The Circuitry Mediating Cocaine-Induced Reinstatement of Drug-Seeking Behavior

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The Journal of Neuroscience, November 1, 2001, 21(21):8655-8663

The Circuitry Mediating Cocaine-Induced Reinstatement of Drug-Seeking Behavior
Krista McFarland and Peter W. Kalivas
Department of Physiology and Neuroscience, Medical University of South Carolina, Charleston, South Carolina 29425

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The role of limbic-striato-pallidal circuitry in cocaine-induced reinstatement was evaluated. The transient inhibition ofbrain nuclei associated with motor systems [including the ventraltegmental area (VTA), dorsal prefrontal cortex (dPFC), core ofthe nucleus accumbens (NAcore), and ventral pallidum (VP)] preventedcocaine-induced reinstatement. However, only the VP proved tobe necessary for food reinstatement, suggesting that the identifiedcircuit is specific to drug-related reinstatement. Supportingthe possibility that the VTA-dPFC-NAcore-VP is a series circuitmediating reinstatement, simultaneous unilateral microinjectionof GABA agonists into the dPFC in one hemisphere and into theVP in the contralateral hemisphere abolished cocaine reinstatement.Although dopamine projections from the VTA innervate all threeforebrain nuclei, the blockade of dopamine receptors only in thedPFC antagonized cocaine-induced reinstatement. Furthermore, DAadministration into the dPFC was sufficient to elicit a reinstatementin drug-related responding. These data demonstrate that dopaminerelease in the dPFC initiates a dPFC-NAcore-VP series circuitthat mediates cocaine-induced drug-seekingbehavior.

Key words: cocaine; dopamine; glutamate; self-administration; craving; reinstatement

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

One of the most insidious problems associated with chronic drug use is the tendency for users to relapse even after extendedperiods of drugs abstinence. Many types of stimuli can increasereports of craving and subsequent relapse in drug addicts, includingreexposure to the drug itself, stress, and cocaine-associatedcues (Jaffe et al., 1989; Childress et al., 1999), and animalreinstatement models of drug-seeking behavior have been establishedto evaluate the neurobiology of reinstatement and relapse (Shahamand Stewart, 1995; Erb et al., 1996; McFarland and Ettenberg,1997; Meil and See, 1997). Although the rewarding effect of acutepsychostimulant administration has been successfully linked tolimbic circuitry, including the mesolimbic dopamine projectionfrom the ventral tegmental area (VTA) to the nucleus accumbens(Koob et al., 1993; Robbins and Everitt, 1996), the circuitrymediating drug seeking in animal models of reinstatement has notbeen as clearlydelineated.

Along with the VTA and nucleus accumbens, the amygdala, prefrontal cortex (PFC), and ventral pallidum (VP) have been examinedfor involvement in drug reward (Pierce and Kalivas, 1997; Wolf,1998; Childress et al., 1999). Topographic analysis of the interconnectionsamong these nuclei has established two subcircuits: one subcircuitcomprising the ventral PFC (vPFC), shell of the accumbens (NAshell),medial VP, amygdala, and the VTA, that is more intimately connectedwith limbic structures, and another subcircuit comprised of thedorsal PFC (dPFC), core of the accumbens (NAcore), dorsolateralVP, and substantia nigra, that is more extensively interconnectedwith motor structures (Zahm and Brog, 1992; Kalivas et al., 1993;Groenewegen et al., 1996). Traditionally, they have been termedthe "limbic" and "motor" subcircuits in deference to this anatomicalspecificity. It is generally assumed that limbic circuitry underliesbehavioral changes associated with chronic drug use (e.g., cravingand relapse), an assumption supported by studies showing thatinactivation of the amygdala prevents cue-induced reinstatement(Meil and See, 1997; Grimm and See, 2000), as well as numerousdata indicating enduring cellular adaptations in limbic nucleiafter repeated administration of drugs of abuse (Nestler and Aghajanian,1997; White and Kalivas, 1998). However, craving and relapse areoften described as compulsive or automatic (Grant et al., 1996;Childress et al., 1999), raising the possibility that these behaviorsmay rely more on activation of motor than limbiccircuitry.

The present study evaluated the nuclei outlined above and tested whether the motor or limbic subregion of each nucleus wasmore critical for drug-induced reinstatement. In an attempt toparallel human addicts who relapse after reexposure to a previouslyself-administered drug, rats were trained to lever press for cocainereinforcement and then underwent a period of behavioral extinctionduring which no cocaine reinforcement was available (de Wit andStewart, 1981). To identify nuclei that are necessary for drug-seekingbehavior, the neuronal activity in individual nuclei was transientlyinhibited with an intracranial microinjection of a combinationof GABA_A and GABA_B agonist before reinstatement testing. GABA-mediatedinhibition was chosen over other inactivation techniques becauseit is both reversible and leaves fibers of passageunaffected.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animal housing and surgery. All experiments were conducted in accordance with the National Institutes of Health Guidelinesfor the Care and Use of Laboratory Animals. The subjects were164 male Sprague Dawley rats (Charles Rivers Laboratories. Wilmington,MA) weighing 250-275 gm on arrival, and they were individuallyhoused in an Association for the Assessment and Accreditationof Laboratory Animal Care-approved facility maintained on a 12hr reversed light/dark cycle (lights on 7:00 P.M.). Subjects wereweighed and handled daily for the duration of the experiment andwere given ad libitum access to food and water until 7 d aftersurgery, when they received a 20 gm daily ration of rat chow forthe remainder of the experiment. This feeding regimen aided inthe acquisition of the operant lever-press response but allowedrats to gain weight throughout the course of theexperiment.

After 1 week of acclimation, animals were anesthetized with ketamine HCl (87.5 mg/kg Ketaset; Fort Dodge Animal Health, FortDodge, IA) and xylazine (5 mg/kg Rompum; Bayer, Shawnee Mission,KS) and implanted with indwelling jugular catheters and bilateralguide cannulas (26 gauge; Small Parts Inc., Roanoke, VA) aimedat one of 10 brain regions according to the atlas of Paxinos andWatson (1998) (all coordinates given relative to bregma): dorsaland ventral PFC, +3.0 mm anteroposterior (AP), ±0.7 mm mediolateral(ML), and $-$ 2.0 mm dorsoventral (DV); NAcore, +1.2 mm AP, ±1.6mm ML, and $-$ 6.5 mm DV; NAshell, +1.5 mm AP, ±0.6 mm ML, and $-$ 6.5DV; VP, $-$ 0.25 mm AP, ±2.4 mm ML, and $-$ 7.9 mm DV; central nucleusof the amygdala (CN), $-$ 2.1 mm AP, ±4.0 mm ML, and $-$ 8.0 mm DV;basolateral amygdala (BLA), $-$ 2.5 mm AP, ±4.7 mm ML, and $-$ 8.5 mmDV; mediodorsal thalamus (MD), $-$ 2.8 mm AP, ±0.7 mm ML, and $-$ 5.5mm DV; VTA, $-$ 5.2 mm AP, ±0.85 mm ML, and 8.15 mm DV with the cannulasangled 6° from the midline; and substantia nigra (SN), $-$ 5.2 mmAP; ±2.1 mm ML, and $-$ 8.0 mm DV). Guide cannulas (cut to 14 mm)were lowered into place and attached to the skull via small stainlesssteel screws and dental acrylic. Obdurators (33 gauge; Small PartsInc.), cut to extend 0.5 mm beyond the tip of each cannula, wereinserted to prevent obstruction bydebris.

For catheter implantation, a guide cannula (C313G; Plastics One Inc., Wallingford, CT), attached to SILASTIC tubing (0.025inner diameter, 0.047 outer diameter; Bio-Sil; Bio-Rad, Hercules,CA) and Marlex mesh via dental cement, was inserted subcutaneouslybetween the shoulder blades and exited the skin via a dermal biopsyhole (3 mm). The other end of the tubing was threaded under theskin, inserted 3 cm into the right jugular vein, and then suturedsecurely to the underlying muscletissue.

Self-administration and extinction procedures. Seven days after surgery, subjects began behavioral training. All self-administrationexperiments were conducted in standard operant chambers (ENV-008;Med Associates Inc., E. Fairfield, VT) fitted with two retractablelevers. Initially, all subjects were trained in one 15 hr sessionto lever press for food on an fixed ratio 1 (FR-1) schedule forreinforcement consisting of one food pellet (45 mg; Noyes, Lancaster,NH). The following day, subjects began lever pressing for cocainereinforcement. Each press of the correct lever resulted in aninfusion of cocaine (0.25 mg/kg over 4 sec), followed by a 20sec time out, in which correct lever presses were counted butresulted in no scheduled consequences. Responses on the incorrectlever never resulted in cocaine delivery and consequently becamevery infrequent over the course of training. Each training triallasted for 2 hr or until the subject had self-administered 200infusions of cocaine. An arbitrary acquisition criterion requiredthat subjects' active lever presses vary by 10% or less over thecourse of 3 consecutive maintenance days before they were movedon to the extinction phase of the experiment. During maintenance,subjects administered an average of 20.25 mg/kg cocaine acrossthe 2 hr session. This average did not differ significantly betweengroups of animals implanted with guide cannulas into differentbrain regions. Once subjects met the maintenance criterion, extinctionprocedures were instituted. During extinction, subjects experienced2 hr daily training sessions; however, saline was substitutedfor cocaine after presses of the active lever. Thus, active leverpresses now resulted in no reinforcer delivery. Subjects remainedin extinction until responding on the active lever fell to <10%of the level duringmaintenance.

Reinstatement testing and microinjection of drug. After extinction, subjects were tested for their propensity to reinstateresponding on the active lever after a systemic injection of cocaine(10 mg/kg, i.p.). Before reinstatement testing, subjects receivedan intracranial infusion of either 0.9% saline vehicle or a combinationof the GABA_A receptor agonist muscimol (mus) and the GABA_B agonistbaclofen (bac). Before injection, obdurators were removed fromthe guide cannulas and 33 gauge microinjection cannula were insertedbilaterally to extend 1 mm below the end of the guide (with theexception of the vPFC, in which injectors were inserted to 3 mmbelow the end of the guide). All infusions were made in a volumeof 0.3 µl over 60 sec. After infusion, 1 min was allowed for diffusion,the microinjectors were removed, obdurators were replaced, andsubjects were given an injection of cocaine before being placedin the chambers for 2 hr. This injection volume and procedurehas been shown previously to functionally distinguish betweenthe NAshell and NAcore and between the VTA and SN (Johnson etal., 1996). All subjects were tested twice with successive testdays separated by additional extinction trials, in which subjectswere required to again meet the extinction criterion before thesecond test trial. During reinstatement testing, active leverpresses resulted only in a delivery of intravenous saline andnotcocaine.

For bac-mus infusions, the drugs were dissolved in saline at a screening dose of 0.3 nmol of baclofen and 0.03 nmol of muscimol(per 0.3 µl injection volume). For any brain area in which therewas an effect of these high doses, a dose-response curve was establishedat half log unit increments of each drug. Each subject was testedonly twice (i.e., saline plus a single dose of bac-mus or twodifferent doses of bac-mus). For the ipsilateral versus contralateraltest of the integrity of the circuit, all testing was conductedwith 0.3 nmol of bac and 0.03 nmol of mus. The combination ofGABA agonists was chosen because projection cells in every nucleusexamined are inhibited by one or both of the GABA_A or GABA_B agonists(Kalivas et al., 1993; Mogenson et al., 1993). Fluphenazine wasalso dissolved in saline in a concentration of 10 nmol per injection(0.3 µl/side). Dopamine was dissolved in saline and administeredin a dose of 30 µg.

Food reinstatement. Food reinstatement experiments were conducted after a procedure that paralleled cocaine reinstatementas closely as possible. After 1 week of handling, subjects werestereotaxically implanted with guide cannulas into the dPFC, NAcore,or VP using the procedure and coordinates described previously.One week after surgery, animals were food restricted to 90% oftheir free-feeding body weights and were maintained at this weightfor the duration of the experiment. Two days after the institutionof food restriction procedures, subjects began behavioral training.They were trained to lever press on an FR-1 schedule for reinforcementconsisting of a single (45 mg) food pellet. On subsequent days,the schedule was increased to an FR-3 and then an FR-5. An intermittentschedule of reinforcement was instituted in animals respondingfor food reinforcement to help ensure robust reinstatement responding.On each schedule, subjects were required to display stable operantbehavior (<10% variation across 3 d), before being moved to thenext schedule. Once each rat displayed stable responding on theFR-5 schedule of reinforcement, extinction procedures were institutedso that lever presses no longer resulted in delivery of food reinforcement.When average responding across three consecutive sessions was<10% of FR-5 reinforced responding, subjects were tested for theability of noncontingent food delivery to reinstate lever-pressresponding after either saline (0.3 µl) or bac-mus infusion (0.3and 0.03 nmol, respectively, in 0.3 µl). One food pellet was placedinto the hopper before beginning the test session, and an additionalfive pellets were dropped at 2 min intervals during the first10 min of the reinstatementsession.

Locomotor testing. Motor activity was monitored in clear Plexiglas boxes (22 × 43 × 33 cm). Each box was monitored by a seriesof 16 photobeams (eight on each horizontal axis) measuring horizontalactivity and eight photobeams measuring vertical activity. Beambreaks were detected, counted, and recorded by a personal computerrunning Digiscan software (AccuScan Instruments Inc., Columbus,OH). Each test period consisted of a 1 hr acclimation period beforetesting. After habituation, each subject was removed from itscage, given a microinfusion (using the procedure described above),and then returned to the cage for 2 hr of activitymonitoring.

Histology and statistics. Rats were overdosed with pentobarbital (120 mg/kg, i.p.) and then perfused transcardially with 0.9%physiological saline followed by 10% formalin. Brains were removedand placed in a 10% formalin solution for at least 24 hr beforeslicing. The brains were blocked and sliced in coronal sections(50 µm thick) through the site of guide cannula implantation.Sections were mounted on gel-coated slides and then stained withcresyl violet to allow for verification of cannula placement byan individual unaware each subject's behavioral responses. Thedata were statistically evaluated using a one-way or two-way ANOVA,and post hoc comparisons between individual treatments were madeusing a Tukey's test. Because subjects were tested only twiceand did not receive all treatment doses, all analyses were doneassuming independent groups, because repeated-measures analyseswere not possible. When time course data for locomotor activitywere evaluated, a two-way ANOVA with repeated measures over timewasused.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neural circuitry mediating cocaine-induced reinstatement

Figure 1 shows the results from nuclei in which infusion of GABA agonists (a combination of the GABA_B agonist baclofen andthe GABA_A agonist muscimol, bac-mus) blocked cocaine-induced reinstatement.An ANOVA conducted on each panel in Figure 1 revealed a significantdose-dependent effect of baclofen-muscimol inactivation of thedPFC, NAcore, VTA, and VP. After microinjection of saline or avery low dose of bac-mus, subjects displayed robust lever-pressresponding after cocaine challenge. However, pretreatment withhigher doses of bac-mus reduced reinstatement responding to extinctionlevels (minimum effective dose of 0.03 nmol/side bac-0.003 nmol/sidemus for each nucleus, except the NAcore in which the dose was0.1 nmol/side bac-0.01 nmol/side mus).

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Figure 1. GABA receptor activation prevented cocaine-induced reinstatement. Pretreatment with combinations of the GABA_B and GABA_A receptor agonists bac-mus into the dPFC (A), ) NAcore (B), VTA (C), and VP (D) blocked the reinstatement elicited by cocaine administration (n = 6-8 for each dose in each nucleus). Subjects pretreated with a screening dose (0.3 and 0.03 nmol/side, respectively) into any of these areas showed no change in active lever presses compared with extinction (EXT) responding, suggesting that neural activation of these areas is critical for the ability of cocaine to elicit reinstatement. Note that, when pretreated with saline vehicle (SAL), all subjects exhibited a robust return to drug seeking. Data depicted as mean + SEM active lever presses. Dose combinations of baclofen and muscimol were 0.3 and 0.03, 0.1 and 0.01, 0.03 and 0.003, and 0.01 and 0.001 nmol/side, respectively. x-Axis labels are designated using the baclofen dose. *p < 0.001, increase in active lever presses compared with EXT. #p < 0.05, responding that was greater than EXT and less than SAL.

Figure 2 reveals that, at the maximum screening dose of bac-mus (0.3 and 0.03 nmol/side, respectively), none of the otherregions tested showed any involvement in cocaine-induced reinstatement,including the vPFC, NAshell, SN, CN, BLA, or MD. There was a maineffect of condition, indicating that there was a significant reinstatementin animals pretreated with a microinjection of saline vehicle.However, Tukey's honestly significant difference post hoc analysesshowed that there was no difference between bac-mus pretreatmentand vehicle pretreatment.

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Figure 2. Inactivation of some brain regions tested was ineffective in altering cocaine-induced reinstatement. Subjects pretreated with a high screening dose of bac-mus (0.3 and 0.03 nmol/side, respectively) into the vPFC, NAshell, SN, CN, BLA, or MD (n = 6-8) displayed robust lever-press responding on reinstatement testing equivalent to that seen after saline (SAL) pretreatment. *p < 0.05, comparing cocaine-induced active lever pressing with extinction (EXT) responding.

These data suggest that the VTA, dPFC, NAcore, and VP form a circuit that is critical for cocaine-induced reinstatement ofdrug-seeking behavior. To test the specificity of the circuitin the control of drug-seeking behavior, each of the targets ofVTA dopamine projections implicated above (i.e., the dPFC, NAcore,and VP) were tested for their involvement in the food-inducedreinstatement of food-seeking behavior. Figure 3 shows that bac-musinhibition of the VP, but not the dPFC or NAcore, blocked theability of food to elicit extinguished food-seeking behavior,suggesting that the identified circuit is specific to the drug-relatedbehavior under examination.

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Figure 3. Reinstatement of food-seeking behavior is blocked by inhibition of the VP but not the dPFC or NAcore. Pretreatment with the screening dose of bac-mus (0.3 and 0.03 nmol/side, respectively) into the VP inhibited lever-press responding elicited by noncontingent food presentation, whereas infusion of bac-mus into the NAcore or PFC (0.3 and 0.03 nmol/side, respectively) resulted in response rates indistinguishable from saline (SAL) pretreatment (i.e., a robust reinstatement). *p < 0.001, comparing food reinstatement responding with extinction (EXT) responding.

An implication of these findings is that the VTA-dPFC-NAcore-VP connections form a functional series circuit that is criticalfor cocaine-induced reinstatement of drug-seeking behavior inrats (i.e., information flows sequentially from one nucleus tothe next and not in parallel pathways) (Fig. 4A). To directlytest this possibility, rats were implanted with guide cannulasinto both the dPFC and the VP. Before reinstatement testing, eachanimal received a bac-mus infusion (0.3 and 0.03 nmol, respectively)into the dPFC and VP on either ipsilateral or contralateral sidesof the brain. Figure 4B reveals that animals having the VP andthe dPFC in the same hemisphere inactivated showed normal reinstatementafter cocaine challenge. However, if the inactivated VP and dPFCwere on alternate sides, animals showed no reliable cocaine-inducedreinstatement. This experiment indicates that a flow of informationin series between the dPFC and VP is required, presumably viaa synapse in the NAcore, because the primary conduit whereby thedPFC gains access to the VP is via a synapse in the NAcore (Sesacket al., 1989; Zahm and Brog, 1992). The VP and dPFC were chosenas targets for the disconnection experiment because there areno direct connections between them. Thus, a positive disconnectionimplicates a serial circuit flowing from the dPFC through theNAcore to the VP in the production of cocaine-induced reinstatement.Selection of any other pair of nuclei (e.g., the dPFC and theNAcore) would implicate only two of these brain regions in thisserial circuitry.

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Figure 4. A series, rather than parallel, circuit is involved in cocaine-primed reinstatement. A, Circuits can be organized in either parallel or series. Parallel circuits would suggest that information could flow simultaneously along multiple pathways, whereas a series circuit would suggest that information flows sequentially from one nucleus to the next. B, Subjects receiving bac-mus (0.3 and 0.03 nmol/side, respectively) infusion into the dPFC and VP on the same side (ipsilateral; n = 5) of the brain displayed vigorous active lever-press responding after cocaine challenge. However, when subjects received bac-mus treatment into one dPFC and the contralateral VP (contralateral; n = 6), responding on the active lever did not differ from extinction (EXT) responding, suggesting these brain regions are in series circuit essential for the ability of cocaine to elicit a reinstatement of drug-seeking behavior. *p < 0.001, comparing ipsilateral with extinction (EXT) responding.

Role of dopamine in response initiation

Acute doses of cocaine increase extracellular levels of dopamine, which presumably serves as the intereoceptive cue to initiatereinstatement because systemically administered dopamine antagonists(De Vries et al., 1999) or GABAergic inhibition of dopamine cellsin the VTA (Fig. 1) inhibit cocaine-induced reinstatement. Dopaminergicprojections from the VTA innervate all three forebrain regionsfound sensitive to GABA agonist-induced inhibition of cocainereinstatement (Kalivas et al., 1993). Figure 5A shows that microinjectionof the D1/D2 antagonist fluphenazine (10 nmol/side) into the dPFC,but not into the NAcore or VP, blocked cocaine-induced reinstatement.

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Figure 5. Role of dopamine in the dPFC in cocaine reinstatement. A, Fluphenazine (FLU) infusion into the dPFC, but not the NAcore or VP (n = 6 in each condition), before reinstatement testing abolished the increase in active lever pressing observed after pretreatment with saline vehicle (SAL). B, After bac-mus (0.3 and 0.03 nmol/side, respectively) activation of the VTA, subjects received either saline (0 nmol; n = 5) or dopamine (30 nmol/side; n = 7) infusions into the dPFC before a cocaine (COC) reinstatement challenge. When no dopamine was infused into the dPFC, subjects exhibited the expected blockade of cocaine-induced reinstatement, similar to that seen after inactivation of the VTA in Figure 1. However, dopamine replacement into the dPFC resulted in a highly significant reinstatement of self-administration behavior. Similarly, dopamine alone into the dPFC was sufficient to induce robust responding. *p < 0.001, comparing extinction (EXT) responding with other treatments.

These data implicate the dopaminergic projection from the VTA to the dPFC as the initial step in producing cocaine-inducedreinstatement. Given that the increase in extracellular dopamineafter cocaine is predominantly action potential dependent (Seidenet al., 1993), it is possible that cocaine is not inducing reinstatementby activating dopamine cells in the VTA but rather is relyingon ongoing activity in these cells to increase dopamine releasein the dPFC. To examine this possibility, animals were preparedwith bilateral guide cannulas aimed at both the VTA and the dPFC.Before reinstatement testing, subjects received bac-mus infusions(0.3 and 0.03 nmol/side, respectively) into the VTA, followedby either saline or dopamine (30 µg/side) into the dPFC. Whensaline was infused into the dPFC, cocaine failed to produce reinstatementwhen the VTA was inactivated by GABA agonists. However, when dopaminetone was returned to the dPFC, cocaine once again elicited a robustreinstatement (Fig. 5B). Furthermore, dopamine (30 µg/side) infusedinto the dPFC in the absence of systemic cocaine was sufficientto elicit a reinstatement of lever-pressing responding. Together,these findings support a permissive role for the VTA rather thanan activation of dopamine cells by the priming injection of cocaine.Indeed, electrophysiological studies indicate that acute cocaineadministration decreases spontaneous action potential generationin dopamine cells (Henry et al., 1989).

Role of locomotor activity

The data presented thus far implicate a VTA-dPFC-NAcore-VP series circuit in the production of cocaine-induced reinstatement,with the projection from the VTA to the dPFC being the dopamine-dependentinitiating step in the process. However, it is possible that theinhibitory effects of GABA agonists or fluphenazine are not specificto the goal-directed behavior under examination and may arisefrom a generalized motoric incapacity. A series of experimentswere conducted examining the effect of intracranial bac-mus orfluphenzine on spontaneous and cocaine-induced locomotor activity.bac-mus (at the minimum dose effective for blocking cocaine-inducedreinstatement) was infused into either the dPFC, NAcore, VTA,or VP before a systemic injection of either saline or cocaine(10 mg/kg, i.p.). Thus, there were four treatment conditions foreach of the target brain nuclei: saline plus saline, bac-mus plussaline, saline plus cocaine, and bac-mus plus cocaine. Two-wayANOVAs were conducted comparing saline with bac-mus pretreatmentacross the 2 hr test session for both spontaneous and cocaine-inducedactivity. Figure 6A shows that microinjection of bac-mus did notsignificantly reduce total photocell counts in any brain regionexamined. However, an analysis of the time course revealed thatGABA receptor activation produced a decrement in cocaine-inducedlocomotion in the VP over the first 20 min of the test session(data not shown). No other brain region tested showed any effectof bac-mus pretreatment at any time point.

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Figure 6. Locomotor activity. Mean ± SEM photocell counts are shown for the 2 hr test sessions for both spontaneous and cocaine-induced motor activity studies. A, Subjects received two treatments before each test: an intracranial infusion of saline (sal) or bac-mus followed by an intraperitoneal injection of either saline (sal) or cocaine (coc) (10 mg/kg; n = 8 in each condition). bac-mus pretreatment did not block either spontaneous or cocaine-induced locomotor activity when infused into the dPFC, NAcore, VTA, or VP. B, Fluphenazine (flu), when infused into the VP or NAcore but not the dPFC, produced a significant reduction in cocaine-induced locomotor activity. *p < 0.01, comparing bac-mus or fluphenazine with saline.

The effect of fluphenazine pretreatment on cocaine-induced locomotor activity was also examined (Fig. 6B). Fluphenazine pretreatmentinto the NAcore or into the VP produced a reliable decrement inlocomotor activity across the first 40 min of the test session.However, fluphenazine did not produce any decrement in cocaine-inducedactivity when microinfused into the dPFC (the only brain sitein which fluphenazine antagonized cocaine reinstatement) (Fig.5A). Together, these data demonstrate that the effects of GABAagonists and dopamine antagonists on self-administration are separablefrom effects on motoriccapacity.

Histology

Figure 7 shows the location of cannula tips from animals used in the self-administration experiments. Placements in the dPFCwere at the interface between the anterior cingulate cortex andthe prelimbic cortex (as depicted by Paxinos and Watson, 1998),whereas cannula tips designated vPFC were ~2 mm more ventral atthe border of the prelimbic and infralimbic cortices (Fig. 7A).Cannula placements in the NAshell were medial to the anteriorcommissure and were not in the ventrolateral limb of the nucleus,whereas placements in the NAcore were clustered around the anteriorcommissure (Fig. 7B). Placements in the VP were generally in thedorsal half of the nucleus in both the subcommissural and sublenticularcompartments (Fig. 7C). Cannulas in the MD were located primarilyin the ventral half of the nucleus, and placements in the amygdalawere clustered at the medial and lateral edges of the CN and BLA,respectively, to maximize the distinction between injections intothese near adjacent nuclei (Fig. 7D). Similarly, distinctionsbetween the VTA and SN were maximized by having cannula placementsin the VTA located in the medial half of the nucleus paranigralisand parabrachialis pigmentosus and injections into the SN madeinto the middle of the pars reticulata (Fig. 7E).

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Figure 7. Location of microinjection cannula tips. This figure depicts the location of the microinjection cannula tips in coronal section based on the atlas of Paxinos and Watson (1998). A, Dorsal () and ventral ( $black-square$ ) PFC; B, NAcore () and NAshell ( $black-square$ ); C, ventral pallidum (); D, basolateral amygdala ( $black-triangle$ ), central nucleus of the amygdala ( $cross$ ), and mediodorsal nucleus of the thalamus ( $black-square$ ); E, VTA () and substantia nigra ( $black-square$ ). Note that the was used in brain regions critical for the normal production of cocaine-induced reinstatement in the inactivation studies. Numbers indicate the distance from bregma in the anteroposterior plane.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study demonstrates that neural activity in the VTA, dPFC, NAcore, and VP is necessary for cocaine-induced reinstatementof drug-seeking behavior. Inactivation of these nuclei using theGABA agonists baclofen and muscimol prevented cocaine-primed drug-seekingbehavior in an animal reinstatement model of relapse. The sametreatment into the vPFC, NAshell, MD, SN, BLA, and CN producedno effect. These data strongly suggest that a limbic-cortico-striato-pallidalcircuit created by VTA-dPFC-NAcore-VP connections form a functionalseries circuit that is crucial for the ability of cocaine to elicitrenewed drug self-administration. Supporting the presence of aseries circuit, simultaneous contralateral (but not ipsilateral)inactivation of the dPFC and the VP blocked the reinstatementof self-administration. Because the dPFC and VP have few if anydirect connections (Sesack et al., 1989; Haber et al., 1995),a multisynaptic connection through the NAcore is likely requiredfor thebehavior.

Notably, inhibition of the dPFC and NAcore did not block the ability of noncontingent food delivery to reinstate food-seekingbehavior, indicating that the circuitry implicated in cocaine-inducedreinstatement does not generalize to all goal-directed responding.This finding strongly suggests that chronic cocaine elicits neuroadaptationsin prefrontal and accumbal motor circuitry in the control of drug-seekingbehavior, a notion consistent with the recent suggestion thatchronic cocaine causes behavioral impulsivity resulting from disinhibitionof frontostriatal function (Jentsch and Taylor, 1999). Inhibitionof the VP, however, blocked both food- and cocaine-seeking behavior,suggesting that outflow of information through the VP might serveas a common pathway by which motivationally relevant informationis transmitted to motorcircuitry.

The effect of drug treatment on reinstatement cannot be explained as a consequence of motoric incapacity, because infusionsof bac-mus into the dPFC, NAcore, and VTA produced no decrementin either spontaneous or cocaine-induced locomotor activity andinhibited cocaine-induced locomotion only in the first 20 minafter infusion into the VP. Notably, microinfusion of fluphenazineinto the NAcore and VP reliably diminished cocaine-induced locomotion,although it had no effect when infused into the dPFC, the onlylocation in which it prevented cocaine-primed drug-seeking behavior.These data suggest that circuitry mediating cocaine-induced reinstatementis distinct from that mediating spontaneous or cocaine-inducedlocomotion.

Mesocortical versus mesoaccumbens dopamine distinguishes reinstatement from reinforcement

Because the primary molecular mechanism of cocaine is blocking dopamine transporters (Povlock and Schenk, 1997), enhancedextracellular dopamine is likely the priming neurochemical signalinitiating reinstatement. Consistent with this possibility, inhibitionof neural activity in the VTA antagonized cocaine reinstatement.Similarly, systemic administration of dopamine antagonists preventspsychostimulant-induced reinstatement (De Vries et al., 1999).Although systemic cocaine administration enhances the extracellularlevels of dopamine in all dopamine axon terminal fields, dopamineantagonist administration in the dPFC, and not in the NAcore orVP, prevented reinstatement after systemic cocaine. These dataargue that enhanced dopamine transmission only in the dPFC isnecessary for cocaine-induced reinstatement. This possibilityis strengthened by the findings that (1) inhibition of cocaine-inducedreinstatement after GABA agonist administration into the VTA wasreversed by dopamine administration directly into the dPFC and(2) infusion of DA into the dPFC is sufficient to cause reinstatementof cocaine-seeking behavior in the absence of systemiccocaine.

In contrast to the findings regarding cocaine-primed reinstatement of drug seeking, studies examining the reinforcing propertiesof psychostimulants clearly implicate enhanced mesoaccumbens dopaminerelease as a critical substrate (Wise and Rompre, 1989; Koob etal., 1993; Robbins and Everitt, 1996). Thus, dopamine releasein the nucleus accumbens is postulated to be critical for thereinforcing capacity of psychostimulants and consequently forestablishing drug-seeking behavior (Robinson and Berridge, 1993).However, some evidence suggests that, once the behavior is well-learnedand automatic, it can become independent of dopamine release inthe nucleus accumbens. For example, along with the present evidenceindicating that cocaine-induced reinstatement of drug seekingproceeds after DA receptor antagonist treatment into the NA, thesame treatment fails to block the reinstatement of food-seekingbehavior in a straight-arm runway (Chausmer and Ettenberg, 1999).

A cortico-striato-pallidal circuit mediates drug-seeking behavior

Pyramidal cells in the PFC provide a dense glutamatergic projection to the nucleus accumbens that is topographically organizedsuch that the dPFC projects most densely to the NAcore and thevPFC selectively innervates the NAshell (Gorelova and Yang, 1997;Pinto and Sesack, 2000). Dopaminergic afferents from the VTA innervateboth interneurons and pyramidal cells in the PFC (Krimer et al.,1997), resulting in a complex electrophysiological impact on corticofugalprojections to the nucleus accumbens. The emerging picture revealsthat pyramidal projection neurons within the PFC display biphasicstates, fluctuating between a membrane potential that is relativelyhyperpolarized "down state" and an "up state" in which the membranepotential is relatively depolarized (Yang et al., 1996), and thatthe increase in dopamine caused by cocaine supports the up state(Lewis and O'Donnell, 2000). Enhanced residence in the up statewould be expected to increase corticofugal excitatory transmissionand is consistent with observations that repeated cocaine resultsin enhanced releasability of glutamate in the NAcore (Pierce etal., 1996; Reid and Berger, 1996) and that such release is partlyprevented by lesioning the dPFC (Pierce et al., 1998). Moreover,intra-accumbens administration of ionotropic glutamate receptorantagonist abolishes cocaine-induced reinstatement (Cornish andKalivas, 2000).

Increased glutamate release augments the firing frequency of medium spiny cells in the NAcore (O'Donnell and Grace, 1995;You et al., 1998), which have a dense GABAergic projection tothe VP (Heimer et al., 1991). Activation of these cells seemscritical for cocaine-primed drug-seeking behavior, because stimulationof GABA receptors in the VP inhibited cocaine-primed drug seeking.It appears contradictory to the postulate that dPFC-induced activationof medium spiny GABAergic cells projecting from the NAcore tothe VP mediates drug-seeking behavior when GABA-mediated inhibitionof VP cells blocks reinstatement. This incongruity may be attributableto a neuromodulatory role for GABA within the VP, such that itcan excite or inhibit behavioral output depending on the balanceof neurotransmission within the nucleus. Consistent with thisargument, GABA agonists have been shown to both inhibit and stimulatelocomotor activity when infused into the VP (Baud et al., 1989;Napier, 1993). Moreover, GABA is colocalized and coreleased witha variety of neuropeptides in efferents from the nucleus accumbensthat can differentially modulate the effect of GABA on VP neurons(Napier, 1993). For example, µ-opioid receptor stimulation inthe VP modulates the firing activity of VP neurons, inhibits GABArelease, initiates locomotor activity, and facilitates motivatedbehavior (Koob, 1992; Johnson and Stellar, 1994; Johnson and Napier,1997; Kalivas et al., 2001).

Another equally viable explanation of the fact that activation of GABAergic projection neurons from the NAcore to the VP seemsto mediate drug-seeking behavior whereas GABA mediated inhibitionof the VP blocks reinstatement relies on the concept of neuralensembles (Pennartz et al., 1994). According to this idea, inputsfrom the dPFC activate only a particular subset (or ensemble)of neurons in the NAcore, which in turn inhibit only a particularsubset of VP neurons. Thus, whereas selective inhibition of thisensemble of neurons, mediated by specific spatiotemporal firingpatterns within the NAcore, initiates reinstatement, broad-rangeinhibition of all VP neurons (such as an infusion of bac-mus)would disrupt these specific patterns of activity within the circuit,and thereby disruptbehavior.

Motor versus limbic subcircuits

Figure 8 illustrates the circuit containing the nuclei examined in this study and highlights topographic organization accordingto associations with limbic or motor subcircuits (Heimer and Alheid,1991; Mogenson et al., 1993). The interconnected nuclei associatedwith motor output were most sensitive to GABA agonist-inducedinhibition of cocaine reinstatement, whereas nuclei generallydescribed as providing integration of motivational stimuli werenot affected. The VTA is the only brain region typically associatedwith limbic integration that was sensitive to GABA agonists. However,this involvement may be permissive as a source of dopamine tothe cortex and not necessarily as an active component of the reinstatementbecause increasing dopamine tone in the dPFC elicits cocaine-inducedreinstatement (Fig. 5B).

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Figure 8. Circuit containing the nuclei injected with GABA agonists. The circuit illustrates the connectivity of the limbic and motor regions that have been implicated in the production of goal-directed behavior. The limbic subcircuit is more closely associated with limbic structures, and the motor subcircuit is more intimately connected with motor structures (Heimer et al., 1991; Zahm and Brog, 1992). Arrowheads indicate the direction of the projection, and bidirectional arrows indicate reciprocal connections. Larger circles and arrows indicate nuclei identified as critical for drug-seeking behavior.

Some nuclei in the circuit, such as the BLA and MD, have been implicated previously in drug reward and cue-induced reinstatementor craving but were found to be not involved in cocaine-inducedreinstatement (Weissenborn et al., 1998; Grimm and See, 2000).This is most readily explained by the fact that different typesof eliciting stimuli (e.g., cocaine versus cocaine-paired cues)depend on differential processing within the motive circuit toproduce their behavioral activating effects. Thus, different stimulimay initiate reinstatement behavior by recruiting nuclei in thelimbic subcircuit, although the execution of the behavior mayrely on the motor subcircuit consisting of the series connectionbetween the dPFC, NAcore, andVP.

The fact that the nuclei shown to be critical for cocaine-induced reinstatement are part of the motor subcircuit argues thatdrug-seeking behavior in a drug-experienced subject requires littlelimbic integration. Thus, in parallel with reports from cocaineaddicts (Childress et al., 1999), the motor behaviors mediatingdrug-seeking behavior are easily primed and relatively automatic.In this sense, drug-seeking behavior resembles other compulsivemotor disorders (Jog et al., 1999) known to involve cortico-striato-pallidalcircuitry.

  FOOTNOTES

Received June 19, 2001; revised Aug. 6, 2001; accepted Aug. 10, 2001.

This research was supported in part by United States Public Health Service Grants DA12513, MH40817, and DA03906 and postdoctoralNational Research Service Award DA05978 (K.M.). We thank ChristopherLapish for his outstanding technicalassistance.
Correspondence should be addressed to Krista McFarland, Department of Physiology and Neuroscience, Medical University of SouthCarolina, 173 Ashley Avenue, Room 403, Charleston, SC 29425. E-mail:mcfarlk{at}musc.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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