Environmental Novelty Differentially Affects c-fos mRNA Expression Induced by Amphetamine or Cocaine in Subregions of the Bed Nucleus of the Stria Terminalis and Amygdala

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The Journal of Neuroscience, January 15, 2001, 21(2):732-740

Environmental Novelty Differentially Affects c-fos mRNA Expression Induced by Amphetamine or Cocaine in Subregions of the Bed Nucleus of the Stria Terminalis and Amygdala
Heidi E. W. Day¹^,³, Aldo Badiani²^,⁴, Jason M. Uslaner², Matthew M. Oates², Nicole M. Vittoz², Terry E. Robinson², Stanley J. Watson Jr¹, and Huda Akil¹
¹ Mental Health Research Institute and ² Psychology Department, University of Michigan, Ann Arbor, Michigan 48109, ³ Psychology Department, University of Colorado, Boulder, Colorado 80309, and ⁴ Department of Human Physiology and Pharmacology, University of Rome "La Sapienza", 00185 Rome, Italy

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The environmental context in which amphetamine or cocaine are administered modulates both their acute psychomotor activatingeffects and their ability to induce sensitization. Here we reportthat environmental context differentially affects patterns ofamphetamine- and cocaine-induced c-fos mRNA expression in thebed nucleus of the stria terminalis (BST) and amygdala of malerats.
In the medial amygdala and medial posterior BST, exposure to novelty resulted in a marked increase in c-fos mRNA. Amphetaminegiven at home did not induce c-fos mRNA, and when given in thenovel environment, did not increase levels beyond that observedfor novelty alone. In the basolateral and lateral amygdala, amphetamineor cocaine at home or exposure to novelty induced c-fos mRNA.When amphetamine or cocaine was given in a novel environment thec-fos mRNA response was significantly enhanced. In the centralnucleus of the amygdala (CEA) and oval subnucleus of the BST (BSTov),amphetamine administration at home produced a robust increasein c-fos mRNA expression, whereas exposure to novelty had littleeffect. In contrast to other brain regions examined, the c-fosmRNA response to amphetamine in a novel versus home environmentwas significantly smaller. In both "home" and "novel" amphetaminegroups, c-fos mRNA in the BSTov and CEA was predominantly expressedin enkephalin-containing cells; coexpression with corticotropin-releasinghormone wasrare.
These data suggest that the context in which psychostimulants are given powerfully and differentially alters the responseof limbic structures that have been functionally implicated indrug reinforcement and emotionalbehaviors.

Key words: amphetamine; cocaine; novelty; environment; c-fos; amygdala; bed nucleus of the stria terminalis; dopamine

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The behavioral and subjective effects of addictive drugs, such as amphetamine or cocaine, are powerfully modulated by thepsychological state of the organism and the context in which drugsare taken (Falk and Feingold, 1987). This is apparent even usinga relatively simple animal model, in which the same dose of drugis administered to two groups of rats in physically identicalenvironments. For one group, the environment is the home cage,whereas for the other group, the environment is completely novel.In this situation, both the acute psychomotor activating effectsand the propensity of these effects to sensitize are greater whenpsychostimulants are given in association with environmental novelty(Badiani et al., 1995a,b; Crombag et al., 1996).

The neurobiological mechanisms by which the pharmacological effects of psychostimulants interact with environmental contextare not clear. Environmental context has no effect on plasma orstriatal levels of amphetamine (Badiani et al., 1997), suggestingthat pharmacokinetic factors are not involved. The primary neuropharmacologicaleffect of psychostimulants is to increase dopamine (DA) effluxin the caudate putamen (CP) and nucleus accumbens (ACB) (Wiseand Bozarth, 1987). However, exposure to a novel environment doesnot alter amphetamine-induced DA release in these areas (Badianiet al., 1998, 2000), suggesting that another mechanism isinvolved.

In an attempt to delineate the neural circuitry potentially engaged by this interaction, we have investigated the expressionof c-fos mRNA after an intraperitoneal injection of amphetamineor saline in a home versus novel environment. We have previouslyreported that in a number of forebrain regions, including theCP and ACB, exposure to novelty enhances amphetamine-induced c-fosmRNA expression (Badiani et al., 1998). We also found, using adual in situ hybridization (ISH) technique to study amphetamine-inducedc-fos mRNA expression in D1 versus D2 DA receptor mRNA containingcells of the striatum, that the combination of amphetamine andnovelty not only produced greater c-fos mRNA expression, relativeto amphetamine or novelty alone, but recruited additional neuralcircuitry (Badiani et al., 1999).

However, evidence suggests the involvement of structures such as the extended amygdala in mediating the behavioral effectsof psychostimulants (Alheid and Heimer, 1988). These limbic regionsare thought to be important in stress and emotional responses,and thus are potential sites where psychostimulant drugs and environmentalstimuli may interact. Previous studies have indicated that exposureto novelty (Emmert and Herman, 1999) or acute administration ofpsychostimulants (Umino et al., 1995; Engber et al., 1998) inducesFos expression in distinct regions of the amygdala. In the currentstudy, we have used semiquantitative ISH to compare the effectof amphetamine, cocaine, or saline administration in a home versusnovel environment on c-fos mRNA expression, in the amygdala andbed nucleus of the stria terminalis (BST) of male rats. The dataindicate that the ability of amphetamine or cocaine to engagedifferent subregions of the amygdala and BST is powerfully anddifferentially modulated by the context in which they aregiven.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1
Details of the experimental protocol have been described previously (Badiani et al., 1998). Briefly, male Sprague Dawley rats(Harlan Sprague Dawley, Indianapolis, IN), weighing 200-225 gmat the time of arrival were housed in standard stainless steelcages in a temperature- and humidity-controlled environment. Ratswere maintained on a 14:10 hr light/dark cycle (lights on 6:00A.M.) and were allowed ad libitum access to food and water throughoutthe experiment. Animals were acclimated to these housing conditionsfor 1 week before any experimentalmanipulation.
6-Hydroxydopamine lesion. All rats received a unilateral 6-hydroxydopamine (6-OHDA) lesion of the mesostriatal dopamine system,with left and right sides counterbalanced, as previously described(Robinson, 1984). This provided a way to quantify the psychomotor-activatingeffects of amphetamine by measuring amphetamine-induced rotationalbehavior. To protect noradrenergic terminals, desipramine hydrochloride(15 mg/kg, i.p.) was administered before induction of anesthesia.After a 10 d recovery period, apomorphine (0.05 mg/kg, s.c.) wasadministered to assess the development of DA receptor supersensitivity,as indicated by contraversive rotational behavior. Animals thatmade less than eight full rotations in a 2 min test period wereexcluded from thestudy.
Administration of amphetamine. Four days after the apomorphine screen, three groups of rats were housed in opaque plasticcylindrical cages. After 7 d of acclimation to the new home cageenvironment, animals were given an injection of saline vehicleintraperitoneally (home-saline; n = 9), 2.0 mg · kg¹ · ml¹ D-amphetamine intraperitoneally (home-amphetamine; n = 12) orremained untreated (untreated; n = 7). Two additional groups ofrats, which had been housed continuously in stainless steel hangingcages, were transported from the colony room to the cylindricalcages, which for them was a completely novel environment. Theywere then immediately given an injection of saline intraperitoneally(novel-saline; n = 9) or 2.0. mg · kg¹ · ml¹ D-amphetamine intraperitoneally (novel-amphetamine; n = 11).All injections were given between 12:00 and 1:00 P.M. Rotationalbehavior was videotaped remotely, and the number of full rotationsmade by the animal during the session were subsequently analyzedby an observer blind to the experimental group. Animals were killedby rapid decapitation 50 min after injection. Untreated rats werekilled at this time also. Brains were removed and frozen in isopentanecooled to $-$ 40 to $-$ 50°C and stored at $-$ 80°C. Coronal sections (10µm) were cut on a cryostat (Bright, Huntingdon, UK) at 200 µmintervals through the BST and amygdala and mounted onto polylysine-coatedslides. Sections were air-dried and stored at $-$ 80°C until processingfor in situhybridization.

Experiment 2
For dual in situ hybridization experiments, the above protocol was repeated, using two groups of rats only: home-amphetamine(n = 8) and novel-amphetamine (n =8).

Experiment 3
Because the 6-OHDA lesion sustained in the first two experiments could potentially influence the c-fos mRNA expression, theexperiment was repeated, with minor modifications, in neurologicallyintact animals. In addition, the effect of cocaine on the amygdalac-fos mRNA response was investigated. Fifty-six male Sprague Dawleyrats (Harlan) weighing 200-250 gm were initially housed in stainlesssteel hanging cages in a temperature- and humidity-controlledenvironment. The rats were kept on a 14:10 hr light/dark cycle(lights on at 7:00 A.M.) and were given food and water ad libitum.The animals were kept in the colony room for 7 d before any experimentalmanipulation. Rats were then assigned to seven groups. Four groupswere housed in 16 × 10 × 8 inch white plastic tubs with groundcorn cob bedding on the floor. Ten days later at 12:00 P.M., therats either received saline (1 ml/kg, i.p.; home-saline; n = 5),amphetamine (1.5 mg · kg¹ · ml¹, i.p.; home-amphetamine; n = 9), cocaine HCl (15 mg · kg¹ · ml¹, i.p.; home-cocaine; n = 9) in these chambers or were left undisturbed(untreated; n = 4). The three remaining groups were transportedfrom the stainless steel hanging cages where they were housed,placed into the white plastic cages described above, which forthem was a novel environment, and immediately were given eitheran intraperitoneal injection of saline (novel-saline; n = 9),amphetamine (1.5 mg/kg; novel-amphetamine; n = 11), or cocaine(15 mg/kg; novel-cocaine; n = 9). Locomotor activity was videotapedremotely, and the number of crossovers (defined as one completetraversal of the long side of the test cage) made by the animalduring the session was subsequently counted by an observer blindto the experimental group. Fifty minutes after treatment the ratswere decapitated, and brains were removed and frozen in isopentane( $-$ 40 to $-$ 50°C) and stored at $-$ 80°C. Sections (10 µm) were cutat 200 µm intervals through the amygdala, mounted on polylysine-coatedslides, and stored at $-$ 80°C until processing for in situhybridization.
In situ hybridization for c-fos mRNA. The method for in situ hybridization was as previously described (Day and Akil, 1996).Briefly, a cRNA probe complementary to c-fos (680 mer; courtesyof Dr. T. Curran, St. Jude Children's Research Hospital, Memphis,TN) was generated and labeled with [³⁵S]CTP and [³⁵S]UTP (AmershamPharmaciaBiotech, Piscataway, NJ), using standardtranscription methods. Brain sections were hybridized with theprobe overnight, and the next day they were treated with RNaseA (200 µg/ml) for 1 hr at 37°C and washed to a final stringencyof 0.1× SSC at 65°C for 1 hr. Sections were exposed to x-ray film(Biomax-MR; Eastman Kodak, Rochester, NY) for 5 d before dippingin photographic emulsion (NTB2; Eastman Kodak) sections were storedin light-tight boxes for 3 weeks at 4°C before developing (D19;Eastman Kodak). Sections were lightly stained with cresyl violet,dehydrated, and coverslipped with a xylene-based mounting medium(Permount) for qualitative microscopicanalysis.
Semiquantitative c-fos mRNA analysis. Levels of c-fos mRNA were analyzed by computer-assisted optical densitometry. All sectionsfrom the BST were processed in a single in situ experiment. Similarly,all sections from the amygdala of an individual experiment wereprocessed in a single ISH experiment. However, because the BSTand amygdala sections were not processed together, and becausesections from experiments 1, 2, and 3 were processed separately,they should not be compared quantitatively. Brain section imagesfrom in situ hybridization experiments were captured digitally(CCD camera, model XC-77; Sony, Tokyo, Japan), and the relativeoptical density of the x-ray film was determined for each brainregion using NIH Image version 1.61 for Macintosh computer. Amacro was written (Dr. Serge Campeau, University of Colorado)that enabled signal above background to be automatically determined.For each section, a background sample was taken over an area ofwhite matter, and the signal threshold was calculated as meangray value of background +3.5 SD. The section was automaticallydensity-sliced at this value, so that only pixels with gray valuesexceeding these criteria were included in the analysis. Resultsare expressed as mean integrated density, which reflects boththe signal intensity and the number of pixels above assigned background(mean signal above background × number of pixels above background).Care was taken to ensure that equivalent areas were analyzed betweenanimals.
Dual in situ hybridization. The method used for dual in situ hybridization has been described previously (Day et al., 1999).Briefly, cRNA probes complementary to c-fos, corticotropin-releasinghormone (CRH) (770 mer; courtesy of Dr. R. Thompson, Universityof Michigan), or enkephalin mRNA (693 mer; courtesy of Dr. J.Douglass, Amgen, Thousand Oaks, CA) were generated and labeledwith [³⁵S]CTP and [³⁵S]UTP or digoxigenin-UTP (dig-UTP; Boehringer Mannheim, Indianapolis,IN) using standard transcription methods. Brain sections throughthe oval subnucleus of the BST (BSTov) and central nucleus ofthe amygdala (CEA) (from experiment 2) were hybridized overnightwith either dig-c-fos and [³⁵S]enkephalin or dig-c-fos and [³⁵S]CRH probes. The next day, sections were treated with RNase A(200 µg/ml) for 1 hr at 37°C and washed to a final stringencyof 0.1× SSC at 65°C for 1 hr. Sections were then processed forvisualization of the digoxigenin-labeled probe. Briefly, sectionswere incubated overnight with an antibody against digoxigeninand conjugated to alkaline phosphatase (sheep anti-dig-AP, Fabfragments; Boehringer Mannheim), diluted 1:20,000. After extensivewashing, sections underwent a color reaction by addition of 0.45%nitro blue tetrazolium chloride (Boehringer Mannheim) and 0.35%5-bromo-4-chloro-3-indoylphosphate 4-toluidine salt (BoehringerMannheim). After completion of the color reaction (~18 hr), sectionswere rinsed and stripped of antibody by incubating with 0.1 Mglycine and 0.5% Triton X-100, pH 2.2, for 10 min. Finally, sectionswere fixed in 2.5% glutaraldehyde for 1 hr. These last steps werefound to help prevent the increase in background after processingfor radioactive signal. After exposure to x-ray film (1 d for[³⁵S]enkephalin and 5 d for [³⁵S]CRH), sections were dipped in liquid emulsion (Ilford KD-5;Polysciences, Warrington, PA) and stored in light-tight boxesat 4°C for 3 d ([³⁵S]enkephalin) or 1 month ([³⁵S]CRH). After this time sections were developed (Kodak D-19),dehydrated, and coverslipped in a xylene-based mounting medium(Permount; Fisher Scientific, Houston, TX). The cellular distributionwas determined using a Leica (Nussloch, Germany; Leitz DMR) microscope.The nonradioactive probe was visualized under bright field asa blue-purple precipitate, whereas the radioactive probe was visualizedunder dark field by silver grain distribution. Sections throughthe BSTov and CEA were analyzed to determine the extent of colocalization.Cells were counted with the aid of an eyepiece grid. For eachanimal, between two and four sections for the BSTov and four toeight sections for the CEA were analyzed bilaterally. At leastfive animals per group were analyzed for each probe combination.No attempt was made to determine absolute cell counts. Rather,we aimed to analyze an adequate number of cells to estimate thepercentage of double-labeledneurons.
Statistical analysis. Rotational data were analyzed by one-way ANOVA (experiment 1: group, 5 levels; experiment 2: group,2 levels), followed by Fisher's protected least significant difference(PLSD) tests. For crossover data (experiment 3), because theywere not statistically different, untreated and home-saline groupswere pooled, and data were analyzed by two-way ANOVA (environmentand drug treatment) followed by Fisher's PLSD tests. Group differencesin c-fos mRNA levels from experiment 1 were analyzed by three-wayANOVA, including lesion type (lesion or intact), environment (homeor novel), and injection (saline or amphetamine). Because therewere interaction effects between environment and injection, butno effects of lesion on c-fos mRNA expression, the data from thelesion and intact conditions were pooled. These data, and thosefrom experiments 2 and 3, were analyzed by a one-way ANOVA (group,two, five, or seven levels as appropriate for brain area and experiment)followed by Fisher's PLSDtests.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1

Behavior
Consistent with previous observations, untreated or saline-treated animals in either home or novel context showed no significantrotational behavior. Animals treated with amphetamine (2 mg/kg,i.p.) in the home environment demonstrated a significant increasein rotational behavior, which was further increased in animalstreated with the same dose of amphetamine in a novel environment(Table 1).


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Table 1. Behavioral data for experiments 1-3

c-fos mRNA expression
For all regions, the levels of c-fos mRNA were quantified separately for the lesioned and intact sides, but there was no effectof the lesion in any of the groups, in any of the regions studied.Hence, data are shown as the mean of lesion and intact sides foreach animal. Environmental novelty and amphetamine administration,alone or in combination, had differential effects on the patternsof c-fos mRNA expression in different subnuclei of the BST andamygdala.
The medial nucleus of the amygdala (MEA) and medial posterior nucleus of the BST (BSTmp) have been associated under the extendedamygdala concept, as proposed by Alheid and Heimer (1988). Inthese regions, untreated animals and those injected with eithersaline or amphetamine in the home environment expressed very lowlevels of c-fos mRNA, with no significant differences betweengroups (Fig. 1A,B). Exposure to novelty, whether associated witha saline injection (p < 0.0001 vs home-saline group for both MEAand BSTmp) or amphetamine injection (p < 0.0001 vs home-amphetaminegroup for both MEA and BSTmp), increased the levels of c-fos mRNAto a similar extent.

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Figure 1. Expression of c-fos mRNA in MEA (A), BSTmp (B), and BLA and LA (C) of 6-OHDA-lesioned rats 50 min after amphetamine (2 mg/kg, i.p.) or saline administration in a home or novel environment (experiment 1). Values represent the mean integrated density (see Materials and Methods for definition) ± SEM. *p < 0.05 with respect to home-saline group; $dagger$ p < 0.001 with respect to novel-saline group; $Dagger$ p < 0.001 with respect to home-amphetamine group.

In the basolateral (BLA) and lateral (LA) nuclei of the amygdala, untreated and home-saline animals expressed very littlec-fos mRNA, with no significant difference between the groups(Fig. 1C). Mere exposure to novelty (in the absence of amphetamine)increased the levels of c-fos mRNA in these regions (p < 0.01vs home-saline group). Amphetamine administration in the homeenvironment also increased the levels of c-fos mRNA (p < 0.05vs home-saline group), to a similar extent as observed with noveltyalone. The combination of novelty plus amphetamine increased thelevels of c-fos mRNA further (p < 0.0001 vs home-saline group;p < 0.001 vs novel-saline group; p < 0.0001 vs home-amphetaminegroup), to a level that was approximately additive with respectto novel-saline and home-amphetamine groups. Unfortunately wewere unable to analyze c-fos mRNA expression in individual nucleibecause sections were taken at relatively rostral levels, so thatthe level of the lateral nucleus in particular was fairly anterior.However, it appeared that c-fos mRNA expression was greater inthe medial aspect of eachnucleus.
A most unusual pattern of c-fos mRNA expression was observed in the CEA (Figs. 2A, 3) and BSTov (Figs. 2B, 4). These nucleihave been associated anatomically within the central extendedamygdala. In these regions, expression of c-fos mRNA was extremelylow in the untreated and home-saline groups, with no significantdifference between groups. Exposure to novelty alone resultedin a trend toward greater expression of c-fos mRNA in both theCEA and BSTov, but these effects were not statistically significant.Amphetamine administered in the home environment resulted in arobust increase in c-fos mRNA levels in both nuclei (p < 0.0001vs home-saline group for both BSTov and CEA). In contrast to theusual additive effect of novelty and amphetamine on c-fos mRNAobserved in most other brain regions (Badiani et al., 1998), amphetamineadministered in the novel environment resulted in a smaller inductionof c-fos mRNA expression in the BSTov and CEA, as compared withthe home-amphetamine group (BSTov, p < 0.01 vs novel-saline andhome-amphetamine groups; CEA, p < 0.001 vs novel-saline group;p < 0.0001 vs home-amphetamine group). In both home- and novel-amphetaminegroups, expression within the CEA was essentially confined tothe lateral division (CEAl), and was highest ventrally towardthe caudal extent of the nucleus.

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Figure 2. Expression of c-fos mRNA in CEA (A) and BSTov (B) of 6-OHDA lesioned rats 50 min after amphetamine (2 mg/kg, i.p.) or saline administration in a home or novel environment (experiments 1 and 2). Note that in experiment 2, only home-amphetamine and novel-amphetamine groups were run. Values represent the mean integrated density (see Materials and Methods for definition) ± SEM. *p < 0.001 with respect to home-saline group; $dagger$ p < 0.01 with respect to novel-saline group; $Dagger$ p < 0.01 with respect to home-amphetamine group.

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Figure 3. Schematic diagram (A) and photomicrographs (B-F) showing c-fos mRNA expression in the CEA, 50 min after amphetamine (amphet; 2 mg/kg, i.p.; E, F) or saline (C, D) administration in a home (B, C, E) or novel (D, F) environment (experiment 1). opt, Optic tract. Scale bar, 1 mm.

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Figure 4. Schematic diagram (A) and photomicrographs (B-F) showing c-fos mRNA expression in the BSTov, 50 min after amphetamine (amphet; 2 mg/kg, i.p.; E, F) or saline (C, D) administration in a home (B, C, E) or novel (D, F) environment (experiment 1). ac, Anterior commissure; BSTju, juxtacapsular nucleus of the BST; ic, internal capsule; LV, lateral ventricle. Scale bar, 300 µm.

Experiment 2

Animals receiving amphetamine in the novel environment exhibited significantly greater rotational behavior than those receivingamphetamine at home (Table 1). As was observed in experiment1, c-fos mRNA expression in the CEA (Fig. 2A) and BSTov (Fig.2B) was significantly greater in animals that had received amphetaminein the home environment, compared with those experiencing amphetaminein a novelenvironment.

Previous studies have shown the existence of two distinct populations of cells within the BSTov and CEAl (Day et al., 1999).One population expresses CRH mRNA and another enkephalin mRNA,with very little overlap between these two cell populations. Inthe current study, dual in situ hybridization experiments revealedthat within the BSTov and CEAl, amphetamine-induced c-fos mRNAexpression was rarely colocalized with CRH mRNA (Table 2, Fig.5A), with <2% of c-fos mRNA-positive cells expressing CRH mRNAin either brain region. In contrast, the majority of cells expressingc-fos mRNA also expressed enkephalin mRNA (Table 2, Fig. 5B).The percentage of c-fos mRNA-expressing cells that expressed enkephalinmRNA varied from ~80-85% for the BSTov to 90% for the CEAl. Thispattern of expression was independent of the environmental contextin which the amphetamine was administered, with a similar proportionof double-labeled cells observed for each group.


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Table 2. Colocalization of c-fos mRNA in CRH or enkephalin mRNA containing cells of the BSTov or CEA (experiment 2)

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Figure 5. Photomicrographs showing dual in situ hybridization of c-fos mRNA (digoxigenin-labeled probe, dark gray cells) with CRH (A) or enkephalin (B) mRNA (³⁵S-labeled probe, clusters of white grains) in the central nucleus of the amygdala, 50 min after amphetamine administration (2 mg/kg, i.p.) in a home environment. Open arrows, Cells labeled for c-fos mRNA only; white arrows, cells labeled for CRH mRNA only; black arrows, cells labeled for c-fos and enkephalin mRNA. Scale bar, 50 µm.

Experiment 3

Behavior
In neurologically intact rats, locomotor activity was very low, as measured by the number of crossovers during the session,in animals that were untreated or received saline at home (Table1). In contrast to rotational behavior observed in experiment1, animals that received a saline injection in the novel environmentexhibited significantly higher locomotor activity as comparedwith the home-saline group (p < 0.0001). Amphetamine administeredin the home environment also resulted in significantly elevatedlocomotor activity, compared with home-saline animals. When amphetaminewas administered in the novel environment, locomotor activitywas further enhanced (p < 0.05 compared with novel-saline group;p < 0.01 compared with home-amphetamine group.) Cocaine administeredin the home environment did not alter locomotor activity, butwhen administered in the novel environment, locomotor activitywas significantly increased (p < 0.05 compared with novel-salinegroup; p < 0.01 compared with home-cocaine group.)

c-fos mRNA expression
In the MEA of neurologically intact rats, amphetamine administration in the home versus novel environment resulted in a verysimilar pattern of c-fos mRNA expression to that observed in 6-OHDA-lesionedanimals (Fig. 6A). That is, exposure to novelty, whether associatedwith a saline injection or amphetamine injection, increased thelevels of c-fos mRNA to a similar extent. Furthermore, cocaineadministration in a home versus novel environment resulted inan almost identical pattern of c-fos mRNA expression (Table 3).Animals receiving cocaine in the home environment exhibited verylittle c-fos mRNA in this region, and those receiving cocainein the novel environment expressed c-fos mRNA to a similar extentto the novel-saline group.

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Figure 6. Expression of c-fos mRNA in MEA (A), BLA and LA (B), and CEA (C) of neurologically intact rats 50 min after amphetamine (1.5 mg/kg, i.p.) or saline administration in a home or novel environment (experiment 3). Values represent the mean integrated density (see Materials and Methods for definition) ± SEM. *p < 0.05 with respect to home-saline group; $dagger$ p < 0.05 with respect to novel-saline group; $Dagger$ p < 0.05 with respect to home-amphetamine group.


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Table 3. Relative c-fos mRNA levels (integrated optical density: arbitrary units) in neurologically intact rats, after cocaine (15 mg/kg, i.p.) or saline administration in a home or novel environment (experiment 3)

In the BLA and LA, the pattern of amphetamine-induced c-fos mRNA expression in intact animals was broadly similar to thatobserved previously in unilateral 6-OHDA-lesioned animals (Fig.6B). Both exposure to novelty and amphetamine at home resultedin significant c-fos mRNA expression. Amphetamine given in combinationwith novelty resulted in enhanced c-fos mRNA expression, so thatthe levels were essentially additive. However, in neurologicallyintact rats, c-fos mRNA levels in the novel-saline group weresignificantly higher than in the home-amphetamine group, whereasin rats with a 6-OHDA lesion, these two groups showed a similarc-fos mRNA response. This may be related to the greater behavioralresponse to a novel environment in intact versus 6-OHDA-lesionedanimals (Table 1). The pattern of expression observed after cocainetreatment was very similar to that seen with amphetamine (Table3).
In the CEA, the pattern of amphetamine-induced c-fos mRNA expression in intact animals again was broadly similar to that observedin rats with a unilateral 6-OHDA lesion (Fig. 6C). Novelty aloneelicited a small, but significant increase in c-fos mRNA (p <0.05 compared with home-saline and untreated animals), whereasamphetamine at home elicited a robust response (p < 0.0001 comparedwith home-saline group). When given in association with a novelenvironment, amphetamine elicited a relatively smaller c-fos mRNAresponse (~50%), as compared with the home-amphetamine group (p< 0.05). Animals treated with cocaine in the home environmentalso expressed robust levels of c-fos mRNA (Table 3). Althoughthere was a trend toward decreased c-fos mRNA expression whencocaine was administered in association with novelty, the effectwas not statisticallysignificant.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study presents further evidence supporting the idea that the neural circuitry engaged by amphetamine or cocaine is nota simple function of their direct pharmacological actions, butrather is dependent on the context in which they are experienced.In most brain regions environmental novelty potentiates amphetamine-inducedc-fos mRNA expression (Badiani et al., 1998, 1999), but here wereport that in the CEA novelty inhibits amphetamine-induced c-fosmRNA expression. These data suggest that patterns of psychostimulantdrug-induced gene expression in widespread neural circuits aremodulated in complex ways by the context in which drugs are experienced.This may be related to the ability of environmental context tomodulate both acute drug responsiveness and their ability to promoteneurobehavioralplasticity.

MEA and BSTmp

The pattern of c-fos mRNA expression observed in the MEA and BSTmp was similar to that observed previously in the neocortexand septum (Badiani et al., 1998). Exposure to novelty increasedc-fos mRNA expression, which was not augmented by amphetamineadministration. This may be because exposure to novelty is stressful,as indicated by increased plasma corticosterone (Badiani et al.,1998, their Fig. 13). Indeed, other "processive" stressors (definedas stressors requiring interpretation by higher brain structures;Herman and Cullinan, 1997) increase c-fos mRNA levels in the MEAand medial BST (Cullinan et al., 1995; Kollack-Walker et al.,1997). Given the lack of induction of c-fos mRNA by amphetamineat home or potentiation of novelty-induced c-fos mRNA, it appearsthat the MEA and BSTmp are not involved in the response to amphetamineper se. This is despite the fact that administration of amphetamineis stressful, as determined by elevated plasma corticosterone(Badiani et al., 1998, their Fig. 13), suggesting that these regionsmay respond selectively to processive rather than "systemic" stressors.Furthermore, the lack of cocaine-induced c-fos mRNA in the MEAsuggests that this region is more likely to be involved in stressresponsiveness than in the response to psychostimulants. It seemslikely that the c-fos mRNA expression elicited by the combinationof amphetamine or cocaine and novelty was attributable entirelyto the novelty component, but we cannot exclude the possibilitythat different neuronal populations were activated under theseconditions.

BLA and LA

In the BLA and LA, novelty alone or amphetamine or cocaine at home increased c-fos mRNA expression. When amphetamine or cocainewas given in association with novelty, c-fos mRNA expression wasfurther enhanced. This pattern has been observed in other brainregions, including the CP and ACB core (Badiani et al., 1998).The LA receives significant sensory input (Doron and LeDoux, 1999)and the relatively high c-fos mRNA response to novelty in intactversus lesioned animals may reflect an increase in sensory inputresulting from increased exploration of the cage. The LA projectsheavily to the majority of other amygdaloid nuclei including theBLA (Pitkanen et al., 1995), which has been implicated in theresponse to affective stimuli and in the process of conditionedreinforcement (Everitt et al., 1999). Furthermore, the BLA hasa substantial projection to the ACB shell (Alheid and Heimer,1988), an area thought to be integral in the reinforcing actionsof drugs ofabuse.

There is considerable evidence that DA plays a significant role in modulating BLA activity. For example, DA levels are increasedin the BLA during learning (Hori et al., 1993) and in responseto stressful stimuli (Herman et al., 1982) or to stimuli predictiveof food reward (Harmer and Phillips, 1999). Furthermore, DA modulatesneuronal firing and afferent drive of the BLA and has been suggestedto augment the response to affective sensory stimuli (Rosenkranzand Grace, 1999). Although the present data do not indicate whetherDA is involved in the observed c-fos mRNA response, the DA-releasingproperties of amphetamine and cocaine and the stressful natureof the novel environment are consistent with the possibility ofDA involvement (but see discussion below). The present data suggestthat quantitatively, the effects of novelty and amphetamine orcocaine on c-fos mRNA in the BLA and LA are additive. This raisesthe possibility that the BLA is important in processing the complexinteractions between the effects of drugs of abuse and environmentalcontext. However, the data do not indicate whether the same cellpopulations are engaged by amphetamine or cocaine and environmentalnovelty. Indeed, we have recently shown that in the CP, amphetamineinduces c-fos mRNA expression in cells positive for D2 DA receptormRNA when given in a novel environment, but not when given athome (Badiani et al., 1999), indicating that different neuralcircuitry is involved in the response to amphetamine in differentenvironmentalcontexts.

CEA and BSTov

In the CEA and BSTov, amphetamine at home induced robust c-fos mRNA expression, but significantly lower expression, when givenin a novel environment. This pattern is highly unusual, differingfundamentally from the patterns found in every other brain regionwe have studied to date (Badiani et al., 1998, 1999). Althougha trend toward this pattern was seen in cocaine-treated animals,the difference was not statistically significant. This may bebecause the dose of cocaine used was not optimal, or this patternof expression could be specific for amphetamine. The CEA and BSTovare involved in the central regulation of autonomic functions,including cardiovascular activity (Saper, 1995). Acute amphetamineincreases both blood pressure and heart rate via peripheral mechanisms,and the CNS is thought to inhibit this effect (Simpson, 1975,1976). It is conceivable that the BSTov and CEA c-fos mRNA responseto amphetamine at home reflects this inhibitory output. For animalsexposed to novelty, the increase in heart rate and blood pressureis thought to result from processing of information at a centralrather than peripheral level (Morimoto et al., 1993), and we speculatethat the BSTov and CEAl may be involved in this regulation. Thus,when amphetamine is administered in a novel environment, thereis a smaller c-fos mRNA response, perhaps via active inhibitionof these structures. To our knowledge, the cardiovascular responseto amphetamine administration in a home versus novel environmenthas not been studied, and would be of interest to investigate.In addition, the CEA may play a role in the reinforcing actionsof drugs of abuse (Koob, 1999). Although this study does not addressthe issue of reinforcement, the ability of novelty to inhibitamphetamine-induced c-fos mRNA in the CEA may have important implicationsfor both an animal's acute and subsequent responses to thedrug.

It is not clear which neuronal circuits are involved in the CEA or BSTov c-fos mRNA responses to amphetamine in differentenvironmental contexts. We have previously demonstrated the existenceof two GABAergic neuronal populations in the BSTov and CEA, containingeither enkephalin or CRH mRNA (Day et al., 1999). Amphetamine-inducedc-fos mRNA was highly colocalized with enkephalin, but rarelywith CRH mRNA, regardless of environmental condition. This doesnot imply that identical neuronal pathways were involved in theresponse. It is possible that novelty inhibits the amphetamine-stimulatedneurons that are responsible for induction of c-fos mRNA in theBSTov and CEA. Alternatively, novelty may activate a differentinhibitory pathway that synapses on the same cells of the BSTovand CEA. Furthermore, it must be recognized that the lack of c-fosmRNA expression in CRH-positive cells does not indicate a lackof involvement. Indeed, it has recently been shown that thereare substantial intranuclear connections within the lateral divisionof the CEA (Petrovich and Swanson, 1997; Jolkkonen and Pitkanen,1998), raising the intriguing possibility that enkephalin-containingcells actively inhibit the CRH-containingcells.

Dopaminergic involvement

The extent of dopaminergic involvement in the BST and amygdala c-fos mRNA response to amphetamine in different environmentsremains to be determined. Dopaminergic input is certainly richto these areas (Freedman and Cassell, 1994; Asan, 1998). The extentof DA depletion in the amygdala or BST of animals sustaining a6-OHDA lesion of the medial forebrain bundle is unclear. The lackof effect of the lesion on amphetamine-induced c-fos mRNA in anyof the regions examined suggests that either the DA input to theseareas was not depleted sufficiently or that DA is not necessaryfor the c-fos mRNA response to amphetamine. Interestingly, the6-OHDA lesion did have some effect in these regions. In the sameanimals we observed that CRH and neurotensin mRNAs were significantlydecreased in the BSTov and CEA on the lesioned side (Day et al.,2000). Conversely, the c-fos mRNA response to amphetamine is notrestricted to animals with a 6-OHDA lesion, because a similarpattern of expression was observed in the amygdala of neurologicallyintactrats.

In conclusion, the differential effects of exposure to a novel environment on amphetamine-induced c-fos mRNA expression inthe BST and amygdala lends support to the idea that the neurocircuitryengaged by amphetamine is not only dependent on its pharmacologicalproperties, but also on the context in which it is experienced.The response in these areas is of particular interest given thepotential role that they play in emotional and associative processesinvolved in the reinforcing effects of amphetamine. Taken togetherwith data from previous studies (Badiani et al., 1998, 1999),the differential effects of environmental context on the magnitudeof response and neurons recruited strongly suggest that an animal'sresponse to amphetamine is not simply quantitatively differentunder the two conditions. Rather, we suggest that the contextin which amphetamine is administered qualitatively alters itsneurobiological effects, and therefore the drugexperience.

  FOOTNOTES

Received July 3, 2000; revised Nov. 1, 2000; accepted Nov. 2, 2000.

This work was supported by National Institute of Mental Health Grants PO1MH42251 (H.A., S.J.W.) and DA04294 (T.E.R.). We thankSharon Burke and Michelle M. Ostrander (University of Michigan)for their technical expertise and input and Dr. Serge Campeau(University of Colorado) for valuable discussion andsupport.
Correspondence should be addressed: Heidi E. W. Day at her present address: Psychology Department, Muenzinger Building, P.O.Box 345, Boulder, CO 80309-0345. E-mail: heididay{at}psych.colorado.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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