Abstract
Major precipitating factors for relapse to drug use are stress and exposure to drug-related environmental stimuli. Group II (mGlu2/3) metabotropic glutamate receptors (mGluRs) are densely expressed within circuitries mediating the motivating effects of stress and drug cues and, therefore, may participate in regulating drug-seeking linked to both of these risk factors. Thus, we tested the hypothesis that pharmacological activation of group II mGluRs modifies both stress- and cue-induced ethanol-seeking, using reinstatement models of relapse. In parallel, brain c-fos expression was examined to identify neural substrates for the behavioral effects of group II mGluR activation. The selective mGlu2/3 agonist LY379268 (1R,4R,5S,6R-2-oxa-4-aminobicyclo[3.1.0]hexane-4,6-dicarboxylate) (0.3, 1.0, and 3.0 mg/kg, s.c.) dose dependently blocked the recovery of extinguished ethanol-seeking induced by either footshock stress or ethanol-associated discriminative stimuli. These effects were accompanied by modulation of c-fos expression in the hippocampus, central nucleus of the amygdala, bed nucleus of the stria terminalis, and medial parvocellular paraventricular nucleus of the hypothalamus. The results implicate group II mGluRs as a shared neuropharmacological substrate for ethanol-seeking elicited by both drug cues and stress and identify group II mGluRs as promising treatment targets for relapse prevention.
Introduction
The development of selective ligands for metabotropic glutamate receptors (mGluRs) has provided novel opportunities for investigating the role of glutamate neurotransmission in psychiatric conditions linked to glutamatergic hyperexcitability, including drug addiction and anxiety disorders. Of particular interest in this respect are group II mGluRs (mGlu2/3) because of their abundance in brain regions mediating drug reward and incentive motivation (Ohishi et al., 1993a,b), as well as circuitries regulating anxiety and behavioral responses to stress (Kenny and Markou, 2004; Swanson et al., 2005). Group II mGluRs negatively modulate excitatory glutamate transmission at the presynaptic, perisynaptic, and postsynaptic levels (Schoepp, 2001). Such actions in brain reward and stress systems, including the nucleus accumbens, amygdala, dorsal hippocampus (HIPPO), and ventral tegmental area (VTA) (Kenny and Markou, 2004; Swanson et al., 2005), are likely to be important for the addictive actions of drugs of abuse as well as addiction-relevant actions of stress. Indeed, mGlu2/3 agonists attenuate some forms of drug-seeking behavior (Baptista et al., 2004; Bossert et al., 2004) and modify several neurobehavioral consequences of acute and chronic psychostimulant or opiate administration (Kenny and Markou, 2004). Additionally, these agents exert anxiolytic-like effects in animals and appear effective in the treatment of anxiety disorders (Swanson et al., 2005).
A significant obstacle for the successful treatment of drug addiction is persistent vulnerability to relapse. Major precipitating factors for the resumption of drug use are stress and exposure to drug-related environmental stimuli (O'Brien et al., 1998; Sinha et al., 2000; See, 2002; Weiss, 2005). Considering the “strategic” distribution of group II mGluRs within brain circuitries that control the motivating effects of stress and drug-related stimuli, these receptors may have a pivotal role in drug-seeking behavior linked to these risk factors and offer a potential treatment target for relapse prevention. This hypothesis is tentatively supported by findings that an mGlu2/3 agonist prevents cocaine- and heroin-seeking behavior induced by drug-related contextual stimuli in reinstatement models of relapse (Baptista et al., 2004; Bossert et al., 2004). The purpose of this study was (1) to determine whether group II mGluR activation by a selective mGlu2/3 agonist [LY379268 (1R,4R,5S,6R-2-oxa-4-aminobicyclo[3.1.0]hexane-4,6-dicarboxylate)] attenuates not only cue- but also stress-induced reinstatement of drug-seeking, using ethanol as a representative substance of abuse, and (2) to identify potential neural substrates through which group II mGluR activation modifies the reinstatement of ethanol-seeking by using c-fos neural mapping.
Materials and Methods
Animals.
Male Wistar rats (Charles River, Raleigh, NC) weighing 180–200 g were housed three per cage on a reversed 12 h light/dark cycle with food and water available ad libitum. All procedures were conducted in accordance with the National Institutes of Health Guide for the Care and Use of Laboratory Animals and were approved by the Institutional Animal Care and Use Committee of The Scripps Research Institute.
Drugs.
The mGlu2/3 receptor agonist LY379268 (Lilly Research Laboratories, Indianapolis, IN) was dissolved in sterile water at volumes of 0.3, 1.0, and 3.0 mg/ml. LY379268 [or vehicle (VEH)] was administered subcutaneously 30 min before behavioral tests.
Ethanol self-administration training.
Rats were trained to orally self-administer ethanol in 30 min daily sessions inside sound-attenuated operant conditioning chambers (Med Associates, St. Albans, VT), using a sweet solution fading procedure. Briefly, responses at an active lever were initially reinforced by 0.1 ml of saccharin (0.2% w/v) on a fixed ratio 1 (FR 1) schedule. After acquisition, ethanol (5% w/v) was added to the saccharin solution. Ethanol concentrations then were gradually increased to 10% (w/v) while saccharin was slowly eliminated. A second inactive lever was then introduced at which responses were recorded but had no programmed consequences.
Footshock reinstatement procedure.
Once stable ethanol self-administration was obtained, daily 30 min sessions continued for 4 weeks. Ethanol-reinforced responding was then extinguished in daily 30 min sessions that continued until a criterion (average of less than or equal to six lever presses over 3 d) was reached by a given animal, which required, on average, 14 d. Reinstatement tests began 1 d after the last extinction session. Thirty minutes after LY379268 (0.3, 1.0, and 3.0 mg/kg, s.c.) administration, rats were exposed to 10 min of variable intermittent footshock (0.5 mA; 0.5 s duration; mean intershock interval, 40 s; range, 10–70 s). After footshock, levers were extended and 60 min reinstatement tests began. Because behavioral responses (including drug-seeking behavior) to footshock are often highly variable, a large sample size (n = 19–20 per group) was selected to ensure sufficient statistical power.
Conditioned reinstatement procedure.
After acquisition of ethanol self-administration in the training phase, rats were trained to associate compound discriminative stimuli with the availability of ethanol versus nonreward. Ethanol was available in the presence of an “S+” consisting of an olfactory cue (banana extract; McCormick & Co, Hunt Valley, MD) paired with a constant white noise (70 dB). Nonreward was signaled by an “S−” consisting of anise extract paired with a constant beeping tone (7 kHz, 70 dB). Olfactory stimuli were generated by depositing six drops (100 μl/drop) of distinct food flavor extracts into the bedding of the operant conditioning chamber 1 min before extension of the lever. The respective stimuli remained present throughout the 30 min sessions. The bedding was changed and trays were cleaned between sessions. Conditioning with the S+ and S− was conducted in random sequence across days until rats completed 20 ethanol and 20 nonreward sessions. Rats then were subjected to daily 30 min extinction sessions, as above, during which both ethanol and discriminative stimuli were withheld until the criterion was reached. Responses at the previously active lever activated the syringe pump motor but had no other scheduled consequences.
One day after the final extinction session, 30 min reinstatement tests began under extinction conditions, except that the discriminative stimuli were reintroduced and remained present throughout the sessions. Rats were tested first in the presence of the S− (after vehicle administration). After an intervening day, rats were tested in the presence of the S+ after LY379268 (0.3, 1.0, and 3.0 mg/kg, s.c.), administered 30 min before the beginning of the session. Drug tests were conducted in separate groups of rats for each dose.
Food-reinforced responding.
To control for possible nonspecific actions of LY379268, the effects of the mGlu2/3 agonist on food-reinforced responding were tested in a group of rats maintained on a food-restricted diet (15 g rat chow per day). These animals were trained to respond for 45 mg food pellet reinforcers (Research Diets, New Brunswick, NJ) on an FR 1 schedule in daily 30 min sessions. After acquisition, daily sessions continued until rats displayed stable food responding (±10% over three consecutive sessions). On the test day, rats were treated with LY379268 (0.3, 1.0, and 3.0 mg/kg, s.c.) using separate groups for each dose (n = 6 per group).
c-fos neural mapping.
To identify potential neural substrates through which LY379268 exerts its inhibitory effects on conditioned and stress-induced reinstatement, c-fos neural mapping was used with the following experimental strategy. Initially, the pharmacological effects of LY379268 on c-fos expression in the absence of behavioral manipulations were determined in two groups of ethanol-naive rats (n = 6 per group) injected with either vehicle or LY379268 (3 mg/kg, s.c.). Next, the effects of ethanol S+ exposure (n = 9) and footshock (n = 8) on c-fos expression in VEH-treated animals were compared with expression levels in rats with the same experimental history and degree of ethanol exposure as the experimental animals but without being subjected to reinstatement tests. For this purpose, brain tissue from a group of rats (n = 5) that had reached the extinction criterion and treated with VEH 30 min before the final extinction session was used. Last, the degree to which the mGlu2/3 agonist alters specific c-fos expression changes induced by the ethanol S+ (n = 8) and footshock (n = 8) was established in rats after completion of reinstatement tests in the 3.0 mg/kg LY379268 groups compared with c-fos expression in the VEH reinstatement conditions. In the case of footshock, animals for c-fos expression analysis were randomly selected from all rats assigned to stress-reinstatement tests.
Fos-protein immunohistochemistry.
At 120 min after LY379268 or vehicle administration (i.e., 90 min after reinstatement or extinction sessions), rats were deeply anesthetized and perfused with 0.9% saline, followed by 4% paraformaldehyde, pH 9.5, 4°C. After cryoprotection, serial 40 μm coronal forebrain sections were cut on a freezing microtome. c-fos expression was gauged by processing sections for Fos-protein immunohistochemistry as described by Dayas et al. (1999). Briefly, sections were incubated in Fos primary antisera (1:5000, rabbit polyclonal, Santa Cruz Biotechnology, Santa Cruz, CA). After Fos-immunolabeling, sections encompassing the VTA were also processed for immunohistochemical detection of the catecholaminergic marker tyrosine hydroxylase (TH) (anti-TH, 1:15,000, mouse-monoclonal; DiaSorin, Stillwater, MN) for identification of A10 dopaminergic neurons. Sections were incubated in appropriate secondary antisera (2 h; Jackson ImmunoResearch, West Grove, PA), followed by avidin–biotin–horseradish peroxidase complex solution (2 h; Vector Elite kit; Vector Laboratories, Burlingame, CA). Nickel diaminobenzidine (DAB) was used to visualize horseradish peroxidase activity in the case of Fos, DAB alone, for TH.
Counts of Fos-positive cells were made within the following: the medial prefrontal cortex (mPFC), incorporating the prelimbic cortex and the Cg1 and Cg2 divisions of the anterior cingulate cortex (2.2–2.86 mm rostral to bregma); nucleus accumbens core (NACc) and shell (NACsh) (1.76 and 1.6 mm rostral to bregma); dorsolateral bed nucleus of the stria terminalis (BST-LD) (0.08 to −0.4 mm relative to bregma); lateral (CeA-L) and medial (CeA-M) divisions of the central amygdala and basolateral amygdala (BLA) (−2.12 to −2.92 mm relative to bregma); HIPPO, including the CA1, CA3, and dentate gyrus (DG) divisions (−2.80 to −3.12 mm relative to bregma); and the medial parvocellular division of the paraventricular nucleus of the hypothalamus (mpPVN) (−1.48 to −2.12 mm relative to bregma). For the VTA, Fos-positive TH-labeled cells were counted over three sections (−5.20 to −5.60 mm relative to bregma).
Statistical analysis.
Effects of LY379268 on stress- and cue-induced reinstatement were analyzed by 4 × 2 mixed-factorial ANOVA with drug dose as a between-subjects factor and experimental phase (extinction vs reinstatement) as a within-subjects factor. Significant interactions were followed by Fisher's PLSD post hoc tests to evaluate differences between extinction and reinstatement responses as well as among drug doses. Effects of LY379268 on food-maintained responding were analyzed by one-way ANOVA, followed by Fisher's PLSD post hoc tests to verify differences between vehicle and drug effects. Fos-immunoreactivity data were analyzed by Mann–Whitney U nonparametric tests. (This nonparametric statistic was used because of violations of normality in raw Fos-positive cell counts.) Separate tests were conducted for each brain region to evaluate the effect of LY379268 versus vehicle treatment and to determine differences in counts between the extinction and reinstatement conditions in each brain region. Fos data are expressed as mean ± SEM of the total number of Fos-positive cells.
Results
Effects of LY379268 on stress-induced reinstatement
The mean ± SEM number of ethanol-reinforced responses across the final three self-administration sessions was 40.8 ± 3.0 (Fig. 1A). Rats reached the extinction criterion within 2 weeks. Footshock elicited significant (p < 0.05) recovery of responding in vehicle-treated rats (mean ± SEM, 11 ± 3.7) (Fig. 1A). LY379268 dose dependently attenuated footshock-induced reinstatement with significant effects at the 1.0 (p < 0.05) and 3.0 (p < 0.01) mg/kg doses (Fisher's PLSD tests after dose × experimental phase interaction, F(3,75) = 2.729; p < 0.05) (Fig. 1A). Several rats showed lever generalization after footshock and responded at both the active and inactive levers. Inactive lever responses, however, did not differ statistically from extinction responses in any group.
Effects of LY379268 on conditioned reinstatement
The mean ± SEM number of ethanol-reinforced responses across the final three sessions of the conditioning phase was 36.0 ± 2.0. Rats reached the extinction criterion within 2 weeks. Presentation of the ethanol S+ elicited significant (p < 0.01) recovery of responding in vehicle-treated rats (mean ± SEM responses, 19.0 ± 3.5) (Fig. 1B). LY379268 dose dependently decreased the response-reinstating actions of the S+ with significant effects at the 1.0 (p < 0.01) and 3.0 (p < 0.01) mg/kg doses (Fisher's PLSD tests after dose × experimental phase interaction, F(3,27) = 8.122; p < 0.01) (Fig. 1B). Responses in the presence of the S− remained at extinction levels. Inactive lever responses were negligible throughout all experimental phases.
Effects of LY379268 on food-reinforced responding
All rats acquired stable food-reinforced responding after 10 d (mean ± SEM responses across the final three sessions, 167.0 ± 4.1). LY379268 did not alter food-reinforced behavior at any dose (Fig. 1C).
Effects of stress and ethanol cue exposure on Fos immunoreactivity
Compared with extinction controls, footshock significantly increased Fos-positive cell counts within the NACc (U = 0; p < 0.01), NACsh (U = 0; p < 0.01), BLA (U = 0; p < 0.01), VTA A10 cells (U = 0; p < 0.01), CeA-L (U = 1.5; p < 0.01), CeA-M (U = 0; p < 0.01), BST-LD (U = 3; p < 0.01), and mpPVN (U = 0; p < 0.01) (see Fig. 3B–D,F). However, within the mPFC and HIPPO, Fos-immunoreactive cell counts in footshock-exposed rats were not significantly different from those in the extinction group (see Fig. 3A–E). To confirm that the rats randomly selected for Fos-protein immunohistochemistry (Fos subgroup) were representative of the entire stress reinstatement group, the behavioral data of these animals (n = 8) were compared with those of the remaining 11 animals (non-Fos subgroup) by mixed-factorial ANOVA. The two subgroups were statistically indistinguishable in terms of both stress-induced responding at the 0 mg/kg dose (i.e., vehicle) of LY379268 (group × experimental phase interaction, F(1,17) = 1.747; NS) and the attenuation of reinstatement at the 3 mg/kg LY379268 dose (group × experimental phase interaction, F(1,18) = 0.699; NS). Rats in the Fos subgroup showed significant reinstatement versus extinction, as well as significantly reduced reinstatement after 3 mg/kg LY379268 (p < 0.05; Fisher's PLSD tests after dose × experimental phase interaction, F(1,14) = 6.104; p < 0.05) (Fig. 2A).
Rats exposed to the ethanol S+ showed significantly increased numbers of Fos-positive cells within the mPFC (U = 3.0; p < 0.05), NACc (U = 0; p < 0.01), NACsh (U = 0; p < 0.01), BLA (U = 4; p < 0.05), VTA A10 cells (U = 4; p < 0.05), CA1 (U = 1; p < 0.01), CA3 (U = 3; p < 0.01), DG (U = 0; p < 0.01), and within the CeA-L (U = 4.0; p < 0.05), CeA-M (U = 0; p < 0.01), and BST-LD (U = 0; p < 0.01) compared with counts in the extinction control group (Fig. 3A–F).
Modification of stress- and cue-induced Fos immunoreactivity by LY379268
Footshock stress
No differences in Fos-positive cell counts were observed between LY379268 and vehicle-treated rats exposed to footshock within the mPFC, the NACc and NACsh, BLA, and VTA A10 cells (Fig. 3A–D). LY379268 reduced Fos-positive cell counts in the hippocampal CA1 (U = 11; p < 0.05) and CA3 (U = 10; p < 0.05) but not the DG division compared with the stress-exposed vehicle group (U = 13.5; p > 0.05) (Figs. 3E). Compared with vehicle, LY379268 increased Fos-positive neurons in rats subjected to footshock within the CeA-L (U = 11; p < 0.05) and CeA-M (U = 13; p < 0.05), the BST-LD (U = 7.5; p < 0.01), and mpPVN (U = 4; p < 0.01) (Fig. 3F).
Ethanol cue exposure
Within the mPFC, and NACc and NACsh, VTA A10 cells, and the BLA, rats exposed to the ethanol S+ showed identical levels of Fos immunoreactivity regardless of treatment condition (LY379268 or vehicle) (Fig. 3A–D). LY379268 significantly reduced Fos-positive cells within the CA1 (U = 11; p < 0.05), CA3 (U = 7; p < 0.01), and DG (U = 12; p < 0.05) of S+-exposed rats compared with S+ effects in the vehicle group, similar to the effects of the drug on stress-induced Fos-immunoreactivity (Figs. 3E, 4C–H). Within the CeA-L (U = 3; p < 0.01) and CeA-M (U = 11; p < 0.05), BST-LD (U = 9; p < 0.05), and mpPVN (U = 5; p < 0.01), Fos-positive cell counts were significantly elevated in rats exposed to the ethanol S+ and treated with LY379268 compared with vehicle-treated animals (Figs. 3F, 4A,B).
Effects of LY379268 in naive animals
The effects of LY379268 on Fos immunoreactivity within experimentally and ethanol-naive rats were similar to those in animals exposed to stress or the ethanol S+ and treated with the mGlu2/3 agonist. Specifically, no differences in Fos immunoreactivity were observed within the mPFC, NAC, VTA, and BLA of LY379268-treated versus VEH-treated rats (3 mg/kg) (Fig. 3A–D). Within the CA1 (U = 4; p < 0.05) and DG (U = 2; p < 0.01), LY379268 significantly reduced Fos-positive cells compared with vehicle (Fig. 3E). LY did not alter Fos-positive cell counts in the CA3. Within the CeA-L (U = 0; p < 0.01), CeA-M (U = 5.5; p < 0.05), BST-LD (U = 4; p < 0.05), and mpPVN (U = 1.5; p < 0.01), Fos-positive cell counts were significantly elevated in LY379268- over vehicle-treated rats (Fig. 3F).
Discussion
Activation of group II mGluRs by a selective mGlu2/3 agonist (LY379268) dose dependently blocked the effects of both stress- and drug-related environmental stimuli on the recovery of extinguished ethanol-seeking behavior. The mGlu2/3 agonist did not interfere with food-maintained responding, consistent with previous work in which LY379268 did not alter behavior reinforced by palatable natural rewards (Baptista et al., 2004; Bossert et al., 2004). Furthermore, at the dose range used here, LY379268 is devoid of motoric side effects (Cartmell et al., 1999, 2000), indicating that the “anti-reinstatement” actions of the drug cannot be attributed to motor impairment or sedation. The behavioral effects of LY379268 therefore confirm that interference with the response-reinstating effects of cocaine- and heroin-related environmental stimuli by LY379268 (Baptista et al., 2004; Bossert et al., 2004) extends to the effects of contextual stimuli conditioned to ethanol, thereby implicating group II mGluR-regulated neural mechanisms in the control of behavior by drug cues regardless of drug class. At the same time, the results provide evidence that the anxiolytic profile of mGlu2/3 agonists emerging in animal and human studies (for review, see Swanson et al., 2005) extends to attenuation of stress-induced ethanol-seeking behavior.
Ethanol S+ exposure increased c-fos expression (compared with extinction controls) in cortical and limbic brain regions with an established role in conditioned reinstatement (i.e., the mPFC, NACc, HIPPO, BLA, and VTA), confirming previous reports of increased c-fos expression within these sites by environments or contextual cues associated with drugs of abuse, including ethanol (Topple et al., 1998; Ciccocioppo et al., 1999; Franklin and Druhan, 2000; Neisewander et al., 2000; Schroeder et al., 2003). Additionally, the ethanol S+ increased Fos immunoreactivity within the CeA and BST-LD, brain regions that regulate behavioral responses to stress, including stress-induced reinstatement of drug- seeking (Shaham et al., 2003). Rats subjected to footshock stress showed strong increases in Fos-positive neurons within the brain stress circuit, including the CeA, mpPVN, and BST-LD, as well as in mesocorticolimbic circuitry components, including the NAC, BLA, and VTA. The lack of significant effects of footshock on hippocampal and mPFC c-fos expression differs from previous reports that acute stress activates both mPFC and HIPPO neurons (Cullinan et al., 1995; Funk et al., 2006). A possible explanation for this discrepancy is that mPFC and HIPPO neurons developed some hyporesponsiveness to stress as a result of the modest but prolonged daily ethanol exposure, as suggested by a previous report showing decreased stress-induced hippocampal and prefrontal cortical c-fos expression after acute ethanol treatment (Ryabinin et al., 1995).
Overall, there was marked overlap in the pattern of neural activation produced by footshock and ethanol cue exposure. However, ethanol cue-exposed rats showed stronger activation of brain regions linked to motivation and reward (i.e., mPFC and HIPPO) than rats subjected to footshock, whereas footshock produced stronger neural activation within brain stress sites, in particular the mpPVN. Both footshock and the ethanol S+ activated the CeA and BST-LD, a finding that may reflect possible stress or anxiety-like effects of the ethanol cue. Such effects would be consistent with the suggestion that frustration associated with the absence of ethanol reward in an ethanol-predictive stimulus environment may trigger an aversive motivational state resulting in stress-like neural activation patterns (Topple et al., 1998). Alternatively, these effects may be related to the possibility that stress and drug cue exposure induce a similar pattern of neural activation, as suggested by recent clinical findings showing that craving states associated with drug cue exposure are accompanied by anxiety and hypothalamic–pituitary–adrenal (HPA) axis activation (Sinha et al., 2003; Fox et al., 2005).
In ethanol-naive rats, LY379268 produced a distinct pattern of neural effects, characterized by increased c-fos expression within the CeA, BST-LD, and mpPVN and decreased c-fos expression in the hippocampus. These effects resemble those produced by LY354740 [(+)-2-aminobicyclo[3.1.0]-hexane-2,6-dicarboxy-late monohydrate] (a selective mGlu2/3 agonist structurally related to LY379268) in drug-naive rats (Linden et al., 2004), suggesting that the pattern of regionally specific changes in c-fos expression observed here represents a neural effect shared by different mGlu2/3 agonists. In rats subjected to reinstatement tests, LY379268 distinctly modified brain c-fos expression induced by footshock and the ethanol cue. These effects, however, remained confined to the same brain regions as in ethanol-naive rats. Furthermore, the direction of changes in neural activation remained consistent with that in ethanol-naive rats. Thus, neither repeated ethanol exposure during the training phase nor acute footshock appeared to alter mGluR function in brain regions that were unresponsive to LY379268 in the ethanol-naive control group.
The predominant neural effect of LY379268 in rats of the ethanol cue reinstatement condition was to decrease c-fos expression in the hippocampus and to increase expression in sites mediating behavioral and physiological responses to stress: the CeA, BST-LD, and mpPVN. Although the c-fos expression data do not establish the mechanism(s) by which LY379268 blocked cue-induced reinstatement, they provide important leads in conjunction with existing knowledge of both the function of the brain regions in which neural activity was altered by LY379268 and the functional role of mGlu2/3 receptor activation in these regions. Group II mGluRs are densely expressed in the amygdala and hippocampus (Kenny and Markou, 2004). Activation of these receptors inhibits glutamate release presynaptically and dampens neural excitability postsynaptically (Schoepp, 2001). In the case of the hippocampal effects of LY379268, the significant reduction in c-fos expression is consistent with electrophysiological evidence that this mGlu2/3 agonist reduces hippocampal neural excitability (Kilbride et al., 1998; Kew et al., 2002). The dorsal hippocampus has an established role in contextual memory retrieval and the occasion-setting action of contextual stimuli (Holland and Bouton, 1999). Moreover, transient lesion studies directly implicate the dorsal hippocampus in the control of drug-seeking by contextual stimuli (Fuchs et al., 2005). One explanation for the attenuation of cue-induced reinstatement by LY379268, therefore, is that decreased excitation of hippocampal glutamatergic efferents by the mGlu2/3 agonist (cf. Swanson et al., 2005) interferes with the processing of drug-related contextual information, reducing its motivational impact. It is also possible that the reversal of conditioned reinstatement by LY379268 is related to the role of the hippocampus in fear and anxiety (Gray, 1982). Microinjection of LY354740 into the dorsal hippocampus produces anxiolytic-like effects in animals (Tatarczynska et al., 2001). Because craving states associated with drug cue exposure in humans are accompanied by anxiety (Sinha et al., 2003; Fox et al., 2005), another mechanism by which LY379268 may have attenuated conditioned reinstatement is by reversing anxiogenic consequences of drug cue exposure at the hippocampal level (as well as via CeA-mediated anti-anxiety actions discussed below).
Consistent with the pattern of neural effects in ethanol-naive rats, LY379268 did not modify c-fos expression induced by the EtOH S+ in the mPFC, VTA, NAC, and BLA. Although group II mGluRs are widely expressed throughout these regions (Kenny and Markou, 2004), this finding suggests that LY379268 does not attenuate conditioned reinstatement through an action in these sites. It cannot be ruled out fully, however, that LY379268 effects in one or more of these brain regions contributed to the reversal of conditioned reinstatement because c-fos is not a universal marker of neural activity. Indeed, LY379268 did not alter S+-induced c-fos expression in the VTA, although intra-VTA administration of LY379268 blocked, albeit not dose dependently, context-induced heroin reinstatement (Bossert et al., 2004). Moreover, it cannot be ruled out that effects in brain regions expressing mGlu2/3 receptors such as the ventral pallidum, thalamus, or rhinal cortical areas (Ohishi et al., 1993a,b) with connections to the hippocampus (brain regions that were not examined) may have played some role in the reduction of conditioned reinstatement by LY379268.
In rats subjected to footshock stress, LY379268 produced effects similar to those in ethanol cue-exposed rats, with increased c-fos expression in stress-regulatory sites, including the CeA, BST-LD, and mpPVN, and decreased expression in the CA1 and CA3 regions of the hippocampus. Discrete intra-CeA administration of LY354740 into the CeA attenuates anxiety-like behavior in the fear potentiated startle model (Walker et al., 2002). Anxiolytic actions of mGlu2/3 receptor activation in the CeA, therefore, are likely to be directly relevant for the attenuation of stress-induced reinstatement. Based on findings that mGlu2/3 receptor activation increases c-fos expression within glutamic acid decarboxylase-positive cells in the CeA-L, it has been suggested that mGlu2/3 receptor activation “disinhibits” GABAergic neurons that innervate the CeA by reducing excitatory glutamatergic input onto intervening GABAergic interneurons (Swanson et al., 2005). Whether a similar “disinhibition” of GABAergic interneurons accounts for the increased c-fos expression in the BST-LD is presently unclear. Moreover, it remains to be determined by what mechanism mGlu2/3 agonist-induced c-fos expression in the CeA (and BST-LD) is linked to anxiolytic action, because both anxiogenic and anxiolytic agents increase immediate early gene expression within these nuclei (Thompson and Rosen, 2006).
In light of the reduction in hippocampal neural activity by LY379268, hippocampal-mediated anti-anxiety actions may also have contributed to the attenuation of stress-induced reinstatement. Because footshock, by itself, did not produce significant elevations in hippocampal Fos immunoreactivity over that in extinction controls, a role of the hippocampus in stress-induced reinstatement could not be confirmed. Nonetheless, it remains possible that mGlu2/3 activation indirectly dampened the effects of footshock at “downstream” neural targets by reducing tonic excitatory glutamatergic output from the hippocampus. Additionally, it cannot be ruled out that direct or indirect effects of LY379268 on neural substrates implicated in stress-induced reinstatement, but not examined in the present study, such as the lateral tegmental nuclei (Shaham et al., 2003), ventral pallidum (McFarland et al., 2004), and lateral hypothalamus (Boutrel et al., 2005) contributed in some manner to the “anti-reinstatement” actions of the mGlu2/3 agonist.
Last, in both the footshock and the ethanol S+ condition, LY379268 increased c-fos expression within the mpPVN, an effect known to be positively correlated with activation of the HPA axis (Buller et al., 1998). Despite this stress-like effect, both cue- and stress-exposed animals showed decreased reinstatement. The activation of mpPVN neurons is perhaps most parsimoniously explained in terms of nonspecific disinhibition of local hypothalamic circuits by LY379268, similar to the effects of other anxiolytic agents that acutely increase c-fos expression in the mpPVN (Salminen et al., 1996).
It is of interest to note that, in a recent report, only a high, locomotor suppressant 5 mg/kg dose of LY379268 was effective in reversing reinstatement induced by ethanol cue exposure paired with noncontingent administration of an ethanol “priming” dose to enhance ethanol-seeking behavior (Backstrom and Hyytia, 2005). The failure to observe suppression of locomotor activity in this study at doses smaller than 5 mg/kg strengthens the conclusion that the effects of LY379268 observed here are not related to nonspecific impairments of motor behavior. With respect to the high LY379268 dose necessary to reverse reinstatement (a finding that contrasts with the present results), it is necessary to keep in mind that ethanol-seeking in this report must be presumed to have been driven primarily by the ethanol priming dose rather than representing conditioned reinstatement. The weak interference by LY379268 with ethanol-directed behavior under these conditions is consistent with evidence that, compared with its effects on cue-induced reinstatement, this mGlu2/3 agonist is considerably less effective in attenuating the acute reinforcing effects of ethanol (Zhao et al., 2005), cocaine (Baptista et al., 2005), and heroin (Bossert et al., 2004, 2005).
In summary, the results implicate group II mGluRs as a common neuropharmacological substrate for ethanol-seeking elicited by both drug cues and stress and point toward the hippocampus and stress-regulatory sites within the extended amygdala as neurocircuitry components through which group II mGluR activation exerts these effects. In view of previous findings that LY379268 attenuates the response-reinstating effects of cocaine and heroin-related environmental stimuli (Baptista et al., 2004; Bossert et al., 2004), the data suggest that mGlu2/3 receptors participate in mediating the effects of contextual stimuli conditioned to drugs of abuse with widely different mechanisms of action. Moreover, based on the current understanding of the neurocircuitry mediating addiction-relevant effects of stress (Shaham et al., 2003), a role of group II mGluRs in stress-induced reinstatement is likely to also hold across different drugs of abuse. Because stress and craving evoked by drug-related environmental stimuli are major risk factors for relapse to drug use, these results identify group II mGluRs as promising targets for relapse prevention.
Footnotes
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This work was supported by National Institutes of Health/National Institute on Alcohol Abuse and Alcoholism Grants AA10531 and AA06420 (F.W.). C.V.D. was supported by a C. J. Martin Fellowship (National Health and Medical Research Council, Australia). We thank Dr. Darryle Schoepp (Lilly Research Laboratories, Indianapolis, IN) for generously providing LY379268, Mike Arends for editorial assistance, Kris Trulock and Charles Peto, (The Salk Institute, La Jolla, CA) for providing expertise and facilities for photomicrograph production, as well as Jeffrey Simms and Kristen Santerre for excellent technical assistance. This is publication 17698-NP from The Scripps Research Institute.
- Correspondence should be addressed to Dr. Christopher V. Dayas, Molecular and Integrative Neurosciences Department, The Scripps Research Institute (SP30-2120), 10550 North Torrey Pines Road, La Jolla, CA 92037. cvdayas{at}scripps.edu