{kappa}-Opioid Receptor Activation Modifies Dopamine Uptake in the Nucleus Accumbens and Opposes the Effects of Cocaine

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The Journal of Neuroscience, December 15, 2000, 20(24):9333-9340

$kappa$ -Opioid Receptor Activation Modifies Dopamine Uptake in the Nucleus Accumbens and Opposes the Effects of Cocaine
Alexis C. Thompson¹, Agustin Zapata¹, Joseph B. Justice Jr², Roxanne A. Vaughan³, Lawrence G. Sharpe¹, and Toni S. Shippenberg¹
¹ Behavioral Neuroscience Branch, National Institute on Drug Abuse, National Institutes of Health, Baltimore, Maryland 21224, ² Department of Chemistry, Emory University, Atlanta, Georgia 30322, and ³ Department of Biochemistry and Molecular Biology, University of North Dakota, School of Medicine and Health Sciences, Grand Forks, North Dakota 58202

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Coadministration of $kappa$ -opioid receptor agonists ( $kappa$ -agonists) with cocaine prevents alterations in dialysate dopamine (DA) concentrationin the nucleus accumbens (Acb) that occur during abstinence fromrepeated cocaine treatment. Quantitative microdialysis was usedto determine the mechanism producing these effects. Rats wereinjected with cocaine (20 mg/kg, i.p.), or saline, and the selective $kappa$ -agonist U-69593 (0.32 mg/kg, s.c.), or vehicle, once daily for5 d. Extracellular DA concentration (DA_ext) and extraction fraction(E_d), an indirect measure of DA uptake, were determined 3 d later.Repeated cocaine treatment increased E_d, whereas repeated U-69593treatment decreased E_d, relative to controls. Coadministrationof both drugs yielded intermediate E_d values not different fromcontrols. In vitro DA uptake assays confirmed that repeated U-69593treatment produces a dose-related, region-specific decrease inDA uptake and showed that acute U-69593 administration increasesDA uptake in a nor-binaltorphimine reversible manner. RepeatedU-69593 also led to a decrease in [¹²⁵I]RTI-55 binding to the DA transporter (DAT), but did not decreasetotal DAT protein. These results demonstrate that $kappa$ -opioid receptoractivation modulates DA uptake in the Acb in a manner oppositeto that of cocaine: repeated U-69593 administration decreasesthe basal rate of DA uptake, and acute U-69593 administrationtransiently increases DA uptake. $kappa$ -agonist treatment also altersDAT function. The action of $kappa$ -agonists on DA uptake or DAT binding,or both, may be the mechanism(s) mediating the previously reported"cocaine-antagonist" effect of $kappa$ -opioid receptoragonists.

Key words: $kappa$ -opioid receptors; dopamine; dopamine uptake; cocaine; nucleus accumbens; striatum; quantitative microdialysis; rotating disk electrode voltammetry; autoradiography; Western blot; rats

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acute cocaine administration increases extracellular dopamine (DA) levels in the nucleus accumbens (Acb) by blocking the DAtransporter and inhibiting DA clearance (Reith, 1988; Ritz etal., 1990). This action underlies the reinforcing effects of cocaineand may lead to the development of compulsive drug use (Wise andBozarth, 1987; Kuhar et al., 1991). A marked enhancement of thepsychomotor stimulant and rewarding effects of cocaine occursafter repeated cocaine administration (Lett, 1989; Stewart andBadiani, 1993; Shippenberg and Heidbreder, 1995; Schenk and Partridge,1997). This phenomenon, referred to as behavioral sensitization,persists for weeks after cessation of cocaine use and is implicatedin the reinstatement of cocaine-seeking behavior (Kalivas andDuffy, 1993a; Henry and White, 1995; Shippenberg and Heidbreder,1995). Behavioral sensitization is associated with an increasein firing rate of mesolimbic DA neurons (Henry et al., 1989),an elevation of basal DA dialysate levels (Kalivas and Duffy,1993a,b; Heidbreder et al., 1996), and an increase in the basalrate of DA uptake (Ng et al., 1991; Parsons et al., 1991; Meiergerdet al., 1994; Jones et al., 1995). These adaptations in presynapticDA activity are thought to contribute to the development and long-termexpression of behavioral sensitization (Kalivas and Stewart, 1991).

Coadministration of $kappa$ -opioid receptor agonists ( $kappa$ -agonists) with cocaine prevents cocaine-induced behavioral sensitization(Heidbreder et al., 1993; Shippenberg et al., 1996) and the increasein basal DA dialysate levels that occurs during cocaine abstinence(Heidbreder and Shippenberg, 1994). Acute administration of $kappa$ -agonistsdecreases DA levels in the Acb (DiChiara and Imperato, 1988; Donzantiet al., 1992; Maisonneuve et al., 1994), and some have hypothesizedthat this action of $kappa$ -agonists, which functionally opposes theacute effect of cocaine, underlies the cocaine-antagonistic effectof repeated $kappa$ -agonists.

Changes in dialysate concentration of a neurotransmitter are traditionally attributed to changes in extracellular concentrationthat are secondary to changes in release. However, recovery ofmonoamines by the dialysis probe has been shown to vary directlywith the rate of monoamine clearance: increases in DA uptake increaseDA recovery, and decreases in DA uptake reduce DA recovery (Bungayet al., 1990; Smith and Justice, 1994; Cosford et al., 1996).Therefore, changes in dialysate monoamine concentration may becaused by changes in either release or clearance, or both. Thepresent study was conducted to test the hypothesis that $kappa$ -agonistsprevent cocaine-induced changes in DA uptake. The no net fluxmicrodialysis method (Lönnroth et al., 1987) was used to characterizebasal DA dynamics in rats after repeated administration of cocaine,the selective $kappa$ -agonist U-69593 (Lahti et al., 1985), or cocainein combination with U-69593. This method provides an unbiasedestimate of extracellular DA concentration and an indirect measureof DA uptake (Bungay et al., 1990; Justice, 1993). Rotating diskelectrode voltammetry, autoradiography, and immunoblotting werethen used, respectively, to directly assess the influence of U-69593,in the presence or absence of cocaine, on the rate of DA uptake,binding to the DA transporter (DAT), and total DAT protein inAcb and dorsal striatum(STR).

  MATERIALS AND METHODS

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Subjects
Subjects were male Sprague Dawley albino rats purchased from Charles River Farms (Wilmington, MA) or Harlan Farms (Prattsville,AL) 2-6 weeks before any manipulation. Rats were maintained infacilities at the National Institute on Drug Abuse (NIDA) (Baltimore,MD; Experiments 1, 3, 4, and 7) or in facilities at Emory University(Atlanta, GA; Experiments 2, 5, and 6). Experiments were conductedin accordance with the guidelines established by the InstitutionalAnimal Care and Use Committee (IACUC) of the Intramural ResearchProgram of the NIDA, National Institutes of Health, and the EmoryUniversity IACUC. The facilities at Emory University were fullyaccredited by the American Association for the Accreditation ofLaboratory Animal Care, and the facilities at NIDA were maintainedaccording to the Guide for Care and Use of Laboratory Animalsof the Institute of Laboratory Animals Resources, National ResearchCouncil, Department of Health, Education and Welfare, Publication(National Institutes of Health 85-23, revised1985).
Rats were housed in a colony room in groups of two, three, or five (except as noted in Experiment 1), where they were maintainedunder a constant temperature (25°C) and a 12 hr light/dark cycle(lights on at 6 A.M., Eastern Standard Time). Food and water wereavailable ad libitum.

Experiment 1: Influence of repeated U-69593 and cocaine treatment on DA_ext and E_d in the Acb
Procedure. Rats (n = 60, 275-450 gm) were implanted unilaterally with a permanent indwelling guide cannula (CMA10, CMA, Inc.,Nagog, MA) aimed at the Acb [anteroposterior, +1.4 mm; mediolateral, $-$ 1.4 mm; dorsoventral, $-$ 5.7 mm, from bregma, as illustrated inPaxinos and Watson (1986)] under sodium pentobarbital (60 mg/kg,i.p.) or Equithesin (3 ml/kg, i.p.; 9.7 gm sodium pentobarbital,42.5 gm chloral hydrate, and 21.3 gm MgSO₄ dissolved in 1 l of11% ethanol and 42% propylene glycol, v/v) anesthesia. After surgery,rats were housed individually in the colony room and allowed torecover for 1 week. After the recovery period, rats were assignedto one of four treatment groups: U-69593 + cocaine, vehicle +cocaine, U-69593 + saline, or vehicle + saline. U-69593 (0.32mg/kg, s.c.), or its vehicle (20% propylene glycol, 1 ml/kg, s.c.),was injected 20 min before the cocaine (20 mg/kg, i.p.), or itsvehicle (saline, 1 ml/kg, i.p.), once per day for 5 d. All drugswere administered in the home cage. Microdialysis was conducted3 d after the last drugtreatment.
Microdialysis. Approximately 10 hr before dialysis sample collection began, rats were placed in Plexiglas microdialysis chambers(40 × 40 × 35 cm) in a separate room where the temperature, light,and feeding conditions were maintained as described previously.A microdialysis probe (CMA10, CMA, Inc.) was inserted throughthe guide cannula and extended 2 mm from the tip of the cannulainto the Acb. The inflow line to the probe was connected to amicroinfusion pump (Harvard 22; Harvard Apparatus, South Natick,MA) via a liquid swivel (quartz-lined) and protected by a springtether. The tether was attached at one end to the liquid swiveland at the other end to a screw embedded in the cranial cementstage on the rat's head. The swivel spring assembly (Instech Laboratories,Plymouth Meeting, PA) was hung from the top of the cage by a balancearm (Instech Laboratories) to allow free movement of the rat inthe cage. The outflow tubing followed the same path as the inflowtubing, ending at the swivel inside a microcentrifuge tube. ArtificialCSF (aCSF) containing (in mM): 145 NaCl, 2.8 KCl, 1.2 CaCl₂, 1.2MgCl₂, 5.4 D-glucose, and 0.25 ascorbic acid, pH 7.2-7.4, wasperfused through the microdialysis probe at a rate of 1 µl/minfor an equilibration period of 8 hr. The flow rate was increasedto 2.2 µl/min, 2 hr before the first sample collection, and remainedat this rate for the duration of theexperiment.
Twenty minute samples were collected over a 4 hr period using the no net flux method of microdialysis as described by Justice(1993). Samples were immediately frozen on dry ice for later quantificationof the dopamine content by HPLC and electrochemical detection.All microdialysis samples were collected between 8 A.M. and 1P.M.
No net flux procedures. Four different concentrations of DA in aCSF (0, 5, 20, and 40 nM DA_in) were perfused in random orderthrough the microdialysis probe. Each concentration was perfusedfor 1 hr. No sample was collected during the first 20 min of perfusion,allowing for a period of equilibration. Thereafter, two 20 minsamples were collected at each DA concentration. Pilot studieswere conducted to determine that a 20 min equilibration time wassufficient for each DA_in, and this was confirmed during the experimentby agreement between duplicate samples at each perfused DA_in.
Histology. At the end of the experiment, rats were decapitated, and their brains were removed and frozen for later histologicalexamination. The placement of the microdialysis probe was determinedin 25 µm coronal sections taken from frozen unfixed brains usinga cryostat (Hacker Instrument, Fairfield, NJ). Data from ratswhose placement fell outside the Acb were excluded from the study(n =3).
Data analysis. The concentration of dopamine in each sample was determined by HPLC and electrochemical detection. Aliquots(20 µl) of each dialysate sample were injected onto an HPLC column(100 × 3.2 mm, inner diameter, C-18, 3 µm particulate silica gel;BAS-Phase II; Bioanalytical Systems, West Lafayette, IN). Themobile phase consisted of 0.15 M NaH₂PO₄, 1.0 mM ethylenediamine-tetra-acetate,1.6 mM sodium octyl sulfate, 13% methanol (v/v), at an apparentpH of 5.0. Mobile phase was perfused through the column at a rateof 1 ml/min using a BAS PM-80 pump. The elution time for DA underthese conditions was 3-4 min. Electrochemical detection was accomplishedusing a BAS LC-4C amperometric detector. The applied potentialwas +0.700 V versus Ag/AgCl. Samples were quantified by comparisonwith an external standard curve constructed from 40 µl aliquotsof DA solutions (0-100 nM in aCSF) prepared fresh each day andtreated in a manner identical to the microdialysis samples. Sensitivityfor DA was >1 nM.
The dialysate DA data from each rat (DA_out) were used to construct a linear equation that described the change in the perfusateDA concentration (DA_in) that resulted from dialysis: the net changein DA (DA_in $-$ DA_out) was regressed against DA_in to derive thislinear equation. The dependent variables were extracellular DAconcentration (DA_ext), an estimate of extracellular DA concentrationthat is independent of relative recovery of DA, and extractionfraction (E_d), the rate of DA delivery from the probe to the tissueand an indirect measurement of the rate of DA uptake. The dependentvariables were determined from the linear regression equationas described by Parsons et al. (1991). In a scatter plot of DA_inby DA_in $-$ DA_out, extracellular DA concentration (DA_ext) is thevalue of DA_in at which DA_in $-$ DA_out equals zero and E_d is theslope of the linearregression.
A two-way ANOVA [ $kappa$ -agonist (U-69593 or vehicle) × cocaine (cocaine or saline)] was used to assess group differences for eachdependent measure, DA_ext and E_d.

Experiment 2: Influence of repeated U-69593 treatment on DA uptake in Acb and STR tissue
Procedure. Rats (n = 14, 250-350 gm) were treated once per day for 5 d with U-69593 (0.32 mg/kg, s.c.) or vehicle. Three daysafter the last treatment, rats were decapitated, the brains wererapidly removed, and the Acb and STR were rapidly dissected toanalyze the rate of DA uptake by rotating disk electrode (RDE)voltammetry. Two additional experiments were conducted in follow-up:additional groups of rats were treated with either varying dosesof U-69593 (0.03, 0.1, or 0.32 mg/kg, s.c.) or vehicle once perday for 5 d, and DA uptake was assessed by RDE voltammetry 3 dlater (n = 28, 250-350 gm), and additional groups of rats weretreated with one dose of U-69593 (0.32 mg/kg, s.c.) or vehicleonce per day for 5 d, and changes in the kinetics of DA uptakewere assessed using RDE voltammetry 3 d later (n = 22, 250-300gm). In the latter experiment, procedures described by Povlockand Schenk (1997) were used to construct a Michaelis-Menton expressionfrom which the V_max and K_m weredetermined.
Dissections. A 4 mm section from the anterior portion of the brain was removed (beginning 3 mm posterior to the anterior pole)with the aid of a metal brain matrix. A 2 mm coronal section wasplaced on an ice-cold plate, and the Acb was removed bilaterallyby dissecting a 3 × 2 mm oval section surrounding the anteriorcommissure, which typically yielded 10-15 mg of tissue. The STRwas removed by cutting out a 4 mm round section from the centerof the left or right STR. Only a single STR was used (left andright sampledalternately).
DA uptake assay. After dissection, the Acb and STR tissues were quickly weighed, placed into 1.5 ml microcentrifuge tubes,and submerged in 500 µl of 4°C physiological saline buffer untilthe start of assay (5 min and 25 min later for the Acb and STR,respectively). The buffer consisted of (in mM): 124 NaCl, 3 KCl,1.24 KH₂PO₄, 1.30 MgSO₄, 2.50 CaCl₂, 26.0 NaHCO₃, and 10 D-glucose,pH 7.4, and gassed with a 95% O₂/5% CO₂ mix. The tissue was washedtwice by removing and then replacing 400 µl of the ice-cold buffer.Next, 400 µl of the cold buffer was replaced with room temperaturebuffer, and the tissue solution was increased to 37°C over 5 min.The tissue was carefully removed from the microcentrifuge tube,placed on a glass dish, and minced with two scalpel blades. Theminced tissue was placed into an electrochemical cell with 300µl of 37°C buffer. During the assay, the tissue was maintainedat 37°C, subjected to a constant stream of 95% O₂/5% CO₂ gas directedover the top of the electrochemical cell, and stirred at 4000rpm.
Voltammetric measurements were made before (~5 min) and for 1 min after a 6 µl addition of DA (100 µM in buffer). The electrochemicalcell and the supporting RDE voltammetry system were describedby Burnette et al. (1996) and Welch and Justice (1996). The appliedpotential was +450 mV versus Ag/AgCl. Data acquisition and analysiswere performed using Origin data acquisition software (MicroCal,Northampton, MA) on a 486PC.
Data analysis. The velocity of DA uptake into Acb and STR tissue was calculated from the initial rate of decay in DA concentrationthat followed the addition of DA to the electrochemical cell,as in Welch and Justice (1996). The 6 µl addition of DA increasedthe DA concentration in the minced tissue solution to 2 µM. Theincrease in DA concentration was detected as an increase in theelectrochemical oxidative current that peaked rapidly and thendecayed. The initial rate of decay in current has been shown toresult solely from the uptake of DA into the tissue through catecholaminetransporters (Schenk et al., 1990; Povlock and Schenk, 1997).Calculation of the initial velocity of DA uptake was made on 10sec of the DA decay data between 1 and 11 sec after the additionof DA to the electrochemical cell. Data were normalized to theweight of the tissue used in each experiment and expressed asthe initial velocity of DA uptake in picomoles per second pergram of wet tissueweight.
Kinetic parameters, V_max and K_m, were determined by following the procedure described in Povlock and Schenk (1997). Acb tissuesuspensions were exposed to increasing concentrations of DA (0.25,0.5, 1, 2, and 3 µM DA final concentration), and after each DAconcentration, the initial velocity was determined as describedabove. Each addition of DA took place when the DA signal fromthe previous addition had returned to the original baseline level.This experimental design has been shown to produce conditionsapproaching the apparent low-to-infinite trans experiment as characterizedby Povlock and Schenk (1997). Values of K_m and V_max were estimatedby fitting experimentally observed values of the initial velocityby each DA concentration to the Michaelis-Menten expression usingcommercially available nonlinear curve fitting software (Prism,San Diego,CA).
One-way ANOVA was used to compare the dependent measure (picomoles per second per gram of tissue weight or kinetic parameter)among treatment groups. When appropriate, specific group differenceswere identified in post hoc analyses using a Newman-Keuls pairwisecomparison of the group means test at p < 0.05.

Experiment 3: Influence of repeated U-69593 and cocaine treatment on [¹²⁵I]RTI-55 binding in Acb and STR
Procedure. Rats (n = 16, 250-350 gm) were treated once per day for 5 d with U-69593 (0.32m/kg, s.c.) or vehicle, and cocaine(20 mg/kg, i.p.) or vehicle. Three days after the last treatment,rats were killed by decapitation, and the brains were rapidlyfrozen in isopentane and stored at $-$ 80°C untilsectioned.
Autoradiography. Frozen coronal sections (20 µm), were cut and thaw-mounted onto chrome alum/gelatin-coated microscope slides,dried, and stored at $-$ 80°C until processed for autoradiography.Two coronal sections within the caudoputamen region were mountedon each slide such that two slides (four consecutive sections)per animal were prepared for labeling with [¹²⁵I]RTI-55, the ligand used to selectively label theDATs.
The brain sections were thawed to room temperature and preincubated for 30 min in 50 mM sodium phosphate buffer (NaH₂PO₄,Na₂HPO₄, pH 7.4) containing 10 mM NaCl and 0.1% bovine serum albumin(BSA). The slides were then incubated at room temperature for4 hr in the above buffer containing 1 × protease inhibitor mixture(1× PIC) and 10 nM [¹²⁵I]RTI-55 (DuPont, NEN, specific activity 2200 Ci/mmol). Sectionsused to assess total binding for DAT were incubated in the samebuffer medium with the addition of unlabeled citalopram (50 nM)to block binding to the serotonin transporter. Nonspecific bindingwas assessed with the addition of unlabeled 10 µM indatraline.After incubation the slides were washed for two 5 min periodsin cold (4°C) sodium phosphate buffer (50 mM, containing 10 mMNaCl and 0.1% BSA), dipped in cold deionized water, and desiccateduntil completely dried (~1hr).
Labeled slides and microscale standards for both radioligands were apposed to Hyperfilm-³H (both from Amersham, Arlington Heights, IL), and after 8 d ofexposure at room temperature, the films were developed using commerciallyavailable x-ray developers andfixers.
Data analysis. A Macintosh Apple Power G3 computer and a scanner (Powerlook 3000 with UMAX software) were used to digitizethe brain sections on film. The NIH Image 1.62 program (developedat the National Institutes of Health and available on the Internetat http://rsb.info.nih.gov/nih-image/) was used to construct thestandard curves and to quantify relative optical densities ofbrain regions. The Rodbard curve, y = c*[(a $-$ x)/(x $-$ d)] $and$ (1/b),was used to quantify all brain regions because it was the curveof best fit. The optical densities from four coronal sections(specific binding) were averaged for each sampled region per animal.The averaged values were converted to femtomoles of radioligandbound per milligram of tissue equivalent (Kuhar and Unnerstall,1990). Two sections per animal were used to average nonspecificbinding, which was <5% of totalbinding.
Group differences in binding (femtomoles per milligram of tissue) in Acb_shell, Acb_core, or dorsal STR were assessed statisticallyby two-way ANOVA [ $kappa$ -agonist (U-69593 or vehicle) × cocaine (cocaineor saline)] followed by simple effectprobes.

Experiment 4: Influence of repeated U-69593 and cocaine treatment on total DAT protein in Acb and STR
Procedure. Rats (n = 12, 350-420 gm) were treated with U-69593 (0.32 mg/kg, s.c.) or vehicle once per day for 5 d or, in asecond study (n = 18, 300-400 gm), treated with cocaine (20 mg/kg,i.p.), saline, or U-69593 + cocaine once per day for 5 d. Threedays later, rats were decapitated, and the Acb and STR were rapidlydissected as described in Experiment 2. The tissue was frozenfor later determination of DAT concentration by immunoblot analysis.Western blotting was performed twice using tissue from three controlrats and three rats from each treatment group each time, witheach tissue sample analyzed intriplicate.
Western blot assay of DAT protein content. Immunoblots of DAT were obtained as described previously (Vaughan et al., 1993)using antiserum 15, generated against rDAT amino acids 6-30 (Vaughanand Kuhar, 1996). Tissue (10-40 mg) from the Acb or STR was homogenized,membranes were solubilized in SDS-polyacrylamide gel sample buffer,and 50-100 µg protein was electrophoresed on 9% SDS polyacrylamidegels. After transfer to 0.45 µM nitrocellulose membranes (Schleicherand Schuell, Keene, NH) and blocking, the membranes were probedfor 1 hr with antiserum 15 diluted 1:100. Antibody binding wasdetected with [¹²⁵I]protein A (0.8 µCi/ml; New England Nuclear, Boston, MA) followedby autoradiography with Kodak Biomax film at $-$ 70°C for 12-36 hr,or by computer analysis with a Molecular Dynamics phosphorimager(Sunnyvale, CA). Standard curves performed in parallel and generatedby tissue dilution showed excellent linearity of response andclearly quantifiable differences to 10% increments in sample amounts(data not shown) (Letchworth et al., 1999).
Data analysis. Data from the two replications were combined, yielding six rats/group, and then expressed as percentage ofthe average control values for comparison in each brain region.Group differences were assessed statistically by one-way ANOVAfollowed by a Newman-Keuls pairwise comparison of the group meanstest at p < 0.05.

Experiments 5 and 6: Influence of acute U-69593 on DA uptake in Acb tissue
Procedure. The rate of DA uptake in the Acb after a single injection of U-69593 was assessed in vitro by RDE voltammetry usingthe same procedures described in Experiment 2. In Experiment 4(time course), rats (250-350 gm, n = 26) were injected with U-69593(0.32 mg/kg, s.c.) or its vehicle, and the rate of DA uptake wasdetermined 1, 2, or 4 hr later. In Experiment 5 (dose-response),rats (250-350 gm, n = 31) were treated with U-69593 (0.03, 0.10,or 0.32 mg/kg, s.c.) or its vehicle, and the rate of DA uptakewas determined 2 hrlater.
Data analysis. The initial rate of DA uptake was calculated as described in Experiment 2, and group differences by time ordose were assessed statistically by one-way ANOVA followed bya Newman-Keuls pairwise comparison of the group means test atp < 0.05.

Experiment 7: Influence of $kappa$ -opioid receptor blockade on the acute U-69593-induced increase in DA uptake in the Acb
Procedure. Rats (n = 23, 350-450 gm) were treated with a single injection of nor-binaltorphimine (nBNI)(10 mg/kg, s.c.) orvehicle (1 ml/mg sterile water), 24-48 hr before treatment withU-69593 (0.32 mg/kg, s.c.) or its vehicle. Rats were decapitated2 hr after the U-69593 treatment, and the Acb was removed foranalysis of DA uptake by RDE voltammetry. The dose and treatmentinterval for nBNI was previously shown to result in the selectiveand long-lasting blockade of $kappa$ -opioid receptors (Horan et al.,1992; Spanagel et al., 1994).
Data analysis. The initial rate of DA uptake was calculated as described in Experiment 2 and group differences were assessedstatistically by two-way ANOVA [ $kappa$ -antagonist (nBNI or vehicle)× $kappa$ -agonist (U-69593 or vehicle)] followed by simple effectprobes.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effect of repeated U-69593 + cocaine treatment on DA_ext and E_d

Histological analysis confirmed placement of the microdialysis probe within the Acb in 93% of the subjects. In these rats(n = 47), the active length of the probe was observed to lie mediallyin the anterior-posterior extent of the Acb and to traverse thedorsal-ventral length of the Acb medial to the anterior commissure(Fig. 1). No systematic group differences in placement were observed.

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Figure 1. Illustration of microdialysis probe placement ( | ) in the Acb (Experiment 1). Diagrams were adapted from Paxinos and Watson (1986) and are labeled in millimeters rostral to bregma. Acb, Nucleus accumbens; STR, dorsal striatum.

The no net flux microdialysis method was used to study changes in presynaptic DA dynamics in vivo. In contrast to conventionalmethods, this method provides an estimate of extracellular analyteconcentration and in vivo extraction fraction (Lönnroth et al.,1987; Lönnroth et al., 1989). Extraction fraction, or E_d, isa measure of the ability of the surrounding tissue to accept DAfrom the probe, and theoretical consideration of the dialysisprocess in neural tissue suggests an association between E_d andchanges in DA clearance (Bungay et al., 1990). This relationshiphas received support from empirical observations in which DA uptake,but not release or metabolism, modifies DA E_d (Justice, 1993;Smith and Justice, 1994). Increasing DA uptake facilitates diffusionof DA from the probe into tissue and increases E_d, whereas decreasingDA uptake reduces diffusion of DA into the tissue and decreasesE_d.

Figure 2 depicts the no net flux plot of the mean (±SEM) change in perfusate DA concentration (DA_in $-$ DA_out) at each DA_inand the average linear regression for each experimental groupassessed in this experiment. Mean (±SEM) basal DA_ext and E_d arereported in Table 1. DA_ext varied from 9.9 ± 2.5 nM (U-69593+ cocaine) to 13.3 ± 2.1 nM (U-69593 + saline), but did not differsignificantly among treatment groups (interaction, F_(1,43) < 1,U-69593 treatment main effect, F_(1,43) < 1; cocaine treatmentmain effect, F_(1,43) < 1). In contrast, main effects of cocainetreatment (F_(1,43) = 4.8, p = 0.03) and U-69593 treatment (F_(1,43)= 10.1, p = 0.003) were significant for E_d. After cocaine treatment,E_d was significantly increased relative to control. In contrast,after U-69593 treatment, E_d was significantly decreased relativeto control. The interaction between U-69593 and cocaine was notsignificant (F_(1,43) < 1). E_d values in rats that had receivedU-69593 with cocaine (U-69593 + cocaine, 0.18 ± 0.03) were notdifferent from controls (vehicle + saline, 0.22 ± 0.03).

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Figure 2. No net flux plot of dialysate DA data obtained from rats treated repeatedly with the $kappa$ -agonist U-69593 (0.32 mg/kg, s.c.) and/or cocaine (20 mg/kg, i.p.). Data were collected under steady-state conditions 3 d after a 5 d repeated drug treatment regimen (once per day). The no net flux plot shows the mean ± SEM gain or loss of DA (DA_in $-$ DA_out) by dialysis from perfusate containing 0, 5, 20, or 40 nM DA (DA_in), and the average linear regression, for each experimental group. An estimate of extracellular DA concentration is given by DA_ext and is that concentration of DA_in from which no DA is gained or lost during dialysis (DA_in $-$ DA_out = 0). The in vivo E_d, an indirect measure of DA uptake, is given in the slope of the line. Data are given by treatment group as follows: $black-square$ = Veh + Coc (20 mg/kg, i.p.; n = 12); = Veh + Sal (n = 12); = U-69+Coc (n = 13); $open circle$ = U-69 (0.32 mg/kg, s.c.) + Sal (n = 10). Cocaine significantly increased E_d, and U-69593 significantly decreased E_d (p < 0.05; main effects identified by two-way ANOVA). No significant group differences in DA_ext were found.


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Table 1. Basal extracellular DA concentration (DA_ext) and in vivo extraction fraction (E_d) in rat Acb 3 d after a 5 d treatment with cocaine with or without the selective $kappa$ -opioid receptor agonist U-69593

Effect of repeated U-69593 treatment on DA uptake in Acb and STR

RDE voltammetry was used to directly measure the effect of U-69593 treatment on the rate of DA uptake in Acb. As predictedfrom the microdialysis experiment, the rate of DA uptake in theAcb was significantly reduced, relative to controls, in rats thathad received the 5 d U-69593 treatment regimen (Fig. 3a) (F_(1,10)= 6.8; p = 0.03). The effect was dose-related (Fig. 3c) (F_(3,23)= 3.2; p = 0.04) and region specific, because no decrease in therate of DA uptake was observed in STR tissue from these same rats(Fig. 3b) (F_(1,12) = 3.1; p = 0.11) regardless of dose (Fig. 3d)(F_(2,24) < 1).

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Figure 3. The effect of repeated U-69593 treatment on the initial rate of DA uptake in Acb and STR. a, b, DA uptake was measured in minced Acb and STR tissue by rotating disk electrode voltammetry, 3 d after a 5 d repeated drug treatment (U-69593, 0.32 mg/kg, s.c., or vehicle, once per day,). c, d, The effect of various doses of repeated U-69593 on the initial rate of DA uptake into Acb and STR was assessed. DA uptake was measured in minced Acb and STR tissue by rotating disk electrode voltammetry, 3 d after a 5 d repeated drug treatment (U-69593 or vehicle, once per day), at the dose indicated on the x-axis. Data are presented as group means ± SEM. The numbers at the bottom of the bar = n. *p $<=$ 0.05 versus 0 mg/kg control group by one-way ANOVA.

The observed changes in the initial velocity of DA clearance after the U-69593 treatment were associated with significantincreases in both K_m (F_(1,20) = 4.84, p < 0.04) and V_max (F_(1,20)= 4.83, p < 0.04) in the Acb (Table 2).


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Table 2. Changes in the kinetic parameters of DA transport into Acb suspensions 3 d after a 5 d treatment with U-69593

Effect of repeated U-69593 + cocaine on [¹²⁵I]RTI-55 autoradiography in Acb and STR

[¹²⁵I]RTI-55 binding (femtomoles per milligram of tissue), in the presence of unlabeled 50 nM citalopram to prevent binding tothe serotonin transporter, was used to determine the influenceof repeated U-69593 treatment alone or in combination with cocaine,on DAT binding density in the Acb_shell, Acb_core, and dorsal STR.The mean (±SEM) binding density is given in Table 3 and illustratedin Figure 4. No significant interactions between U-69593 treatmentand cocaine treatment were found (F_(1,12) < 1 in each analysis).However, in the Acb, a significant main effect of U-69593 on [¹²⁵I]RTI-55 binding was found in both the shell and core regions(F_(1,12) = 5.30, p = 0.04 and F_(1,12) = 5.01, p = 0.04, respectively).In each region, repeated U-69593 treatment significantly decreased[¹²⁵I]RTI-55 binding (33 and 35% in the shell and core, respectively).The decrease in [¹²⁵I]RTI-55 binding was evident in both U-69593 + saline and U-69593+ cocaine tissues (Table 3). A similar trend, although not statisticallysignificant, was observed in the dorsal STR (F_(1,12) = 4.46, p= 0.056). No differences as a result of cocaine administrationwere observed in any statistical analyses.


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Table 3. Binding density of [¹²⁵I]RTI-55 (femtomoles per milligram of tissue) in rat Acb and dorsal STR 3 d after a 5 d treatment with cocaine and/or the selective $kappa$ -opioid receptor agonist U-69593

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Figure 4. A modified composite of the forebrain at the levels of the STR showing how four regions were sampled for [¹²⁵I]RTI-55 binding comparing control (left) and U-69593 (right) treatment. Acb core, Nucleus accumbens core subdivision; Acb shell, nucleus accumbens shell subdivision; STR, caudoputamen; Tu, olfactory tubercles. Statistical analysis on group data indicated that DAT binding was significantly reduced in U-69593 treatment rats (Table 3).

Effect of repeated U-69593 + cocaine treatment on DAT concentration in the Acb and STR

The concentration of DAT in Acb and STR tissue was assessed by immunoblot to determine whether the changes in the rate ofDA uptake induced by U-69593 and cocaine, or the combination,were the result of a change in DAT protein. The results are reportedin Table 4, and a representative Western Blot is illustratedin Figure 5. Relative to controls, DAT immunoreactivity was unchangedby repeated administration of U-69593 in either Acb (F_(1,10) =1.4, p = 0.27) or STR (F_(1,10) < 1). In contrast, a significantdifference was found between controls, repeated cocaine treatment,and repeated U-69593 + cocaine treatment groups in the Acb (F_(2,15)= 3.9, p = 0.04). In this case, repeated coadministration of cocainewith U-69593 resulted in a significant increase in DAT immunoreactivityin Acb homogenates (p < 0.05). Cocaine treatment alone producedintermediate levels of DAT immunoreactivity not statisticallydifferent from either controls or U-69593 + cocaine treatment.Similar effects were not found in the STR (F_(2,15) = 1.6, p =0.23).


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Table 4. DAT immunoreactivity in the Acb and dorsal STR 3 d after a 5 d treatment with cocaine and/or the selective $kappa$ -opioid receptor agonist U-69593

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Figure 5. Western blot analysis of dopamine transporter. Representative DAT immunoreactivity in Acb or STR homogenates from rats treated with U-69593 or vehicle (left panels), and vehicle, cocaine, or cocaine + U-69593 (right panels). Tissue was collected 3 d after a 5 d repeated treatment regimen. Comparable results were obtained in two independent experiments in which tissue from three rats per treatment group was assessed in triplicate. Statistical analyses on group data revealed a significant increase in DAT immunoactivity in Acb homogenates from U-69593 + cocaine-treated rats (Table 4).

Effect of an acute U-69593 treatment on DA uptake in Acb

In view of the changes in DA uptake after repeated treatment with U-69593, experiments were conducted to characterize theeffect of acute U-69593 administration on DA uptake. Figure 6ashows the rate of DA uptake in Acb at various time points aftera single U-69593 (0.32 mg/kg, s.c.) or vehicle injection. A significanttime-dependent increase in the rate of DA uptake in the Acb wasobserved after U-69593 administration (F_(3,22) = 5.3, p = 0.007).The greatest increase in uptake was apparent 2 hr after the injection.Figure 6b shows that this effect was dose-related (F_(3,27) = 4.2,p = 0.02).

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Figure 6. The acute effect of U-69593 on the initial rate of DA uptake in Acb. In a, DA uptake was measured in tissue minces by rotating disk electrode voltammetry 1, 2, or 4 hr after a single U-69593 injection (0.32 mg/kg, s.c.). In b, DA uptake was measured in tissue minces by rotating disk electrode voltammetry 2 hr after the various doses of U-69593 were administered. In c, the effect of nBNI (10 mg/kg, s.c.), a selective $kappa$ -opioid receptor antagonist, on the U-69593-induced increase in the rate of DA uptake in the Acb was assessed. nBNI was administered 24-48 hr before the U-69593 treatment. The initial rate of DA uptake (mean ± SEM) was determined in Acb tissue by rotating disk electrode voltammetry 2 hr after U-69593 (0.32m/kg, s.c.) treatment. Data are presented as group means ± SEM. n = the numbers at the bottom of the bars. *p < 0.05 versus control group (a, b), by one-way ANOVA. *p < 0.05 versus control group by two-way ANOVA (c).

Effect of nBNI on the acute action of U-69593 on DA uptake

nBNI (10 mg/kg, s.c.), a $kappa$ -opioid receptor antagonist, was used to determine the role of $kappa$ -opioid receptors in mediating theacute effect of U-69593 on DA uptake in the Acb. A significanttwo-way interaction between nBNI treatment and U-69593 treatmentwas found (F_(1,19) = 6.67, p < 0.02) (Fig. 6c). nBNI treatmentblocked the increased rate of DA uptake induced by a single U-69593injection. No significant effect of nBNI alone on DA uptake wasobserved.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Repeated systemic U-69593 or cocaine treatment produces opposing adaptations in presynaptic DA activity

The no net flux microdialysis method was used here to determine whether repeated administration of the selective $kappa$ -agonist,U-69593, with cocaine prevents the cocaine-induced changes inDA uptake and release that occur during the early phase of abstinencefrom cocaine. This microdialysis method provides additional informationabout the mechanism(s) that underlies changes in monoamine dialysateconcentration that cannot be obtained by conventional dialysismethods (see Results). Marked and opposing effects of repeatedU-69593 and cocaine treatment on basal DA uptake in the Acb wereobserved (Fig. 2). DA E_d was increased 3 d after the cessationof repeated cocaine administration (20 mg/kg, i.p., once per dayfor 5 d), whereas extracellular DA levels were unchanged. Thisfinding is in line with previous reports (Parsons et al., 1991;Kalivas et al., 1993a). Repeated U-69593 administration significantlydecreased DA E_d but did not change DA_ext, suggesting that in contrastto repeated cocaine administration, repeated $kappa$ -agonist administrationleads to a decrease in DA uptake andrelease.

In rats that had received U-69593 with cocaine, E_d was intermediate to that produced by each drug alone and approximated controllevels. Statistical analysis revealed significant main effectsfor U-69593 and cocaine treatments and no significant interaction,suggesting that each drug alone modified DA uptake. Thus, repeatedactivation of $kappa$ -opioid receptors during cocaine administrationmay prevent cocaine-induced alterations in DA neurotransmissionby producing long-term alterations in basal DA uptake and releasethat are opposite to those produced bycocaine.

DA uptake is decreased after repeated systemic U-69593 treatment

Direct evidence to support the conclusion that repeated U-69593 treatment decreases DA uptake was obtained using RDE voltammetrythat measures DA uptake in vitro. The initial rate of DA uptakein the Acb from U-69593-treated rats was significantly lower thanin vehicle-treated controls. The magnitude of the effect was dosedependent, and the effective doses (0.1 and 0.32 mg/kg, i.p.)were those previously shown to block behavioral sensitizationto cocaine (Heidbreder et al., 1993; Shippenberg et al., 1996).DA uptake was unaltered in STR tissue, suggesting that the effectof U-69593 administration on DA uptake is region specific (Fig.3). The changes in uptake observed in the Acb were associatedwith a significant increase in K_m (37%) and V_max (15%) (Table2). The change in K_m is consistent with the observed decreasein DA uptake; however, this effect is counteracted at least inpart by an increase in V_max. Further analysis of the kinetic consequencesof repeated $kappa$ -agonist treatment would require additional informationsuch as the number of functionaltransporters.

DAT binding and total DAT protein are altered after repeated systemic U-69593 treatment alone, or in combination with cocaine

Repeated U-69593 treatment also reduced [¹²⁵I]RTI-55 binding in the core and shell of the Acb (Fig. 4). These results providethe first demonstration that repeated U-69593 treatment downregulatesDAT in the Acb and suggest that U-69593-induced decreases in DAuptake may result from a decrease in DAT activity. Preliminarystudies suggest that the U-69593 treatment regimen decreases theB_max of [³H]WIN 35,428 (Izenwasser et al., 1997) or [¹²⁵I]RTI-55 (Sharpe et al., 1999) to DAT in the Acb. These effects,however, do not appear to be mediated by loss of protein, becauseimmunoblotting revealed no decrease in DAT immunoreactivity afterU-69593 treatment. Alternatively, repeated U-69593 treatment maylead to post-translational modifications of DAT that affect antagonistbinding and DA uptake. For example, repeated $kappa$ -agonist treatmentis associated with an upregulation of protein kinase C (PKC) activityin brain tissue (Feng et al., 1996). Activation of PKC is knownto increase DAT phosphorylation (Huff et al., 1997; Vaughan etal., 1997), promote its internalization, and decrease DA uptake(Daniels and Amara, 1999; Melikian and Buckley, 1999), consistentwith the results observed on DA uptake here. Internalization ofDAT may also affect its availability to bind [¹²⁵I]RTI-55 and DA, leading to decreased DAT binding in the absenceof a decrease in total DAT protein. Protein kinase C is also activatedby acute $kappa$ -opioid receptor stimulation, as are other signalingcascades (Belcheva et al., 1998; Zhang and Wong, 1998; Bohn etal., 2000). However, whether these effects mediate the observedchanges in DA uptake after acute $kappa$ -agonist treatment isunclear.

Repeated administration of cocaine increased DA uptake but produced no changes in total DAT protein or [¹²⁵I]RTI-55 binding to DAT. This suggests that the increases in DAuptake observed during the early phase of cocaine abstinence (Parsonset al., 1991; Meiergerd et al., 1994) (see Experiment 1 here)are not caused by an upregulation in DAT. In contrast, repeatedadministration of cocaine in combination with U-69593 produceda significant decrease in DAT binding to [¹²⁵I]RTI-55 and a significant increase in total DAT protein in theAcb (Figs. 4, 5). It is unclear how increases in DAT expression,in the face of decreased transporter binding, can account forthe normalization of DA uptake observed in rats receiving repeatedcocaine with U-69593. However, increasing evidence suggests thatchanges in DAT function (e.g., increases or decreases in DA uptake)can be dissociated from changes in protein expression and ligandrecognition sites (Kitayama et al., 1992; Lee et al., 1996 ; Kokoshkaet al., 1998).

DA uptake is increased after the acute administration of U-69593

The acute administration of $kappa$ -agonists decreases basal DA dialysate levels in the Acb (DiChiara and Imperato, 1988; Donzantiet al., 1992; Spanagel et al., 1992), an effect that has beenattributed to a decrease in DA cell firing and DA release. Thepresent voltammetry studies provide the first demonstration thatacute $kappa$ -opioid-receptor stimulation increases DA uptake ratherthan, or in addition to, decreasing DA release in the Acb (Fig.6b). The increase in DA uptake was nBNI-reversible, supportinga receptor-specific effect (Fig. 6c), and the effective dose wasthat which decreased DA uptake after repeated administration.The time course study revealed that the increase in DA uptakewas not immediate. Maximal effects were observed 2 hr after U-69593injection (Fig. 6a). These findings are particularly noteworthybecause $kappa$ -agonist-induced decreases in dialysate levels developslowly over 30-60 min. Together these data suggest that acute $kappa$ -opioid receptor activation may decrease DA neurotransmissionby two distinct mechanisms: an inhibition of release and a later-onsetincrease in DA uptake. These data also suggest that the decreasein DA uptake produced by repeated U-69593 treatment may be a compensatoryresponse to the increase in DA uptake produced by acute $kappa$ -opioidreceptoractivation.

One mechanism by which $kappa$ -agonists attenuate the behavioral and neurochemical effects of cocaine may be by modifying DA uptakein the Acb. $kappa$ -agonists may block some or all of the acute effectsof cocaine on DA activity by increasing the rate of DA uptakeor decreasing DA release, or both (Smith et al., 1992). A similarmechanism may also underlie the ability of $kappa$ -agonists to preventalterations in behavior and DA activity in the Acb. The presentstudies, however, also indicate that $kappa$ -agonists may prevent changesin behavior and DA activity that occur after cessation of repeatedcocaine administration by inducing an opposing neuronal adaptation.If this were true, concurrent administration of a $kappa$ -agonist withcocaine would not be necessary to "reverse" the cocaine-inducedneurochemical alterations. Indeed, previous work suggests that $kappa$ -agonist and cocaine treatment need not be coincidental (Shippenbergand Heidbreder, 1995; Mello and Negus, 1998).

In conclusion, the activation of $kappa$ -opioid receptors regulates DA uptake in the Acb. DA uptake is increased after acute $kappa$ -opioidreceptor activation and decreased 3 d after repeated $kappa$ -agonisttreatment. These effects oppose both the acute and long-term effectsof cocaine on presynaptic DA activity in the Acb and provide aplausible mechanism by which $kappa$ -agonists prevent alterations inbehavior that occur in response to the repeated administrationofcocaine.

  FOOTNOTES

Received May 26, 2000; revised Oct. 2, 2000; accepted Oct. 9, 2000.

Correspondence should be addressed to Dr. Alexis C. Thompson, Behavioral Neuroscience Program, Department of Psychology, ParkHall, State University of New York at Buffalo, Buffalo, NY 14260.E-mail: act2{at}buffalo.edu.
This research was supported by Intramural Research Funds from the National Institute on Drug Research to T.S.S., and NationalInstitutes of Health Grants DA10896 and DA11176 to J.B.J. Manythanks to William Rea and Heather Holden for their excellent technicalassistance.

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