Functional Properties of AMPA and NMDA Receptors Expressed in Identified Types of Basal Ganglia Neurons

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Volume 17, Number 1, Issue of January 1, 1997 pp. 204-215
Copyright ©1997 Society for Neuroscience

Functional Properties of AMPA and NMDA Receptors Expressed in Identified Types of Basal Ganglia Neurons

Thomas Götz¹, Udo Kraushaar¹^,³, Jörg Geiger¹^,³, Joachim Lübke², Thomas Berger¹, and Peter Jonas¹
¹ Physiologisches Institut der Universität Freiburg, ² Anatomisches Institut der Universität Freiburg, and ³ Institut für Biologie III der Universität Freiburg, 79104 Freiburg, Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

AMPA- and NMDA-type glutamate receptors (AMPARs and NMDARs) mediate excitatory synaptic transmission in the basal gangliaand may contribute to excitotoxic injury. We investigated thefunctional properties of AMPARs and NMDARs expressed by six maintypes of basal ganglia neurons in acute rat brain slices (principalneurons and cholinergic interneurons of striatum, GABAergic anddopaminergic neurons of substantia nigra, globus pallidus neurons,and subthalamic nucleus neurons) using fast application of glutamateto nucleated and outside-out membrane patches. AMPARs in differenttypes of basal ganglia neurons were functionally distinct. Thoseexpressed in striatal principal neurons exhibited the slowestgating (desensitization time constant $tau$ = 11.5 msec, 1 mM glutamate,22°C), whereas those in striatal cholinergic interneurons showedthe fastest gating (desensitization time constant $tau$ = 3.6 msec).The lowest Ca²⁺ permeability of AMPARs was observed in nigral dopaminergic neurons(P_Ca/P_Na = 0.10), whereas the highest Ca²⁺ permeability was found in subthalamic nucleus neurons (P_Ca/P_Na= 1.17). NMDARs of different types of basal ganglia neurons wereless variable in their functional properties; those expressedin nigral dopaminergic neurons exhibited the slowest gating (deactivationtime constant of predominant fast component $tau$ ₁ = 150 msec, 100µM glutamate), and those of globus pallidus neurons showed thefastest gating ( $tau$ ₁ = 67 msec). The Mg²⁺ block of NMDARs was similar; the average chord conductance ratiog_60mV/g_+40mV was 0.18-0.22 in 100 µM external Mg²⁺. Hence, AMPARs expressed in different types of basal ganglianeurons are markedly diverse, whereas NMDARs are less variablein functional properties that are relevant for excitatory synaptictransmission and neuronal vulnerability.
Key words: AMPA receptors; NMDA receptors; deactivation; desensitization; Ca²⁺ permeability; Mg²⁺ block; basal ganglia neurons; fast application; glutamate

INTRODUCTION

The basal ganglia are composed of several synaptically interconnected subcortical nuclei (the striatum, globus pallidus, substantianigra, and subthalamic nucleus) that participate in the controlof movement. The extrinsic innervation of the basal ganglia, originatingin the neocortex and the thalamus, is primarily glutamatergic(for review, see Parent and Hazrati, 1995a,b). By contrast, theintrinsic synaptic circuit of the basal ganglia mainly uses $gamma$ -aminobutyrate(GABA) as its transmitter. GABAergic neurons mainly predominatein the striatum, globus pallidus, and substantia nigra pars reticulata,whereas glutamatergic neurons are restricted to the subthalamicnucleus (Rinvik and Ottersen, 1993). In addition, large interneuronsof the striatum use acetylcholine, and neurons of the substantianigra pars compacta use dopamine as transmitters (Yung et al.,1991; Kawaguchi, 1993). Hence, the intrinsic synaptic circuitryof the basal ganglia, unlike that in other CNS regions (hippocampusand neocortex), is based primarily on GABAergic neurons.

In the basal ganglia, as in other brain regions, synaptically released glutamate activates three principal types of glutamatereceptors (GluRs): AMPA receptors (AMPARs)/kainate receptors,NMDA receptors (NMDARs), and metabotropic glutamate receptors(mGluRs). AMPARs and NMDARs mediate fast synaptic transmissionin the basal ganglia (Kawaguchi, 1992; Mori et al., 1994), whereasmGluRs seem to be involved in the induction of long-term changesof synaptic efficacy (Calabresi et al., 1992). In addition, long-lastingactivation of GluRs may be important in the pathophysiology ofbasal ganglia disorders. Activation of AMPARs/kainate receptorsand NMDARs leads to excitotoxic neuronal death via GluR-mediatedCa²⁺ inflow (Choi, 1988; Beal et al., 1991; Chen et al., 1995), whereasactivation of metabotropic GluRs either enhances or reduces excitotoxicity(for review, see Nicoletti et al., 1996). It was proposed thatthe action of excitotoxins on GluRs is a main factor in the developmentof both acute CNS injury (hypoxia, ischemia) and chronic neurologicaldisorders (e.g., Huntington's disease, Parkinson's disease; Young,1993). This raises the question of whether the selective degenerationof striatal principal neurons in Huntington's disease or nigraldopaminergic neurons in Parkinson's disease could be related todifferent functional properties of ionotropic GluRs expressedby these neurons.

Several AMPAR, kainate receptor, and NMDAR subunits were identified by molecular cloning (for review, see Hollmann and Heinemann,1994). In recombinant AMPARs assembled from GluR-A to -D subunits,the Ca²⁺ permeability is determined by the GluR-B subunit (Hollmann andHeinemann, 1994), whereas the gating properties are regulatedby GluR-B and GluR-D subunits (Burnashev, 1993; Mosbacher et al.,1994). In recombinant NMDARs assembled from NR1 and NR2A to NR2Dsubunits, the NR2 subunit confers both the gating properties andthe strength of Mg²⁺ block (Monyer et al., 1994). In situ hybridization and immunocytochemicalanalysis suggested that different types of basal ganglia neuronsexpress distinct subsets of AMPAR and NMDAR subunits (Martin etal., 1993; Standaert et al., 1994; Landwehrmeyer et al., 1995).The functional properties of the native GluRs in these neurons,however, remain unknown. Using the patch-clamp technique in brainslices, we functionally characterized AMPARs and NMDARs in identifiedbasal ganglia neurons. AMPARs differed substantially in gatingand Ca²⁺ permeability, whereas NMDARs were relatively similar with regardto gating and Mg²⁺ sensitivity.

MATERIALS AND METHODS
Brain slice preparation and visualization of different types of neurons in the basal ganglia. Slices 300 µm thick were cutfrom the brains of 10- to 15-d-old Wistar rats with a vibratome(Campden, Loughborough, England). Striatal and midbrain sliceswere cut in the frontal plane, and globus pallidus slices werecut in the parasagittal plane. The mammillary nuclei and the mammillaryrecess of the third ventricle served as landmarks to distinguishthe substantia nigra from the adjacent subthalamic nucleus inmidbrain slices. Slices containing the substantia nigra were fromthe region caudal to the mammillary nuclei and the mammillaryrecess; the pars reticulata of the substantia nigra was locatedventrolaterally, and the pars compacta was located dorsomedially.Slices containing the subthalamic nucleus were from the regiondirectly rostral to the mammillary nuclei, where the mammillaryrecess of the third ventricle was visible (Paxinos and Watson,1986). Neurons were identified by infrared differential interferencecontrast (IR-DIC) videomicroscopy (Stuart et al., 1993) with aNewvicon camera (C2400, Hamamatsu, Hamamatsu City, Japan) andan infrared filter (RG9, Schott, Mainz, Germany) mounted to anupright microscope (Axioskop FS, Zeiss, Oberkochen, Germany).

Patch-clamp recording and fast application of agonists. Patch pipettes were pulled from borosilicate glass tubing (2.0 mmouter diameter, 0.5 mm wall thickness; Hilgenberg, Malsfeld, Germany).When filled with internal solution, they had a resistance of 2-5M $Omega$ . Identified neurons were approached with patch pipettes undervisual control with positive pressure (Stuart et al., 1993). Onlyneurons with resting potentials more negative than $-$ 60 mV wereused. To obtain nucleated patches (Sather et al., 1992), we appliednegative pressure (100-200 mm Hg) during the withdrawal of thepatch pipette. The average diameter of the nucleated patches was8.6-10.9 µm in the types of neurons investigated.

Functional properties of AMPARs and NMDARs were investigated via fast application of agonists (Colquhoun et al., 1992) tonucleated patches, with the exception of AMPAR pharmacology andgating that were examined in outside-out patches to achieve thefastest possible solution exchange. The double-barreled applicationpipette was made from $theta$ glass tubing (2 mm outer diameter, 0.3mm wall thickness, 0.12 mm septum; Hilgenberg), and the Piezo-electricelement used was a PI-275.50 (Physik Instrumente, Waldbronn, Germany)driven by a P-270 high-voltage amplifier. The perfusion rate was50-70 µl min¹ for experiments on nucleated patches and 200 µl min¹ for experiments on outside-out patches. The exchange time (20-80%),measured with an open-patch pipette during a change between Na⁺-rich and 10% Na⁺-rich solution, was 200-300 µsec for the low flow rate and 50-150µsec for the high flow rate. Fast application experiments werestarted as soon as possible after patch excision (1-2 min afteraccess to the cell interior was obtained). Agonist pulses wereapplied every 5 or 8 sec. After completion of the experiment,the patch was blown off and the zero current potential was measured;it was less than ± 3 mV.

Membrane currents were recorded with an Axopatch 200A amplifier (Axon Instruments, Foster City, CA). AMPAR-mediated currentswere filtered at 2-5 kHz and NMDAR-mediated currents at 1 kHzwith the internal four-pole low-pass Bessel filter of the amplifier.Data were digitized and stored on-line with a CED 1401plus interface(CED, Cambridge, England) connected to a personal computer. Thesampling frequency was twice the filter frequency. All recordingswere made at room temperature (20-24°C). Traces shown representsingle sweeps (I-V AMPAR-mediated current), averages from 3 or6 sweeps (I-V NMDAR-mediated current), or averages from 10-40sweeps (kinetics of AMPAR- or NMDAR-mediated current).

Analysis. The decay time constants of the AMPAR- and NMDAR-mediated current were determined by least-squares fit of the decayphase after the peak current. AMPAR deactivation and desensitizationtime course was evaluated by using a fitting interval of 25 msec(deactivation) and 100 msec (desensitization), respectively; theamplitude of the nondesensitizing current was measured at theend of the 100 msec pulse. NMDAR deactivation time course wasanalyzed by using a fitting interval of 3000 msec. Data pointsof the I-V relations were fit by a fifth order polynomial, fromwhich the value of the interpolated reversal potential (V_rev)was calculated. Chord conductance ratios (g_V1/g_V2; g_+40mV/g_80mVfor AMPAR-mediated currents and g_60mV/g_+40mV for NMDAR-mediatedcurrents) were calculated by using the values of the fit I-V curveat V_rev + $Delta$ V_{1, 2}. The P_Ca/P_Na values were calculated from themeasured values of the reversal potential after correction forjunction potentials and ion activities, as described previously[See Experimental Procedures and equation 1 in Geiger et al. (1995)].All numerical values denote mean ± SEM. In the bar graphs, thenumber of patches is shown in parentheses on top of each bar.Statistical significance was assessed by one-way ANOVA at thesignificance level indicated.

Biocytin staining and double labeling. To confirm visual identification, we filled subsets of cells with biocytin (Sigma,St. Louis, MO) in K-gluconate internal solution for 30 min inthe whole-cell recording configuration. Slices were fixed (12hr, 4°C) in 0.1 M phosphate buffer (PB) containing 1% paraformaldehydeand 1% glutaraldehyde, incubated (12 hr, 4°C) in avidin-horseradishperoxidase (HRP) complex (ABC-Elite, Camon, Wiesbaden, Germany)and 0.1% Triton X-100 (Merck, Darmstadt, Germany), and finallyvisualized with 3,3 $'$ -diaminobenzidine as a chromogen (Horikawaand Armstrong, 1988). To assess the immunoreactivity of biocytin-filledstriatal neurons for choline acetyltransferase (ChAT), we fixedslices (30 min, 4°C) in PB containing 4% paraformaldehyde, 0.1%glutaraldehyde, and 1% saturated picric acid and pretreated them(1 hr, 22°C) with 0.5% Triton X-100 in PB. Then slices were incubated(48 hr, 22°C) in a mixture of rat monoclonal antibody againstChAT (final concentration 3.3 µg/ml; Boehringer, Mannheim, Germany),10% goat serum, and 0.1% Triton X-100 and subsequently (24 hr,22°C) with rhodamine-conjugated avidin (diluted 1:200; Vector,Burlingame, CA) and goat anti-rat fluorescein isothiocyanate (FITC)-conjugatedantibody (final concentration 15 µg/ml; Jackson ImmunoResearch,West Grove, PA). Between the incubation steps, slices were rinsedwith PB. After they were washed and mounted in Mowiol (Hoechst,Frankfurt, Germany), double-labeled cells were examined with epifluorescenceillumination (Zeiss filter sets 9 and 14). Control experimentsperformed on three large striatal interneurons indicated thatno FITC staining was observed when the antibody against ChAT wasreplaced by unspecific rat IgG (Sigma).

Solutions and chemicals. Slices were superfused continuously with physiological extracellular solution containing (in mM):125 NaCl, 25 NaHCO₃, 2.5 KCl, 1.25 NaH₂PO₄, 2 CaCl₂, 1 MgCl₂,and 25 glucose, bubbled with 95% O₂/5% CO₂. The HEPES-bufferedNa⁺-rich external solution used for fast application contained (inmM): 135 NaCl, 5.4 KCl, 1.8 CaCl₂, 1 MgCl₂, and 5 HEPES, pH-adjustedto 7.2 with NaOH. The Ca²⁺-rich external solution contained (in mM): 30 CaCl₂, 105 N-methyl-D-glucamine(NMDG), and 5 HEPES, pH-adjusted to 7.2 with HCl. To study AMPARsin isolation, we added 50 µM of the specific NMDAR antagonistD-2-amino-5-phosphonopentanoic acid (D-AP5) to the external solution(both barrels). To study NMDARs in isolation, we either omittedMgCl₂ (referred to as Mg²⁺-free) or reduced it (to 100 µM) and added 10 µM glycine and 10µM of the specific AMPAR/kainate receptor antagonist 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX) (both barrels). With these solutions, fast applicationof glutamate evoked AMPAR- and NMDAR-mediated currents in almostevery nucleated patch isolated.

The internal solution was either K⁺-rich internal solution containing (in mM): 140 KCl, 10 EGTA, 2 MgCl₂, 2 Na₂ATP, and 10HEPES, pH-adjusted to 7.3 with KOH, or Cs⁺-rich internal solution containing (in mM): 140 CsCl, 10 EGTA,2 MgCl₂, 2 Na₂ATP, and 10 HEPES, pH-adjusted to 7.3 with CsOH.To examine the action potential pattern, we used an internal solutioncontaining 145 KCl, 0.1 EGTA, 2 MgCl₂, 2 Na₂ATP, and 10 HEPES,pH-adjusted to 7.3 with KOH in some experiments (see Fig. 2A).The internal solution for intracellular staining contained (inmM): 13 biocytin, 120 K-gluconate, 20 KCl, 10 EGTA, 2 MgCl₂, 2Na₂ATP, and 10 HEPES, pH-adjusted to 7.3 with KOH.
Fig. 2. Confirmation of visual identification of striatal neurons by electrophysiological properties, biocytin staining, and immunocytochemistry.A, Membrane potential changes in response to injection of 0.5sec hyperpolarizing and depolarizing current pulses. Whole-cellcurrent-clamp recording. Top traces are from a medium-sized striatalprincipal neuron, and bottom traces are from a large striatalinterneuron. Currents injected were $-$ 50/130 and $-$ 60/120 pA, respectively.The resting potentials of the two cells were $-$ 71 and $-$ 64 mV; themembrane potentials were set to $-$ 70 mV (dashed lines) by injectionof a small constant current. Note the marked afterhyperpolarizationthat follows each single action potential in the striatal interneuron.B, Camera lucida drawing of a large striatal interneuron filledwith biocytin. The soma and the dendrites of the cell are drawnin black; the axonal arborization is drawn in red. The arrow pointsto the axon close to its origin at one of the primary dendrites.The filled circle in the inset indicates the location of the somaof the filled neuron (Str, striatum; LV, lateral ventricle; Cor,neocortex; D, dorsal; L, lateral). C, Fluorescence microphotographsof a large striatal interneuron filled intracellularly with biocytinand double-labeled with rhodamine-conjugated avidin (left, epi-illumination,510-560 nm) and rat monoclonal antibody against ChAT/FITC-conjugatedgoat anti-rat antibody (right, epi-illumination, 450-490 nm).
[View Larger Version of this Image (54K GIF file)]

L-AMPA, kainate, CNQX, and D-AP5 were obtained from Tocris (Essex, England); other chemicals were from Sigma or Merck. Stocksolutions of 100 mM glutamate and kainate and 25 mM AMPA wereprepared either in distilled water or in the final solution; thepH was adjusted with NaOH or NMDG (free base), depending on themajor cation in the final solution.

RESULTS

Identification of the main types of neurons in the basal ganglia
Figure 1 shows a schematic drawing of the main components of the basal ganglia circuitry and their glutamatergic synapticconnections. Using IR-DIC videomicroscopy (Stuart et al., 1993),we identified the different cell types in this circuitry primarilyon the basis of their location and the size and shape of theirsomata (Fig. 1 and legend). In the striatum, the somata of putativeGABAergic principal neurons were medium-sized and spherical (Str-PN),whereas those of putative cholinergic interneurons were much largerand polygonal (Str-IN). In the substantia nigra, the somata ofputative GABAergic neurons were relatively small and fusiform(SNR), whereas those of putative dopaminergic neurons were largerand polygonal (SNC). In the globus pallidus adjacent to the striatum,mostly neurons with exceptionally large polygonal somata (GP)were found. In the subthalamic nucleus adjacent to the substantianigra, neurons with medium-sized spherical somata predominated(STN). In addition to soma size, the different types of neuronsin the basal ganglia could be distinguished by the shape of theirdendrites. Putative GABAergic neurons of the substantia nigramostly had two, and globus pallidus neurons typically had fourthick primary dendrites that could be followed for ~100 micrometersin the IR-DIC image. By contrast, the other types of neurons exhibitedthinner and less clearly visible dendritic processes.
Fig. 1. Identification of the main types of neurons in the basal ganglia circuitry. Center, Schematic drawing of the main componentscomprising the basal ganglia and their glutamatergic synapticinnervation (Parent and Hazrati, 1995a,b). Left and right, IR-DICimages of neurons in different components of the basal ganglia.Str-PN, Medium-sized striatal principal neurons; Str-IN, largestriatal putative cholinergic interneurons (~2% of all striatalneurons); SNR, substantia nigra pars reticulata, putative GABAergicneurons; SNC, substantia nigra pars compacta, putative dopaminergicneurons; GP, globus pallidus neurons; STN, subthalamic nucleusneurons. The size of the somata of these basal ganglia neuronsis in agreement with published morphological properties. Measuredand published soma diameters were as follows: Str-PN, 13-16 µm(13 µm; Kawaguchi, 1993); Str-IN, 23-34 µm (27 µm; Kawaguchi,1993); SNR, 20-25 µm longitudinal diameter × 10-15 µm transversediameter (20 µm, Poirier et al., 1983); SNC, 20-25 µm (34 × 20µm; Yung et al., 1991); GP, 31-43 µm × 14-23 µm (25-40 µm × 15-25µm; Millhouse, 1986); and STN, 10-15 µm (17 µm; Afsharpour, 1985).
[View Larger Version of this Image (75K GIF file)]

To confirm the visual identification of cell types on the basis of the IR-DIC image, we measured the action potential patternin the current-clamp configuration before patch excision. In thestriatum, principal neurons generated a train of action potentialson sustained injection of a depolarizing current (Fig. 2A, toptrace), whereas putative cholinergic interneurons produced onlya few action potentials, each followed by a marked and long-lastingafterhyperpolarization (Fig. 2A, bottom trace; Kawaguchi, 1993).In the substantia nigra, putative GABAergic neurons fired actionpotentials at a maximal frequency of 30-50 Hz during depolarization,whereas dopaminergic neurons exhibited a characteristic sag duringhyperpolarization (Yung et al., 1991) (data not shown). Globuspallidus neurons exhibited an action potential pattern similarto that of nigral GABAergic neurons, but the degree of adaptationwas more variable, in agreement with published results (Nambuand Llinás, 1994). Subthalamic nucleus neurons showed a characteristicrebound burst of up to five action potentials after hyperpolarizingpulses (Nakanishi et al., 1987; Yung et al., 1991) (data not shown).

In the striatum, visual identification of neuron types was confirmed further by intracellular staining and by immunocytochemicalanalysis. Light microscopic examination of putative cholinergicstriatal interneurons filled with biocytin revealed that theirdendrites were sparsely spiny or aspiny (12 of 12 cells; Fig.2B). The axonal arborization was local and confined to a regionof <500 µm around the soma, with no obvious projections outsidethe striatum (Fig. 2B). Choline acetyltransferase (ChAT) immunoreactivitywas detected in the majority of biocytin-filled large striatalneurons examined (13 of 14 cells tested were positive for ChAT;Fig. 2C). These morphological and immunocytochemical propertiesindicated that the large striatal neurons were cholinergic interneurons.

Activation of AMPARs in basal ganglia neurons by different agonists
To investigate the functional properties of GluRs present in the somatic membrane of basal ganglia neurons, we used fast applicationof agonists to nucleated (Sather et al., 1992) and conventionaloutside-out membrane patches. In conditions that allowed us tostudy AMPA/kainate receptors in isolation (1 mM external Mg²⁺ and 50 µM D-AP5; membrane potential, $-$ 60 mV), 100 msec pulsesof 1 mM glutamate, AMPA, or kainate evoked currents in outside-outpatches in all types of basal ganglia neurons investigated. InFigure 3A, this is exemplified for nigral dopaminergic neurons.Currents produced by 100 msec pulses of glutamate or AMPA werevery similar, showing a rapid rise (20-80% rise time 200-400 µsec),followed by a slower, almost complete desensitization (Fig. 3A,top and middle traces). For both agonists, the amplitude of thenondesensitizing current remaining at the end of the pulse was0.4-7.4% of the peak current amplitude measured at the beginningof the pulse (Fig. 3B).
Fig. 3. Activation of AMPARs in basal ganglia neurons by different agonists. A, Traces of currents activated by 100 msec pulses of1 mM glutamate, AMPA, and kainate in outside-out patches isolatedfrom nigral dopaminergic neurons. Glutamate- and kainate-activatedcurrent are from the same patch, and AMPA-activated current isfrom a different patch. B, Bar graph of the average amplitudeof the nondesensitizing current component relative to that ofthe respective peak current activated by 1 mM glutamate, AMPA,and kainate for the populations of basal ganglia neurons investigated.The amplitude of the nondesensitizing current was measured atthe end of the 100 msec agonist pulse. C, Cross-desensitizationof kainate-activated currents by AMPA in a nucleated patch isolatedfrom a subthalamic nucleus neuron. Top and bottom traces, Currentactivated by 500 µM AMPA. Middle trace, Application of 1 mM kainatein the maintained presence of 500 µM AMPA did not evoke detectablecurrents; recording was obtained between top and bottom tracesfrom the same nucleated patch. Membrane potential, $-$ 60 mV; Na⁺-rich external solution (50 µM D-AP5) in all experiments.
[View Larger Version of this Image (23K GIF file)]

By contrast, currents activated by 100 msec pulses of 1 mM kainate were much smaller in amplitude than those activated byglutamate or AMPA and were only weakly desensitizing (Fig. 3A,bottom trace). The average amplitude of the nondesensitizing currentmeasured at the end of a 100 msec kainate pulse was 60-90% ofthe respective peak current amplitude at the beginning of thepulse in the populations of neurons investigated (Fig. 3B).

Maintained application of AMPA resulted in a complete cross-desensitization of kainate-activated currents in nucleated patchesisolated from all types of neurons examined. In Figure 3C, thisis exemplified for a patch from a subthalamic nucleus neuron.In the presence of 500 µM AMPA, application of 1 mM kainate didnot activate detectable currents (middle trace), whereas pulsesof 500 µM AMPA produced large inward currents in the same patch(top and bottom traces). Identical results were obtained for theother types of neurons (3-5 patches for each cell type). Thisindicates that the currents activated by glutamate, AMPA, andkainate in basal ganglia neurons are mediated by AMPARs, similarto those in hippocampal neurons (Patneau and Mayer, 1991; Patneauet al., 1993).

Gating properties of AMPARs expressed in basal ganglia neurons
Although their pharmacological properties were similar, AMPARs expressed in different types of basal ganglia neurons differedin their gating properties (deactivation and desensitization).In Figure 4, this is exemplified for outside-out patches isolatedfrom the cell types that express AMPARs with the most divergentgating kinetics. The deactivation of AMPARs after 1 msec pulsesof glutamate was twofold faster in patches isolated from globuspallidus neurons than in those from striatal principal neurons(average deactivation time constant $tau$ = 1.1 vs 2.2 msec, 1 mMglutamate; Fig. 4A, Table 1). The average deactivation $tau$ in theother types of basal ganglia neurons (striatal cholinergic interneurons,nigral GABAergic neurons, nigral dopaminergic neurons, and subthalamicnucleus neurons) ranged from 1.2 to 1.7 msec (Fig. 4B, Table 1).
Fig. 4. AMPARs expressed in different types of basal ganglia neurons differ in deactivation and desensitization kinetics. A, Tracesof current activated by 1 msec glutamate pulses in outside-outpatches. Top trace, Striatal principal neuron patch; bottom trace,globus pallidus neuron patch. B, Bar graph of average deactivationtime constants of AMPAR-mediated currents in the types of basalganglia neurons investigated. C, Traces of current activated by100 msec glutamate pulses in outside-out patches. Top trace, Striatalprincipal neuron patch; bottom trace, striatal cholinergic interneuronpatch. D, Bar graph of average desensitization time constantsof AMPAR-mediated currents in the types of basal ganglia neuronsinvestigated. All data are from outside-out patches. Membranepotential, $-$ 60 mV; glutamate concentration, 1 mM; Na⁺-rich external solution (50 µM D-AP5) in all experiments.
[View Larger Version of this Image (22K GIF file)]

Table 1. Functional properties of AMPARs in neurons of the basal ganglia

Cell type Deactivation $tau$ (msec) Desensitization $tau$ (msec) P_Ca/P_Na Rectification index (g_+40mV/g_80mV) Peak current NP, $-$ 60 mV (pA)

Striatum

Striatal principal neurons 2.2 ± 0.1 (10) 11.5 ± 0.9 (10) 0.11 ± 0.00 (9) 0.93 ± 0.02 (9) 692 ± 95 (9)

Striatal cholinergic interneurons 1.2 ± 0.1 (10) 3.6 ± 0.4 (10) 1.16 ± 0.16 (10) 0.49 ± 0.06 (10) 246 ± 18 (10)

Substantia nigra

Nigral GABAergic neurons 1.7 ± 0.2 (8) 3.6 ± 0.3 (9) 0.11 ± 0.01 (8) 1.08 ± 0.17 (7) 326 ± 46 (7)

Nigral dopaminergic neurons 1.6 ± 0.1 (8) 6.1 ± 0.8 (9) 0.10 ± 0.01 (6) 1.01 ± 0.07 (7) 571 ± 90 (7)

Globus pallidus and subthalamic nucleus

Globus pallidus neurons 1.1 ± 0.1 (5) 5.1 ± 0.8 (5) 0.67 ± 0.14 (7) 0.70 ± 0.06 (7) 166 ± 60 (7)

Subthalamic nucleus neurons 1.6 ± 0.1 (8) 3.6 ± 0.4 (9) 1.17 ± 0.30 (6) 0.60 ± 0.06 (6) 285 ± 60 (6)

Deactivation and desensitization time constants of AMPARs were determined using 1 and 100 msec pulses of glutamate, respectively.The P_Ca/P_Na of AMPARs was calculated from the shift of reversalpotential of glutamate-activated currents on exchange of Na⁺-rich by Ca²⁺-rich (30 mM) external solution. The rectification index of theAMPAR-mediated current, g_+40mV/g_80mV, was determinedin Na⁺-rich external solution. The peak current amplitude at $-$ 60 mVwas determined in Na⁺-rich external solution. All data were obtained from nucleatedpatches (NP) using 3 mM glutamate, with the exception of AMPARkinetics, which was studied in outside-out patches using 1 mMglutamate.

The desensitization of AMPARs during 100 msec pulses of glutamate was approximately threefold faster in outside-out patchesisolated from striatal cholinergic interneurons, nigral GABAergicneurons, and subthalamic nucleus neurons than in those from striatalprincipal neurons (average desensitization $tau$ = 3.6 vs 11.5 msec,1 mM glutamate; Fig. 4C, Table 1). The average desensitization $tau$ in the other classes of cells ranged from 5.1 to 6.1 msec (Fig.4D, Table 1). The differences in both deactivation and desensitization $tau$ among the cell populations investigated were highly significant(p < 2 · 10⁴ and p < 10⁴, respectively, one-way ANOVA).

Ca²⁺ permeability and current rectification of AMPARs in basal ganglia neurons
AMPARs expressed in different types of basal ganglia neurons differed markedly in their permeability to Ca²⁺. This is exemplified by nigral dopaminergic neurons that expressAMPARs with the lowest Ca²⁺ permeability (Fig. 5A) and by subthalamic nucleus neurons thatexpress AMPARs with the highest Ca²⁺ permeability (Fig. 5B, Table 1). In Na⁺-rich external solution, the reversal potential of the AMPAR-mediatedpeak current was close to 0 mV for nucleated patches isolatedfrom both cell types ( $-$ 3.5 ± 0.7 mV and $-$ 1.1 ± 1.0 mV). When theNa⁺-rich external solution was exchanged with a Ca²⁺-rich solution, the reversal potential of the glutamate-activatedpeak current shifted to negative values in dopaminergic neuronpatches but changed very little in subthalamic nucleus neuronpatches (reversal potentials in Ca²⁺-rich solution were $-$ 68.0 ± 1.2 mV and $-$ 15.0 ± 4.4 mV, respectively;Fig. 5A, B). The P_Ca/P_Na value calculated from the shift in reversalpotential was ~10-fold higher for subthalamic nucleus neuron AMPARs(P_Ca/P_Na = 1.17) than for nigral dopaminergic neuron AMPARs (P_Ca/P_Na= 0.10; Fig. 5C, Table 1). In striatal cholinergic interneuronsand in globus pallidus neurons, AMPARs were also highly permeableto Ca²⁺ (P_Ca/P_Na = 0.67-1.16), whereas in striatal principal neuronsand nigral GABAergic neurons the Ca²⁺ permeability of AMPARs was low (P_Ca/P_Na = 0.11; Fig. 5C, Table1).
Fig. 5. AMPARs expressed in different types of basal ganglia neurons differ in Ca²⁺ permeability. A, B, I-V relations of glutamate-activated peakcurrents recorded from nucleated patches in Na⁺-rich (open circles) and Ca²⁺-rich (30 mM, filled circles) external solution. A, Patch froma dopaminergic neuron of the substantia nigra pars compacta. B,Patch from a subthalamic nucleus neuron. Recordings of glutamate-activatedcurrents at $-$ 100 mV and +50 mV are shown as inset: top tracesin Na⁺-rich solution and bottom traces in Ca²⁺-rich external solution. The continuous curves represent polynomialsof the fifth order fit to the data points. Reversal potentialsin Ca²⁺-rich solution are indicated by arrows. C, Bar graph of the averagerelative Ca²⁺ permeability (P_Ca/P_Na) of AMPARs expressed in the types of basalganglia neurons investigated, determined from the reversal potentialsof glutamate-activated currents in Na⁺-rich and Ca²⁺-rich external solution. All data are from nucleated patches.External solutions contained 50 µM D-AP5 in all cases.
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Correlated with their relative Ca²⁺ permeability, AMPARs expressed in different types of basal ganglia neurons differed in theshape of the I-V relation of glutamate-activated peak currentin Na⁺-rich external solution. AMPARs with low Ca²⁺ permeability in nucleated patches isolated from striatal principalneurons and nigral GABAergic and nigral dopaminergic neurons hada virtually linear I-V relation; the average values of the rectificationindex (g_+40mV/g_80mV) were close to unity (0.93-1.08;Table 1). By contrast, AMPARs with high Ca²⁺ permeability in nucleated patches from subthalamic nucleus neurons,striatal cholinergic interneurons, and globus pallidus neuronshad a doubly rectifying I-V relation with a region of reducedslope between 0 and +40 mV (Fig. 5B). Accordingly, the averagevalues of the rectification index were between 0.49 and 0.70 (Table1). The differences in both Ca²⁺ permeability and rectification index among different types ofbasal ganglia neurons were highly significant (p < 10⁴ in both cases; one-way ANOVA).

Gating properties of NMDARs expressed in basal ganglia neurons
In conditions that allowed us to study NMDARs in isolation (Mg²⁺-free external solution, 10 µM glycine, and 10 µM CNQX), 10 msecpulses of 100 µM glutamate activated currents in nucleated patcheswith a rising phase of ~10 msec duration (20-80% rise time, 5.7-8.3msec), followed by a substantially slower deactivation that wasbiexponential in all types of basal ganglia neurons investigated.The values of the deactivation time constants, however, differedamong the cell types examined. This is exemplified by the NMDARsexpressed in nigral dopaminergic neurons that showed the slowestdeactivation (Fig. 6A) and those in globus pallidus neurons thatshowed the fastest deactivation (Fig. 6B). The average time constantsof both the fast and the slow component of deactivation were approximatelytwofold lower in nucleated patches from globus pallidus neurons( $tau$ ₁ = 67 msec and $tau$ ₂ = 382 msec, contributing 59 and 41% to thetotal decay amplitude, respectively; Table 2) than in patchesfrom nigral dopaminergic neurons ( $tau$ ₁ = 150 msec and $tau$ ₂ = 1049msec, contributing 66 and 34% to the total decay amplitude; Table2). In the other types of neurons (striatal principal neurons,striatal cholinergic interneurons, nigral GABAergic neurons, andsubthalamic nucleus neurons), the deactivation time course wassimilar to that of NMDARs in nigral dopaminergic neurons (Fig.6C, Table 2). ANOVA tests revealed significant differences amongthe populations of neurons in $tau$ ₁ (p < 0.005), in $tau$ ₂ (p < 0.05),and in the total charge carried by the two components (A₁ · $tau$ ₁+ A₂ · $tau$ ₂, in which A₁ and A₂ denote the relative amplitudes ofthe two components; p < 0.05). No significant differences, however,were found with respect to the values of A₁ and A₂ (p > 0.1).
Fig. 6. NMDARs expressed in different types of basal ganglia neurons differ in gating kinetics. A, B, Traces of current activatedby 10 msec pulses of 100 µM glutamate in nucleated patches andthe biexponential function fit to the decay phase (3), shown superimposedwith its exponential components (1, 2). A, Patch from a dopaminergicneuron of the substantia nigra pars compacta; $tau$ ₁ = 166 msec (64%)and $tau$ ₂ = 1158 msec (36%). B, Patch from a globus pallidus neuron; $tau$ ₁ = 66 msec (78%) and $tau$ ₂ = 356 msec (22%). C, Bar graphs of theaverage time constants of the predominant fast component ( $tau$ ₁,top panel) and the slow component ( $tau$ ₂, bottom panel) of deactivationof NMDARs in the populations of basal ganglia neurons investigated.All data are from nucleated patches. Membrane potential, $-$ 60 mV;Na⁺-rich external solution (Mg²⁺-free, 10 µM glycine, and 10 µM CNQX) in all cases.
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Table 2. Functional properties of NMDARs in neurons of the basal ganglia

Cell type Deactivation $tau$ ₁ (msec) $tau$ ₂ (msec) Amplitude fast (%) Mg²⁺ block (g_60mV/g_+40mV) Peak current NP, $-$ 60 mV (pA)

Striatum

Striatal principal neurons 147 ± 19 1088 ± 255 (5) 73 ± 4 0.21 ± 0.01 (7) 65 ± 12 (7)

Striatal cholinergic interneurons 130 ± 18 687 ± 110 (6) 61 ± 3 0.20 ± 0.02 (8) 59 ± 13 (6)

Substantia nigra

Nigral GABAergic neurons 142 ± 5 797 ± 158 (5) 70 ± 2 0.22 ± 0.01 (6) 137 ± 44 (5)

Nigral dopaminergic neurons 150 ± 12 1049 ± 107 (7) 66 ± 4 0.21 ± 0.03 (8) 154 ± 31 (7)

Globus pallidus and subthalamic nucleus

Globus pallidus neurons 67 ± 10 382 ± 80 (6) 59 ± 6 0.21 ± 0.02 (6) 60 ± 14 (6)

Subthalamic nucleus neurons 137 ± 16 833 ± 225 (6) 73 ± 6 0.18 ± 0.03 (6) 169 ± 61 (7)

The deactivation time constants of NMDARs were determined by using 10 msec pulses of 100 µM glutamate in Mg²⁺-free Na⁺-rich external solution and fitting the decay phase with the sumof two exponentials. The contribution of the fast component tothe total decay amplitude also was assessed from the biexponentialfit. The rectification index of the NMDAR-mediated current, g_60mV/g_+40mV,was determined from the I-V relation in Na⁺-rich external solution containing 100 µM Mg²⁺. The peak current amplitude at $-$ 60 mV was determined in Mg²⁺-free Na⁺-rich external solution. All data were obtained from nucleatedpatches (NP).

Mg²⁺ block of NMDARs in basal ganglia neurons
Although the deactivation time course of NMDARs differed among basal ganglia neurons, their Mg²⁺ sensitivity was similar. This was assessed from the shape ofthe I-V relation of NMDAR-mediated currents in Na⁺-rich external solution containing 100 µM Mg²⁺. As an example, Figure 7A shows a peak I-V relation of NMDAR-mediatedcurrents in a nucleated patch isolated from a subthalamic nucleusneuron. Glutamate-activated currents reversed close to 0 mV andshowed a region of negative slope conductance at membrane potentialsbelow $-$ 40 mV (Fig. 7A), caused by the voltage-dependent blockby external Mg²⁺. Similar results were obtained for the other types of basal ganglianeurons investigated; the average values of the rectificationindex g_60mV/g_+40mV were between 0.18 and 0.22 (Fig.7B, Table 2) but were not significantly different among the populationsof basal ganglia neurons investigated (p > 0.5; one-way ANOVA).This indicates that NMDARs expressed in all types of basal ganglianeurons are blocked by external Mg²⁺ with high sensitivity.
Fig. 7. NMDARs expressed in basal ganglia neurons show similar sensitivity to external Mg²⁺. A, I-V relation of glutamate-activated peak currents in Na⁺-rich external solution containing 100 µM Mg²⁺ in a nucleated patch isolated from a subthalamic nucleus neuron.Traces of glutamate-activated currents at membrane potentialsvaried from $-$ 100 mV to +40 mV in 20 mV steps are shown as inset.The continuous curve represents a polynomial of the fifth orderfit to the data points. B, Bar graph of the average rectificationindex, g_60mV/g_+40mV, of the NMDAR-mediated currentin the types of basal ganglia neurons investigated. All data arefrom nucleated patches. Na⁺-rich external solution (100 µM external Mg²⁺, 10 µM glycine, and 10 µM CNQX) in all experiments.
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DISCUSSION
Both AMPARs and NMDARs are present in the somatic membrane of basal ganglia neurons. The present paper provides, to our knowledge,the first description of their gating and permeation properties.AMPARs are markedly diverse, whereas NMDARs are less variablein their functional characteristics.

Functional properties of AMPARs and NMDARs expressed in basal ganglia neurons
AMPARs expressed in different types of basal ganglia neurons differed in their gating properties. Deactivation and desensitizationof AMPARs in striatal principal neurons were slow (deactivation $tau$ = 2.2 msec and desensitization $tau$ = 11.5 msec; Table 1), resemblingAMPAR gating in hippocampal and neocortical pyramidal cells (deactivation $tau$ = 2.5-3.0 msec and desensitization $tau$ = 11.2-15.2 msec) (Hestrin,1993; Geiger et al., 1995). By contrast, deactivation and desensitizationof AMPARs expressed in the other types of basal ganglia neuronswere much faster (deactivation $tau$ = 1.1-1.7 msec and desensitization $tau$ = 3.6-6.1 msec; Table 1), comparable to AMPAR gating in hippocampaland neocortical GABAergic interneurons (deactivation $tau$ = 1.4-2.1msec and desensitization $tau$ = 3.3-6.1 msec) (Hestrin, 1993; Livseyet al., 1993; Jonas et al., 1994; Geiger et al., 1995).

AMPARs expressed in different types of basal ganglia neurons also differed markedly in their Ca²⁺ permeability. AMPARs in striatal principal neurons and nigralGABAergic and dopaminergic neurons were almost impermeable toCa²⁺ (P_Ca/P_Na = 0.10-0.11; Table 1), like those in hippocampal andneocortical pyramidal neurons (0.07-0.10; Geiger et al., 1995;Mayer and Westbrook, 1987). Surprisingly, AMPARs expressed instriatal cholinergic interneurons, subthalamic nucleus neurons,and globus pallidus neurons were highly Ca²⁺ permeable (P_Ca/P_Na = 0.67-1.17; Table 1); the P_Ca/P_Na valuewas comparable to that reported for hippocampal and neocorticalGABAergic interneurons [0.69-1.59; Geiger et al. (1995), recordedunder experimental conditions identical to those in the presentpaper].

In the hippocampus and neocortex, the neuron types that express Ca²⁺-permeable AMPARs are characterized by three main properties:the use of GABA as their transmitter, the specific expressionof Ca²⁺-binding proteins (parvalbumin, calbindin, or calretinin), andthe generation of high-frequency trains of action potentials onsustained injection of depolarizing current (for review, see Jonasand Burnashev, 1995). In the basal ganglia, a more complex pictureemerges. First, the neurons that express Ca²⁺-permeable AMPARs are thought to use various transmitters (acetylcholine,GABA, and glutamate; Parent and Hazrati, 1995a,b). Second, theseneurons also differ in their content of Ca²⁺-binding proteins and their action potential pattern. Whereasglobus pallidus neurons and subthalamic nucleus neurons generatetrains of action potentials on sustained injection of depolarizingcurrent and are positive for parvalbumin (Celio, 1990), striatalcholinergic interneurons produce only a few action potentialsseparated by long-lasting afterhyperpolarizations (Fig. 2A) anddo not express parvalbumin, calbindin, or calretinin (Kawaguchiet al., 1995).

Functional differences among NMDARs expressed in different types of basal ganglia neurons also were noted but were much smallerthan among AMPARs. NMDARs expressed in basal ganglia neurons deactivatedwith time constants $tau$ ₁ = 130-150 msec and $tau$ ₂ = 687-1088 msec (Table2), with the exception of NMDARs in globus pallidus neurons thatshowed significantly faster deactivation ( $tau$ ₁ = 67 msec and $tau$ ₂= 382 msec; Table 2). In all types of basal ganglia neurons,NMDAR deactivation was faster than in hippocampal pyramidal neurons( $tau$ ₁ = 175-288 msec and $tau$ ₂ = 1190-2920 msec; Spruston et al., 1995).

NMDARs expressed in basal ganglia neurons were highly sensitive to external Mg²⁺, like those in hippocampal and neocortical pyramidal neuronsand interneurons (Nowak et al., 1984; Koh et al., 1995; Sprustonet al., 1995). The rectification index g_60mV/g_+40mVof NMDAR-mediated currents in the presence of 100 µM externalMg²⁺ was 0.18-0.22 (Table 2), not significantly different among thepopulations of neurons examined.

Putative subunit composition of native AMPARs and NMDARs in the basal ganglia
Immunocytochemical analysis indicated that AMPARs in different types of basal ganglia neurons differ in their subunit composition(Petralia and Wenthold, 1992; Martin et al., 1993). Striatal principalneurons express predominantly GluR-A and -B/-C subunit protein,whereas striatal cholinergic interneurons express GluR-A and -D.Nigral GABAergic neurons are positive for GluR-A, -B/-C, and -D,whereas dopaminergic neurons are enriched in GluR-A and GluR-B/-C.Globus pallidus neurons mostly express GluR-A subunit protein,but subsets of cells also express GluR-B/-C and -D. Finally, subthalamicnucleus neurons predominantly express GluR-A (Martin et al., 1993).

These immunocytochemical results are consistent with the previous suggestion that the GluR-B subunit in the flip splice versionis a determinant of slow gating, whereas the GluR-D subunit, particularlyin the flop version, is a determinant of rapid gating of bothrecombinant AMPARs (Burnashev, 1993; Mosbacher et al., 1994; Partinet al., 1994) and native AMPARs (Geiger et al., 1995). In thebasal ganglia, striatal principal neurons express high levelsof GluR-B/-C, but not GluR-D, resulting in the formation of AMPARswith the slowest gating, whereas striatal cholinergic interneuronsexpress undetectable levels of GluR-B/-C and high amounts of GluR-D,leading to the assembly of AMPARs with the fastest gating in thebasal ganglia. GluR-D subunits apparently dominate over GluR-Bsubunits in heteromeric combinations, as suggested by the rapidgating of AMPARs expressed in nigral GABAergic neurons (Table1).

The results are also consistent with the hypothesis that the GluR-B subunit determines both Ca²⁺ permeability and current rectification of recombinant and nativeAMPARs (for review, see Hollmann and Heinemann, 1994; Jonas andBurnashev, 1995). Striatal principal neurons and nigral GABAergicand dopaminergic neurons express GluR-B/-C subunits at high levels,resulting in the formation of AMPARs with low Ca²⁺ permeability and linear conduction properties. Striatal cholinergicinterneurons, subthalamic nucleus neurons, and possibly globuspallidus neurons express low amounts of GluR-B/-C subunits, leadingto the formation of highly Ca²⁺-permeable receptors with inwardly or doubly rectifying I-V relations(for review, see Jonas and Burnashev, 1995).

In situ hybridization studies indicated differential expression of NMDAR subunits and splice variants (Standaert et al., 1994;Landwehrmeyer et al., 1995). The NR1 subunit is expressed abundantlyin all types of basal ganglia neurons. The C-terminal deletionvariant (NR1_x0x), however, is expressed selectively in striatalprincipal neurons, whereas the N-terminal insertion variant (NR1_1xx)is found exclusively in subthalamic nucleus neurons (Standaertet al., 1994). Striatal principal neurons express predominantlyNR2B subunit mRNA, together with small amounts of NR2A mRNA, whereasthe other cell types investigated predominantly express NR2D,together with small amounts of NR2B and NR2C (Standaert et al.,1994; Landwehrmeyer et al., 1995).

Given the differential expression of NR1 splice variants and NR2 subunits, it was surprising that only relatively minor functionaldifferences of NMDAR properties among different cell types wereobserved. Unlike the native receptors, recombinant NMDARs assembledfrom different subunits differ in their gating kinetics and Mg²⁺ sensitivity. Deactivation of recombinant NR1/NR2D receptors isslower than that of recombinant NR1/NR2A, NR2B, or NR2C receptors( $tau$ = 4.8 vs 120-400 msec; Monyer et al., 1994), and the Mg²⁺ sensitivity of recombinant NR1/NR2C and NR2D NMDARs is lowerthan that of NR1/NR2A and NR2B NMDARs (Ishii et al., 1993; Monyeret al., 1994). Native NMDARs in striatal principal neurons (presumablyNR1/NR2B heteromeric receptors), however, were not different fromthose in striatal cholinergic interneurons, nigral GABAergic anddopaminergic neurons, and subthalamic nucleus neurons (possiblyNR1/NR2D receptors) in the functional characteristics examined.Conversely, the difference in NMDAR deactivation kinetics betweenglobus pallidus neurons (possibly NR1/NR2D receptors) and theother cell types could not be traced back to any known differencein subunit composition. A possible explanation may be that theNR2B subunit is dominant in determining the functional propertiesof heteromeric NMDARs, because all types of neurons in the basalganglia express NR2B, albeit in small amounts. It cannot be excluded,however, that certain NMDAR subunits are targeted to peripheraldendrites or presynaptic elements and thus may be absent fromnucleated patches.

Functional significance: cell-specific regulation of glutamatergic synaptic transmission and selective vulnerability
The present results suggest that excitatory synaptic currents in different types of neurons of the basal ganglia circuitryare mediated by functionally distinct AMPARs and NMDARs. On thebasis of the difference in deactivation and desensitization timecourse, it is expected that AMPARs in striatal principal neuronswill mediate relatively slow EPSCs, whereas AMPARs in all othertypes of basal ganglia neurons may generate faster EPSCs, similarto those in neurons of other motor systems (e.g., cerebellar granulecells; Silver et al., 1996). In striatal principal neurons andnigral GABAergic and dopaminergic neurons, synaptic activationis expected to produce Ca²⁺ inflow through NMDARs, but not AMPARs, whereas in the other typesof neurons, synaptically released glutamate very likely activatesa dual pathway of GluR-mediated Ca²⁺ entry. It seems possible, therefore, that excitatory synapsesin the basal ganglia exhibit different forms of synaptic plasticity,dependent on the functional properties of their postsynaptic GluRs(Gu et al., 1996).

Activation of AMPARs, NMDARs, and certain subtypes of mGluRs by sustained elevation of glutamate leads to a rise in intracellularCa²⁺ concentration that is thought to trigger excitotoxin-mediatedneuronal death (Choi, 1988). Although the presence of AMPARs andNMDARs in all types of basal ganglia neurons is consistent withthis view, our results cannot explain cell-specific differencesin vulnerability directly. After acute application of excitotoxinsin vitro, striatal principal neurons degenerate, whereas cholinergicinterneurons are preserved (Beal et al., 1991). Chronic neurodegenerativedisorders, e.g., Huntington's and Parkinson's disease, also specificallyaffect certain cell types (striatal principal neurons and nigraldopaminergic neurons, respectively; Young, 1993). Hence, the typesof basal ganglia neurons expressing Ca²⁺-permeable AMPARs seem to be less vulnerable than those expressingCa²⁺-impermeable AMPARs. A relation may exist, however, between thegating kinetics of GluRs and the vulnerability of neurons, becausethe cell types expressing AMPARs and NMDARs with the slowest gatingseem to be the most susceptible. Various additional factors, however,including metabotropic GluRs or Ca²⁺-binding proteins, may contribute to selective neuronal degeneration.

A hallmark of several basal ganglia diseases is the disturbed balance between the activity of the "direct pathway" that facilitatesmovement and the "indirect pathway" that inhibits movement viathe subthalamic nucleus (Albin et al., 1989). Because the functionof the indirect pathway is dependent on both the stimulation byacetylcholine released from striatal interneurons and the activityof subthalamic nucleus neurons, a block of Ca²⁺-permeable AMPARs may result in selective suppression of the indirectpathway. Hence, substances blocking Ca²⁺-permeable AMPARs, perhaps derived from polyamine toxins (Blaschkeet al., 1993), may be useful agents in the treatment of basalganglia diseases.

FOOTNOTES

Received July 22, 1996; revised Oct. 7, 1996; accepted Oct. 17, 1996.

This work was supported by Deutsche Forschungsgemeinschaft Grant BE1859 to T.B. and SFB505/C5 to P.J. We thank Mrs. B. Plessow-Freudenbergfor help with the immunocytochemistry, Dr. M. Häusser for adviceconcerning the preparation of midbrain slices, and Drs. J. Bischofberger,G. B. Landwehrmeyer, and M. Martina for critically reading thismanuscript.

Correspondence should be addressed to Dr. Peter Jonas, Physiologisches Institut der Universität Freiburg, Hermann-Herder-Strasse7, D-79104 Freiburg, Germany.

T.G. and U.K. contributed equally to this work.

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Volume 17, Number 1, Issue of January 1, 1997 pp. 204-215 Copyright ©1997 Society for Neuroscience

Functional Properties of AMPA and NMDA Receptors Expressed in Identified Types of Basal Ganglia Neurons

Volume 17, Number 1, Issue of January 1, 1997 pp. 204-215
Copyright ©1997 Society for Neuroscience