo[t]quinoxaline-2,3-dione(NBQX), D( $-$ )-2-amino-5-phosphono-pentanoic acid (D-AP5; all fromTocris Cookson, Ballwin, MO), nimodipine (Research Biochemicals,Natick, MA), $omega$ -agatoxin IVA (Pfizer, Groton, CT), and $omega$ -conotoxinGVIA (Peptides International, Louisville,KY).

In some experiments the exogenous application of NMDA (10-200 µM) or AMPA (1-2 µM; S isomer used; both from Tocris Cookson)was used. For these studies NMDA or AMPA was dissolved in bathsaline and applied by a brief (1 sec) microperfusion pulse froma pipette (1-3 µm tip diameter) placed under visual control nearthe target neurons. A dye (fast green) was included in the agonistsolution to monitor neuronal exposure to theagonist.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hippocampal neurons exhibit intracellular Ca²⁺ oscillations that are enhanced by the opioid receptor agonist DAMGO

Hippocampal neurons were studied in cultures ranging in age from 6 to 37 d in vitro (DIV). The neurons were identified bymorphological criteria developed from immunohistochemical studiesby using an antibody to MAP-2, a cytoskeletal protein found inneurons. Immunostaining with an antibody to the transmitter glutamateor GABA showed that both glutamate-containing (data not shown)and GABA-containing neurons (Fig. 1A,B) were present in the cultures.The neurons formed extensive processes and synaptic connectionsin culture and exhibited physiological properties reflective ofhippocampal neurons in vivo, including network synaptic activity(see below).

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Figure 1. Effect of DAMGO on baseline intracellular Ca²⁺ oscillations in cultured hippocampal neurons. Shown are phase contrast (A) and bright-field (B) micrographs of hippocampal neurons in cultures immunostained with an antibody to the neurotransmitter GABA. The cultures contain a variety of neuronal types based on morphological characteristics and immunostaining for GABA, glutamate, and peptides (e.g., somatostatin; D. Gruol, unpublished data). The neurons grow on a background of astrocytes, identified by immunostaining with an antibody to GFAP. The white arrow points to a neuron immunostained with an antibody for GABA; the dark arrow points to a neuron that did not immunostain with the antibody. Calibration bar, 60 µm. C1, C2, Representative recordings of intracellular Ca²⁺ oscillations in six cultured hippocampal neurons in a microscopic field (different field than in A) under baseline control conditions (C1) and after the addition of DAMGO to the bath saline (C2). Each neuron is represented by a different symbol. Small intracellular Ca²⁺ oscillations were observed under baseline conditions, and these oscillations were enhanced dramatically in amplitude by the addition of DAMGO to the bath saline. DAMGO also synchronized the oscillations among the neurons in the field. C3, Mean values ± SEM for the amplitude of the intracellular Ca²⁺ oscillations (peak to trough measurement) in a population of control and DAMGO-treated neurons in the same culture dish as the recordings shown in C1 and C2. *Significant difference from control (p < 0.05; ANOVA). In these and all other experiments the Mg²⁺ concentration of the bath saline was 30 µM, and the bath saline contained glycine (5 µM).

Intracellular Ca²⁺ levels were measured in the somatic region of the cultured hippocampal neurons under control conditions andafter the addition of the opioid receptor agonist DAMGO to thebath saline. Under control conditions the spontaneous intracellularCa²⁺ oscillations of varying amplitude were observed in the majorityof neurons that were studied. The Ca²⁺ oscillations often were synchronized among several neurons ina microscopic field, suggesting that network synaptic activityplayed a role in the generation of the oscillations. Bath applicationof TTX, a treatment that blocks synaptic transmission in the hippocampalcultures, blocked the intracellular Ca²⁺ oscillations (data not shown), consistent with a dependence ofthe oscillations on network synapticactivity.

When applied to the bath saline at a standard test dose of 1 µM, DAMGO significantly increased the amplitude of the baselineCa²⁺ oscillations (Fig. 1C; >10 culture sets tested). In addition,DAMGO further synchronized the Ca²⁺ oscillations among the neurons in a microscopic field (Fig. 1C).However, DAMGO did not induce intracellular Ca²⁺ oscillations in cultures pretreated withTTX.

The enhancement of the intracellular Ca²⁺ oscillations by DAMGO was reversed by the addition of the opioid receptor antagonistnaloxone (1 µM) to the bath saline (five culture sets tested;Fig. 2). Moreover, the addition of naloxone to the bath beforeDAMGO blocked the enhancement of the spontaneous Ca²⁺ oscillations by DAMGO (Fig. 2B). Naloxone alone had no effecton baseline Ca²⁺ oscillations (Fig. 2B). These results show that opioids can modulateintracellular Ca²⁺ oscillations in hippocampal neurons and that opioid receptorsmediate these effects.

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Figure 2. The effect of DAMGO was blocked by the opioid receptor antagonist naloxone. A, Representative recordings of Ca²⁺ oscillations in cultured hippocampal neurons under baseline control conditions, in the presence of DAMGO, and after the addition of naloxone to cultures treated with DAMGO. The recordings are from three different microscopic fields; five neurons are shown for each condition. Naloxone reversed the enhancing effects of DAMGO on the Ca²⁺ oscillations. B, Mean ± SEM normalized amplitude of Ca²⁺ oscillations for control, DAMGO alone, naloxone alone, and DAMGO plus naloxone (Nal/DAMGO) conditions. In other experiments, naloxone before DAMGO blocked the effects of DAMGO (data not shown). Oscillations were measured as in Figure 1. Results represent the data from three experiments. *Significant difference from control (p < 0.05; ANOVA).

Involvement of glutamate receptors in the regulation of intracellular Ca²⁺ oscillations by DAMGO

Baseline Ca²⁺ oscillations and the effect of DAMGO on the oscillations were blocked by TTX, consistent with an involvement ofnetwork synaptic activity in these functions. Network synapticactivity in the hippocampal cultures involves excitatory synaptictransmission mediated by glutamate receptors. Therefore, it wasof interest to determine whether the enhancement of intracellularCa²⁺ oscillations by DAMGO was dependent on one or more of the glutamatereceptor subtypes known to be expressed by hippocampal neurons.Bath application of DNQX (10 µM; five culture sets tested) orNBQX (10 µM; one culture set tested), antagonists at the AMPAsubtype of glutamate receptor (AMPAR), increased the amplitudeof baseline intracellular Ca²⁺ oscillations. These results suggest that AMPARs are not requiredfor the generation of the intracellular Ca²⁺ oscillations but can modulate the oscillations. Presumably, AMPARantagonists block activation of inhibitory GABAergic interneurons,resulting in disinhibition of the network synaptic activity. Inthe presence of an AMPAR antagonist, DAMGO still elicited prominentalterations in baseline intracellular Ca²⁺ oscillations (Fig. 3A).

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Figure 3. Effects of glutamate receptor antagonists on the enhancement of intracellular Ca²⁺ oscillations by DAMGO. A, B, Representative recordings of intracellular Ca²⁺ oscillations in cultured hippocampal neurons under baseline control conditions, after the addition of the AMPAR antagonist DNQX (A) or the mGluR antagonist MCPG (B) to the bath saline, and after the subsequent addition of DAMGO (antagonist present). Mean values ± SEM for the amplitude of the intracellular Ca²⁺ oscillations (peak to trough measurement) in a population of neurons studied under the same conditions as in the representative recordings are shown at the right. Blocking AMPARs enhanced the intracellular Ca²⁺ oscillations but did not block the effects of DAMGO. Blocking mGluRs had only minor effects on baseline intracellular Ca²⁺ oscillations and did not block the effects of DAMGO. C, Studies with the NMDAR antagonist D-AP5. Shown are representative recordings of intracellular Ca²⁺ oscillations in cultured hippocampal neurons under baseline control conditions, after the addition of DAMGO to the bath saline, and after the subsequent addition of D-AP5. Blocking NMDARs reversed the effects of DAMGO on intracellular Ca²⁺ oscillations. D-AP5 also reduced baseline oscillations. In other experiments the addition of D-AP5 before DAMGO reduced baseline oscillations and blocked enhancement of the intracellular Ca²⁺ oscillations by DAMGO (data not shown). Mean values ± SEM for the amplitude of the intracellular Ca²⁺ oscillations (peak to trough measurement) in a population of neurons studied under the same conditions as the representative recordings are shown at the right. For all three antagonists the representative recordings are from different microscopic fields in the same culture dish; five neurons are shown for each condition. In the graphs of mean values the amplitude of the oscillations in the various treatment groups was normalized to the mean amplitude of oscillations under the respective baseline control conditions. *Significant difference from control values (p < 0.05; ANOVA). +, Significant difference from DNQX (A), MCPG (B), or DAMGO (C).

The metabotropic glutamate receptor (mGluR) antagonist MCPG (1 mM; four culture sets tested) produced small changes in theamplitude or degree of synchrony of baseline intracellular Ca²⁺ oscillations but did not block the effects of DAMGO on intracellularCa²⁺ oscillations (Fig. 3B). In contrast, the NMDAR antagonist D-AP5(50 µM; four culture sets tested) significantly reduced baselineintracellular Ca²⁺ oscillations and blocked the enhancement of the Ca²⁺ oscillations by DAMGO (data not shown). The addition of D-AP5after DAMGO reversed the enhancement of the Ca²⁺ oscillations by DAMGO (Fig. 3C). Finally, in a related seriesof studies, neither the GABA_A receptor antagonist picrotoxin northe GABA_B receptor antagonist CGP55845A blocked the action ofDAMGO to enhance intracellular Ca²⁺ oscillations (data not shown). Taken together, these resultsshow that NMDAR-mediated responses elicited by network synapticactivity play a prominent role in the generation of baseline intracellularCa²⁺ oscillations and in the augmentation of these oscillations byDAMGO, whereas synaptic events mediated by AMPARs, mGluRs, GABA_A,or GABA_B receptors are not essential for either of thesefunctions.

Involvement of Ca²⁺ channels in the regulation of intracellular Ca²⁺ oscillations by DAMGO

Activation of NMDARs depolarizes hippocampal neurons and, if the depolarization is large enough, can elicit action potentials.Voltage-sensitive Ca²⁺ channels contribute to the action potentials. Thus, network synapticactivity in the hippocampal cultures could activate voltage-sensitiveCa²⁺ channels, resulting in Ca²⁺ influx that contributes to the intracellular Ca²⁺ oscillations. To determine whether voltage-sensitive Ca²⁺ channels play a role in the intracellular Ca²⁺ oscillations, we tested the effects of L- and P-type Ca²⁺ channel blockers on the baseline Ca²⁺ oscillations and the ability of DAMGO to enhance the oscillations.The P-type Ca²⁺ channel blocker $omega$ -agatoxin IVA (200 nM; two culture sets tested)almost completely blocked baseline Ca²⁺ oscillations. Moreover, DAMGO did not induce intracellular Ca²⁺ oscillations in cultures pretreated with $omega$ -agatoxin IVA (datanot shown). These results are similar to results obtained withTTX treatment and may reflect a blockade of synaptic transmissionvia $omega$ -agatoxin IVA-mediated inhibition of presynaptic Ca²⁺ channels. Nimodipine (5 µM; three culture sets tested), an L-typeCa²⁺ channel blocker, had variable effects on baseline intracellularCa²⁺ oscillations. However, nimodipine significantly reduced the enhancementof the intracellular Ca²⁺ oscillations by DAMGO. Representative data are shown in Figure4. These results indicate that L-type Ca²⁺ channels contribute to baseline Ca²⁺ oscillations and play a prominent role in the enhancement ofintracellular Ca²⁺ oscillations by DAMGO.

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Figure 4. Effect of nimodipine on the modulation of intracellular Ca²⁺ oscillations by DAMGO. A, Representative recordings of intracellular Ca²⁺ oscillations under baseline control conditions, in the presence DAMGO, and after the addition of the L-type channel Ca²⁺ blocker nimodipine to the bath saline. Recordings are from different microscopic fields in the same culture dish; five neurons are shown for each condition. Nimodipine blocked the enhanced intracellular Ca²⁺ oscillations produced by DAMGO. Mean values ± SEM for the amplitude of the intracellular Ca²⁺ oscillations (peak to trough measurement) in a population of neurons under the same conditions as the representative recordings (same culture dish as representative recordings) are shown to the right. B, Representative recordings of intracellular Ca²⁺ oscillations under baseline control conditions, after the addition of the L-type channel Ca²⁺ blocker nimodipine to the bath saline, and after the subsequent addition of DAMGO to the bath. Recordings are from different microscopic fields in the same culture dish; five neurons are shown for each condition. Nimodipine blocked baseline intracellular Ca²⁺ oscillations and reduced the enhancement of the oscillations by DAMGO. Mean values ± SEM for the amplitude of the intracellular Ca²⁺ oscillations (peak to trough measurement) in a population of neurons under the same conditions as the representative recordings (same culture dish as representative recordings) are shown to the right. In the graphs of mean values the amplitudes of the intracellular Ca²⁺ oscillations in the various treatment groups were normalized to the mean amplitude under baseline control conditions. *Significant difference from control values (p > 0.05; ANOVA). +, Significant difference from DAMGO for DAMGO/Nimodipine; Nimodipine for Nimodipine/DAMGO.

Effect of DAMGO on membrane properties and spontaneous network electrical activity

In current-clamp recordings the cultured hippocampal neurons exhibit prominent spontaneous burst events composed of synapticpotentials and action potentials. This activity was blocked byTTX (data not shown). The intracellular Ca²⁺ oscillations also were blocked by TTX, suggesting that the burstevents contribute to generation of the intracellular Ca²⁺ oscillations. Technical limitations prevented recording of theintracellular Ca²⁺ oscillations and burst events in the same neurons. However, comparisonof intracellular Ca²⁺ oscillations and burst activity confirmed similarities in timecourse and frequency (Fig. 5; see below). Therefore, we used electrophysiologicalrecordings of the burst activity under a variety of conditionsto help elucidate the mechanisms responsible for the effects ofDAMGO on the intracellular Ca²⁺ oscillations.

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Figure 5. DAMGO alters spontaneous, synaptically driven burst activity in hippocampal neurons. A, B, Electrophysiological recordings of spontaneous burst activity in a cultured pyramidal-like hippocampal neuron under baseline control conditions and after the addition of DAMGO (1 µM) to the bath saline. The neuron exhibited repetitive burst activity under control conditions. The amplitude of the membrane depolarization during the burst and the number of spikes that were evoked were enhanced in the presence of DAMGO. C, D, For comparison purposes, representative recordings of intracellular Ca²⁺ oscillations are shown under the same conditions as in electrophysiological studies. The Ca²⁺ recordings are from in five neurons in a microscopic field. The time scale is the same for the intracellular Ca²⁺ and electrophysiological recordings. Note the similarity in the pattern of activity of spike bursts and intracellular Ca²⁺ oscillations in the presence of DAMGO.

All electrophysiological recordings were performed as outlined for the Ca²⁺ imaging experiments, and the same doses of agonists and antagonistswere used. Mean resting membrane potential (RMP) values underthe various conditions tested in the electrophysiological recordingsare shown in Table 1. In general, there was no significant effectof the treatments on RMP. However, the addition of DAMGO to thebath saline significantly enhanced the spontaneous burst events,as evidenced by an increase in amplitude of the burst depolarizationsand/or the number of action potentials comprising the burst event(Fig. 5, Table 1). The intrinsic excitability of the neurons,as determined by the number of current-evoked spikes, was notaltered by DAMGO (Table 1). In addition, DAMGO did not significantlyalter input resistance (determined from the slope of current-voltagecurves) measured at membrane potentials depolarized from rest(Table 1), indicating that alterations in passive membrane propertieswere unlikely to account for the enhancement of the burst eventsby DAMGO. DAMGO did decrease input resistance at membrane potentialshyperpolarized to rest (Table 1), perhaps because of the opioidactivation of K⁺ conductances, as has been shown to occur in acutely isolatedhippocampal neurons (Wimpey and Chavkin, 1991).


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Table 1. Effect of DAMGO on electrophysiological measurements

In the Ca²⁺ imaging studies, NMDARs were found to play a major role in the generation of baseline and DAMGO-induced intracellularCa²⁺ oscillations, whereas AMPARs were not essential (see Fig. 3).In electrophysiological recordings the AMPAR antagonists NBQX(5 µM) or DNQX (10 µM) produced some alterations in the generalform of the spontaneous burst events. However, subsequent exposureto DAMGO still enhanced the spontaneous burst events by increasingthe amplitude of the burst depolarization and/or increasing thenumber of action potentials comprising the burst event (Fig. 6,Table 1). In the presence of an AMPAR antagonist the additionof the NMDAR antagonist D-AP5 to the bath saline abolished theburst potentials observed under baseline conditions or in thepresence of DAMGO (data not shown), indicating that NMDARs areessential for the generation of the burst events.

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Figure 6. AMPARs are not required for the actions of DAMGO. Shown are electrophysiological recordings of spontaneous burst activity in a cultured hippocampal neuron under baseline control conditions after the addition of the AMPAR antagonist DNQX to the bath saline, followed by the subsequent addition of 1 µM DAMGO. DNQX produced some alterations in baseline activity but did not block the ability of DAMGO to enhance the amplitude and spike number of spontaneous burst events.

In addition to excitatory transmission mediated by glutamate receptors, inhibitory input mediated by GABA_A receptors (GABA_ARs)plays an important role in synaptic transmission in the hippocampus.Immunostaining with an antibody to GABA showed that GABA-containingneurons are present in the hippocampal cultures (see Fig. 1A,B),and these neurons could contribute an inhibitory influence tothe burst events. Opiates are known to depress inhibitory GABAsystems via both µ- and $delta$ -opioid receptors in hippocampal slicepreparations (Nicoll et al., 1980; Lupica and Dunwiddie, 1991;Cohen et al., 1992; Capogna et al., 1993; Lupica, 1995). As aconsequence, inhibitory synaptic input from the GABA-containinginterneurons to the pyramidal neurons is reduced and there isan overall increase in pyramidal neuron excitability [i.e., adisinhibitory mechanism; (Zieglgansberger et al., 1979)]. To determinewhether such a disinhibitory mechanism mediated the enhancementof the burst events by DAMGO, we investigated the ability of theGABA_AR antagonist picrotoxin to block the enhancement of the burstevents byDAMGO.

In cultures pretreated with NBQX (5 µM) to block AMPARs and simplify the synaptic network activity, the addition of picrotoxin(100 µM) to the bath saline increased the amplitude of the spontaneousburst events (Fig. 7). However, the subsequent addition of DAMGOfurther enhanced the amplitude of the burst events (Fig. 7, Table1). These results indicate that DAMGO can enhance spontaneousNMDAR-mediated burst events in the cultured hippocampal neuronsand that this enhancement is not attributable to a disinhibitorymechanism.

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Figure 7. GABA_ARs are not required for the actions of DAMGO. Shown are electrophysiological recordings of spontaneous burst activity in a cultured hippocampal neuron under baseline control conditions (5 µM NBQX is present to block AMPARs) and after the addition of the GABA_AR antagonist picrotoxin to the bath saline, followed by the subsequent addition of 1 µM DAMGO (NBQX and picrotoxin are still present). In the presence of NBQX and picrotoxin, DAMGO still enhanced the amplitude and spike number of spontaneous burst events.

DAMGO enhances the membrane response and intracellular Ca²⁺ signals to exogenously applied NMDA

The above results show that DAMGO can enhance spontaneous, synaptically driven burst events and intracellular Ca²⁺ oscillations in cultured hippocampal neurons and that these effectsinvolve NMDARs. Opiates are known to alter hippocampal synaptictransmission via both pre- and postsynaptic opioid receptors (Simmonsand Chavkin, 1996). To determine whether postsynaptic opioid receptorsare involved in the effects of DAMGO on the cultured hippocampalneurons, we tested the effect of DAMGO on membrane responses producedby brief microperfusion application of NMDA (10-200 µM; 0.25-1sec pulse) to the hippocampal neurons. In these studies the bathsaline contained TTX (0.5 µM), NBQX (5 µM), and picrotoxin (100µM) to block Na⁺ channels, AMPARs, and GABA_ARs, respectively. Micropressure applicationof NMDA elicited a prominent membrane depolarization under theseconditions (Fig. 8A). The addition of DAMGO to the bath salinesignificantly increased (p < 0.05; paired t test) the amplitudeand significantly decreased (p < 0.05; paired t test) the durationof the depolarization to NMDA in 13 of 15 neurons tested (Fig.8A). Mean values for the peak amplitude of the membrane depolarizationto NMDA for the 13 DAMGO-sensitive neurons were 40 ± 2 mV undercontrol conditions and 45 ± 2 mV in the presence of DAMGO. Meanvalues for the duration of the membrane depolarization to NMDAin the same population of neurons were 55 ± 6 sec under controlconditions and 35 ± 6 sec in the presence of DAMGO.

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Figure 8. DAMGO selectively enhances the membrane depolarization elicited by the exogenous application of NMDA. A, Representative recordings of membrane depolarizations elicited in two hippocampal neurons by brief (1 sec) micropressure application of NMDA or AMPA (at the arrows) under control conditions and after the addition of DAMGO to the bath saline. DAMGO (1 µM) increased the amplitude and decreased the duration of the membrane depolarization to NMDA. DAMGO also induced an increase in Ca²⁺ spiking (arrowhead) and a prominent AHP (double arrows) after the depolarizing phase of the response to NMDA. The response to AMPA was unaltered by DAMGO. C, In parallel Ca²⁺ imaging experiments DAMGO enhanced the intracellular Ca²⁺ signal to NMDA. Graphs show four cells in a control microscopic field and four cells in another microscopic field in the same culture dish after the addition of DAMGO to the recording saline.

In 5 of the 13 DAMGO-sensitive neurons, DAMGO altered the recovery phase of the depolarization to DAMGO by revealing (Fig.8A) or enhancing an afterhyperpolarization (AHP) that followedthe depolarizing phase of the membrane response to NMDA. Measurementof the AHP in these neurons showed that the amplitude and theduration of AHP were increased significantly by DAMGO. The meanamplitude of the AHP was 0.4 ± 0.4 mV under control conditionsas compared with 3.8 ± 1.2 mV after the addition of DAMGO to thebath saline. The mean duration of the AHP was 29 ± 29 sec undercontrol conditions as compared with 102 ± 28 sec after the additionof DAMGO to the bathsaline.

In parallel Ca²⁺ imaging studies DAMGO significantly enhanced the intracellular Ca²⁺ signal elicited by the exogenous application of NMDA to the hippocampalneurons (Fig. 8C), consistent with the larger membrane responseobserved in the electrophysiological studies (Fig. 8A). Mean valuesfor the peak amplitude of the intracellular Ca²⁺ signal to NMDA (resting levels subtracted) were 32 ± 1 nM (n= 184) under control conditions and 40 ± 1 nM (n = 235) in thepresence of DAMGO (p < 0.05; unpaired t test), an ~28% increase.DAMGO also produced a small but significant increase in restingCa²⁺ levels in these studies. The mean resting Ca²⁺ level was 45 ± 1 nM (n = 184) under control conditions and 52± 1 nM (n = 235) in the presence of DAMGO (p < 0.05; unpairedt test), an ~13%increase.

DAMGO does not alter the membrane response to exogenously applied AMPA

In addition to NMDARs, AMPARs are involved in glutamate-mediated synaptic transmission in the hippocampal cultures. Thus,it was of interest to determine whether the effects of DAMGO wereselective for membrane depolarizations mediated by NMDARs or whethermembrane depolarizations mediated by AMPARs could be affectedas well. For these studies the bath saline contained TTX (0.5µM), D-AP5 (100 µM), and picrotoxin (100 µM) to block Na⁺ channels, NMDARs, and GABA_ARs, respectively. Brief microperfusionof AMPA (1-2 µM; 1 sec pulse; applied as for NMDA) elicited amembrane depolarization in all seven cultured hippocampal neuronsthat were tested (Fig. 8B). The addition of DAMGO to the bathsaline had no effect on the membrane depolarization to AMPA (Fig.8B); mean values for the peak amplitude and duration of the responseto AMPA were 24 ± 4 mV and 68 ± 12 sec, respectively, under bothconditions (p > 0.05; paired ttest).

DAMGO enhances Ca²⁺ spiking

Large membrane depolarizations in response to NMDA application elicited Ca²⁺-dependent spikes in the cultured hippocampal neurons (TTX, NBQX,and picrotoxin present in the recording medium; Fig. 8A). TheCa²⁺ spiking was more pronounced after the addition of DAMGO to therecording medium (Fig. 8A), possibly because of the enhancementof the depolarization to NMDA by DAMGO. Alternatively, DAMGO couldact to enhance Ca²⁺ spiking by affecting either Ca²⁺ or K⁺ currents directly. To test this possibility, we examined theeffect of DAMGO on Ca²⁺ spiking elicited by depolarizing current pulses. In 6 of 11 neuronsthat showed Ca²⁺ spiking under baseline conditions, DAMGO increased the numberor amplitude of the Ca²⁺ spikes (Fig. 9). In the remaining five neurons the Ca²⁺ spikes were unaltered or slightly depressed by DAMGO. Nimodipine(1-5 µM) reduced the Ca²⁺ spikes in six of six neurons that were tested (data not shown),suggesting that L-type Ca²⁺ channels contributed to the Ca²⁺ spiking. Nimodipine did not alter the enhancement of the membranedepolarization to NMDA by DAMGO, indicating that the actions ofDAMGO on network synaptic activity involve multiple mechanisms.The mean values for the peak amplitude of the membrane depolarizationto NMDA in five neurons tested were 34 ± 3 mV under control conditions,40 ± 4 mV in the presence of DAMGO, and 43 ± 2 after the additionof nimodipine to the recording saline (DAMGO still present).

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Figure 9. DAMGO enhances Ca²⁺ spiking. A, B, Voltage responses elicited by intracellular application of two depolarizing (+150 and +250 pA) and two hyperpolarizing ( $-$ 30 and $-$ 50 pA) current pulses in a hippocampal neuron under control conditions and after the addition of DAMGO to the bath saline. TTX, NBQX, and picrotoxin were present in the bath saline. DAMGO increased the Ca²⁺ spiking elicited by the depolarizing current pulses.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study we identified a novel opioid mechanism in cultured hippocampal neurons that may play a role in opioid regulationof neuronal activity in synaptic pathways in situ. The opioidreceptor agonist DAMGO significantly increased the amplitude ofTTX-sensitive intracellular Ca²⁺ oscillations in the cultured hippocampal neurons, with synchronizationof the Ca²⁺ oscillations across neurons in a given field. These actions ofDAMGO were blocked by the opioid receptor antagonist naloxone,indicating that opioid receptors, presumably µ-opioid receptors,mediated the opioid effects. Spontaneous TTX-sensitive burst depolarizationsalso were shown to be enhanced by DAMGO in the cultured hippocampalneurons and to be likely initiators of the Ca²⁺ oscillations. Studies with selective glutamate receptor antagonistsrevealed that functional NMDARs were required for the enhancementof intracellular Ca²⁺ oscillations and burst events by DAMGO, whereas AMPARs and mGluRswere not essential. Further studies showed that intracellularCa²⁺ signals and depolarizing responses evoked by exogenously appliedNMDA were augmented by DAMGO, supporting a link between opioidreceptors and NMDARs in the hippocampal neurons. The NMDARs presumablyprovide a major pathway for the Ca²⁺ influx that contributes to the intracellular Ca²⁺ oscillations. In addition, L-type Ca²⁺ channels were identified as important contributors to the enhancementof the Ca²⁺ oscillations by DAMGO, and their involvement appears to resultfrom an enhancement of Ca²⁺-dependent spiking by DAMGO. Taken together, these results showthat the activation of opioid receptors can influence severalcomponents of neuronal Ca²⁺ signaling pathways in cultured hippocampal neurons and, as aconsequence, enhance intracellular Ca²⁺levels.

Several lines of evidence indicate that the spontaneous intracellular Ca²⁺ oscillations and burst depolarizations observed under baselineconditions (low Mg²⁺) and in the presence of DAMGO were generated by network synapticactivity. The intracellular Ca²⁺ oscillations and burst depolarizations showed a similar patternof activity, sensitivity to TTX (which blocks synaptic transmission),and sensitivity to transmitter receptor antagonists. These observationsare consistent with studies of cultured cortical neurons (Roseet al., 1990; Murphy et al., 1992; Robinson et al., 1993) andcultured hippocampal neurons (Shen et al., 1996), in which spontaneousperiodic intracellular Ca²⁺ oscillations were shown to correlate with spontaneous synapticpotentials and to be blocked by TTX. In studies of cultured corticalneurons Rose et al. (1990) found that the spontaneous intracellularCa²⁺ oscillations could be blocked by the NMDAR antagonist D-AP5,as in the current study. In contrast, Shen et al. (1996) reportedthat spontaneous intracellular Ca²⁺ oscillations in cultured hippocampal neurons were blocked bythe AMPA/kainate receptor antagonist CNQX, whereas D-AP5 causedonly a partial depression. These combined results show that intracellularCa²⁺ oscillations in CNS neurons can be mediated by NMDA and/or non-NMDAsubtypes of glutamatergic receptors. Similar conclusions werereached in studies of cultured cortical neurons by Murphy et al.(1992) and Robinson et al. (1993). Several factors are likelyto play a role in determining the relative contribution of NMDARsand non-NMDARs to the intracellular Ca²⁺ oscillations and associated synaptic events in the cultured neurons,such as the neuronal composition of the cultures, the circuitryestablished, and the experimental conditions (e.g., Mg²⁺ level in the bathsaline).

DAMGO increased the amplitude of the intracellular Ca²⁺ oscillations in the cultured hippocampal neurons. DAMGO also enhancedspontaneous burst events, consistent with a role of the burstevents in the generation of the intracellular Ca²⁺ oscillations. The enhancement of burst events by DAMGO couldarise from an increase in excitatory synaptic transmission ora decrease in inhibitory synaptic transmission (i.e., a disinhibitorymechanism). Blockade of GABA_AR-mediated responses with picrotoxinenhanced the amplitude of the spontaneous burst events in thehippocampal neurons, showing that GABA-containing neurons providedan inhibitory component to the network synaptic activity. However,treatment with picrotoxin did not prevent the augmentation ofthe burst events by DAMGO. Thus, an opioid disinhibitory mechanismdoes not appear to explain ourresults.

Although GABA_ARs were not required for the enhancement of the spontaneous Ca²⁺ oscillations and burst events by DAMGO in the cultured hippocampalneurons, our results show that glutamate and NMDARs play a criticalrole. The near-total blockade of opioid-induced intracellularCa²⁺ oscillations by the NMDAR antagonist D-AP5, an action that mimickedthe effects of TTX, suggests that NMDARs presynaptic (i.e., "upstream")to the imaged neurons could be involved in the enhanced intracellularCa²⁺ oscillations and burst events. Alternatively, the opioid enhancementof the Ca²⁺ oscillations could arise from potentiation of postsynaptic currentsmediated by NMDARs, as described by Chen and Huang (1991) andMartin et al. (1997). This possibility is supported by our findingof DAMGO potentiation of membrane depolarizations elicited byexogenous application of NMDA (but not AMPA) to the hippocampalneurons. The potentiation of NMDA responses by opioid receptoragonists in spinal neurons appears to be mediated by the activationof protein kinase C (PKC; Chen and Huang, 1991). A similar PKC-dependenteffect could be involved in the presentfindings.

In the current study the P-type Ca²⁺ channel antagonist $omega$ -agatoxin IVA blocked the spontaneous and opioid-induced intracellularCa²⁺ oscillations in the cultured hippocampal neurons. P-type Ca²⁺ channels are implicated in transmitter release (Luebke et al.,1993), supporting a role for synaptic transmission in the generationof the Ca²⁺ oscillations. Moreover, the synchronization of the Ca²⁺ oscillations across neurons in a microscopic field strongly supportsthe participation of presynaptic elements, probably via the networkor feedback interconnectivity functions of the cultures. Opioidregulation of N- and P/Q-types of Ca²⁺ channels has been demonstrated in native neurons (Gross and MacDonald,1987; Schroeder and McCleskey, 1993; Moises et al., 1994) andhas been thought to contribute to opioid depression of synaptictransmission (North and Lovinger, 1993). Although an inhibitionof synaptic responses by DAMGO was not observed in the currentstudy, opioid actions at N- or P/Q-type Ca²⁺ channels could contribute in a covert way to the effects of DAMGOon network synapticactivity.

In addition to the regulation of N and P/Q Ca²⁺ channels, opioid receptors have been shown to regulate L-type Ca²⁺ channels. Thus, opioids increase intracellular Ca²⁺ by inducing Ca²⁺ influx via dihydropyridine-sensitive (i.e., L-type) Ca²⁺ channels in neuronal-like cell lines that express opioid receptors(Jin et al., 1992; Tang et al., 1994). In the current study theL-type Ca²⁺ channel blocker nimodipine reduced the enhancement of intracellularCa²⁺ oscillations by DAMGO with variable effects on baseline Ca²⁺ oscillations. This result suggests that postsynaptic L-type Ca²⁺ channels are involved in the DAMGO enhancement of the intracellularCa²⁺ oscillations, because L-type Ca²⁺ channels are reported to be localized predominantly postsynapticallyin hippocampal neurons (Westenbroek et al., 1990). A role forpostsynaptic Ca²⁺ channels is supported further by our finding that DAMGO enhancedthe Ca²⁺-dependent spikes evoked by intracellular depolarizing currentinjections, and these spikes were blocked by the L-type Ca²⁺ channel blockernimodipine.

Recent studies in neuron-like cell lines and transfected cells have shown that opioid receptors are coupled to various signalingpathways involved in Ca²⁺ homeostasis, including inhibition (Jin et al., 1992, 1993; Fieldset al., 1995) or activation (Jin et al., 1992; Tang et al., 1994)of Ca²⁺ channels, mobilization of Ca²⁺ from intracellular stores (Tomura et al., 1992; Jin et al., 1994;Fields et al., 1995; Connor et al., 1997), and activation of phospholipaseC (Okajima et al., 1993; Johnson et al., 1994), the enzyme responsiblefor generation of the Ca²⁺ mobilizing messenger inositol 1,4,5-trisphosphate (IP₃). In thecurrent studies the potential involvement of intracellular Ca²⁺ stores in the enhancement of the intracellular Ca²⁺ oscillations by DAMGO was not evaluated. However, in the presenceof GABA_AR and glutamate receptor antagonists, DAMGO elicited asmall increase in baseline Ca²⁺ levels, an effect that could involve the release of Ca²⁺ from intracellular stores. Actions of DAMGO on other Ca²⁺-sensitive pathways or components such as membrane pumps or transportsystems cannot be eliminated at this time. Membrane potentialchanges are unlikely to mediate the effects on baseline Ca²⁺ levels, because DAMGO did not alter resting membrane potentialwhen synaptic transmission was blocked by GABA_AR and glutamatereceptorantagonists.

The dual action of opioids in augmenting responses mediated by NMDARs and L-type Ca²⁺ channels provides a novel mechanism through which opioids cancontrol the excitability of CNS neurons. NMDARs and L-type Ca²⁺ channels often are activated simultaneously by synaptic signalsand could interact synergistically to influence excitatory driveand regulate biochemical pathways controlled by intracellularCa²⁺ concentrations. Moreover, Ca²⁺ oscillations are known to be a particularly effective regulatorymechanism for the control of gene expression (Dolmetsch et al.,1998; Li et al., 1998). By virtue of the large number of cellularprocesses regulated by Ca²⁺, increased intracellular Ca²⁺ or enhanced Ca²⁺ oscillatory activity could play a major role in the opioid regulationof CNS neuronal function. Such second messenger regulation couldaccount for some of the long-term effects of opioids such as opioideffects on synaptic plasticity and genomic regulation (Nestlerand Aghajanian, 1997).

  FOOTNOTES

Received May 20, 1999; revised Aug. 24, 1999; accepted Sept. 1, 1999.

This work was supported by National Institutes of Health Grants AA06420 (D.L.G.), DA03665 (G.R.S.), and Fullbright Fellowship18619 (R.P.). We thank Jody Caguioa for technical assistance andperforming some of the experiments, Floriska Chizer for secretarialassistance, Pfizer for the gift of $omega$ -agatoxin IVA, and Novartisfor the gift ofCGP55845A.
Correspondence should be addressed to Dr. Donna Gruol, Department of Neuropharmacology, CVN 11, The Scripps Research Institute,10550 North Torrey Pines Road, La Jolla, CA92037.

Dr. Przewlocki's present address: Department of Molecular Neuropharmacology, Institute of Pharmacology, SMETNA 12, 31-343Krakow,Poland.

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Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH
Hazardous Substances DB
CALCIUM COMPOUNDS
CALCIUM, ELEMENTAL
NALOXONE
TETRODOTOXIN