Dopamine Modulates the Responsivity of Mediodorsal Thalamic Cells Recorded In Vitro

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The Journal of Neuroscience, December 15, 1998, 18(24):10566-10578

Dopamine Modulates the Responsivity of Mediodorsal Thalamic Cells Recorded In Vitro
A. Lavin and A. A. Grace
Departments of Neuroscience and Psychiatry, Center for Neuroscience, University of Pittsburgh, Pittsburgh, Pennsylvania 15260

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The mediodorsal thalamic nucleus (MD) receives convergent inputs from subcortical limbic structures that overlap with a dopaminergic(DA) innervation. In this study, we describe the effects of DAagonists on the basal and evoked electrophysiological activityof identified thalamic cells of rats recorded in vitro. Administrationof the D1 agonist SFK 38393 (10 µM) did not produce a clear effecton the physiological properties of the thalamic cells recorded.In contrast, bath administration of the D2 agonist quinpirole(10 µM) resulted in an enhancement of membrane excitability, facilitationof the occurrence of low-threshold spikes (LTSs), and changesin the resting membrane potential of the thalamic cells tested.The quinpirole-mediated responses were reversed by administrationof the D2 antagonist haloperidol. Results from experiments performedwith different [K⁺] and K⁺ channel blockers suggest that the effects of quinpirole are mediatedat least in part by changes in K⁺ conductances. The results from this study suggest that DA canmodulate the excitability of thalamic cells and in turn may influencethe way that the thalamocortical system integratesinformation.

Key words: thalamus; dopamine; low-threshold spikes; K⁺ conductances; D1 agonist; D2 agonist

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The mediodorsal thalamic nucleus (MD) is a site through which the majority of limbic structures influence cortical processing.This nucleus receives input from dopamine-rich regions of thelimbic system, including projections from the nucleus accumbensand the ventral pallidum (Haber et al., 1985; Zahm et al., 1987;Groenewegen, 1988, Groenewegen and Berendse, 1994; Lavin and Grace,1994). Anatomical studies have described a dopaminergic innervationof the MD and paraventricular nuclei (PV) of the thalamus as well.The dopaminergic innervation of the thalamus was first describedin 1974 (Lindvall and Björklund, 1974) and is believed to arisefrom the A11 and A13 dopaminergic cell groups that represent thehypothalamic dopamine neurons (Füxe, 1965). Subsequent studiesusing autoradiographic techniques showed the presence of anterogradelylabeled axons ascending from the ventral tegmental area (VTA)and terminating in the medial part of the mediodorsal thalamicnuclei (Beckstead et al., 1979). Furthermore, injections of theretrograde tracer HRP-wheat germ agglutinin (WGA) into the medialand lateral MD labeled neurons in large numbers within the midlineVTA (Cornwall and Phillipson, 1988). This VTA-MD projection wasconfirmed to be at least partially dopaminergic in studies usingcombined retrograde and anterograde tracers (Groenewegen, 1988)and immunohistochemical staining for tyrosine hydroxylase(TH).

Although the dopaminergic innervation of the thalamus is not as extensive as that of striatal regions, several studies haverevealed the presence of D1, D2, D4, and D5 subtypes of DA receptorsin the MD thalamic region (Fields et al., 1977; Boyson et al.,1986; Dawson et al., 1986; Camps et al., 1989; Mansour et al.,1990, 1992; Young and Wilcox, 1991; Huang et al., 1992; Janowskiet al., 1992; Levant et al., 1992; Machida et al., 1992; Civelliet al., 1993; Hall et al., 1996; Sedvall and Farde, 1996). Furthermore,neurochemical studies suggest that although the density of DAfibers in the thalamus is moderate, this monoamine has a widespreaddistribution in both the human and rodent thalamus (Lindvall andBjörklund, 1974; Oke et al., 1980, 1983; Santiago et al., 1989;Aizawa et al., 1991; Young and Wilcox, 1991).

Several studies suggested that the MD may have an involvement in schizophrenia (Carlsson and Carlsson, 1990; Pakkenberg, 1990;Berendse and Groenewegen, 1991; Andreasen et al., 1995; Younget al., 1995; Blennow et al., 1996; Buchsbaum et al., 1996; Heckers,1997); however, few physiological studies have been performedto assess the possible functional significance of a dopaminergicinnervation in this region. In the present study, we examinedthe effects of DA agonists on the basal and evoked activity ofneurons located in the MD and PV nuclei of the rat thalamus recordedin vitro.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Intracellular current-clamp recordings were performed from neurons within sagittal slices of the MD and PV nuclei of the thalamusof adult rats (200-250 gm; Zivic Miller Labs). All procedureswere performed in accordance with the Guide for the Care and Useof Laboratory Animals published by the United States Public HealthService; the experimental protocol was approved by the Universityof Pittsburgh Institutional Animal Care and Use Committee. Therats were deeply anesthetized with chloral hydrate (400 mg/kg,i.p.) before transcardial perfusion with ice-cold physiologicalsaline (124 mM NaCl, 5 mM KCl, 1.2 mM KH₂PO₄, 2.4 mM CaCl₂, 1.3mM MgSO₄, 26 mM NaHCO₃, and 10 mM glucose, and saturated with95% O₂%/5% CO₂; an additional 115 mM sucrose was added to freshstandard superfusate for use with perfusion). The brain was thenremoved rapidly, and 4-mm-thick sagittal blocks containing theMD and PV were made using a Rat Brain Matrix (RBM 4000 S). Theblocks were placed on a Vibratome (Pelco, Series 1000) and sectionedinto 400-µm-thick slices in ice-cold physiological saline. Theslices were then incubated at room temperature in continuouslyoxygenated physiological saline for at least 1 hr beforerecording.

In vitro electrophysiological recording procedure. Recordings were performed using a submersion-type recording chamber. Thechamber was superfused with oxygenated physiological saline maintainedat 33-35°C at a flow rate of 1-2 ml/min (Llinás and Sugimori,1980) controlled by a peristaltic pump (Haake-Büchler, modelMCP 2500). The time required for a complete exchange of mediawithin the chamber was 3 min. Sharp electrodes were constructedfrom 1 mm outside diameter Omegadot (WPI, New Haven, CT) borosilicateglass tubing using a horizontal puller (Flaming-Brown P-80/PC).The electrodes were filled with 3.0 M K⁺ acetate and had resistances of 55-90 M $Omega$ measured in situ. Thelocation of the recording site was determined by visual inspectionof the placement of the recording electrode using a stereomicroscope(Nikon SMZ-2B), with the MD and PV divisions identified usinga rat brain stereotaxic atlas (Paxinos and Watson, 1986). Theelectrodes were connected to the head stage component of a NeuroDataintracellular amplifier (IR-183). Current was injected into neuronsthrough an active bridge circuit integral to the amplifier, withthe amplitude of the current injected and the electrode voltagemonitored on an oscilloscope (Kikusui COS5020-ST). Data were digitizedand stored on VHS videotapes for subsequent off-line analysis.The analysis was performed using custom software (Neuroscope)running on a windows-based microcomputer. The input resistance,spike threshold, current threshold, resting membrane potential(RMP), spike amplitude, and amplitude of the evoked low-thresholdspikes (LTSs) were compared in neurons in control conditions andafter drug treatment. The input resistance was measured by injectinga series of hyperpolarizing constant current pulses of increasingamplitude (150 msec duration) into the cell and measuring theresultant changes in membrane potential. To assess activationand inactivation potentials of the LTSs, a series of hyperpolarizingpulses (150 msec duration) was injected into the cell until aclear LTS was evoked, and then constant hyperpolarizing or depolarizingcurrent was injected into the cells to alter the steady-statemembrane potential. The first derivative of the LTS was obtainedusing the Neuroscope program, and the amplitude of the derivativewas plotted against the value of the membrane potential at whichit was evoked. All data are shown as mean ±SD.

Pharmacological treatment. All drugs were applied by first dissolving them in physiological saline. After obtaining stablebaseline data and recording the responses to intracellular currentinjection, the perfusion lines were switched from control physiologicalsaline to the drug-containing media while maintaining stable perfusionpressure and fluid volume via the peristaltic pump delivery system.The drugs used were quinpirole (10 µM), SKF 38393 (10 µM), SCH23390 (10 µM), Co²⁺ (2.4 mM), Cs⁺ (2 mM), haloperidol (10 µM), and clozapine (10 µM).

Statistics. The following tests were used: Student's t test, ANCOVA, and McNemar comparison test

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The results presented here were obtained from 63 neurons recorded in vitro in the MD that exhibited stable intracellular impalements(duration = 30 min to 3 hr). Stability was defined as exhibitingresting membrane potentials more negative than $-$ 55 mV and spikeaction potentials with amplitudes of 55 mV or greater. The effectsof bath application of the DA D1 agonist SKF 38393 and the DAD2 agonist quinpirole on passive membrane properties were examinedon 11 and 40 MD neurons,respectively.

Basic morphological and physiological properties of thalamic cells recorded in vitro

The morphology of the thalamic cells recorded was examined by intracellular staining with the dye Lucifer yellow. Consistentwith other reports, the cells exhibited somata with diametersranging between 20 and 40 µm that were round or fusiform in shape.Dense clusters of dendrites emanated from the poles of the soma(Fig. 1). All of the cells stained in the present study exhibitedsimilar morphological characteristics (n = 4) that were consistentwith the primary class of relay cells in the MD.

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Figure 1. Photomicrograph of a neuron recorded in the MD thalamus and labeled by intracellular injection with Lucifer yellow. This neuron had a round soma that measured 30 µm in diameter and exhibited a dense array of dendritic processes.

Intracellular recordings in vivo and in vitro have shown that thalamic neurons have two basic patterns of firing, dependingon the level of depolarization or hyperpolarization of the membranepotential: tonic irregular spiking (approximately $-$ 58 mV) andrhythmic burst firing (approximately $-$ 70 mV) (for review, seeSteriade and Deschênes, 1984; Steriade and Llinás, 1988; McCormick,1992). As reported by others, the burst firing recorded in MDthalamic cells was composed of an LTS that triggers the dischargeof 2-10 spikes (Fig. 2).

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Figure 2. Effects of quinpirole on the input resistance and facilitation of LTSs. The input resistance (IR) of this neuron recorded before (A) and after (B) administration of quinpirole (10 µM) was determined by examining the membrane voltage deflections (top traces) produced in response to injections of current (bottom trace) and calculating the input resistance from the I-V regression line (bottom graph). After quinpirole administration, a facilitation of the LTS is observed during injection of depolarizing currents pulses. Moreover, an increase in membrane excitability is revealed, with excitability defined as a reduction in the amount of current required to produce a given level of depolarization of the membrane potential. In the I-V curve, 0 mV corresponds to the RMP.

Effects of D1 agonist on MD cell physiology

Bath-applied SKF 38393 (10 µM) did not produce changes in the resting membrane potential, input resistance, or spike thresholdin 10 of 11 cells tested (Table 1). A slight but nonsignificantdecrease (27%) in the threshold current required to evoke spikefiring was observed after administration of the D1 agonist.


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Table 1. Effect of D1 agonist SKF 38393 and D1 antagonist SCH 23390 on basic membrane properties of thalamic cells

To assess the specificity of DA agonist effects on thalamic cells, the D1 selective antagonist SCH 23390 (10 µM) and the preferentialD2 antagonist haloperidol (13 µM) were tested by bath application.The D1 antagonist SCH 23390 (four cells) and the mixed D1/D2 antagonisthaloperidol (two cells) were tested after 5 min of SKF 38393 administration.Neither antagonist altered the response to SKF 38393; however,haloperidol appeared to produce a depolarization of the membranepotential (RMP control = $-$ 67.5 ± 6.5; SKF 38393 = 66.1 ± 1.1;haloperidol = $-$ 57.4 ± 4.5) without altering the inputresistance.

Effects of D2 agonist on MD cell physiology

Resting membrane potential and input resistance
The pre-drug fluctuations in RMP typically did not exceed ± 3mV; therefore, post-drug changes in RMP greater than ± 5 mV wereoperationally defined as different from baseline. When the D2agonist quinpirole (10 µM) was applied, 19 of 37 (51.3%) of theneurons tested exhibited a 5.9 ± 4.9 mV hyperpolarization of theirmembrane potential [t₍₃₆₎ = $-$ 5.50; p < 0.00003] (Table 2, Figs.3, 4). In contrast, 6 of 37 cells (19%) exhibited a significantdepolarization of the resting membrane potential measured 5 minafter administration of the D2 agonist [3.4 ± 0.7 mV; t₍₃₆₎ =2.57; p < 0.006] (Table 2, Fig. 4). Finally, in 29.7% of thecells tested (11 of 37), quinpirole did not produce changes inthe average resting membrane potential.


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Table 2. Effects of D2 agonist quinpirole and D2 antagonist haloperidol on basic membrane properties of thalamic cells

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Figure 3. The facilitation of the LTS observed after quinpirole administration persisted after the membrane potential of the cell was adjusted by current injection to the original pre-drug control values. A, A cell recorded during control conditions exhibits an evoked action potential in response to depolarizing current injection (RMP = $-$ 66.15). B, Quinpirole administration caused a hyperpolarization of the membrane of this cell by 2.4 mV, in addition to facilitating the expression of the LTS. C, After depolarizing the membrane potential of this cell back to the original pre-drug RMP by current injection, the LTS could still be evoked by small amplitudes of membrane depolarization. It should be noted that LTSs were not evoked at this RMP in the absence of quinpirole administration. mp, Membrane potential.

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Figure 4. Quinpirole administration altered the excitability and spike discharge in half of the MD cells tested. A1, Spikes evoked by current injection during the control period. A2, Quinpirole administration (10 µM) hyperpolarized the membrane potential of this cell, facilitated the expression of the LTS, and increased cell excitability. B1, An LTS evoked by current injection during the control period. B2, Quinpirole administration (10 µM) caused a depolarization of the membrane potential of this cell without altering the LTS. C1, A tonic pattern of firing was evoked in this neuron by current injection during the control period. C2, Administration of quinpirole (10 µM) caused a small hyperpolarization of the membrane potential of the cell, facilitated expression of the LTS, and markedly increased cell excitability. C3, Haloperidol administration (13 µM) reversed the quinpirole-induced hyperpolarization of this cell to control values. The current-evoked action potential now occurred independent of a prominent LTS. The cell excitability also returned to control levels. The bottom traces in each panel indicate the amplitude of the current injected. The bottom dashed line indicates the control RMP, the middle dashed line indicates the spike threshold during the control period, and the top dashed line represents the peak amplitude of the action potential.

Quinpirole did not affect input resistance in the cells that exhibited depolarization of the resting membrane potential orhyperpolarization of the membrane potential, or those that didnot show changes in membrane potential after drug application(Fig. 2). Furthermore, the quinpirole effect on membrane potentialdid not correlate with changes in inputresistance.
Because other drug-induced changes may be secondary to the changes in RMP, we determined whether the effects of quinpiroleon spike threshold, threshold current, and input resistance werecorrelated with the effects on RMP. The factors used in subsequentANOVAs of these variables were based on this correlational analysis(seebelow).

Spike threshold
Because of the trend for effects on membrane potential and given the fact that spike threshold can depend on membrane potential,the possibility was tested that quinpirole would have an effecton spike threshold that was dependent on its effect on membranepotential. Therefore, the effects of quinpirole on spike thresholdwere analyzed with a repeated measures ANCOVA using the effectof quinpirole on membrane potential as a covariate. This analysisrevealed a significant positive correlation between the effectof quinpirole on membrane potential and spike threshold (r = 0.73;p < 0.01), confirming that the effect of quinpirole on spike thresholdcould be predicted in large part by its effects on membrane potential.When this effect was accounted for, the effect of quinpirole onspike threshold was not significant (r (1,1,15) = 2.4; p = 0.15).When the cells were separated according to the quinpirole effectson RMP, the D2 agonist was found to produce an increase in thespike threshold only in the cells that also were depolarized byquinpirole (Table 2). In contrast, in cells in which quinpiroleadministration resulted in either a hyperpolarization or no changein RMP, it also failed to significantly alter spikethreshold.

Afterhyperpolarization
In several cases (n = 5 of 16) (Fig. 5), quinpirole administration was observed to increase the amplitude and duration ofthe post-spike afterhyperpolarization (AHP) (amplitude control,7.9 ± 2.3 mV; amplitude quinpirole, 13.1 ± 6.5 mV; p < 0.08; durationcontrol, 12.9 ± 6.1 msec; duration quinpirole, 28.1 ± 9.5 msec).

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Figure 5. Effects of quinpirole administration on spike AHPs. In several cases quinpirole administration caused the evoked spikes to have longer duration and larger amplitude spike afterhyperpolarizations than in the control conditions. A, An action potential evoked during the control period exhibited a small amplitude and short duration AHP. B, After quinpirole administration (10 µM), the AHP of this cell was increased by 67% in amplitude and 125% in duration. A quinpirole-induced increase in excitability was also noted.

Current-evoked spike discharge
The effects of quinpirole on RMP did not correlate with its effects on the threshold current required to trigger spike discharge;therefore, data from all cells were analyzed as a single group.Quinpirole administration was found to cause a significant decreasein threshold current in the cells tested [t₍₂₉₎ = 4.14; p < 0.001].

Low-threshold spikes
Before drug administration, 8 of 31 (25.8%) of the cells tested exhibited an LTS in response to spike threshold levels ofmembrane depolarization. However, after 10 µM quinpirole administration,48.8% (15 of 31) of these cells exhibited threshold current-evokedLTSs (Table 2, Figs. 2-4). Using a McNemar test that compares thefrequency of LTSs before and after quinpirole, the probabilityof evoking an LTS after quinpirole administration was found tobe significantly greater than during pre-drug conditions (p <0.0005). The effects of quinpirole administration on the depolarization-dependentinactivation curve of the LTS also was analyzed. For membranepotential values between $-$ 55 and $-$ 70 mV, quinpirole produced asmall shift of the curve to the right, indicating that quinpiroleadministration caused a relative facilitation of the evoked LTSsat these membrane potential values. However, between $-$ 70 and $-$ 82mV, quinpirole caused the curve to shift to the left (Fig. 6).In fact, at membrane potential values between $-$ 55 and $-$ 65 mV,the average rate of change in the amplitude of the LTS was largerafter quinpirole administration (55-60 mV: control, 0.023 mV/sec;quinpirole, 0.0580 mV/sec; 61-65 mV: control, 0.0342 mV/sec; quinpirole,0.0593 mV/sec, respectively). In three of the above cells thatexhibited LTSs after quinpirole, the cells also began to exhibitspontaneous spike discharge (Fig. 7). In the cells that were hyperpolarizedby quinpirole administration, the current threshold required toevoke an LTS was decreased; however, this decrease did not reachstatistical significance. Nonetheless, in the cells depolarizedby quinpirole administration, there was a significant decreasein the current threshold required to evoke the LTSs (p < 0.0005;t = 5.38). In 16 of 29 cases (55%), the latency of the LTS orspike after quinpirole was increased significantly (p < 0.00007;t = $-$ 6.8). In addition to the responses produced by administrationof 10 µM quinpirole, the effects of quinpirole administered atdoses of 5 and 50 µM were tested in three cells. At a dose of5 µM, quinpirole had variable effects in that it caused the appearanceof LTSs in 1 of 3 cells, whereas at a dose of 50 µM quinpiroleproduced a hyperpolarization of the membrane potential and evokedLTSs in all of the cases tested

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Figure 6. Effects of quinpirole on the voltage-dependent modulation of the rate of rise of the LTS. When the first derivative of the LTS amplitude was plotted against the membrane potential, the data between $-$ 65 and $-$ 85 mV could be fit to a sigmoidal function. Furthermore, quinpirole appeared to facilitate the LTS for membrane potential values between $-$ 65 and $-$ 70 mV. However, for values of membrane potential between $-$ 56 and $-$ 65 mV, quinpirole caused a substantially larger facilitation of LTSs but could not be fitted to a sigmoidal function. Every point represents the average of seven cells collected during control conditions ( $bullet$ ) and after quinpirole administration ( $open circle$ ).

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Figure 7. Effects of quinpirole administration on spontaneous spike activity of thalamic neurons recorded in vitro. Although thalamic neurons rarely exhibit spontaneous spike discharge in vitro, quinpirole administration was found to trigger spontaneous activity in these cells. A, After quinpirole administration (10 µM), a gradual increase in depolarizing events was found to give rise to full action potentials firing in a tonic-like pattern. B, Quinpirole administration caused this neuron to initiate spontaneous action potential firing in a burst-like pattern, with spikes riding on top of LTSs. C, Shown at faster time base, the burst (B, asterisk) was found to consist of three action potentials.

Effects of antipsychotic drug administration on quinpirole-induced responses
Administration of haloperidol was found to reverse the primary responses produced by quinpirole in four of five cells tested.In this group, haloperidol (13 µM) reversed the membrane hyperpolarizationcaused by quinpirole (Table 3, Fig. 4). Haloperidol administrationalso restored spike threshold to baseline levels and caused theneuron to respond with tonic spike discharge instead of LTSs whencurrent was injected. However, haloperidol did not reverse thesmall decrease in the threshold current required for spike generation;instead it caused a further significant decrease in this value(control = 0.31 ± 0.02 nA; quinpirole = 0.27 ± 0.20 nA; haloperidol= 0.09 ± 0.09 nA; p < 0.03). In cells in which haloperidol wasapplied alone (i.e., without quinpirole pretreatment), it didnot alter any of the basic electrophysiological properties tested(data not shown).


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Table 3. Effects of haloperidol on basic membrane properties of thalamic cells

The responses to bath application of the atypical antipsychotic drug clozapine (10 µM) were also examined. In the three casestested, clozapine was found to reverse the quinpirole-inducedmembrane hyperpolarization (RMP control, $-$ 67.8 ± 0.3 mV; quinpirole, $-$ 72.3 ± 11.5 mV; clozapine, $-$ 61.2 ± 6.5 mV). However, in contrastto haloperidol administration, clozapine failed to reverse thequinpirole-mediated increase in spike threshold, and instead causeda further increase in this parameter (control, $-$ 67.6 ± 15.56 mV;quinpirole, $-$ 52.4 ± 22.7 mV; clozapine, $-$ 46.1 ± 5.4mV).

Possible membrane conductance changes underlying quinpirole-mediated responses

To determine the mechanism through which quinpirole modulates the excitability of MD neurons, experiments were performed toassess the membrane conductance changes that may have contributedto this response. Our initial focus was on the potassium conductances,given the evidence that DA acting on D2-type receptors in striataland substantia nigra zona compacta cells activates K⁺ conductances (Uchimura et al., 1986; Lacey et al., 1987, 1988;Freedman and Weight, 1988, 1989; Surmeier and Kitai, 1993; Liuet al., 1994; Seeman and Van Tol, 1994; Greif et al., 1995). Toassess whether K⁺ conductances play a role in the responses observed after D2 agonistadministration, we retested these responses using different concentrationsof K⁺ in the superfusion fluid (i.e., 2.5, 6.5, and 10 mM). Cell responseswere analyzed separately depending on whether quinpirole causeda facilitation of the LTS. For cells in which the LTS was facilitatedby quinpirole, the reversal potentials for the quinpirole-mediatedresponses were as follows: in 2.5 mM K⁺ = $-$ 89.7 ± 7.0 mV (n = 3); in 6.5 mM K⁺ = $-$ 74.5 ± 8.2 mV (n = 13), and in 10 mM K⁺ = $-$ 66.4 ± 11.2 mV (n = 3). The slope of the regression line forthis group was calculated to be 25.5 mV/log unit K⁺ concentration (Fig. 8). Furthermore, administration of the potassiumchannel blocker cesium (Cs⁺; 2 mM) was found to reverse the quinpirole-induced hyperpolarizationof the membrane potential (RMP control, $-$ 74.3 ± 5.8 mV; quinpirole, $-$ 84.5 ± 2.1 mV; Cs⁺, $-$ 70.4 ± 13.0 mV), and it also reversed the increase in spikethreshold (control, $-$ 53.7 ± 15.3 mV; quinpirole, $-$ 48.9 ± 27 mV;Cs⁺, $-$ 58.2 ± 2.8 mV; n = 3) (Fig. 9). In addition, in the presenceof Cs⁺, quinpirole failed to produce facilitation of the LTS.

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Figure 8. Effects of varying the potassium concentration in the superfusion medium on the reversal potential of the quinpirole-mediated membrane hyperpolarization. The plot shows the reversal potential of quinpirole in cells that also exhibited a quinpirole-induced facilitation of the LTS (quinpirole-facilitated LTS) and in cells in which the LTS was not affected by quinpirole (nonfacilitated LTS) at 2.5, 6.5, and 10 mM K⁺ concentrations. In comparison, the K⁺ reversal potentials as determined by the Nernst equation are illustrated. Quinpirole was found to shift the reversal potential at low [K⁺] concentration to more positive values, whereas at higher [K⁺] concentrations quinpirole shifted the reversal potential to more negatives values.

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Figure 9. The effects of the K⁺ blocker Cs⁺ and the calcium blocker Co²⁺ on the quinpirole-mediated alteration of LTSs. A, MD thalamus neurons exhibit prominent LTSs. A1, Control. A2, Quinpirole administration (10 µM) caused a 2 mV hyperpolarization of the membrane potential and increased the prominence of the LTSs. A3, Administration of Cs⁺ (2 mM) in the presence of quinpirole abolished the LTSs without altering spike discharge. B, MD thalamus neuron without prominent LTSs. B1, Control. B2, Quinpirole administration (10 µM) caused a 5 mV depolarization of the membrane potential and a facilitation of LTS occurrence. B3, Administration of Cs⁺ (2 mM) abolished the LTS and caused the cell to fire in a tonic discharge pattern. C, Effects of calcium blockade on two responses to quinpirole. C1, Control. C2, Administration of quinpirole (10 µM) caused a 10 mV hyperpolarization of the neuron and facilitation of the LTS. C3, Replacement of calcium in the superfusion medium by Co²⁺ (2.4 mM) abolished the LTSs. The bottom dashed line indicates the RMP, the middle dashed line indicates the spike threshold during the control period, and the top dashed line represents the peak amplitude of the action potential.

As a further test of the specificity of this response, recordings were performed under conditions in which the Ca²⁺ in the superfusate had been replaced with Co²⁺. In cases in which the buffer was switched before quinpiroleadministration, facilitation of the LTS by quinpirole did notoccur; however, quinpirole administration was still capable ofcausing a depolarization of the membrane potential (12 mV; RMPcontrol = $-$ 68.6 ± 5.8; quinpirole + Co²⁺ = $-$ 56.3 ± 0.3 mV). In the cases in which the switch to Ca²⁺-free-Co²⁺ buffer was made after quinpirole administration, the facilitationof the LTS by quinpirole was abolished, and the spike thresholdwas returned to control values (control, $-$ 47.1 mV; quinpirole, $-$ 33.7 mV; Co²⁺, $-$ 42.3 mV) (Fig. 9).

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

These experiments show that stimulation of DA D2 receptors by quinpirole resulted in changes in the passive membrane propertiesof thalamic neurons. More specifically, administration of theD2 agonist quinpirole but not the D1 agonist SKF 38393 enhancedthe excitability of MD thalamic neurons in two ways: (1) it increasedthe response of the neuron to depolarizing current pulses and(2) it facilitated the occurrence of LTSs at membrane potentialvalues at which these spikes were not typically triggered. Theexperiments with Co²⁺, Cs⁺, and different potassium concentrations indicated that theseeffects occurred, at least in part, via changes in K⁺ conductances. The D2 selectivity of the quinpirole-mediated responseswas further substantiated by the ability of the preferential D2antagonist haloperidol to reverse theseeffects.

Dopaminergic agonist effects on MD cell excitability

Overall, bath application of either the D1 or D2 agonist to MD cells either failed to alter or produced small and inconsistentchanges in resting membrane potential. Although the administrationof the D1 agonist SKF 38393 did not appear to change the RMP inany of the cells tested, the D2 agonist quinpirole caused a hyperpolarizationin approximately half of the neurons tested, with the remainingcells showing either a small depolarization or no changes in RMP.Neither agonist produced significant changes in the input resistanceof theseneurons.

In contrast, the most consistent effect produced by the D2 agonist quinpirole was to increase the overall excitability ofall MD cells tested, with excitability defined on the basis ofthe amount of depolarizing current required to evoke a spike.This increase in excitability occurred independent of the effectsof quinpirole on resting membrane potential. In other systems,DA has been reported to exert variable effects on excitability.In the striatum, DA appears to decrease excitability of striatalcells via D1- and D2-dependent mechanisms (Norcross and Spehlmann,1978; Mercuri et al., 1985; Uchimura et al., 1986; Calabresi etal., 1987; Hu and Wang, 1988; Hu et al., 1990; Akaoka et al.,1992; Hernandez-Lopez et al., 1997), although DA has been reportedto increase the excitation produced by NMDA receptor activation(Cepeda et al., 1993). In contrast, in the cortex, DA appearsto increase excitability through a D1-dependent mechanism (Bernardiet al., 1982; Penit-Soria et al., 1987; Yang and Seamans, 1996;Shi et al., 1997). In the ventral pallidum it has been reportedthat 72% of the cells tested were inhibited by iontophoretic applicationof DA, whereas 27% were excited (Maslowski and Napier, 1991).However, this is the first report in which DA is observed to affectcell excitability via an effect on theLTSs.

Facilitation of low-threshold spikes by quinpirole

In this study, quinpirole was found to increase the probability of evoking an LTS in MD thalamic neurons. The LTS is consideredto be an important property for regulating thalamocortical function.Electrophysiological studies have revealed that thalamic neuronshave two basic modes of firing: tonic single-spike activity anda rhythmic burst-firing pattern (Deschênes al., 1984; Steriadeand Deschênes, 1984; Steriade and Llinás, 1988; McCormick andPape, 1990) in which the burst activity is driven by LTSs (Steriadeand Deschênes, 1984). In contrast, tonic spike activity predominatesduring waking states or rapid eye movement (REM) sleep. The tonicfiring is associated with depolarized membrane potentials ( $-$ 50to $-$ 55 mV). In this state the cells are depolarized by a pacemakerpotential and repolarized by depolarization-activated K⁺ currents to produce the tonic firing pattern (Jahnsen and Llinás,1984). The bursting firing pattern is characteristic of slow-wavesleep, deep anesthesia, or absence seizures (Hirsch et al., 1983;McCarley et al., 1983; Fourment et al., 1985; Gloor and Fariello,1988; Buzsaki et al., 1990; Curro Dossi et al., 1991; Steriadeet al., 1991). The burst firing of thalamic cells is reportedto be caused by a Ca²⁺-mediated LTS (Jahnsen and Llinás, 1984; Steriade and Deschênes,1984; Coulter et al., 1989; Crunelli et al., 1989; Hernandez-Cruzand Pape, 1989). This low-threshold Ca²⁺ conductance is deinactivated at $-$ 55 mV, reaching a maximum levelof deinactivation at $-$ 75 mV (Llinás and Jahnsen, 1982). The fasteractivation time course of the Ca²⁺ current allows depolarization from hyperpolarized membrane potentialsto generate LTSs that in turn activate one to eight high-frequencyNa⁺ spikes that occur at frequencies of 250-500 Hz. In many cases(10 of 15 in the present study), the occurrence of the LTS waslinked to quinpirole-induced hyperpolarization of the membranepotential. Furthermore, blockade of K⁺ conductances by Cs⁺ reversed the effect of quinpirole on the membrane potential andcaused the facilitated LTS discharge to be replaced by a tonicspike-firing pattern. Although the mechanisms through which DAfacilitates the LTS are unknown, several possibilities may beadvanced based on these data and in comparison with other systems.In fact, a persistent sodium conductance (I_NaP) has recently beendescribed in thalamocortical neurons (Parri and Crunelli, 1998).The activation of this I_NaP at relatively negative potentials(approximately $-$ 70 mV) is consistent with a potential involvementof this conductance in the generation of the LTSs. Because theD2 agonist quinpirole has been shown to play a role in the modulationof TTX-sensitive Na⁺ currents, we cannot exclude the possibility that the effectsproduced by quinpirole in the MD may be mediated by a modulationof this I_NaP.

D2 receptor-mediated regulation of K⁺ conductances

As reviewed above, the most consistent effect produced by quinpirole administration was a significant increase in MD cellexcitability, which appears to be related at least in part toquinpirole-induced facilitation of the LTS. Examination of theeffects of varying K⁺ concentrations and the reversal of these actions by the K⁺ channel blocker cesium supports a K⁺-dependent mechanism for the D2 response. One possible conductancechange that could account for these actions is a D2-dependentmodulation of the I_h. This Na⁺/K⁺ current is reported to underlie the pacemaker potential thatproduces the slow depolarizations between spikes in the thalamus(for review, see McCormick, 1992). The rate at which the I_h isactivated can determine the delay period between subsequent LTSs.Alternately, the I_h may also be affecting the LTS by shiftingits apparent voltage dependence to more depolarized levels, atleast as measured at the soma. In this manner, quinpirole couldproduce its observed effects on the LTS by combined effects onI_h, K⁺ currents, and modulation of LTS threshold. As a result, the LTSwould be evoked at more depolarized RMPs and allow the triggeringof Na⁺ spikes at these more depolarized membrane potentials. The factthat the excitability is increased independent of the effect ofquinpirole on RMP or spike threshold would be consistent withthese events and the fact that the reversal potential for quinpiroleis shifted to more positive potentials at low [K⁺]. However, the significant increase in onset latency for spikesevoked after quinpirole administration suggests that the D2 agonistalso may be activating I_K(A) currents. In neurons of the substantianigra zona compacta, DA administration has been shown to hyperpolarizethe resting potential (Lacey et al., 1987, 1989), and using voltage-clamptechniques this was shown to be mediated by a DA-activated conductance.The reversal potential of this outward current was reported tobe close to the reversal potential for K⁺ (Lacey et al., 1987, 1989). Pharmacological manipulations demonstratedthat this effect was caused by D2 receptor stimulation. In theexperiments presented here, quinpirole also produced a hyperpolarizationin 19 of 32 neurons and in three cases increased the amplitudeof the AHP following action potentials. The reversal potentialfor the quinpirole-mediated hyperpolarization, its dependenceon extracellular K⁺ concentration, and its blockade by Cs⁺ suggest that this is mediated by a change in a K⁺ conductance as well. However, because the change in the quinpirolereversal potential did not precisely follow the predictions ofthe Nernst equation with respect to alterations in K⁺ concentrations, other factors may also play a role in this response.Nonetheless, a quinpirole-mediated change in K⁺ conductance could account for each of the findings reported here,including (1) hyperpolarization of the membrane potential, (2)facilitation of LTS spiking, (3) the increase in spike threshold,(4) the augmentation of the AHP, and (5) the increase in onsetspikelatency.

A proposed role of DA in the modulation of thalamocortical activity

DA has been postulated to play a role in learning processes and goal-directed behavior (Le Moal and Simon, 1991), sensoryinformation processing (Clark and White, 1987), and time perception(Rammsayer, 1989). The thalamus is also likely to play a rolein such processes, because lesions of the reticular thalamic nucleus,which regulates thalamic rhythmic activity (Steriade and Deschênes,1984; Steriade and Llinás, 1988), lead to confusional statesand deficits in information processing (Friedberg and Ross, 1993).Moreover, studies have shown that rhythmic activity states underlyingsleep stages are a result of thalamocortical interactions (Steriadeand Deschênes, 1984; Steriade and Llinás, 1988), and REM sleepdeprivation can lead to disorganized thinking and abnormal socialbehavior in humans (Spiegel, 1982; Naitoh et al., 1990) that hasbeen compared with a state of acute psychosis (Gove, 1970). Itis interesting to note that in studies in rats, sleep deprivationhas been associated with alterations in D2 receptor density inMD thalamic target regions (Brooks et al., 1995).

These correlations may have functional implications with respect to the results presented here. Thus, because D2 stimulationenhances rhythmic activity in the thalamus, alterations in D2stimulation could be predicted to lead to abnormalities in thalamocorticalrhythms. Moreover, nonmedicated schizophrenics have been reportedto show abnormalities in slow-wave sleep (Keshavan et al., 1995)that have been correlated with the state of spindle activity andsynchronization of cortical activity (Steriade and Deschênes,1984; Steriade and Llinás, 1988). Indeed, it has been proposedthat a combination of increased activity of dopaminergic and cholinergicneurons could explain most of the sleep disturbances observedin schizophrenics (Tandon and Greden, 1989; Tandon et al., 1990,1992). Within this framework, one possibility is that the proposeddecrease in tonic DA in schizophrenics (Grace, 1991) may underliesome of the sleep disturbances and EEG alterations observed inthesepatients.

  FOOTNOTES

Received Aug. 12, 1998; revised Sept. 18, 1998; accepted Sept. 22, 1998.

This work was supported by a fellowship from the National Alliance for Research on Schizophrenia and Depression (A.L.) andUnited States Public Health Service Grants MH01055, MH57440, andMH45156. We thank Mr. Brian Lowry for providing the computer programfor data analysis (Neuroscope). We also thank Dr. H. Moore forher advice on the statistical analysis and for critical commentsand usefuldiscussions.
Correspondence should be addressed to Dr. Antonieta Lavin, Department of Neuroscience, 446 Crawford Hall, University of Pittsburgh,Pittsburgh, PA15260.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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