A Role for Dopamine D1 Receptors of the Nucleus Accumbens Shell in Conditioned Taste Aversion Learning

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The Journal of Neuroscience, September 1, 2001, 21(17):6897-6904

A Role for Dopamine D1 Receptors of the Nucleus Accumbens Shell in Conditioned Taste Aversion Learning
Sandro Fenu, Valentina Bassareo, and Gaetano Di Chiara
Department of Toxicology and Consiglio Nazionale delle Ricerche, Center for Neuropharmacology, University of Cagliari, 09126 Cagliari, Italy

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The involvement of dopamine (DA) in conditioned taste aversion (CTA) learning was studied with saccharin or sucrose as theconditioned stimulus (CS) and intraperitoneal lithium as the unconditionedstimulus (US). The dopamine D₁ antagonist R(+)-7-chloro-8-hydroxy-3-methyl-1-phenyl-2,3,4,5-tetrahydro-1H-3-benzazepinehydrochloride (SCH 23390) (12.5-50 µg/kg, s.c.), given 5 min afterthe CS, impaired the acquisition of CTA in a paradigm consistingof three or a single CS-lithium association. SCH 23390 failedto impair CTA acquisition given 45 min after, 30 min before, orright before the CS. ( $-$ )-trans-6,7,7a,8,9,13b-hexahydro-3-chloro-2-hydroxy-N-methyl-5a-benzo-(D)-naphtho-(2,1b)azepine (SCH 39166) (12.5-50.0 µg/kg, s.c), a SCH 23390 analogthat does not bind to 5HT₂ receptors, also impaired CTA. No significantimpairment of CTA was obtained after administration of the specificD₂/D₃ antagonist raclopride (100 and 300 µg/kg, s.c.). The abilityof SCH 23390 to impair CTA learning was confirmed by its abilityto reduce the conditional aversive reactions to a gustatory CS(sweet chocolate) as estimated in a taste reactivity paradigm.SCH 39166 impaired CTA also when infused in the nucleus accumbens(NAc) shell 5 min after the CS. No impairment was obtained fromthe NAc core or from the bed nucleus stria terminalis. The resultsindicate that D₁ receptor blockade impairs CTA learning by disruptingthe formation of a short-term memory trace of the gustatory CSand that endogenous dopamine acting on D₁ receptors in the NAcshell plays a role in short-term memory processes related to associativegustatorylearning.

Key words: dopamine; D₁ receptors; nucleus accumbens shell; conditioned taste aversion; short-term memory; SCH 23390; SCH 39166; lithium chloride

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Organisms have the unique property of emitting responses or performing actions finalized to their survival and to the survivalof their species (Bindra, 1974; Epstein, 1982; Toates, 1986).This general process of motivation can be envisioned to startwith the evolutionary assignment of motivational valence (positiveor negative) to certain stimuli (primary motivational stimuli).Positive (appetitive) stimuli are innately capable of promotingapproach, contact, and consumption of the object stimulus; negative(aversive) stimuli, however, elicit reactions intended to avoidor terminate the stimulus. Drive state can affect the motivationalproperties of stimuli, increasing or decreasing it; learning,on the other hand, can assign a specific motivational valenceto otherwise neutral stimuli or change that of primary ones (Toates,1986).

Since the early observations of a loss of dopamine (DA) in the putamen of Parkinsonian patients (Ehringer and Hornykiewicz,1960) and the view (Mogenson et al., 1980) of the ventral striatumas an interface between motivation and action, DA has been traditionallyinvolved in the expression of motivated behavior. Accordingly,DA has been attributed different roles, activational (Salamone,1988), sensory-motor (Marshall and Teitelbaum, 1977; Salamone,1992), incentive-motivational (Wise, 1982; Berridge and Robinson,1998), all related to response expression. A role of DA in responseexpression, however, has always plagued any effort to demonstratea role of DA in the acquisition ofmotivation.

In principle a role of DA in this process might derive from its involvement in the hedonic properties of rewards (Wise etal., 1978) or in learning of the association between the stimuliand reward (Pavlovian learning), between responses and their outcome(instrumental learning), or between stimuli and responses (habitlearning) (Mackintosh, 1983; Dickinson and Balleine, 1994). Ifthe hypothesis of a role of DA in hedonia has been revised toinclude an incentive-motivational account (Wise, 1982), that ofa role of DA in associative learning, while strongly advocated,is not supported by as strong evidence (Beninger, 1983; Di Chiara,1995, 1999; Montague et al., 1996; Berridge and Robinson, 1998).

We have reported that D₁ receptor antagonists impair the acquisition of conditioned place preference as well as place aversioninduced by a variety of drugs (Acquas et al., 1989; Acquas andDi Chiara, 1994). On this basis we hypothesized that DA, actingon D₁ receptors, plays a role in appetitive as well as in aversivelearning (Acquas and Di Chiara, 1994; Di Chiara, 1995). Conditionedtaste aversion (CTA) (Garcia et al., 1955) is a form of Pavlovianlearning whose peculiar property is that of allowing a long interval(up to 6 hr) for efficient association of the gustatory CS withthe malaise-inducing US (Bûres et al., 1988; Yamamoto et al.,1994). These properties make CTA a unique paradigm for the studyof the mechanism of action of D₁ antagonists in associative learning.In the present study we have investigated the effect of systemicand intracerebral administration of the D₁ antagonists R(+)-7-chloro-8-hydroxy-3-methyl-1-phenyl-2,3,4,5-tetrahydro-1H-3-benzazepinehydrochloride (SCH 23390) and ( $-$ )-trans-6,7,7a,8,9,13b-hexahydro-3-chloro-2-hydroxy-N-methyl-5a-benzo-(D)-naphtho-(2,1b)azepine (SCH 39166) on the acquisition ofCTA.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals
Male Sprague Dawley rats (Charles River, Calco, Italy) weighing 250-275 gm were used. All animals were individually housedin Plexiglas cages placed in a temperature- and humidity-controlledroom with food and water ad libitum. Lights were on from 8:00A.M. to 8:00 P.M. All experiments were performed in the home cage.Except for the taste-reactivity experiments, in which rats hadwater ad libitum, in all CTA experiments involving drinking frombottles as a measure of taste aversion, rats had access to fluid(water, sucrose, or saccharin-glucose solution depending on thestage of the experiment, see "Experimental procedures") for 20min each day starting the day before the beginning of the experimentalprocedure and throughout its whole duration. The use of such afluid restriction protocol is common in CTA studies involvingdrinking from bottles and is justified by the need to ensure reproducibledrinking during a given time interval (Wagner et al., 1981; Mackeyet al., 1986; Blancquaert et al., 1987; Roldan and Bûres, 1994;Caulliez et al., 1996). Each rat was used only for one experiment,being killed within 24 hr from completion of the extinctionsessions.
All animal experimentation was conducted in accordance with the statement revised and approved by the Society for Neurosciencein January 1995 and with the guidelines for care and use of experimentalanimals of the European Commission (86/609; D.L.: 27.01.1992;number116).

Experimental procedures
CTA, multiple trials (experiment 1). This procedure was performed for 10 d and consisted of three phases. In the first, baselinetraining phase (days 1-3), the animals were trained to drink awater solution of saccharin (0.1%) plus glucose (3%) for 20 mineach day; the intake (milliliters per 20 min) of this solutionwas recorded for each rat. At the end of this phase the animalswere randomly assigned to the various experimental groups (saline+ saline; SCH 23390 6.0, 12.5, 25.0, and 50.0 µg/kg, s.c. + saline;saline + lithium; and SCH 23390 6.0, 12.5, 25.0, and 50.0 µg/kg,s.c. + lithium). In the second, conditioning phase (days 4-6),the saccharin-glucose solution was presented each day for 20 min,and its intake was recorded; the last drinking session beforeany exposure to lithium (i.e., trial on day 4) was taken as thetrial session. All subsequent drinking sessions were consideredas test sessions and were numbered as first (day 5), second (day6), etc. Five minutes after each drinking session, animals weregiven saline or SCH 23390 subcutaneously and, after a further30 min they received lithium chloride (40 mg/kg, i.p.) or saline.In the third, extinction phase (days 7-10), the saccharin-glucosesolution was presented for 20 min every day, and the intake wasrecorded. Data are expressed as test per trial ratio (millilitersper milliliter) of saccharin intake [ratio of the saccharin intakeon test i.e., 24 hr after each pairing with lithium (days 5, 6etc.) and that on the first day (day 4) of pairing with lithium(trial)].
CTA, single trials (experiments 2 and 3). In this procedure rats were trained to drink water for 20 min each day for 5 d (baselinetraining) and were conditioned by a single lithium-saccharin (plus3% glucose) association; thus, 5 min after the saccharin presentation(experiment 2) or 30 min before or at the start of saccharin presentation,5 or 45 min after the end of saccharin presentation (experiment3), rats received different doses of SCH 23390 (6.0, 12.5, 25.0,50.0 µg/kg, s.c.) or saline. One hour after saccharin, rats wereadministered with lithium chloride (125 mg/kg, i.p.) or with saline;the extinction phase lasted 3 d and consisted of three saccharin(plus 3% glucose) tests on the seventh, eighth, and ninth days.To evaluate the effect of D1 receptors in CTA learning using adifferent CS, the above procedure was repeated using a 15% sucrosesolution in tap water in place of the saccharin-glucose solution.In this case, doses of SCH 23390 (6.0 and 12.5 µg/kg, s.c.) wereused with the same protocol described for the saccharin-glucoseexperiments. In these experiments with sucrose as CS, the morespecific D₁ receptor antagonist SCH 39166, an analog of SCH 23390,or a D₂ receptor antagonist (raclopride), were also tested withthe same protocol used for SCH23390.
Taste reactivity (experiment 4). The taste reactivity paradigm has been used to evaluate the hedonic impact of tastes by quantifyingbehavioral reactions elicited by intraoral infusion of solutions(Grill and Norgren, 1978). Here we have used as taste a sweetchocolate solution that elicited intense and clear-cut hedonictaste reactions. An oral catheter was inserted 24 hr before theexperimental session at the level of the first molar; polyethylenetubing was passed along the skull and fixed to it with glasionomericcement (CX-Plus; Shofu, Tokyo, Japan). Each rat underwent a conditioningand an extinction session. On conditioning, a chocolate solutionwas pumped at a constant rate of 0.2 ml/min for a total amountof 1 ml. Five minutes after chocolate infusion, rats were administeredSCH 23390 (25 µg/kg, s.c.) or saline. Fifty-five minutes afterSCH 23390 rats received lithium chloride (125 mg/kg, i.p.). Duringchocolate infusion animals were videotaped, and three classesof affective taste reactivity patterns were scored: hedonic, aversive,and neutral. Hedonic reactions were: lateral tongue protrusions,rhythmic tongue protrusions, and paw licks; aversive reactionswere: gapes, chin rubs, face washing, forelimb flails, paw tread,locomotion, and head dog shakes; neutral reactions were: rhythmicmouth movements and passive drip of the solution (Berridge andRobinson, 1998). Each lateral and rhythmic tongue protrusion,gape, chin rub, forelimb flail, and paw tread was counted as anindividual event, and each event was assigned one point. Otherevents were assigned one point if the duration was between 1 and5 sec and 2 points if the duration was >5 sec. On extinction sessions,24 hr after conditioning, rats received an infusion of chocolate(1 ml) at a constant rate of 0.2 ml/min, and taste reactivitywasevaluated.
Local intracerebral drug infusion (experiment 5). Under anesthesia (chloral hydrate 400 mg/kg, i.p.) the animals were placedin the stereotaxic apparatus and bilaterally implanted with stainlesssteel guide cannulas in nucleus accumbens (NAc) shell [coordinates:anterior (A) +2.0, lateral (L) ±1.1, ventral (V) $-$ 7.8], in theNAc core (coordinates: A +1.5, L ±2.0, V $-$ 7.2), in the lateralhypothalamic area (LHA) (coordinates: A $-$ 2.6, L ±2, V $-$ 8.4), andin the bed nucleus stria terminalis (BNST) (coordinates: A $-$ 0.1,L ±1.1, V $-$ 7.6) according to Paxinos and Watson (1998). The guidecannulas were cemented 5 mm above the aimed site of injectionto prevent the injected solutions from leaking out of the cannulas.After a 3 d recovery, rats were trained to drink water, 20 mineach day, for 5 d (training). On the sixth day (conditioning),the rats were given access to a 0.1% saccharin plus 3% glucosesolution in tap water for 20 min in their home cage. The amount(in milliliters) of 0.1% saccharin (plus 3% glucose) solutionconsumed after a 20 min session was recorded, and 5 or 45 minthereafter each rat was bilaterally microinjected with SCH 39166or saline. For intracerebral drug infusion, rats were held byhand, and stainless steel cannulas, connected with a 10 µl Hamiltonsyringe by polyethylene tubing, were carefully inserted into theguide cannula. A volume of 1 µl was infused into the specificareas at a speed of 0.5 µl/min. After completion of the infusion,the cannula was left in place for 1 min; 55 or 15 min later ratsreceived an intraperitoneal injection of a single dose (80 or125 mg/kg) of a 0.15 M lithium chloride solution or of salineand were returned to their home cages. Twenty-four hours after,saccharin (plus 3% glucose) was presented for 20 min, and thevolume consumed was recorded. Twenty-four hours after the lasttest animals were anesthetized with chloral hydrate (400 mg/kg,i.p.) and perfused transcardially with saline followed by 10%formaldehyde to verify the site of injection. Brains were cutcoronally (40 µm) with a vibratome (Series 1000; Technical ProductsInternational, St. Louis, MO), and the cannula track was reconstructed.As described before, this procedure was also performed using a15% sucrose solution in tap water. Data are expressed as testper trial ratio of fluidconsumed.
Drugs and substances. Lithium chloride (Merck, Milan, Italy) was dissolved in water to make an isotonic solution (0.15 M)and injected intraperitoneally in a volume of 1.7 ml (40 mg/kg,i.p.), 3.4 ml (80 mg/kg, i.p.), or 5.3 ml (125 mg/kg, i.p.). SCH23390 (Research Biochemicals, Milan, Italy) was dissolved in salinesolution and injected subcutaneously in a volume of 0.1 ml/100gm of body weight. SCH 39166 (Schering Plough, Milan, Italy) wasdissolved in saline. Saccharin (Original Hermesetas, Bracco, Milan,Italy) and sucrose (Eridania, Genova, Italy) were dissolved intap water. Chocolate syrup (Yoo-hoo; Yoo-hoo Chocolate BeverageCorporation, Carlsbad, NJ) contained: sucrose 40%, corn syrup,water, cocoa, nonfat milk, salt, preservative E202, emulsifierE415, and artificial flavor and was infused intraorally as a 1:1solution in tap water. Raclopride (Research Biochemicals) wasdissolved in saline and injected subcutaneously in a volume of0.1 ml/100 gm of bodyweight.

Statistics
The significance of differences between groups was evaluated by one way, two-way or three-way ANOVA-MANOVA) and Tukey's posthoc test with significance set at p < 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effect of systemic SCH 23390 on multiple trials CTA (experiment 1)

Figure 1 shows the development of CTA to saccharin induced by three saccharin-lithium associations as well as the effect ofvarious doses of SCH 23390 (6, 12.5, 25, 50 µg/kg, s.c.) given5 min after saccharin in association with lithium or saline intraperitoneally(top panel). Three-way ANOVA revealed a significant effect oftest days (F_(2,76) = 14.5; p < 0.0001) and of lithium (F_(1,36)= 138.6; p < 0.0001) and a significant test × lithium interaction(F_(2,76) = 11.3; p < 0.0001). Post hoc analysis showed that saccharinintake was progressively reduced on test days after each saccharin-lithiumassociation trial. A progressive recovery underwent on the extinctionperiod that followed the last association with lithium (fourth,fifth, and sixth tests; data not shown). Post hoc analysis showeda maximal reduction of saccharin intake on the third test (Fig.1), whereas on the sixth test saccharin intake had almost completelyrecovered (data not shown).

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Figure 1. Effect of systemic SCH 23390 or saline on saccharin intake conditioned by multiple association with lithium chloride (top panel) or unconditioned (bottom panel). SCH 23390 was given subcutaneously 5 min after saccharin, whereas lithium chloride was given 30 min thereafter. Each bar represents the mean ± SEM of test per trial ratio of saccharin intake in 20 min. ⁺p < 0.05 or ⁺⁺p < 0.005 versus intraperitoneal saline; *p < 0.05 or **p < 0.005 versus lithium.

Three-way ANOVA also showed a significant interaction between SCH 23390 dose and lithium (F_(4,38) = 5.4; p < 0.001). SCH 23390did not exert significant effects on saccharin intake in the absenceof lithium (F_(4,17) = 1.4; p = 0.275) (Fig. 1, bottom panel).Post hoc analysis showed that SCH 23390 significantly reducedCTA at doses of 12.5, 25.0, and 50.0 µg/kg but not of 6 µg/kg,given subcutaneously, and that maximal impairment of CTA was obtainedat doses of 25 µg/kg of SCH 23390. Post hoc analysis also showedthat higher doses of SCH 23390 (50.0 µg/kg) were less effectivein impairing CTA than doses of 12.5 and 25 µg/kg (Fig. 1, toppanel).

Effect of systemic SCH 23390 and SCH 39166 on single-trial CTA (experiment 2)

The effect of SCH 23390 (6, 12.5, 25, 50 µg/kg, s.c.) was also tested on single-trial CTA with saccharin as CS on a singleassociation with lithium (125 mg/kg, i.p.), and the results areshown in Figure 2. Two-way ANOVA revealed a significant effectof lithium (F_(1,89) = 167.83; p < 0.0001) and of SCH 23390 (F_(4,89)= 32.91; p < 0.006) and a significant interaction between SCH23390 dose and lithium (F_(4,89) = 6.50; p < 0.0001). Post hoctests showed a significant effect of doses of 12.5, 25, and 50µg/kg of SCH 23390, but not of 6.0 µg/kg. A significant differencewas observed between the lowest dose (6.0 µg/kg) and the dosesof 12.5, 25.0, and 50.0 µg/kg of SCH 23390 given subcutaneously.The effect on saccharin intake of the association between SCH23390 and saccharin in the absence of lithium was also testedin a group of rats administered with SCH 23390 5 min after saccharinfollowed, 55 min later, by saline in place of lithium. Under theseconditions SCH 23390 did not exert significant effects on saccharinintake (F_(4,17) = 0.71; p = 0.59) (Fig. 2).

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Figure 2. Effect of SCH 23390 and SCH 39166 on the intake of saccharin or sucrose either unconditioned or conditioned by lithium chloride. Each bar represents the mean ± SEM of test per trial ratio of saccharin intake in 20 min. a, 6.0 µg/kg, s.c.; b, 12.5 µg/kg, s.c.; c, 25 µg/kg, s.c.; d, 50 µg/kg, s.c. ⁺⁺p < 0.005 versus intraperitoneal saline; *p < 0.05 or **p < 0.005 versus lithium.

To exclude a role of 5-HT₂ receptors in the action of SCH 23390, the analog SCH 39166 (25 and 50 µg/kg, s.c.), devoid of 5-HT₂actions, was tested, and the results are shown in Figure 2. Two-wayANOVA revealed a significant interaction between SCH 39166 doseand lithium (F_(2,55) = 4.197; p < 0.05). Post hoc tests showeda significant effect of the dose of 50 µg (Fig. 2). Pairing ofsaccharin with SCH 39166 in the absence of lithium did not exertany effect on saccharin intake 24 hr later (F_(2,11) = 0.38; p= 0.69) (Fig. 2).

The effect of SCH 23390 (6 and 12.5 µg/kg, s.c.) and SCH 39166 (12.5 and 25 µg/kg, s.c.) on CTA learning was also studiedusing sucrose as CS, and the results are shown in Figure 2. Two-wayANOVA revealed a significant effect of lithium (F_(1,33) = 88.5;p < 0.0001) and a significant interaction between SCH 23390 doseand lithium (F_(2,33) = 5.11; p < 0.01). Post hoc analysis revealedthat lithium (125 mg/kg, i.p.) induced a strong CTA also to sucrose.Two-way ANOVA also showed a significant interaction between SCH39166 dose and lithium (F_(2,33) = 7.08; p < 0.005). Post hoc analysisrevealed that SCH 39166 (12.5 and 25 µg/kg, s.c.) reduced CTAto sucrose (Fig. 2). Pairing of sucrose with the D₁ antagonistsin the absence of lithium did not exert any significant effecton sucrose intake 24 hr later (F_(4,17) = 0.91; p = 0.48; NS) (Fig.2).

To investigate the role of D₂ dopamine receptors on lithium-induced CTA, the dopamine D₂/D₃ receptor antagonist raclopridewas tested. Two-way ANOVA showed that raclopride (100 and 300µg/kg, s.c.) injected 5 min after sucrose intake failed to impairCTA induced by lithium chloride (F_(2,27 = 1.89; p = 0.17). Pairingof sucrose with raclopride in the absence of lithium did not changesucrose intake 24 hr later (F_(2,11) = 0.60; p = 0.56; NS; datanotshown).

Role of delay between CS presentation and systemic SCH 23390 (experiment 3)

To investigate the mechanism of the effect of SCH 23390 on CTA learning, the drug was administered 5 or 45 min after saccharinat a dose of 25 µg/kg. Figure 3 (top panel) reports the resultsobtained. Three-way ANOVA showed a significant effect of time(F_(1,72) = 6.27; p < 0.05) and a significant interaction betweenthe dose of SCH 23390 and lithium (F_(1,72) = 11.13; p < 0.005).Post hoc analysis revealed that SCH 23390 (25 µg/kg, s.c.) reducedlithium-induced CTA when given 5 min, but not 45 min, after saccharin.

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Figure 3. Effect of delay between systemic SCH 23390 and saccharin (top panel) or sucrose (bottom panel) on CTA learning. ⁺⁺p < 0.005 versus intraperitoneal saline; **p < 0.005 versus lithium.

In a second series of experiments using sucrose as CS, SCH 23390 (12.5 µg/kg, s.c.), was administered either 30 min before,at the same time, 5 min, or 45 min after the presentation of theCS. Figure 3 (bottom panel) reports the results obtained. Three-wayANOVA showed a significant interaction between SCH 23390 doseand lithium (F_(1,69) = 8.33; p < 0.005). Post hoc analysis showedthat SCH 23390 was able to impair CTA learning only when administered5 min after the presentation of the CS (Fig. 3, bottom panel).

Effect of SCH 23390 on lithium-induced taste reactivity to chocolate (experiment 4)

To evaluate if the impairment of lithium-induced CTA learning by SCH 23390 resulted in a reduction of the aversive propertiesof a taste after its association with lithium, the effect of SCH23390 (25 µg/kg, s.c.) was evaluated in a taste reactivity paradigmusing chocolate as CS. During conditioning sessions rats showedintense hedonic reactions to chocolate with virtually no aversivereactions (Fig. 4A,A'). As shown in Figure 4, B and B', previousassociation with lithium resulted in strong aversive reactionsto chocolate on tests 24 hr later and virtually no hedonic reactions.One-way ANOVA revealed a significant effect of group (F_(1,7) =5.74; p = 0.04). Post hoc analysis showed that SCH 23390, givenduring conditioning, resulted in a reduction of aversive reactionsto chocolate and in the recovery of some hedonic reactions thatwere particularly evident at the beginning of the intraoral infusion(Fig. 4B').

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Figure 4. Effect of SCH 23390 (25 µg/kg, s.c.) on the acquisition of aversive reactions to chocolate induced by a single association with lithium chloride (125 mg/kg, i.p.). Conditioning (trial): hedonic and aversive reactions to chocolate (A, individual; A', total). Extinction (test): aversive and hedonic reactions to chocolate after saline (open bars) or SCH 23390 (filled bars) plus lithium (B, individual; B', total). Each bar represents the means ± SEM of hedonic and aversive reactions. a, Rhythmic tongue protrusion; b, sniffing; c, paw licks; d, gapes; e, chin rubs; f, paw tread. *p < 0.05 versus subcutaneous saline.

Effect of intracerebral SCH 39166 on single-trial CTA (experiment 5)

To investigate the locus of action of systemic D₁ blockade on CTA learning, SCH 39166 was infused bilaterally in various brainareas, 5 min after exposure to the CS (saccharin or sucrose),followed, 55 min later, by saline or lithium chloride. Figure5 shows the results obtained with saccharin as CS. Two-way ANOVAshowed a significant effect of lithium in all groups (NAc shell,F_(1,38) = 108, p < 0.0001; NAc core, F_(1,19) = 336.22, p < 0.0001;LHA, F_(1,16) = 441.25, p < 0.0001). Two-way ANOVA also revealeda significant interaction between the dose of SCH 39166 infusedin the NAc shell and lithium (F_(3,38) = 5.60; p < 0.005). Posthoc analysis showed a significant effect of 25 and 50 ng, butnot 10 ng of SCH 39166. Two-way ANOVA further showed a significantinteraction between SCH 39166 dose and lithium also when SCH 39166(25 and 50 ng) was infused in the LHA (F_(2.16) = 6.71; p < 0.05).No significant effect was observed when SCH 39166 was infusedin the NAc core (F_(2,19) = 0.88; p = 0.42 ) (Fig. 5, top panel).SCH 39166, as shown in Figure 5 (bottom panel), did not exertany significant effect on saccharin intake when injected in theNAc shell, NAc core, LHA, and BNST followed by saline in placeof lithium (F_(8,23) = 1.19; p = 0.35; NS).

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Figure 5. Effect of infusion of SCH 39166 or saline in the NAc shell, NAc core, LHA, and BNST on saccharin intake conditioned by lithium chloride (80 or 125 mg/kg, i.p; top panel) or unconditioned (bottom panel). Differences between groups were evaluated by two-way ANOVA followed by Tukey's post hoc test. ⁺⁺p < 0.005 versus intraperitoneal saline; *p < 0.05 or **p < 0.005 versus lithium.

The effect of intracerebral SCH 39166 was also investigated on CTA induced by a dose of lithium (125 mg/kg, i.p.); this doseinduced a stronger CTA than lithium 80 mg/kg, given intraperitoneally.Also in this case, two-way ANOVA showed a significant interactionbetween SCH 39166 dose and lithium (F_(2,24) = 23.43; p < 0.00001).As shown in Figure 5 (top panel) SCH 39166 (25 and 50 ng) infusedin the NAc shell reduced CTA induced by 125 mg/kg lithium givenintraperitoneally. It is notable that at the dose of 50 ng theinhibition of lithium-induced CTA by SCH 39166 was close to beingcomplete. No effect on CTA learning was observed when SCH 39166was injected in theBNST.

These studies were duplicated using a 15% sucrose instead of a 0.1% saccharin solution as the CS. Also with sucrose as CS,SCH 39166 did not exert any significant effect on sucrose intakewhen injected alone into brain areas (F_(5,16) = 0.63; p = 0.68;NS) (Fig. 6, bottom panel). Two-way ANOVA revealed a significanteffect of lithium in all groups (NAc shell, F_(1,36) = 273.52,p < 0.00001; NAc core, F_(1,14) = 147.69, p < 0.00001; LHA, F_(1,14)= 94.32, p < 0.00001), and a significant interaction between SCH39166 dose and lithium (F_(2,36) = 4.41; p < 0.05). As shown inFigure 6 (top panel) SCH 39166 (25, 50, and 100 ng/µl) impairedCTA acquisition when infused in the NAc shell but not in the NAccore 5 min after sucrose. Post hoc analysis showed a significanteffect of 50 and 100 ng, but not of 25 ng of SCH 39166. Two-wayANOVA showed a significant interaction between SCH 39166 doseand lithium also when SCH 39166 was infused in the LHA (F_(1,14)= 7.07; p < 0.05). SCH 39166 (50 ng) did not affect CTA learningwhen infused into the NAc shell 45 min after the presentationof CS (F_(1,46) = 0.227; p = 0.63; NS). Figure 7 shows the injectionsites.

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Figure 6. Effect of infusion of SCH 39166 or saline in the NAc shell, NAc core, LHA, and BNST on sucrose intake conditioned by lithium chloride (80 or 125 mg/kg, i.p.; top panel) or unconditioned (bottom panel). Differences between groups were evaluated by two-way ANOVA followed by Tukey's post hoc test. ⁺⁺p < 0.005 versus saline; *p < 0.05 or **p < 0.005 versus lithium.

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Figure 7. Brain sections showing intracerebral injection sites. Section levels are according to Paxinos and Watson (1999). Filled circles, Correct injection sites; filled squares, incorrect injection sites (cc, corpus callosum; Cpu, caudate putamen; NAc Sh, nucleus accumbens shell; NAc Co, nucleus accumbens core; LHA, lateral hypothalamic area).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The main findings of the present study are threefold: first, systemic administration of low doses of DA D₁ receptor antagonistsimpairs CTA learning; second, this effect takes place at a criticalstage in the associative process between the gustatory CS andthe US corresponding to the formation and consolidation of a short-termmemory trace of the gustatory CS; third, this action can be reproducedby placing low, nanogram amounts of SCH 39166 in the NAc shelland in the LHA, but not in the NAc core or in theBNST.

Time-dependent impairment of CTA learning by D₁ receptor antagonists

The present CTA study was initially intended to duplicate with a different paradigm our previous observation that D₁ receptorblockade impairs acquisition of place conditioning to rewardingand aversive drug stimuli (Acquas et al., 1989; Acquas and DiChiara, 1994). For this reason we selected a CTA procedure involvingthree CS-US (saccharin-lithium) associations as in the place conditioningparadigm; also the dose of lithium (40 mg/kg) was the same previouslyused in our place conditioning studies (Acquas and Di Chiara,1994). With this schedule, which resulted in a progressive developmentof CTA, SCH 23390 impaired CTA at very low doses (12-50 µg/kg,s.c.) even lower than those found to impair acquisition of placeaversion to lithium (Acquas and Di Chiara, 1994).

In a second series of experiments we used a CTA procedure involving a single association of saccharin or sucrose with a highdose of lithium in rats trained to drink tap water. Also underthese conditions, low doses of SCH 23390 (12.5-50 µg/kg, s.c.)administered systemically impaired the acquisition of CTA. Themore selective D₁ antagonist SCH 39166 (Chipkin et al., 1988)exerted a similar effect at doses superimposable to those of SCH23390, in agreement with the similar in vivo potency of the twodrugs as antagonists of D₁ receptors. SCH 23390 not only reducedlithium-conditioned avoidance of sucrose or saccharin but alsoreduced the conditioned aversive properties of palatable tastestimuli in a taste reactivity paradigm. This observation indicatesthat SCH 23390 impaired the mechanism by which negative hedonicvalue is attributed to the taste, thus reducing the conditionalaversive properties of the taste stimulus, rather than impairingitsavoidance.

The present conclusions contrast with those of Berridge and Robinson (1998) who, on the basis of 6-hydroxy DA lesion studies,excluded that mesolimbic DA is involved in the acquisition ofCTA as estimated by taste reactivity. At least two explanationscan be offered for this discrepancy: first, that the lesions didnot completely destroy the critical DA substrate in the NAc shell;second, that adaptive mechanisms taking place in non-DA neuronsduring the 8-17 d of postlesion recovery did compensate for anylesion-inducedimpairment.

SCH 23390 impaired CTA when given 5 min but not 45 min after the presentation of the CS (saccharin or sucrose) (i.e., 55 or15 min, respectively, before lithium). Therefore, SCH 23390 didnot impair CTA when the time course of its effect was superimposedto that of lithium. These observations exclude that the effectof SCH 23390 on CTA is related to an interference with the aversiveproperties of the US (lithium). On the other hand, SCH 23390 didnot impair CTA when given 30 min before or at the start of thepresentation of the taste CS, excluding that the effect of SCH23390 given 5 min after drinking was attributable to an interferencewith some stimulus properties of the taste CS (aftertaste?). Finally,a nonspecific state-dependent mechanism (Overton, 1964) is excludednot only by the fact that both on trial and on test the CS waspresented in the absence of the D₁ antagonist but also by thefailure of a D₂ antagonist to reproduce the effect of a D₁ antagonist.The observation that the D₁ antagonist impaired CTA given aftertaste trials but was ineffective if administered concurrentlywith the taste CS proves a fortiori that its effect is unrelatedto a state-dependentmechanism.

According to Bûres et al. (1991), CTA is acquired through various phases: (1) initial processing of the taste stimulus; (2)formation and storage of a gustatory short-term memory trace;(3) association of the gustatory trace with the primary aversive(lithium) state (US); and (4) transfer of the CS-US associationinto a long-term memorystore.

The observation that SCH 23390 impaired CTA when given 5 min but not 45 min after the CS indicates that SCH 23390 acts onstage 2, i.e., on the formation and storage of the gustatory short-termmemory trace. Blockade of DA D₁ receptors might accelerate thedecay of the gustatory trace or, alternatively, impair its transferto an area where association with the aversive state can takeplace. Therefore, endogenous DA acting on D₁ receptors seems criticalfor the formation and consolidation of a gustatory short-termmemory trace or for its transfer and storage into an area wherecan be associated with a visceral aversivestate.

Impairment of CTA learning by D₁ antagonist infusion in the nucleus accumbens shell

Local intracerebral infusion of SCH 39166 shows that the NAc shell is critical for the effect of D₁ blockade on CTA learning.This effect was site-specific because placements dorsal or lateralto the NAc shell in an area that includes the NAc core (Heimeret al., 1991) or in the BNST did not impair CTA learning. Theeffect of local D₁ receptor blockade in the NAc shell showed thesame temporal properties of the systemic effect because it tookplace when SCH 39166 was infused 5 min but not 45 min after theCS (see Results). In agreement with Caulliez et al. (1996), SCH39166 impaired CTA when microinfused into theLHA.

A role of NAc shell in CTA learning is consistent with the fact that this area receives gustatory input from the agranularinsular cortex and the basolateral amygdala and relays it to theparabrachial nucleus-nucleus tracti solitarii area (Heimer etal., 1991). The observation that the LHA shares with NAc shella role in CTA acquisition is consistent with the existence ofreciprocal connections between these areas (Heimer et al., 1991;Kirouac and Ganguly, 1995). Evidence for a facilitatory effectof D₁ receptor stimulation in the caudate on memory consolidationhas been provided (Packard and White, 1991). In these studies,however, drugs were administered after the stimulus-reinforcerassociation had taken place, thus implicating consolidation ofthe CS-US association into long-term memory rather than consolidationof the short-term memory trace of the CS before its associationwith the US, as in the presentstudy.

Nucleus accumbens shell dopamine and gustatory learning

The present observations might provide a role for the response properties of DA transmission in the NAc shell to unfamiliartastes. According to Mark et al. (1991) intraoral saccharin increasesDA release in the NAc before but decreases it after associationwith lithium. On the other hand, feeding of a novel palatablefood stimulates DA release in the NAc shell, but this responseundergoes one-trial habituation (Bassareo and Di Chiara, 1997)and is prevented by presentation of a predictive olfactory stimulus(Bassareo and Di Chiara, 1999). These properties are consistentwith a role of phasic DA release in the NAc shell in associativegustatory learning. Thus, DA released on D₁ receptors of the NAcshell by novel palatable tastes might act to modulate the efferentneurons of the shell in the processing of the gustatory stimulusafter its perception. Therefore, DA release in the NAc shell mightbe the substrate of a consolidation mechanism by which a gustatoryshort-term memory trace is formed to remain available for enoughlong time to be associated with postingestivechanges.

The mechanism of the influence of endogenous DA in CTA learning can account not only for the role of DA in aversive learning,as in the present study, but also in appetitive learning, as inthe case of place preference (Acquas and Di Chiara, 1994; Di Chiara,1995). If, as suggested by the present study, DA affects associativelearning by acting before the presentation of the US it might,depending on the valence of the US, exert its enabling actionon either appetitive or aversive learning. Thus, the functionof phasic DA release in the NAc rather than that of mediatingthe hedonic properties of rewards (Wise, 1982), might be thatof facilitating the association between stimuli and their biologicaloutcomes independently from the motivational valence of theoutcome.

The observations of the present study might impact on issues beyond the strict boundaries of taste aversion learning. Thus,most drugs of abuse have been shown to increase, in a nonadaptive(nonhabituating) manner, DA transmission in the NAc shell (DiChiara, 1998 and 1999). One might speculate that this action,by facilitating consolidation of drug-associated stimuli intoshort-term memory, promotes the acquisition of conditional incentiveproperties by these stimuli that, after chronic drug exposure,come to control behavior in that excessive, compulsive mannerthat is typical of addiction (Di Chiara, 1998, 1999).

  FOOTNOTES

Received April 16, 2001; revised June 1, 2001; accepted June 11, 2001.

This work was performed with funds from Ministero dell'Università della Ricerca Scientifica e Tecnologica (40 and 60%) andfrom Consiglio Nazionale delle Ricerche (Center for Neuropharmacology).We thank Dr. Elio Acquas for help with thestatistics.
Correspondence should be addressed to Prof. Gaetano Di Chiara, Dipartimento di Tossicologia, Viale A. Diaz 182, 09126 Cagliari,Italy. E-mail: diptoss{at}tin.it.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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