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The Journal of Neuroscience, November 15, 1999, 19(22):9780-9787
Amphetamine Depresses Excitatory Synaptic Transmission via Serotonin Receptors in the Ventral Tegmental Area
Susan Jones and Julie A. Kauer Department of Neurobiology, Duke University Medical Center, Durham, North Carolina 27710
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The ventral tegmental area (VTA) is the origination zone for dopaminergic neurons involved in reward and addictive properties of a variety of abused substances. A major excitatory projection to VTA neurons originates in the medial prefrontal cortex, and several lines of evidence suggest that glutamatergic synapses on VTA neurons are activated and modified during exposure to psychostimulant drugs. Here, we report for the first time that amphetamine depresses excitatory glutamatergic synaptic transmission onto VTA neurons in the midbrain slice preparation. Unexpectedly, this depression is mediated not by activation of dopamine receptors, but instead by activation of serotonin receptors. Our findings suggest that an acute effect of amphetamine exposure is the release of serotonin in the VTA, which in turn modulates excitation of VTA neurons. This process may be an important early component of permanent changes occurring in the reward pathway that contribute to drug addiction.
Key words: ventral tegmental area (VTA); amphetamine; psychostimulants; excitatory synaptic transmission; serotonin; glutamatergic
INTRODUCTION
The ventral tegmental area (VTA) of the midbrain is the source of dopaminergic neurons that form the mesocorticolimbic projection, a major limb of the reward pathway and a target for drugs of abuse. Glutamatergic afferents originating in medial prefrontal cortex (PFC) drive VTA neurons and control their firing patterns (Gariano and Groves, 1988
; Svensson and Tung, 1989
The increased drug craving that accompanies compulsive drug taking in human drug addiction has been modeled experimentally as behavioral sensitization, a progressive and permanent augmentation of behavioral responses to drugs of abuse, including psychostimulants such as amphetamine and cocaine (Kalivas and Stewart, 1991
Substantial evidence supports the involvement of VTA dopamine cells and dopamine release in drug addiction and behavioral sensitization (DiChiara and Imperato, 1988
Despite considerable evidence that glutamatergic afferents control the firing of VTA neurons and that this pathway is essential in the development of sensitization, the effects of psychostimulants on excitatory synaptic transmission have never been tested. Here, we directly examined the acute effects of amphetamine on glutamatergic synaptic transmission, using whole-cell patch-clamp recordings from VTA neurons in midbrain slices. We also explored the hypothesis that dopamine and/or serotonin alter excitatory synaptic transmission in the VTA. We report that amphetamine directly depresses glutamatergic synaptic transmission onto VTA neurons. This is a consequence of serotonin release and does not involve dopamine receptors. The depression of excitatory synaptic transmission is a likely early event following psychostimulant administration in the naïve brain. Our results implicate serotonin in the modification of dopaminergic function in the reward pathway.
MATERIALS AND METHODS
Preparation of brain slices. Sprague Dawley rats, 16- to 23-d-old, were anesthetized with halothane and quickly decapitated. The brain was rapidly removed into ice-cold artificial CSF (ACSF) containing (in mM): NaCl 119, KCl 2.5, MgSO4 1.3, CaCl2 2.5, NaH2PO4 1.0, NaHCO3 26.0, and glucose 11, continuously gassed with 95% O2-5% CO2, pH 7.4, osmolarity of 290 mOsm. Kynurenic acid (1 mM) was included in the ACSF during slice preparation and storage. Horizontal midbrain slices (250 µm thick), dorsal to the interpeduncular fossa and containing the VTA, were cut using a vibratome, transferred to a submersion chamber at 30°C containing ACSF, and used for recordings from 1 to 6 hr after preparation.
Electrophysiology. Midbrain slices were continuously perfused with ACSF (without kynurenic acid) and warmed to 28-32°C at a flow rate of 2-4 ml/min. Picrotoxin (100 µM) was added to block GABAA receptors, to study excitatory synaptic transmission in isolation. Under low-power magnification, the location of the VTA was identified medial to the substantia nigra pars compacta and the medial terminal nucleus of the accessory optic tract. Using a 40× water immersion objective with differential interference contrast and a CCD camera, individual cells in the VTA were visualized on a monitor for whole-cell patch-clamp recordings.
Patch pipettes had resistances of 2-4 M
when filled with (in mM): potassium gluconate 100, MgCl2 5, HEPES 40, EGTA 0.6, Na2-ATP 2, and Na2-GTP 0.3, pH 7.25, osmolarity of 280 mOsm. Biocytin (0.4%) was added to allow post hoc identification of recorded cells for immunolabeling experiments (see below). Signals were amplified through an Axoclamp 2B amplifier (Axon Instruments, Foster City, CA) used in either bridge mode to record voltage signals or continuous single electrode voltage-clamp mode to record evoked EPSCs. In bridge mode, cells were allowed to fire spontaneous action potentials from their resting potential of between
50 and
The membrane potential was then voltage clamped at
Pharmacology. All drugs were added directly to the ACSF perfusing the slice chamber. Controls for solution switches were routinely performed. All agonists were added for 10 min, allowing adequate time for equilibration. Dopamine, norepinephrine, and serotonin solutions were prepared immediately before use. All antagonists were added at least 10-15 min before agonist application. In dopamine depletion experiments, littermates were given either the tyrosine hydroxylase inhibitor
-methyl-para-tyrosine or saline vehicle in double-blind experiments [200-300 mg/kg, i.p., at least 2 hr before slice preparation (Spector et al., 1965
Drug effects were assessed by averaging EPSC amplitudes for 5-10 min during the peak response and comparing this value with 10 min of averaged data just before drug application and are reported as mean ± SEM throughout the text. Significance was measured using unpaired t tests.
Immunolabeling for tyrosine hydroxylase. Immediately after recording, slices were fixed in 4% paraformaldehyde for at least 24 hr. Slices were immersed in a 30% sucrose solution and resectioned at 50-90 µm on a freezing microtome. Slices were then preincubated for 2 hr in 0.5% BSA with 0.1% Triton X-100 and incubated overnight in mouse anti-tyrosine hydroxylase antibody (1:1000) at 4°C. This was followed by incubation for 1 hr in cy3-conjugated goat anti-mouse secondary antibody (1:500) and then a 1 hr incubation in FITC-conjugated extravidin (1:200).
Identification of dopamine neurons. To determine whether cells used for recordings were dopamine cells or VTA interneurons, a combination of physiology and immunohistochemistry was used (Table 1; Fig. 1). Thirty-three percent (43 of 129) of biocytin-labeled cells were recovered, and of these, 63% (27 of 43 cells) were positive for TH (the rate-limiting enzyme in catecholamine synthesis). In general, these TH-positive cells had clear dopamine cell physiological characteristics (described below), although four cells with nondopamine cell characteristics were also TH-positive. All cells showing TH-positive staining were considered to be dopamine cells, regardless of physiological characteristics. Cells were classified into three groups based on the presence of a depolarizing sag in response to negative current step injections. Those showing a >25% end-of-step change in voltage were classed as dopamine cells (81%, 104 of 129 cells) (Fig. 1B). Those showing a <15% end-of-step change in voltage, or no sag (6%, 8 of 129 cells), were classed as nondopamine cells unless TH-positive (2 of 8 of these cells were TH-positive). Those showing end-of-step voltage changes of between 15 and 25% (intermediate sags; 9%, 12 of 129 cells) were classed as dopamine cells only if TH-positive (2 of 12 cells). In the dopamine cell class, mean spontaneous firing rate was 1.5 ± 0.2 Hz in 87 cells tested (22% of these cells showed no spontaneous activity). Cells showing no sag were either silent or fired at high frequency (>5 Hz). Intermediate cells spontaneously fired similarly to dopamine cells (1.6 ± 0.5 Hz; n = 11; 36% showed no spontaneous activity). All figure legends report the number of cells classed as dopamine cells for each experimental group.
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Table 1. Classification of VTA cells by tyrosine hydroxylase immunolabeling and physiology
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Figure 1. Characterization of VTA cells. A, Left (i) shows biocytin fill of the recorded cell, and right (ii) shows that the same cell is TH-positive. B, Physiological responses from the cell pictured in A showing typical dopamine cell characteristics: spontaneous firing and a distinctive voltage sag response to hyperpolarizing current.
Materials. Standard lab chemicals were obtained from Mallinckrodt (St. Louis, MO), Aldrich (Milwaukee, WI), or Fluka (Buchs, Switzerland). Biocytin, extravidin, and BSA were obtained from Sigma (St. Louis, MO), ATP and GTP were obtained from Boehringer Mannheim (Indianapolis, IN), TH monoclonal antibody was obtained from DiaSorin (Stillwater, MN), and goat anti-mouse IgG was obtained from Chemicon (Temecula, CA). All agonists, antagonists, and amphetamine were obtained from Research Biochemicals (Natick, MA).
RESULTS
Neurons recorded from within the VTA were classed as dopamine cells or nondopamine cells based on their physiological and morphological characteristics; a typical dopamine cell is shown in Figure 1. The data from all cells are summarized in Table 1. EPSCs recorded from dopamine neurons at
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Figure 2. Excitatory postsynaptic currents in a VTA dopamine cell (TH-positive). Single records from one experiment showing (from top to bottom) a typical EPSC recorded at
Psychostimulants increase extracellular glutamate levels in the VTA measured using in vivo microdialysis (Kalivas and Duffy, 1995
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Figure 3. Effect of amphetamine on EPSCs in VTA cells. Aa, Time course data from one dopamine cell showing reproducible depression of EPSC amplitude (normalized to predrug values) in response to repetitive applications of amphetamine (10 µM, 10 min; bars). Ab, Example records (average of 5-10 traces) showing control EPSCs and EPSCs in the presence of amphetamine at the indicated times during the experiment (1-3). B, Averaged time course data from seven experiments showing the reversible depression of the EPSC by amphetamine (10 µM, 10 min; bar). For this and all figures showing averaged data, only every third error bar is shown for clarity. Five of the seven cells were dopamine cells. C, Concentration-response graph for depression of EPSC amplitude (percentage) by amphetamine. Nineteen of 26 cells included in this graph were dopamine cells.
Having found that amphetamine decreases glutamate synaptic transmission, we next tested the idea that amphetamine causes this depression of the glutamatergic EPSC via the release of dopamine. When we examined the effect of exogenously applied dopamine, we found that, at high concentrations, dopamine mimicked amphetamine, depressing the amplitude of the EPSC (38 ± 5% depression) (Fig. 4A). The threshold for the effect of dopamine was ~10 µM, with 100 µM causing a robust response (Fig. 4A, inset). To determine which dopamine receptors might mediate the effect of amphetamine, selective agonists and antagonists for D1 and D2 dopamine receptors were used. Although dopamine depressed the EPSC, the D1 antagonist SCH 23390 (2 µM), the D2 antagonist sulpiride (10 µM), or a combination of both antagonists did not affect the ability of amphetamine to depress the EPSC (Fig. 4B,C); this result suggested that dopamine receptors are not involved in depressing excitatory synaptic transmission. In agreement with this interpretation, the D1 agonist SKF 82958 (10 µM) and the D2 agonist quinpirole (30 µM) evoked only very small depressions of the EPSC amplitude (SKF 82958, 8 ± 3%; n = 4; quinpirole, 14 ± 4%; n = 5) (data not shown).
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Figure 4. Dopamine does not mediate the effect of amphetamine. A, Time course data from eight experiments showing the reversible depression of EPSC amplitude (normalized to control values) by a high concentration of dopamine (100 µM, 10 min). Seven of the eight cells were dopamine cells. Inset shows concentration dependence of the depression of EPSC amplitude by dopamine. Thirteen of 15 cells used for this bar chart were dopamine cells. B, Time course data showing the combined data from four cells (open symbols) illustrating that the effect of amphetamine on EPSC amplitude in the presence of both 2 µM SCH 23390 and 10 µM sulpiride is superimposable with the control response (filled symbols; from Fig. 3A). C, Bar chart summarizing the lack of effect of the dopamine D1 and D2 antagonists SCH 23390 (2 µM) and sulpiride (10 µM) on the response to amphetamine (patterned bars). Thirteen of 16 cells used for the dopamine antagonist studies were dopamine cells. The filled bar illustrates that pretreatment of animals with the tyrosine hydroxylase inhibitor
As a control to ensure that amphetamine was able to release dopamine in our slices, we monitored the effect of amphetamine on the spontaneous activity of dopamine cells, in either cell-attached patch mode or whole-cell current-clamp mode, allowing the cells to fire action potentials. In both configurations, amphetamine (10 µM) completely suppressed spontaneous firing in two cells (data not shown); in two other cells, this effect of amphetamine on spontaneous activity was prevented by sulpiride (10 µM) (data not shown), demonstrating that D2 receptors are responsible, as reported previously (Seutin et al., 1991
Because the effect of amphetamine on glutamate synaptic transmission does not appear to be via dopamine release and activation of dopamine receptors, this suggested that it might be via the known effect of amphetamine on transporters for either norepinephrine or serotonin. Norepinephrine itself had little effect on EPSC amplitude, causing 11.3 ± 1.8% depression at 10 µM (n = 4). Furthermore, the effect of amphetamine was not significantly inhibited by
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Figure 5. Serotonin mimics the effect of amphetamine. A, Time course data from one dopamine cell showing reversible depression of EPSC amplitude (normalized to predrug values) in response to serotonin (10 µM, 10 min; bar). Inset shows example records (average of 5-10 traces) showing control EPSCs and EPSCs in the presence of serotonin. B, Time course data from six cells showing the reversible depression of EPSC amplitude (normalized to control values) by serotonin (10 µM, 10 min; 5-HT). Four of six cells were dopamine cells. Inset shows concentration dependence of the effect of serotonin in depressing EPSC amplitude (percentage). Nine of 13 cells used for this bar chart were dopamine cells.
To elucidate the involvement of serotonin receptors in mediating the effect of amphetamine, we examined the effects of amphetamine in the presence of serotonin receptor antagonists. Ketanserin (100 nM), a selective 5-HT2 receptor antagonist, did not block the effects of amphetamine (amphetamine-induced depression of the EPSC, 32 ± 4%; n = 3) (data not shown). However, two broad spectrum serotonin receptor antagonists prevented amphetamine from depressing excitatory synaptic transmission. Methysergide (10 µM) completely blocked the effect of amphetamine on the EPSC (amphetamine-induced depression of EPSC in the presence of methysergide, 3 ± 2%; n = 5) (Fig. 6A). Methiothepin (1 µM), a structurally distinct serotonin antagonist, also significantly inhibited the effect of amphetamine on EPSCs (amphetamine-induced depression of EPSC in the presence of methiothepin, 11 ± 5%; n = 5) (Fig. 6B); in two of five cells, methiothepin caused a complete block of the response to amphetamine. Methysergide also inhibited the depressant effect of 10 µM serotonin (to 18 ± 4%; n = 5). The effect of 100 µM dopamine was also blocked by methysergide (to 15 ± 5%; n = 3), supporting the idea that, at this high concentration, dopamine actually binds to serotonin receptors to reduce the EPSC. These results strongly suggest that the depression of excitatory synaptic transmission onto VTA dopamine neurons by amphetamine is mediated by serotonin receptors.
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Figure 6. Serotonin receptors mediate the effect of amphetamine. A, Time course data from five cells (open symbols) illustrating that the effect of amphetamine is almost completely blocked in the presence of methysergide (10 µM) compared with control data (filled symbols; from Fig. 3A). Four of five cells were dopamine cells. B, Time course data from five cells (open symbols) showing that the effect of amphetamine is inhibited in the presence of methiothepin (1 µM) compared with control data (filled symbols; from Fig. 3A). Four of five cells were dopamine cells.
DISCUSSION
This work is the first demonstration of the acute effects of psychostimulants on excitatory synaptic transmission in the VTA. We report that amphetamine produces a rapid and reproducible decrease in excitatory synaptic transmission onto VTA neurons in slices from drug-naïve animals. In general, previous work on psychostimulant action has focused on dopaminergic mechanisms; our results demonstrate that psychostimulant-mediated release of serotonin importantly modulates excitatory synaptic transmission in the reward pathway.
Glutamatergic synaptic transmission is reduced by amphetamine
Based on previous findings using in vivo microdialysis, we expected amphetamine to increase glutamate release rather than to decrease it. Kalivas and Duffy (1995)
Amphetamine does not depress EPSCs via dopamine receptors
Surprisingly, we found that dopamine receptors do not mediate the depression of excitatory synaptic transmission by amphetamine. Amphetamine does release dopamine in the midbrain slice preparation used because, in a separate experiment, dopamine evoked D2 receptor-mediated inhibition of spontaneous firing. Dopamine at high concentrations also mimics the effect of amphetamine on the EPSC amplitude. However, antagonists at D1-type dopamine receptors [including D1 and D5 subtypes; (Sibley and Monsma, 1992
Amphetamine depresses glutamatergic transmission via serotonin
Amphetamine depresses excitatory synaptic transmission via activation of serotonin receptors, as two different serotonin receptor antagonists block the effect. To account for this, it is possible that amphetamine itself binds directly to serotonin receptors within the slice to reduce the EPSC; amphetamine is known to bind with low affinity to 5-HT2 receptors (Ritz and Kuhar, 1989
Our findings emphasize that one acute effect of amphetamine in the naïve VTA is activation of serotonin receptors, causing potent depression of glutamatergic synapses in the VTA. This result was unexpected, given the considerable evidence that dopamine mediates the rewarding effects of amphetamine in many animal models of drug addiction (Kalivas and Stewart, 1991
Amphetamine modulates excitatory transmission onto both dopamine and nondopamine neurons
Previous work has demonstrated that prefrontal cortical afferents form excitatory synapses with both dopaminergic and nondopaminergic neurons within the VTA (Sesack and Pickel, 1992
Glutamatergic afferents drive VTA dopamine neurons
Glutamatergic afferents ordinarily have a profound effect on VTA dopamine cell activity. Stimulation of medial PFC elicits burst firing of midbrain dopamine cells in vivo (Gariano and Groves, 1988
Effects of amphetamine change with multiple exposures
It will be particularly interesting to test whether the inhibitory effects of an initial exposure to amphetamine will change during subsequent drug exposures, because evidence supports the idea that the effects of amphetamine are altered with repeated exposure. Thus, whereas a sensitizing regimen of amphetamine had no effect on midbrain dopamine cell firing or its modulation by PFC stimulation immediately after withdrawal, at 10 d after withdrawal, dopamine cell firing in response to PFC stimulation was potently enhanced (Tong et al., 1995
In conclusion, the present experiments demonstrate that amphetamine substantially depresses glutamatergic synaptic transmission to VTA cells via serotonin receptor activation. Our results suggest that serotonin is an important modulator of excitatory drive to VTA neurons and that a rapid early effect of psychostimulant exposure is release of this modulator. These experiments emphasize the importance of serotonergic systems in the complex modulation of elements in the reward pathway and provide new insight into the cellular effects of a drug abused by humans.
FOOTNOTES Received May 25, 1999; revised Aug. 13, 1999; accepted Sept. 1, 1999.
This work was supported by National Institutes of Health Grant DA11289.We thank Drs. Yong Li, Donald Lo, Lori McMahon, and Johanna Kornblum for helpful comments and discussion of this manuscript, and Andrew Pittman for excellent technical assistance.
Correspondence should be addressed to J. A. Kauer, Department of Neurobiology, Duke University Medical Center, Box 3209, Durham, NC 27710. E-mail: juliek{at}neuro.duke.edu.
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