Behavioral Evidence of Depolarization Block of Dopamine Neurons after Chronic Treatment with Haloperidol and Clozapine

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Hazardous Substances DB
APOMORPHINE
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HALOPERIDOL

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The Journal of Neuroscience, February 1, 2000, 20(3):1229-1239

Behavioral Evidence of Depolarization Block of Dopamine Neurons after Chronic Treatment with Haloperidol and Clozapine
Sandra M. Boye¹ and Pierre-Paul Rompré¹^,²
¹ Center for Studies in Behavioral Neurobiology, Concordia University, Montreal, Québec, Canada, H3G 1M8, and ² Centre de Recherche de l'Hôpital du Sacré-Coeur et Département de Psychiatrie, Université de Montréal, Montréal, Québec, Canada, H3C 3J7

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiological studies have shown that chronic treatment with haloperidol causes depolarization block (DB) of dopaminecells in anesthetized and paralyzed rats. It has been proposedthat the emergence of DB underlies the therapeutic and side effectsof this drug. However, the relevance of DB to the clinical actionsof haloperidol has been questioned on the grounds that chronicdrug-induced DB has not yet been demonstrated in freely movinganimals. In this study, responding for rewarding electrical brainstimulation was used to assess the occurrence of DB in rats chronicallytreated with haloperidol or clozapine. The time course of theeffects of acute haloperidol (7.8-500 µg/kg) and clozapine (5-40mg/kg) and of withdrawal from chronic drug treatment on rewardand performance measures were also characterized. Haloperidoland clozapine dose-dependently attenuated reward and performance,haloperidol producing a predominant suppression of performance,and clozapine preferentially attenuating reward. Chronic (21 d)treatment with haloperidol (500 µg/kg) caused responding to ceasein the six rats tested, and repeated injection with apomorphinerestored the behavior in all of them; such an effect of apomorphinewas observed in only two of six rats treated acutely with thesame dose of haloperidol. Chronic treatment with clozapine (20mg/kg) increased reward thresholds, an effect that was reversedby apomorphine in chronically, but not acutely, treated rats.The times at which chronic haloperidol-treated rats resumed respondingwas positively correlated with indices of behavioral supersensitivityafter withdrawal, suggesting that the effect of apomorphine wasnot caused by direct stimulation of upregulated postsynaptic receptors.These findings constitute the first behavioral evidence of DBin unanesthetized, freely moving animals treated chronically withantipsychotics. They also demonstrate that the neural substratesmediating reward and performance are functionally independentand differentially sensitive to haloperidol andclozapine.

Key words: apomorphine; behavioral supersensitivity; clozapine; depolarization block; dopamine; haloperidol; reward

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acutely, classical antipsychotics are potent stimulants of midbrain dopamine (DA) cell firing. Chronically, however, classicalantipsychotics produce complete cessation of firing activity ina majority of midbrain DA cells (Bunney and Grace, 1978), a phenomenonresulting from sustained depolarization of the membrane potentialas a consequence of prolonged excitation (Grace and Bunney, 1986);firing activity in these cells can be reinstated after repolarizationof the membrane potential. Repeated treatment with atypical antipsychoticsalso produces depolarization block (DB) of midbrain DA cells.However, although both classical and atypical antipsychotics inactivatemesolimbic (A10) DA cells, only the former additionally inactivatenigrostriatal (A9) DA cells (Chiodo and Bunney, 1983; White andWang, 1983b; Skarsfeldt, 1988). It has been proposed that DB ofA10 and A9 DA cells may contribute, respectively, to the therapeuticeffect and extrapyramidal syndromes associated with classicalantipsychotics (e.g., haloperidol), whereas the selective inactivationof A10 DA cells may reflect the reduced propensity for extrapyramidalsyndromes associated with atypical antipsychotics (e.g., clozapine)(for review, see Grace et al., 1997).

Two behavioral studies have provided findings consistent with induction of DB of midbrain DA cells. In both, responding forrewarding electrical brain stimulation (EBS) ceased after acuteneuroleptic treatment combined with either morphine (Rompré andWise, 1989) or a partial DA lesion (Doherty and Gratton, 1991).That the absence of responding was attributable to DB is supportedby the finding that, in both studies, responding was restoredwith drugs that normally hyperpolarize DA cells. In a third study,acute neuroleptic challenge produced greater catalepsy and akinesiain rats with partial DA lesions than in controls, a differenceattributed to induction of DB (Hollerman et al., 1992). To date,it has not been demonstrated that chronic exposure to antipsychoticdrugs leads to DB in intact, freely moving animals. Moreover,although early electrophysiological studies performed on unanesthetizedrats have provided evidence of DB after repeated exposure to antipsychoticdrugs (Bunney and Grace, 1978; Chiodo and Bunney, 1985), two recentstudies have failed to replicate this finding (Mereu et al., 1994,1995; Melis et al., 1998). These inconsistent findings and thelack of behavioral data from chronically treated animals haveled some to propose that DB results from the combined influenceof anesthesia and the stimulatory effects of haloperidol and thesampling procedure (Mereu et al., 1994, 1995; Melis et al., 1998).

The primary purpose of this study was to test the hypothesis that chronic treatment with haloperidol leads to the developmentof DB in freely moving animals responding for rewarding EBS. Thisbehavioral paradigm was chosen because it is sensitive to manipulationsof central dopamine neurotransmission (Gallistel and Karras, 1984;Gallistel and Freyd, 1987; Rompré and Wise, 1989), and it hasbeen used previously to infer DB of DA cells (Rompré and Wise,1989; Doherty and Gratton, 1991). For comparison, the effectsof chronic treatment with clozapine were also studied. To betterunderstand the results of the DB test, the effects of acute andpostwithdrawal haloperidol and clozapine on reward and performancewere alsocharacterized.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects. Subjects were male Long-Evans rats weighing between 350 and 450 gm at the time of surgery. Each rat was individuallyhoused, had access to food and water ad libitum, and was maintainedon a 14/10 hr light/dark cycle (lights off at 5:30 P.M.). Behavioraltesting was performed during the lightphase.

Surgery. Twenty minutes before surgery, rats were treated with atropine sulfate (0.5 mg/kg) to reduce mucous secretion. Undersodium pentobarbital anesthesia (Somnotol, 65 mg/kg, i.p.), animalswere stereotaxically implanted with a moveable stimulation electrode(Kinetrods, SME-01) aimed at the medial mesencephalic centralgray using the following flat skull coordinates: 7.6 mm behindbregma, 0.0 mm lateral to bregma, and 6.6 mm below the skull (Paxinosand Watson, 1986). A flexible wire connected at one end to a maleamphenol pin and wrapped around six stainless steel mounting screwsthat were threaded into the cranium served as the inactive electrode(anode). Acrylic dental cement was used to chronically securethe electrode assembly to theskull.

Apparatus. Behavioral testing was performed in operant chambers made from plywood and Plexiglas. Each chamber was equippedwith a lever (Lehigh Valley, Allentown, PA) that protruded fromthe left wall, 5 cm above the wire-mesh floor. To minimize disturbancescaused by noise, chambers were encased in wooden boxes insulatedwith Styrofoam; a Plexiglas front window allowed constant viewingof therat.

Each depression of the lever triggered a constant-current generator to deliver a single 200 msec train of 0.1 msec cathodalrectangular pulses. Each stimulation train was followed by an800 msec intertrain interval during which stimulation was notavailable (Boye and Rompré, 1996). Current intensity was monitoredon an oscilloscope by reading the voltage drop across a 1 K $Omega$ resistorin series with therat.

Behavioral training. Forty-eight to 72 hr after surgery, animals were trained to lever press for stimulation of the mesencephaliccentral gray region using conventional shaping procedures. Ifthe stimulation induced aversive reactions or did not supportlever pressing, the electrode was lowered by 0.32 mm and the nextsite was tested; generally, lowering the electrode once was sufficient.Once the lever-pressing response was established, rats were allowedto lever press continuously for 1 hr at stimulation parametersset to support vigorous responding. Rats were then tested duringsessions in which the stimulation current intensity was held constantand the number of pulses per train was systematically reduced.A "pass" consisted of testing a descending series of pulse numbers,in ~0.1 log unit steps, ranging from a value that sustained maximalresponse rates (31 pulses per train, 155 Hz) to a value that failedto sustain responding (two pulses per train, 10 Hz). To ensurethat the rat was within proximity of the lever at the time thatthe highest pulse number was delivered, an additional pulse number(26 pulses per train, 130 Hz) was included at the beginning ofeach pass; responses to this pulse number were not included indata analyses. On a given pass, each pulse number was tested duringa single 45 sec trial; the first 5 sec of each trial were considereda "frequency adaptation" period, and only responses emitted duringthe last 40 sec were used for analysis. Each trial was precededby five noncontingent (priming) trains of stimulation that wereidentical to those available during the trial. A 30 sec intertrialinterval separated the testing of each pulse number. In each ofthe experiments reported here, the same range of pulse numbers(from 31 to 2 pulses per train) was tested during baseline (predrug)and drugconditions.

Data obtained from each pass generated a curve that described response rates as a function of pulse number (response-numbercurve). From each curve, an index of rewarding efficacy of thestimulation (reward threshold) was extrapolated and operationallydefined as the pulse number that sustained a half-maximal rateof responding (M50 index). Training was considered complete whenreward thresholds varied by <0.1 log units across several days.Each response-number curve yielded two measures: (1) rewardingefficacy of the stimulation (reward threshold) and (2) performance(maximal response rate). In each of the three experiments thatfollow, rats treated with haloperidol, clozapine, or vehicle weretested inparallel.

Experiment 1: acute haloperidol-clozapine. On the test day, four baseline response-number curves were first determined. Ratswere then removed from their cages and injected subcutaneouslywith haloperidol (7.8, 15.63, 31.25, 62.5, 125, or 500 µg/kg),clozapine (5, 10, 20 or 40 mg/kg), or vehicle (0.3% tartaric acidin physiological saline). Each rat was tested with only one dose,and each dose was tested on a total of six rats. Rats were immediatelyreturned to their respective test cages, and a response-numbercurve was determined every 30 min, beginning immediately, forthe next 6.5-10 hr. For any given curve, responding was not consideredstable unless response rates for at least two consecutive pulsenumbers were both greater than five responses per trial and wereboth higher than the half-maximal rate. In cases in which ratsceased responding, the entire range of pulse numbers was nonethelesstested. All rats received the same amount of priming stimulation(five trains), and no attempt was made to deliver extra stimulationto induceresponding.

Experiment 2: test of depolarization block. Rats were divided into five groups (n = 12), each of which received a differentdrug regimen for 21 d: 500 µg · kg¹ · d¹ haloperidol [chronic haloperidol (CHAL)], 20 mg · kg¹ · d¹ clozapine [chronic clozapine (CCLOZ)], 3 mg · kg¹ · d¹ tartaric acid [chronic vehicle (CVEH)], or CVEH for 20 d plus500 µg/kg haloperidol or 20 mg/kg clozapine on day 21 (CVEHH orCVEHC, respectively). All drugs were administered subcutaneously,between 10 A.M. and 12 P.M. Some of the rats used in this secondexperiment had been used previously in experiment 1. Rats thatwere treated with haloperidol in experiment 1 (n = 11) were assignedto the CHAL group, those treated with clozapine (n = 6) to theCCLOZ group, and those treated with vehicle to the CVEH (n = 4),CVEHH (n = 4), or CVEHC (n = 6) groups. Before the start of thechronic drug regimen, four response-number curves were determinedfor each rat, and mean threshold and response rate values werecalculated from the last three curves; this constituted baselinevalues for each rat. For those rats that had been tested previouslyin experiment 1, baseline values for experiment 2 were the sameas for experiment1.

Two hours after the 21st injection, rats were tested on two initial passes (at 120 and 140 min after injection). Immediatelyafter the end of the second pass, half of the rats in each group(n = 6) were treated with an intraperitoneal injection of apomorphine(APO) and immediately tested on a third pass. In total, five dosesof APO were administered (12.7, 25.4, 50.8, 101.7, and 203.3 µg/kg),each separated by a period of testing (a single pass) that lasted~20 min. Cumulative administration of APO was used as a test ofDB because this treatment has been shown previously to reverseDA cell DB in electrophysiological studies (Grace and Bunney,1986). The second half of each group (n = 6) received five vehicle(VEH) injections (0.2 mg/kg ascorbic acid in physiological saline).After the last APO or VEH injection, rats were tested on threeconsecutive passes, followed by a single pass every 30 min. Intotal, the test session lasted ~4 (CCLOZ and CVEHC) to 8 hr (CHAL,CVEHH, andCVEH).

Experiment 3: withdrawal from chronic haloperidol-clozapine. Beginning 24 hr after the test of DB (experiment 2), all subjectswere tested daily for an additional 28 d. Testing consisted offour daily response-number curve determinations. Mean reward thresholdsand maximal response rates were calculated only from the lastthree curves. For each rat, the baseline threshold and responserate values that were used in this experiment were the same asthose of experiment2.

Histology. Subjects were anesthetized with sodium pentobarbital, and the stimulation site was marked with a small lesion causedby passing direct anodal current through the stimulation electrode(100 µA, 20 sec). Rats were then intracardially perfused withsaline, followed by 10% formalin in saline. Brains were removedand immersed in 10% formalin containing 3% potassium ferrocyanide,3% potasssium ferricyanide, and 0.5% trichloroacetic acid; thisresulted in a blue staining of the lesion site. Twenty-four hourslater, brains were removed from this solution and kept in 10%formalin. Forty-eight hours before slicing, brains were immersedin 10% formalin containing 30% sucrose. Frozen brains were slicedinto 40 µm sections, dried, and stained with thionine for lightmicroscopicverification.

Drugs. Haloperidol (Research Biochemicals Inc., Natick, MA) and clozapine (Sandoz, Dorval, Quebec) were dissolved in 0.9%saline containing 0.3% (w/v) tartaric acid. Apomorphine (Sigma,St. Louis, MO) was dissolved in 0.9% saline containing 0.02% (w/v)ascorbic acid. All drugs were aliquotted into 1 ml Eppendorf tubesand kept frozen until just beforeuse.

Data analysis. The data were analyzed with one-way ANOVA or two-way mixed ANOVA (with drug dose as the between-subject factorand time as the repeated measure). Post hoc analyses involvingmultiple comparisons with a single control group were made withDunnett's tests, whereas multiple comparisons between two groupswere done with Tukey tests. A priori comparisons were done withStudent's t tests with Bonferroni corrections. All probabilityvalues are two-tailed. In experiment 1, the effects of acute treatmentwith 62.5, 125, and 500 µg/kg haloperidol were analyzed by calculatingthe 95% confidence interval for the vehicle control conditionand determining which values in the three drug groups differedstatistically.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1: acute haloperidol-clozapine

The three lowest doses of haloperidol increased reward thresholds and reduced response rates. The largest increase in rewardthresholds (33%) was observed after 31.25 µg/kg, an effect thatlasted ~180 min (Fig. 1a). Results of a two-way ANOVA revealeda significant effect of dose (F_(3,20) = 4.74; p < 0.05) and asignificant dose × time interaction (F_(27,180) = 1.55; p < 0.05),but no effect of time (F_(9,180) = 0.86; p = 0.56). Post hoc testsrevealed that the 7.8 µg/kg dose caused a significant increasein reward thresholds at 60, 120, and 180 min and the 31.25 µg/kgdose at all time intervals between 0 and 180 min. Reward thresholdswere not altered after treatment with 15.63 µg/kg. The greatestreduction in response rates (41%) occurred 60 min after treatmentwith 31.25 µg/kg (Fig. 1b). A two-way ANOVA revealed a significanteffect of dose (F_(3,20) = 7.24; p < 0.01), time (F_(9,180) = 8.69;p < 0.0001), and a dose × time interaction (F_(27,180) = 1.70;p < 0.05). Post hoc tests revealed that response rates were significantlyreduced between 30 and 60 min after treatment with 15.63 µg/kgand at all time intervals after 31.25 µg/kg. Response rates didnot change after treatment with 7.8 µg/kg.

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Figure 1. Time course of changes in reward thresholds (a) and maximal response rates (b) after treatment with haloperidol [7.8 µg/kg ( $open circle$ ), 15.63 µg/kg ( $triangle$ ), and 31.25 µg/kg ()] and vehicle ( $black-down-triangle$ ), as a function of time after injection. Each point (n = 6) is expressed as percent of baseline and represents the mean ± SEM. Threshold and response rate data obtained from the vehicle (control) group are the same in this figure and Figure 2. Although the test session in the vehicle control condition lasted 630 min, rats treated with the three lowest doses of haloperidol were tested only for 270 min because of the short time course of the effects of these doses. For clarity, only data collected between 0 and 270 min after vehicle injection are illustrated. For ease of comparison between reward thresholds and response rates, in all the figures, changes in the latter are also plotted on a semilogarithmic scale. $dagger$ p < 0.05, 7.8 µg/kg versus vehicle; *p < 0.05, 15.63 µg/kg versus vehicle; #p < 0.05, 31.25 µg/kg versus vehicle; Dunnett's tests.

Treatment with the three highest doses of haloperidol caused some animals to cease responding (Fig. 2). Because of the low(e.g., n = 1) and unequal number of animals responding at sometime periods, the data could not be subjected to ANOVA. Instead,the 95% confidence interval for the vehicle data were calculatedand used to determine significant differences between drug andvehicle groups. The 62.5 µg/kg dose produced a maximal increaseof 125% in reward thresholds (30 min) and reduced response ratesby 65% (60 min) (Fig. 2a,b). At this dose, five of the six ratsceased responding during at least one time interval, and whenthe behavior was restored, threshold values were not differentfrom vehicle; response rates, however, remained significantlyreduced throughout the entire session. At a dose of 125 µg/kg,haloperidol caused a maximal increase of 98% in reward thresholds(first point) and reduced response rates by 80% (30 min) (Fig.2c,d). In five of six animals, responding ceased for at least1.5 hr (from 30 to 120 min after injection). At this dose, theinhibitory effects of haloperidol had a similar time course onthresholds and response rates. Treatment with 500 µg/kg causeda maximal increase of 197% in reward thresholds (first point)and reduced maximal response rates by 75% (480 min) (Fig. 2e,f).At this dose, one animal stopped responding immediately afterinjection, and another never resumed, even after 10.5 hr. Noneof the rats treated with 500 µg/kg responded between 30 and 360min after injection. Again, maximal response rates remained significantlyreduced throughout the entire test session and, compared withreward thresholds, were characterized by a late and gradual recovery.

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Figure 2. Time course of changes in reward thresholds ( $open circle$ , top) and maximal response rates ( $triangle$ , bottom) after treatment with haloperidol (62.5, 125, and 500 µg/kg) and vehicle ( $black-down-triangle$ ), as a function of time after injection. Numbers above or below each point indicate the number of rats responding at each time interval. Each point (n = 6) is expressed as percent of baseline and represents the mean ± SEM. Filled symbols in the drug conditions indicate values that lie beyond the 95% confidence interval of the vehicle curve (p < 0.05).

Immediately after injection (first point), clozapine doses of 5-40 mg/kg increased reward thresholds dose-dependently, aneffect that reached a maximum (82% increase) at the highest dose(Fig. 3a). Results of a two-way ANOVA revealed a significant effectof dose (F_(4,25) = 7.85; p < 0.001), time (F_(13,325) = 3.87; p< 0.0001), and a dose × time interaction (F_(52,325) = 2.06; p< 0.0001). Post hoc tests revealed that reward thresholds werenot statistically different from vehicle control values afterthe 5 mg/kg dose but were significantly higher immediately afterinjection of 10 mg/kg, and at all time intervals except 60 and240 min after 20 mg/kg. The highest dose of clozapine (40 mg/kg)caused a significant increase in reward thresholds between 0 and150 min and at 210 min after injection. Clozapine also reducedmaximal response rates, an effect that reached a maximum (50%decrease) 30 min after treatment with 40 mg/kg (Fig. 3b). A two-wayANOVA revealed a significant effect of dose (F_(4,25) = 3.00; p< 0.05), time (F_(13,325) = 7.87; p < 0.0001), and a dose × timeinteraction (F_(52,325) = 2.09; p < 0.0001). Post hoc tests revealedthat clozapine reduced maximal response rates significantly between30 and 180 min after 10 and 40 mg/kg, and between 30 and 120 minand between 180 and 240 min after 20 mg/kg.

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Figure 3. Time course of changes in reward thresholds (a) and maximal response rates (b) after treatment with clozapine [5 mg/kg ( $open circle$ ), 10 mg/kg ( $triangle$ ), 20 mg/kg (), and 40 mg/kg ( $diamond$ )] and vehicle ( $black-down-triangle$ ), as a function of time after injection. Each point (n = 6) is expressed as percent of baseline and represents the mean ± SEM. $dagger$ p < 0.05, 10 mg/kg versus vehicle; *p < 0.05, 20 mg/kg versus vehicle; #p < 0.05, 40 mg/kg versus vehicle; Dunnett's tests.

Experiment 2: test of depolarization block

Effect of APO on CVEH-treated rats
In animals treated chronically with vehicle (CVEH), APO increased reward thresholds by 32% (Fig. 4a) and reduced maximal responserates by 23% (Fig. 4b). During this time, animals displayed hypomobility.A two-way ANOVA performed on threshold data did not reveal aneffect of treatment (F_(1,10) = 0.04; p = 0.84), time (F_(19,190)= 1.25; p = 0.23), or a treatment × time interaction (F_(19,190)= 1.16; p = 0.29). A two-way ANOVA performed on response ratedata did not reveal an effect of treatment (F(1,10)=0.28, p =0.61) or time (F_(19,190) = 1.06; p = 0.40) but yielded a significanttreatment × time interaction (F_(19,190) = 3.03; p < 0.0001). Posthoc tests showed that, compared with VEH-treated rats, maximalresponse rates in the APO-treated group were significantly lowerat 120, 200, and 220 min.

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Figure 4. Time course of changes in reward thresholds (a) and maximal response rates (b) after treatment with cumulative doses (12.7, 25.4, 50.8, 101.7, and 203.3 µg/kg) of APO or VEH in CVEH-treated rats. Values are expressed as percent of baseline and are plotted as a function of time since the 21st injection of vehicle. Each point (n = 6) represents the mean ± SEM. Arrows indicate times of APO or VEH injection. Thresholds: , CVEH+APO; $open circle$ , CVEH+VEH. Response rates: $black-triangle$ , CVEH+APO; $triangle$ , CVEH+VEH. **p < 0.01; Tukey tests.

Effect of APO on CHAL-treated rats
Eight of the 12 rats treated chronically with haloperidol (CHAL, 500 µg/kg) did not initially respond for the stimulation(Figs. 5b,c,e,f, 6a-c,e), and three others stopped respondingafter behavioral testing had begun (Figs. 5a,d, 6d). One rat respondedat all time periods (Fig. 6f). Every rat (six of six) treatedwith APO resumed responding before the end of the test session,200-400 min after the 21st injection of haloperidol. In contrast,treatment with VEH restored responding in only two of four rats,both at 490 min after the 21st injection of haloperidol (Fig.6b,c). Note that responding was considered to have ceased whenthe animals failed to lever press on two consecutive passes. Likewise,the behavior was not considered restored unless it was presenton two consecutive passes.

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Figure 5. Time course of changes in reward thresholds () and maximal response rates ( $black-triangle$ ) after administration of APO to rats treated with CHAL (500 µg/kg). Data obtained from individual animals are shown. Values are expressed as percent of baseline and are plotted as a function of time since the 21st injection of haloperidol. Arrows indicate times of APO injection. NO SS, No self-stimulation.

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Figure 6. Time course of changes in reward thresholds () and maximal response rates ( $black-triangle$ ) after administration of VEH to rats treated with CHAL (500 µg/kg). Data obtained from individual animals are shown. Values are expressed as percent of baseline and are plotted as a function of time since the 21st injection of haloperidol. Arrows indicate times of VEH injection. NO SS, No self-stimulation.

Effect of APO on CVEHH-treated rats
Of the 12 rats that were treated chronically with vehicle followed by acute haloperidol (500 µg/kg) on day 21 (CVEHH), ninedid not initially respond (Figs. 7a,c-f, 8a,c,d,f), and the remainingthree stopped after the first pass (Figs. 7b, 8b,e). Respondingresumed in only 4 of 12 rats: two after treatment with APO (Fig.7e,f) and two after VEH (Fig. 8e,f). Two additional rats respondedduring single passes only (Fig. 8c,d).

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Figure 7. Time course of changes in reward thresholds () and maximal response rates ( $black-triangle$ ) after administration of APO to rats treated with CVEHH (chronic vehicle for 20 d plus 500 µg/kg haloperidol on day 21). Data obtained from individual animals are shown. Values are expressed as percent of baseline and are plotted as a function of time since injection of haloperidol. Arrows indicate times of APO injection. NO SS, No self-stimulation.

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Figure 8. Time course of changes in reward thresholds () and maximal response rates ( $black-triangle$ ) after administration of VEH to rats treated with CVEHH (chronic vehicle for 20 d plus 500 µg/kg haloperidol on day 21). Data obtained from individual animals are shown. Values are expressed as percent of baseline and are plotted as a function of time since injection of haloperidol. Arrows indicate times of VEH injection. NO SS, No self-stimulation.

The bar graph in Figure 9 summarizes the above findings by illustrating the percentage of rats in each group that resumedlever pressing and the mean time at which this occurred. A $chi$ ² test revealed that a significantly higher number of CHAL+APO-treatedrats resumed responding compared with those treated with CHAL+VEH,CVEHH+APO, or CVEHH+VEH (p < 0.05). Note that the effectivenessof APO in restoring the behavioral response was seen only in CHAL-treatedrats, because the number of CVEHH+APO-treated rats that resumedresponding did not differ from those treated with CVEHH+VEH. Last,those animals treated with CHAL+APO resumed responding sooner(282 ± 33.90 min) than those treated with CHAL+VEH (490 min; Bonferronit₍₆₎ = 3.36; p < 0.05), CVEHH+APO (475 ± 45 min; Bonferroni t₍₆₎= 2.95; NS), or CVEHH+VEH (460 ± 35 min; Bonferroni t₍₆₎ = 2.80;NS).

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Figure 9. Percentage of animals in each drug condition that resumed responding (on at least 2 consecutive passes) before the end of the test session (open bars) and the times at which this occurred (hatched bars; bar heights represent mean ± SEM). *p < 0.05; $chi$ ² test.

Effect of APO on CCLOZ- and CVEHC-treated rats
None of the rats treated with CCLOZ (20 mg/kg) ceased responding at any time interval (Fig. 10a,b). A two-way ANOVA performedon threshold data did not reveal a significant effect of treatment(F_(1,10) = 0.09; p = 0.77), but a significant effect of time (F_(11,110)= 7.09; p < 0.0001) and a significant treatment × time interaction(F_(11,110) = 2.56; p < 0.01) were found. Post hoc tests indicatedthat, in animals treated with APO, thresholds were significantlylower than in VEH-treated animals at 310 and 340 min (Fig. 10a).A two-way ANOVA on response rate data did not reveal any effectof treatment (F_(1,10) = 0.55; p = 0.47), time (F_(11,110) = 1.09;p = 0.37), or a treatment × time interaction (F_(11,110) = 0.88;p = 0.56) (Fig. 10b). Likewise, animals treated chronically withvehicle followed by acute clozapine (20 mg/kg) on day 21 (CVEHC)responded at all time periods (Fig. 10c,d). A two-way ANOVA performedon threshold data did not reveal an effect of treatment (F_(1,10)= 0.36; p = 0.56), time (F_(11,110) = 1.88; p = 0.05), or a treatment× time interaction (F_(11,110) = 1.56; p = 0.12) (Fig. 10c). A two-wayANOVA performed on response rate data yielded a significant effectof time (F_(11,110) = 13.23; p < 0.0001) and a treatment × timeinteraction (F_(11,110) = 3.35; p < 0.001) but no effect of treatment(F_(1,10) = 1.93; p = 0.19). Post hoc tests revealed that maximalresponse rates differed significantly between APO- and VEH-treatedrats 140-370 min after clozapine (Fig. 10d). Inspection of datafrom individual rats revealed that the high response rates inthe CVEHC+VEH group are mainly caused by the unusually high (67-161%above baseline) response rates of a single rat. If the contributionof this rat is removed, the difference between APO- and VEH-treatedgroups disappears between 120 and 160 min and is reduced by approximatelyhalf at all other time intervals (data not shown).

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Figure 10. Left, Time course of changes in reward thresholds (a) and maximal response rates (b) after administration of APO or VEH to rats treated with CCLOZ (20 mg/kg). Thresholds: , CCLOZ+APO; $open circle$ , CCLOZ+VEH. Response rates: $black-triangle$ , CCLOZ+APO; $triangle$ , CCLOZ+VEH. Right, Time course of changes in reward thresholds (c) and maximal response rates (d) after administration of APO or VEH to rats treated with CVEHC (chronic vehicle for 20 d plus 20 mg/kg clozapine on day 21). Thresholds: , CVEHC+APO; $open circle$ , CVEHC+VEH. Response rates: $black-triangle$ , CVEHC+APO; $triangle$ , CVEHC+VEH. Values are expressed as percent of baseline and are plotted as a function of time after injection of clozapine. Each point (n = 6) represents the mean ± SEM. Arrows indicate times of APO or VEH injection. *p < 0.05; **p < 0.01; Tukey tests.

Chronic drug treatment resulted in differences in animal weights. Results of a one-way ANOVA performed on total percent weightincrease on day 21 revealed a significant effect of dose (F_(4,55)= 15.58; p < 0.0001). Post hoc tests showed that, compared withthe CVEH group (16.9 ± 1.0%), total weight gain was significantlylower in the CHAL (12.9 ± 1.0%; p < 0.05) and CCLOZ (13 ± 1.0%;p < 0.05) groups and significantly higher in the CVEHH group (21.5± 1.0; p < 0.01). Animal weights in the CVEHC group (19 ± 0.58%)did not differ fromcontrol.

Experiment 3: withdrawal from chronic haloperidol-clozapine

Possible differences in baseline reward thresholds or maximal response rates as a consequence of treatment with APO or VEHin experiment 2 were determined separately in each drug group(CHAL, CCLOZ, and CVEH) with two-way ANOVA. These analyses revealedno significant effect of treatment or treatment × time interactionsfor either reward thresholds or maximal response rates. Consequently,data from rats preexposed to APO or VEH were pooled within eachdrug group (n = 12 in eachgroup).

Inspection of individual response-number curves revealed time-dependent transformations in the shape of the curves. Thesetransformations were particularly pronounced in the CHAL-treatedgroup and were characterized by a selective increase in responserates at high stimulation frequencies (i.e., in the asymptoticportion of the curves). The nature of these transformations violatesa major assumption that validates the use of M50 (half-maximalrate of responding) as a reliable index of the rewarding efficacyof the stimulation. Consequently, reward thresholds were inferredfrom the pulse number that just fails to induce responding (thetazero index); this behavioral criterion is insensitive to nonscalartransformations of the response-number curve as detected in thisexperiment (Miliaressis et al., 1986).

A two-way ANOVA performed on reward thresholds did not reveal a significant effect of treatment (F_(2,33) = 0.49; p = 0.61)or a treatment × time interaction (F_(54,891) = 1.21; p = 0.15),but a significant effect of time was found (F_(27,891) = 3.89;p < 0.01) (Fig. 11a). A two-way ANOVA performed on maximal responserates did not reveal a significant effect of treatment (F_(2,33)= 0.41; p = 0.66), but a significant effect of time (F_(27,
891)= 1.58; p < 0.05) and a treatment × time interaction were found(F_(54,891) = 3.63; p < 0.01). Post hoc tests revealed that maximalresponse rates after withdrawal from CHAL treatment were significantlyhigher than CVEH values on days 3-13 and 15 and were significantlylower on days 24, 27, and 28 (Fig. 11b). Response rates increasedin all but two CHAL-treated animals; in these two rats, responserates were reduced by ~33 and 40%. The magnitude of the maximumincrease in response rates was variable in the remaining 10 animals,ranging from 12 to 99%.

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Figure 11. Time course of changes in reward thresholds (a) and maximal response rates (b) after withdrawal from CHAL ( $open circle$ ), CCLOZ (), and CVEH ( $black-triangle$ ) treatment. Values are expressed as percent of baseline and are plotted as a function of days after drug withdrawal. Each point (n = 12) represents the mean ± SEM. *p < 0.05; Dunnett's tests.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acute haloperidol-clozapine

Acute treatment with haloperidol and clozapine resulted in significant increases in thresholds and reductions in responserates, suggesting that these drugs attenuated both rewarding efficacyand performance, respectively. However, haloperidol had a longer-lastinginhibitory effect on response rates. This effect was most clearlyobserved after treatment with the three highest doses of haloperidoland was characterized by a fast and near-complete restorationof reward thresholds but a slow and gradual recovery of maximalresponse rates. The inhibitory effects of clozapine on thresholdsand response rates differed from those of haloperidol. First,immediately after injection, the three highest doses of clozapinecaused significant increases in thresholds in the absence of anysubstantial reduction in response rates; these were significantlyreduced only after 30 min. Second, clozapine had a longer-lastinginhibitory effect on thresholds than on response rates. Third,the magnitude of the effect of clozapine on reward thresholdsappeared to saturate with 20 mg/kg, whereas the peak reductionin response rates produced by 40 mg/kg was approximately twicethat of 20 mg/kg. Together, these findings strongly suggest thatthe underlying rewarding effect and the animals' capacity to respondare mediated by different neural substrates and that these aredifferentially sensitive to the inhibitory effects of haloperidolandclozapine.

Test of depolarization block

The primary aim of this experiment was to determine whether CHAL treatment leads to DB of midbrain DA cells in intact, freelymoving animals. We chose EBS as a behavioral paradigm becauseit is sensitive to changes in DA neurotransmission (Wise and Rompré,1989; Wise, 1996); we chose APO to test for DB because it hyperpolarizesDA cells (Grace and Bunney, 1985, 1986; Freeman and Bunney, 1987;Akaoka et al., 1992) and has been shown to reverse DB in electrophysiologicalstudies (Bunney and Grace, 1978; White and Wang, 1983a,b; Graceand Bunney, 1986). Two main findings suggest that CHAL treatmentresulted in DB of midbrain DA cells. First, the majority of CHAL-treatedrats did not respond when initially tested, but the behavior wasreinstated in every rat treated with APO. Thus, although APO byitself inhibited responding, it restored the behavior in ratstreated with CHAL. Moreover, the effectiveness of APO in repolarizingthe membrane potential of DA cells in a state to DB predicts afaster behavioral restoration in CHAL-treated rats injected withAPO than in those injected with VEH; this effect was also observedin experiment 2. In fact, the two CHAL-treated rats that resumedresponding after VEH injections did so at times that coincidewith the spontaneous recovery seen in acutely treated rats (compareFig. 6 with Figs. 2 and 8). Second, APO restored responding inrats treated chronically, but not acutely, with haloperidol. Infact, in the group of rats treated with CVEHH+APO, only 33% (twoof six) resumed responding, whereas all rats (six of six) treatedwith CHAL+APO did so. The differential effect of APO in animalstreated acutely and chronically with haloperidol suggests thatthe mechanisms underlying response cessation in these two groupsare different. In the CVEHH-treated group, the number of ratsthat resumed responding after APO or VEH did not differ, and thetimes at which responding resumed were also very similar betweenthese and rats treated with 500 µg/kg haloperidol in experiment1 (Fig. 2). These findings suggest that the absence of respondingin CVEHH-treated animals reflects (1) blockade of a significantproportion of postsynaptic DA receptors by haloperidol and (2)the inefficiency of APO in displacing the antagonist from postsynapticreceptor sites. Indeed, 2 hr after an acute subcutaneous injectionof 500 µg/kg haloperidol, ~80% of striatal DA D2 receptors arestill occupied (Schotte et al., 1993). Conversely, the effectivenessof APO in reinstating responding in CHAL-treated rats, despitethe continued presence of haloperidol, suggests DB in additionto blockade of postsynaptic receptors. Under these conditions,APO reinstates firing activity in previously inactivated DA cells,an effect that may be sufficient to overcome the postsynapticDA receptor blockade byhaloperidol.

Alternatively, the effect of APO in CHAL-treated rats may have been caused by direct stimulation of upregulated postsynapticDA receptors (Burt et al., 1977). Although the specific mechanismof action of APO cannot be determined solely on the basis of thepresent behavioral results, two main observations suggest thatthe contribution of direct postsynaptic stimulation by APO waslikely minimal. First, despite the availability of unoccupiedpostsynaptic receptor sites in CVEH-treated rats, APO had an inhibitoryeffect on responding, suggesting predominant stimulation of DAautoreceptors (Fouriezos and Francis, 1992). Although the totalcumulative dose of APO used in the present work (0.39 mg/kg) iswithin the range of doses known to stimulate postsynaptic DA receptorswhen administered in a bolus subcutaneous injection (Robertsonand Macdonald, 1986), intraperitoneal administration results in5-fold to 12-fold reductions in the stimulatory potency of APO(Barros et al., 1989). In addition, the brain elimination half-lifeof APO is ~25 min (Melzacka et al., 1978), suggesting submaximalsummation between successive doses of APO (i.e., administrationof each dose was separated by ~20 min). Second, chronic blockadeof DA D2 receptors also causes upregulation of somatodendritic(Stefanini et al., 1991) and terminal DA autoreceptors (Nowaket al., 1983; Saller and Salama, 1985). In fact, upregulationof DA D2 receptors in substantia nigra appears to be greater thanin striatum (76 vs 38%, respectively) (Stefanini et al., 1991).Greater upregulation of somatodendritic autoreceptors, togetherwith the greater sensitivity of these to DA and DA agonists (Skirbollet al., 1979), suggests a predominant role of these autoreceptors,rather than postsynaptic sites, in reinstating thebehavior.

All rats treated with CCLOZ responded throughout the test session. However, the increase in reward thresholds seen in CCLOZ-treatedrats was reversed by APO but not by VEH. In addition, APO restoredthreshold values in rats treated chronically, but not acutely,with clozapine. On the other hand, neither CCLOZ nor APO had anysubstantial effect on response rates. These findings may constitutea behavioral counterpart to electrophysiological work. Electrophysiologicalstudies have shown that CCLOZ treatment (20 mg/kg) results inselective DB of A10 DA cells (Chiodo and Bunney, 1983; White andWang, 1983b; Skarsfeldt, 1988, 1994) but leaves unaltered (Whiteand Wang, 1983b; Skarsfeldt, 1988, 1994) or increases (Chiodoand Bunney, 1983, 1985) the number of spontaneously active A9DA cells. Furthermore, White and Wang (1983b) have shown thatdoses of APO sufficient to reverse DB in A10 DA cells are ineffectivein altering the number of active A9 DA cells. It should be noted,however, that although DA neurotransmission in A10 DA cells isbelieved to be important for reward (Wise and Rompré, 1989),the degree to which response rates depend on A9 DA cell activityremains to bedetermined.

In summary, the findings of this second experiment reveal that DB of midbrain DA cells can be observed in awake, freely movinganimals, subsequent to chronic antipsychotic drug treatment. Althoughthese findings are consistent with electrophysiological findingsin anesthetized (Bunney and Grace, 1978; Chiodo and Bunney, 1983;White and Wang, 1983a,b) and conscious (Bunney and Grace, 1978;Chiodo and Bunney, 1985) animals, they do not support those ofMereu and colleagues (Mereu et al., 1994, 1995; Melis et al.,1998). Last, it is worth noting that only a subgroup of midbrainDA cells go into DB after chronic antipsychotic drug treatment.Recent electrophysiological work has shown that a subgroup ofmidbrain DA cells are indirectly stimulated by rewarding EBS ofthe mesencephalic central gray (Moisan and Rompré, 1998). Thepresent findings suggest that it is those DA cells that can entera state of DB that are important for the rewarding effect of thestimulation.

Withdrawal from chronic haloperidol-clozapine

Withdrawal from CHAL treatment did not produce any enduring change in reward thresholds. Thresholds were back to baselinevalues within 48 hr after drug withdrawal and remained stablefor the next 4 weeks. However, withdrawal from CHAL resulted ina significant increase in maximal response rates. This effectwas present 3 d after drug withdrawal and disappeared after ~2weeks. These findings suggest functional changes selectively inthose processes important for motoriccapacity.

Withdrawal from CCLOZ treatment did not suggest functional changes in either the neural substrates important for reward orperformance. These data contrast findings from a series of EBSstudies that used the same dose of clozapine and treatment regimenas those used here. In these earlier studies, CCLOZ treatmentcaused significant increases in response rates and reductionsin current-reset thresholds for stimulation sites in the ventraltegmental area but not the substantia nigra (Seeger and Gardner,1979; Gardner and Seeger, 1988; Gardner et al., 1993). Deliveryof EBS within the area of DA cell bodies in these earlier studiesrenders it difficult to make direct comparisons between previousand present findings and may in fact constitute the critical variablethat accounts for the observeddifferences.

The findings with CHAL have implications for interpretation of the behavioral restoration in CHAL+APO-treated rats in experiment2. First, the behaviorally supersensitive response was initiallyobserved 3 d after drug withdrawal. This suggests that, althoughreceptor upregulation may in fact have occurred during CHAL treatment,its behavioral consequences may have been masked by the presenceof haloperidol, a hypothesis consistent with previous findings(Clow et al., 1980; Rupniak et al., 1984, 1985). More importantly,direct stimulation of postsynaptic receptors by APO would predicta negative correlation between time of resumed responding in CHAL+APO-treatedrats and degree of behavioral supersensitivity. In fact, our datashow that those animals that eventually expressed the highestdegree of behavioral supersensitivity resumed responding laterthan those that expressed the lowest (Fig. 12). These findingsare not consistent with a significant contribution of supersensitivepostsynaptic receptors to the restoration of responding in CHAL+APO-treatedrats.

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Figure 12. Correlation between time (in minutes) of resumed responding in the six animals treated with CHAL+APO in experiment 2 and their highest degree of behavioral supersensitivity (percent of increase in maximal response rates) in experiment 3.

  FOOTNOTES

Received July 8, 1999; revised Nov. 9, 1999; accepted Nov. 9, 1999.

This work was supported by a grant from the Medical Research Council of Canada to P.-P.R. Clozapine was a generous gift fromSandoz (Dorval, Québec,Canada).
Correspondence should be addressed to P.-P. Rompré at his present address: Centre de Recherche Fernand-Seguin, Hôpital Louis-H.Lafontaine, 7331 Hochelaga, Montréal, Québec, Canada, H1N 3V2.E-mail: prompre{at}crfs.umontreal.ca.

Dr. Boye's present address: Department of Pharmacology and Therapeutics, McGill University, Montréal, Québec, Canada, H3G1Y6.

  REFERENCES

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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