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The Journal of Neuroscience, July 16, 2003, 23(15):6245-6254
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Receptor Subtypes Involved in the Presynaptic and Postsynaptic Actions of Dopamine on Striatal Interneurons
Diego Centonze,1 Cristina Grande,2 Alessandro Usiello,3 Paolo Gubellini,1 Eric Erbs,3 Ana B. Martín,2 Antonio Pisani,1 Nadia Tognazzi,3 Giorgio Bernardi,1 Rosario Moratalla,2 * Emiliana Borrelli,3 * andPaolo Calabresi1 * 1Clinica Neurologica, Dipartimento di Neuroscienze, Università "Tor Vergata," 00133 Rome, Italy, and Istituto di Ricovero e Cura a Carattere Scientifico Fondazione Santa Lucia, 00179 Rome, Italy, 2Instituto Cajal, Consejo Superior de Investigaciones Científicas, 28002 Madrid, Spain, and 3Institut de Génétique et de Biologie Moléculaire et Cellulaire, Centre National de la Recherche Scientifique–Institut National de la Santé et de la Recherche Médicale–Université Louis Pasteur, BP 10142, CU de Strasbourg, France
Abstract
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Abstract
Introduction
By stimulating distinct receptor subtypes, dopamine (DA) exerts presynaptic and postsynaptic actions on both large aspiny (LA) cholinergic and fast-spiking (FS) parvalbumin-positive interneurons of the striatum. Lack of receptor- and isoform-specific pharmacological agents, however, has hampered the progress toward a detailed identification of the specific DA receptors involved in these actions.To overcome this issue, in the present study we used four different mutant mice in which the expression of specific DA receptors was ablated. In D1 receptor null mice, D1R-/-, DA dose-dependently depolarized both LA and FS interneurons. Interestingly, SCH 233390 (10 µM), a D1-like (D1 and D5) receptor antagonist, but not L-sulpiride (3–10 µM), a D2-like (D2, D3, D4) receptor blocker, prevented this effect, implying D5 receptors in this action. Accordingly, immunohistochemical analyses in both wild-type and D1R-/- mice confirmed the expression of D5 receptors in both cholinergic and parvalbumin-positive interneurons of the striatum.
In mice lacking D2 receptors, D2R-/-, the DA-dependent inhibition of GABA transmission was lost in both interneuron populations. Both isoforms of D2 receptor, D2L and D2S, were very likely involved in this inhibitory action, as revealed by the electrophysiological analysis of the effect of the DA D2-like receptor agonist quinpirole in two distinct mutants lacking D2L receptors and expressing variable contents of D2S receptors.
The identification of the receptor subtypes involved in the actions of DA on different populations of striatal cells is essential to understand the circuitry of the basal ganglia and to develop pharmacological strategies able to interfere selectively with specific neuronal functions.
Key words: basal ganglia; D1 receptors; D2L receptors; D2S receptors; electrophysiology; GABA transmission; mutant mice
Introduction
Nigrostriatal dopamine (DA) innervation plays an essential role in the control of striatal neuron activity by interacting with multiple membrane conductances (Calabresi et al., 1987; Schiffmann et al., 1995
On the basis of the main transmitter released, striatal interneurons are differentiated into two distinct groups: cholinergic cells and GABAergic cells. They comprise only 2–4% of the neuronal population of the striatum, the remaining being represented by medium spiny projection cells (Kawaguchi, 1992
DA controls striatal interneuron activity via presynaptic and postsynaptic actions and distinct receptor subtypes. Pharmacological studies in slices have revealed that DA receptors of the D1-like subfamily (D1 or D5 receptors) are involved mainly in the direct membrane depolarization of both large aspiny (LA) cholinergic cells (Aosaki et al., 1998
In the present in vitro electrophysiological studies, we used four different mutant mice, in which the expression of specific DA receptors is either ablated or altered to clarify the involvement of the most abundant DA receptors expressed in the striatum, D1 and D2, in these functions. To do this, D1 and D2 receptor-deficient mice were used to identify the receptor subtype involved in the depolarizing and presynaptic effects, respectively, of DA on both LA and FS interneurons. In addition, to detail which receptor isoform of the D2 receptor mediates the inhibitory action of DA on the GABAergic inputs to these cells, we used two recently generated mice. These mice are characterized by the complete absence of the long isoform of the D2 receptors (D2L) but by variable expression of the D2S isoform.
Materials and Methods
Male mice lacking DA D1 (D1R-/-) (Xu et al., 1994Electrophysiology
Corticostriatal coronal slices (200–300 µm) were prepared from tissue blocks of the brain with the use of a vibratome (Calabresi et al., 1997Whole-cell patch-clamp recordings were made with borosilicate glass pipettes (1.8 mm outer diameter; 3–5 M
) containing (in mM): 125 K +-gluconate, 10 NaCl, 1.0 CaCl2, 2.0 MgCl2, 0.5 BAPTA, 19 HEPES, 0.3, 1.0 Mg-ATP, adjusted to pH 7.3 with KOH.
The striatum could be readily identified under low-power magnification, whereas individual neurons were visualized in situ using a differential interference contrast (Nomarski) optical system. This used an Olympus BX50WI (Tokyo, Japan) noninverted microscope with 40x water immersion objective combined with an infrared filter, a monochrome CCD camera (COHU 4912), and a PC-compatible system for analysis of images and contrast enhancement (WinVision 2000, Delta Sistemi, Rome, Italy). Recording pipettes were advanced toward individual cells in the slice under positive pressure, and on contact, tight G
To study spontaneous GABAA-mediated IPSCs, the recording pipettes (5–8 M
Drugs were applied by dissolving them to the desired final concentration in saline. CNQX and MK-801 were from Tocris (Bristol, UK). Bicuculline, quinpirole, and SCH 23390 were from RBI (Natick, MA). DA, tetrodotoxin (TTX), and L-sulpiride were from Sigma (St. Louis, MO).
Animals and tissue preparation for immunoassays
Adult male D1R-/- and WT mice were deeply anesthetized with sodium pentobarbital and perfused intracardially with 4% paraformaldehyde in 0.1 M phosphate buffer (PB), pH 7.4. Their brains were removed and postfixed in the same solution for 2 hr at 4°C. Fixed brains were cryoprotected with 30% sucrose in 0.1 M PBS, frozen in dry ice and sectioned (25 µm thick) with a freezing microtome. Coronal sections through the striatum were collected and stored in PBS with 0.02% sodium azide at 4°C for immunocytochemistry. All of the studies were approved by the appropriate animal care committee at the Cajal Institute, Consejo Superior de Investigaciones Científicas (CSIC), and all efforts were made to minimize the number of animals used and their suffering.Antisera information
To localize DA D5 receptors, we used a polyclonal rabbit antiserum developed and characterized at the Cajal Institute, CSIC (see below). The dilution used was 1:2000. Striatal interneurons were identified with a polyclonal goat antiserum against choline acetyltransferase (ChAT; 1:1000 dilution; Chemicon, Temecula, CA) for cholinergic neurons and a monoclonal mouse antibody against parvalbumin (PV; 1:1000 dilution; Sigma). All primary antibodies were diluted in 0.1 M PBS, with 0.2% Triton X-100 (PBS-TX), 1% bovine serum albumin, and 0.1% sodium azide.Generation of a polyclonal antiserum against D5 dopamine receptor
A specific polyclonal antiserum against the mouse dopamine D5 receptor was raised at the Cajal Institute, CSIC.Generation of a glutathione S-transferase–D5 receptor fusion protein. A fragment of cDNA encoding the C terminus of the mouse dopamine D5 receptor (amino acids 377–477) was generated by PCR using specific primers designed from the published sequence. The sequence of the forward primer was 5'-CGGGATCCGTGCAGACGGTAAACATC-3' and that of the reverse primer was 5'-GCGAATTCCTAACAGTTTTATGGAAAC-3'. These primers incorporate BamHI and EcoRI sites at their 5' ends, respectively, to ensure successful subcloning and fragment orientation. PCR reaction conditions were 94°C for 4 min, 55°C for 30 sec, and 72°C for 30 sec, followed by 25 cycles of 94°C for 30 sec, 55°C for 30 sec, and 72°C for 30 sec. Then, the reaction product was incubated for 2 min at 72°C and quickly taken to 4°C in ice-chilled water. The PCR product was purified by GEN-CLEAN (Q-Biogen), digested with BamHI and EcoRI, and purified once again with GEN-CLEAN. The DNA fragment was ligated between the BamHI and EcoRI sites of the plasmid pGEX-2T for bacterial expression of a fusion protein composed of glutathione S-transferase (GST) and the C terminus of D5 receptor.
Generation of anti-D5 receptor antiserum. Bacterial expression of GST/D5 receptor was induced in exponentially growing Escherichia coli BclI with 0.5 mM isopropyl-
-thiogalactopyranoside for 8 hr. The recombinant fusion protein was then purified using glutathione Sepharose 4B beads (Amersham Biosciences), and it was used subsequently to inoculate two rabbits following standard protocols. Serum samples were collected at different times after inoculation to monitor antibody production with an enzyme-linked immunosorbent assay.
Purification of anti-D5 receptor antiserum by high-affinity chromatography. We have used the immunospecific method that exploits the antigen–antiserum binding specificity. Purified GST–D5 fusion protein (8 mg) was immobilized on 1 gm of cianogen bromide-activated Sepharose resin (Amersham Biosciences) using a coupling buffer (0.1 M NaHCO3/0.5 M NaCl, pH 8.3). Then, the resin was incubated in 0.2 M glycine, pH 8.0, to block the remaining active groups and rinsed three times with coupling buffer and distilled water. The resin was equilibrated with PBS buffer, and then 1 ml of the anti-D5 antiserum (diluted 10 times in Tris-HCl buffer) was mixed and incubated with the beads for 4 hr. This sample was transferred into a Bio-Rad column (Bio-Rad, Hercules, CA), rinsed with 20 vol of 10 mM Tris, pH 7.5, and rinsed again with 10 vol of 50 mM Tris and 100 mM NaCl, pH 7.5. After that, the antibody was eluted in 20 bed-volumes of 100 mM glycine, pH 2.5, and collected in 1 ml elution fractions. Antibody-containing fractions were pooled and dialyzed overnight in 0.1 M PBS with 0.02% sodium azide. The specificity of the anti-D5 receptor antiserum was determined by immunohistochemistry and Western blot analysis.
Immunoblot analysis
Brains were removed rapidly from decapitated WT mice and rats. Prefrontal cortex and striatum were isolated and frozen immediately on dry ice. Brain samples were dounce-homogenized in 20 vol of buffer containing 20 mM HEPES, pH 7.9, 0.4 M NaCl, 20% glycerol, 5 mM MgCl2, 0.5 mM EDTA, 0.1 mM EGTA, 1% IGEPAL CA-630, 10 mg/ml leupeptin, 0.1 mM p-aminobenzamidine, 1 mg/ml pepstatin, 0.5 mM phenylmethylsufonyl fluoride, and 5 mM dithiothreitol. Samples were incubated in this buffer for 30 min at 4°C, and insoluble material was removed by centrifugation at 15,000 x g for 30 min. Protein concentration in resulting extracts was assayed using the Bio-Rad Bradford method.Aliquots of protein extracts (containing 70 µg of protein) were boiled for 3 min and separated by size on a minigel SDS-PAGE apparatus (Bio-Rad) using 10% polyacrylamide gel (with a 29:1 ratio of acrylamide to N, N'-methylenebisacrylamide). Proteins were transferred electrophoretically to a nitrocellulose membrane (Schleicher & Schuell, Dassel, Germany). Blots were incubated with antiserum at 1:1000 dilution in buffer containing 5% nonfat dairy milk for 4 hr. Goat anti-rabbit IgG conjugated to horseradish peroxidase was used to detect the binding of anti-D5 antibody. The immunoreactive bands were detected autoradiographically using Hyperfilm-enhanced chemiluminescence (ECL) films (Amersham Biosciences) and an ECL kit (Amersham Biosciences). Molecular weights were determined on the basis of the mobility of prestained SDS-PAGE standards, broad range (Bio-Rad).
Immunohistochemical procedures
Free-floating double-labeled immunocytochemistry was performed in brain sections from WT and D1R-/- mice following Rivera et al. (2002a
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Table 1. Combination of antisera used in each double-immunolabeling reaction
Results
Electrophysiological identification of striatal LA and FS interneurons in WT and mutant mice
In striatal slices prepared from WT, D1R-/-, D2R-/-, D2L-/-, and D2R-/-;D2L-/- mice, striatal LA and FS interneurons (at least 14 cells for each group of interneurons and each group of mice) were identified by morphological and electrophysiological criteria. LA interneurons were easily recognized in striatal slices for their large somata (25–55 µm diameter), whereas no morphological feature allowed us to distinguish the rare FS interneurons (1 of 60 recorded cells) from the more frequently encountered medium spiny projection cells. The identification of FS cells, therefore, was only electrophysiological, 3–5 min after rupture by suction of a tight G
LA cells had resting membrane potentials of approximately -60 mV, larger input resistances, lower thresholds for spike generation, and afterhyperpolarizations of longer duration and amplitude than the other classes of striatal cells. In addition, during hyperpolarizing current pulses, they showed a time-dependent decline of the electrotonic potential, which has been demonstrated to follow the activation of a hyperpolarization-activated cation current (Ih) (Jiang and North, 1991
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Figure 1. Electrophysiological responses of distinct neuronal subtypes of the striatum to the injection of depolarizing and hyperpolarizing current steps. Note that whereas medium spiny projection neurons (MS) exhibit tonic firing activity with little afterhyperpolarization during positive current pulses, LA and FS interneurons present distinct firing patterns and pronounced afterhyperpolarizations. The dotted line represents the resting membrane potential of the three neurons. See Results for further details.
Effects of DA receptor stimulation on the resting membrane potential of LA and FS interneurons of WT and D1R-/- mice
Recent electrophysiological evidence showed that stimulation of DA D1-like receptors depolarizes both LA (Aosaki et al., 1998
Bath application of DA (10–100 µM; 5–7 min; n = 7) produced a membrane depolarization in LA interneurons recorded from WT mice. This effect was reversible at the wash-out of the drug and was prevented by the DA D1-like receptor antagonist SCH 23390 (10 µM) (n = 4; p < 0.01) but not by the DA D2-like receptor antagonist L-sulpiride (3–10 µM)(n = 5; p > 0.05). The depolarizing effect of DA persisted unchanged in the presence of the sodium channel blocker TTX (1 µM), indicating that it was mediated by the activation of D1-like receptors located on the somatodendritic region of the recorded cells (n = 6; p < 0.001).
Essentially similar results were obtained when the effects of DA were measured on the membrane properties of FS interneurons of WT mice. DA (10–100 µM; 5–7 min bath application; n = 8), indeed, dose-dependently depolarized these cells. As with LA interneurons, 10 µM SCH 23390 blocked this effect (n = 3), whereas neither L-sulpiride (10 µM; n = 4) nor TTX (1 µM; n = 6) had any effect.
In D1R-/- mice, DA was still able to depolarize both LA (n = 6) and FS interneurons (n = 5). In both neuronal subtypes, the DA-dependent membrane depolarizations were comparable between the two genotypes. This suggests that D5 receptors are the main receptors involved in the excitatory effects of DA on these interneurons. Accordingly, also in D1R-/- mice, preincubation of the slices with the DA D1 and D5 receptor blocker SCH 23390 (10 µM) prevented the DA excitation in both neuronal subtypes (n = 4 for both LA and FS cells), whereas L-sulpiride (10 µM) was ineffective (n = 4 for LA cells and n = 3 for FS interneurons) (Fig. 2).
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Figure 2. Dopamine depolarizes LA and FS interneurons of both WT and D1R-/- mice. A, The graph shows the dose–response relationship for the depolarizing effect of DA on LA interneurons from WT and D1R-/- mice (in the control condition and in the presence of 10 µM SCH 23390). Electrophysiological traces from a single experiment show that bath application of 30 µM DA (black line), in the presence of 1 µM TTX, produces a reversible membrane depolarization in a D1R-/- LA interneuron (top trace). In the same cell, the depolarizing effect of DA is fully prevented by the DA D1-like receptor antagonist SCH 23390 (10 µM; bottom trace). B, The graph shows the dose–response relationship for the depolarizing effect of DA on FS interneurons from WT and D1R-/- mice (in the control condition and in the presence of 10 µM SCH 23390). Electrophysiological traces from a single experiment show that bath application of 30 µM DA (black line), in the presence of 1 µM TTX, produces a membrane depolarization in a D1R-/- FS interneuron (top trace). In the same neuron, the depolarizing effect of DA is fully prevented by the DA D1-like receptor antagonist SCH 23390 (10 µM; bottom trace). Resting membrane potentials are -58 mV in A and -78 mV in B.
Expression of D5 receptors in cholinergic and PV-containing striatal interneurons
In a previous study in the rat caudoputamen (Rivera et al., 2002b
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Figure 3. Confocal laser photomicrographs illustrating the colocalization of D5 receptors with choline acetyltransferase (ChAT) and parvalbumin (PV) in striatal interneurons of WT and DA D1R-/- mice. A, D, Striatal neurons expressing DA D5 receptors in WT (A) and in D1R-/- mice (D); B, E, striatal interneurons containing ChAT in WT (B) and in D1R-/- mice (E). C and F show paired images illustrating double-labeled cells with D5/ChAT in WT (C) and D1R-/- mice (F). Note in C and F that ChAT-positive neurons express D5 receptors in WT and D1R-/- mice. Open arrowheads in D–F indicate a cholinergic partial cell that also expresses D5 receptors. G, J, Striatal neurons expressing DA D5 receptors in WT (G) and in D1R-/- mice (J); H, K, PV-containing interneurons located in the striatum of WT (H) and D1R-/- mice (K). Paired images in I and L show double-labeled cells with D5/PV in WT (I) and D1R-/- mice (L). White arrows indicate single-labeled cells for D5 receptors, and arrowheads indicate double-labeled cells in the corresponding images. Note in I and L that PV-containing neurons also express D5 receptors in WT and in D1R-/- mice. Scale bars, 25 µm.
Most of the PV-positive neurons also expressed D5 receptors. As in a previous report in the rat (Rivera et al., 2002b
Immunoblot characterization of the D5 receptor antiserum
Affinity-purified anti-D5 receptor antiserum was characterized to study its specificity by Western blot analysis in tissue extracts from cortex, striatum, and hippocampus of mouse and rat brains. Figure 4A shows representative results obtained with murine tissue extracts. The bands observed consisted of a doublet and a single band migrating with a molecular mass of
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Figure 4. Western blot analysis of anti-D5 antiserum immunoreactivity in mouse brain tissue extracts. A, Immunoreactive bands obtained in tissue extracts of the mouse brain stained with an anti-D5 receptor antiserum (lanes 1–3) or with the antiserum previously preabsorbed with the D5-fusion protein (lanes 4–6). Note three bands with a molecular weight
Occasionally another immunoreactive band of a higher molecular weight (
Effects of DA D2-like receptor stimulation on GABAA-mediated synaptic inputs to WT and D2R-/- striatal interneurons
Stimulation of DA D2-like receptors depresses GABAA-mediated inhibitory synaptic inputs to both LA (Pisani et al., 2000To identify the receptor subtype mediating the effects of DA D2-like receptor stimulation on striatal interneuron inhibitory inputs, we tested the effects of the genetic ablation of D2 receptors on the quinpirole-mediated inhibition of striatal IPSCs recorded from both LA and FS cells. The DA D2-like receptor agonist quinpirole (1–30 µM; 5–7 min) failed to affect GABAergic IPSCs in both LA (n = 6; p > 0.05) and FS interneurons of D2R-/- mice (n = 5; p > 0.05), whereas it produced a significant and reversible inhibition of IPSC amplitude in both neuronal subtypes of WT mice (n = 5 and p < 0.001 for LA and FS cells) (Fig. 5). Furthermore, in WT interneurons, the depressant action of 10 µM quinpirole on IPSC amplitude was effectively antagonized by subsequent application of 10 µM L-sulpiride (n = 2 for LA cells and n = 3 for FS cells), confirming that it was mediated by the stimulation of D2Rs (data not shown).
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Figure 5. Stimulation of DA D2-like receptor inhibits GABAergic synaptic transmission in WT but not in D2R-/- mice. A, The graph shows the dose-dependent inhibition of GABAergic synaptic transmission by quinpirole in LA interneurons of WT but not D2R-/- mice. The traces from single experiments show the effect of 10 µM quinpirole on IPSCs recorded from LA neurons of WT and D2R-/- animals. B, The graph shows the dose-dependent inhibition of GABAergic synaptic transmission by quinpirole in FS interneurons from WT and D2R-/- mice. Similar to LA cells, FS interneurons from the D2R-/- group are not sensitive to quinpirole. The traces from single experiments show the effect of 10 µM quinpirole on IPSCs recorded from FS neurons of WT and D2R-/- animals.
Effects of quinpirole on GABAA-mediated IPSCs recorded from LA and FS interneurons of D2L-/- and D2R-/-;D2L-/- mice
Two isoforms of the D2 receptor are generated from the same gene by alternative splicing: D2L and D2S isoform. Interestingly, D2L and D2S receptors display differential affinities for inhibitory G-proteins (Guiramand et al., 1995In both LA (n = 5) and FS interneurons (n = 5) of D2L-/- mice, quinpirole (1–30 µM) caused a dose-dependent depression of IPSC amplitude, which was prevented by preincubation of the slices with L-sulpiride (10 µM; n = 3 for both neuronal subtypes) and was essentially identical to that observed in the WT counterparts (n = 4 for both LA and FS interneurons) (Fig. 6).
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Figure 6. Effects of D2 receptor stimulation in D2L-/- and D2R-/-;D2L-/- mice. A, The graph shows the inhibitory effect of different doses of quinpirole (1–30 µM) on the amplitude of GABAergic IPSCs recorded from LA interneurons of WT, D2L-/-, and D2R-/-; D2L-/- mice. Although WT and D2L knock-outs respond to quinpirole in a similar manner, D2R-/-;D2L-/- mice show a significant reduction of sensitivity to quinpirole (p < 0.05 at 10 and 30 µM compared with control amplitudes, and p < 0.01 at 3, 10, and 30 µM quinpirole compared with WT and D2L-/- neurons). B, The graph shows the inhibitory effect of different doses of quinpirole (1–30 µM) on the amplitude of GABAergic IPSCs recorded from FS interneurons of WT, D2L-/-, and D2R-/-;D2L-/- mice. FS interneurons from WT and D2L knock-outs respond to quinpirole in a manner similar to that LA cells, whereas those from D2R-/-;D2L-/- animals show a significant reduction of sensitivity to quinpirole (p < 0.05 at 10 and 30 µM compared with control amplitudes, and p < 0.01 at 3, 10, and 30 µM quinpirole compared with WT and D2L-/- neurons recorded in the presence of this agonist).
Increased expression of D2S receptors has been described in D2L-/- mice (Usiello et al., 2000
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Table 2. [3H]-spiperone binding in WT, D2L -/-, and D2R -/-;D2L -/- mice
In LA (n = 4) and FS interneurons (n = 4) of D2R-/-; D2L-/- mice, quinpirole was still able to depress GABA IPSCs (p < 0.05 for both LA and FS cells at 10 and 30 µM), although to lower levels (p < 0.01 at 3, 10, and 30 µM quinpirole compared with WT and D2L-/- neurons recorded in the presence in quinpirole) (Fig. 6).
Effects of quinpirole on spontaneous GABAA-mediated IPSCs in LA interneurons of WT, D2R-/-, D2L-/-, and D2R-/-; D2L-/- mice
To analyze further the action of quinpirole on GABAA transmission, its effect on the frequency and amplitude of spontaneous GABA-mediated IPSCs was examined. Spontaneous GABAergic IPSCs were recorded from LA interneurons by using cesium chloride-based patch pipettes. These pipettes significantly altered the action potential properties of the recorded neurons, thereby preventing the unequivocal identification of FS cells. At the holding potential of -60 mV and in the presence of 10 µM CNQX and 30 µM MK-801, bicuculline-sensitive (n = 5) IPSCs were detected as inward currents. As expected for a presynaptic effect, quinpirole (10 µM; 7–10 min application) caused in LA interneurons recorded from WT mice (n = 4) a significant (p < 0.01) reduction of the frequencies of IPSCs, without altering the amplitudes. This effect was abolished in D2R-/- mice (n = 5; p > 0.05), remained intact in D2L-/- mice (n = 4; p < 0.01), and was diminished in D2R-/-;D2L-/- LA cells [n = 6; p < 0.05 compared with pre-quinpirole levels and with spontaneous IPSCs (sIPSCs) recorded in WT and D2L-/- cells in the presence of quinpirole] (Figs. 7, 8).
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Figure 7. Effects of quinpirole on GABAergic sIPSCs recorded from LA interneurons of WT, D2R-/-, D2L-/-, and D2R-/-;D2L-/- mice. The graphs are single-cell plots from patch-clamp experiments. In a WT LA interneuron (A), 10 µM quinpirole reduces the frequency of sIPSCs (expressed as inter-event interval). The effect of quinpirole is absent in the D2R-/- LA neuron (B), although it is similar to WTs in the D2L-/- cell (C). In D2R-/-;D2L-/- LA interneurons (D), the effect of quinpirole is reduced.
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Figure 8. Effect of D2 receptor stimulation on sIPSC frequency and amplitude of WT and mutant LA interneurons. A, The histogram shows the average effect of 10 µM quinpirole on the frequency of GABAergic sIPSCs recorded from LA interneurons. Cells from WT, D2L-/-, and D2R-/-;D2L-/- mice are significantly affected by this drug (p < 0.01 for both WT and D2L-/- mice and p < 0.05 for D2R-/-;D2L-/- mice). The quinpirole-mediated synaptic inhibition observed in D2R-/-;D2L-/- neurons, however, was significantly less pronounced than the one observed in WT and D2L-/- mice (p < 0.05 compared with both WT and D2L-/- neurons). B, In the three genotypes, the reduction of sIPSC frequency is not paralleled by changes in their amplitude (p > 0.05), suggesting a presynaptic mechanism for this phenomenon.
Discussion
The results of the present study demonstrated that DA controls striatal interneuron excitability through postsynaptic D5 receptors and presynaptic D2 receptors located on GABAergic nerve terminals. In addition, these studies strongly point to an involvement of both isoforms of the D2 receptor in the presynaptic effects of DA on GABA transmission. Indeed, the inhibitory effect of D2 receptor stimulation on both evoked and spontaneous GABAA currents, lost in D2R-/- animals, is preserved in D2L-/- mice, which express an equal number of D2 binding sites as WT animals, although composed exclusively of the D2S isoform. However, the response of D2L-/- mice was less pronounced when the number of D2S sites was reduced by 50%, leading to a condition of D2S expression closer to that found in WT animals.D1 receptors are not necessary for the excitatory effects of DA on striatal interneurons
In D1R-/- as well as WT mice, DA was equally effective in depolarizing LA and FS cells of the striatum. The dose–response relationship of the DA effects in both genotypes was similar also at low concentrations, suggesting no participation of D1 receptors in this electrophysiological effect. Overexpression and over-functioning of D5 receptors in D1R-/- mice, however, might potentially explain the virtually coincident dose–response curve for the DA effects observed in WT and D1R-/- interneurons. Clearly, the use of the recently generated D5 receptor-lacking mice (Holmes et al., 2001The D1 receptor subtype in the striatum is much more abundant than the D5 receptor subtype. We now know that the pattern of expression of these two receptor subtypes in the striatum is complementary to a large extent. Although D1 receptors are strongly expressed in projection neurons (Surmeier et al., 1996
In the same direction, the presence of D1 receptors in FS PV-positive neurons in the striatum is still inconclusive. However, our double-label immunofluorescence data indicating the presence of D5 receptors in PV cells in D1R-/- mice provides strong evidence that the D5 receptor is the DA receptor subtype involved in the depolarizing action of DA in these striatal interneurons.
D2 receptors mediate the inhibitory action of DA on GABAergic inputs to striatal interneurons
GABA-mediated inputs to both LA and FS interneurons have an essentially identical sensitivity to DA D2 receptor stimulation. Genetic manipulation of D2 receptor expression leads to comparable changes of the sensitivity of both neuronal types. These results strongly suggest that LA and FS interneurons receive the same type of GABAergic afferents. Interestingly, GABAergic innervation of the striatum is almost totally intrinsic, originating from recurrent collaterals of projection neurons or from GABAergic interneurons (Wilson and Groves, 1980The origin of the GABAergic input to striatal interneurons, however, remains to be clarified. Dual recordings suggested that it does not come from projection neurons (Koos and Tepper, 1999
Concluding remarks
DA is a crucial regulator of striatal function. Loss of nigrostriatal DAergic projection, in fact, causes severe motor abnormalities in Parkinson's disease patients and in animal models of parkinsonism (Bergman et al., 1998In this study we identified components of the DA receptor family involved in DA regulation of striatal interneurons. This is an important step in understanding the physiology of the basal ganglia and in developing pharmacological compounds that are able to target selectively a specific neuronal function.
Footnotes
Received Dec. 16, 2002; revised Apr. 24, 2003; accepted Apr. 24, 2003.This work was supported by grants from Institut National de la Santé et de la Recherche Médicale, Centre National de la Recherche Scientifique, Hopitaux Universitaires de Strasbourg, and Mission Inteministérielle de Lutte contre la Drogue et la Toxicomanie (E.B.); from Spanish Ministerio de Ciencia y Tecnología SAF200-0122, Plan National Sobre Drogas and Fundación La Caixa, Spain (R.M.); and from Consiglio Nazionale delle Ricerche and Ministero della Salute, Progetto Finalizzato Schizofrenia (P.C.).
Correspondence should be addressed to one of the following: Paolo Calabresi, Clinica Neurologica, Dipartimento di Neuroscienze, Università di Roma "Tor Vergata," Via Montpellier 1, 00133 Rome, Italy, E-mail: paolo.calabresi{at}uniroma2.it; or Rosario Moratalla, Instituto Cajal, Consejo Superior de Investigaciones Científicas, Avenida Dr. Arce 37, 28002, Madrid, Spain, E-mail: moratalla{at}cajal.csic.es; or Emiliana Borrelli, Institut de Génétique et de Biologie Moléculaire et Cellulaire, Centre National de la Recherche Scientifique–Institut National de la Santé et de la Recherche Médicale–ULP1, Rue L. Fries, BP10142, 67404 Illkirch Cedex, C.U. de Strasbourg, France, E-mail: eb{at}titus.u-strasbg.fr.
Copyright © 2003 Society for Neuroscience 0270-6474/03/236245-10$15.00/0
* R.M., E.B., and P.C. contributed equally to this work.
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