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The Journal of Neuroscience, October 1, 2001, 21(19):7781-7787
Differential Regulation of the Mesoaccumbens Circuit by Serotonin 5-Hydroxytryptamine (5-HT)2A and 5-HT2C Receptors
Lance R. McMahon1, Malgorzata Filip2, and Kathryn A. Cunningham1 1 Department of Pharmacology and Toxicology, The University of Texas Medical Branch, Galveston, Texas 77555-1031, and 2 Department of Pharmacology, Institute of Pharmacology, Polish Academy of Sciences, Krakow 31-343, Poland
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Serotonin [5-hydroxytryptamine (5-HT)] 5-HT2A and 5-HT2C receptors (5-HT2ARs and 5-HT2CRs), which innervate the dopamine mesoaccumbens pathway, may play an important role in the behavioral effects of cocaine. To test this hypothesis, the present study measured cocaine-evoked locomotor activity after bilateral microinjection of selective 5-HT2AR and 5-HT2CR antagonists into the ventral tegmental area (VTA) or the nucleus accumbens (NAc) shell. Locomotor activity was measured after intracranial microinjection of saline (0.2 µl/side), the selective 5-HT2AR antagonist R-(+)-
-(2,3-dimethoxyphenyl)-1-[2-(4-fluorophenylethyl)]-4-piperidine methanol (M100907) (0.1 or 0.3 µg · 0.2 µl
1 · side
Key words: behavior; cocaine; nucleus accumbens; serotonin; 5-HT2A receptor; 5-HT2C receptor; ventral tegmental area
INTRODUCTION
An effective pharmacotherapy for cocaine dependence remains elusive (Klein, 1998
) despite significant advances in unraveling the neurobiological mechanisms of cocaine. Cocaine inhibits dopamine (DA), serotonin [5-hydroxytryptamine (5-HT)], and norepinephrine reuptake into presynaptic nerve terminals (Koe, 1976
Despite our understanding of the role of DA in the behavioral effects of cocaine, the utility of DA ligands as effective pharmacotherapeutic medications has been limited (Klein, 1998
Of the 14 characterized 5-HT receptors (Barnes and Sharpe, 1999
The present study used intracranial microinjection techniques and selective antagonists to examine the locus of action for 5-HT2ARs and 5-HT2CRs in regulating the mesoaccumbens pathway. Spontaneous and cocaine-stimulated activity were measured after microinjection of the selective 5-HT2AR antagonist M100907 or the selective 5-HT2CR antagonist RS 102221 into the VTA or NAc shell. M100907 was chosen for these studies because of its ~100-fold greater affinity for 5-HT2ARs versus 5-HT2CRs (Kehne et al., 1996
MATERIALS AND METHODS
Animals. Male Sprague Dawley rats (n = 60; Harlan, Houston, TX) weighing 250-300 gm at the beginning of the experiment were used. The rats were housed three per cage in standard plastic rodent cages in a colony room maintained at 21 ± 2°C and at 40-50% humidity under a 12 hr light/dark cycle (lights on at 7:00 A.M.). Rats surgically fitted with indwelling bilateral guide cannulas were housed individually. Each rat was provided with tap water and rodent chow ad libitum except during experimental sessions. All experiments were conducted during the light phase of the light/dark cycle (between 9:00 A.M. and 2:00 P.M.). All experiments were performed in accordance with the National Institutes of Health Guide for the Care and Use of Laboratory Animals.
Guide cannula surgery. Rats underwent surgical implantation of 22 gauge stainless steel bilateral guide cannulas (Small Parts Inc., Miami Lakes, FL) aimed 2 mm above the VTA (n = 32) or the NAc shell (n = 28). Each rat was anesthetized using an intramuscular injection of 43 mg/kg ketamine, 8.6 mg/kg xylazine, and 1.5 mg/kg acepromazine in physiological saline (0.9% NaCl). With the upper incisor bar of a Kopf stereotaxic instrument (David Kopf Instruments, Tujunga, CA) positioned at
3.8 mm below the interaural line and using the intersection of the bregma and the longitudinal sutures as the origin, the ventral surfaces of the bilateral guide cannulas were positioned 2 mm above the VTA [at a ±6° angle from the midsagittal plane; anteroposterior (AP),
Apparatus. Locomotor activity was monitored and quantified using an open-field activity system (San Diego Instruments, San Diego, CA). Each clear Plexiglas chamber (40 × 40 × 40 cm) was housed within a sound-attenuating enclosure and was surrounded with a 4 × 4 photobeam matrix located 4 cm from the floor surface. Interruptions of the photobeams resulted in counts of activity in the peripheral and central fields of the chamber. Activity recorded in the inner 16 × 16 cm of the open field was counted as central activity, whereas the field bounded by the outer 16 cm band registered peripheral activity. Separate counts of peripheral and central activity were made by the control software (Photobeam Activity Software; San Diego Instruments) and stored for subsequent statistical evaluation. Video cameras positioned above the chambers permitted continuous observation of behavior without disruption.
Intracranial microinjections. Surgically implanted rats were maintained in the colony room for a minimum of 1 week before behavioral testing for acclimation to daily handling procedures. In addition, all rats were habituated to the brief confinement associated with the intracranial microinjection technique by removing the 28 gauge internal obturators, gently restraining the rat for ~3 min, and replacing the obturators. All rats were habituated to the testing environment for the 2 d (2 hr/daily) immediately preceding the start of the experiment. The animals were assigned to one of four groups according to antagonist treatment (M100907 or RS 102221) and brain locus (NAc shell or VTA). The groups received saline (0.2 µl/side) or M100907 (0.1 or 0.3 µg/side) into the NAc shell (n = 16) or VTA (n = 16) and saline (0.2 µl/side) or RS 102221 (0.05, 0.15, or 0.5 µg/side) into the NAc shell (n = 12) or VTA (n = 16). For each microinjection, the 28 gauge bilateral obturators were removed and two 33 gauge stainless steel bilateral internal cannulas (Small Parts) were positioned so as to extend 2 mm ventral to the bilateral guide cannula tips. The bilateral internal cannulas were attached to two 5 µl syringes (Hamilton Co., Reno, NV) via PE-50 tubing (Clay Adams, Parsippany, NJ). A microsyringe drive (Baby Bee; Bioanalytical Systems, Inc., West Lafayette, IN) driven by a programmable controller (Bee Hive Controller; Bioanalytical Systems) delivered a volume of 0.2 µl/side at a rate of 0.1 µl/min. After each microinjection, the bilateral internal cannulas were left in place for 1 min and the obturators were then replaced. Each microinjection was followed immediately by an injection of either saline (1 ml/kg, i.p.) or cocaine (10 mg/kg, i.p.). Horizontal locomotor activity counts were recorded and divided into 5 min bins for a total of 1 hr. Test sessions were conducted every 3 d and the order of microinjections for saline or the highest dose of antagonist was based on a Latin square design. Subsequent injections of antagonists were administered in descending order for a total of six (M100907) or eight (RS 102221) tests. Systemic cocaine injections were given every other test and only once per week.
Histology. At the end of the experiment, rats were overdosed with chloral hydrate (800 mg/kg, i.p.); brains were removed and stored in a 20% sucrose/10% formalin solution for at least 3 d before sectioning. Brain sections (50 µm) were mounted onto gelatin-coated glass slides. The brain sections were defatted, stained with cresyl violet, cleared with xylene, and coverslipped. The cannula placements were verified according to the atlas plates of Paxinos and Watson (1998)
Data analysis. Peripheral and central activity counts were combined into a single measure of horizontal activity counts and were totaled across the 60 min session for each animal. Analyses were conducted with a two-way ANOVA for repeated measures for the factors of pretreatment (0, 0.1, or 0.3 µg/side M100907 or 0, 0.05, 0.15, or 0.5 µg/side RS 102221), treatment (0 or 10 mg/kg cocaine, i.p.), and pretreatment × treatment interaction (SAS for Windows, version 6.12; SAS Institute, Cary, NC). The Student-Newman-Keuls procedure was used to analyze preplanned, pairwise comparisons; all comparisons were conducted with an experimentwise
Drugs. Drugs were dissolved in sterile 0.9% NaCl. Cocaine hydrochloride (National Institute on Drug Abuse, Bethesda, MD) was injected intraperitoneally in a volume of 1 ml/kg. R-(+)-
RESULTS
Histology
For each animal included in the analyses below, the injection cannulas projected bilaterally past the outer guide cannulas into the VTA or NAc. Figure 1 illustrates the cannula tip locations for the experiments in which M100907 was infused into the VTA (Fig. 1, left panels) and RS 102221 was infused into the NAc (Fig. 1, right panels). Inspection of brain tissue revealed slight evidence of gliosis at the site of injection, although surrounding tissue was generally intact.
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Figure 1. Histological verification of infusion sites. The location of infusions is shown for all rats that received intra-VTA infusions of M100907 (left panels) and intra-NAc infusions of RS 102221 (right panels). Plates are taken from Paxinos and Watson (1997)
Intra-VTA or NAc shell microinjection of saline
Microinjection of saline into the VTA or NAc shell followed by systemic injection of saline resulted in levels of activity (~500 counts/60 min) (Figs. 2-5) similar to those reported after systemic saline injection tested alone under identical conditions (McCreary and Cunningham, 1999
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Figure 2. Basal and cocaine-stimulated locomotor activity after microinjection of the 5-HT2AR antagonist M100907 into the VTA. A, Mean (±SEM) total horizontal activity (counts per 60 min) after intra-VTA microinjection of saline (Sal) or M100907 (M100) (0.1 or 0.3 µg/side) followed by intraperitoneal injection of saline or cocaine (Coc) (10 mg/kg). *p < 0.05 versus Sal + Sal; p < 0.05 versus Sal + Coc (Student-Newman-Keuls test). The time course of horizontal activity plotted in 15 min bins across the 60 min test session is depicted for basal (B) and Coc-stimulated (C) activity.
Intra-VTA microinjection of the 5-HT2AR antagonist M100907
To test the hypothesis that antagonism of 5-HT2ARs in the VTA would alter spontaneous or cocaine-stimulated horizontal activity, 16 rats were implanted with bilateral guide cannulas and received a microinjection of saline or M100907 (0.1 or 0.3 µg/side) followed by systemic injection of saline or cocaine (10 mg/kg). Of these, six rats exhibited cannula placements bilaterally positioned in the VTA at the level of the paranigral-parabrachial nuclei (Fig. 1, left panels). For these rats, a main effect of pretreatment (F(2,10) = 9.70; p < 0.01), treatment (F(1,5) = 18.39; p < 0.01), and a pretreatment × treatment interaction (F(2,10) = 7.55; p < 0.01) was observed for total horizontal activity summed across the 60 min session. Intra-VTA pretreatment with M100907 at a dose of 0.3 µg/side significantly attenuated horizontal activity stimulated by cocaine (p < 0.05) (Fig. 2) to levels that were not significantly different from saline-saline control levels (p > 0.05). In contrast, intra-VTA pretreatment with M100907 (0.1 or 0.3 µg/side) did not alter spontaneous horizontal activity (p > 0.05) (Fig. 2). The dose-effect nature of observed attenuation of cocaine-induced hyperactivity by intra-VTA M100907 was not dependent on the order of test as indicated by the one-way ANOVA conducted for the factor of order of test (F(5,30) = 1.35; p > 0.05).
In this experiment, five rats exhibited cannula placements at levels dorsal and dorsolateral to the VTA in the prerubral field and medial lemniscus, respectively, and these rats were assigned to an anatomical control group. For these rats, a significant main effect of treatment (F(1,4) = 20.48; p < 0.05) was observed for total horizontal activity summed across the 60 min session (data not shown). There was no main effect of pretreatment (F(2,8) = 3.19; p > 0.05) or a pretreatment × treatment interaction (F(2,8) = 0.57; p > 0.05).
Intra-VTA microinjection of the 5-HT2CR antagonist RS 102221
Sixteen rats received a microinjection of saline or the 5-HT2CR antagonist RS 102221 (0.05, 0.15, or 0.5 µg/side) followed by systemic injection of saline or cocaine (10 mg/kg). Of these, nine rats exhibited cannula placements bilaterally positioned in the VTA at the level of the paranigral-parabrachial nuclei. For these rats, a main effect of treatment (F(1,8) = 54.57; p < 0.001) was observed for total horizontal activity summed across the 60 min session (Fig. 3). There was no significant effect of pretreatment (F(3,24) = 2.27; p > 0.05) or a pretreatment × treatment interaction (F(3,24) = 1.05; p > 0.05).
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Figure 3. Basal and cocaine-stimulated locomotor activity after microinjection of the 5-HT2CR antagonist RS 102221 into the VTA. See legend to Figure 2 for explanation of this figure.
In this experiment, five rats exhibited cannula placements at levels dorsal and dorsolateral to the VTA in the prerubral field and medial lemniscus, respectively, and these rats were assigned to an anatomical control group. For these rats, a main effect of treatment (F(1,3) = 15.89; p < 0.05) was observed for total horizontal activity summed across the 60 min session (data not shown). There was no main effect of pretreatment (F(3,9) = 1.98; p > 0.05) or a pretreatment × treatment interaction (F(3,9) = 0.81; p > 0.05).
Intra-NAc shell microinjection of the 5-HT2AR antagonist M100907
Sixteen rats received a microinjection of saline or the 5-HT2AR antagonist M100907 (0.1 or 0.3 µg/side) followed by systemic injection of saline or cocaine (10 mg/kg). Of these, nine rats exhibited cannula placements bilaterally positioned in the ventromedial portion of the NAc shell at +1.7 to +2.2 mm posterior to bregma. For these rats, a main effect of treatment (F(1,8) = 76.71; p < 0.001) was observed for total horizontal activity summed across the 60 min session (Fig. 4). There was no main effect of pretreatment (F(2,16) = 0.59; p > 0.05) or a pretreatment × treatment interaction (F(2,16) = 0.86; p > 0.05). Similarly, microinfusion of M100907 (0.1 or 0.3 µg/side) ventromedial to the NAc shell (n = 4) or into the NAc core (n = 1) did not alter basal or cocaine-stimulated activity levels (data not shown)
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Figure 4. Basal and cocaine-stimulated locomotor activity after microinjection of the 5-HT2AR antagonist M100907 into the NAc shell. See legend to Figure 2 for explanation of this figure.
Intra-NAc shell microinjection of the 5-HT2CR antagonist RS 102221
To test the hypothesis that antagonism of 5-HT2CRs in the NAc shell would alter basal or cocaine-stimulated horizontal activity, 12 rats were implanted with bilateral guide cannulas and received a microinjection of saline or RS 102221 (0.05, 0.15, or 0.5 µg/side) followed by systemic injection of saline or cocaine (10 mg/kg). Of these, seven rats exhibited cannula placements bilaterally positioned in the ventromedial portion of the NAc shell at +1.7 to +2.2 mm posterior to bregma (Fig. 1B). For these rats, a main effect of pretreatment (F(3,18) = 7.02; p < 0.01), treatment (F(1,6) = 62.44; p < 0.001), and a pretreatment × treatment interaction (F(3,18) = 3.55; p < 0.05) were observed for total horizontal activity summed across the 60 min session. Intra-NAc shell pretreatment with RS 102221 at doses of 0.15 or 0.5 µg/side significantly attenuated horizontal activity stimulated by cocaine (p < 0.05) (Fig. 5) to levels that were not significantly different from saline-saline control levels (p > 0.05). In contrast, intra-NAc shell pretreatment with RS 102221 (0.05, 0.15, or 0.5 µg/side) did not alter spontaneous horizontal activity (p > 0.05) (Fig. 5). In this experiment, two rats exhibited cannula placements in the core subregion, and there was no effect of microinjection of RS 102221 (0.05, 0.15, or 0.5 µg/side) on basal or cocaine-stimulated activity in these animals (data not shown). The dose-effect nature of observed attenuation of cocaine-induced hyperactivity by intra-NAc RS 102221 was not dependent on the order of test as indicated by the one-way ANOVA conducted for the factor of order of test (F(7,48) = 1.24; p > 0.05).
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Figure 5. Basal and cocaine-stimulated locomotor activity after microinjection of the 5-HT2CR antagonist RS 102221 into the NAc shell. See legend to Figure 2 for explanation of this figure.
DISCUSSION
An effective antagonism of cocaine-induced hyperactivity was observed after microinjection of the selective 5-HT2AR antagonist M100907 (0.3 µg/side) into the VTA or the selective 5-HT2CR antagonist RS 102221 (0.15 or 0.5 µg/side) into the NAc shell. In contrast, cocaine-evoked hypermotility was unchanged after microinjection of RS 102221 into the VTA or M100907 into the NAc shell, and spontaneous locomotor activity was not altered by microinjection of M100907 or RS 102221 into either region. Based on previous findings that systemic administration of 5-HT2AR and 5-HT2B/2CR antagonists can influence some of the behavioral effects of cocaine (see the introductory remarks), the present study is the first to identify brain nuclei in which 5-HT2R subtypes function to control behavior evoked by cocaine.
The dose-related reduction of cocaine-stimulated activity but not spontaneous activity that was observed after microinjection of M100907 into the VTA, but not the NAc shell, suggests that 5-HT2ARs may exert control over the behavioral effects of cocaine through direct or indirect actions on DA cell bodies which serve as the origin of the mesoaccumbens pathway. Systemic administration of cocaine has been reported to increase 5-HT and DA efflux in the VTA in vivo (Chen and Reith, 1994
Microinjection of RS 102221 into the NAc shell, but not the VTA, antagonized the hypermotility evoked by cocaine in a dose-related manner, suggesting that functional 5-HT2CR control of mesoaccumbens pathways is distinctly regional. Systemic administration of cocaine has been shown to increase 5-HT and DA efflux in the NAc in vivo (Reith et al., 1997
Tonic stimulation of 5-HT2CRs in the NAc shell does not appear to regulate basal locomotor activity and underlying DA function, because spontaneous activity was unaffected after intra-NAc shell microinjection of RS 102221. These observations are in contrast to other studies that suggest 5-HT2CRs inhibit basal DA neurotransmission (De Deurwaerdere and Spampinato, 1999
The effective antagonism of cocaine-induced hyperactivity by intra-VTA M100907 occurred in the absence of changes in basal activity, a finding that has been consistently noted with systemic administration of M100907 (Kehne et al., 1996
Both M100907 and RS102221 are among the most selective antagonists at the 5-HT2AR and 5-HT2CR, respectively. However, both drugs do exhibit affinity for other receptors. For instance, M100907 possesses a moderate affinity for 5-HT2C,
receptors (Ki = 88, 128, and 87 nM, respectively) (Kehne et al., 1996
Previous studies have shown that stimulation of
In summary, hyperactivity evoked by systemic administration of cocaine was blocked by antagonism of 5-HT2ARs in the VTA or 5-HT2CRs in the NAc shell. These results indicate that the behavioral profile for cocaine is regulated by 5-HT2R subtypes in separate regions of the mesoaccumbens DA pathway. To the extent that specific behaviors induced by cocaine are differentially mediated by 5-HT2R subtypes located in the origin or terminal field of the mesoaccumbens pathway, the consequences of giving a nonselective 5-HT2R antagonist systemically will depend on differential control of these regions by a specific 5-HT2R subtype. Finally, determination of the potential utility of selective manipulations of 5-HT2ARs and 5-HT2CRs in the treatment of cocaine dependence will require careful analysis of whether 5-HT2ARs in the VTA and 5-HT2CRs in the NAc shell modulate other behavioral effects of cocaine in the distinctly regional manner reported here.
FOOTNOTES Received Feb. 27, 2001; revised July 9, 2001; accepted July 13, 2001.
This research was supported by the National Institute on Drug Abuse Grants DA05708 and DA06511 to K.A.C. and DA05879 to L.R.M., by a National Science Foundation-North Atlantic Treaty Organization Visiting Scientist Fellowship to M.F., and by the United States-Poland Joint Commission Maria Sklodowska-Curie Fund (M.F., K.A.C.).
L.R.M. and M.F. contributed equally to the research presented in this manuscript.
Correspondence should be addressed to Dr. Kathryn A. Cunningham, Department of Pharmacology and Toxicology, The University of Texas Medical Branch, Galveston, TX 77555-1031. E-mail: cunningham{at}utmb.edu.
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