CNQX but not NBQX Prevents Expression of Amphetamine-Induced Place Preference Conditioning: A Role for the Glycine Site of the NMDA Receptor, but not AMPA Receptors

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Vol. 290, Issue 1, 9-15, July 1999

CNQX but not NBQX Prevents Expression of Amphetamine-Induced Place Preference Conditioning: A Role for the Glycine Site of the NMDA Receptor, but not AMPA Receptors¹

Andy N. Mead and David N. Stephens

University of Sussex, Brighton, United Kingdom

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

We investigated the role of the $alpha$ -amino-3-hydroxy-5-methyl-4-isoxazole propionate (AMPA) receptor in the induction and expressionof an amphetamine-induced conditioned place preference (CPP) inmice. The selective AMPA-receptor antagonist 2,3-dihydroxy-6-nitro-7-sulfamoyl-benzo(f)quinoxaline(NBQX) failed to prevent the induction of a CPP, except at a dose(30 mg/kg) that also produced a conditioned place aversion. NBQXalso failed to affect the expression of a CPP at a dose high enoughto reduce activity levels. In contrast, the less selective AMPAreceptor antagonist 6-cyano-7-nitroquinoxalone-2,3-dione (CNQX)prevented the expression of a CPP at doses (1-10 mg/kg) that hadno effect on activity levels. We therefore tested the possibilitythat CNQX exerted its effects due to antagonism at the glycinesite of the N-methyl-D-aspartate receptor. The glycine-site antagonist7-chloro-4-hydroxy-3-(2-phenoxy)phenyl-2(1H)-quinolone also preventedthe expression of a CPP at doses that had no effect on activitylevels (0.1-0.3 mg/kg). These results suggest that neither theinduction nor the expression of an amphetamine-induced CPP requiresAMPA receptor-mediated transmission and that effects found inprevious studies using the less selective AMPA receptor antagonistsmay be due to the effects of these compounds at the glycine siteof the N-methyl-D-aspartatereceptor.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

The conditioned place preference (CPP) paradigm has frequently been used as a method of assessing the reinforcing propertiesof drugs of abuse and to study the neural mechanisms underlyingconditioned reinforcement. The majority of drugs abused by humans,including psychostimulants, opiates, ethanol, and benzodiazepines,will also produce a CPP (see, Carr et al., 1989, for review).During recent years, it has been reported that both the developmentand expression of a CPP are dependent on glutamatergic transmission.Specifically, it has been proposed that there are different rolesfor two of the main receptor subtypes for glutamate: the N-methyl-D-aspartate(NMDA) and $alpha$ -amino-3-hydroxy-5-methyl-4-isoxazole propionate (AMPA)receptors (Cervo and Samanin, 1995; Tzschentke and Schmidt, 1997).

Transmission via the NMDA receptor subtype has been argued to be necessary for both the induction and the expression of aCPP because the NMDA channel blocker MK-801 prevented the inductionof a cocaine (Cervo and Samanin, 1995), methamphetamine (Kim andJang, 1997), and morphine CPP in rats (Tzschentke and Schmidt,1995, 1997; Kim et al., 1996). This effect has been replicatedwith the competitive NMDA receptor antagonist CGP37849, preventingthe induction of a morphine CPP, again in rats (Tzschentke andSchmidt, 1995). However, Hoffman (1994) reported that MK-801 failedto affect the induction of an amphetamine (AMPH)-induced CPP.Studies investigating the effect of NMDA receptor antagonistson the expression of a CPP reveal conflicting results. MK-801failed to prevent the expression of a cocaine-induced CPP (Cervoand Samanin, 1995) but did prevent the expression of a morphine-inducedCPP (Tzschentke and Schmidt, 1997). Furthermore, Bespalov (1996)reported that the competitive antagonist (±)-3-(2-carboxy-piperazine-4-yl)-propyl-1-phosphonicacid prevented the expression of an AMPH-induced CPP.

The underlying involvement of AMPA receptors in CPP appears to be much clearer. First, the AMPA receptor antagonist 6,7-dinitroquinoxaline-2,3-dione(DNQX) prevented the expression of a CPP induced by cocaine (Cervoand Samanin, 1995; Kaddis et al., 1995), AMPH, and morphine (Layeret al., 1993). Second, the noncompetitive AMPA receptor antagonistGYKI 52466 has been reported to prevent the expression of botha morphine and an AMPH-induced CPP (Tzschentke and Schmidt, 1997).Although DNQX infused into the nucleus accumbens was shown tobe ineffective against the induction of a morphine CPP (Layeret al., 1993) and intracerebroventricular DNQX was ineffectiveagainst the induction of a cocaine-induced CPP (Cervo and Samanin,1995), intra-accumbens DNQX did attenuate the induction of anAMPH (Layer et al., 1993) and a cocaine-induced CPP (Kaddis etal., 1995). Therefore, the current literature suggests that AMPAreceptors mediate the expression of drug-induced CPPs but thatAMPA receptor antagonists show a more inconsistent profile whentested on theinduction.

One consistent problem with the studies investigating the role of AMPA receptors is that they have all involved the use ofAMPA receptor antagonists that have relatively low selectivityat the AMPA receptor. DNQX also possesses antagonistic propertiesat the strychnine-insensitive glycine site of the NMDA receptor(Kessler et al., 1989; Pellegrini-Giampietro et al., 1989; Sheardownet al., 1990; Goldstein and Litwin, 1993; Yoneda et al., 1993;Birch et al., 1988), and there is evidence that GYKI 52466 mayalso influence NMDA receptor-mediated transmission (Steppuhn andTurski, 1993), although it does not act at NMDA receptors (Honoré,1991; Ouardouz and Durand, 1991). Because NMDA receptor antagonistscan prevent the expression of a CPP (Bespalov, 1996; Tzschentkeand Schmidt, 1997), caution must be exercised in interpretingthe results from the less selective AMPA receptorantagonists.

The purpose of the studies reported here was to assess the role of glutamatergic transmission via AMPA receptors in an AMPH-inducedCPP in mice using the selective competitive AMPA receptor antagonist2,3-dihydroxy-6-nitro-7-sulfamoyl-benzo(f) quinoxaline (NBQX)(Sheardown et al., 1990). For comparison, we also investigatedthe effect of the less selective AMPA receptor antagonist 6-cyano-7-nitroquinoxalone-2,3-dione(CNQX), which has a similar pharmacological profile to DNQX (Birchet al., 1988; Harris and Miller, 1989; Kessler et al., 1989; Pellegrini-Giampietroet al., 1989), although its selectivity for AMPA receptors comparedwith NMDA receptors is slightly higher than that for DNQX (Sheardownet al., 1990). Subsequently, we explored the involvement of theglycine site of the NMDA receptor by assessing the effect of thestrychnine-insensitive glycine-site antagonist L-701,324. Theresults of these studies allowed us to make conclusions concerningthe reliability of the previous studies investigating AMPA receptorinvolvement in a drug-induced CPP.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Animals

Male C57Bl/6J × SV129 mice, bred at the University of Sussex, were used in all experiments. Animals weighed 21 to 29 g atthe start of experiments and were housed in groups of two or threeunder a 12:12-h light/dark cycle (lights on at 7:00 AM) with adlibitum access to food and water. Holding room temperature wasmaintained at 20-21°C, and humidity was 40 to 60%. Experimentswere performed between 8:30 AM and 3:00 PM. All experiments werecarried out under U.K. legislation on animalexperimentation.

Apparatus

All experiments were performed in a three-compartment place conditioning apparatus. The two outer compartments (200 × 200× 200 mm) were separated by a central compartment (200 × 50 ×200 mm) and differed in visual and tactile cues. One outer compartmenthad white walls with a perforated metal floor, whereas the otherhad black and white walls (each wall was split along the diagonal,with the top half painted black and the bottom half painted white)with a smooth clear Perspex floor. The central compartment allowedmovement from one compartment to the other and could also be blockedfrom the outer compartments with clear doors, to restrict animalsto a particular compartment during the conditioning phase. Themovement and location of animals during the preconditioning andtest phases were recorded using a video camera (Sony SPT-M108CE)connected to a video cassette recorder (Panasonic AG-5700) toallow subsequent analysis of preference andactivity.

Procedure

Four separate experiments were performed, for which the basic protocol was identical. In all experiments, we used an AMPH-induced(0.25 mg/kg) CPP as the paradigm to assess the role of glutamatergicmechanisms in conditioned reinforcement. In experiments 1 and2, we investigated the effect of NBQX on the induction and theexpression of a CPP. In experiments 3 and 4, we investigated theeffect of CNQX and 7-chloro-4-hydroxy-3-(2-phenoxy)phenyl-2(1H)-quinolone(L-701,324) on the expression of a CPP. The design of these experimentsis shown in Table 1.

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TABLE 1
Experimental design for CPP experiments
Amphetamine (AMPH) at 0.25 mg/kg or saline administered i.p. immediately before conditioning. NBQX, CNQX, and vehicles administered i.p. 20 min before conditioning or test. L-701,324 and vehicle administered i.p. 25 min before test. For drug dose ranges, see the text.

CPP Procedure

The CPP procedure took place over 10 days and consisted of the following threephases.

Preconditioning Phase (Day 1). Animals received vehicle (t = $-$ 20 min), followed by saline (t = 0). Consequently, they were placed in the CPP apparatus andallowed to explore freely for 10 min. The behavior of the animalswas recorded for subsequent analysis. These data provided thebaseline preferences for the two compartments. Initial preferencesfor the two compartments did not differ significantly (mean ±S.E.M. time, 199 ± 3.7 s in compartment A, 201 ± 4.1 s in compartmentB during a 10-min test, calculated from allexperiments).

Conditioning Phase (Days 2-9). On every second day, in experiment 1, animals received NBQX (vehicle, 3, 10, or 30 mg/kg) 20 min before AMPH or NBQX (vehicle,30 mg/kg) 20 min before saline, immediately before confinementto one compartment of the CPP apparatus. On every second day,in experiments 2, 3, and 4, animals received vehicle 20 min beforeAMPH and confinement to one compartment. In all four experiments,on alternate days, all animals received vehicle 20 min beforesaline and confinement to the other compartment. Confinement tocompartments lasted for 20 min. Assignment of drug-paired compartmentswas performed randomly and was fully counterbalanced acrossgroups.

Test Phase (Day 10). Animals received NBQX vehicle (experiment 1), NBQX vehicle or 10 mg/kg (experiment 2), CNQX vehicle, 1, 3, or 10 mg/kg (experiment3) 20 min before saline, or L-701,324 vehicle, 1, 3, or 10 mg/kg(test 1) or L-701,324 vehicle, 0.03, 0.1, or 0.3 mg/kg (test 2)25 min before saline (experiment 4). After the saline injection,animals were allowed to freely explore the apparatus for 10 min.The behavior of the animals was recorded for subsequent analysisto determine the extent of place conditioning and activitylevels.

Drugs

d-AMPH sulfate was obtained from Sigma Chemical (Poole, Dorset, UK). NBQX and CNQX were donated by Schering AG (Berlin, Germany).L-701,324 was donated by Merck Sharp and Dohme (Essex, UK). AMPHwas dissolved in 0.9% saline. NBQX was dissolved in 1 M sodiumhydroxide, and 0.1 M hydrochloric acid was added to take the pHback toward neutral. The solution was made up to its final volumewith distilled water. This resulted in drug solutions of pH 9to 10. NBQX vehicle was pH matched to drug by adding 0.1 M sodiumhydroxide to distilled water. CNQX and L-701,324 were suspendedin 0.3% Tween-80 in distilled water, which was also used as thevehicle. All drugs were administered i.p. at an injection volumeof 10 ml/kg. All doses refer to drugbase.

Data Analysis

The time spent in each compartment and activity within the compartments were scored blind. An animal was considered to bein a compartment only when its entire body was within that compartment.Activity was measured as line crossings of two perpendicular linescrossing the midpoint and extending to the walls of the compartment.For analysis of place conditioning, the time spent in the drug-pairedcompartment minus the time spent in the vehicle-paired compartmentwas used as the dependent variable. For analysis of activity levels,total line crossings in both compartments were used as the dependentvariable. Data for place conditioning were initially analyzedusing a two-way mixed-factor ANOVA (except for test 1 in experiment4), with test session (preconditioning and test phase) and treatmentas independent variables. After a significant interaction, a one-waybetween-subject ANOVA was performed on the test session data only.If this produced a significant effect of treatment, post hoc analysiswas performed using the Duncan's test. Due to the sedative effectof the higher dose range of L-701,324 (experiment 4, test 1),the variance between groups was heterogeneous, and the data werenot suitable for parametric analysis. For this reason, a comparisonof the preference during the test phase and the preconditioningphase for each group was made using Wilcoxon's signed rank testto deduce whether conditioning had occurred. Data for activitylevels were analyzed using a one-way ANOVA on activity levelsduring the test phase, followed by Duncan's test if a significanteffect of treatment was found. All statistical analysis was performedusing the SPSS statistical package for Windows (Version 6.1, SPSSInc., Chicago,IL).

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

CPP. The results from experiment 1, showing the effect of NBQX on the induction of place conditioning, are shown in Fig. 1. Analysisrevealed a significant interaction between treatment and testsession (F_5,53 = 4.90, p < .01). The one-way ANOVA on the preferencefor the AMPH-paired compartment during the test phase revealeda significant effect of treatment (F_5,53 = 12.1, p < .001), indicatingthat significant place conditioning had taken place. Post hoccomparisons showed a significant effect of AMPH compared withsaline, indicating place conditioning (p < .05). NBQX, at dosesof 3 and 10 mg/kg, failed to affect the induction of place conditioning,whereas a dose of 30 mg/kg significantly attenuated the preference(p < .05). NBQX, at a dose of 30 mg/kg, also produced a significantplace aversion, compared with saline controls (p < .05).

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Fig. 1. The effect of NBQX on the induction of an AMPH-induced CPP. The data shown represent mean seconds spent in the drug-paired [AMPH 0.25 mg/kg (Amph CPP) or saline (saline CPP)] compartment minus seconds spent in the saline-paired compartment (±S.E.M.) during the 10-min test sessions (preconditioning or test phase). All groups received NBQX vehicle (veh) 20 min before saline, immediately before test session (n = 9 or 10/group). *p < .05 compared with saline CPP plus NBQX vehicle during test phase. $dagger$ p < .05 compared with Amph CPP plus NBQX vehicle during test phase (Duncan's test).

The results from experiment 2, showing the effect of NBQX on the expression of AMPH-induced place conditioning, are shownin Fig. 2. The two-way ANOVA on treatment by test session revealeda significant interaction (F_3,31 = 3.88, p = .018) and a subsequentone-way ANOVA on test-phase data revealed a significant effectof treatment (F_3,31 = 3.53, p = .026). Post hoc analysis showedthat groups conditioned to AMPH displayed a significant placepreference compared with saline-conditioned groups (p < .05).NBQX at 10 mg/kg had no effect on this place conditioning.

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Fig. 2. The effect of NBQX on the expression of an AMPH-induced CPP. The data shown represent mean seconds spent in the drug-paired [AMPH 0.25 mg/kg (Amph CPP) or saline (saline CPP)] compartment minus seconds spent in the saline-paired compartment (±S.E.M.) during the 10-min test sessions (preconditioning or test phase). All groups received NBQX (veh, 10 mg/kg) 20 min before saline, immediately before test session (n = 8/9/group). *p < .05 compared with saline CPP plus NBQX vehicle during test phase (Duncan's test).

The effect of CNQX on the expression of an AMPH-induced CPP (experiment 3) is shown in Fig. 3. A two-way ANOVA on treatmentby test session revealed a significant interaction (F_5,52 = 3.35,p = .011), and a subsequent one-way ANOVA on test-phase data revealeda significant effect of treatment (F_5,52 = 3.25, p = .013). Posthoc analysis again showed significant place conditioning, withAMPH treatment resulting in more time spent in the drug compartmentthan saline treatment (p < .05). CNQX, at doses ranging from 1to 10 mg/kg, blocked the expression of this CPP (p < .05).

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Fig. 3. The effect of CNQX on the expression of an AMPH-induced CPP. The data shown represent mean seconds spent in the drug-paired [AMPH 0.25 mg/kg (Amph CPP) or saline (saline CPP)] compartment minus seconds spent in the saline-paired compartment (±S.E.M.) during the 10-min test sessions (preconditioning or test phase). All groups received CNQX (veh, 1, 3, or 10 mg/kg) 20 min before saline, immediately before test session (n = 8-10/group). *p < .05 compared with saline CPP plus CNQX vehicle during test phase. $dagger$ p < .05 compared with Amph CPP plus CNQX vehicle during test phase (Duncan's test).

Figure 4 shows the results of experiment 4, in which the effect of the higher dose range of L-701,324 on the expression ofan AMPH-induced CPP was assessed. The extreme variation observedin groups treated with L-701,324 was due to a large spread inthe preference scores, which appeared to occur as a result ofthe locomotor suppressant effects of the compound. Wilcoxon'ssigned rank test revealed that only the group conditioned to AMPHand tested with L-701,324 vehicle displayed significant placeconditioning (z = $-$ 2.80, p < .01). Groups conditioned to AMPHand tested with L-701,324 (1-10 mg/kg) failed to exhibit placeconditioning.

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Fig. 4. The effect of the higher dose range of L-701,324 (1-10 mg/kg) on the expression of an AMPH-induced CPP (test 1). The data shown represent median seconds spent in the drug-paired [AMPH 0.25 mg/kg (Amph CPP) or saline (saline CPP)] compartment minus seconds spent in the saline-paired compartment (±semi-interquartile range) during the 10-min test sessions (preconditioning or test phase). All groups received L-701,324 (veh, 1, 3, or 10 mg/kg) 25 min before saline, immediately before test session (n = 10/group). **p < .01 compared with preconditioning preference for same treatment (Wilcoxon's signed rank test).

The effects of the lower dose range of L-701,324 on the expression of an AMPH-induced CPP are shown in Fig. 5. Two-way ANOVArevealed a significant treatment by test-session interaction (F_5,54= 5.19, p < .01), and subsequent ANOVA on the test-session datarevealed a significant effect of treatment (F_5,54 = 4.49, p <.01). Post hoc analysis revealed that AMPH produced a significantCPP (p < .05), which was prevented by L-701, 324 at doses of 0.1and 0.3 mg/kg. A dose of 0.03 mg/kg L-701,324 failed to preventthe expression of the AMPH CPP.

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Fig. 5. The effect of the lower dose range of L-701,324 (0.03-0.3 mg/kg) on the expression of an AMPH-induced CPP (test 2). The data shown represent mean seconds spent in the drug-paired [AMPH 0.25 mg/kg (Amph CPP) or saline (saline CPP)] compartment minus seconds spent in the saline-paired compartment (±S.E.M.) during the 10-min test sessions (preconditioning or test phase). All groups received L-701,324 (veh, 0.03, 0.1, or 0.3 mg/kg) 25 min before saline, immediately before test session (n = 10/group). *p < .05 compared with saline CPP plus L-701,324 vehicle during test phase. $dagger$ p < .05 compared with Amph CPP plus L-701,324 vehicle during test phase (Duncan's test).

Activity during CPP Test. Figure 6 shows the effects of the various drug treatments on activity levels during the test phase. Figure 6A shows the activitylevels during the test assessing the effect of NBQX on the expressionof the CPP (experiment 2). One-way ANOVA revealed a significanteffect of treatment (F_3,31 = 3.31, p < .05), and post hoc analysisindicated that the groups receiving AMPH-NBQX and saline-NBQXdisplayed a significant reduction in activity compared with thegroup receiving AMPH-vehicle (p < .05). In contrast, CNQX (experiment3) had no effect on activity levels during the test phase (F_5,52= 0.69, p > .05), as shown in Fig. 6B. The effects of L-701,324are shown in Fig. 6, C and D. At the higher dose range (Fig. 6C),one-way ANOVA revealed a significant effect of group (F_5,54 =7.78, p < .001). Subsequent post hoc analysis revealed that L-701,324significantly reduced activity at all three doses (1-10 mg/kg)compared with groups that received L-701,324 vehicle. At the lowerdose range (Fig. 6D), one-way ANOVA revealed no effect of L-701,324(0.03-0.3 mg/kg) on activity during the test-phase (F_5,54 = 1.16,p > .05).

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Fig. 6. The effect of glutamatergic antagonists on activity levels during the test phase of experiments 2, 3, and 4. Data represent mean number of line crossings (±S.E.M.) during the 10-min test session. NBQX and CNQX were administered i.p. 20 min before testing. L-701,324 was administered i.p. 25 min before testing. All animals were previously conditioned to either 0.25 mg/kg AMPH (Amph CPP) or saline (saline CPP). A, effect of NBQX (veh, 10 mg/kg) on activity levels during test phase (n = 8 or 9/group). B, effect of CNQX (veh, 1-10 mg/kg) on activity levels during the test phase (n = 8-10/group). C, effect of L-701,324 (veh, 1-10 mg/kg) on activity levels during the test phase (n = 10/group). D, effect of L-701,324 (veh, 0.03-0.3 mg/kg) on activity levels during the test phase (n = 10/group). *p < .05 compared with Amph CPP plus vehicle treatment (Duncan's test).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The studies reported here show that the selective, competitive AMPA receptor antagonist NBQX does not prevent the inductionof an AMPH-induced CPP, except at a dose that also produces asignificant conditioned place aversion (CPA). NBQX also had noeffect on the expression of an AMPH-induced CPP at a dose highenough to cause a significant reduction in activity. Conversely,both the less selective AMPA receptor antagonist CNQX and theglycine-site antagonist L-701,324 prevented the expression ofan AMPH-induced CPP at doses that did not affect activity levels.A summary of the relative affinities of the tested compounds forthe AMPA receptor and glycine site of the NMDA receptor is shownin Table 2.

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TABLE 2
Affinities of NBQX, CNQX, and L-701,324 for AMPA receptors and the glycine site of the NMDA receptor
IC₅₀ values for displacement of [³H]AMPA,^a [³H]glycine,^b or [³H]L-689,560^c binding in rat brain membranes. L-689,560 is a highly selective antagonist at the strychnine- insensitive glycine site of the NMDA receptor (Leeson et al., 1992

The fact that NBQX affected the induction of a CPP only at a dose that also produced a CPA suggests that AMPA receptors donot mediate the induction of an AMPH-induced CPP (experiment 1).The attenuation of the CPP seen at a dose of 30 mg/kg NBQX ismost likely explained by the aversive properties of the drug,as shown by the production of a CPA, counteracting the reinforcingeffect of AMPH. This result is consistent with previous studiesthat reported that DNQX did not prevent the induction of a CPPto cocaine and morphine (Layer et al., 1993; Cervo and Samanin,1995). However, there also are reports of intra-accumbens DNQXpreventing the induction of a CPP to cocaine (Kaddis et al., 1995)and AMPH (Layer et al., 1993). A potential problem with thesestudies is that neither included a control group that receivedDNQX alone during the conditioning phase. As experiment 1 shows,an AMPA receptor antagonist is capable of producing a marked CPA,and therefore one possible explanation for the apparent effectof DNQX is that the antagonist possesses aversive properties thatcounteract the reinforcing properties of cocaine or AMPH. In linewith this possibility, both studies reported an attenuation ofthe CPP due to DNQX, rather than a complete blockade, which isvery similar to the effect seen in the experiment reported here,at the 30 mg/kg dose of NBQX.

The fact the NBQX did not prevent the expression of the CPP at a dose (10 mg/kg) that caused a significant, although small,reduction in activity levels suggests that AMPA receptors do notmediate the expression of an AMPH-induced CPP (experiment 2).Although this study involved the use of a single dose of NBQX,testing of higher doses was not possible because of profound disruptionof locomotor activity. We have shown previously that NBQX is behaviorallyactive in the mouse strain used in this experiment at doses aslow as 3 mg/kg i.p. (Mead and Stephens, 1998). There also is evidenceto suggest that NBQX provides an effective block of AMPA receptorsin mice at doses lower than 10 mg/kg (Steppuhn and Turski, 1993;Swedberg et al., 1995). Finally, analysis of activity levels duringthe test phase of this experiment revealed that NBQX was behaviorallyactive, in that it produced a significant reduction in activitylevels.

The results from experiment 2 stand in apparent contrast to a number of reports of AMPA receptor antagonists preventing theexpression of a CPP to morphine, AMPH, and cocaine (Layer et al.,1993; Cervo and Samanin, 1995; Kaddis et al., 1995). To our knowledge,there are no previous reports of AMPA receptor antagonists failingto prevent the expression of a drug-induced CPP. One possibleexplanation of the contradiction between the current study andprevious work is that although this study used mice, all previousstudies have used rats. A second possibility is that the differencesare due to the selectivity of the antagonist used. All reportsto date revealing an attenuation or a prevention of the expressionof a CPP have involved the use of DNQX or GYKI 52466. Both ofthese compounds have an influence on NMDA-mediated transmission.DNQX has significant affinity for the glycine site of the NMDAreceptor (Kessler et al., 1989; Pellegrini-Giampietro et al.,1989; Sheardown et al., 1990; Goldstein and Litwin, 1993; Yonedaet al., 1993; Birch et al., 1988), whereas GYKI 52466 shows functionalantagonism of NMDA-induced seizures (Steppuhn and Turski, 1993).Both of these possibilities were examined in experiments 3 and4.

Experiment 3 revealed that the less selective AMPA receptor antagonist CNQX prevented the expression of an AMPH-induced CPPat doses devoid of effects on activity. CNQX is an antagonistwith a similar pharmacological profile to DNQX (Birch et al.,1988; Harris and Miller, 1989; Kessler et al., 1989; Pellegrini-Giampietroet al., 1989), although its selectivity for AMPA receptors isslightly higher (Sheardown et al., 1990). First, the fact thatan effect of CNQX was seen in our experiment at doses (1-10 mg/kgi.p) that did not affect activity levels argues against the possibilityof a species difference, as the effect of CNQX in mice was consistentwith effects of DNQX in rats. Second, it suggests that the routeof drug administration was not a decisive factor in explainingdifferences in published results. The previous reports on AMPAreceptor antagonists preventing the expression of CPP variousroutes of administration used, including intra-accumbens, intracerebroventricular,and systemic. The present study confirms that the less selectiveAMPA receptor antagonists prevent the expression of drug-inducedCPPs when given systemically. This appears to suggest that thereason for the different results found with NBQX and the otherAMPA receptor antagonists (DNQX, CNQX, and GYKI 52466) is thatthe latter substances influence NMDA receptor-mediated transmission.In particular, the affinity of CNQX and DNQX for the glycine siteof the NMDA receptor may be important for their activity in CPPexperiments. We therefore predict that a glycine-site antagonistwould also prevent the expression of an AMPH-induced CPP.

The results of experiment 4 provide evidence in support of this explanation. The selective glycine site antagonist L-701,324prevented the expression of an AMPH-induced CPP, at doses thatdid not affect activity levels. The results of test 1 were complicatedby the sedative effects of the higher dose range of L-701,324(1-10 mg/kg), although analysis revealed that these doses preventedthe expression of the CPP. Test 2, however, revealed a dose-dependenteffect of L-701,324 on the expression of the CPP, with the twohigher doses (0.1 and 0.3 mg/kg i.p.) preventing the CPP, whereasa dose of 0.03 mg/kg reduced the CPP but not significantly. Allthree of these lower doses did not affect activity levels. Recently,a similar effect of L-701,324 has been reported by Danysz et al.(1998), whereby an attenuation in the expression of a morphine-inducedCPP in rats wasobserved.

The results of the present study suggest that previous findings with the less selective AMPA receptor antagonists may be misleading.We report here that the effects of an antagonist such as CNQXdiffer from those found with the more selective antagonist NBQX.Furthermore, we report that this difference can be explained bythe action of CNQX at the modulatory strychnine-insensitive glycinesite of the NMDA receptor, as an antagonist at this site showsa similar behavioral profile to CNQX. The implications of thisstudy are not necessarily restricted to the AMPH-CPP paradigm.Further work is necessary to see whether this finding extendsto other drugs of abuse that produce a CPP, such as morphine andcocaine, although the report by Danysz et al. (1998) suggeststhat this may be the case. Perhaps more importantly, care mustbe taken in interpreting previous in vivo studies using the classof less selective AMPA receptor antagonists in otherparadigms.

It has been suggested that AMPA receptors play an important role in mediating AMPH-enhanced responding for conditioned reinforcement(Burns et al., 1994) and responding for a drug-paired stimulus(Hitchcott and Phillips, 1997). Both of these studies involvedthe use of CNQX as a method of investigating AMPA receptor involvementin the behavioral response. Similarly, many reports of drug-inducedbehavioral sensitization have also used CNQX and DNQX as toolsfor studying AMPA receptor involvement in the behavioral effectsof drugs of abuse (Karler et al., 1991, 1994; Pierce et al., 1996).Our present findings suggest it may be necessary to reexaminethe conclusions of these studies if more selective antagonistsgive rise to differenteffects.

In summary, the selective competitive AMPA receptor antagonist NBQX did not affect either the induction or the expressionof an AMPH-induced CPP. In contrast, both the less selective AMPAreceptor antagonist CNQX and the selective glycine-site antagonistL-701,324 prevented the expression of an AMPH-induced CPP. Theseresults suggest that the induction and the expression of an AMPH-inducedCPP in mice do not depend on glutamatergic transmission via AMPAreceptors but that the expression of the response is dependenton modulation of NMDA receptor-mediated transmission via the glycinesite. This importance of the glycine site of the NMDA receptorin mediating drug-induced conditioned reinforcement suggests thatcompounds acting at this site may have therapeutic potential inthe treatment of drug craving. The present study also raises doubtsconcerning the conclusions drawn from previous studies using theless selective AMPA receptor antagonists, such as DNQX and CNQX.Further work is necessary to deduce whether the conclusions drawnfrom these studies are indeedmisleading.

	Acknowledgments

We thank Dr. E. Ottow (Schering AG) for a generous gift of NBQX and CNQX and Dr. P. Hutson (Merck Sharp and Dohme) for thegenerous donation of L-701,324.

	Footnotes

Accepted for publication February 28, 1999.

Received for publication November 24, 1998.

¹ This work was supported by the Ernst Schering Forschungsgesellschaft,Berlin.

Send reprint requests to: Dr. D. N. Stephens, Laboratory of Experimental Psychology, School of Biological Sciences, University of Sussex, Falmer, Brighton BN1 9QG, United Kingdom. E-mail: dns{at}epunix.biols.susx.ac.uk

	Abbreviations

AMPH, amphetamine; CPP, conditioned place preference; NBQX, 2,3-dihydroxy-6-nitro-7-sulfamoyl-benzo(f)quinoxaline; CPA, conditioned place aversion; AMPA, $alpha$ -amino-3-hydroxy-5-methyl-4-isoxazole propionate; DNQX, 6,7-dinitroquinoxaline-2,3-dione; CNQX, 6-cyano-7-nitroquinoxalone-2,3-dione; L-701,324, 7-chloro-4-hydroxy-3-(2-phenoxy)phenyl-2(1H)-quinolone; GYKI 52466, 1-(4-aminophenyl)-4-methyl-7,8-methylene-dioxy-5H-2,3-benzodiazepine; NMDA, N-methyl-D-aspartate.

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CNQX but not NBQX Prevents Expression of Amphetamine-Induced Place Preference Conditioning: A Role for the Glycine Site of the NMDA Receptor, but not AMPA Receptors1

CNQX but not NBQX Prevents Expression of Amphetamine-Induced Place Preference Conditioning: A Role for the Glycine Site of the NMDA Receptor, but not AMPA Receptors¹