Amphetamine Blocks Long-Term Synaptic Depression in the Ventral Tegmental Area

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (59)

Citing Articles via Google Scholar

Google Scholar

Articles by Jones, S.

Articles by Kauer, J. A.

Search for Related Content

PubMed

PubMed Citation

Articles by Jones, S.

Articles by Kauer, J. A.

Previous Article  |  Next Article

The Journal of Neuroscience, August 1, 2000, 20(15):5575-5580

Amphetamine Blocks Long-Term Synaptic Depression in the Ventral Tegmental Area
Susan Jones, Johanna L. Kornblum, and Julie A. Kauer
Department of Neurobiology, Duke University School of Medicine, Durham, North Carolina 27710

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The mesolimbic dopamine system is essential for reward-seeking behavior, and drugs of abuse are thought to usurp the normalfunctioning of this pathway. A growing body of evidence suggeststhat glutamatergic synapses on dopamine neurons in the ventraltegmental area (VTA) are modified during exposure to addictivedrugs, producing sensitization, a progressive augmentation inthe rewarding properties of psychostimulant drugs with repeatedexposure. We have tested the hypothesis that psychostimulant exposureinterferes with the synaptic plasticity of glutamatergic inputsto the VTA. We find that excitatory synapses onto VTA dopamineneurons exhibit long-term depression (LTD) in response to low-frequencystimulation and modest depolarization. LTD in the VTA is NMDAreceptor-independent but is dependent on intracellular Ca²⁺ and can be induced by driving Ca²⁺ into the dopamine neuron. Brief exposure to amphetamine entirelyblocks LTD at glutamatergic synapses in the VTA, by releasingendogenous dopamine that acts at D2 dopamine receptors. The blockof LTD is selective, because amphetamine has no effect on hippocampalLTD. The LTD we have discovered in the VTA is likely to be animportant component of excitatory control of the reward pathway;amphetamine will inhibit LTD, removing this normal brake on theglutamatergic drive to dopamine neurons. This effect of amphetaminerepresents an important mechanism by which normal function ofthe brain reward system may be impaired during substanceabuse.

Key words: long-term depression; VTA; dopamine; amphetamine; sensitization; psychostimulant; addiction

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Daily administration of amphetamine, cocaine, or morphine results in a progressive enhancement or sensitization to many ofthe behavioral effects of the drug (Kalivas and Stewart, 1991;White, 1996). In rats, the enhancement is observed as progressiveaugmentation of spontaneous locomotor activity. In humans, thepsychomotor stimulant effects of abused drugs are thought to relateto arousal and intense euphoria, and sensitization may underlieprogressively more rewarding properties of drugs of abuse associatedwith craving (Robinson and Berridge, 1993; Kalivas et al., 1998;Self, 1998). Sensitization lasts for months in rats and perhapsmany years in humans, suggesting that psychostimulants persistentlymodify brainfunction.

Despite the fact that amphetamine, cocaine, and morphine have distinct mechanisms of action, the ventral tegmental area ofthe midbrain (VTA) has consistently proven to be required forthe development of sensitization to all three. The VTA containsdopamine neurons that project to cortical and limbic areas ofthe brain and is believed to be involved in reward-seeking behavior,drug abuse, and the initiation of sensitization (Wise and Bozarth,1987; Wise and Rompre, 1989; Kalivas and Stewart, 1991; Koob,1992; Wise, 1996; Schultz, 1998; White and Kalivas, 1998). Intra-VTAinjections of amphetamine sensitize animals to peripherally deliveredamphetamine and cocaine (Kalivas and Weber, 1988; Vezina and Stewart,1993), whereas inhibitors of sensitization are effective whenmicroinjected directly into the VTA. These data strongly suggestthat the VTA is the initiation site forsensitization.

Considerable evidence suggests that sensitization is triggered by changes in glutamatergic transmission within the VTA (Wolf,1998). Glutamate receptor antagonists block sensitization (Karleret al., 1989; Stewart and Druhan, 1993; Carlezone et al., 1999;Li and Wolf, 1999), and injection of an NMDA receptor antagonistdirectly into the VTA also blocks sensitization (Kalivas and Alesdatter,1993). Lesions of the prefrontal cortex, which provides a majorglutamatergic afferent input to the VTA, block sensitization toamphetamine (Wolf et al., 1995; Wolf and Xue, 1999). Moreover,repeated electrical stimulation of glutamatergic afferents tothe VTA sensitizes animals to subsequent cocaine administration(Schenk and Snow, 1994). Finally, increased glutamate receptorexpression and enhanced responsiveness to glutamate have beenreported in the VTA in sensitized animals (Tong et al., 1995;White et al., 1995; Fitzgerald et al., 1996; Zhang et al., 1997).These data suggest the hypothesis that stimulant exposure causesplasticity at excitatory synapses on VTA dopamine neurons, leadingto behavioralsensitization.

Long-term potentiation (LTP), a persistent increase in excitatory synaptic transmission, has been demonstrated recently atexcitatory synapses on midbrain dopamine neurons (Bonci and Malenka,1999; Overton et al., 1999). In the hippocampus and other brainregions expressing LTP, synaptic strength can also be downregulatedby an opposing process, long-term depression (LTD) (Bear and Abraham,1996). We report that in addition to exhibiting LTP, excitatorysynapses on VTA neurons also exhibit LTD. LTD is entirely blockedby amphetamine, the first demonstration of modulation of synapticplasticity in the dopaminergic reward pathway by a drug ofabuse.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slice preparation. Sprague Dawley rats (16-28 d old) were decapitated, after deep halothane anesthesia. The brain was rapidlyremoved and placed in ice-cold artificial CSF (ACSF; in mM): 119NaCl, 26 NaHCO₃, 2.5 KCl, 1 NaH₂PO₄, 2.5 CaCl₂, 1.3 MgSO₄, and10 glucose, saturated with 95% O₂ and 5% CO₂, pH 7.4. For VTArecordings, horizontal slices (250-350 µm) were prepared and storedwith 1 mM kynurenic acid added to the ACSF (Jones and Kauer, 1999).For hippocampal recordings, coronal slices (400 µm) were preparedwithout kynurenate (Tecott et al., 1998). Slices were later transferredto a recording chamber where the slice was submerged in warmedACSF without kynurenate (28-32°C). For VTA recordings, 100 µMpicrotoxin was added to block GABA_A receptors to study excitatorysynaptic transmission in isolation. Extracellular CaCl₂ was raisedto 5 mM in experiments using repetitive voltage steps (see Figs.3, 4).

Electrophysiology. Individual cells in the VTA were either recorded "blind" or were visualized using differential interferencecontrast on an upright microscope for whole-cell voltage-clamprecordings. Patch pipettes were filled with cesium gluconate-basedinternal solution (in mM): 117 cesium gluconate, 2.8 NaCl, 5 MgCl₂,0.5 CaCl₂, 2 ATP-Na⁺, 1.7 GTP-Na⁺, 5 EGTA, and 20 HEPES. Experiments with intracellular BAPTA useda similar solution except that 90 mM cesium gluconate and 20 mMBAPTA were used, with no added CaCl₂ or EGTA. Biocytin (0.4%)was added to allow post hoc identification of recorded cells byimmunolabeling. Neurons were voltage-clamped at $-$ 60 mV exceptas noted. The cell input resistance and series resistance weremonitored throughout the experiment, and experiments were discardedif these values changed by >10% during theexperiment.

A bipolar stainless steel stimulating electrode was placed rostral to the recording site in the VTA to stimulate glutamatergicafferents at 0.1 Hz (stimulus intensities were typically 40-200µA; 100 µsec). LTD was induced by stimulating excitatory afferentsat 1 Hz for 6 min, while depolarizing the neuron to $-$ 40 mV. Duringthis depolarization, the neurons often escaped the voltage clamp,firing action currents. It is likely that even when the cell didnot fire, the synaptic regions were sufficiently unclamped topermit voltage fluctuations in response to synapticcurrents.

Extracellular recordings from the CA1 region of hippocampal slices were performed as described previously, while stimulatingCA3 afferents in the stratum radiatum (Tecott et al., 1998). HippocampalLTD was induced by delivering paired pulses 50 msec apart for7.5 min at 1 Hz. This stimulus train was then repeated 10 minlater to maximizeLTD.

Drugs were added directly to the ACSF perfusing the slice chamber at known concentrations at least 10 min before LTD induction.EPSC amplitudes and hippocampal field EPSP initial slopes weremeasured off-line using LabView software kindly donated by Dr.Daniel Madison. For statistical analysis, levels of LTD were assessedby averaging EPSC amplitudes or EPSP slopes for 10 min just beforeLTD induction and comparing this value with averaged values collectedduring the 10 min period from 10 to 20 min after LTD induction,except as noted. The mean values from this period for each testgroup were compared with the control using an unpaired, two-tailedt test; p values $<=$ 0.05 were considered significant. Our dataexhibit a normal distribution (there is no significant differencebetween the mean and median values for each data group, indicatingthat there is no skew in the distribution), and the variance forthe different data sets is the same (the SDs of the data setsare not significantly different). Values are reported as means±SEM.

Identification of dopamine neurons. Immediately after recording, VTA slices were fixed in 4% paraformaldehyde for at least24 hr. Slices were then double-labeled for biocytin (to detectthe recorded cell) and for tyrosine hydroxylase (TH) (to identifydopamine-synthesizing neurons). To classify cells as dopamine(DA) cells or nondopamine cells, we used a combination of physiologyand immunohistochemistry as described previously (Jones and Kauer,1999). Briefly, we tested for the presence of I_h, the pacemakercurrent prominent in dopamine neurons and absent in non-DA cells(Grace and Onn, 1989; Johnson and North, 1992). We also checkedfor TH immunoreactivity. When a cell was TH-positive, it was classedas a DA cell. When a cell was not recovered after fixation orwas not apparently TH-positive (as happens frequently after lengthywhole-cell recordings), then if it had a prominent I_h we alsoclassed the cell as a DA cell. Other neurons were classed as non-DAcells.

Materials. Salts and BAPTA were obtained from Sigma (St. Louis, MO), and all other drugs were obtained from Research BiochemicalsInternational (Natick, MA), with the exception of 7-(hydroxyimino)cycloprop[b]chroman-1a-carboxylateethyl ester (CPCCOE), which was purchased from Tocris Cookson(Ballwin, MO). Stock solutions of amphetamine, eticlopride, sulpiride,spiperone, and CPCCOEt were made fresh daily; amphetamine andeticlopride were dissolved in water; sulpiride and spiperone weredissolved in 0.1N HCL; CPCCOEt was dissolved in DMSO. Ryanodinewas dissolved in DMSO and stored at $-$ 20°C. Stock solutions werediluted 1:1000 for use inACSF.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Stimulation of excitatory afferents to the VTA at 1 Hz for 6 min, during depolarization of cells to $-$ 40 mV, produced long-termdepression of glutamatergic EPSCs recorded from VTA neurons (Fig.1A). The EPSC amplitude was depressed to 72 ± 3% of control valuesafter LTD induction (n = 25; Fig. 1B). EPSCs from 22 of 25 cellswere depressed by >10% 20 min after LTD induction (range, 101-41%of control EPSC amplitude; n = 25). These results are the firstdemonstration of LTD in the VTA and suggest that LTD is a mechanismnormally present to dampen excitatory input.

View larger version (29K):
[in this window]
[in a new window]
Figure 1. Stimulation (1 Hz) elicits long-term depression at excitatory synapses in the VTA. A, A single experiment in which a VTA neuron was recorded from during excitatory afferent stimulation. At the arrow, electrical stimulation was delivered at 1 Hz while the neuron was held at $-$ 40 mV. Responses during the 1 Hz stimulation are omitted for clarity. Afterward, the stimulation frequency was returned to 0.1 Hz, and LTD was observed. Inset, The averages of five EPSCs taken just before (1) and after 1 Hz (2) stimulation. Calibration: 50 pA, 10 msec. B, Averaged results from 30 experiments eliciting LTD as described in A. Peak EPSC amplitudes were normalized and plotted over time. LTD could be induced in both dopamine and non-dopamine neurons within the VTA using this stimulation protocol (n = 22 dopamine neurons; n = 8 non-dopamine neurons). All cells tested were included in the ensemble average, regardless of whether or not they exhibited robust LTD.

We tested whether LTD in the VTA shares properties with LTD in other brain areas. NMDA receptors are required for LTD inductionat many synapses, and evidence suggests that sensitization topsychostimulants and opiates requires activation of NMDA receptorsin the VTA. However, blockade of NMDA receptors with APV did notprevent LTD in the VTA (Fig. 2A). At various synapses, includingthe CA3-to-CA1 synapse in the hippocampus, elevation of Ca²⁺ in the postsynaptic neuron is necessary for LTD induction (Lindenand Connor, 1995; Cummings et al., 1996). In our experiments,inclusion of the Ca²⁺ chelator BAPTA (20 mM) in the whole-cell recording pipette forat least 30 min before LTD induction entirely blocked LTD (Fig.2B). The block of LTD was not caused by dialysis during long recordings,because control neurons recorded from for 30 min before LTD inductionwithout BAPTA in the pipette solution did exhibit LTD after 1Hz afferent stimulation (n = 7). These results show that LTD inductionin the VTA requires an elevation of postsynaptic Ca²⁺ levels and that this Ca²⁺ must arise from sources other than the NMDA receptor.

View larger version (33K):
[in this window]
[in a new window]
Figure 2. NMDA receptors are not required, but intracellular Ca²⁺ elevation is required for LTD induction. A, Control data from Figure 1 (open circles; n = 30) are shown; 50 µM D-APV (closed circles) was present in the bathing medium throughout the experiment and for at least 10 min before inducing LTD. D-APV did not block LTD induced by 1 Hz stimulation during depolarization to $-$ 40 mV (n = 6, 5 identified dopamine neurons). This concentration of D-APV blocks NMDA receptors on VTA neurons (Jones and Kauer, 1999). LTD in the presence of APV is 79 ± 9% of control values (n = 5; not significantly different from control LTD). B, Control data from Figure 1 (open circles; n = 30) are shown; whole-cell recordings (closed circles ) were made from neurons using pipettes containing 20 mM BAPTA (see Materials and Methods) for 30-60 min before delivering 1 Hz stimulation during depolarization to $-$ 40 mV. Intracellular BAPTA significantly attenuated LTD (n = 8, all identified dopamine neurons). LTD with intracellular BAPTA is 91 ± 6% of control values (n = 7).

The metabotropic glutamate receptor mGluR1 is present on dopamine neurons (Kosinski et al., 1998) and can increase intracellularCa²⁺ levels by releasing Ca²⁺ from ryanodine-sensitive stores (Fiorillo and Williams, 1998).We therefore tested whether interfering with these processes alsoblocked LTD. We found that blocking mGluR1 using the selectiveantagonist CPCCOEt (100 µM) had no effect on LTD induction (EPSCamplitude 5-10 min after LTD induction, 70 ± 14% of baseline values;n = 8). Additionally, robust LTD was triggered in the presenceof ryanodine (10 µM; EPSC amplitude, 64 ± 14% of baseline values;n = 4). These data suggest that activation of mGluR1 and subsequentrelease of Ca²⁺ from ryanodine-sensitive Ca²⁺ stores are not required for LTDinduction.

To determine whether an increase in postsynaptic Ca²⁺ alone is sufficient to induce LTD without synaptic stimulation, we repetitivelydepolarized the dopamine neuron to activate voltage-gated Ca²⁺ channels. After resuming synaptic stimulation, we found thatLTD had been induced (Fig. 3). This result suggests the hypothesisthat any event inducing a rise in postsynaptic Ca²⁺ can induce LTD. If the LTD induced artificially by driving Ca²⁺ into the postsynaptic neuron shares underlying mechanisms withsynaptically induced LTD, then maximizing synaptic LTD shouldprevent further depression by the voltage-step protocol. Thiswas indeed observed, indicating that synaptically induced LTDuses the same mechanisms used during LTD induced by repetitivedepolarization (Fig. 4). Taken together, our data indicate thatelevation of intracellular Ca²⁺ is necessary and sufficient to trigger LTD at VTA excitatorysynapses.

View larger version (33K):
[in this window]
[in a new window]
Figure 3. Elevation of postsynaptic intracellular Ca²⁺ is sufficient to trigger LTD. A, A single example of a neuron recorded from for 40 min while collecting baseline EPSCs. At the arrow, synaptic stimulation was stopped, and the neuron was repetitively stepped 20 times to +10 mV for 3 sec, once every 5 sec. Synaptic stimulation was then resumed at 0.1 Hz. This protocol was sufficient to induce LTD. Inset, The averages of five EPSCs taken at the times indicated on the graph. Calibration: 200 pA, 10 msec. B, The average of 12 such experiments. All experiments in this figure were performed in ACSF containing 5 mM Ca²⁺. LTD elicited by repetitive depolarization is 79 ± 7% of control values (n = 11, 6 identified dopamine neurons).

View larger version (32K):
[in this window]
[in a new window]
Figure 4. Synaptically induced LTD occludes LTD produced by repetitive depolarization. A, Synaptic LTD was maximally induced by pairing 1 Hz stimulation with depolarization to $-$ 40 mV three times until no further LTD was elicited (open arrowheads). At this point, synaptic stimulation was stopped, and the neuron was repetitively stepped 20 times to +10 mV for 3 sec, once every 5 sec (arrow). No further LTD was apparent after repetitive depolarizations. Inset, The averages of five EPSCs taken at the times indicated on the graph are shown. Calibration: 200 pA, 10 msec. B, After maximally inducing LTD by pairing 1 Hz stimulation with depolarization to $-$ 40 mV two to four times until no further LTD was elicited, neurons were repetitively depolarized as described above (n = 7). LTD induced after repetitive depolarizations is 96 ± 8% of control values (n = 6). All experiments in this figure were performed in ACSF containing 5 mM Ca²⁺.

We hypothesized that psychostimulants might interfere with LTD, removing a normal brake on the excitation of dopamine neuronsin the VTA. We therefore tested the effects of amphetamine onLTD by bathing VTA slices from drug-naïve animals in amphetaminefor 15 min before an LTD-inducing protocol. LTD of VTA synapseswas entirely blocked by 1 µM amphetamine (Fig. 5; EPSC amplitude,100 ± 6% of control values; p < 0.005). Long-term depression wasfirst described at synapses in the hippocampus (Dudek and Bear,1992; Mulkey and Malenka, 1992), and dopamine is known to modulatesynaptic function in the hippocampus (Otmakhova and Lisman, 1996,1998, 1999). To test the specificity of amphetamine's effectson LTD, we examined whether amphetamine can also block hippocampalLTD at the CA3-to-CA1 synapse. In contrast to its effects in theVTA, amphetamine (1 µM) had no effect on LTD at these hippocampalsynapses (Fig. 6). These data indicate that amphetamine has selectiveeffects on synaptic plasticity at excitatory synapses on midbraindopamine neurons.

View larger version (30K):
[in this window]
[in a new window]
Figure 5. Amphetamine blocks LTD in VTA neurons. A, LTD was blocked in the presence of 1 µM amphetamine (horizontal bar) applied for 15 min before synaptic stimulation at 1 Hz for 6 min during depolarization to $-$ 40 mV. Insets, The averages of five EPSCs taken at the times indicated on the graph are shown. Calibration: 100 pA, 10 msec. B, The average of nine such experiments (6 identified dopamine neurons) is shown.

View larger version (33K):
[in this window]
[in a new window]
Figure 6. Amphetamine does not block LTD at CA3-to-CA1 synapses in the hippocampus. A, Two independent afferent pathways in st. radiatum were stimulated alternately at 0.1 Hz while field EPSPs were recorded. At the arrows (top graph), stimulation to Pathway 2 was stopped, and LTD was induced in Pathway 1, using two trains of 1 Hz stimulation (see Materials and Methods). After induction of LTD in Pathway 1, 1 µM amphetamine was added to the bathing medium. Fifteen minutes later, stimulation to Pathway 1 was stopped, and LTD-inducing stimuli were delivered to Pathway 2 (arrows in bottom graph). Amphetamine had no effect on LTD induction or maintenance. B, Averaged experiments show that identical LTD was induced in hippocampal slices whether or not 1 µM amphetamine was included in the bathing solution [closed circles, control solution (n = 4); open circles, 1 µM amphetamine present for at least 10 min before 1 Hz stimulation (n = 5)]. Responses during the 1 Hz stimulation are omitted for clarity.

Amphetamine blocks and reverses the action of the dopamine transporter, thereby increasing dopamine levels where the transporteris present. Dopamine depresses voltage-gated Ca²⁺ channel function in a variety of peripheral and central neurons(Stack and Suprenant, 1991; Seabrook et al., 1994; Yan et al.,1997; Kuzhikandathil and Oxford, 1999), including midbrain dopaminecells (Cardozo and Bean, 1995). We hypothesized that dopaminereleased locally by amphetamine might block LTD by inhibitingCa²⁺ entry into VTA neurons during the LTD induction protocol. Dopamineand the D2 receptor agonist quinpirole block VTA LTD, acting viaD2 dopamine receptors (Thomas et al., 2000), indicating that amphetaminemay block LTD at VTA synapses by releasing endogenous dopamine,which then acts at D2 receptors. We therefore examined whetherD2 receptor antagonists interfere with the block of LTD by amphetamine.VTA slices were perfused with D2 receptor antagonists, and LTDwas induced using 1 Hz stimulation and depolarization to $-$ 40 mV.The effect of amphetamine was attenuated by 30 nM eticloprideand was blocked by 100 nM eticlopride (Fig. 7). The less-selectiveD2 receptor antagonist spiperone (5 µM) also significantly blockedamphetamine's effects (EPSC amplitude after LTD induction, 75± 4% of control levels; n = 4). These data indicate that the blockof LTD by amphetamine is mediated by D2 receptor activation.

View larger version (22K):
[in this window]
[in a new window]
Figure 7. The D2 receptor antagonist eticlopride reverses the effects of amphetamine on LTD. Eticlopride was included in the bathing solution before 1 µM amphetamine was added. LTD was induced by depolarizing to $-$ 40 mV while stimulating synaptic afferents at 1 Hz for 6 min. A, Eticlopride (30 nM) attenuates the effects of amphetamine on LTD (n = 8, with 7 dopamine cells). B, Eticlopride (100 nM) attenuates the effects of amphetamine on LTD (n = 5, with all dopamine cells). C, The bar chart shows the amount of LTD measured from 10 to 20 min after LTD induction in control cells (n = 25), amphetamine-treated cells (Amphet 1 µM; n = 8), cells treated with 30 nM eticlopride + 1 µM amphetamine (Etic 30 nM + Amph; n = 7), or cells treated with 100 nM eticlopride + 1 µM amphetamine (Etic 100 nM + Amph; n = 4). Asterisks indicate significant differences from cells treated with 1 µM amphetamine (p $<=$ 0.05).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our results are the first to show that excitatory synapses on VTA dopamine neurons can express LTD in addition to expressingLTP, exhibiting bidirectional modification depending on the patternof afferent input and membrane potential. Under normal conditions,LTD will modulate information flow into the VTA, limiting excitationof dopamine neurons. The block of LTD by amphetamine is the firstdemonstration of an effect of an addictive drug on synaptic plasticityin the reward pathway. We speculate that the block of LTD, whichoccurs within minutes after a first exposure to amphetamine, isa rapid cellular consequence of amphetamineabuse.

Postsynaptic Ca²⁺ entry triggers LTD

A rise in intracellular Ca²⁺ is both necessary and sufficient to trigger LTD in VTA dopamine cells. Where does the Ca²⁺ come from during the protocol pairing modest depolarization withlow-frequency synaptic stimulation? LTD at these synapses, unlikeLTP (Bonci and Malenka, 1999; Overton et al., 1999), is not NMDAreceptor-dependent, so Ca²⁺ entry through NMDA receptors is not necessary. Metabotropic glutamatereceptors that release Ca²⁺ from ryanodine-sensitive intracellular stores and Ca²⁺-permeable AMPA channels are apparently not required for LTD (seealso Thomas et al., 2000). Instead, the most likely hypothesisis that Ca²⁺ enters the cell through voltage-dependent Ca²⁺ channels, many types of which are expressed by VTA dopamine neurons(Grace and Onn, 1989; Kang and Kitai, 1993; Cardozo and Bean,1995). Because Ca²⁺ channels are also essential for neurotransmitter release, itis difficult to test this hypothesis directly, and further workwill be necessary to define precisely the channel types involved.Repetitive depolarization using voltage steps is likely to triggerCa²⁺ entry through multiple voltage-gated Ca²⁺ channel types, particularly the high-voltage-activated L, N,P, and Q channels. The voltage-step protocol alone produces LTD,even without synaptic stimulation, demonstrating that LTD inductionoccurs postsynaptically and does not require synaptic activityor glutamate release. LTD elicited after voltage steps sharesa common mechanism with LTD produced by pairing sustained modestdepolarization with synaptic activity, because voltage steps haveno further effect after synaptically triggered LTD is maximal.It is thus likely that whenever intracellular Ca²⁺ rises sufficiently, excitatory synapses onto VTA dopamine cellswill bedepressed.

We also observed LTD in nondopaminergic VTA neurons after pairing depolarization to $-$ 40 mV with synaptic stimulation at 1Hz. Previous work showed that a protocol that triggers LTP inVTA dopamine neurons does not enhance synaptic transmission ontonondopamine neurons (Bonci and Malenka, 1999). Thus, althoughonly dopamine cell synapses can be potentiated, excitatory synapseson both major types of VTA neurons can be depressed. Because ourstudy focused primarily on dopamine neurons, further work willbe required to determine whether the mechanisms underlying LTDat synapses on nondopamine cells are the same as those in dopaminecells and whether amphetamine can block LTD at synapses on nondopaminecells.

Amphetamine blocks LTD by activating D2 dopamine receptors

Treatment with 1 µM amphetamine entirely blocks LTD at synapses on dopamine neurons. Amphetamine interferes with LTD via aD2 receptor-mediated mechanism, because eticlopride, at 30-100nM, attenuated amphetamine's effects. Dopamine and a D2 receptoragonist, quinpirole, also block LTD (Thomas et al., 2000). Severalstudies have shown that D2 receptor activation attenuates a varietyof Ca²⁺ currents, including both low-voltage-activated T currents andhigh-voltage-activated L, N, P, and Q currents (Carbone and Lux,1989; Stack and Suprenant, 1991; Seabrook et al., 1994; Cardozoand Bean, 1995; Yan et al., 1997; Kuzhikandathil and Oxford, 1999;Wolfe et al., 1999). We therefore hypothesize that amphetamineblocks and reverses the dopamine transporter to elevate extracellulardopamine, which activates D2 receptors and thereby depresses voltage-dependentCa²⁺ currents. The inhibition of Ca²⁺ entry may reduce Ca²⁺ levels below the threshold needed to trigger LTD. Alternatively,other cellular sequelae of amphetamine-mediated dopamine receptoractivation may interfere with LTDinduction.

Modulation of LTD by dopamine and psychostimulants

VTA dopamine cells both in vitro and in vivo have unusually positive membrane potentials and action potential thresholds (Graceand Bunney, 1983; Grace, 1988), and it is not unlikely that theirmembrane potentials often remain near $-$ 40 mV for long periodsof time. Because LTD induction in vitro requires only relativelylow-frequency synaptic activation, and because dopamine neuronsusually fire at 1-8 Hz in vivo (Grace and Bunney, 1984), it ispossible that in the brain under normal conditions VTA excitatorysynapses often exist in a relatively depressed state. LTD maynormally protect VTA dopamine neurons from excessive glutamatergicexcitation. In the presence of amphetamine this protective brakeis removed, permitting unrestricted excitation of dopamine neuronsby glutamateafferents.

One important question raised by our results is whether endogenous dopamine blocks LTD under physiological conditions, aswell as during psychostimulant-mediated dopamine elevation. Dopaminecan be released from somatodendritic sites (Geffen et al., 1976;Cheramy et al., 1981), raising the possibility that LTD may bemodulated by endogenous dopamine. This modulation is likely tooperate on the seconds-to-minutes time scale, after local dopaminerelease and before removal of the neurotransmitter by the transporter.A transient block of LTD resulting from somatodendritic dopaminerelease could provide a window during which LTP is facilitatedat synapses on dopamine cells, thus acting as a gate for strengtheningafferent excitatory input. In contrast, after psychostimulantadministration, psychostimulant levels remain high for hours,and levels of dopamine in the VTA may consequently also remainelevated for prolonged periods. The resulting persistent blockadeof LTD would be expected to promote glutamatergic activity fromcortical and subcortical regions and to increase the likelihoodof NMDA receptor-dependentLTP.

Overactivity of dopaminergic neurotransmission in the VTA is postulated to contribute to the development of psychotic symptoms,both in schizophrenia and in amphetamine psychosis. Antipsychoticdrugs effective in treating both disorders have D2 receptor antagonistproperties. Somatodendritic dopamine release does not have a dramaticeffect on the firing rate of most dopamine neurons (Bunney andAghajanian, 1975; Pucak and Grace, 1996), but our findings suggestthat, acutely, D2 receptor antagonists may promote the developmentof LTD in the VTA, reducing dopamine neuron activity in the short-term.The effects of longer-term exposure to these drugs have yet tobetested.

Amphetamine effects in the VTA promote behavioral sensitization

NMDA receptor-dependent LTP has been proposed as a possible mechanism involved in the onset of behavioral sensitization (Tonget al., 1995; White, 1996; Wolf, 1998). Three mechanisms havebeen identified by which amphetamine will promote the abnormalexcitation of VTA dopamine neurons by glutamatergic afferents.First, although a rapid effect of psychostimulants is hyperpolarizationof dopamine neurons via autoreceptors, this effect desensitizesin the presence of amphetamine, removing one source of inhibition(Seutin et al., 1991). Second, psychostimulants potently elevateextracellular glutamate in the VTA, perhaps as a result of decreasedglutamate reuptake (Xue et al., 1996; Kalivas and Duffy, 1998;Wolf and Xue, 1999). Finally, our results indicate that amphetaminestrongly modulates excitatory synaptic transmission by blockingLTD. We propose that these three mechanisms will act in concertto promote NMDA receptor-dependent LTP, resulting in an abnormalstrengthening of excitatory synapses on dopamine neurons in theVTA. This hypothesis can account for the block of sensitizationby intra-VTA administration of an NMDA receptor antagonist (Vezinaand Stewart, 1993) and the ability of high-frequency electricalstimulation of glutamate afferents to the VTA by itself to producesensitization to peripherally administered psychostimulants (Schenkand Snow, 1994). The resulting glutamatergic excitation of dopamineneurons may represent an early trigger in the development of sensitizationandaddiction.

  FOOTNOTES

Received April 4, 2000; accepted April 24, 2000.

This work was supported by National Institutes of Health Grant DA 11289. We wish to thank Andrew Pittman and Katherine Papastephanoufor excellent technical assistance and Drs. Lawrence Katz, DonaldLo, Richard Mooney, and Yong Li for helpful comments on thismanuscript.
S.J. and J.L.K. contributed equally to thiswork.

Correspondence should be addressed to Dr. Julie Kauer at her present address: Brown University, Department of Molecular Pharmacology,Physiology, and Biotechnology, P.O. Box G-B4, Providence, RI02912.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bear MF, Abraham WC (1996) Long-term depression in hippocampus. Annu Rev Neurosci 19:437-462[Web of Science][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].
Bunney BS, Aghajanian GK (1975) Evidence for drug actions on both pre- and postsynaptic catecholamine receptors in the CNS. In: Pre- and postsynaptic receptors (Usdin E, Bunney WE, eds), pp 89-122. New York: Dekker.
Carbone E, Lux HD (1989) Modulation of Ca channels in peripheral neurons. Ann NY Acad Sci 1560:346-357.
Cardozo DL, Bean BP (1995) Voltage-dependent calcium channels in rat midbrain dopamine neurons: modulation by dopamine and GABA_B receptors. J Neurophysiol 74:1137-1148[Abstract/Free Full Text].
Carlezone Jr WA, Rasmussen K, Nestler EJ (1999) AMPA antagonist LY293558 blocks the development, without blocking the expression, of behavioral sensitization to morphine. Synapse 31:256-262[Medline].
Cheramy A, Leviel V, Glowinski J (1981) Dendritic release of dopamine in the substantia nigra. Nature 289:537-542[Medline].
Cummings JA, Mulkey RM, Nicoll RA, Malenka RC (1996) Ca²⁺ signaling requirements for long-term depression in the hippocampus. Neuron 16:825-833[Web of Science][Medline].
Dudek SM, Bear MF (1992) Homosynaptic long-term depression in area CA1 of hippocampus and effects of N-methyl-D-aspartate receptor blockade. Proc Natl Acad Sci USA 89:4363-4367[Abstract/Free Full Text].
Fiorillo CD, Williams JT (1998) Glutamate mediates an inhibitory postsynaptic potential in dopamine neurons. Nature 394:78-82[Medline].
Fitzgerald LW, Ortiz J, Hamedani AG, Nestler EJ (1996) Drugs of abuse and stress increase the expression of GluR1 and NMDAR1 glutamate receptor subunits in the rat ventral tegmental area: common adaptations among cross-sensitizing agents. J Neurosci 16:274-282[Abstract/Free Full Text].
Geffen LB, Jessell TM, Cuello AC, Iversen LL (1976) Release of dopamine from dendrites in rat substantia nigra. Nature 260:258-260[Medline].
Grace AA (1988) In vivo and in vitro intracellular recordings from rat midbrain dopamine neurons. Ann NY Acad Sci 537:51-76[Web of Science][Medline].
Grace AA, Bunney BS (1983) Intracellular and extracellular electrophysiology of nigral dopaminergic neurons. 1. Identification and characterization. Neuroscience 10:301-315[Web of Science][Medline].
Grace AA, Bunney BS (1984) The control of firing pattern in nigral dopamine neurons: single spike firing. J Neurosci 4:2866-2876[Abstract].
Grace AA, Onn S-P (1989) Morphology and electrophysiological properties of immunocytochemically identified rat dopamine neurons recorded in vitro. J Neurosci 9:3463-3481[Abstract].
Johnson SW, North RA (1992) Two types of neurone in the rat ventral tegmental area and their synaptic inputs. J Physiol (Lond) 450:455-468[Abstract/Free Full Text].
Jones S, Kauer JA (1999) Amphetamine depresses excitatory synaptic transmission in the ventral tegmental area via serotonin receptors. J Neurosci 19:9780-9787[Abstract/Free Full Text].
Kalivas PW, Alesdatter JE (1993) Involvement of NMDA 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 (1998) Repeated cocaine administration alters extracellular glutamate in the ventral tegmental area. J Neurochem 70:1497-1502[Web of Science][Medline].
Kalivas PW, Stewart J (1991) Dopamine transmission in the initiation and expression of drug- and stress-induced sensitization of motor activity. Brain Res Rev 16:223-244[Medline].
Kalivas PW, Weber B (1988) Amphetamine injection into the ventral mesencephalon sensitizes rats to peripheral amphetamine and cocaine. J Pharmacol Exp Ther 245:1095-1101[Abstract/Free Full Text].
Kalivas PW, Pierce RC, Cornish J, Sorg BA (1998) A role for sensitization in craving and relapse in cocaine addiction. J Psychopharmacol 12:49-53.
Kang Y, Kitai ST (1993) A whole cell patch-clamp study on the pacemaker potential in dopaminergic neurons of rat substantia nigra compacta. Neurosci Res 18:209-221[Web of Science][Medline].
Karler R, Calder LD, Chaudhry IA, Turkanis SA (1989) Blockade of "reverse tolerance" to cocaine and amphetamine by MK-801. Life Sci 45:599-606[Web of Science][Medline].
Koob GF (1992) Drugs of abuse: anatomy, pharmacology, and function of reward pathways. Trends Pharmacol Sci 13:177-184[Medline].
Kosinski CM, Standaert DG, Testa CM, Penney Jr JB, Young AB (1998) Expression of metabotropic glutamate receptor 1 isoforms in the substantia nigra pars compacta of the rat. Neuroscience 86:783-798[Web of Science][Medline].
Kuzhikandathil EV, Oxford GS (1999) Activation of human D3 dopamine receptor inhibits P/Q-type calcium channels and secretory activity in AtT-20 cells. J Neurosci 19:1698-1707[Abstract/Free Full Text].
Li Y, Wolf ME (1999) Can the "state-dependency" hypothesis explain prevention of amphetamine sensitization in rats by NMDA receptor antagonists? Psychopharmacology (Berl) 141:351-361[Medline].
Linden DJ, Connor JA (1995) Long-term synaptic depression. Annu Rev Neurosci 18:319-357[Web of Science][Medline].
Mulkey RM, Malenka RC (1992) Mechanisms underlying induction of homosynaptic long-term depression in area CA1 of the hippocampus. Neuron 9:967-975[Web of Science][Medline].
Otmakhova NA, Lisman JE (1996) D1/D5 dopamine receptor activation increases the magnitude of early long-term potentiation at CA1 hippocampal synapses. J Neurosci 16:7478-7486[Abstract/Free Full Text].
Otmakhova NA, Lisman JE (1998) D1/D5 dopamine receptors inhibit depotentiation at CA1 synapses via a cAMP-dependent mechanism. J Neurosci 18:1270-1279[Abstract/Free Full Text].
Otmakhova NA, Lisman JE (1999) Dopamine selectively inhibits the direct cortical pathway to the CA1 hippocampal region. J Neurosci 19:1437-1445[Abstract/Free Full Text].
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[Web of Science][Medline].
Pucak ML, Grace AA (1996) Effects of haloperidol on the activity and membrane physiology of substantia nigra dopamine neurons recorded in vitro. Brain Res 713:44-52[Web of Science][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].
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[Web of Science][Medline].
Schultz W (1998) Predictive reward signal of dopamine neurons. J Neurophysiol 80:1-27[Abstract/Free Full Text].
Seabrook GR, Knowles M, Brown N, Myers J, Sinclair H, Patel S, Freedman SB, McAllister G (1994) Pharmacology of high-threshold calcium currents in GH4C1 pituitary cells and their regulation by activation of human D2 and D4 dopamine receptors. Br J Pharmacol 112:728-734[Web of Science][Medline].
Self DW (1998) Neural substrates of drug craving and relapse in drug addiction. Ann Med 30:379-389[Web of Science][Medline].
Seutin V, Verbanck P, Massotte L, Dresse A (1991) Acute amphetamine-induced subsensitivity of A10 dopamine autoreceptors in vitro. Brain Res 558:141-144[Web of Science][Medline].
Stack J, Suprenant A (1991) Dopamine actions on calcium currents, potassium currents and hormone release in rat melanotrophs. J Physiol (Lond) 439:37-58[Abstract/Free Full Text].
Stewart J, Druhan JP (1993) Development of both conditioning and sensitization to the behavioral activating effects of amphetamine is blocked by the non-competitive NMDA receptor antagonist, MK-801. Psychopharmacology (Berl) 110:125-132[Medline].
Tecott LH, Logue SF, Wehner JM, Kauer JA (1998) Perturbed dentate gyrus function in serotonin 5-HT_2C receptor mutant mice. Proc Natl Acad Sci USA 95:15026-15031[Abstract/Free Full Text].
Thomas MJ, Malenka RC, Bonci A (2000) Modulation of long-term depression by dopamine in the mesolimbic system. J Neurosci 20:5581-5586[Abstract/Free Full Text].
Tong Z-Y, Overton PG, Clark D (1995) Chronic administration of (+)-amphetamine alters the reactivity of midbrain dopaminergic neurons to prefrontal cortex stimulation in the rat. Brain Res 674:63-74[Web of Science][Medline].
Vezina P, Stewart J (1993) 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.
White FJ (1996) Synaptic regulation of mesocorticolimbic dopamine neurons. Annu Rev Neurosci 16:405-436.
White FJ, Kalivas PW (1998) Neuroadaptations involved in amphetamine and cocaine addiction. Drug Alcohol Depend 51:141-153[Web of Science][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].
Wise RA (1996) Addictive drugs and brain stimulation reward. Annu Rev Neurosci 19:319-340[Web of Science][Medline].
Wise RA, Bozarth MA (1987) A psychomotor stimulant theory of addiction. Psychol Rev 94:469-492[Web of Science][Medline].
Wise RA, Rompre P-P (1989) Brain dopamine and reward. Annu Rev Psychol 40:191-225[Web of Science][Medline].
Wolf ME (1998) The role of excitatory amino acids in behavioral sensitization to psychomotor stimulants. Prog Neurobiol 54:1-42[Web of Science][Medline].
Wolf ME, Xue CJ (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 K (1995) Effects of lesions of prefrontal cortex, amygdala, or fornix on behavioral sensitization to amphetamine: comparison with NMDA antagonists. Neuroscience 69:417-439[Web of Science][Medline].
Wolfe SE, Howard DE, Schetz JA, Cheng CJ, Webber R, Beatty DM, Chronwall BM, Morris SJ (1999) Dopamine D2-receptor isoforms expressed in AtT20 cells inhibit Q-type high-voltage-activated Ca²⁺ channels via a membrane-delimited pathway. J Neurochem 72:479-490[Web of Science][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[Web of Science][Medline].
Yan Z, Song W-J, Surmeier DJ (1997) D2 dopamine receptors reduce N-type Ca²⁺ currents in rat neostriatal cholinergic interneurons through a membrane-delimited, protein-kinase-C-insensitive pathway. J Neurophysiol 77:1003-1015[Abstract/Free Full Text].
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].

Copyright © 2000 Society for Neuroscience 0270-6474/00/20155575-06$05.00/0

This article has been cited by other articles:

R. Spanagel
Alcoholism: A Systems Approach From Molecular Physiology to Addictive Behavior
Physiol Rev, April 1, 2009; 89(2): 649 - 705.
[Abstract] [Full Text] [PDF]

C. H. Good and C. R. Lupica
Properties of distinct ventral tegmental area synapses activated via pedunculopontine or ventral tegmental area stimulation in vitro
J. Physiol., March 15, 2009; 587(6): 1233 - 1247.
[Abstract] [Full Text] [PDF]

G. D. Stuber, M. Klanker, B. de Ridder, M. S. Bowers, R. N. Joosten, M. G. Feenstra, and A. Bonci
Reward-Predictive Cues Enhance Excitatory Synaptic Strength onto Midbrain Dopamine Neurons
Science, September 19, 2008; 321(5896): 1690 - 1692.
[Abstract] [Full Text] [PDF]

F. S. Nugent and J. A. Kauer
LTP of GABAergic synapses in the ventral tegmental area and beyond
J. Physiol., March 15, 2008; 586(6): 1487 - 1493.
[Abstract] [Full Text] [PDF]

S. N. Blythe, J. F. Atherton, and M. D. Bevan
Synaptic Activation of Dendritic AMPA and NMDA Receptors Generates Transient High-Frequency Firing in Substantia Nigra Dopamine Neurons In Vitro
J Neurophysiol, April 1, 2007; 97(4): 2837 - 2850.
[Abstract] [Full Text] [PDF]

M. J. Beckstead and J. T. Williams
Long-Term Depression of a Dopamine IPSC
J. Neurosci., February 21, 2007; 27(8): 2074 - 2080.
[Abstract] [Full Text] [PDF]

X. Sun, Y. Zhao, and M. E. Wolf
Dopamine Receptor Stimulation Modulates AMPA Receptor Synaptic Insertion in Prefrontal Cortex Neurons
J. Neurosci., August 10, 2005; 25(32): 7342 - 7351.
[Abstract] [Full Text] [PDF]

A. Rajadhyaksha, I. Husson, S. S. Satpute, K. D. Kuppenbender, J. Q. Ren, R. M. Guerriero, D. G. Standaert, and B. E. Kosofsky
L-Type Ca2+ Channels Mediate Adaptation of Extracellular Signal-Regulated Kinase 1/2 Phosphorylation in the Ventral Tegmental Area after Chronic Amphetamine Treatment
J. Neurosci., August 25, 2004; 24(34): 7464 - 7476.
[Abstract] [Full Text] [PDF]

M. E. Wolf
Addiction: Making the Connection Between Behavioral Changes and Neuronal Plasticity in Specific Pathways
Mol. Interv., June 1, 2002; 2(3): 146 - 157.
[Abstract] [Full Text] [PDF]

M. Federici, S. Natoli, G. Bernardi, and N. B Mercuri
Dopamine selectively reduces GABAB transmission onto dopaminergic neurones by an unconventional presynaptic action
J. Physiol., April 1, 2002; 540(1): 119 - 128.
[Abstract] [Full Text] [PDF]

M. Giorgetti, G. Hotsenpiller, P. Ward, T. Teppen, and M. E. Wolf
Amphetamine-Induced Plasticity of AMPA Receptors in the Ventral Tegmental Area: Effects on Extracellular Levels of Dopamine and Glutamate in Freely Moving Rats
J. Neurosci., August 15, 2001; 21(16): 6362 - 6369.
[Abstract] [Full Text] [PDF]

M. J. Thomas, R. C. Malenka, and A. Bonci
Modulation of Long-Term Depression by Dopamine in the Mesolimbic System
J. Neurosci., August 1, 2000; 20(15): 5581 - 5586.
[Abstract] [Full Text] [PDF]

M. Federici, S. Natoli, G. Bernardi, and N. B. Mercuri
Dopamine selectively reduces GABAB transmission onto dopaminergic neurones by an unconventional presynaptic action
J. Physiol., February 8, 2002; (2002) 200101393.
[Abstract] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (59)

Citing Articles via Google Scholar

Google Scholar

Articles by Jones, S.

Articles by Kauer, J. A.

Search for Related Content

PubMed

PubMed Citation

Articles by Jones, S.

Articles by Kauer, J. A.