Abstract
The principle neurons of the striatum are GABAergic medium spiny neurons (MSNs), whose collateral synapses onto neighboring neurons play critical roles in striatal function. MSNs can be divided by dopamine receptor expression into D1-class and D2-class MSNs, and alterations in D2 MSNs are associated with various pathological states. Despite overwhelming evidence for D2 receptors (D2Rs) in maintaining proper striatal function, it remains unclear how MSN collaterals are specifically altered by D2R activation. Here, we report that chronic D2R stimulation regulates MSN collaterals in vitro by presynaptic and postsynaptic mechanisms. We used corticostriatal cultures from mice in which MSN subtypes were distinguished by fluorophore expression. Quinpirole, an agonist for D2/3 receptors, was used to chronically activate D2Rs. Quinpirole increased the rate and strength of collateral formation onto D2R-containing MSNs as measured by dual whole-cell patch-clamp recordings. Additionally, these neurons were more sensitive to low concentrations of GABA and exhibited an increase in gephyrin puncta density, suggesting increased postsynaptic GABAA receptors. Last, quinpirole treatment increased presynaptic GABA release sites, as shown by increased frequency of sIPSCs and mIPSCs, correlating with increased VGAT (vesicular GABA transporter) puncta. Combined with the observation that there were no detectable differences in sensitivity to specific GABAA receptor modulators, we provide evidence that D2R activation powerfully transforms MSN collaterals via coordinated presynaptic and postsynaptic alterations. As the D2 class of MSNs is highly implicated in Parkinson's disease and other neurological disorders, our findings may contribute to understanding and treating the changes that occur in these pathological states.
Introduction
GABAergic medium spiny neurons (MSNs) mediate the integration of information within the striatum, ultimately controlling proper motor movement and behavior (Graybiel et al., 1994). Nearly 95% of all striatal neurons are GABAergic MSNs, which can be further divided by their differential dopamine (DA) receptor expression into D1 or D2 MSNs (Gerfen and Young, 1988; Bolam et al., 2000; Kreitzer and Malenka, 2008). As MSN axons branch extensively onto nearby neurons, MSNs have the capacity to tightly regulate striatal activity and output (Wilson, 1994; Plenz, 2003). Despite the overwhelming role for D2 receptors (D2Rs) in maintaining proper striatal function, it remains unclear how MSN collaterals are specifically altered by D2R activation.
The D2R is a G-protein-coupled receptor that is critical in maintaining proper function in the CNS (Girault and Greengard, 2004). Aberrant changes in D2R expression and function in the striatum are closely related to schizophrenia, substance abuse, and obesity (Abi-Dargham et al., 2000; Volkow et al., 2001; Asensio et al., 2010; Johnson and Kenny, 2010). The D2R is also the primary target of action for many antipsychotics (Seeman et al., 1975; Kapur et al., 2000) and for Parkinson's disease therapy (Lieberman and Goldstein, 1985). Interestingly, D2 MSNs of the striatum have been shown to be the first population of neurons affected by DA depletion in Parkinsonism, resulting in alterations of D2 MSN morphology and function (Albin et al., 1989; Day et al., 2006; Gittis and Kreitzer, 2012; Zold et al., 2012). In fact, recent evidence points to the specific reduction in D2 MSN collaterals of the striatum in a mouse model of Parkinson's disease (Taverna et al., 2008).
To investigate the role of D2R activation on GABAergic transmission, we developed a corticostriatal culture model using transgenic mice that express different fluorescent proteins to allow for simultaneous live identification of D1 and D2 MSNs [Gene Expression Nervous System Atlas project (GENSAT); Gong et al., 2003; Shuen et al., 2008]. An in vitro model allows for direct pharmacological control of DA receptor activation while maintaining neuronal integrity (Deyts et al., 2009). This provides the unique opportunity to specifically compare the effects of D2R activation on the two major subtypes of striatal neurons. In the current study, we present direct evidence for the regulation of synaptic frequency and efficacy at MSN collateral synapses by chronic D2R activation. Our data suggest that D2R activation causes distinctive changes in MSN morphology with coordinated increases in the number of synaptic sites and density of postsynaptic GABAA receptor clusters. Together, our results demonstrate that GABAergic transmission between MSNs is significantly regulated by D2R activation, and this occurs via coordinated presynaptic and postsynaptic modifications at specific MSN collaterals.
Materials and Methods
Corticostriatal cultures.
We adapted the procedure originally described in Segal et al. (2003). BAC drd1a-tdTomato mice and BAC drd2-EGFP (enhanced green fluorescent protein) mice harbor bacterial artificial chromosome (BAC) transgenes with td-Tomato reporter downstream of D1 receptor promoter and EGFP reporter downstream of the D2 receptor promoter, respectively (GENSAT; Gong et al., 2003; Shuen et al., 2008). Crossing these two strains resulted in healthy mice pups, a subset of which coexpressed tdTomato in D1 cells and EGFP in D2 cells. Primary cultures were prepared from the progeny of this cross. Pups of either sex were decapitated at postnatal day 0 in accordance with the guidelines of the American Veterinary Medical Association Panel on Euthanasia and the Georgetown University Animal Care and Use Committee. Whole brains were removed and placed into ice-cold Krebs solution with 0.3% BSA, and subsequently examined for fluorophore expression using Dual Fluorescent Protein Flashlight (Nightsea). Striata from brains expressing both tdTomato and EGFP were dissected using GFP expression as a guide (Fig. 1A). Cortical tissue from littermates that did not express either fluorophore was separately dissected. Tissue was enzymatically (trypsin, 0.03%; Sigma-Aldrich) and mechanically dissociated to yield a single-cell suspension. Cells were diluted and combined to achieve a 1:3 ratio of cortical to striatal neurons at a final concentration of 5 × 105 cells/ml. Then, 250 μl of the cell suspension was plated onto poly-d-lysine (10 μg/ml; Sigma-Aldrich)-coated glass coverslips (1.13 cm2). The coverslips had been previously incubated in Basal Eagle's medium (Invitrogen). Cells were cultured in Neurobasal medium supplemented 0.25% glutamine, 1% penicillin-streptomycin, 2% B27 (all from Invitrogen), 50 ng/ml BDNF (Alomone), and 30 ng/ml GDNF (Sigma-Aldrich; Gertler et al., 2008) and maintained at 37°C in 95% O2/5% CO2. At 2 d in vitro (DIV), one quarter of the medium was replaced with fresh Neurobasal medium with BDNF and GDNF as described above. Media was exchanged twice weekly, although BDNF and GDNF were not included after DIV 2 (Tian et al., 2010).
The drd2-EGFP line in our colony was backcrossed with a C57BL/6 line (Chan et al., 2012) to avoid the abnormalities reported in Kramer et al. (2011). The characteristics of MSNs in the presence and absence of treatments were also confirmed in cultures harvested from two separate mouse strains: drd2-cre;rosa26-tdTomato (Madisen et al., 2010) and npy-EGFP;drd1a-tdTomato (Shuen et al., 2008; Partridge et al., 2009). These mice were derived from FVB/B6/129/Swiss and C57BL/6- B6SJLF1 strains, respectively. As we did not detect any significant differences between strains, these data were excluded from the results section for consistency.
Treatments.
Neurons were pharmacologically stimulated between DIV 18 and 21. To activate DA D2 receptors, neurons were treated with the selective D2/3 receptor agonist (±)-quinpirole dihydrochloride (10 μm; Sigma-Aldrich) diluted in Neurobasal media (Deyts et al., 2009). To study nonspecific actions of quinpirole, we pretreated a subset of coverslips for 10 min with D2/3 receptor antagonist sulpiride (10 μm; Sigma-Aldrich). We then chronically treated the cells with 10 μm sulpiride plus 10 μm quinpirole for 72 h.
A smaller subset of coverslips was treated with a low dose of quinpirole (500 nm). Control neurons were given an equal volume of Neurobasal media without the addition of drug. All cells were returned to the incubator for 72 h before experimentation.
Electrophysiology.
Whole-cell voltage-clamp and current-clamp recordings were performed on striatal neurons identified by either tdTomato or EGFP fluorescence. Cells were visualized with a Nikon TE-2000S inverted microscope with a 40× phase-contrast objective. All recordings were done at room temperature (RT) in extracellular solution (ES) continuously perfused at a rate of 2.5 ml/min. ES was composed of the following (in mm, except for phenol red), all from Fisher Scientific: 145 NaCl, 5 KCl, 1 MgCl2, 1 CaCl2, 5 HEPES, 5 glucose, 15 sucrose, phenol red (0.25 mg/L), adjusted to pH 7.4 with NaOH. Recording electrodes were pulled on a two-step vertical pipette puller (PP-83, Narishige) from borosilicate glass capillaries (Wiretrol II, Drummond) with resistances of 3–5 MΩ. To characterize basic electrophysiological properties, electrodes were filled with intracellular solution containing the following (in mm): 145 K-gluconate, 10 HEPES, 5 ATP . Mg, 0.2 GTP . Na, and 0.5 EGTA, adjusted to pH 7.2 with KOH. The equilibrium potential (ECl−) for Cl− in this condition was −71.4 mV. To study inhibitory synaptic transmission, 100 mm K-gluconate plus 44 mm KCl was substituted for 145 mm K-gluconate. The ECl− for this solution was −29.6 mV, allowing GABAergic currents to be recorded as inward at −70 mV while preventing series resistance errors created by extremely large currents. The calculated liquid junction potentials for these conditions were 15.8 and 12.2 mV, respectively, and the values reported have been compensated accordingly. Whole-cell voltage-clamp recordings were performed with a Multiclamp 700B amplifier (Molecular Devices) and access resistance was monitored throughout the recordings. Currents were filtered at 1 kHz with an eight-pole low-pass Bessel filter and digitized at 5 kHz using an IBM-compatible microcomputer equipped with Digidata 1322A data acquisition board and pCLAMP10 software.
Stock solutions of bicuculline methobromide (BMR), tetrodotoxin (TTX), 2,3-dihydroxy-6-nitro-7-sulfamoyl-benzo[f]quinoxaline-2,3-dione (NBQX; all from Abcam), and 4,5,6,7-tetrahydroisoxazolo[5,4-c]pyridin-3-ol (THIP; Sigma-Aldrich) were prepared in water and diluted in ES to a final concentration of 25 μm, 500 nm, 5, and 1 μm, respectively. Stock solutions of etomidate, flumazenil, and diazepam (all from Sigma-Aldrich) were prepared in dimethyl sulfoxide (DMSO) and diluted in ES (final DMSO concentration <0.01%). GABA (Sigma-Aldrich) was dissolved in water and diluted in ES to the desired concentrations. Solutions were rapidly exchanged using the Y-tube method (Murase et al., 1989).
Synaptic connections were studied in paired recordings while both neurons were held in voltage-clamp configuration at −70 mV. Cells were alternately stimulated at 3 s intervals with a voltage step to induce an action potential (+100 mV, 4 ms). Neurons were considered coupled if the presynaptic action potential induced an evoked IPSC (eIPSC) in the postsynaptic cell (Fig. 2B). Preceding stimulation, a test voltage pulse (−5 mV, 20 ms) was given to monitor series and input resistance and experiments with unstable holding currents were discarded. For variance–mean (V–M) analyses, changes in extracellular Ca2+ ([Ca2+]o) were induced with the Y-tube application of four [Ca2+]o concentrations and resulting variances of eIPSC peaks were studied (Clements and Silver, 2000).
IPSC parameters were examined in Clampfit 10.2 (Molecular Devices). eIPSC averages were based on >20 events with failures removed. The decay phase of the averaged eIPSCs was fit to a double-exponential function and τw was calculated as the following: where τ1 and τ2 are the fast and slow decay time constants, respectively, and A1 and A2 are the contribution of the first and second exponentials to the amplitude (Nusser et al., 2001). Miniature (in TTX and NBQX) and spontaneous events were identified using semiautomated threshold-based software (Mini Analysis, Synaptosoft) and visually confirmed (Ade et al., 2008). More than 100 events were averaged per cell and decay kinetics were determined using a single-exponential equation.
Histochemistry.
Anatomical reconstruction was achieved by including 1% biocytin in the intracellular solution of a subset of neurons (Partridge et al., 2009). To preserve the cell body, the pipette was carefully removed after 5–8 min to form an outside-out patch. Coverslips containing recorded, filled neurons were placed in 4% paraformaldehyde/4% sucrose/PBS solution for 15 min at RT, rinsed 3 times in 1× PBS and subsequently permeabilized and stained with fluorescein-avidin dye (Vector Labs) at 2.5 μl/ml for 120 min. Coverslips were briefly washed in PBS and mounted on glass slides using VectaShield antifade solution (H-1000, Vector Labs).
To better study D2 MSN synapses, mature neurons were fixed and washed as described above. Next, coverslips were permeabilized and blocked, as in Tian et al. (2010), and incubated with antibodies to either rabbit α-GFP (1:200; Invitrogen) and mouse α-gephyrin (1:500; Synaptic Systems), or mouse α-GFP (1:500; Invitrogen) and rabbit α-VGAT (α vesicular GABA/glycine transporter; 1:1000; Abcam) for 2 h at RT. Appropriate secondary antibodies conjugated with Alexa-488 or Texas Red were diluted 1:1000. Coverslips were washed three times and mounted with VectaShield for visualization.
Microscopy and image analysis.
Images of fixed and stained neurons at DIV 21–24 were acquired using a Nikon FS1 upright microscope equipped with a two-channel confocal imaging module (CLS-2HS, Thorlabs). Single confocal images were taken and basic morphological properties and Sholl analyses were conducted in ImageJ software [National Institutes of Health (NIH)].
Biocytin-injected cells were traced with the ImageJ NeuronJ plugin and dendritic arborization was analyzed with Sholl analysis plugin. Three to five neurons were analyzed per condition in three separate cultures and results were plotted as the number of intersections per 10 μm concentric circle from the soma.
Puncta measures were quantified with a custom macro for NIH ImageJ software (courtesy of F. Vanevski). Analyses were performed on puncta that were associated with either GFP+ or non-GFP neurons. One representative 70–100 μm dendritic segment was chosen per cell starting at the base of the primary dendrite. At least 10 neurons from different coverslips and cultures were analyzed for each condition. Puncta density and fluorescence intensity of immunoreactive puncta were calculated by thresholding images at two times background. Means from each representative dendrite per neuron were averaged to obtain population means.
Statistics.
Kolmogorov–Smirnov tests were conducted on all datasets to check for normal distribution and appropriate statistics were chosen dependent upon these results. Statistical tests and graphical plots were performed in Prism 5 software (GraphPad) and are detailed in Results and figure legends. All data values in the text and figures are presented as mean ± SEM.
Results
Drd1a-tdTomato; drd2-EGFP corticostriatal cultures develop accurately in vitro
To perform a targeted study of D1 and D2 MSNs, we took advantage of drd1a-tdTomato; drd2-EGFP mice to further develop the model originally described by Segal et al. (2003) and extended by Tian et al. (2010). We cocultured striata that coexpressed EGFP and tdTomato with cortices from wild-type littermates; this avoided culturing cortical neurons that expressed fluorescently labeled D1 and/or D2 receptors. MSNs developed typical anatomical features in these culture conditions: by 2 weeks in vitro, neurons displayed extensive dendritic arborization and spiny protrusions (Fig. 1B). MSNs retained the expression of both fluorescent proteins in vitro, and mature neurons maintained a stable cell density of green, red, and nonfluorescent cells observed at densities of 43 ± 4, 49 ± 4, and 46 ± 6 cells/mm2, respectively (p > 0.05; Friedman test). Interestingly, 11% of neurons (17 ± 3 cells/mm2) coexpressed both fluorescent markers (p < 0.0001 compared with all other cell types; Friedman test). Neurons that expressed both fluorophores were not included in this study (data obtained in 79 fields from three culture preparations; DIV, >18).
To ensure that MSNs expressed characteristic electrophysiological properties, whole-cell patch-clamp recordings were performed from fluorescently identified D1 and D2 MSNs between DIV 21 and 24 using a potassium gluconate internal solution. Both MSN subtypes exhibited membrane properties reminiscent of those reported in brain slices (Dehorter et al., 2011), including action potential firing patterns, inward rectifying potassium currents, and the delay to first action potential suggestive of A-type potassium channel expression (Fig. 1C, Table 1). We also observed spontaneous membrane potential fluctuations that led to bursts of action potentials, likely due to up and down states as previously reported in organotypic slices (Plenz and Kitai, 1998) and dissociated cultures (Randall et al., 2011; Fig. 1D). Up and down states, paired with the occurrence of spines, suggest the successful innervation of MSNs by excitatory cortical neurons (Segal et al., 2003; Tian et al., 2010). The characteristics of MSNs observed in cultures from drd1a-tdTomato; drd2-EGFP remained consistent across three additional mouse strains and genotypes (drd2-EGFP, drd2-cre;rosa26-tdTomato, and npy-EGFP;drd1a-tdTomato; data not shown).
Paired recordings from MSN subtypes reveal reciprocal synaptic connectivity
Recurrent axon collaterals provide the striatal network with the capacity to integrate and store complex signals (Churchill and Sejnowski, 1992; Plenz, 2003). Thus, we investigated the occurrence of synaptic coupling between MSNs in our culture model. Concurrent whole-cell recordings were established from identified MSN pairs within the same visual field (Fig. 2A). As MSN synapses are GABAergic, pipettes were filled with an enhanced [Cl−]i intracellular solution to achieve an ECl− at −30 mV (see Materials and Methods) to allow eIPSCs to be detected as inward. Cells were recorded in voltage-clamp at −70 mV and action potentials were artificially elicited in each cell to determine the presence of synaptic coupling. As seen in the example recording in Figure 2B, eIPSCs could be studied in this configuration. In addition to synaptic currents, we discovered the frequent occurrence of what appeared to be autaptic currents immediately following stimulation (Fig. 2B). Though autaptic currents were often detected in both recorded MSNs, this issue was not extensively pursued. Upon local perfusion with the GABAA receptor antagonist BMR (25 μm), both synaptic and autaptic currents were eliminated, demonstrating that activity from MSN collaterals in this preparation were indeed mediated by GABAA receptors (Fig. 2B, blue trace). eIPSCs were also blocked by perfusion with 0.5 μm TTX, and were unaffected by 5 μm NBQX (data not shown). Figure 2C shows a schematic of the potential synaptic arrangement between MSNs, revealing that a maximum of four synapses can be simultaneously studied in this configuration.
To determine whether eIPSCs were a result of direct monosynaptic or indirect polysynaptic connections, we examined eIPSC latency to peak and failure rate. MSNs consistently displayed rapid and homogenous latency to peak (4.3 ± 0.2 ms), and low rates of failures (8.9 ± 2%), suggesting that eIPSCs were a result of direct monosynaptic connections (n = 50 cells from six culture preparations). Although we occasionally observed clear evidence of multipeaked, long-lasting eIPSCs suggestive of polysynaptic activity, we found this in <5% of the MSN pairs examined and these neurons were excluded from the study. A summary of the relative occurrence of the synaptic and autaptic currents detected between the two MSN subtypes is shown in Figure 2D,E (open bars).
Chronic D2R activation increases coupling onto D2 MSNs
It has been shown that MSN collaterals are negatively regulated by DA depletion (Taverna et al., 2008), but it remains unknown to which DA receptor these changes can be attributed. To investigate whether D2R activation affects GABAergic coupling between MSN subtypes, we examined neurons in an environment where DA levels could be tightly regulated. As corticostriatal cultures are devoid of dopaminergic input, we treated mature cultures with the D2R-class agonist quinpirole (10 μm) for 72 h. Pilot experiments determined this treatment regimen as optimal. Cultures treated with the D1-class receptor agonist SKF (1 μm) and quinpirole (1 μm) at DIV 2 showed no difference in connectivity between D2 MSNs at DIV 14 (n = 10 per condition, p = 0.606; χ2 test). Although cultures treated with quinpirole (10 μm) at DIV 10 exhibited increased connectivity between D2 MSNs by DIV 13 (n = 8 per condition, p = 0.021; χ2 test), cultures >18 DIV were used for experimentation to avoid confounds that could be attributable to development in vitro. To address potential nonspecific effects of 10 μm quinpirole, we conducted additional paired recordings from coverslips cotreated with 10 μm quinpirole and 10 μm D2R selective antagonist sulpiride. In this condition, D2 MSNs were detected as coupled in 40% of 58 synaptic pairs, from two culture preparations (p = 0.025 when compared with nontreated D2 MSN pairs; χ2 test). Coverslips treated in parallel with 500 nm quinpirole exhibited 75% coupling in 28 pairs (p = 0.156 when compared with nontreated D2 MSN pairs; χ2 test).
We first examined whether chronic D2R activation with 10 μm quinpirole altered the rate of functional synapse formation between MSN pairs. We observed that postsynaptic D2 MSNs were more likely to receive coupling in the treated condition, regardless of presynaptic partner (Fig. 2D). Interestingly, the rate of autapse formation also increased with quinpirole treatment, again in exclusively D2 MSNs (Fig. 2E). In support of this observed increase in connectivity, the likelihood in which two D2 neurons were reciprocally coupled was also significantly increased: while reciprocal connections were found in 26 of 67 (39%) cells analyzed in nontreated conditions, reciprocal connections increased to 60 of 97 (62%) analyzed cells after chronic D2R activation (p = 0.004; χ2 test).
We compared the size and kinetics of eIPSCs between the two conditions to study changes in synapse strength following quinpirole treatment. Charge transfer and time to decay (τw) increased in treated D2 MSNs, regardless of presynaptic partner (Fig. 3A,B). Similar results were seen for peak amplitude in D2 MSNs (−89 ± 22, n = 35 cells to −191 ± 25, n = 54 cells, p = 0.0002; Mann–Whitney test) but not D1 MSNs (−74 ± 20, n = 32 cells to −96 ± 24, n = 31 cells, p = 0.213; Mann–Whitney test). These results correlated with a decrease in failure rate (Fig. 3B), as well as a decrease in coefficient of variation for postsynaptic D2 MSNs (0.50 ± 0.05, n = 45 cells to 0.34 ± 0.02, n = 55 cells, p = 0.007; Mann–Whitney test) but not D1 MSNs (0.42 ± 0.04%, n = 30 cells to 0.39 ± 0.02, n = 27 cells, p = 0.867; Mann–Whitney test). Together, paired recordings from identified MSNs suggest that activation of the D2R increases the rate of collateral formation onto D2 MSNs and these collaterals form larger, longer, and more reliable eIPSCs when compared with nontreated controls.
D2R activation influences D2 MSN morphology and synapse formation
It has been previously reported that the presence of DA alters D2 MSN morphology (Gertler et al., 2008, Day et al., 2008). We therefore examined whether quinpirole treatment altered D2 MSN morphology in a subset of MSNs (n = 11–12/condition from three cultures). Biocytin injections allowed for morphological reconstruction and subsequent analysis of the dendritic arbor (Fig. 4A,B). A plot of dendritic complexity (Fig. 4C) illustrates slight but significant increases in dendritic arborization with the treatment. Analysis of phase-contrast images confirms an increase in primary dendrite number (Fig. 4D) and reports a reduction in soma diameter (Fig. 4E) in treated D2 MSNs while D1 MSNs remain unchanged (n > 50/condition).
As increased dendritic arborization may improve the likelihood of synapse formation, we studied possible alterations in presynaptic terminals using α-VGAT antibody, which is a marker for vesicular GABA transporter. D2 MSNs showed an increase in VGAT puncta density after D2R activation specifically in GFP-labeled dendrites (Fig. 5A,B). A correlated increase in the frequency of spontaneous (Fig. 5C,E) and miniature (Fig. 5D,E) IPSC events was also observed. D1 MSNs displayed no change in mIPSC frequency (2.3 ± 1.5, n = 8 cells to 2.15 ± 0.5, n = 8 cells, p = 0.869; unpaired t test). As no change in peak amplitude of mIPSCs was noted in D2 MSNs between treatments, the smaller average sIPSC peak and increased mIPSC frequency are possibly the result of a preferential increase in small events in the treated condition (Fig. 5F). τw was not significantly affected by D2R activation (Fig. 5G). It is important to keep in mind that mIPSCs and sIPSCs need not originate exclusively from MSNs; striatal or cortical interneurons could contribute as well. Quantal content, determined by dividing the average amplitude of eIPSCs by the average mIPSC per cell, was also significantly affected in D2 MSNs (6.9 ± 1.8, n = 14 cells to 16.4 ± 2.7, n = 32 cells, p = 0.030; unpaired t test) but not in D1 MSNs (8.2 ± 1.6, n = 10 cells to 7.4 ± 5.1, n = 5 cells, p = 0.853; unpaired t test). The increase in quantal content and the decrease in failure rate of treated D2 MSN eIPSCs further supports a potential increase in either the number of release sites or the release probability following quinpirole treatment.
To evaluate these two possibilities, we used a V–M analysis of eIPSC amplitudes as described by Clements and Silver (2000). The relationship between amplitude variation and amplitude mean with changes in external calcium concentrations ([Ca2+]o) can be plotted to determine quantal size (Q), number of release sites (N), and the average probability of vesicular transmitter release (Pr). As expected, changing [Ca2+]o from 0 to 0.5 mm and then to 1 mm led to increases in eIPSC amplitude variance and amplitude mean in D2 neurons from both treated and nontreated conditions. When [Ca2+]o was increased to 2 mm [Ca2+]o, nontreated D2 MSNs again displayed an increase in eIPSC amplitude variance and amplitude mean (Fig. 6A). D2 MSNs in the treated condition, on the other hand, exhibited an increase in eIPSC amplitude mean but a reduction of amplitude variance (Fig. 6B). As illustrated in Figure 6C, the V–M plot of D2 MSNs in the nontreated condition was relatively linear, indicating increased variance at higher [Ca2+]o concentrations. On the other hand, the V–M plot of treated D2 MSNs formed a distinct parabola (Fig. 6D). These data support the hypothesis that D2R activation via quinpirole increases the number of GABA release sites (N) or vesicular GABA release probability (Pr). However, the lack of parabolic mean–variance relationship in the nontreated condition prevents us from truly distinguishing between these two possibilities.
As the effects of the treatment on eIPSCs were observed only when the postsynaptic target was a D2 MSN, we hypothesize that D2R activation preferentially affects postsynaptic D2 MSNs, independent of the presynaptic partner. The increased frequency of sIPSC and mIPSC events in quinpirole-treated D2 MSNs, along with the reduction in failures of eIPSCs, suggests an increase in the number of MSN collaterals and a potential increase in clusters of postsynaptic GABAA receptors.
Chronic D2R activation increases GABA sensitivity of D2 MSNs
We therefore examined postsynaptic GABAA receptor clusters with an α-gephyrin antibody. Gephyrin is a synaptic anchoring protein that colocalizes with postsynaptic GABAA and glycine receptors (Sassoè-Pognetto et al., 2000). Immunohistochemical analysis of gephyrin clusters in D2 MSN dendrites revealed a significant increase of gephyrin puncta density after quinpirole treatment in exclusively D2 MSN dendrites (Fig. 7A,B), supporting a postsynaptic increase of GABAA receptors with chronic D2R activation.
To directly assess changes in GABAA receptor expression, we investigated the action of several GABA concentrations (0.3, 1, 3, and 10 μm) on whole-cell currents in D1 and D2 MSNs. In the nontreated condition, D1 and D2 MSNs exhibited similar sensitivity to all concentrations of GABA. With chronic quinpirole treatment, however, D2 MSNs displayed a higher sensitivity at 0.3 and 1 μm GABA (Fig. 7C–E). Similarly, at 3 μm GABA, currents were 94 ± 33 pA, n = 12, and 250 ± 65 pA, n = 11, in nontreated and treated D2 MSNs, respectively (p = 0.032; Mann–Whitney test). At 10 μm, currents were 201 ± 39 pA, n = 23, and 313 ± 46 pA, n = 29, in nontreated and treated D2 MSNs, respectively (p = 0.074; Mann–Whitney test). The larger currents in response to GABA in treated D2 MSNs point strongly to a postsynaptic mechanism for DA, but whether this is due to an increase in GABAA receptor number, as suggested by increased gephyrin clusters, or a change in GABAA receptor subtype required further elucidation.
Different GABAA receptor subunits influence receptor conductance, open probability, and ligand affinity (Macdonald and Olsen, 1994). The δ subunit-containing extrasynaptic GABAA receptor has been shown to be more sensitive to GABA (Farrant and Nusser, 2005). As D2 MSNs displayed increased GABA sensitivity with the quinpirole treatment, we hypothesized that this may be a result of increased expression of the δ subunit-containing GABAA receptor. THIP, a preferring agonist for δ subunit-containing GABAA receptor, was locally perfused while MSNs were in whole-cell configuration. Response to 1 μm THIP did not significantly change with the quinpirole treatment in either MSN subtype (Fig. 7C,D). Interestingly, D2 MSNs exhibited larger currents in response to THIP compared with D1 MSNs, suggesting a greater expression of extrasynaptic GABAA receptors in D2 MSNs basally in vitro (Fig. 7E). Synaptic GABAA receptors in the striatum contain the β3 subunit (Janssen et al., 2011). Etomidate has been shown to consistently modulate the β2/3 subunit-containing GABAA receptor and was therefore used to assess any potential changes in synaptic GABAA receptors. As with THIP, there were no detectable differences in peak current responses to etomidate within MSN subtype when compared between conditions (Fig. 7C,D).
These experiments suggest that the increased sensitivity to GABA observed in quinpirole-treated D2 MSNs is not related to changes in β2/3 or δ subunit expression. Thus, together, the increase in mIPSC frequency and GABA sensitivity point to an increase in number of postsynaptic GABAA receptors with treatment. As we did not observe a correlated increase in mIPSC amplitude, the data point to an increase in the number of inhibitory synaptic sites with chronic D2R stimulation. Although we cannot exclude a preferential increase in other GABAA receptor subtypes, or postsynaptic modifications of existing receptors, the most plausible explanation is an increase in the density of GABAA receptor clusters with quinpirole treatment.
Pharmacology of inhibitory synaptic connections between MSNs
To further investigate changes in GABAA receptor subtypes, we used benzodiazepine pharmacology. Benzodiazepine sensitivity relies on the presence of specific α and γ2 subunits to increase frequency of opening of the targeted GABAA receptor subtypes (Macdonald and Olsen, 1994). If the targeted subunit is present, an enhancement of IPSC decay time (τw) is expected.
Flumazenil, a potentiator of α4, β3, and γ2 subunit-containing GABAA receptors (Ramerstorfer et al., 2010), failed to prolong IPSC decay in either condition, excluding a role for the α4 subunit (data not shown). Diazepam acts as a positive allosteric modulator at the benzodiazepine site of α1–3-containing or α5-containing GABAA receptors. Local perfusion of 5 μm diazepam revealed a prolongation of eIPSCs in both nontreated and treated D2 MSNs, indicating that D2 MSNs in both conditions express these subunits (in nontreated D2 MSNs, τw increased from 38 ± 3 to 48 ± 3 ms, n = 5, p = 0.025, paired t test; in treated D2 MSNs, τw increased from 56 ± 5 to 79 ± 3 ms, n = 8, p = 0.035, paired t test). Interestingly, the increase in τw of eIPSCs from baseline was larger in quinpirole-treated (41%) versus nontreated (23%) D2 MSNs (p < 0.0001; unpaired t test). Amplitude of eIPSCs was not affected by the presence of the benzodiazepine (data not shown).
To investigate whether quinpirole treatment induced a greater expression of benzodiazepine-sensitive GABAA receptors over other GABAA receptor subtypes, we studied the effect of diazepam on mIPSCs. As an mIPSC reflects the response to a single quantum of neurotransmitter, if benzodiazepine-induced prolongation of mIPSC τw was enhanced following quinpirole, this would suggest increased relative expression of diazepam-sensitive GABAA receptors. We observed that diazepam significantly prolonged mIPSC decay: in nontreated D2 MSNs, τw increased from 25 ± 2 to 33 ± 1 ms, n = 12 (p < 0.0001; paired t test); in treated D2 MSNs, τw increased from 27 ± 3 to 39 ± 3 ms, n = 8 (p < 0.0001; paired t test). However, unlike eIPSCs, the diazepam-induced change in mIPSC τw did not differ between conditions (32% nontreated and 44% quinpirole-treated, p = 0.08; unpaired t test). The possibility that mIPSCs and eIPSCs may be derived from different presynaptic terminals should be considered. However, the slower decay of eIPSCs compared with mIPSCs suggests they reflect asynchronous summation of multiple synaptic currents produced at distinct sites (Mody et al., 1994). Thus, the enhanced effect of diazepam on eIPSCs compared with mIPSCs in treated D2 MSNs may be due to increased number of synaptic connections on D2 MSNs with chronic quinpirole treatment.
Discussion
Collateral inhibition between MSNs allows for proper integration of information within the striatum (Czubayko and Plenz, 2002; Tunstall et al., 2002; Koos et al., 2004; Gustafson et al., 2006; Tecuapetla et al., 2007). Using paired patch-clamp recordings from identified MSNs in vitro, our results provide evidence for three novel conclusions. First, D2R activation with chronic quinpirole treatment increases the frequency and strength of synapse formation in postsynaptic D2 MSNs. These functional synapses are stronger and more reliable, and they exhibit substantially prolonged decay time. Second, quinpirole-treated D2 MSNs display increased dendritic complexity, a morphological change that may enhance the likelihood of synapse formation. Third, an increased GABA sensitivity without obvious changes in GABAA receptor subtype suggests an increase in postsynaptic GABAA receptor number with this treatment. Together, our data indicate that chronic D2R activation results in a greater synaptic efficacy via a coordinated increase of synaptic GABAA receptor clusters and GABA release sites.
MSN collaterals in vitro
An in vitro model that allows for simultaneous identification of both MSN subtypes is useful for the targeted investigation of the role of D2Rs in striatal networks. We report that corticostriatal cultures from drd1a-tdTomato; drd2-EGFP mice retain their fluorescent properties through time in vitro. Neurons in these cocultures have profiles comparable to MSN development observed in vivo, including action potential firing patterns, up-and-down states, developed dendritic morphology, and spine formation. MSNs in our primary culture concurrently display properties that are not typically seen ex vivo, such as autaptic currents and colocalization of D2 and D1 MSNs markers. The absence of natural targets for MSNs in culture may explain the high rate of autapse formation, as is exemplified with in vitro microislands (Bekkers, 2005). The considerable extent of neurons that coexpress both D1 and D2 markers in primary culture may be a consequence of harvesting MSNs at an early developmental stage (Goffin et al., 2010).
Studies of striatal MSNs in primary culture or organotypic slice models (Plenz and Aertsen, 1996; Segal et al., 2003; Gertler et al., 2008; Tian et al., 2010; Kaufman et al., 2012) offer advantages and disadvantages compared with acute slice preparations. Primary cultures enable manipulation of the extracellular environment and consequently allow close comparisons between experimental conditions. In addition, in vitro models are useful to distinguish cell-autonomous contributing factors from environmental contributing factors (Gertler et al., 2008). These benefits come with inherent limitations: dissociated culture models disrupt the natural development of cytoarchitecture, potentially altering cellular and network phenotypes. However, while in vitro culture models report enhanced rates of functional connectivity, ex vivo slice preparations unavoidably reduce the estimated extent of coupling due to slice thickness and depth of neurons (Chuhma et al., 2011). Therefore, in vitro preparations are useful for dissecting out changes in MSN collaterals.
Lack of DA in vivo has been found not to affect the development of MSNs or proper neural circuits in a DA-deficient mouse model (Zhou and Palmiter, 1995). As our primary cultures do not contain dopaminergic cells of the substantia nigra pars compacta but should nevertheless permit normal MSN and circuit development, our cocultures provide us the unique opportunity to study how D2R activation alters synaptic function. The use of transgenic mice that allow for live identification of two populations of neurons provides us an additional, straightforward internal control.
D2R activation increases collateral frequency and strength
The rate of functional synaptic connectivity in our coculture model was consistently higher in D2–D2 MSN pairs than any other configuration. Despite the difference in frequency of functional synapses in basal conditions, eIPSC size and kinetics remained consistent between MSN pairs. Chronic D2R activation with 72 h of 10 μm quinpirole treatment, however, increased both the rate and size of eIPSCs specifically in D1–D2 and D2–D2 pairs, suggestive of a postsynaptic mechanism of D2R activation. This increase was not seen in pairs that had been treated with a combination of quinpirole and D2/3 antagonist sulpiride, demonstrating that 10 μm quinpirole is effectively targeting D2 MSNs.
Sholl analyses revealed that chronic D2R activation increased both the number of primary dendrites and the dendritic arborization of D2 MSNs. While this correlates with the increased number of functional synapses onto treated D2 MSNs, it has recently been reported that chronic D2R upregulation in vivo in the mouse increases MSN excitability and decreases dendritic arborization by the downregulation of inward rectifying potassium channels (Cazorla et al., 2012). There are several reasons underlying the divergence of our study from these results. It is likely that there are distinct intracellular pathways and compensatory mechanisms activated by D2R upregulation compared with chronic D2R activation. In addition, there are inherent differences in the in vivo versus in vitro the experimental settings. In fact, the number of primary dendrites of MSNs in dissociated cultures (4–6) is consistent with what has been previously reported, and is lower than what has been observed in slices (6–8; Gertler et al., 2008). Day et al. (2006) provide evidence that DA depletion reduces primary dendrite number selectively in D2 MSNs from six to four. In combination with the reported reduction in primary dendrites of corticostriatal cultures, which inherently lack DA input (Gertler et al., 2008), these two studies further support the idea that DA activation of D2Rs regulates D2 MSN morphology.
Coordinated presynaptic and postsynaptic mechanisms
Consistent with an increase in functional synapses onto D2 MSNs, we observed an increase in presynaptic GABA sites and postsynaptic gephyrin clusters along D2 MSN dendrites with quinpirole treatment. These results parallel the enhanced sensitivity to low concentrations of GABA in treated D2 MSNs. However, the possibility of differential GABAA receptor subtype expression should also be considered.
The pharmacological dissection of native GABAA receptor subtypes is challenging because of the specificity of available modulators and heterogeneity of endogenous subunit expression. Based on reported expression studies by Pirker et al. (2000), striatal GABAA receptors should be predominantly composed of α2, β1/3, and γ2 subunits. α1, α4, α5, And δ subunits have been also shown to be expressed. Previous studies in our group have suggested that the presence of specific DA receptors in MSNs affect synaptic and extrasynaptic GABAA receptor function (Ade et al., 2008, Janssen et al., 2009), with a key role for β3 subunits (Janssen et al., 2011). The present results, however, show that the sensitivity to etomidate, a β2/3 subunit-containing agonist, does not change with chronic D2R activation. Furthermore, currents in response to THIP, a superagonist of the extrasynaptic δ subunit-containing receptor (Brown et al., 2002), are unaltered by the treatment, suggesting the increase in GABA sensitivity is specific for synaptic receptors.
Our data show that diazepam prolongs the synaptic decay of GABA IPSCs in both nontreated and treated MSNs, but the actions on τw were enhanced in quinpirole-treated D2 MSNs. This effect was observed to a greater degree on eIPSCs and not on mIPSCs; therefore, we conclude that this is a result of increased asynchronous summation of synaptic release from multiple sites. The possibility that mIPSCs and eIPSCs represented distinct inputs should be kept in mind when interpreting these results. It remains to be determined whether the increase in synaptic sites in treated D2 MSNs is due to a morphological change in dendritic branching (Day et al., 2006), or whether it is due to a facilitation of GABAA receptor insertion at newly formed inhibitory synapses. The changes in dendritic morphology (Fig. 4) and the increased sensitivity of treated D2 MSNs to low doses of GABA that parallels increases in gephyrin clusters (Fig. 7) support the hypothesis of a coordinated dopaminergic control of GABAA receptor clusters and dendritic morphology in D2 MSNs. The effect of quinpirole treatment is selective for postsynaptic D2 MSNs and independent from the presynaptic cell being D1 or D2 MSN. This supports the hypothesis that D2R activation in postsynaptic D2 MSNs has its effect through one of the multiple intracellular cascades that regulates GABAA receptor trafficking (Vithlani et al., 2011) and dendritic morphology (Day et al., 2008).
The role of D2R is central in neuropsychiatric disorders. Our results begin to elucidate the powerful action of biochemical cascades following activation of these receptors in contributing to synapse formation and functionality (Girault and Greengard, 2004). We provide a model for future studies that may define the relative role of distinct components of this cascade, and compare the role of D1 receptor activation. One must consider when comparing results of DA receptor stimulation that, while DA is released in a context-dependent manner in vivo, selective agonists are always present in culture. Prolonged agonist application may alter receptor signaling paradigms, potentially producing different effects compared with discontinuous stimulation.
Previous studies have shown that DA regulates the efficacy of MSN collaterals (Taverna et al., 2008). Our results extend these findings and provide an experimental assay to mechanistically analyze this effect. Together, our data suggest that DA D2 receptor activation facilitates inhibitory synapse formation via coordinated presynaptic and postsynaptic changes.
Footnotes
This work was supported by the National Institutes of Health (MH64797). We thank Filip Vanevski for sharing the ImageJ macros for puncta quantification.
The authors declare no competing financial interests.
- Correspondence should be addressed to Rupa R. Lalchandani, Graduate Program in Physiology and Biophysics, Georgetown University School of Medicine, Basic Science Building Room 228, 3900 Reservoir Road NW, Washington, DC 20007. rrl23{at}georgetown.edu