Suppression of Ethanol-Reinforced Behavior by Naltrexone Is Associated with Attenuation of the Ethanol-Induced Increase in Dialysate Dopamine Levels in the Nucleus Accumbens

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The Journal of Neuroscience, December 15, 1998, 18(24):10663-10671

Suppression of Ethanol-Reinforced Behavior by Naltrexone Is Associated with Attenuation of the Ethanol-Induced Increase in Dialysate Dopamine Levels in the Nucleus Accumbens
Rueben A. Gonzales¹ and Friedbert Weiss²
¹ Institute for Neuroscience, University of Texas at Austin, Austin, Texas 78712, and ² Department of Neuropharmacology, The Scripps Research Institute, La Jolla, California 92037

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The opiate antagonist naltrexone suppresses ethanol-reinforced behavior in animals and decreases ethanol intake in humans.However, the mechanisms underlying these actions are not wellunderstood. Experiments were designed to test the hypothesis thatnaltrexone attenuates the rewarding properties of ethanol by interferingwith ethanol-induced stimulation of dopamine activity in the nucleusaccumbens (NAcc). Simultaneous measures of the effects of naltrexoneon dialysate dopamine levels in the NAcc and on operant respondingfor oral ethanol were used. Male Wistar rats were trained to self-administerethanol (10-15%, w/v) in 0.2% (w/v) saccharin during daily 30min sessions and were surgically prepared for intracranial microdialysis.Experiments began after reliable self-administration was established.Rats were injected with naltrexone (0.25 mg/kg, s.c.) or salineand 10 min later were placed inside the operant chamber for a20 min waiting period with no ethanol available, followed by 30min of access to ethanol. A transient rise in dialysate dopaminelevels was observed during the waiting period, and this effectwas not altered by naltrexone. Ethanol self-administration reliablyincreased dopamine levels in controls. Naltrexone significantlysuppressed ethanol self-administration and prevented ethanol-inducedincreases in dialysate dopamine levels. Subsequent dose-effectanalyses established that the latter effect was not merely a functionof reduced ethanol intake but that naltrexone attenuated the efficacyof ethanol to elevate dialysate dopamine levels. These resultssuggest that suppression of ethanol self-administration by opiateantagonists is the result of interference with dopamine-dependentaspects of ethanol reinforcement, although possible additionaleffects via nondopaminergic mechanisms cannot be eliminated asa factor in opiate antagonist-induced reduction of ethanolintake.

Key words: ethanol; naltrexone; reinforcement; dopamine; microdialysis; nucleus accumbens

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Opiate antagonists inhibit the self-administration of ethanol in a variety of animal models, suggesting that opioid pathwaysin the brain participate in the mediation of ethanol-seeking behavior.For example, the nonselective opiate receptor antagonists naloxone,naltrexone, and nalmefene reduce ethanol intake in rats and monkeys(Altshuler et al., 1980; Samson and Doyle, 1985; Froehlich etal., 1990; Weiss et al., 1990; Hubbell et al., 1991; Kornet etal., 1991; Gauvin et al., 1993; Hyytiä and Sinclair, 1993; Davidsonand Amit, 1996). µ and $delta$ receptor-selective antagonists have alsobeen reported to suppress ethanol self-administration in rats(Hyytiä, 1993; Krishnan-Sarin et al., 1995; Honkanen et al.,1996). Finally, a growing number of clinical studies suggest thatnaltrexone is an effective pharmacological adjunct for reducingrelapse in human alcoholics (O'Malley et al., 1992; Volpicelliet al., 1992; O'Brien et al., 1996).

The neurochemical mechanisms underlying the attenuation of volitional ethanol intake by opiate receptor antagonists are notwell understood but may involve an interaction with dopaminergicneurotransmission. The mesolimbic dopamine pathway that projectsfrom the ventral tegmental area (VTA) to the nucleus accumbens(NAcc) has been implicated as a key site for the reinforcing actionsof many drugs of abuse including ethanol (Wise and Rompre, 1989;Koob, 1992; Di Chiara, 1995). Systemic administration of ethanolincreases the firing rate of mesolimbic dopamine neurons (Gessaet al., 1985; Diana et al., 1992) and increases extracellulardopamine concentrations in the NAcc as measured by microdialysis(Imperato and Di Chiara, 1986; Yoshimoto et al., 1991; Blanchardet al., 1993; Blomqvist et al., 1993; Rossetti et al., 1993; Kiianmaaet al., 1995; Mocsary and Bradberry, 1996; Yim et al., 1998).More direct evidence of a role of dopamine in ethanol reward comesfrom findings that oral ethanol self-administration elevates extracellulardopamine in the NAcc (Weiss et al., 1993, 1996), that rats self-administerethanol directly into the VTA cell body region of mesolimbic dopamineneurons (Gatto et al., 1994), and that pharmacological manipulationof dopamine neurotransmission modifies ethanol-reinforced operantresponding and ethanol preference (e.g., Weiss et al., 1990; Samsonet al., 1993; George et al., 1995; Panocka et al., 1995). Boththe NAcc and VTA are rich in opioid peptides and receptors (Wamsleyet al., 1980; Lewis et al., 1983; Dilts and Kalivas, 1989, 1990).Afferent projections to these areas as well as local interneurons(Khachaturian et al., 1993; de Waele et al., 1995) provide a potentialanatomical substrate by which endogenous opioids may modulatethe dopaminergic and, ultimately, the rewarding effects of ethanol.In fact, opiate antagonists can blunt ethanol-induced increasesin extracellular dopamine in the NAcc. For example, the nonselectiveopiate antagonist naltrexone has been reported to inhibit therise in extracellular dopamine concentrations elicited by reversemicrodialysis of 5% (v/v) ethanol (Benjamin et al., 1993). Althoughthe pharmacological relevance of local perfusion with such highethanol concentrations [~800 mM in Benjamin et al. (1993)] hasbeen questioned (Gonzales et al., 1998), this finding suggestsa possible role for opioid receptors in ethanol-induced dopaminergicactivation. This possibility is supported further by the findingthat reverse transcerebral microdialysis of the selective $delta$ -opioidantagonist naltrindole completely blocked the increases in extracellulardopamine levels in the NAcc induced by systemic ethanol administration(Acquas et al., 1993).

On the basis of these findings, one may hypothesize that interference with ethanol-induced stimulation of dopamine releaseis one of the mechanisms by which opiate antagonists suppressethanol self-administration. This possibility remains to be confirmed,however, by the demonstration that reductions in ethanol-reinforcedbehavior produced by opiate antagonists are predictably coupledto decreases in the efficacy of ethanol to increase extracellulardopamine concentrations in the NAcc. The purpose of the presentstudy was to test this hypothesis by measuring simultaneouslythe effects of the nonselective opiate receptor antagonist naltrexoneon operant responding for oral ethanol and on dialysate dopaminelevels in the NAcc of rats and by examining the consequences ofnaltrexone treatment on the dose-effect function for ethanol-stimulateddialysate dopaminelevels.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Subjects. Male Wistar rats (Charles River Laboratories, Wilmington, MA) weighing between 450 and 550 gm at the time of testingwere used. The rats were housed in groups of two or three in ahumidity- and temperature (22°C)-controlled environment. The light/darkcycle was 12:12 hr (lights on at 6 A.M. and off at 6 P.M.), andanimals had food and water available ad libitum. All procedureswere conducted in strict adherence with the National Institutesof Health Guide for the Care and Use of Laboratory Animals.

Behavioral testing apparatus. Ethanol self-administration training and microdialysis were conducted in standard operant chambers(Coulbourn Instruments, Allentown, PA) modified to accommodatethe microdialysis perfusion system as described previously (Weisset al., 1993). The operant chambers contained a retractable leverthat, when activated, delivered 0.1 ml of a solution into a receptacle(volume capacity, 0.15 ml) located 4 cm above the grid floor inthe center of the front plate of the chamber. The chambers wereenclosed within sound-attenuating, ventilated environmental cubicles(Coulbourn Instruments). Fluid delivery and the recording of behavioraldata were controlled by amicrocomputer.

Ethanol self-administration training. Rats were trained to orally self-administer an ethanol-saccharin solution in daily 30min sessions using previously described procedures (Weiss et al.,1993). Briefly, rats were initially placed on a 22 hr water restrictionschedule for the first 4 d of training, during which time theywere trained to respond to 0.2% (w/v) saccharin on a scheduleof continuous reinforcement. After operant responding was acquiredsuccessfully, water was made available again ad libitum in thehome cage for the remainder of the experiment. On the fourth dayof training, ethanol (5%, w/v) was added to the 0.2% saccharinsolution. Over a period of 3-4 weeks, the ethanol concentrationwas gradually increased to 10-15% while the saccharin concentrationwas unaltered. During this time, a "waiting period" that precededaccess to the drinking solution was gradually introduced by placingrats in the operant chamber for increasing amounts of time (1extra minute per day) before extension of the lever and onsetof the session. The final length of the waiting period was 20min. This procedure was adopted as a precaution because of previousobservations that exposure to an environment associated with ethanolavailability can produce a transient (15-20 min) rise in dialysatedopamine levels in the NAcc (Weiss et al., 1993). Thus, the waitingperiod served the purpose of minimizing the effects of possibleincreases in dialysate dopamine levels induced by environmentalstimuli that might otherwise confound the subsequent measurementof the effects of ethanol on accumbal dopamine efflux. Rats remainedin the operant chambers for 10 min after the lever was retractedat the end of each 30 min self-administration session. Duringthe self-administration training phase after surgery (see below),the animals were habituated to the microdialysis perfusion andtethering system. This consisted of a stainless steel cannulaconnector that was attached to a liquid swivel suspended froma balanced lever arm that was positioned over the center of thechamber. During this time, the rats were also habituated to thedrug injection procedure by receiving subcutaneous injectionsof saline on several occasions before being placed in the operantchambers. The final self-administration session involving microdialysisand opiate antagonist drug tests was conducted 7 d after the lasttrainingsession.

Implantation of guide cannulae. After reliable self-administration of ethanol was established, unilateral stainless steelguide cannulae (Plastics One, Roanoke, VA) were stereotaxicallyimplanted into the rats under halothane anesthesia aimed at theNAcc as described previously (Weiss et al., 1996). Coordinateswere (in mm) 1.7 anterior, ±1.4 medial, and $-$ 6.1 ventral, relativeto bregma (Paxinos and Watson, 1986). The rats were allowed torecover for 7 d before resumption of ethanol self-administrationtraining.

Microdialysis procedures. Microdialysis probes were constructed using the methods of Pettit and Justice (1991). Fused silicatubing (inner diameter, 40 µm) was used as inlet and outlet toa hollow fiber dialysis membrane (outer diameter, 270 µm; molecularweight cutoff, 13,000; Spectrum, Houston, TX) that was sealedat both ends with epoxy. The active dialysis area was 2 mm, whichwas the distance between the ends of the inlet tubing and theoutlet tubing. The probe inlet was connected to a liquid swivel(centered above the cage suspended from the balanced arm) thatwas connected to a syringe containing artificial CSF (aCSF; NaCl145 mM, KCl 2.8 mM, MgCl₂ 1.2 mM, CaCl₂ 1.2 mM, ascorbate 0.25mM, and glucose 5.4 mM, pH 7.2-7.4) that was pumped through thesystem using a pulseless syringe pump (Bioanalytical Systems,West Lafayette, IN). The probe outlet was placed into a 0.25 mlplastic vial for collection of dialysate that was changed manually.Samples were frozen immediately on dry ice and stored at $-$ 70°Cuntilanalyzed.

On the evening before the experiments, the microdialysis probes perfused with aCSF at a rate of 0.2 µl/min were slowly loweredinto place through the guide cannulae while the rats were brieflyanesthetized with halothane. After recovery from the anesthesia,the rats remained in the home cage overnight with food and wateravailable. During this time the perfusion flow rate remained at0.2 µl/min. The next morning the flow rate was increased to 0.5µl/min, and dialysate samples were collected at 10 min intervalsbeginning 2 hr after changing the flowrate.

Experimental design and procedures. Dialysate dopamine concentrations were monitored under the following conditions. On themicrodialysis day, baseline samples were taken for 1 hr. Thiswas followed by a subcutaneous injection of either the nonselectiveopiate receptor antagonist naltrexone (0.25 mg/kg) or its vehicle(saline), after which the rats were returned to their home cages.Ten minutes after the naltrexone or vehicle treatment, the animalswere placed into the operant chambers. The test session consistedof a 20 min waiting period without access to the lever and drinkingsolution, a 30 min ethanol self-administration period, and a 10min period after the session such that the rats remained in thechamber for a total of 60 min/session. Immediately after removalfrom the operant chambers, tail blood samples were taken for determinationof blood alcohol levels in those animals that exhibited significantethanolintake.

HPLC analysis of dopamine. Dialysate dopamine concentrations were determined by microbore reverse-phase HPLC. Dialysate wasinjected (3-4.5 µl) onto a Sepstik column (100 × 1 mm; 3 µm ODS;Bioanalytical Systems) using a Valco injector. Mobile phase (19mM citric acid, 40 mM sodium phosphate, 0.2 mM EDTA, and 0.21mM 1-decanesulfonic acid containing 19% (v/v) methanol, pH 5.25)was pumped through the column using an ISCO (Lincoln, NE) syringepump at 25 µl/min. Dopamine was detected using a glassy carbonworking electrode controlled by a Model 400 Princeton AppliedResearch (Princeton, NJ) electrochemical detector. The appliedpotential was 0.7 V (vs Ag/AgCl). Chromatograms were recordedusing a Kipp and Zonen strip-chartrecorder.

Blood alcohol determination. In a subset of animals, a tail blood sample was collected after the self-administration session.The blood sample (200 µl) was collected into a 1.5 ml microfugetube that contained 4 µl of heparin USP (1000 units/ml), and 10µl of whole blood was immediately transferred into a headspacegas chromatography vial and sealed with a rubber septum. Sampleswere stored at 4°C until analyzed. A Perkin-Elmer (Emeryville,CA) Sigma 2000 gas chromatograph (stainless steel column, 80/100Porapak Q5 and 6 feet × 1/8 inch, Supelco) with an HS-100 headspaceanalyzer was used for ethanol analysis. Nitrogen was used as acarrier gas (flow rate, 30 ml/min). The injector temperature wasset to 90°C, and the oven temperature was 190°C. The retentiontime of ethanol was ~1.8min.

Histology. The placement of the microdialysis probes was verified by histological analysis of brains after completion of theexperiments. Rats were killed by administration of an overdoseof halothane, and their brains were removed and placed in formalin.Fifty micrometer frozen sections were prepared and stained withcresyl violet. In 25 out of the 28 rats, at least 70% of the activedialysis area was located within the NAcc. Two rats were includedwhose probes extended into the ventral striatal/pallidal area.In one animal the probe location could not be verified becauseof loss of the sample duringslicing.

Statistical analysis. The dopamine concentration data were transformed to percent of basal values and analyzed by a 2 × 12mixed-factorial ANOVA for differences in dialysate dopamine levelsbetween the saline- and naltrexone-treated animals. Basal dopaminelevels were defined as the average of six baseline samples ineach animal. There were 7 missing data points out of the 384 collectedbecause of technical problems with sample collection or HPLC.These points were estimated by interpolation, and the degreesof freedom for the ANOVA were corrected for these estimates. Ethanolintake data were analyzed by a 2 × 2 × 6 mixed-factorial ANOVAwith two within-subject variables (intake in 5 min bins and day).Differences between individual means (after confirmation of significantinteractions in the overall ANOVA) were determined by one-wayANOVAs or planned contrasts using Bonferroni corrections to controlfor experimentwise error. Relationships between ethanol intakeand the maximal percent increase in dialysate dopamine concentrationduring ethanol self-administration as well as differences betweenthe slopes of the dose-effect functions of the naltrexone versusvehicle groups were analyzed by linear regression (Kenakin, 1997).Significance was accepted when p < 0.05.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Blood ethanol levels after ethanol self-administration

In eight of the control and four of the naltrexone-treated animals, a sample of tail blood was taken after collection of thelast dialysate fraction. The time elapsed between cessation ofresponding for ethanol and blood sampling ranged from 30 to 55min. Figure 1 shows that there was a significant relationshipbetween ethanol intake and blood alcohol level. These resultsare similar to those obtained previously in male Wistar rats usingthe alcohol dehydrogenase method for determination of blood alcohollevels (Weiss et al., 1993).

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Figure 1. Relationship between ethanol intake and blood alcohol levels. Tail blood samples were taken in a subset of rats 30-55 min after termination of ethanol self-administration. Blood alcohol concentrations were determined by gas chromatography and analyzed by linear regression (r = 0.88; p < 0.05).

Naltrexone and ethanol self-administration

During the last self-administration session (baseline) before the drug and microdialysis test day, the mean responding forethanol in the subgroups of animals assigned to the saline (control)and naltrexone groups was virtually identical (Fig. 2). Mean ethanolintake in the saline control group remained essentially unalteredon the test day, suggesting that the microdialysis procedure perse did not interfere with ethanol self-administration. In contrast,ethanol consumption was substantially reduced in naltrexone-treatedrats compared with both their own baseline levels of intake andethanol intake in vehicle-treated rats on the test day. The differencesin ethanol intake were confirmed by a significant interactionbetween groups and self-administration session [F_(1,27) = 11.2;p < 0.05] and by a significant difference between baseline versustest day for the naltrexone group [F_(1,27) = 20.9; p < 0.05; posthoc ANOVA, Bonferroni-corrected]. Additional post hoc analysesconfirmed that ethanol intake of the naltrexone group was significantlylower than that of the saline group on the test day [F_(1,54) =6.9; p < 0.05].

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Figure 2. Effects of naltrexone (0.25 mg/kg, s.c.) on ethanol self-administration. Mean (± SEM) ethanol intake during 30 min self-administration sessions is shown for baseline and test (dialysis) days. Shaded and open bars show data from rats assigned to the saline (n = 13; SAL) and naltrexone (n = 16; NALT) groups, respectively. All animals received either saline vehicle or naltrexone injections on the test day, whereas only vehicle was available on the baseline day for both groups. There was no significant main effect of treatment group [F_(1,27) = 0.89; p > 0.05], but there was a significant main effect of session [baseline vs microdialysis day; F_(1,27) = 7.7; p < 0.05]. Post hoc analyses shown on the figure were performed based on a significant interaction between the main effects as explained in the text; * denotes a significant (p < 0.05) difference from the respective control condition as explained in the text.

Examination of the distribution of responding over the 30 min self-administration sessions revealed that in the saline groupmost of the ethanol intake occurred within the first 5 min onboth the baseline and test day (Fig. 3). The time course and thetotal amount of ethanol intake in the naltrexone group duringthe baseline day was similar to that of the control group. Thiswas reflected in a nonsignificant interaction between group andtime course of intake for the baseline day [F_(1,54) = 1.1; p >0.05]. In contrast, on the test day, the naltrexone group showeda significant decrease in ethanol intake during the initial 5min [F_(1,140) = 55; p < 0.05; one-way ANOVA after significantoverall interaction, F_(1,54) = 19; p < 0.05] without large changesin the pattern of intake during the remainder of the session.The analysis of interactions described above was justified onthe basis of a significant three-way interaction for group, session,and the time course of intake within the session [F_(5,135) = 10.1;p < 0.05].

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Figure 3. Distribution of mean (± SEM) ethanol intake over the 30 min self-administration phase during the baseline and test (dialysis) days. The figure represents the same data presented in Figure 2 but shown in 5 min bins.

Effects of ethanol and naltrexone on dialysate dopamine levels

Analysis of the time course of dialysate dopamine concentrations across baseline, injection, waiting, and self-administrationperiods revealed a significant interaction between time and drugtreatment condition [F_(11,290) = 1.9; p < 0.05]. There was nosignificant main effect of drug treatment [F_(1,27) = 1.3; p >0.05], but there was a significant main effect of time [F_(11,290)= 11.8; p < 0.05]. Analyses of simple effects and contrasts betweenmeans were then performed to determine the source of the significantinteraction. Data are shown in Figure 4 as the concentration ofdopamine in the dialysate and in Figure 5 as the percent of baseline.

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Figure 4. Effect of naltrexone on mean (± SEM) dialysate dopamine concentrations from the nucleus accumbens before, during, and after self-administration of ethanol. Basal (BASAL) represents dialysate dopamine levels while rats were resting in their home cage. The arrows indicate the administration of naltrexone (n = 16) or vehicle (saline; n = 13). A, The effects of the injection and the response during the waiting (WAITING) period during which rats were placed in the operant chambers but did not have access to ethanol. B, The same basal shown in A for comparison with the response during the 30 min self-administration session (SELF-ADMIN) and the 10 min period after the session ended (POST). Data for the waiting period were not shown in this panel to facilitate comparison of basal with the response during self-administration; * indicates a significant difference from the respective pooled basal concentration (p < 0.05, determined by planned contrasts, Bonferroni-corrected, after significant interaction between groups and time in the overall ANOVA).

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Figure 5. Effect of naltrexone on mean (± SEM) dialysate dopamine response expressed as the percent of basal during ethanol self-administration in the same rats shown in Figure 4. Data are presented as described in the legend to Figure 4 except that concentration values were transformed to the percent of basal for each rat.

Dopamine concentrations in the two groups of rats were stable during the last 50 min of the 1 hr baseline collection period(Figs. 4, 5), and the mean (± SEM) basal dopamine levels in thesaline and naltrexone groups were not significantly differentfrom each other (1.77 ± 0.32 and 1.34 ± 0.23 nM, respectively).The samples collected 10 min after the administration of salineor naltrexone showed a slight increase in dopamine concentrationcompared with the basal level in both groups, although this increasewas statistically significant only in the naltrexone group [F_(1,182)= 12.7; p < 0.05].

Dialysate dopamine levels transiently increased during the 20 min waiting period (Figs. 4A, 5A) in both groups of rats [saline,F_(1,182) = 20.3; p < 0.05; naltrexone, F_(1,182) = 36.2; p < 0.05].In both groups the maximal mean increases in dopamine levels occurredduring the first 10 min of this 20 min experimental phase. Bythe end of the waiting period, dialysate dopamine concentrationsin the naltrexone group were no longer significantly differentfrom basal values, whereas dopamine levels in the saline controlgroup remained significantlyelevated.

There were clear differences in dialysate dopamine concentrations between the two treatment groups during the ethanol self-administrationphase of the experiment. Figures 4B and 5B illustrate that thesaline group showed a significant increase in dopamine concentrationcompared with basal levels during the 30 min session includingthe last dialysate sample collected 10 min after the session hadended [F_(1,182) > 12.4; p < 0.05 for the four contrasts]. Dopamineconcentrations in the naltrexone group were not significantlydifferent from basal levels during the self-administration period.Therefore, the major source of the overall interaction betweendrug treatment conditions and changes in dopamine concentrationsover the experimental phases resided in the differences betweenthe effect of ethanol self-administration on dialysate dopaminelevels in the naltrexone- versus saline-treatedgroups.

Inspection of the temporal profile of dialysate dopamine concentrations over the experimental phases (Figs. 4, 5) revealeda biphasic change suggestive of an overlap between the late effectsof introduction in the operant chamber (waiting phase) and theearly effects of ethanol on dialysate dopamine levels. Specifically,in both groups dopamine levels were transiently elevated duringthe waiting period. Although this increase in dopamine effluxdecreased toward the end of the waiting period, it did not reachbaseline levels before the onset of the ethanol self-administrationphase. In the saline-treated group, ethanol self-administrationmaintained dopamine levels significantly above baseline with asecond modest increase early during the self-administration phase.In contrast, in the naltrexone group the residual elevation indopamine levels at the end of the waiting phase was not maintainedduring the self-administration phase, and dopamine efflux returnedtobaseline.

Dose-effect relationships between self-administered ethanol and the stimulation of dialysate dopamine levels after naltrexone

The analyses above revealed significantly lower levels of dopamine in dialysates of ethanol self-administering rats pretreatedwith naltrexone compared with that in controls. It was important,however, to ascertain that the lower dopamine levels in this groupwere not merely a function of substantially lower ethanol intakebut that naltrexone, in fact, attenuated the efficacy of ethanolto elevate extracellular dopamine concentrations in the NAcc.To accomplish this, dose-response relationships were establishedbetween total ethanol intake and the maximal increase in dialysatedopamine concentration (expressed as the percent of basal values)observed during the 30 min self-administration session. As illustratedin the dose-effect plots (Fig. 6A), there was a significant positiverelationship between ethanol intake and maximal dopaminergic responsein the vehicle control group but not in the naltrexone group [saline,F_(1,11) = 10.4; p < 0.05; naltrexone, F_(1,14) = 0.7; NS] (i.e.,the slope of the dose-effect function of the naltrexone groupwas not significantly different from zero). The difference betweenthe slopes of the dose-effect functions of the saline and naltrexone-treatedrats was verified by linear regression analysis [F_(1,25) = 6.9;p < 0.05], confirming that naltrexone significantly reduced theefficacy of ethanol to increase dopamine efflux over the rangeof doses self-administered by the naltrexone-treated rats.

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Figure 6. Dose-effect regression lines for increases in dopamine output in response to self-administered ethanol in saline- and naltrexone-treated rats. A, Maximal (percent of basal) increases in dopamine release during the 30 min self-administration session are plotted against total ethanol intake. Data from all rats shown in Figures 2-4 are shown. The saline-treated group showed a significant correlation between ethanol intake and the dopamine response (r = 0.70; p < 0.05), whereas the naltrexone-treated group did not (r = 0.22). B, Only a subset of rats from the control and naltrexone-treated groups, which had a comparable range of ethanol intake, was used for this analysis. The relationship between ethanol intake and the maximal increase in dialysate dopamine levels was significant in the saline-treated controls (r = 0.69; p < 0.05), but there was no significant relationship in naltrexone-treated rats (r = 0.35). C, Comparison of naltrexone effects against a dose-effect function generated from the pooled data of the present control group and a large sample of Wistar rats tested in previous work involving ethanol self-administration under similar conditions (see Results) is shown. The entire set of controls had a correlation coefficient of 0.55 (p < 0.05), and the slope of this regression was significantly different from that of the naltrexone group (p < 0.05).

Because the average ethanol intake in naltrexone-treated rats was substantially lower than that in the saline-treated controls,an additional regression analysis was performed on a restrictedsample from both groups to provide comparable distributions ofethanol intake (0 < intake < 1.2 gm/kg). For this purpose, animalsof the control group with levels of ethanol intake greater thanthe maximum intake observed in the naltrexone group, as well asrats that did not drink ethanol (mostly in the naltrexone group),were excluded. This was done to eliminate a potential bias inthe data introduced by the nonhomogenous distribution of ethanolintake in the two groups. The dose-effect functions for this moreconservative analysis are shown in Figure 6B. The results of thisanalysis were similar to those obtained with the unrestricteddata set in that a significant positive correlation between ethanolintake and dopamine levels [F_(1,7) = 6.5; p < 0.05] was obtainedin saline-treated controls but not in the naltrexone group [F_(1,9)= 1.3; NS]. In addition, the slopes of the two regressions weresignificantly different from each other [F_(1,16) = 6.8; p < 0.05].

To examine the generality of these results, we compared the present ethanol self-administration dose-effect functions witha dose-effect function generated from the data of a pooled largesample of Wistar rats tested in previous work involving ethanolself-administration under near identical conditions with the exceptionthat saccharin had been eliminated from the ethanol drinking solutions(Weiss et al., 1993, 1996; Katner et al., 1996). Thus, this comparisonalso served the purpose of establishing that there are no differencesbetween the effects of saccharin- versus nonsaccharin-containingethanol solutions on dialysate dopamine levels. No significantdifferences in the slope of the dose-effect relationships forthe effect of ethanol on dialysate dopamine concentrations werefound between the present saline control group and the previouslytested sample [F_(1,24) = 3.4; p > 0.05], confirming that the increasesin extracellular dopamine induced by self-administration of saccharin-versus nonsaccharin-containing ethanol solutions are very similar.The data of the saline group were, therefore, pooled with thoseof the previously tested animals for comparison with the naltrexonegroup. The Pearson correlation coefficient for the pooled setof controls was 0.55 [F_(1,26) = 11.1; p < 0.05], and the slopeof this regression line differed significantly from that of thenaltrexone group [F_(1,35) = 8.3; p < 0.05; Fig. 6C]. The resultsof these analyses confirm the reliability of the dose-effect relationshipbetween the amount of self-administered ethanol and the increasesin dialysate dopamine concentrations across experiments and, thereby,corroborate the finding that naltrexone diminishes the dopaminergiceffects ofethanol.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The results support the hypothesis that interference with ethanol-induced stimulation of dopamine release is one of the mechanismsby which opiate antagonists suppress ethanol self-administration.The concurrent measurement of dopamine output in the NAcc andof ethanol-reinforced behavior revealed a direct association betweenthe pharmacological and behavioral effects of naltrexone. Naltrexonesignificantly reduced the ability of ethanol to increase extracellulardopamine concentrations (as reflected by dialysate dopamine levels)in the NAcc that are induced by self-administration of ethanol,and more importantly, the dose-effect analyses suggest that theinhibition of the response by naltrexone (Figs. 4, 5) was notaccounted for simply by reduced ethanol intake. The validity ofthese dose-effect analyses was corroborated by the excellent correspondencewith dose-effect relationships of ethanol-evoked elevations inextracellular dopamine levels in previous work. These findingsstrongly suggest that naltrexone reduced the efficacy of ethanolto increase extracellular dopamine concentrations in the NAccover the range of self-administered doses examined and implicatethis effect of naltrexone in the suppression of ethanol consumption.The results also extend previous evidence that opiate antagonistscan blunt increases in accumbal dialysate dopamine levels aftersystemic or local administration of ethanol (Acquas et al., 1993;Benjamin et al., 1993) by showing that this action of opiate antagonistsis accompanied by a reduction in the reinforcing effects ofethanol.

Before these conclusions can be fully accepted, however, it is necessary to consider two issues. First, dialysate dopamineconcentrations that increased during the waiting period had notcompletely returned to baseline at the beginning of the self-administrationphase in the control group. As will be discussed in greater detailbelow, the dopaminergic activation during the waiting phase mayperhaps be related to the presence of alcohol-associated environmentalstimuli that predict the availability of ethanol (Vavrousek-Jakubaet al., 1991; Weiss et al., 1993; Katner et al., 1996). Thus,it is possible that the increase in dopamine efflux during theself-administration phase may reflect the additive effects ofthe direct dopaminergic actions of ethanol plus some residualnonpharmacological dopaminergic activation related to processesoperative during the waiting phase. Previous work suggests thatthe increase in extracellular dopamine during a pre-ethanol waitingperiod can indeed carry over into the ethanol self-administrationphase, although this effect was significant only in a line ofgenetically selected alcohol-preferring rats (i.e., the IndianaP line) and not in genetically heterogeneous Wistars as used inthe present study (Katner et al., 1996). Nonetheless, some contributionof the increase in extracellular dopamine during the waiting periodto the elevation of dopamine levels during the self-administrationphase cannot be eliminated completely. The question, therefore,is not only whether the effects of naltrexone (i.e., lower dopaminelevels during the self-administration phase) are simply the resultof lower ethanol intake but also whether naltrexone perhaps reducedthe proportion of extracellular dopamine attributable to residualwaiting period effects rather than, or in addition to, interferingwith ethanol-induced increases in extracellular dopamine. Althoughthis issue cannot be fully resolved on the basis of the presentdata, the interpretation that naltrexone directly suppresses ethanol-inducedincreases in extracellular dopamine concentrations is well supportedby the literature (Acquas et al., 1993; Benjamin et al., 1993)and, therefore, a more parsimonious account of the data than theinterpretation of attenuated carry-over effects from the waitingperiod into the self-administrationphase.

A second issue relevant for the interpretation of the results is that, unlike in similar previous studies, saccharin was retainedin the ethanol drinking solution throughout the experiment. Itcould be argued, therefore, that the presence of the sweetenermay have been a factor in the increase in accumbal dopamine outputduring self-administration. However, self-administration of saccharinsolutions, which support rates of operant responding similar tothose maintained by ethanol in the present study, do not significantlyincrease dialysate dopamine concentrations in the NAcc (Weisset al., 1993; Katner et al., 1996). More importantly, the comparisonof the present with previous dose-effect data indicated that theeffects of saccharin- versus nonsaccharin-containing ethanol solutionson dialysate dopamine concentrations do not differ and eliminatesthe possibility that saccharin influenced the results by alteringthe neurochemical actions of ethanol. It is also unlikely thatthe naltrexone-induced decrease in self-administration of thedrinking solution can be attributed to a reduction in the reinforcingefficacy of saccharin as opposed to ethanol. Opiate antagonistscan inhibit behavior maintained by both ethanol and nondrug reinforcerssuch as saccharin (Cooper, 1980; Ostrowski et al., 1980; Weisset al., 1990; Gauvin et al., 1993; Krishnan-Sarin et al., 1995).However, mean baseline ethanol intake in the present study wasremarkably similar to that in previous work with a nonsaccharin-containingethanol solution such that the sweetener seems to have added littleto the reinforcing efficacy of the drinkingsolution.

Therefore, the conclusion that the suppressant effects of naltrexone on ethanol self-administration are the result of interferencewith ethanol-induced increases in extracellular dopamine in theNAcc seems well justified. Interestingly, a dopaminergic linkin the suppression of ethanol self-administration by naltrexonewas reflected also in the specific behavioral changes inducedby the drug. Although the behavioral data were not recorded bymeans of cumulative response records precluding a more fine-grainedbehavioral analysis, closer inspection of the distribution ofresponding in terms of 1 min intervals revealed that naltrexonedid not seem to delay the onset of ethanol self-administration(data not shown). Instead, the marked reduction in ethanol intakeduring the first 5 min of the self-administration phase seemedto be the result of an early termination of responding for ethanolas indicated by the complete suppression of ethanol intake duringthe subsequent recording intervals. This pattern of effects issimilar to that induced by dopamine antagonists that shorten theduration of ethanol drinking bouts and accelerate the offset ofethanol-reinforced responding (Samson and Hodge, 1996). Thus,the specific changes in ethanol-maintained behavior by naltrexonewere consistent with the neurochemical data. These observationsnot only strengthen the conclusion that opiate antagonists suppressethanol self-administration by interfering with ethanol-inducedstimulation of accumbal dopamine activity but also provide furthersupport for the view that dopamine has a central role in ethanolreward.

The present behavioral effects of naltrexone are consistent with several previous reports that a single injection of an opiateantagonist does not affect the initiation of ethanol-seeking behaviorbut reduces alcohol intake after consumption has begun (Schwarz-Stevenset al., 1992; Hyytiä and Sinclair, 1993). In conjunction withthe present neurochemical data, these behavioral observationsmay provide some insight into the processes that underlie thesuppression of ethanol consumption by opiate antagonists. Repeatedpairing of opiate antagonist treatment with access to alcoholcan lead to a progressive decline in ethanol intake followed bycontinued suppression of alcohol intake after termination of thechronic drug treatment (Hyytiä, 1993). This pattern of behavioraleffects is indicative of extinction of ethanol-reinforced behavior.Thus, it is possible that by inhibiting the pharmacological effectsof ethanol on accumbal dopamine activity, opiate antagonists maydiminish the rewarding properties of ethanol and, thereby, leadto eventual extinction of ethanol-seekingbehavior.

Finally, the inhibition of the effect of ethanol by naltrexone during the self-administration phase also implicates activationof endogenous opioid systems in the dopaminergic effects of ethanol.Opioid peptides are released in response to acute ethanol administration(de Waele and Gianoulakis, 1990, 1993; Gianoulakis, 1990; de Waeleet al., 1992, 1994), although this has not yet been demonstratedin the context of ethanol self-administration. Nonetheless, thepresent results support the hypothesis that direct or indirectactivation of opioid peptide systems is part of the mechanismby which ethanol increases extracellular dopamine levels in theNAcc and maintains ethanol-reinforced behavior. However, it cannotbe eliminated that nondopaminergic mechanisms coupled to opioidreceptors may have contributed to the suppression of ethanol intakebynaltrexone.

Confirming previous observations (Weiss et al., 1993), a transient rise in dialysate dopamine concentrations was observedduring the presession waiting period in both groups of rats. Thesignificance of this dopaminergic activation is, at present, stillunclear. It is possible that this effect is a consequence of thepresence of incentive motivational stimuli that are predictiveof impending availability of ethanol (see also Vavrousek-Jakubaet al., 1991; Katner et al., 1996) and may have an "attentional"function or play a role in the initiation of ethanol-seeking behavior.This phenomenon is not accounted for by effects of nonspecificarousal as a result of handling and transfer of the animals fromthe home to the test cage because it is not seen under conditionsin which no reinforcer is expected (Weiss et al., 1993). Similar"anticipatory" increases in dopamine release have been observedwith saccharin and food reinforcers (Weiss et al., 1993; Wilsonet al., 1995), and recent data suggest that expectation of a positivereinforcer is associated with a discrete increase in the firingrate of mesolimbic dopamine neurons (Schultz et al., 1997). Thus,stimulation of dopamine neuronal activity and release seems tobe associated with the anticipation of reinforcing stimuli ingeneral and is not restricted to drugreinforcers.

Naltrexone seemed to augment the increase in dialysate dopamine concentrations during the early stage of the presession waitingperiod. The naltrexone effects during the waiting period mustbe viewed with some caution, however. Although the rise in dopamineduring the waiting period was greater in the naltrexone groupwhen the data are examined in terms of the relative (percent ofbasal) increase in neurotransmitter levels, the actual net increasein dopamine concentrations (in nanomolar) was virtually identicalin the two groups, and statistical analysis of the raw (dopamineconcentration) data did not reveal significant differences orinteractions between the effects of naltrexone and saline treatmentduring this experimental phase. Therefore, the apparent groupdifferences in the percent of baseline values were attributableto the slightly (but not significantly) lower average baselinedopamine concentrations in the naltrexone versus the control group,which resulted in an inflation of the percent of baseline valuesafter transformation of thedata.

The apparent lack of suppression by naltrexone of the increase in dialysate dopamine levels during the waiting period contrastssharply with the significant attenuation of ethanol-induced dopamineoutput during the self-administration phase. This is an intriguingobservation because it may suggest that activation of accumbaldopamine release in response to anticipation of the drug reinforcermay be mediated by different neural mechanisms than are the dopaminergiceffects of ethanol. The interpretation of the naltrexone effectsduring the waiting period is complicated, however, by pharmacokineticconsiderations. Because the present study was designed to investigatethe effects of naltrexone on ethanol self-administration and theefficacy of ethanol to increase extracellular dopamine levels,the timing of naltrexone administration (i.e., 30 min pre-ethanol)was scheduled with respect to the onset of the self-administrationsession. Consequently, at the onset of the waiting period only10 min had elapsed since naltrexone injections, a time that coincideswith the rising phase of the brain and blood levels of the drug(Misra et al., 1976; Wall et al., 1984). Whether or not naltrexonecan alter the dopaminergic response to the anticipation of ethanolcan, therefore, not be conclusively determined on the basis ofthe present data. In view of the inhibitory effects of naltrexoneon ethanol craving and relapse in human alcoholics (Volpicelliet al., 1995; Jaffe et al., 1996; O'Malley, 1996) and on ethanol-seekingbehavior in animal models of relapse (Katner et al., 1999; C.Heyser, K. Mog, and G. Koob, unpublished observations), it willbe important to more systematically examine the interactions betweenthis opiate antagonist and the effects of environmental stimulipredictive of ethanolavailability.

In summary, the results indicate that both ethanol-reinforced behavior and ethanol-induced elevation of extracellular dopaminein the NAcc are inhibited by acute administration of naltrexone,a nonselective opiate receptor antagonist, at a dose that is selectivefor opiate receptor blockade in vivo. Analysis of dose-effectfunctions revealed a significant positive correlation betweenethanol intake and increases in accumbal extracellular dopaminelevels in saline-treated controls but not in naltrexone-treatedrats. Confirming previous observations, a significant rise indialysate dopamine concentrations was observed during a waitingperiod that preceded access to ethanol. In contrast to ethanol-induceddopaminergic activation, this effect was not clearly modifiedby naltrexone under the present experimental conditions. Thesedata support the conclusion that reduction in the efficacy ofethanol to increase extracellular dopamine concentrations in theNAcc contributes to the suppression of ethanol self-administrationby naltrexone and, presumably, other opiateantagonists.

  FOOTNOTES

Received Aug. 27, 1998; accepted Sept. 29, 1998.

This work was supported by the National Institute on Alcohol Abuse and Alcoholism Grants AA10531 (F.W.) and AA00147 (R.A.G.).This manuscript is publication No. 11488NP from The Scripps ResearchInstitute. We wish to thank Dr. Charles O'Brien for inspirationalcomments and discussion. We also thank Tony Kerr and BrigitteNadeau for skillful technical assistance with microdialysis andwith analytical and behavioralprocedures.
Correspondence should be addressed to Dr. Rueben Gonzales, Department of Pharmacology, College of Pharmacy, University ofTexas at Austin, Austin, TX78712.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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J. Pharmacol. Exp. Ther., March 1, 2002; 300(3): 882 - 889.
[Abstract] [Full Text] [PDF]

F. Weiss, C. S. Maldonado-Vlaar, L. H. Parsons, T. M. Kerr, D. L. Smith, and O. Ben-Shahar
Control of cocaine-seeking behavior by drug-associated stimuli in rats: Effects on recovery of extinguished operant-responding and extracellular dopamine levels in amygdala and nucleus accumbens
PNAS, April 11, 2000; 97(8): 4321 - 4326.
[Abstract] [Full Text] [PDF]

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