Modulation of Amphetamine-Stimulated [3H]Dopamine Release from Rat Pheochromocytoma (PC12) Cells by sigma  Type 2 Receptors

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Vol. 289, Issue 1, 278-284, April 1999

Modulation of Amphetamine-Stimulated [³H]Dopamine Release from Rat Pheochromocytoma (PC12) Cells by $sigma$ Type 2 Receptors¹

John K. Weatherspoon and Linda L. Werling

Department of Pharmacology, The George Washington University Medical Center, Washington, DC

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

An important regulatory mechanism of synaptic dopamine (DA) levels is activation of the dopamine transporter (DAT), whichis a target for many drugs of abuse, including amphetamine (AMPH). $sigma$ receptors are located in dopaminergic brain areas critical toreinforcement. We found previously that agonists at $sigma$ ₂ receptorsenhanced the AMPH-stimulated release of [³H]DA from slices of rat caudate-putamen. In the present study,we modeled this response in undifferentiated pheochromocytoma-12(PC12) cells, which contain both the DAT and $sigma$ ₂ receptors butnot neural networks that can complicate investigation of individualneuronal mechanisms. We found that enhancement of AMPH-stimulated[³H]DA release by the $sigma$ agonist (+)-pentazocine was blocked by $sigma$ ₂receptor antagonists. Additionally, the reduction in the effectof (+)-pentazocine by the inclusion of ethylene glycol bis( $beta$ -aminoethylether)-N,N,N',N'-tetraacetic acid led us to hypothesize that $sigma$ ₂receptor activation initiated a Ca²⁺-dependent process that resulted in enhancing the outward flowof DA via the DAT. The source of Ca²⁺ required for the enhancement of reverse transport did not appearto be via N- or L-type voltage-dependent Ca²⁺ channels, because it was not affected by nitrendipine or $omega$ -conotoxin.However, two inhibitors of Ca²⁺/calmodulin-dependent protein kinase II blocked enhancement inAMPH-stimulated release by (+)-pentazocine. Our findings suggestthat $sigma$ ₂ receptors are coupled to the DAT via a Ca²⁺/calmodulin-dependent protein kinase II transduction system inPC12 cells, and that $sigma$ ₂ receptor antagonists might be useful inthe treatment of drug abuse by blocking elevation of DA levelsvia reversal of theDAT.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Regulation of catecholamine levels in brain is critical to maintenance of mood and emotional well being. In particular, thereward system is dependent upon dopaminergic activity in the nucleusaccumbens. Several drugs of abuse, including amphetamine (AMPH)and cocaine exert their primary effects via actions at the dopaminetransporter (DAT), which is responsible for the reaccumulationof ~80% of released dopamine (DA). Recently, much emphasis hasbeen placed on regulation of transporter activity as a means oftreating drugabuse.

$sigma$ Receptors are present in dopaminergic brain areas (Gundlach et al., 1986), including striatum and nucleus accumbens. Althoughthe distribution and binding profiles of $sigma$ receptors are fairlywell established, relatively little is known about their functionand less about their associated signal transduction mechanisms.We have reported previously that agonists acting at $sigma$ ₂, but not $sigma$ ₁ receptors, enhance [³H]DA release stimulated by AMPH acting via the DAT (Izenwasseret al., 1998). In contrast, agonists acting at $sigma$ receptors ofboth the $sigma$ ₁ and $sigma$ ₂ types inhibit release of vesicular [³H]DA from dopaminergic terminal fields in rodent brain (Gonzalez-Alvearand Werling, 1994; Weatherspoon et al., 1996). Measuring the releaseof catecholamines and the mechanisms underlying the regulationof release in brain tissue presents difficulties including a complexneural network, problems associated with drug penetration, andthe presence of multiple types of $sigma$ receptors. For these reasons,in the present study we have further investigated the interactionsbetween AMPH-stimulated [³H]DA release and $sigma$ receptors using rat pheochromocytoma (PC12)cells (Greene and Tischler, 1976) as a model system. PC12 cellsare of a uniform population and have been reported to bear $sigma$ receptorsprimarily of the $sigma$ ₂ type (Hellewell and Bowen, 1990). These investigatorsdid not detect the presence of $sigma$ ₁ receptors in PC12 cells, althougha recent report on differentiated PC12 cells discussed the possibleexpression of the $sigma$ ₁ receptor (Sagi et al., 1996). UndifferentiatedPC12 cells are also well characterized in terms of their abilityto accumulate, store, and release DA via the DAT (Kadota et al.,1996) and have been used previously to examine second messengersystems involved in vesicular catecholamine release (Shafer andAtchison, 1991). Although a protein with binding characteristicsof the $sigma$ ₁ receptor has been cloned (Hanner et al., 1996), at thistime no report of $sigma$ ₂ receptor cloning has beenmade.

In the present study, we show that activation of $sigma$ ₂ receptors by the agonist (+)-pentazocine enhances the ability of AMPHto stimulate [³H]DA release from PC12 cells. The enhancement is reversed by nonsubtype-selective $sigma$ receptor antagonists and by a $sigma$ ₂ receptor-selective antagonistbut not by a $sigma$ ₁ receptor-selective antagonist. We also demonstratethat although the AMPH-stimulated [³H]DA release is not dependent upon exogenous Ca²⁺, addition of the calcium chelator ethylene glycol bis( $beta$ -aminoethylether)-N,N,N',N'-tetraacetic acid (EGTA) reduces the enhancementof stimulated release by (+)-pentazocine. We also provide evidencethat the enhancement of AMPH-stimulated [³H]DA release by (+)-pentazocine is dependent upon Ca²⁺/calmodulin-dependent protein kinase II (Ca²⁺/CaM kinase II) by showing that two different inhibitors of theenzyme block the enhancing effects of (+)-pentazocine. Togetherthese findings provide the first evidence for a second messengersystem associated with $sigma$ receptor regulation of DAT activity inPC12cells.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Chemicals and Reagents. The following drugs and reagents were kindly provided by or obtained from the following sources: AMPH, 1,2-bis(2-amino-phenoxy)ethane-N,N,N,N-tetraaceticacid acetoxymethyl ester (BAPTA-AM), domperidone, 1,3-di(2-tolyl)guanidine(DTG), 1-[2-[bis(4-fluorophenyl)methoxy]ethyl]-4-[3-phenylpropyl]piperazinedihydrochloride (GBR-12909), 2-[N-(4'-methoxybenzenesulfonyl)]amino-N-(4'-chlorophenyl)-2-propenyl-N-methylbenzylaminephosphate (KN-92), N-[2-[[[3-(4'-chlorophenyl)-2-propenyl]methylamino]methyl]phenyl]-N-(2-hydroxyethyl)-4'-methoxy-benzene-sulfonamidephosphate (KN-93), nisoxetine hydrochloride, nitrendipine, andyohimbine hydrochloride (Research Biochemicals International,Natick, MA); N-[2-(3,4-dichlorophenyl)-ethyl]N-methyl-2-pyrrolidinyl)ethylamine (BD1008) (Dr. Wayne Bowen and Dr. Brian de Costa, NationalInstitute of Diabetes and Digestive and Kidney Diseases, NationalInstitutes of Health, Bethesda, MD); endo-N-(8-methyl-8-azabicyclo[3.2.1.]oct-3-yl)-2,3-dihydro-(1-methyl)ethyl-2-oxo-1H-benzimidazole-1-carboxamidehydrochloride;(BIMU-8) (Dr. Doug Bonhaus, Roche Bioscience, Palo Alto, CA);[³H]DA (specific activity, 46 to 51 Ci/mmol) and [³H]NE (specific activity, 42 Ci/mmol) (Amersham Corp., ArlingtonHeights, IL); Dulbecco's Modified Eagle's Medium (DMEM), fetalbovine serum (heat-inactivated), penicillin/streptomycin, andtrypsin-EDTA (Life Technologies, Inc., Grand Island, NY); 1-(cyclopropylmethyl)-4-2'-4"-fluorophenyl)-2'-oxoethyl)-piperidinehydrogen bromide DuP734 (Drs. William Tam and Rob Zaczek, Du PontMerck Pharmaceutical Co., Wilmington, DE); EGTA and $omega$ -conotoxinfrom Conus geographus (GVIA) ( $omega$ -CgTX; Sigma Chemical Co., St.Louis, MO); horse serum (Biofluids, Rockville, MD); KN-62 (Calbiochem,La Jolla, CA); and (+)-pentazocine (Research Technology Branch,National Institute on Drug Abuse, Rockville,MD).

Tissue Culture of PC12 Cells. Adherent PC12 cells were obtained from Dr. Anne Murphy (Department of Biochemistry, The George Washington University MedicalCenter, Washington, DC). This line of PC12 cells was originallyobtained from John A. Wagner of the Cornell Medical College (NewYork, NY). The PC12 cells were routinely maintained in 175 cm² culture flasks (Nunclon) in 5% CO₂/95% air at 37°C in DMEM (LifeTechnologies, Inc.) containing 10% fetal bovine serum (heat-inactivated;Life Technologies, Inc.), 5% horse serum (Biofluids), 100 units/mlpenicillin, and 100 µg/ml streptomycin (Life Technologies, Inc.).Cells were fed approximately three times/week and passaged bygentle trituration approximately twice a week at a split ratioof 1:4. Cells were harvested using 0.05% trypsin/0.53 mM EDTA(Life Technologies, Inc.) and counted using 0.04% trypan blue(in PBS) with a Bright-Line hemacytometer (Reichert ScientificInstruments) and an inverted microscope (Cambridge Instruments).Cells of passage number no greater than 20 were used forexperiments.

Measurement of [³H]DA Release Using PC12 Cells. Release of [³H]DA from PC12 cells was determined using methods adapted from procedures established in this lab for brain tissueslices (Gonzalez-Alvear and Werling, 1994). PC12 cells were maintainedin DMEM and harvested at a density of ~6.0 × 10⁶ to 1.0 × 10⁷ cells/ml for a total cell number of ~1.0 × 10⁸ to 2.0 × 10⁸ cells per experiment, which were ultimately divided into 18 samples.This cell number was found to elicit consistent, measurable DArelease in each experiment. The cells were then centrifuged at1500 rpm for 3 min, and the medium was removed. Cells were resuspendedin 20 ml of oxygenated modified Krebs-HEPES buffer containingMg²⁺ but no Ca²⁺ (MKB: 127 mM NaCl, 5 mM KCl, 1.3 mM NaH₂PO₄, 15 mM HEPES, 10mM glucose, and 1.2 mM MgSO4; pH adjusted to 7.4 with NaOH). Thecell suspension was dispersed using a vortex mixer and again centrifugedat 1500 rpm for 3 min, and the buffer supernatant was removed.The cells were then resuspended in 20 ml ofMKB, gently dispersedusing a vortex mixer, and incubated with 15 nM [³H]DA, 0.1 mM ascorbic acid, and 100 nM nisoxetine for 30 min whileoxygenated at 37°C. Nisoxetine was included to reduce any contributionof the NE transporter to accumulation of [³H]DA by the PC12 cells. At the end of the 30-min incubation, thecells were centrifuged at 1500 rpm for 3 min, and the supernatantwas removed. The cells were resuspended in 20 ml of MKB, centrifugedagain, and the supernatant was removed. Cells were then resuspendedin a final volume of 5 ml MKB containing 1 µM domperidone (MKD)and gently dispersed by a vortex mixer. Domperidone was includedin all subsequent steps of the experiment to prevent activationof DA autoreceptors by the released [³H]DA. The total uptake of [³H]DA was typically between 0.5 and 1 pmol/batch of cells usedin an experiment. The cells were then distributed in 250-µl aliquotsbetween glass fiber filter discs into chambers of a BRANDEL (Gaithersburg,MD) superfusion apparatus. MKB was superfused over the tissueat a flow rate of 0.6 ml/min. Buffers were oxygenated throughoutthe experiments. A low, stable baseline release of ~0.9% per 2-mincollection interval was established over a 30-min period. In initialexperiments, we established that a 6-min exposure to AMPH as astimulus was required to produce reproducible, measurable release.After the 6-min S1 period, the inflow was returned to a nonstimulatingbuffer (interstimulus interval) for a period of 10 min. If a potentialinhibitor of release was being tested, it was introduced duringthis time. The cells were then stimulated a second time for 6min with AMPH in the presence or absence of another drug as appropriate(stimulus 2; S2). Inflow was again returned to nonstimulatingbuffer to allow re-establishment of baseline release. The meanfractional [³H]DA release stimulated by 25 µM AMPH in S1 was 3.9 ± 0.28% oftotal [³H]DA in the tissue at the beginning of the S1. The typical ratioof S2/S1 for AMPH stimulation was 0.6. In experiments to examinefor potential effects of EGTA on [³H]DA release, 1 mM EGTA was included in the buffer throughoutthe experiment. Radioactivity remaining in the tissue was thenextracted by a 45-min exposure to 0.2 N HCl. Superfusates werecollected at 2-min intervals in scintillation vials, and releasedradioactivity was determined by liquid scintillationspectroscopy.

In control experiments in which we sought to determine whether $sigma$ receptor agonists had any effect on AMPH-stimulated [³H]NE release from PC12 cells, the same conditions were used formeasuring [³H]DA release as described above, except for the following. Thecells were loaded with 50 nM [³H]NE and 0.1 mM ascorbic acid in the presence of a 100 nM concentrationof GBR-12909, a selective DA reuptake inhibitor, for the 30-minincubation period. We included GBR-12909 in these experimentsto prevent any accumulation of [³H]NE into the cells via the DAT. We have demonstrated previouslythat this concentration of GBR-12909 completely blocks DA reuptakevia the DAT (Izenwasser et al., 1990

; Weatherspoon et al., 1996

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Our previous results in rat brain tissue revealed that a 10 µM concentration of AMPH produced a consistent, measurable releaseof preloaded [³H]DA (Izenwasser et al., 1998) from rat striatal slices. We constructeda concentration-response curve for AMPH (0.1-50.0 µM) in PC12cells and observed a concentration-related increase in stimulationof [³H]DA release, with a fractional release at 25 µM AMPH of 3.9 ±0.28%. Stimulation with 25 µM AMPH produced a more consistentsignal that was enhanced by (+)-pentazocine with a lower variabilitythan stimulation of release by a 10 µM concentration of AMPH,which we had used in brain slices. We therefore adopted 25 µMAMPH as our standardstimulus.

We have determined previously that, at the concentrations that produced enhancement of AMPH-stimulated [³H]DA release from slices of rat caudate putamen, (+)-pentazocine(10 nM to 100 µM) had no effect on the uptake of [³H]DA in either slices or synaptosomes prepared from the same brainregion (Izenwasser et al., 1998). In the present study, we testeda range of concentrations of (+)-pentazocine on [³H]DA release stimulated by 25 µM AMPH in PC12 cells. In theseexperiments, the higher concentrations of (+)-pentazocine (500to 1000 nM) significantly enhanced release stimulated by AMPH(Fig. 1), suggesting that activation of $sigma$ ₂ receptors was morelikely responsible for the enhancement than activation of $sigma$ ₁ receptors.

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Fig. 1. Effects of (+)-pentazocine on AMPH-stimulated [³H]DA release from PC12 cells. Data are expressed as percentage of control-stimulated release with baseline release subtracted. Release of [³H]DA was stimulated by 25 µM AMPH in the presence of the indicated concentration of (+)-pentazocine. *Significantly different from control by ANOVA with posthoc Dunnett's (p < .05). Statistical analysis was performed on untransformed data (S2/S1) as described in Materials and Methods; n = 7.

In additional experiments, we sought to confirm whether the enhancement by (+)-pentazocine was mediated via activation ofeither $sigma$ ₁ or $sigma$ ₂ receptors. In brain tissue, (+)-pentazocine hasa K_i at $sigma$ ₁ receptors of 2-6 nM and at $sigma$ ₂ receptors of about 1.5µM (Vilner and Bowen, 1992). In PC12 cells, the K_i for (+)-pentazocineat $sigma$ ₂ receptors has been reported to be 1 µM (Hellewell and Bowen,1990). We tested the effects of several $sigma$ receptor antagonistsat concentrations chosen to occupy $>=$ 50% of their preferred $sigma$ receptorsubtype on [³H]DA release stimulated by 25 µM AMPH in the presence of 500 nM(+)-pentazocine. The $sigma$ ₂ receptor antagonists BIMU-8 (100 nM),as well as the nonsubtype selective $sigma$ antagonists DTG (100 nM)and BD1008 (10 nM), each produced a significant reversal of theenhancement of AMPH-stimulated release by 500 nM (+)-pentazocine(Fig. 2). In contrast, the $sigma$ ₁ receptor-selective antagonist DuP734(100 nM) did not have a significant effect on the enhancementof release by (+)-pentazocine. No $sigma$ receptor antagonist testedhad any significant effect on basal release. Basal fractionalrelease in the absence of drug was 0.9 ± 0.21% per 2-min collectioninterval, whereas basal fractional release for the same time intervalin the presence of BIMU-8 was 0.84 ± 0.42%, in the presence ofDuP734 was 1.3 ± 0.84%, in the presence of DTG was 1.0 ± 0.47%,and in the presence of BD1008 was 1.8 ± 0.9%.

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Fig. 2. Effects of $sigma$ receptor antagonists on (+)-pentazocine-mediated enhancement of 25 µM AMPH-stimulated [³H]DA release from PC12 cells. Release was stimulated by 25 µM AMPH in the presence or absence of (+)-pentazocine (500 nM) and a $sigma$ receptor antagonist as indicated. Concentrations of drugs were: BIMU-8, 100 nM; DuP734, 100 nM; DTG, 100 nM; and BD1008, 10 nM. Data are expressed as percentage of release stimulated by AMPH alone (percentage of control-stimulated release). *Enhancement of stimulated release by (+)-pentazocine (500 nM) alone was significantly different from control by ANOVA and posthoc Dunnett's (two-tailed; p < .05). #Enhancement by (+)-pentazocine alone was significantly different from release in the presence of (+)-pentazocine plus antagonist by ANOVA and posthoc Dunnett's (two-tailed; p < .05). Statistical analysis was performed on untransformed data (S2/S1) as described in Materials and Methods; n = 3.

Because DA is the precursor for the synthesis of NE, we also tested whether activation of $sigma$ ₂ receptors could regulate therelease of [³H]NE via the norepinephrine transporter (NET). We observed thatthe total uptake of [³H]NE was low in these experiments, as compared with the totaluptake of [³H]DA observed in other experiments using PC12 cells; the totaluptake (mean ± S.D.) of [³H]NE was 18.3 ± 4.9% of total [³H]DA uptake under the same conditions (n = 2). AMPH did not consistentlystimulate a reliably measurable amount of [³H]NE release, probably due to the low accumulation of transmitter.We did not detect any effect of (+)-pentazocine on [³H]NE release stimulated by 25 µM AMPH; the mean values ± S.D.for percentage of stimulated release were 100 ± 10.8% (AMPH alone),91.6 ± 16.1% [AMPH + 500 nM (+)-pentazocine], and 95.6 ± 7.3%[AMPH + 1 µM (+)-pentazocine] (n = 2). These results suggest thatthe (+)-pentazocine-mediated enhancement of AMPH-stimulated [³H]DA release we observed in PC12 cells was due to actions at theDAT and not theNET.

Because we have shown previously that chelation of Ca²⁺ with EGTA prevents the (+)-pentazocine-mediated enhancement of AMPH-stimulated[³H]DA release from rat striatal slices by $sigma$ receptor agonists (Izenwasseret al., 1998), we performed experiments to determine whether Ca²⁺ would similarly be required for the (+)-pentazocine-mediatedeffect in PC12 cells. In this set of experiments, (+)-pentazocineagain produced an enhancement of AMPH-stimulated [³H]DA release at the higher concentrations tested (500 to 1000nM) as compared with control (p < .05 by ANOVA with posthoc Dunnett's),as found previously. In the presence of 1 mM EGTA, (+)-pentazocinedid not produce a significant enhancement of [³H]DA release stimulated by 25 µM AMPH at any concentration tested(Fig. 3). A significant difference was detected comparing theeffect of 500 nM and 1000 nM (+)-pentazocine in the presence versusthe absence of EGTA. These results suggest that Ca²⁺ is required for (+)-pentazocine to enhance release stimulatedby AMPH in PC12 cells. We also tested the intracellular Ca²⁺ chelator BAPTA-AM (10 µM) in an attempt to identify the sourceof Ca²⁺ required to support the (+)-pentazocine-mediated effect. Althoughthe BAPTA-AM treatment did not affect cell viability as measuredby trypan blue exclusion, the inclusion of BAPTA-AM in the superfusionbuffer greatly reduced the ability of AMPH to stimulate release,making it impossible to detect whether it specifically influencedthe effect of (+)-pentazocine on release. We therefore chose otherapproaches to investigate the potential role of calcium in the(+)-pentazocine-mediated effects on AMPH-stimulated [³H]DA release.

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Fig. 3. Effects of EGTA in the presence or absence of (+)-pentazocine on AMPH-stimulated [³H]DA release from PC12 cells. Data are expressed as percentage of control-stimulated release with baseline release subtracted. Release of [³H]DA was stimulated by 25 µM AMPH in the presence or absence of (+)-pentazocine and in the absence (hatched columns) or presence (open columns) of EGTA (1 mM). *Significantly different from control by ANOVA with posthoc Dunnett's (p < .05) and also different from the same concentrations of (+)-pentazocine in the presence of EGTA. There was no significant effect of (+)-pentazocine compared with control at any concentration in the presence of EGTA. Statistical analysis was performed on untransformed data (S2/S1) (see Materials and Methods); n = 7 for control and 4 for EGTA.

If the Ca²⁺ required for the (+)-pentazocine-mediated effect in PC12 cells originates externally, it might enter via a voltage-dependentcalcium channel (VDCC). Both L- and N-type VDCC are present inPC12 cells (Shafer and Atchison, 1991). We evaluated the effectof nitrendipine, a selective inhibitor of L-type VDCC, as wellas the selective N-type VDCC blocker $omega$ -conotoxin GVIA ( $omega$ -CgTX)on $sigma$ receptor regulation of AMPH-stimulated [³H]DA release. Both compounds were tested at 100 nM, a concentrationthat should produce complete blockade of the respective VDCC.Whereas nitrendipine alone had no effect compared with control-stimulatedrelease, $omega$ -CgTX produced a slight enhancement of release in theabsence of (+)-pentazocine, but this effect was not statisticallysignificant. As seen previously, (+)-pentazocine (1 µM) alonesignificantly enhanced [³H]DA release stimulated by 25 µM AMPH, compared with release stimulatedby AMPH alone (Fig. 4). The release in the presence of (+)-pentazocine+ $omega$ -conotoxin was also significantly different from control stimulatedrelease. Neither nitrendipine nor $omega$ -CgTX had any significant effecton the enhancement mediated by (+)-pentazocine. Thus, it appearedthat neither the L- nor the N- type VDCC was responsible for supplyingthe Ca ²⁺ needed to support the enhancing effect of (+)-pentazocine onAMPH-stimulated release.

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Fig. 4. Effects of nitrendipine (NTP) and $omega$ -CgTX on (+)-pentazocine-mediated enhancement of AMPH-stimulated [³H]DA release from PC12 cells. Release was stimulated by 25 µM AMPH in the presence or absence of (+)-pentazocine (1 µM) and nitrendipine (100 nM) or $omega$ -CgTX (100 nM) as indicated. Data are expressed as a percentage of release stimulated by AMPH alone (percentage of control-stimulated release). *Significantly different from control by ANOVA and posthoc Dunnett's at p < .05. Statistical analysis was performed on untransformed data (S2/S1) as described in Materials and Method; n = 5 for control and (+)-pentazocine treatments, n = 3 for other treatments. There were no significant differences detected among (+)-pentazocine alone and (+)-pentazocine in the presence of either VDCC blocker.

We also tested inhibitors of Ca²⁺/CaM kinase II for potential effects on (+)-pentazocine-mediated enhancement of AMPH-stimulated[³H]DA release. In experiments to examine the effects of KN-62,(+)-pentazocine (1 µM) alone produced a significant enhancementof [³H]DA release stimulated by 25 µM AMPH, compared with release stimulatedby AMPH alone (p < .05; two-way ANOVA and posthoc Dunnett's test)(Fig. 5). Enhancement of AMPH-stimulated release by 1 µM (+)-pentazocinewas significantly attenuated in the presence of 10 µM KN-62. Thissame concentration of KN-62 alone had no effect on control AMPH-stimulatedrelease. The vehicle in which KN-62 was dissolved, DMSO, had noeffect on either unstimulated or AMPH-stimulated release.

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Fig. 5. Effects of KN-62 on (+)-pentazocine-mediated enhancement of AMPH-stimulated [³H]DA release from PC12 cells. Release was stimulated by 25 µM AMPH in the presence or absence of (+)-pentazocine (1 µM) and KN-62 (10 µM) or DMSO (the vehicle for KN-62) as indicated. Data are expressed as percentage of release stimulated by AMPH alone (percentage of control-stimulated release). *Enhancement of stimulated release by (+)-pentazocine (1 µM) alone was significantly different from control by ANOVA and posthoc Dunnett's (two-tailed; p < .05). #Enhancement by (+)-pentazocine alone was significantly different from release in the presence of (+)-pentazocine plus KN-62 by ANOVA and posthoc Dunnett's (two-tailed; p < .05) Statistical analysis was performed on untransformed data (S2/S1) as described in Materials and Methods; n = 3.

We also evaluated the effects of another selective inhibitor of Ca²⁺/CaM kinase II, KN-93, a compound that is structurally dissimilarfrom KN-62 (Sumi et al., 1991), as well as KN-92, a structuralanalog of KN-93 that does not inhibit Ca²⁺/CaM kinase II and has been used as a negative control for KN-93(Pierce and Kalivas, 1997). We chose a concentration of 10 µMfor both KN-93 and KN-92, based on a reported inhibition constant(K_i) obtained from binding studies (K_i = 0.37 µM; Sumi et al.,1991). At 10 µM, neither compound tested alone had any effecton control-stimulated release (Fig. 6). The enhancement of AMPH-stimulatedrelease mediated by 1 µM (+)-pentazocine was significantly attenuatedby the presence of a 10 µM concentration of KN-93. In contrast,10 µM KN-92 had no effect on the enhancement of AMPH-stimulatedrelease mediated by (+)-pentazocine.

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Fig. 6. Effects of KN-92 and KN-93 on (+)-pentazocine-mediated enhancement of AMPH-stimulated [³H]DA release from PC12 cells. Release was stimulated by 25 µM AMPH in the presence or absence of (+)-pentazocine (1 µM) and KN-92 (10 µM) or KN-93 (10 µM) as indicated. Data are expressed as percentage of release stimulated by AMPH alone (percentage of control-stimulated release). *Enhancement of stimulated release by (+)-pentazocine (1 µM) alone was significantly different from control by ANOVA and posthoc Dunnett's (two-tailed; p < .05). #Enhancement by (+)-pentazocine alone was significantly different from release in the presence of (+)-pentazocine plus KN-93 by ANOVA and posthoc Dunnett's (two-tailed; p < .05) Statistical analysis was performed on untransformed data (S2/S1) as described in Materials and Methods; n = 3.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Previous studies support the role of the DAT in regulation of catecholamine function in brain (Giros and Caron, 1993). TheDAT is a target for drugs of abuse; therefore, regulation of theDAT could be therapeutically beneficial. Because we had foundthat in rat striatal tissue, (+)-pentazocine, acting via the pharmacologicallyidentified $sigma$ ₂ receptor, enhanced outward transport of DA via theDAT (Izenwasser et al., 1998), we modeled the apparent regulationin PC12 cells, where study of underlying mechanisms might befacilitated.

Undifferentiated PC12 cells synthesize and release DA and NE (Koike and Takashima, 1986) and bear both the DAT and the NET(Shafer and Atchison, 1991; Kadota et al., 1996). Hellewell andBowen (1990) identified receptors with a $sigma$ ₂-like pharmacologyin PC12 cells. We now report that the agonist (+)-pentazocine,acting at $sigma$ ₂ receptors, can modulate AMPH-stimulated release of[³H]DA from PC12 cells; we believe this system to be a novel modelfor $sigma$ ₂ receptorfunction.

We used AMPH, a substrate for the DAT, to stimulate the release of [³H]DA. The stimulant effects of AMPH are caused by the releaseof biogenic amines from central nervous system nerve terminals(Philips et al., 1982; Sulzer et al., 1995). A two-component modelof AMPH-stimulated release postulates that AMPH stimulates DArelease from synaptic vesicles to the cytosol, which results inreverse transport and release of DA via the plasma membrane DAT(Schuldiner et al., 1993; Pifl et al., 1995; Sulzer et al., 1995;Floor and Meng, 1996).

We demonstrated previously that (+)-pentazocine at concentrations >100 nM enhances AMPH-stimulated [³H]DA release from slices of rat caudate putamen (Izenwasser etal., 1998). Additionally, we demonstrated that concentrationsof (+)-pentazocine between 10 nM and 10 µM produced no effecton [³H]DA uptake. Also, (+)-pentazocine (10 nM to 10 µM) had no effecton basal DA release. If (+)-pentazocine were inhibiting reuptake,it should also enhance apparent basal DA release. In the presentstudy, concentrations of (+)-pentazocine $>=$ 500 nM significantlyenhanced AMPH-stimulated [³H]DA release from PC12cells.

The enhancing effects of (+)-pentazocine on AMPH-stimulated [³H]DA release appear to be specific to the DAT. Nisoxetine wasalways present during the incubation period with [³H]DA to prevent uptake via the NET. Also, in experiments to assesspotential contribution of conversion of [³H]DA to [³H]NE, there was little uptake of [³H]NE, and no measurable effect of (+)-pentazocine on AMPH-stimulated[³H]NE release under the conditions used in thisstudy.

At concentrations of (+)-pentazocine that enhanced AMPH-stimulated [³H]DA release, $sigma$ ₂ receptors would be activated, because the K_iof (+)-pentazocine at $sigma$ ₂ has been reported as 1.5 µM in rat braintissue (Vilner and Bowen, 1992), 1.3 µM in rat liver (Hellewellet al., 1994), and 1 µM in PC12 cells (Hellewell and Bowen, 1990).A higher concentration of (+)-pentazocine was required to enhanceAMPH-stimulated release in PC12 cells than we found using ratstriatum, although the reasons for this difference are unclear.It is possible that the receptors classified as $sigma$ ₂ in the varioustissues are not absolutely identical, despite their very similarpharmacological sensitivities. In neither brain nor PC12 cellsdid concentrations of (+)-pentazocine that would preferentiallyactivate $sigma$ ₁ receptors produce any effect on AMPH-stimulated orbasal [³H]DA release. The $sigma$ ₁ receptor has a K_i for (+)-pentazocine ofbetween 2 and 6 nM (Walker et al., 1990); therefore, it is unlikelythat $sigma$ ₁ receptors contributed to the (+)-pentazocine-mediatedenhancement. The ability of a 100 nM concentration of the $sigma$ ₂-selectiveantagonist BIMU-8 (Weatherspoon et al., 1997) at a concentrationthat should occupy 80% of $sigma$ ₂ receptors (K_i at $sigma$ ₂ = 20 nM), butno $sigma$ ₁ receptors (K_i = 6.9 µM; Bonhaus et al., 1993), to reversethe (+)-pentazocine-mediated enhancement supports the identificationof the receptor involved as $sigma$ ₂. Likewise, the nonsubtype-selective $sigma$ receptor antagonists DTG at 100 nM (K_i at $sigma$ ₂ = 38 nM; Walkeret al., 1990) and BD1008 at 10 nM (K_i at $sigma$ undifferentiated forsubtype = 1.2 nM) both fully reversed the (+)-pentazocine-mediatedenhancement. The reversal of the effect of (+)-pentazocine byDTG in the present study is in contrast to our finding of a slightbut nonsignificant reversal by DTG of the (+)-pentazocine effectin our previous study (Izenwasser et al., 1998). Perhaps in ourearlier study, increasing the concentration of DTG would haveproduced significant reversal. The reasons for the discrepancyare unclear but may be related to slight differences in the sensitivityof $sigma$ ₂ receptors in PC12 cells. It also bears noting that althoughDTG behaves as a $sigma$ antagonist in our own assays of neurotransmitterrelease, others have identified $sigma$ -agonist activity of DTG. Incontrast to the actions of $sigma$ ₂ antagonists in the present study,the $sigma$ ₁-selective antagonist DuP734 (K_i at $sigma$ ₁ = 10 nM, K_i at $sigma$ ₂>1 µM; Culp et al., 1992) did not significantly reduce the (+)-pentazocine-mediatedenhancement of stimulated release. It should be noted that whereasCa²⁺ has long been known to be required for vesicular transmitterrelease, the potential role of Ca²⁺ in transporter-mediated transmitter release remains to be determined(Bowyer et al., 1984). Several studies indicate that transporter-dependentstimulation of DA release in response to AMPH may occur in theabsence of exogenous Ca²⁺, although release of Ca²⁺ from internal stores may be critical (Sulzer et al., 1995; Wallet al., 1995).

Ca²⁺ may be important for receptor-mediated regulation of DA uptake and release via the DAT. Ca²⁺ plays a role in the effects of nicotine, mediated via nicotinicacetylcholine receptors, on DA uptake in PC12 cells that possessthe DAT (Yamashita et al., 1995), suggesting that ligands actingvia other receptor types might also affect transporter-mediateduptake and release in a Ca²⁺-dependent manner. Furthermore, the DAT is known to possess anumber of phosphorylation sites that may be phosphorylated byCa²⁺-dependent intracellular second messenger molecules such as proteinkinase C, thus affecting DAT function (Giros and Caron, 1993).

The reduction in enhancement of (+)-pentazocine-mediated enhancement of AMPH-stimulated [³H]DA by 1 mM EGTA release in both striatal tissue (Izenwasseret al., 1998) and PC12 cells suggested that Ca²⁺ was required for that effect. These results do not indicate whetherthe source(s) of Ca²⁺ important for the enhancement is extracellular and/or intracellular,because chelating extracellular Ca²⁺ might result in secondary changes in intracellular Ca²⁺ levels. Attempts to elucidate the role of intracellular Ca²⁺ using BAPTA-AM were unsuccessful; therefore, we tested whethercompounds that interfere with L- and N-type VDCC would affect $sigma$ ₂ receptor-mediated regulation of AMPH-stimulated DA release.Neither nitrendipine nor $omega$ -CgTX had a significant effect, although $omega$ -CgTX itself slightly, but not significantly, enhanced releaseabove basal. Therefore, entry of Ca²⁺ through L- or N-type VDCC did not appear to be the source ofCa²⁺ for the (+)-pentazocine-mediatedeffect.

Previous studies have demonstrated that depletion of intracellular stores of Ca²⁺, in response to receptor-mediated activation of the IP₃ secondmessenger pathway and subsequent IP₃-mediated release of [Ca²⁺]_i, activates Ca²⁺ entry across the plasma membrane. This has been referred to ascapacitative Ca²⁺ entry (Clapham, 1995; Ko et al., 1996). Capacitative Ca²⁺ entry increases cytoplasmic Ca²⁺ in response to depletion of intracellular Ca²⁺ stores and has potentially important roles in many Ca²⁺-dependent cellular functions (Ghosh and Greenberg, 1995). Insupport of this hypothesis that EGTA may affect capacitative Ca²⁺ entry in our study, thapsigargin, a Ca²⁺-ATPase inhibitor, has been shown to mediate an EGTA-sensitiveincrease in [Ca²⁺]_i via capacitative Ca²⁺ entry in other cell models (Ko et al., 1996; Louzao et al., 1996).Chelation of extracellular Ca²⁺ with EGTA has also been associated with Ca²⁺ extrusion from rat parotid acinar cells, resulting in decreased[Ca²⁺]_i (Takemura et al., 1990). Ligands acting at $sigma$ ₂ receptors canrelease Ca²⁺ from intracellular stores in indo-1-loaded human SK-N-SH neuroblastomacells (Vilner and Bowen, 1995; Bowen et al., 1996). If (+)-pentazocinemediates Ca²⁺ release from intracellular stores, this might activate capacitativeCa²⁺ entry across the plasma membrane. In that case, the enhancementof AMPH-stimulated DA release by (+)-pentazocine would requireboth the release of [Ca²⁺]_i and subsequent capacitative Ca²⁺ entry. EGTA, via chelation of extracellular Ca²⁺, would remove the Ca²⁺ necessary for capacitative Ca²⁺ entry across the plasma membrane of the PC12 cells, making thenet effect of EGTA a decrease in the cytoplasmic Ca²⁺ available for (+)-pentazocine to mediate enhancement of AMPH-stimulatedDArelease.

EGTA has also been shown to modify physiological effects produced by AMPH. Administration of EGTA to mice has been shown toinhibit AMPH-induced circling behavior, which indicates a rolefor Ca²⁺ in the response (Fung and Schwarz, 1983). These studies did notassess the relative contributions of extracellular and/or intracellularCa²⁺ in the effects mediated byAMPH.

In conclusion, we report a model of $sigma$ ₂ receptor function using PC12 cells. This represents the first such model that enablesidentification of signal transduction mechanisms involved in $sigma$ ₂receptor regulation of catecholamine release. Our results suggestthat (+)-pentazocine, acting via a $sigma$ ₂ receptor, enhances AMPH-stimulatedDA release either by directly altering the function of the DATor by mobilizing a vesicular pool of DA by altering the outwardflux of DA through the vesicular amine transporter. We are currentlyinvestigating these possibilities. Our results suggest an importantrole for Ca²⁺/CaM kinase II in $sigma$ ₂ receptor regulation of AMPH-stimulated DArelease. $sigma$ ₂ receptors may be important in the effects of AMPHthat are associated with drug abuse and other conditions thatinvolve enhanced levels of synaptic DA. For instance, recent evidencefrom positron emission tomography scans suggests that schizophreniais associated with enhanced AMPH-induced DA release in both drugnaive and antipsychotic-treated patients (Breier et al., 1997).

	Acknowledgments

We thank Dr. Robert Zaczek for the gift of DuP734, Dr. Wayne Bowen for the gift of BD1008, and Dr. Douglas Bonhaus for thegift of BIMU-8. We also thank Alicia E. Derbez and Rupal M. Modyfor performing some of theexperiments.

	Footnotes

Accepted for publication November 24, 1998.

Received for publication July 16, 1998.

¹ This work was supported by a grant from the National Institute on Drug Abuse and a Faculty Research Enhancement Fund Awardto L.L.W. J.K.W. was a predoctoral student in the Department ofPharmacology, The George Washington Institute for Biomedical Sciences.This work was from a dissertation presented to the above departmentin partial fulfillment of the requirements for the Ph.D. degree.The findings herein were reported in preliminary form in Weatherspoonand Werling (1997) The Pharmacologist 39:89 and Weatherspoon,Mody, Derbez and Werling (1998) Soc Neurosci Abstr 24:1595.

Send reprint requests to: Linda L. Werling, Ph.D., Department of Pharmacology, The George Washington University Medical Center, 2300 Eye Street NW, Washington, DC 20037. E-mail phmllw{at}gwumc.edu

	Abbreviations

AMPH, amphetamine; BAPTA-AM, 1,2-bis(2-aminophenoxy)ethane-N,N,N,N-tetraacetic acid acetoxymethyl ester; Ca²⁺/CaM kinase II, Ca²⁺/calmodulin-dependent protein kinase II; DA, dopamine; DAT, dopamine transporter; DTG, 1,3-di(2-tolyl)guanidine; EGTA, ethylene glycol bis( $beta$ -aminoethyl ether)-N,N,N',N'-tetraacetic acid; GBR-12909, 1-[2-[bis(4-fluorophenyl)methoxy]ethyl]-4-[3-phenylpropyl]piperazine dihydrochloride; KN-62, 1-[N,O-bis-(5-isoquinolinesulfonyl)-N-methyl-L-tyrosyl]-4-phenylpiperazine; KN-92, 2-[N-(4'-methoxybenzenesulfonyl)]amino-N-(4'-chlorophenyl)-2-propenyl-N-methylbenzylamine phosphate; KN-93, N-[2-[[[3-(4'-chlorophenyl)-2-propenyl]methylamino]methyl]phenyl]-N-(2-hydroxyethyl)-4'-methoxy-benzene-sulfonamide phosphate; BD1008, N-[2-(3,4-dichlorophenyl)-ethyl]N-methyl-2-pyrrolidinyl)ethylamine; BIMU-8, endo-N-(8-methyl-8-azabicyclo[3.2.1.]oct-3-yl)-2,3-dihydro-(1-methyl)ethyl-2-oxo-1H-benzimidazole-1-carboxamide hydrochloride; DuP734, 1-(cyclopropylmethyl)-4-2'-4"-fluorophenyl)-2'-oxoethyl)-piperidine hydrogen bromide; NE, norepinephrine; NET, norepinephrine transporter; PC12, pheochromocytoma-12 cells; VDCC, voltage-dependent calcium channel; $omega$ -CgTX, $omega$ -conotoxin from Conus geographus(GVIA); DMEM, Dulbecco's Modified Eagle Medium.

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Modulation of Amphetamine-Stimulated [3H]Dopamine Release from Rat Pheochromocytoma (PC12) Cells by Type 2 Receptors1

Modulation of Amphetamine-Stimulated [³H]Dopamine Release from Rat Pheochromocytoma (PC12) Cells by $sigma$ Type 2 Receptors¹