Amphetamine-Induced Plasticity of AMPA Receptors in the Ventral Tegmental Area: Effects on Extracellular Levels of Dopamine and Glutamate in Freely Moving Rats

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The Journal of Neuroscience, August 15, 2001, 21(16):6362-6369

Amphetamine-Induced Plasticity of AMPA Receptors in the Ventral Tegmental Area: Effects on Extracellular Levels of Dopamine and Glutamate in Freely Moving Rats
Marco Giorgetti, Gregory Hotsenpiller, Peter Ward, Tara Teppen, and Marina E. Wolf
Department of Neuroscience, Finch University of Health Sciences/The Chicago Medical School, North Chicago, Illinois 60064-3095

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previous electrophysiological studies suggested that the initiation of behavioral sensitization to cocaine and amphetamineinvolves a transient increase in AMPA receptor responsivenessin the ventral tegmental area (VTA). To test this, we used invivo microdialysis to examine the effects of intra-VTA administrationof AMPA (10 µM) and NMDA (100 µM) on dopamine (DA) and glutamateefflux in the VTA and the nucleus accumbens (NAC), an importanttarget of VTA DA neurons. We compared rats treated for 5 d withsaline or 5 mg/kg amphetamine and withdrawn for 3 or 10-14 d.After 3 d of withdrawal, intra-VTA AMPA increased both NAC andVTA DA levels to a greater extent in the amphetamine group, whereasNMDA produced similar effects in the saline and amphetamine groups.This enhanced responsiveness to AMPA was no longer evident inrats tested 10-14 d after the last injection. In addition, intra-VTAAMPA but not NMDA increased both VTA and NAC glutamate levelsin rats tested 3 d after the last injection of amphetamine butnot in saline controls. After 10-14 d, the responsiveness of glutamatelevels to AMPA was no longer evident in the NAC but persistedin the VTA. Additional studies indicated that the glutamate effectin the NAC may involve increased responsiveness of DA receptorswithin the NAC. These findings establish an in vivo animal modelwith which to explore the consequences of repeated drug administrationfor AMPA receptor plasticity in the VTA. They also indicate thatrepeated amphetamine leads to potentiated interactions betweenDA and glutamatetransmission.

Key words: amphetamine; AMPA receptors; behavioral sensitization; microdialysis; nucleus accumbens; plasticity; ventral tegmental area

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Repeated amphetamine administration leads to a progressive augmentation of many behavioral effects of the drug (behavioralsensitization). Sensitization is of interest as a model for drug-inducedneuroplasticity in neuronal circuits important for addiction.In rodents, sensitization is observed as a progressive augmentationof locomotor activity that may relate to an increase in the incentiveto obtain drugs (Robinson and Berridge, 1993; Lorrain et al.,2000). There is also evidence of sensitization in human drug users(Satel et al., 1991) and normal subjects (Strakowski and Sax,1998).

Previous studies have shown that amphetamine sensitization is initiated by drug actions within the ventral tegmental area(VTA; Kalivas and Weber, 1988; Vezina and Stewart, 1990). TheVTA contains dopamine (DA) neurons, which project to the nucleusaccumbens (NAC) and other corticolimbic regions and are thoughtto constitute the anatomical substrate for drugs of abuse. Glutamateprojections to the VTA are important in determining the activityof VTA DA neurons (White, 1996), and considerable evidence suggeststhat sensitization is triggered by changes in glutamate transmissionwithin the VTA (Wolf, 1998).

Previous electrophysiological studies demonstrated an increase in the responsiveness of VTA DA neurons to the excitatory effectsof AMPA in rats tested shortly after discontinuing repeated amphetamineor cocaine administration (White et al., 1995; Zhang et al., 1997).By increasing excitatory drive, enhancement of AMPA transmissioncould account for the transient increase in DA cell activity thoughtto be critical in "transferring" sensitization to forebrain regionssuch as the NAC that are important in its maintenance and expression(Wolf, 1998). We therefore hypothesized that the induction ofbehavioral sensitization is associated with a transient long-termpotentiation (LTP)-like potentiation of AMPA transmission ontoVTA DA neurons. This hypothesis is supported by recent studiesin brain slices demonstrating that VTA DA neurons exhibit LTPand long-term depression (LTD) and that amphetamine modulatesLTD (Bonci and Malenka, 1999; Overton et al., 1999; Jones et al.,2000; Thomas et al., 2000).

Although in vitro studies are essential for characterizing synaptic plasticity in the VTA, it is well established that theinduction of sensitization involves complex neuronal circuitry(Wolf, 1998). It is therefore desirable to develop an animal model,preferably in awake rats, to study AMPA receptor plasticity afterchronic drug administration. On the basis of previous resultsdemonstrating enhanced electrophysiological responsiveness ofVTA DA neurons to AMPA (above), we predicted that increased AMPAreceptor responsiveness should be detectable in microdialysisexperiments as an increase in the ability of AMPA to drive DAcells and thus elicit DA release in the NAC. A dual-probe procedureallowed us to monitor the ability of a low dose of AMPA, administereddirectly into the VTA, to modulate extracellular levels of DAand glutamate both locally within the VTA and within the ipsilateralNAC. We found evidence of potentiated AMPA transmission withinthe VTA, as expected, and also found striking changes in the abilityof DA cell activity to modulate glutamate transmission in theNAC andVTA.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects. Male Sprague Dawley rats (Harlan, Indianapolis, IN), weighing 200-225 gm at the beginning of the experiment, wereused. After 3 d of adaptation, one group of animals was treatedwith amphetamine (5 mg/kg, i.p.), and another group was treatedwith saline (1 mg/kg, i.p.) once a day for 5 consecutive days.This amphetamine regimen produces robust behavioral sensitizationthat is evident throughout the withdrawal period examined in thepresent study (Wolf and Jeziorski, 1993). Probes were implanted48 hr after the last injection, and the microdialysis experimentwas performed 24 hr after the probe implantation surgery. Theanimals, maintained on a 12 hr light/dark cycle, were housed twoor three per cage before surgery and individually after surgery.Food and water were available ad libitum. All experimental procedureswere performed in strict accordance with the National Institutesof Health Guide for the Care and Use of Laboratory Animals andwere approved by the Institutional Animal Care and UseCommittee.

Surgery. Before surgery, rats were anesthetized with sodium pentobarbital (50 mg/kg, i.p.; Abbott Laboratories, North Chicago,IL) and then placed in a stereotaxic frame. Microdialysis probeswere implanted ipsilaterally in the right NAC and VTA at the followingcoordinates relative to bregma and the dura: anteroposterial (AP),1.7; lateral (L), 1.0; and dorsoventral (DV), $-$ 8 (for the rightNAC); and AP, $-$ 5.8; L, 0.5; and DV, $-$ 9 (for the right VTA). NACprobes had 2 mm of exposed membrane, whereas VTA probes had 1mm of exposed membrane. These coordinates were determined accordingto the atlas of Paxinos and Watson (1997). Dialysis probes wereprepared using 23 gauge stainless steel and silica capillary tubing.The dialysis fiber (inner diameter, 0.22 mm; outer diameter, 0.31mm; 2 mm long; Dasco) was prepared from a polyacrilonitrile-sodiummethalyl sulfonate copolymer with a molecular weight cutoff of $>=$ 15,000Da.

In vivo microdialysis. Twenty-four hours after probe implantation, saline- or amphetamine-pretreated rats were connected toa microperfusion pump (CMA 100; CMA Microdialysis, North Chelmsford,MA) with a plastic syringe (1 ml vol; Becton Dickinson, MountainView, CA). The NAC and VTA were perfused simultaneously usingartificial CSF with the following composition (in mM): NaCl, 145;KCl, 2.7; MgCl₂, 1; CaCl₂, 1.2; and Na₂HPO₄, 2, pH 7.40. The perfusionrate was set at 2 µl/min with a collection time for each sampleof 30 min, such that 60 µl of perfusate was collected. The samplewas immediately split for separate HPLC analysis of glutamateand DA; 40 µl was used to determine DA levels, and 20 µl was usedfor glutamate analysis. However, treatment group numbers for DAand glutamate levels are not always equivalent, primarily becauseof problems with chromatography for some glutamate samples. Ina second study (see Fig. 6), additional saline- and amphetamine-treatedrats were implanted with a single probe in the right NAC to investigatethe effects of local administration of DA and DA agonists (SKF38393 and quinpirole) on extracellular glutamatelevels.

Measurement of DA levels in microdialysis samples. The perfusate was assayed for DA content by reverse-phase HPLC coupledwith electrochemical detection. The mobile phase was composedof 75 mM NaH₂PO₄, 1.5 mM SDS, 25 µM EDTA, 15% acetonitrile, and12.5% methanol; this was adjusted to pH 5.6 with sodium hydroxide.The mobile phase was delivered at a flow rate of 1 ml/min (model582, Solvent Delivery Module; ESA, Chelmsford, MA) through a HR-80column (C18, 4.6 × 80 mm, 3 µm; ESA). DA was detected using acoulometric detector (Coulochem II, 5200A; ESA) coupled to a dualelectrode analytical cell (model 5014B; ESA) tailored for usein the analysis of microdialysates. The potential applied to theworking electrode was 150 mV; under these conditions, the limitof detection of DA was ~2-3 fmol. Data were taken by a chart recorder(model RYYT; Bioanalytical Systems, West Lafayette, IN) and quantifiedusing DA standards at differentconcentrations.

Measurement of glutamate levels in microdialysis samples. Analysis of amino acids was performed as described previously (Xueet al., 1996). An internal standard (carboxymethylcysteine; Sigma,St. Louis, MO) was added after collection, and dialysates werefrozen ( $-$ 80°C) for 1-7 d before analysis. Precolumn derivitizationwith o-pthalaldehyde and $beta$ -mercaptoethanol was performed by anautoinjector (SIL-10A; Shimadzu Scientific Instruments, Columbia,MD) as described by Donzanti and Yamamoto (1988). Samples in theautoinjector were maintained at 14°C by a Peltier thermoelectricsample cooler. The sample and reagent were allowed to react for2 min. Then a portion of the mixture was injected onto a Primesphere5 µm C18-HC column (100 × 4.6 mm; Phenomonex) fitted with a Primesphereguard column (30 × 4.6 mm). The mobile phase was 0.1 M phosphatebuffer containing 0.01 M EDTA, pH 6.35. Acetonitrile was usedas the organic eluent, with a gradient profile of 13-28%. Aminoacid derivatives were detected using an RF-10A fluorescence detectorwith excitation and emission wavelengths set at 325 and 425 nm,respectively. Data were taken by a personal computer using EZChrom1-2 software and quantified on the basis of peak area by comparisonwith standards injected throughout the run. Alanine was measuredas a control (nontransmitter) amino acid. Data were used onlyif alanine levels remained relatively stable during the experiment(i.e., the first and last samples were within 15% of themean).

Histological analysis. At the completion of microdialysis experiments, the animals were given an overdose of pentobarbitaland perfused through the heart with PBS followed by 10% formalinand isotonic saline. Brain coronal slices (100 µm) were stainedwith cresyl violet, and probe placement was determined by lightmicroscopy in the NAC and VTA. Rats were included in data analysisonly if at least 80% of the active region of the microdialysismembrane was located within the anatomical borders of the targetedsite. Probe locations were nearly identical to those describedand illustrated in our previous studies (Xue et al., 1996; Wolfand Xue, 1998, 1999). NAC probes were located mainly in the shell,although some sampled both core and shell. Most VTA probes werelocated between AP $-$ 5.8 to $-$ 5.3 and L 0.6-0.9. Any rat with theVTA probe $>=$ 1 mm lateral to the midline was not included. In ourprevious electrophysiological studies showing that VTA DA neuronsrecorded from amphetamine-sensitized rats exhibit increased responsivenessto glutamate and AMPA, recordings were made from 0.2 to 1.0 Lat approximately the same AP coordinates used in the present study(White et al., 1995; Zhang et al., 1997). Thus, microdialysisprobes in the present study were sampling the same area of VTArecorded in previous electrophysiologicalstudies.

Data analysis. Basal DA and glutamate levels for each rat were defined as the average of the first four samples obtained beforeAMPA administration in the VTA (or other experimental manipulation).Data are expressed as percentage of baseline. All statisticalanalysis was done with SuperAnova software (Abacus Concepts, Berkeley,CA). Within-group analyses were conducted by one-way ANOVA withtime as the repeated measure to determine whether a treatmenthad a significant effect within each experimental group (salineand amphetamine). If a significant effect was found, specificsamples within a group were compared by contrast analysis (protectedt tests that enabled comparison of the weighted mean of baselinesamples with an experimental sample or with the weighted meanof a group of experimental samples). Saline and amphetamine groupswere compared using two-way ANOVA (group × time) with repeatedmeasures on one variable (time). Post hoc between-group comparisonsof specific samples were performed using t tests with Bonferronicorrections. In all cases, significance was set at p < 0.05.

Drugs. (+)-Amphetamine sulfate was purchased from Sigma-Aldrich. Amphetamine dose refers to the salt weight. DA and AMPA wereobtained from Sigma-Aldrich. SKF 38393, quinpirole, and NMDA werepurchased from Research Biochemicals-Sigma (Natick,MA).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effect of intra-VTA administration of AMPA or NMDA on DA efflux in the NAC

Previous electrophysiological studies showed that the excitatory effect of AMPA on VTA DA cell activity was greater in ratsthat had received repeated amphetamine or cocaine injections,compared with saline controls, and that this effect was evidentat a short withdrawal time (3 d) but not a longer withdrawal time(10-14 d; Zhang et al., 1997). One goal of the present study wasto determine whether similar results could be obtained with microdialysisusing DA efflux in the NAC as a measure of mesoaccumbens DA cellactivity. Figure 1 shows results from rats treated repeatedlywith saline or amphetamine and tested 3 d after the last injection.Local administration of 10 µM AMPA in the ipsilateral VTA elicitedan increase in DA efflux from the NAC of both experimental groups,with peak levels reached 30-60 min after the onset of AMPA perfusion.However, the magnitude of the increase in DA efflux was considerablygreater in the amphetamine group. Figure 2 shows results fromdifferent saline and amphetamine groups tested 10-14 d after thelast injection. At this later withdrawal time, DA efflux in theNAC was increased to a similar extent in both groups by intra-VTAAMPA. In electrophysiological studies, the increased responsivenessseen after 3 d of withdrawal was specific to AMPA, because responsesto intra-VTA NMDA were not different between the saline and amphetaminegroups (Zhang et al., 1997). Similarly, we found no differencebetween the saline and amphetamine groups in the effect of intra-VTAadministration of 100 µM NMDA on DA efflux in the ipsilateralNAC (Fig. 3). This concentration of NMDA was chosen on the basisof a previous microdialysis study (Karreman et al., 1996).

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Figure 1. Effect of local administration of 10 µM AMPA into the VTA on DA efflux from the ipsilateral NAC of amphetamine- and saline-pretreated rats tested 3 d after the last injection. In this and all subsequent figures, the first four samples were used to calculate basal efflux, and values are expressed as a percentage of the mean basal efflux. AMPA was administered locally into the VTA for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in DA efflux over time in both the saline group (F_(7,42) = 4.36; p < 0.01) and the amphetamine group (F_(7,28) = 15.86; p < 0.001). Contrast analysis indicated significant differences between the weighted means of baseline samples (1-4) and post-AMPA samples (5-8) for both groups (p < 0.001). In the saline group, individual post-AMPA samples 6 and 7 differed significantly from baseline (p < 0.001). In the amphetamine group, individual samples 5 (p < 0.05), 6 and 7 (p < 0.001), and 8 (p < 0.01) differed from baseline. Two-way ANOVA with time as the repeated measure indicated a significant difference between the amphetamine and saline groups (group × time effect, F_(7,70) = 3.11; p < 0.01). Post hoc comparisons of individual samples between the saline and amphetamine groups revealed significantly higher DA efflux in the amphetamine group for samples 6 and 7 (*p < 0.05, t tests with Bonferroni corrections). In this and all subsequent figures, the results are expressed as mean ± SEM. Basal DA levels were 63.2 ± 5.3 fmol/sample in the saline group (n = 7) and 50.1 ± 6.5 fmol/sample in the amphetamine group (n = 5) and did not differ significantly between groups.

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Figure 2. Effect of local administration of 10 µM AMPA into the VTA on DA efflux from the ipsilateral NAC of amphetamine- and saline-pretreated rats tested 10-14 d after the last injection. AMPA was administered locally into the VTA for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in DA efflux over time in both the saline group (F_(7,35) = 5.08; p < 0.001) and the amphetamine group (F_(7,28) = 4.70; p < 0.01). Contrast analysis indicated significant differences between the weighted means of baseline samples (1-4) and post-AMPA samples (5-8) for both groups (p < 0.001). Two-way ANOVA with time as the repeated measure indicated no significant difference between the amphetamine and saline groups (group × time effect, F_(7,63) = 0.11; p = 0.99). Basal DA levels were 34.1 ± 6.2 fmol/sample in the saline group (n = 6) and 37.6 ± 3.6 fmol/sample in the amphetamine group (n = 5) and did not differ significantly between groups.

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Figure 3. Effect of local administration of 100 µM NMDA into the VTA on DA efflux from the ipsilateral NAC of amphetamine- and saline-pretreated rats tested 3 d after the last injection. NMDA was administered locally into the VTA for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a trend toward a significant change in DA efflux over time in both the saline group (F_(7,28) = 2.32; p = 0.053) and the amphetamine group (F_(7,28) = 2.31; p = 0.054). Two-way ANOVA with time as the repeated measure indicated no significant difference between the amphetamine and saline groups (group × time effect, F_(7,56) = 0.41; p = 0.89). Basal DA levels were 46.5 ± 4.5 fmol/sample in the saline group (n = 5) and 40.9 ± 4.9 fmol/sample in the amphetamine group (n = 5) and did not differ significantly between groups.

Effect of intra-VTA administration of AMPA or NMDA on glutamate efflux in the NAC

Because some studies have reported modulation of NAC glutamate efflux by DA agonists, it was of interest to see whether thedifference in NAC DA levels observed in saline and amphetaminegroups after 3 d of withdrawal was associated with a differencein NAC glutamate levels. Thus, NAC samples obtained at this withdrawaltime were split to also enable analysis of extracellular glutamatelevels. Administration of 10 µM AMPA into the VTA had no effecton NAC glutamate efflux in the saline group. However, in the amphetaminegroup, intra-VTA AMPA elicited a robust increase in extracellularglutamate levels in the ipsilateral NAC (Fig. 4). Intra-VTA NMDAdid not significantly alter glutamate efflux in the NAC of eithergroup (Fig. 5).

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Figure 4. Effect of local administration of 10 µM AMPA into the VTA on glutamate efflux from the ipsilateral NAC of amphetamine- and saline-pretreated rats tested 3 d after the last injection. AMPA was administered locally into the VTA for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in glutamate efflux over time in the amphetamine group (F_(7,56) = 4.85; p < 0.001) but not the saline group (F_(7,35) = 1.38; p = 0.24). Within the amphetamine group, contrast analysis indicated significant differences between the weighted means of baseline samples (1-4) and post-AMPA samples (5-8) (p < 0.001). Contrast analysis comparing the weighted mean of baseline samples to individual post-AMPA samples indicated significant increases for samples 6-8 (**p < 0.001; *p < 0.05). Basal glutamate levels were 22.1 ± 3.5 pg/µl in the saline group (n = 6) and 23.8 ± 3.3 pg/µl in the amphetamine group (n = 9) and did not differ significantly between groups.

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Figure 5. Effect of local administration of 100 µM NMDA into the VTA on glutamate efflux from the ipsilateral NAC of amphetamine- and saline-pretreated rats tested 3 d after the last injection. NMDA was administered locally into the VTA for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated no significant change in glutamate efflux over time in the saline group (F_(7,21) = 0.82; p = 0.59) or the amphetamine group (F_(7,21) = 0.92; p = 0.51). Two-way ANOVA with time as the repeated measure indicated no significant difference between the amphetamine and saline groups (group × time effect, F_(7,42) = 0.47; p = 0.85). Basal glutamate levels were 21.9 ± 4.8 pg/µl in the saline group (n = 4) and 5.7 ± 0.8 pg/µl in the amphetamine group (n = 4) and did not differ significantly between groups.

A number of mechanisms could explain the ability of intra-VTA AMPA to influence extracellular glutamate levels in the NACof the amphetamine group. To determine whether this effect mightinvolve a change in responsiveness to DA receptor stimulationwithin the NAC, we investigated the effects of DA agonists, applieddirectly to the NAC by reverse dialysis, on glutamate efflux insaline- and amphetamine-pretreated rats (Fig. 6). Local administrationof DA (100 µM) for 30 min elicited a significant increase in glutamateefflux from the NAC of amphetamine-treated rats, whereas the salinegroup exhibited a trend toward increased glutamate efflux thatdid not attain statistical significance. After recovery from theeffects of DA perfusion, the NAC of the same rats was perfusedwith a combination of the D1 receptor agonist SKF 38393 and theD2 receptor agonist quinpirole, each at a concentration of 10µM. The combined administration of D1 and D2 agonists eliciteda sustained increase in glutamate efflux from the NAC of amphetamine-treatedrats, whereas no significant increase was observed in the NACof control rats (Fig. 6).

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Figure 6. Effect of intra-NAC administration of 100 µM DA and a combination of 10 µM SKF 38393 and 10 µM quinpirole on glutamate efflux from the NAC of amphetamine- and saline-pretreated rats tested 3 d after the last injection. DA was administered for 30 min during sample 5. The combination of SKF 38393 and quinpirole was administered for 30 min during sample 10, after recovery from the effects of DA perfusion. One-way ANOVA with time as the repeated measure indicated a significant change in glutamate efflux over time within the amphetamine group (F_(13,52) = 2.26; p < 0.05) but not the saline group (F_(13,39) = 1.36; p = 0.22). Within the amphetamine group, contrast analysis revealed a statistically significant difference between the weighted means of the baseline samples (1-4) and the post-DA samples (5, 6) (p < 0.05, indicating a significant effect of DA), no difference between baseline samples (1-4) and "post-DA baseline samples" (7-9) (p = 0.76, indicating recovery of baseline after termination of DA perfusion), and a significant difference between baseline samples (1-4) and post-SKF+Quin samples (11-14) (p < 0.001, indicating a significant effect of the drug combination). Contrast analysis comparing the weighted mean of the baseline samples with individual postdrug samples indicated significantly higher efflux of glutamate for samples 6 and 10-14 (**p < 0.01; *p < 0.05). Basal glutamate levels were 16.5 ± 1.0 pg/µl in the saline group (n = 4) and 13.4 ± 0.8 pg/µl in the amphetamine group (n = 5) and did not differ significantly between groups.

Effect of intra-VTA administration of AMPA or NMDA on DA and glutamate efflux in the VTA

To determine whether AMPA regulated somatodendritic DA efflux differently in the saline and amphetamine groups, we comparedthe effects of intra-VTA AMPA (10 µM AMPA for 30 min) on extracellularDA levels in the VTA. Figure 7 shows results from experimentsperformed 3 d after the last injection. One-way ANOVA indicateda significant increase in DA levels over time in the amphetaminegroup, whereas the saline group showed a similar trend that didnot attain statistical significance. This suggests an augmentedresponse in the amphetamine group that parallels the effect observedin the NAC (see above). However, two-way ANOVA failed to showa significant difference between the saline and amphetamine groups.In different groups of rats tested 10-14 d after the last injection,both saline- and amphetamine-treated rats showed a significantincrease in DA levels as a result of AMPA administration, similarin magnitude to that observed in the saline group at the 3 d withdrawaltime. Two-way ANOVA did not indicate a difference between theamphetamine and saline groups (Fig. 8).

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Figure 7. Effect of local administration of 10 µM AMPA on DA efflux from the VTA of amphetamine- and saline-pretreated rats tested 3 d after the last injection. AMPA was administered for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in DA efflux over time within the amphetamine group (F_(7,28) = 5.38; p < 0.001) but not the saline group (F_(7,21) = 1.43; p = 0.25). Contrast analysis within the amphetamine group revealed a statistically significant difference between the weighted means of the baseline samples (1-4) and the post-AMPA samples (5-8) (p < 0.001). Contrast analysis comparing the weighted mean of the baseline samples with individual post-AMPA samples (5-8) indicated a significant increase in sample 6 (*p < 0.001). Basal DA levels were 31.7 ± 2.9 fmol/sample in the saline group (n = 4) and 37.0 ± 4.1 fmol/sample in the amphetamine group (n = 5) and did not differ significantly between groups.

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Figure 8. Effect of local administration of 10 µM AMPA on DA efflux from the VTA of amphetamine- and saline-pretreated rats tested 10-14 d after the last injection. AMPA was administered for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in DA efflux over time within the saline group (F_(7,35) = 2.46; p < 0.05) and the amphetamine group (F_(7,42) = 5.92; p < 0.001). Contrast analysis within the saline group revealed a statistically significant difference between the weighted mean of the baseline samples (1-4) and individual post-AMPA samples (5-7) (p < 0.05). Within the amphetamine group, there was a significant difference for samples 5-8 (p < 0.05). However, two-way ANOVA did not indicate a difference between the two groups (F_(7,77) = 0.59; p = 0.77). Basal DA levels were 20.8 ± 1.8 fmol/sample in the saline group (n = 6) and 18.3 ± 1.7 fmol/sample in the amphetamine group (n = 7) and did not differ significantly between groups.

The same samples were analyzed for glutamate to determine the effect of intra-VTA AMPA administration on glutamate effluxin the VTA. In studies performed 3 d after the last injection,a small difference was observed between the saline and amphetaminegroups. One-way ANOVAs indicated that intra-VTA AMPA had no effecton glutamate efflux in the VTA of saline-treated rats but didsignificantly alter glutamate efflux in the amphetamine group.However, two-way ANOVA did not indicate a significant group difference(Fig. 9). After 10-14 d of withdrawal, intra-VTA AMPA was withouteffect in the saline group but produced a robust increase in theamphetamine group (Fig. 10).

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Figure 9. Effect of local administration of 10 µM AMPA on glutamate efflux from the VTA of amphetamine- and saline-pretreated rats tested 3 d after the last injection. AMPA was administered for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in glutamate efflux over time within the amphetamine group (F_(7,49) = 3.32; p < 0.01) but not the saline group (F_(7,42) = 1.72; p = 0.13). Within the amphetamine group, contrast analysis revealed a statistically significant difference between the weighted means of the baseline samples (1-4) and the post-AMPA samples (5-8) (p < 0.001). Contrast analysis comparing the weighted mean of the baseline samples with individual post-AMPA samples (5-8) indicated significantly higher efflux of glutamate for samples 5-8 (**p < 0.01; *p < 0.05). Basal glutamate levels were 18.8 ± 2.7 pg/µl in the saline group (n = 7) and 18.0 ± 2.3 pg/µl in the amphetamine group (n = 8) and did not differ significantly between groups.

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Figure 10. Effect of local administration of 10 µM AMPA on glutamate efflux from the VTA of amphetamine- and saline-pretreated rats tested 10-14 d after the last injection. AMPA was administered for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in glutamate efflux over time within the amphetamine group (F_(7,35) = 2.59; p < 0.05) but not the saline group (F_(7,35) = 0.78; p = 0.61). Within the amphetamine group, contrast analysis revealed a statistically significant difference between the weighted means of the baseline samples (1-4) and the post-AMPA samples (5-8) (p < 0.01). Contrast analysis comparing the weighted mean of the baseline samples with individual post-AMPA samples (5-8) indicated significantly higher efflux of glutamate for samples 6 (*p < 0.05) and 7 (**p < 0.001). Basal glutamate levels were 16.5 ± 2.4 pg/µl in the saline group (n = 6) and 11.5 ± 1.3 pg/µl in the amphetamine group (n = 6) and did not differ significantly between groups.

Intra-VTA administration of NMDA increased VTA DA efflux to the same magnitude in both groups, with a slightly delayed effectobserved in the amphetamine group (Fig. 11). Analysis of the samesamples for glutamate suggested a trend toward increased glutamateefflux in both groups, although one-way ANOVA failed to indicatea statistically significant change over time in either group (Fig.12). Two-way ANOVA indicated no difference between the groups.

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Figure 11. Effect of local administration of 100 µM NMDA on DA efflux from the VTA of amphetamine- and saline-pretreated rats tested 3 d after the last injection. NMDA was administered for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated a significant change in DA efflux over time within the saline group (F_(7,28) = 9.87; p < 0.001) and the amphetamine group (F_(7,28) = 14.52; p < 0.001). For both groups, contrast analysis revealed a statistically significant difference between the weighted means of the baseline samples (1-4) and the post-AMPA samples (5-8) (p < 0.01). Two-way ANOVA with time as the repeated measure indicated a significance difference between the amphetamine group and the saline group (group × time effect, F_(7,56) = 2.32; p < 0.05). Post hoc comparisons of individual samples between the saline and amphetamine groups revealed significantly higher DA efflux in the amphetamine group for sample 6 (*p < 0.05, t tests with Bonferroni corrections). Basal DA levels were 23.5 ± 4.7 pg/µl in the saline group (n = 5) and 30.1 ± 4.9 pg/µl in the amphetamine group (n = 5) and did not differ significantly between groups.

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Figure 12. Effect of local administration of 100 µM NMDA on glutamate efflux from the VTA of amphetamine- and saline-pretreated rats tested 3 d after the last injection. NMDA was administered for 30 min during sample 5. One-way ANOVA with time as the repeated measure indicated no significant change in glutamate efflux over time within the saline group (F_(7,28) = 1.73; p = 0.14) or the amphetamine group (F_(7,21) = 1.17; p = 0.36). Two-way ANOVA with time as the repeated measure indicated no significance difference between the amphetamine group and the saline group (group × time effect, F_(7,49) = 0.45; p = 0.86). Basal glutamate levels were 10.4 ± 1.8 pg/µl in the saline group (n = 5) and 12.7 ± 2.2 pg/µl in the amphetamine group (n = 4) and did not differ significantly between groups.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

There is increasing evidence that regulation of AMPA transmission in the VTA is important for neuroadaptations related tosensitization. Using in vivo microdialysis, we have demonstratedthat repeated amphetamine administration profoundly alters theability of VTA AMPA receptors to influence DA and glutamate transmissionboth locally in the VTA and downstream in the NAC. Although multipleapproaches will be necessary to characterize AMPA receptor plasticityin the VTA, the availability of a microdialysis model is an importantadvance. First, all neuronal circuits are intact, which is importantbecause brain regions other than the VTA participate in the developmentof sensitization (Kalivas and Alesdatter, 1993; Wolf et al., 1995;Khan and Shoaib, 1996; Bedingfield et al., 1997; Karler et al.,1997). Second, studies are performed in awake rats, avoiding concernsabout effects of anesthetics on glutamate transmission (Moghaddamand Bolinao, 1994).

Mesoaccumbens DA neurons are more sensitive to intra-VTA AMPA after repeated amphetamine

Intra-VTA AMPA produced a greater increase in NAC DA levels in rats treated for 5 d with amphetamine and tested after 3 dof withdrawal. Similar to results in naïve rats (Karreman etal., 1996), saline-treated rats administered a threshold doseof AMPA (10 µM) directly into the VTA showed a small increase(40-50%) in NAC DA levels. However, the same dose of AMPA eliciteda more robust increase (100%) in amphetamine-treated rats. Thisaugmented response to AMPA was transient, because it was not present10-14 d after the last injection. It was specific for AMPA, becauseintra-VTA NMDA administration produced a trend toward increasedNAC DA levels that did not differ between groups. Thus, our microdialysisdata are in complete agreement with previous electrophysiologicalstudies using the same amphetamine regimen. In those studies,AMPA (applied by microiontophoresis) was more effective at increasingDA cell firing rates after repeated amphetamine treatment; theeffect was observed 3 but not 10-14 d after the last injection,and there was no change in responsiveness to NMDA (Zhang et al.,1997).

Together, microdialysis and electrophysiological findings support the hypothesis that the excitatory drive to VTA DA neuronsis increased shortly after discontinuation of repeated stimulantadministration (Wolf, 1998). Many other findings support a linkbetween increased DA cell activity and induction of sensitization.For example, augmented responses to psychostimulant challenge(i.e., a state resembling sensitization) can be produced by repeatedelectrical stimulation of the VTA (Ben-Shahar and Ettenberg, 1994),electrical kindling of the prefrontal cortex (Schenk and Snow,1994), and pharmacological disinhibition of VTA DA cells (Steketeeand Kalivas, 1991). The transient nature of the increased responsivenessto AMPA suggests that this alteration, like other sensitization-relatedchanges in the VTA, is an early step in a cascade leading to morepersistent alterations in the NAC and other forebrain regions(Wolf, 1998). In fact, the present findings are the first to demonstratea link between chronic stimulant-induced alterations in DA cellexcitability at the level of the VTA and a change in DA (and glutamate)output in theNAC.

The mechanism by which repeated amphetamine administration alters AMPA receptor responsiveness in the VTA is unclear. Acutely,amphetamine produces a long-lasting increase in extracellularglutamate levels in the VTA (Xue et al., 1996; Wolf and Xue, 1998,1999; Wolf et al., 2000) and blocks LTD in VTA DA neurons viastimulation of D2-like receptors (Jones et al., 2000; Thomas etal., 2000). Perhaps increased glutamate levels, combined witha loss of "braking" effects normally provided by LTD, promotesstrengthening of excitatory synapses on VTA DA neurons via LTP(Jones et al., 2000; Thomas et al., 2000; Wolf, 2001).

Alterations in DA and glutamate levels in the VTA after repeated amphetamine treatment

Amphetamine- but not saline-treated rats showed a significant increase in VTA DA levels in response to intra-VTA AMPA. Thisis likely related to the increased NAC DA levels produced by intra-VTAAMPA in the amphetamine group, because both effects were evidentonly after 3 d of withdrawal and were not produced by intra-VTANMDA. Insofar as somatodendritic DA release is related to DA cellactivity, an increase in AMPA-driven DA cell firing could accountfor increased DA levels in both the VTA andNAC.

Intra-VTA AMPA increased VTA glutamate levels in amphetamine- but not saline-treated rats at both withdrawal times, althoughthe effect appeared more pronounced after 10-14 d of withdrawal.What mechanism underlies this effect? The VTA contains glutamatenerve terminals but not cell bodies. A direct effect of AMPA onglutamate release from these terminals is unlikely, given scantevidence of presynaptic AMPA receptors (Takumi et al., 1999).At the 3 d withdrawal time, it is possible that increased VTAglutamate levels are related to the AMPA-induced increase in VTADA levels (via a local effect) or the AMPA-induced increase inNAC DA levels (via a polysynaptic pathway), because both of thelatter effects are also seen at this withdrawal time. However,the saline and amphetamine groups did not differ in VTA or NACDA levels after 10-14 d of withdrawal. Alternatively, the glutamateresponse in the amphetamine group may be unrelated to a differencein DA levels per se but instead may reflect a change in VTA systemsthat respond to DA. Consistent with this, systemic cocaine elevatedVTA glutamate levels via a D1 receptor-dependent mechanism incocaine-treated rats but not saline-treated rats (Kalivas andDuffy, 1998). This effect was observed 21 d after the last cocaineinjection and could therefore be related to our findings at bothearly and late withdrawal times. On the other hand, we have reporteddecreased glutamate efflux during intra-VTA perfusion of a D1agonist in saline-treated rats and attenuation of this effectby repeated amphetamine administration (Wolf and Xue, 1998). Differencesin experimental conditions (the timing of probe implantation andcomposition of perfusion solution) may contribute to divergentfindings with D1 agonists (Wolf and Xue, 1998). The timing ofprobe implantation in the present study is most similar to thatof Kalivas and Duffy (1998).

If intra-VTA AMPA does increase VTA glutamate levels in the amphetamine group through a mechanism involving DA release andD1 receptor stimulation, that mechanism is likely to be complex.One possibility is that it involves GABA transmission. WhereasD1 receptors augment GABA_B transmission in the VTA of controlanimals, D1 receptors suppress GABA_B transmission after chroniccocaine or morphine (Bonci and Williams, 1996). We have foundthat glutamate efflux in the VTA of amphetamine-pretreated ratsis under strong inhibitory control by GABA_B receptors (Giorgettiand Wolf, 2000). If D1 receptor stimulation suppresses this inhibitorymechanism, its loss could contribute to an increase in glutamatelevels.

Repeated amphetamine alters dopaminergic regulation of NAC glutamate levels

Intra-VTA AMPA increased glutamate levels in the NAC of amphetamine- but not saline-treated rats. A possible explanation isthat AMPA activated polysynaptic circuits originating in the VTAthat ultimately increase the activity of glutamate projectionsto the NAC. This is difficult to test because of the complexityof reciprocal circuits connecting VTA and its targets (Carr andSesack, 2000). Alternatively, it could reflect direct effectsof DA on glutamate efflux from nerve terminals in the NAC, becauseintra-VTA AMPA also increased NAC DA levels in the amphetaminegroup. Testing this by application of DA antagonists to the NACis not feasible, because DA antagonists increase DA efflux viaautoreceptors and feedback loops (Moghaddam and Bunney, 1990).Therefore, we examined the effect of intra-NAC perfusion of DAitself or the combination of D1 and D2 agonists and found thatboth treatments increased NAC glutamate efflux in the amphetaminegroup but not the saline group. These results suggest that DAreceptors in the NAC are involved in mediating the increased glutamateefflux produced by intra-VTA AMPA and that these receptors aremore sensitive after repeated amphetamine treatment. Consistentwith this, intra-VTA NMDA failed to increase NAC DA levels ineither group and also failed to increase NAC glutamatelevels.

Our results are somewhat consistent with studies reporting an enhanced ability of a systemic cocaine injection to increaseNAC glutamate levels in cocaine-sensitized rats (Pierce et al.,1996; Reid and Berger, 1996; Bell et al., 2000), although we didnot observe this phenomenon in amphetamine-sensitized rats (Xueet al., 1996). In untreated rats, direct NAC application of amphetamineor quinpirole (1-100 µM) decreased glutamate efflux (Kalivas andDuffy, 1997). On the other hand, Dalia et al. (1998) found nochange in glutamate levels after perfusing NAC with D1 or D2 agonistsalone, whereas combined administration of SKF 38393 (20 mM) andquinpirole (20 or 50 mM) or administration of 10 mM amphetamineincreased glutamate levels. Neither study examined rats previouslyexposed to psychostimulants. However, a recent study showed thatAMPA receptor antagonists blocked reinstatement of drug-seekingbehavior produced by either DA or AMPA administration into theNAC (Cornish and Kalivas, 2000).

Conclusions

Shortly after discontinuation of repeated amphetamine administration, there is an enhancement of the ability of VTA AMPA receptorsto regulate DA and glutamate transmission in the VTA and the NAC.This transient alteration in AMPA transmission at the level ofthe VTA may represent a switching mechanism that enables downstreamchanges more directly involved in behavioral manifestations ofchronic drugexposure.

  FOOTNOTES

Received March 5, 2001; revised May 15, 2001; accepted May 16, 2001.

This work was supported by United States Public Health Service Grants DA09621 and DA13006, by Independent Scientist AwardDA00453, and by a grant from the National Alliance for Researchon Schizophrenia and Depression (M.E.W.). We are grateful to Dr.Matthew P. Galloway for helpfuldiscussions.
Correspondence should be addressed to Dr. Marina E. Wolf, Department of Neuroscience, Finch University of Health Sciences/TheChicago Medical School, 3333 Green Bay Road, North Chicago, IL60064-3095. E-mail: marina.wolf{at}finchcms.edu.

M. Giorgetti's present address: Department of Psychiatry, University of California San Francisco, San Francisco, CA 94143-0984.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bedingfield JB, Calder LD, Thai DK, Karler R (1997) The role of the striatum in the mouse in behavioral sensitization to amphetamine. Pharmacol Biochem Behav 56:305-310[Medline].
Bell K, Duffy P, Kalivas PW (2000) Context-specific enhancement of glutamate transmission by cocaine. Neuropsychopharmacology 23:335-344[ISI][Medline].
Ben-Shahar O, Ettenberg A (1994) Repeated stimulation of the ventral tegmental area sensitizes the hyperlocomotor response to amphetamine. Pharmacol Biochem Behav 48:1005-1009[ISI][Medline].
Bonci A, Malenka RC (1999) Properties and plasticity of excitatory synapses on dopaminergic and GABAergic cells in the ventral tegmental area. J Neurosci 19:3723-3730[Abstract/Free Full Text].
Bonci A, Williams JT (1996) A common mechanism mediates long-term changes in synaptic transmission after chronic cocaine or morphine. Neuron 16:631-639[ISI][Medline].
Carr DB, Sesack SR (2000) Projections from the rat prefrontal cortex to the ventral tegmental area: target specificity in the synaptic associations with mesoaccumbens and mesocortical neurons. J Neurosci 20:3864-3873[Abstract/Free Full Text].
Cornish JL, Kalivas PW (2000) Glutamate transmission in the nucleus accumbens mediates relapse in cocaine addiction. J Neurosci 20:RC89(1-5).
Dalia A, Uretsky NJ, Wallace LJ (1998) Dopaminergic agonists administered into the nucleus accumbens: effects on extracellular glutamate and locomotor activity. Brain Res 788:111-117[Medline].
Donzanti BA, Yamamoto BK (1988) An improved and rapid HPLC-EC method for the isocratic separation of amino acid neurotransmitters from brain tissue and microdialysis perfusates. Life Sci 43:913-922[ISI][Medline].
Giorgetti M, Wolf ME (2000) Modulation of dopamine and glutamate efflux in ventral tegmental area (VTA) and nucleus accumbens (NAC) by GABA_B and AMPA receptors in the VTA: effect of repeated amphetamine treatment. Soc Neurosci Abstr 26:789.
Jones S, Kornblum JL, Kauer JA (2000) Amphetamine blocks long-term synaptic depression in the ventral tegmental area. J Neurosci 20:5575-5580[Abstract/Free Full Text].
Kalivas PW, Alesdatter JE (1993) Involvement of N-methyl-D-aspartate receptor stimulation in the ventral tegmental area and amygdala in behavioral sensitization to cocaine. J Pharmacol Exp Ther 267:486-495[Abstract/Free Full Text].
Kalivas PW, Duffy P (1997) Dopamine regulation of extracellular glutamate in the nucleus accumbens. Brain Res 761:173-177[ISI][Medline].
Kalivas PW, Duffy P (1998) Repeated cocaine administration alters extracellular glutamate in the ventral tegmental area. J Neurochem 70:1497-1502[ISI][Medline].
Kalivas PW, Weber B (1988) Amphetamine injection into the ventral mesencephalon sensitizes rats to peripheral amphetamine and cocaine. J Pharmacol Exp Ther 245:1095-1102[Abstract/Free Full Text].
Karler R, Bedingfield JB, Thai DK, Calder LD (1997) The role of the frontal cortex in the mouse in behavioral sensitization to amphetamine. Brain Res 757:228-235[ISI][Medline].
Karreman M, Westerink BHC, Moghaddam B (1996) Excitatory amino acid receptors in the ventral tegmental area regulate dopamine release in the ventral striatum. J Neurochem 67:601-607[ISI][Medline].
Khan MA, Shoaib M (1996) Neuroanatomical localization of the effects of (+)-HA966 on locomotor activity after cocaine injections to the nucleus accumbens of rats. Brain Res 719:198-202[Medline].
Lorrain DS, Arnold GM, Vezina P (2000) Previous exposure to amphetamine increases incentive to obtain the drug: long-lasting effects revealed by the progressive ratio schedule. Behav Brain Res 107:9-19[ISI][Medline].
Moghaddam B, Bolinao ML (1994) Glutamatergic antagonists attenuate ability of dopamine uptake blockers to increase extracellular levels of dopamine: implications for tonic influence of glutamate on dopamine release. Synapse 18:337-342[ISI][Medline].
Moghaddam B, Bunney BS (1990) Acute effects of typical and atypical antipsychotic drugs on the release of dopamine from prefrontal cortex, nucleus accumbens, and striatum of the rat: an in vivo microdialysis study. J Neurochem 54:1755-1760[ISI][Medline].
Overton PG, Richards CD, Berry MS, Clark D (1999) Long-term potentiation at excitatory amino acid synapses on midbrain dopamine neurons. NeuroReport 10:221-226[ISI][Medline].
Paxinos G, Watson C (1997) In: The rat brain in stereotaxic coordinates, Compact Ed 3. San Diego: Academic.
Pierce RC, Born B, Adams M, Kalivas PW (1996) Repeated intra-ventral tegmental area administration of SKF-38393 induces behavioral and neurochemical sensitization to a subsequent cocaine challenge. J Pharmacol Exp Ther 278:384-392[Abstract/Free Full Text].
Reid MS, Berger SP (1996) Evidence for sensitization of cocaine-induced nucleus accumbens glutamate release. NeuroReport 7:1325-1329[ISI][Medline].
Robinson TE, Berridge KC (1993) The neural basis of drug craving: an incentive-sensitization theory of addiction. Brain Res Rev 18:247-291[Medline].
Satel SL, Southwick SM, Gawin FH (1991) Clinical features of cocaine-induced paranoia. Am J Psychiatry 148:495-498[Abstract/Free Full Text].
Schenk S, Snow S (1994) Sensitization to cocaine's motor activating properties produced by electrical kindling of the medial prefrontal cortex but not of the hippocampus. Brain Res 659:17-22[ISI][Medline].
Steketee JD, Kalivas PW (1991) Sensitization to psychostimulants and stress after injection of pertussis toxin into the A10 dopamine region. J Pharmacol Exp Ther 259:916-924[Abstract/Free Full Text].
Strakowski SM, Sax KW (1998) Progressive behavioral response to repeated D-amphetamine challenge: further evidence for sensitization in humans. Biol Psychiatry 44:1171-1177[ISI][Medline].
Takumi Y, Matsubara A, Rinvik E, Ottersen OP (1999) The arrangement of glutamate receptors in excitatory synapses. Ann NY Acad Sci 868:474-482[ISI][Medline].
Thomas MJ, Malenka RC, Bonci A (2000) Modulation of long-term depression by dopamine in the mesolimbic system. J Neurosci 20:5582-55856.
Vezina P, Stewart J (1990) Amphetamine administered to the ventral tegmental area but not to the nucleus accumbens sensitizes rats to systemic morphine; lack of conditioned effects. Brain Res 516:99-106[ISI][Medline].
White FJ (1996) Synaptic regulation of mesocorticolimbic dopamine neurons. Annu Rev Neurosci 19:405-436[ISI][Medline].
White FJ, Hu X-T, Zhang X-F, Wolf ME (1995) Repeated administration of cocaine or amphetamine alters neuronal responses to glutamate in the mesoaccumbens dopamine system. J Pharmacol Exp Ther 273:445-454[Abstract/Free Full Text].
Wolf ME (1998) The role of excitatory amino acids in behavioral sensitization to psychomotor stimulants. Prog Neurobiol 54:679-720[ISI][Medline].
Wolf ME (2001) The neuroplasticity of addiction. In: Toward a theory of neuroplasticity (Shaw C, McEachern J, eds), pp 359-372. Philadelphia: Taylor & Francis.
Wolf ME, Jeziorski M (1993) Coadministration of MK-801 with amphetamine, cocaine or morphine prevents rather than transiently masks the development of behavioral sensitization. Brain Res 613:291-294[ISI][Medline].
Wolf ME, Xue C-J (1998) Amphetamine and D1 receptor agonists produce biphasic effects on glutamate efflux in rat ventral tegmental area: modification by repeated amphetamine administration. J Neurochem 70:198-209[ISI][Medline].
Wolf ME, Xue C-J (1999) Amphetamine-induced glutamate efflux in the rat ventral tegmental area is prevented by MK-801, SCH 23390, and ibotenic acid lesions of the prefrontal cortex. J Neurochem 73:1529-1538[Medline].
Wolf ME, Dahlin SL, Hu X-T, Xue C-J, White FJ (1995) Effects of lesions of prefrontal cortex, amygdala, or fornix on behavioral sensitization to amphetamine: comparison with N-methyl-D-aspartate antagonists. Neuroscience 69:417-439[ISI][Medline].
Wolf ME, Xue C-J, Li Y, Wavak D (2000) Amphetamine increases glutamate efflux in the rat ventral tegmental area by a mechanism involving glutamate transporters and reactive oxygen species. J Neurochem 75:1634-1644[Medline].
Xue C-J, Ng JP, Li Y, Wolf ME (1996) Acute and repeated systemic amphetamine administration: effects on extracellular glutamate, aspartate, and serine levels in rat ventral tegmental area and nucleus accumbens. J Neurochem 67:352-363[ISI][Medline].
Zhang X-F, Hu X-T, White FJ, Wolf ME (1997) Increased responsiveness of ventral tegmental area dopamine neurons to glutamate after repeated administration of cocaine or amphetamine is transient and selectively involves AMPA receptors. J Pharmacol Exp Ther 281:699-706[Abstract/Free Full Text].

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