{Delta}FosB in the Nucleus Accumbens Regulates Food-Reinforced Instrumental Behavior and Motivation

doi:10.1523/JNEUROSCI.1124-06.2006

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The Journal of Neuroscience, September 6, 2006, 26(36):9196-9204; doi:10.1523/JNEUROSCI.1124-06.2006

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Behavioral/Systems/Cognitive
${Delta}$ FosB in the Nucleus Accumbens Regulates Food-Reinforced Instrumental Behavior and Motivation
Peter Olausson,¹ J. David Jentsch,² Natalie Tronson,¹ Rachel L. Neve,³ Eric J. Nestler,⁴ and Jane R. Taylor¹
¹Department of Psychiatry, Division of Molecular Psychiatry, Yale University School of Medicine, New Haven, Connecticut 06508, ²Department of Psychology, University of California, Los Angeles, California 90095, ³Department of Psychiatry, Harvard Medical School, McLean Hospital, Belmont, Massachusetts 02178, and ⁴Department of Psychiatry and Center for Basic Neuroscience, The University of Texas Southwestern Medical Center, Dallas, Texas 75390

   Abstract

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Alterations in motivation have been implicated in the pathophysiologyof several psychiatric disorders, including substance abuseand depression. Repeated exposure to drugs of abuse or stressis known to persistently induce the transcription factor ${Delta}$ FosBin the nucleus accumbens (NAc) and dorsal striatum, effectshypothesized to contribute to neuroadaptations in dopamine-regulatedsignaling. Little is known, however, about the specific involvementof ${Delta}$ FosB in dysregulation of appetitively motivated behaviors.We show here that inducible overexpression of ${Delta}$ FosB in NAc anddorsal striatum of bitransgenic mice, or specifically in theNAc core of rats by use of viral-mediated gene transfer, enhancedfood-reinforced instrumental performance and progressive ratioresponding. Very similar behavioral effects were found afterprevious repeated exposure to cocaine, amphetamine, MDMA [(+)-3,4-methylenedioxymethamphetamine],or nicotine in rats. These results reveal the powerful regulationof motivational processes by ${Delta}$ FosB, and provide evidence thatdrug-induced alterations in gene expression via induction of ${Delta}$ FosB within the NAc core may play a critical role in the impactof motivational influences on instrumental behavior.

Key words: addiction; psychostimulant; reinforcement; dopamine; gene expression; transcription factors

   Introduction

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Repeated drug exposure causes temporally dynamic alterationsin gene transcription that produce lasting neuroadaptationswithin the nucleus accumbens (NAc) (Nestler, 2004). This brainregion plays a critical role in both drug and natural reinforcementprocesses (Kelley and Berridge, 2002), although little is knownabout the transcription factors that impact on behavior motivatedby nondrug, appetitive reinforcers such as food. ${Delta}$ FosB is a transcriptionfactor activated within the NAc and dorsal striatum by chronicdrug exposure (Konradi et al., 1994; Nye et al., 1995; Chenet al., 1997; Pich et al., 1997; Shaw-Lutchman et al., 2003)and compulsive wheel-running (Werme et al., 2002). It is alsoinduced in these regions by several forms of chronic stress(Perrotti et al., 2004). The enhancement of drug reinforcementprocesses associated with induction of striatal ${Delta}$ FosB is wellestablished (Kelz et al., 1999; Colby et al., 2003; Zachariouet al., 2006). The consequences of elevated ${Delta}$ FosB levels in theseregions on instrumental behavior motivated by natural reinforcersare, however, not known.
The performance of instrumental responses is a necessary componentof drug-taking behavior that can become dysregulated or inflexibleas the transition to addiction progresses (Jentsch and Taylor,1999; Berke and Hyman, 2000; Berridge and Robinson, 2003; Everittand Robbins, 2005). The NAc is involved in multiple aspectsof instrumental behavior with relevance for addiction (Balleineand Killcross, 1994; Corbit et al., 2001; de Borchgrave et al.,2002; Di Ciano and Everitt, 2004b; Everitt and Robbins, 2005).It is therefore likely that drug-induced neuroadaptations withinthe NAc could affect performance of instrumental actions. Indeed,chronic cocaine exposure enhances sucrose-reinforced instrumentalperformance (Miles et al., 2004) and manipulations thought toblock neuroplasticity within the NAc core, including inhibitionof PKA (protein kinase A) or protein synthesis, interfere withfood-rewarded instrumental responses (Baldwin et al., 2002a;Hernandez et al., 2002). The NAc core also mediates the motivationalimpact of conditioned influences on instrumental behavior (Parkinsonet al., 1999; Corbit et al., 2001; Hall et al., 2001; Di Cianoand Everitt, 2004a; Ito et al., 2004), providing a neurobiologicalsubstrate whereby ${Delta}$ FosB induction might powerfully affect instrumentalperformance and motivation for appetitive reinforcers such asfood, water, or drugs of abuse.
Here, we investigated the effects of ${Delta}$ FosB on food-motivatedinstrumental behavior using two complementary genetic approaches:(1) inducible overexpression of ${Delta}$ FosB within the NAc and dorsalstriatum of bitransgenic mice (NSE-tTA x TetOp- ${Delta}$ FosB) and (2)overexpression of ${Delta}$ FosB in the NAc core specifically by use ofviral-mediated gene transfer in rats. We also evaluated whetherprevious repeated exposure to cocaine, amphetamine, (+)-3,4-methylenedioxymethamphetamine(MDMA), or nicotine, under conditions reported to increase ${Delta}$ FosB,would enhance food-reinforced instrumental responding and/ormotivation using a progressive ratio schedule, as has been shownfor drug-reinforced self-administration (Horger et al., 1990,1992; Piazza et al., 1990; Vezina et al., 2002; Miles et al.,2004). Our results demonstrate persistent effects of ${Delta}$ FosB oninstrumental behavior and suggest that this transcription factormay act in the NAc core as a regulator of motivational function.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Animals and animal care
Experimentally naive Sprague Dawley rats were acquired fromCharles River Laboratories (Wilmington, MA). Male bitransgenic11A mice were derived from a cross between homozygous transgenicmice expressing a neuron-specific enolase (NSE)-tTA tetracyclinetransactivator protein (line A) and mice expressing TetOp (tetracycline-responsivepromoter)- ${Delta}$ FosB (line 11); the parental lines were maintainedon an outbred mixed background (50% ICR and 50% C57BL6 x SJL)(Chen et al., 1998; Kelz et al., 1999). These bitransgenic 11Amice express ${Delta}$ FosB only when: (1) both transgenes are presentin the same cell, and (2) the transcriptional activation bytTA is not inhibited by the presence of tetracycline antibioticssuch as doxycycline. The administration of doxycycline to thesemice can thus exert a temporal control over the expression of ${Delta}$ FosB and be used to prevent the expression during development;indeed, doxycycline administration is associated with no detectableleak expression of ${Delta}$ FosB (Chen et al., 1998; Kelz et al., 1999).Moreover, the 11A line of bitransgenic mice were chosen forthe present experiments, because they display an expressionpattern that is primarily restricted to dynorphin-containingstriatal neurons (both NAc and dorsal striatum), very similarto the pattern of ${Delta}$ FosB induction by chronic drug exposure (Kelzet al., 1999). Moreover, the quantification of this striatalexpression of ${Delta}$ FosB has been quantified previously (Chen et al.,1998; Kelz et al., 1999). The mice were generated at Universityof Texas Southwestern and maintained and tested in the Yalefacilities. Throughout gestation and development, all mice weremaintained on doxycycline until 8–9 weeks of age at aconcentration of 100 µg/ml in the drinking water, conditionsknown to maintain TetOp-driven transgenes in the "off" state,and used starting 6 weeks off doxycycline when ${Delta}$ FosB expressionbecomes maximal (Kelz et al., 1999). All experiments involvedthe comparison of littermate bitransgenic mice on versus offdoxycycline, which by itself has no effect on motivated behavior(Kelz et al., 1999; McClung and Nestler, 2003; Zachariou etal., 2006).
All experimental subjects were housed in pairs (rats) or ingroups (mice; four to five per cage) under controlled temperatureand humidity conditions under a 12 h light/dark cycle (lighton at 7:00 A.M. and off at 7:00 P.M.). They were allowed atleast 7 d to adjust to the housing facilities before any study.Animals had ad libitum access to water at all times and limitedaccess to food as detailed below. All animal use was conductedin accordance with the National Institutes of Health Guide forthe Care and Use of Laboratory Animals and was approved by theAnimal Care and Use Committees at University of Texas Southwesternand Yale University.
Drugs
Cocaine hydrochloride [kindly provided by the National Instituteon Drug Abuse (NIDA)], D-amphetamine sulfate (Sigma, St. Louis,MO), MDMA hydrochloride (kindly provided by NIDA), and (–)-nicotinehydrogen tartrate (Sigma) were dissolved in sterile physiologicalsaline (0.9%) and injected intraperitonally at a volume of 5ml/kg (mice) or 2 ml/kg (rats). The pH of the nicotine solutionwas adjusted with sodium bicarbonate before injection.
Viral vectors
Viral-mediated gene transfer was performed as previously described(Carlezon et al., 1998; Perrotti et al., 2004). In short, cDNAsencoding the specific proteins were inserted into the herpessimplex virus (HSV) amplicon HSV-PrPUC and packaged into thevirus using the helper 5dl1.2. The vectors driving expressionof either HSV-LacZ, coding for the control protein $beta$ -galactosidase,or HSV- ${Delta}$ FosB, coding for ${Delta}$ FosB, were subsequently infused intothe NAc core according to the experimental protocol.
Experimental procedure
Outline. Experiment 1 examined the effects of previous repeated drugexposure on food-reinforced instrumental performance and progressiveratio responding. Rats were randomly divided into five experimentalgroups (n = 9–10/group). These groups received twice dailyinjections (intraperitoneally; at 9:00 A.M. and 5:00 P.M.) withsaline or one of the following drugs: nicotine, 0.35 mg/kg;MDMA, 2.5 mg/kg; cocaine, 15 mg/kg; or amphetamine, 2.5 mg/kgfor 15 consecutive days. The doses were selected based on ourpreviously published data (Taylor and Jentsch, 2001; Olaussonet al., 2003), and the drug-induced locomotor stimulation wasmonitored on treatment days 1 and 15. After 5 d of withdrawal,animals were trained on instrumental responding for 10 consecutivedays and subsequently tested on progressive ratio respondingon the next day. Two animals were excluded from the statisticalanalysis because they did not acquire the instrumental response,making no more than one active lever response on each of thethree final training sessions.
Experiments 2 and 3 examined the effects of inducible striataloverexpression of ${Delta}$ FosB in bitransgenic mice on instrumentalperformance and responding on a progressive ratio of reinforcement.The inducible overexpression of ${Delta}$ FosB in these mice has previouslybeen demonstrated to mimic the effects of repeated drug exposurein the locomotor activity and conditioned place preference paradigms(Kelz et al., 1999; Zachariou et al., 2006). These mice canprovide critical information about the contribution of striatal ${Delta}$ FosB to specific behavioral processes. Genotyped male mice weremaintained on doxycycline or were switched to tap water at 8weeks of age. Experiments were initiated after 6 weeks of doxycyclinewithdrawal, at which time transgene expression is maximal (Kelzet al., 1999). In experiment 2, animals (n = 16) were food restrictedand trained on the instrumental procedure described below (seebelow, Instrumental responding and progressive ratio testing)for 10 consecutive days. After the completion of instrumentaltesting, cocaine-induced locomotor stimulation was evaluatedin these mice. In experiment 3, a separate group of mice (n= 18) were trained on the instrumental response for 10 consecutivedays under conditions during which a maximum of 50 reinforcerswere delivered. On day 11, all mice were tested on progressiveratio responding. On day 12, we determined the effects of reinforcerdevaluation by prefeeding on progressive ratio responding.
Experiments 4 and 5 examined the effects of viral-mediated overexpressionof ${Delta}$ FosB specifically within the NAc. Experiment 4 tested theeffects of ${Delta}$ FosB overexpression on instrumental performance.Here, rats were infused with HSV- ${Delta}$ FosB (n = 8) or HSV-LacZ (n= 8) in the NAc core and trained on the instrumental procedurebeginning 40 h later. After 10 daily training sessions, baselineactivity levels were assessed for all animals in the locomotoractivity monitoring equipment as described below (see below,Locomotor activity). Experiment 5 evaluated the effects of NAc ${Delta}$ FosB overexpression specifically on progressive ratio responding.Here, the rats were initially trained for 15 consecutive days,assigned to experimental groups, and subsequently infused withHSV- ${Delta}$ FosB (n = 8) or HSV-LacZ (n = 7) in the NAc core. Animalswere left untested and untreated for 4 d to allow for ${Delta}$ FosB expressionto peak. On day 5 after infusion, all animals were tested forlever pressing on the progressive ratio schedule. After thelast day of testing, all rats were killed and the placementof infusion cannulas in the NAc core verified histochemically.Based on the placement of infusion cannulas, two rats were excludedfrom experiment 4 and one rat from experiment 5.
Characterization of gene expression was made in a separate groupof animals. Here, HSV-LacZ was infused into the NAc core andanimals were killed 3 d later. The expression of $beta$ -galactosidasewas subsequently assessed immunohistochemically.
Locomotor activity. Locomotor activity was measured using activity meters (Digiscananimal activity monitor; Omnitech Electronics, Columbus, OH).The activity meters were equipped with two rows of infraredphotosensors, each row consisting of 16 sensors placed 2.5 cmapart. The activity meters were controlled by and data fromthe activity meters collected by a PC computer using the Microprosoftware (Omnitech Electronics).
The experimental animals were placed in transparent plasticboxes (25 x 45 x 20 cm) that were put into the activity meters.Animals were initially allowed to habituate to the locomotoractivity recording equipment for 30 min. In some experiments,animals were subsequently taken out, injected with cocaine,amphetamine, nicotine, or vehicle according to the experimentaldesign, and placed back into the boxes. The locomotor activitywas then recorded for 60 min, starting 5 min after drug injectionto avoid nonspecific injection-induced hypermotility. All experimentswere performed during the animals’ light phase (between9:00 A.M. and 6:00 P.M.).
Instrumental responding and progressive ratio testing. Instrumental responding was assessed using standard operantchambers for rats (30 x 20 x 25 cm) or mice (16 x 14 x 13 cm)controlled by the MedPC software (Med Associates, St. Albans,VT). Each chamber was housed in a sound-attenuating outer chamberequipped with a white noise generator and a fan to reduce theimpact of external noise. A house light mounted on the backwall illuminated the chamber. A pellet dispenser delivered foodpellets (20 or 45 mg; Bio-Serv, Frenchtown, NJ) as the reinforcerinto the magazine. Head entries were detected by a photocellmounted above the reinforcer receptacle. In this magazine wasa stimulus light. For rats, one lever was placed on each sideof the magazine. For mice, two nosepoke apertures were placedon the back wall of the chambers (i.e., opposite to the reinforcermagazine).
During the 5 d immediately before the start of training, animalswere restricted to 90 min access to food per day and exposedto grain-based food pellets (mice, 20 mg; rats, 45 mg) in theirhome cages. During the testing period, food pellets were intermittentlyavailable in the operant chambers according to the behavioralprotocol (see below) as well as in unlimited amounts in thehome cage for 90 min, beginning 30 min after the daily testingsession. This food access schedule allows for each individualanimal to reach their individual satiety point and reduces thevariability caused by competition between dominant and subordinateanimals. In our hands, this schedule allows for a slow weightgain after the initial weight loss to $~$ 85–90% of free-feedingweights. Animal weights were monitored throughout the experiment.
All subjects were initially habituated to the testing apparatusfor 2 d; during these sessions, food pellets were deliveredinto the reinforcer magazine on a fixed-time 15 s (FT-15) schedule.Beginning on the next day, the subjects received daily trainingsessions for 10 consecutive days. Responding for food was testedbased on previously published instrumental conditioning procedures(Baldwin et al., 2002b). Responding on the correct (i.e., active)lever/nosepoke was reinforced, whereas responding on the other(inactive) lever/nosepoke had no programmed consequences. Theposition of the active nosepoke or lever (left/right) was balancedfor all experimental groups. Completion of the response requirement(see below) resulted in onset of the magazine stimulus light,followed 1 s later by delivery of a single food pellet. Twoseconds later, the stimulus light was turned off. The first10 reinforcers were obtained after successful completion ofresponding according to a fixed ratio (FR1) schedule, afterwhich pellets were available after responding on a variableratio (VR2) schedule. The session lasted for 15 min.
Experiments 3 (mice) and 5 (rats) used alternative trainingschedules to avoid the potential impact of differences in instrumentalperformance during training on subsequent progressive ratioresponding (detailed below). In experiment 3, mice were trainedon a FR1 schedule for 2 d and then on an FR2 schedule for 8d. The first 3 d of testing used 60 min sessions. On the last7 training days, the session was terminated when 50 reinforcershad been acquired. In experiment 5, rats were trained on theFR1/VR2 schedule in 15 min sessions as described above for allother experiments with two exceptions. First, a maximal numberof 150 pellets/session was delivered. Second, these animalsreceived 5 additional days of training (i.e., a total of 15d) to allow for the establishment of stable performance beforeany experimental manipulation.
Animals were also tested on responding for food on a progressiveratio schedule of reinforcement. In this test, the responserequirement to obtain food was initiated as a FR1 schedule butprogressively increased by 2 to obtain a subsequent reinforcer(i.e., 1, 3, 5, 7..., X + 2 responses). In the drug treatmentexperiment using rats, the schedule was progressively increasedby 5, yielding a final schedule of 1, 6, 11, 16..., X + 5. Allother parameters were kept identical to the training proceduredetailed above. The test was terminated when no active responsehad been made for 5 min.
Reinforcer devaluation. The effect of reinforcer devaluation was examined using reinforcer-specificprefeeding. Here, mice were allowed to eat unlimited grain-basedfood pellets in their home cage during 3 h before testing onthe progressive ratio schedule of reinforcement as describedabove.
Surgical techniques. Animals were anesthetized using Equithesin [a mixture containingpentobarbital (35 mg/kg) and chloral hydrate (183.6 mg/kg) inethanol (10% v/v) and propylene glycol (39% v/v); administeredat 4.32 ml/kg, i.p.]. Cannulas (Plastics One, Roanoke, VA) weresurgically implanted aimed above the NAc core, using Kopf stereotacticequipment. The stereotactic coordinates used relative to bregmawere as follows: anterior/posterior, +1.5 mm; lateral/medial,±1.5 mm; ventral/dorsal, –6.0 mm (Paxinos and Watson,1986). The cannulas were anchored to the skull using screwsand dental cement. Obturators were placed into the guide cannulasto prevent blocking. After surgery, animals were subjected tostandard postoperative care and were allowed to recover for5 d before the start of any experiment.
Infusions. Intracerebral infusions of viral vectors were performed bilaterally40 h before the onset of training (see below). Injection syringes(31 gauge), extending 1 mm below the tip of the guide cannulas,were slowly lowered simultaneously into the left and the rightNAc, and 1.0 µl/side was infused over a 4 min period atan infusion rate of 0.25 µl/min using a microinfusionpump (PHD-5000; Harvard Apparatus, Holliston, MA). The infusionneedles were left in place for 1 min after the infusion wascompleted, and the dummy cannulas were replaced. Cannula placementswere histologically verified after the completion of the behavioralexperiments (see Fig. 6B), and only animals with correctly placedcannulas were included in the statistical analysis of the experimentaldata.
Histological analyses and immunostaining. After the completion of the experiments, animals that had receivedsurgeries as part of the experiment were anesthetized with Equithesinand perfused transcardially with 0.1 M PBS (5 min) and 10% formalin(10 min) according to standard procedures. Brains were postfixedin formalin and subsequently placed in a phosphate-bufferedsucrose solution (30%). All brains were then cut in 40 µmsections on a microtome and used for histological analyses ofcannula placement and protein expression.
Cannula placement was made in sections counterstained with neutralred and mounted on microscope slides in distyrene plasticizerand xylene (DPX) after ethanol dehydration. Immunohistochemistrywas performed as previously described (Hommel et al., 2003).In short, expression of $beta$ -galactosidase after HSV-LacZ infusionwas determined by immunofluorescent staining using a goat anti- $beta$ -galactosidaseprimary antibody (1:5000; Biogenesis, Kingston, NH). After overnightincubation, sections were rinsed and subsequently incubatedwith a fluorescent donkey anti-goat secondary antibody conjugatedto Cy2 (1:200; Jackson ImmunoResearch, West Grove, PA). Sectionswere washed again followed by ethanol dehydration and mountingin DPX. Adjacent control sections were treated identically withoutthe inclusion of primary antibodies. Immunofluorescence wasassessed at 520 nm using a Zeiss (Oberkochen, Germany) microscopewith FITC filter and images captured at identical exposure timeswith Zeiss Axiovision digital imaging system.
Statistics
The data from all experiments were evaluated using a one-, two-,or three-way ANOVA followed by Scheffe's or Dunnett's post hoctest, correcting for multiple comparisons where appropriateusing Holm's sequential rejection test. A value of p $≤$ 0.05 wasconsidered statistically significant.

   Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Experiment 1: effects of repeated drug exposure on instrumental performance and progressive ratio responding
To confirm that our repeated drug exposure paradigm producedfunctionally significant neuroadaptations, we first assessedlocomotor sensitization as a prototypical behavioral measureof chronic drug action. Rats were given twice daily injectionsof nicotine (0.35 mg/kg), MDMA (5 mg/kg), cocaine (15 mg/kg),or amphetamine (2.5 mg/kg), and locomotor activity was testedafter the first injection on treatment days 1 and 15 (supplementalFig. 1A–E, available at www.jneurosci.org as supplemental material).Statistical analysis revealed a significant treatment by dayinteraction (F_(4,42) = 9.335; p $≤$ 0.0001). With the exceptionof MDMA (p = 0.62), all drugs induced significantly greaterlocomotor activity (i.e., sensitization) on day 15 comparedwith day 1 (nicotine, p $≤$ 0.001; cocaine, p $≤$ 0.001; amphetamine,p $≤$ 0.01). Repeated saline injections had no effect. None ofthe drug treatments altered baseline locomotor activity measuredduring the habituation period on day 15 (supplemental Fig. 2A,available at www.jneurosci.org as supplemental material).
Five days after the last drug injection, we examined the effectsof previous repeated nicotine, MDMA, cocaine, or amphetamineexposure on food-reinforced instrumental behavior. The dataare presented for each drug separately in Figure 1A–Husing the same saline control group for comparisons. We foundthat previous exposure to each of these drugs significantlyand selectively increased food-reinforced instrumental responding(treatment by lever by training day, F_(36,378) = 1.683; p $≤$ 0.01;post hoc analysis: nicotine, p $≤$ 0.01; MDMA, p $≤$ 0.05; cocaine,p $≤$ 0.01; amphetamine, p $≤$ 0.001). The persistent elevation ininstrumental responding observed at asymptotic performance suggesteda possible enhancement in motivation, consistent with previouslyreported increases after repeated psychostimulant exposure (seeDiscussion). We therefore tested whether previous repeated drugexposure enhanced motivation using a progressive ratio schedule.There was a statistical effect of previous drug exposure onresponding on the active lever (treatment by lever interaction,F_(4,42) = 3.340; p $≤$ 0.05) (Fig. 2A) as well as the final breakpoint (F_(4,42) = 5.560; p $≤$ 0.001) (Fig. 2B). Additional analysisshowed that all treatments increased both the number of activeresponses (nicotine, p $≤$ 0.001; MDMA, p $≤$ 0.05; cocaine, p $≤$ 0.001;amphetamine, p $≤$ 0.001) and the break point (nicotine, p $≤$ 0.001;MDMA, p $≤$ 0.01; cocaine, p $≤$ 0.0001; amphetamine, p $≤$ 0.0001) consistentwith an effect of these treatments on motivation. Given thelack of effect of the drugs on baseline locomotor activity,and the lack of effect on inactive lever presses, it is unlikelythat the increased responding for food under these conditionsreflects nonspecific increases in motor activity.

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Figure 1. Effect of previous repeated injections of nicotine (0.35 mg/kg), MDMA (2.5 mg/kg), cocaine (15 mg/kg), or amphetamine (2.5 mg/kg) twice daily for 15 d on subsequent instrumental behavior. The animals were tested together, but for clarity the effects of each drug are presented separately, using the same saline-treated control group. A (active responses) and B (inactive responses) show the effects of previous nicotine exposure; C, D, MDMA; E, F, cocaine; G, H, amphetamine. Data are represented as means ± SEM.

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Figure 2. Effect of previous repeated treatment (twice daily, 15 d) with saline, nicotine (0.35 mg/kg), MDMA (2.5 mg/kg), cocaine (15 mg/kg), or amphetamine (2.5 mg/kg) on instrumental responding on a progressive ratio schedule of reinforcement. Data are represented as means ± SEM. ***p < 0.001; **p < 0.01; *p < 0.05. Sal, Saline; Nic, nicotine; Coc, cocaine; Amph, amphetamine; PR, progressive ratio.

Previous drug exposure also had no effect on body weight recordedbefore food restriction, on the first or last day of instrumentaltraining, or immediately before the progressive ratio test (supplementalFig. 2B, available at www.jneurosci.org as supplemental material).The restricted food access for 3 d did initially reduce bodyweight to on average 91–92% of free-feeding weights. Atthe end of behavioral testing, weights had returned to 97–99%of prerestriction body weight, and no differences were observedbetween drug-exposed and saline-treated animals. Alterationsin body weight and differences in hunger or appetite shouldthus not contribute significantly to the observed enhancementof instrumental performance or motivation.
Experiment 2: inducible overexpression of ${Delta}$ FosB in bitransgenic mice; instrumental performance
We next examined whether instrumental performance was also increasedin bitransgenic mice that inducibly overexpress ${Delta}$ FosB with markedselectivity in the NAc and dorsal striatum (Kelz et al., 1999).In this experiment, ${Delta}$ FosB-overexpressing mice were compared withlittermate controls that do not overexpress ${Delta}$ FosB because theyare maintained on doxycycline (see Materials and Methods). Wefound that overexpression of ${Delta}$ FosB significantly increased food-reinforcedresponding (gene expression by lever by training day, F_(9,126)= 3.156; p $≤$ 0.01) (Fig. 3A). The number of nosepoke responsesmade in the inactive aperture was not different between thetwo groups (Fig. 3B). Together, these data indicate that ${Delta}$ FosBoverexpression in NAc and dorsal striatum selectively increasedinstrumental performance.

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Figure 3. Effect of inducible striatal overexpression of ${Delta}$ FosB in bitransgenic mice on instrumental performance. A, Active responses. B, Inactive responses. Data are represented as means ± SEM.

To rule out that the enhancement of instrumental performancein ${Delta}$ FosB-overexpressing animals could be explained by alterationsin appetite or hunger, body weight was recorded before foodrestriction and on the first and last days of training. ${Delta}$ FosBhad no effect on body weight before food restriction, nor wasthere an effect on body weight during behavioral testing. Here,restricted food access for 3 d reduced body weight to an averageof 87–89% of free-feeding weights. At the end of behavioraltesting, animal weights were 97–99% of prerestrictionbody weights, with equivalent changes seen in the ${Delta}$ FosB and controlmice (supplemental Fig. 3A, available at www.jneurosci.org assupplemental material). It is thus unlikely that potential effectsof ${Delta}$ FosB overexpression on hunger or appetite could account forenhancements in instrumental responding observed.
When testing on instrumental performance had been completed, ${Delta}$ FosB overexpression did not alter baseline locomotor activitymeasured during a 30 min period (supplemental Fig. 3B, availableat www.jneurosci.org as supplemental material). This observationsupports the view that nonspecific alteration in activity doesnot contribute to the enhanced instrumental performance observedin these animals. However, ${Delta}$ FosB-overexpressing bitransgenicmice have been reported to exhibit enhanced locomotor responsesto acute and repeated cocaine (Kelz et al., 1999). Because weused a slightly different schedule of withdrawal from doxycyclineto induce gene expression (6 weeks with food restriction), weset out to confirm this phenotype. Indeed, ${Delta}$ FosB-overexpressingmice demonstrated a significantly greater increase in locomotoractivity when injected with cocaine compared with their littermatecontrols maintained on doxycycline (treatment by gene expression,F_(1,44) = 4.241; p $≤$ 0.05) (supplemental Fig. 3C, available atwww.jneurosci.org as supplemental material).
Experiment 3: inducible overexpression of ${Delta}$ FosB in bitransgenic mice; progressive ratio
Given that previous drug exposure induces striatal ${Delta}$ FosB (Nestleret al., 2001) and was found here to increase progressive ratioresponding, we next tested whether transgenic striatal overexpressionof ${Delta}$ FosB also increases performance on a progressive ratio scheduleof reinforcement. A new group of mice were trained on instrumentalresponding under conditions (see Materials and Methods) thatdid not produce significant differences in instrumental performancebefore testing on progressive ratio responding (F_(1,16) <1). However, in the progressive ratio test we observed a significantgene expression by lever interaction (F_(1,16) = 5.30; p $≤$ 0.05)(Fig. 4A) and found that ${Delta}$ FosB-overexpressing mice, comparedwith littermate control mice maintained on doxycycline, madea greater number of active responses (p $≤$ 0.05), whereas thenumber of inactive lever responses was not different. ${Delta}$ FosB-overexpressingmice also reached a higher break point (F_(1,16) = 5.73; p $≤$ 0.05)(Fig. 4B). These data suggest that, like previous psychostimulantexposure, striatal overexpression of ${Delta}$ FosB increases motivation.Because the number of inactive responses was not altered inthe ${Delta}$ FosB-overexpressing mice, nonspecific increases in activityare not likely to contribute to these effects. This view wasfurther supported by assessments of baseline locomotor activityin which there was no difference between mice overexpressing ${Delta}$ FosB and littermate control mice maintained on doxycycline.No gross differences in body weight between ${Delta}$ FosB-overexpressingand control animals were evident as measured on the test day.Thus, although ${Delta}$ FosB-overexpressing animals will emit more food-motivatedinstrumental responses, they do not appear to consume more foodwhen it is freely available. The most likely explanation forthis observation is that, although motivation determines howhard an animal will work to acquire a reinforcer, numerous additionalfactors (appetite, satiety, metabolic state, etc.) influencefeeding behavior and the actual consumption of food.

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Figure 4. Effect of inducible overexpression of FosB in bitransgenic mice on instrumental responding on a progressive ratio schedule of reinforcement, before and after satiety-induced reinforcer devaluation. A, B, Baseline: lever responses (A), break point (B). C, D, After reinforcer devaluation: lever responses (C), break point (D). Data are represented as means ± SEM. *p < 0.05.

The ${Delta}$ FosB bitransgenic mice used here express ${Delta}$ FosB throughoutthe striatum. Whereas the ventral striatum (including the NAc)has been implicated in motivational processes, the dorsal striatumis argued to be involved in the acquisition of instrumentalhabits (Yin et al., 2004; Faure et al., 2005). Although we didnot observe differences in instrumental performance during thetraining phase using a low ratio schedule with maximal reinforcementlimits, conditions relatively resistant to the development ofinstrumental habits (Dickinson, 1985), it is possible that theestablishment of habits could influence responding under theprogressive ratio schedule. This possibility was tested directlyby evaluating the effect of reinforcer devaluation by prefeedingon progressive ratio responding. Such prefeeding obliteratedthe effect of ${Delta}$ FosB on progressive ratio responding, with nodifferences in responding or break points observed between ${Delta}$ FosB-overexpressingand control mice (F_(1,16) < 1) (Fig. 4C,D). Together, thesedata suggest that striatal overexpression of ${Delta}$ FosB did not alterthe sensitivity to changes in the value of rewarded outcomesusing this testing schedule. Rather, the instrumental respondingobserved in the progressive ratio test appears to be goal-directedand the increased break point observed in ${Delta}$ FosB-overexpressingmice is likely attributable to augmented motivation and notto elevated habit-like responding.
Experiment 4: viral-mediated overexpression of ${Delta}$ FosB in the NAc core: instrumental performance
To assess whether ${Delta}$ FosB overexpression selectively in the NAccould account for the behavior observed in the bitransgenicmice, we infused HSV- ${Delta}$ FosB, or HSV-LacZ as a control, selectivelyinto the NAc core of rats and studied the effect of this manipulationon food-reinforced instrumental performance (Fig. 5A,B). Aftermagazine training, HSV- ${Delta}$ FosB or HSV-LacZ was infused into theNAc core 40 h before the initiation of behavioral testing. Thelocation of the infusion and the extent of viral-mediated geneexpression are shown in Figure 6, A and B. NAc infusions ofHSV- ${Delta}$ FosB produced a sustained increase in the number of activeresponses made (gene expression by lever, F_(1,12) = 8.534; p $≤$ 0.05) (Fig. 5A), which persisted throughout the experiment.These effects were selective, because there were no significanteffects of ${Delta}$ FosB overexpression within the NAc core on the numberof inactive responses (Fig. 5B) or on baseline locomotor activityrecorded the day after the completion of the experiment (datanot shown). Overexpression of ${Delta}$ FosB in the NAc thus mimickedthe behavioral effects of previous drug exposure or striataloverexpression of ${Delta}$ FosB.

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Figure 5. Effect of infusions of HSV- ${Delta}$ FosB into the NAc core before training on instrumental responding. A, Active responses. B, Inactive responses. Data are represented as means ± SEM.

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Figure 6. A, Placements of infusion sites for the viral vector experiments. Top, The filled black circles correspond to the intended infusion site. Only infusions made within $~$ 0.5 mm of this area (i.e., within the NAc core), as indicated by the circle, were considered acceptable. Animals with infusions made outside of this area were excluded from statistical analyses. Bottom, Infusion site within the NAc in a representative animal. B, Immunohistochemical verification of protein expression after infusion of HSV-LacZ. The top panels demonstrate $beta$ -galactosidase expression within the NAc core (2.5 and 10x magnification). The bottom panels demonstrate the lack of immunofluorescence in adjacent control sections using the same immunohistochemical procedure without the inclusion of the primary antibody.

Experiment 5: viral-mediated overexpression of ${Delta}$ FosB in the NAc core: progressive ratio
The final experiment directly determined whether restrictedoverexpression of ${Delta}$ FosB in the NAc core using the viral-mediatedgene transfer approach was sufficient to enhance motivationin rats. Here, HSV- ${Delta}$ FosB was infused only after instrumentaltraining had been completed, eliminating any potential influenceof ${Delta}$ FosB overexpression during training on the subsequent progressiveratio test. A new group of rats were trained, as before, anddivided into balanced experimental groups based on their performanceon the final days of training. Animals subsequently receivedbilateral infusions of HSV- ${Delta}$ FosB or HSV-LacZ into the NAc coreand were tested on progressive ratio responding after 5 d ofoverexpression. Statistical analysis revealed a significantgene expression by lever interaction (F_(1,12) = 14.91; p $≤$ 0.01)(Fig. 7A). Rats infused with HSV- ${Delta}$ FosB made more active responses(p $≤$ 0.01) compared with those infused with HSV-LacZ, whereasresponding on the inactive lever was not affected. Consistentwith this increase, rats infused with HSV- ${Delta}$ FosB also had a higherbreak point (F_(1,12) = 18.849; p $≤$ 0.001) (Fig. 7B) than animalsinfused with HSV-LacZ. There was no effect of ${Delta}$ FosB on baselinelocomotor activity tested 1 h before the progressive ratio test(supplemental Fig. 4A, available at www.jneurosci.org as supplemental material).There were also no differences in body weight on the day ofprogressive ratio testing (supplemental Fig. 4B, available atwww.jneurosci.org as supplemental material). These findingssupport our observations with transgenic ${Delta}$ FosB-overexpressingmice, and indicate that selective overexpression of ${Delta}$ FosB inthe NAc is sufficient to enhance food-associated motivation.

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Figure 7. Effect of infusions of HSV- ${Delta}$ FosB 5 d before testing on instrumental responding on a progressive ratio schedule of reinforcement. A, Lever responses. B, Break point. Data are represented as means ± SEM. ***p < 0.001; **p < 0.01.

   Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The present study demonstrates that overexpression of ${Delta}$ FosB withinthe NAc enhances food-reinforced instrumental behavior. Previousexposure to cocaine, amphetamine, MDMA, or nicotine enhancedproduced a lasting increase in subsequent instrumental performance.These drug exposures also increased food-motivated behaviorunder a progressive ratio schedule of reinforcement. These effectsof previous drug exposure were mimicked by restricted overexpressionof ${Delta}$ FosB in the striatum, using inducible bitransgenic (NSE-tTAx TetOP- ${Delta}$ FosB) mice or using a novel viral vector to express ${Delta}$ FosB selectively in the NAc. Notably, overexpression of ${Delta}$ FosBin the NAc core, after instrumental responding had already beenacquired, enhanced motivation for food under the progressiveratio schedule. Together, our findings identify ${Delta}$ FosB in theNAc core as a potential mediator of drug-induced neuroadaptationsthat can promote instrumental behavior, extending the role forthis transcription factor to include processes with relevanceto motivational influences on the performance of food-reinforcedbehavior. They also raise the possibility that conditions thatinduce ${Delta}$ FosB expression in the NAc may influence the motivationalproperties of both natural and drug reinforcers.
${Delta}$ FosB accumulates in dynorphin-expressing medium spiny neuronsof both the NAc and dorsal striatum after chronic, but not acute,exposure to drugs of abuse. This regional pattern of expressionis reproduced in the inducible bitransgenic ${Delta}$ FosB-overexpressingmice used here. In these mice, elevated striatal levels of ${Delta}$ FosBincrease the animals' sensitivity to cocaine and morphine asmeasured by conditioned place preference (Kelz et al., 1999;Zachariou et al., 2006). It also augments progressive ratioresponding for cocaine suggesting that motivation to self-administercocaine is enhanced by striatal ${Delta}$ FosB overexpression (Colby etal., 2003). Here, we found that striatal ${Delta}$ FosB overexpressionin these mice also increased progressive ratio responding fora food reinforcer and that these effects were reproduced byrestricted viral-mediated overexpression of ${Delta}$ FosB in the NAccore in rat. Our data suggest that ${Delta}$ FosB may act as a transcriptionalmodulator of motivation for primary reinforcers, be they food,drugs, or perhaps exercise, an idea consistent with preliminaryobservations that striatal expression of ${Delta}$ FosB is increased afterchronic wheel running or sucrose drinking (McClung et al., 2004).These data suggest that NAc overexpression of ${Delta}$ FosB can enhancethe motivational impact of both natural and drug reinforcers.
Subregions of the NAc have been argued to differentially mediatethe influence of pavlovian or instrumental incentive processeson instrumental performance (Corbit et al., 2001; de Borchgraveet al., 2002), whereas more general motivational influenceson instrumental performance may be encoded by other regionssuch as the central nucleus of the amygdala (Corbit and Balleine,2005). The NAc core has, however, also been proposed to be acritical site for acquisition of goal-directed instrumentallearning (Smith-Roe and Kelley, 2000; Baldwin et al., 2002a,b;Kelley, 2004). We show equivalent effects of previous drug exposuresand transgenic striatal ${Delta}$ FosB overexpression on enhancing instrumentalbehavior. Infusions of HSV- ${Delta}$ FosB restricted to the NAc core alsoincreased food-reinforced instrumental responding. Althoughthese experiments do not exclude a contribution of the dorsalstriatum in these behaviors, they strongly suggest that ${Delta}$ FosB-inducedalterations in gene expression within the NAc are sufficientto increase food-motivated responding. Because progressive ratioresponding was also enhanced when ${Delta}$ FosB was expressed after stableinstrumental performance had previously been achieved, a rolefor motivational influences on instrumental behavior seems likely.The possibility that our manipulations also affect instrumentallearning processes can, however, not be completely excluded.In support of our conclusions, the increase in instrumentalperformance observed after previous oral cocaine exposure (Mileset al., 2004) has been argued to involve motivational alterationsconsistent with the ability of chronic nicotine treatment toincrease progressive ratio responding in mice (Brunzell et al.,2006). Furthermore, dopamine transporter knock-out mice, inwhich extracellular dopamine levels are increased, display bothenhanced ${Delta}$ FosB immunoreactivity and food-reinforced motivation,but not altered learning (Cagniard et al., 2006). Moreover,we found that overexpression of striatal ${Delta}$ FosB in mice did notaffect performance when food was "devalued" by prefeeding. Thesedata indicate that animals were sensitive to the motivationalvalue of the reinforcer and that responding was goal directed.
Previous repeated drug exposure can also enhance behavioralcontrol exerted by conditioned stimuli associated with naturalreinforcers, measured by pavlovian approach (Harmer and Phillips,1998; Taylor and Jentsch, 2001; Olausson et al., 2003), conditionedreinforcement (Taylor and Horger, 1999; Olausson et al., 2004),and pavlovian-to-instrumental transfer (Wyvell and Berridge,2001). There is now compelling evidence that the NAc core, asopposed to the shell, is involved in the control of drug-motivatedbehavior by pavlovian conditioned stimuli (Parkinson et al.,1999, 2002; Hall et al., 2001; Dalley et al., 2002; Ito et al.,2004). Our results may suggest that drug-induced induction of ${Delta}$ FosB in the NAc may be one mechanism by which behavioral controlis enhanced in these procedures. It is also possible that pavlovianconditioned stimuli, acting as conditioned reinforcers, contributeto the present behavioral effects. Enhanced control over behaviorby such conditioned stimuli mediated by increases in striatal ${Delta}$ FosB may also contribute to the effect of the protein on drug-inducedconditioned place preference (Kelz et al., 1999; Zachariou etal., 2006) and progressive ratio responding for cocaine (Colbyet al., 2003). Alterations in motivational processes have beenhypothesized to contribute to the development and the maintenanceof addictive behavior (Robinson and Berridge, 1993; Jentschand Taylor, 1999; Robbins and Everitt, 1999; Nestler, 2004).The present data are also consistent with other theories thatemphasize multiple instrumental and pavlovian processes in addictivebehavior (Everitt and Robbins, 2005). Additional work is nowneeded to define the role of drug- and ${Delta}$ FosB-induced neuroadaptationsin NAc and other limbic-striatal subregions with respect tothe specific associative or motivational factors that may facilitateinstrumental performance and contribute to compulsive behavior.
Although the precise molecular mechanisms by which changes withinthe NAc influence behavior motivated by primary or conditionedreinforcers are not known (Kelley and Berridge, 2002), the GABAergicmedium spiny neurons of the NAc are considered a critical substratefor drug- and experience-dependent plasticity. Here, dopaminergicinput from the ventral tegmental area and glutamatergic inputfrom corticolimbic afferents converge onto common dendritesand dendritic spines (Sesack and Pickel, 1990; Smith and Bolam,1990). Chronic psychostimulant exposure increases the densityof such spines on neurons in the NAc shell and core (Robinsonand Kolb, 1999; Robinson et al., 2001; Li et al., 2003, 2004).Recently, the induction of behavioral sensitization was associatedspecifically with an increase in dendritic spines within theNAc core (Li et al., 2004). Notably, cocaine-induced increasesin spine density persist only in D₁-positive neurons that coexpress ${Delta}$ FosB (Robinson and Kolb, 1999; Lee et al., 2006). ${Delta}$ FosB in theNAc core may thus contribute to lasting synaptic plasticitythat could impact on instrumental behavior. Indeed, a criticalrole for dopamine-glutamate neurotransmission (Smith-Roe andKelley, 2000), protein kinase A activity (Baldwin et al., 2002a),and de novo protein synthesis (Hernandez et al., 2002) withinthe NAc core on instrumental performance have previously beenreported. We now identify ${Delta}$ FosB as a transcription factor thatcan persistently enhance food-reinforced responding when overexpressedin the NAc core. The specific genes or proteins involved inthese effects remain to be precisely defined. ${Delta}$ FosB regulatesthe expression of multiple proteins in the NAc involved in neuroplasticity(McClung and Nestler, 2003). A recent microarray analysis characterizedgene expression patterns in the NAc of the bitransgenic miceexpressing ${Delta}$ FosB used here, and identified a subset of genesthat were regulated by relatively short-term expression of ${Delta}$ FosB(McClung and Nestler, 2003). BDNF was one such gene, and BDNFin this neural circuit is known to enhance responding for drug-and food-associated cues (Horger et al., 1999; Grimm et al.,2003; Lu et al., 2004). An additional gene of interest is cyclin-dependentkinase 5 (Bibb et al., 2001), which is also induced by ${Delta}$ FosB,and can regulate both the cocaine-induced structural plasticity(Norrholm et al., 2003) and motivation measured by progressiveratio responding for natural or drug reinforcers (J. R. Taylor,unpublished observations). Still additional candidates are theGluR2 subunit of AMPA glutamate receptors (Kelz et al., 1999)and the transcription factor NF ${kappa}$ B (nuclear factor ${kappa}$ B) (Ang etal., 2001). It would be important to evaluate these and otherregulated proteins in NAc subregions as candidates for mediatingthe behavioral effects of ${Delta}$ FosB on instrumental performance andmotivation.
The present series of experiments provides evidence that overexpressionof ${Delta}$ FosB within the NAc can enhance food-motivated behavior andthereby regulate instrumental performance, as has previouslybeen shown for drug rewards. These data provide new evidencethat ${Delta}$ FosB may act as a general molecular switch associated withenhancements in the motivational aspects of reinforcers on goal-directedbehavior. Our findings raise the possibility that inductionof NAc ${Delta}$ FosB by, for example, addictive drugs, stress, or perhapshighly rewarding foods, may be a critical mechanism by whichdysfunctional motivational states result in psychiatric disordersassociated with compulsive behavior.

   Footnotes

Received March 15, 2006; revised June 23, 2006; accepted Aug. 2, 2006.
This work was supported by grants from the National Instituteon Drug Abuse, the National Institute of Mental Health, andthe National Institute of Alcohol Abuse and Alcoholism. We gratefullyacknowledge the valuable assistance of Dilja Krueger, Drew Kiraly,Dr. Ralph DiLeone, Robert Sears, and Dr. Jonathan Hommel atthe Department of Psychiatry, Yale University. We are also gratefulto Dr. Jennifer Quinn and Dr. Paul Hitchcott for providing helpfulcomments on this manuscript.
Correspondence should be addressed to Jane R. Taylor, Department of Psychiatry, Division of Molecular Psychiatry, Yale University School of Medicine, Ribicoff Research Facilities, Connecticut Mental Health Center, 34 Park Street, New Haven, CT 06508. Email: jane.taylor{at}yale.edu
Copyright © 2006 Society for Neuroscience 0270-6474/06/269196-09$15.00/0

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