The Switch of Subthalamic Neurons From an Irregular to a Bursting Pattern Does Not Solely Depend on Their GABAergic Inputs in the Anesthetic-Free Rat

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The Journal of Neuroscience, October 1, 2002, 22(19):8665-8675

The Switch of Subthalamic Neurons From an Irregular to a Bursting Pattern Does Not Solely Depend on Their GABAergic Inputs in the Anesthetic-Free Rat
Nadia Urbain¹, Nicolas Rentéro¹, Damien Gervasoni², Bernard Renaud¹, and Guy Chouvet¹
¹ Laboratoire de Neuropharmacologie et Neurochimie, Institut National de la Santé et de la Recherche Médicale U512, Université Claude-Bernard-Lyon 1, 69373 Lyon, France, and ² Department of Neurobiology, Duke University Medical Center, Durham, North Carolina 27710

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The subthalamic nucleus (STN) powerfully controls basal ganglia outputs and has been implicated in movement disorders observedin Parkinson's disease because of its pathological mixed burstfiring mode and hyperactivity. A recent study suggested that reciprocallyconnected glutamatergic STN and GABAergic globus pallidus (GP)neurons act in vitro as a generator of bursting activity in basalganglia. In vivo, we reported that GP neurons increased theirfiring rate in wakefulness (W) compared with slow-wave sleep (SWS)without any change in their random pattern. In contrast, STN neuronsexhibited similar firing rates in W and SWS, with an irregularpattern in W and a bursty one in SWS. Thus, the pallidal GABAergictone might control the STN pattern. This hypothesis was testedby mimicking such variations with microiontophoresis of GABA receptorligands. GABA agonists specifically decreased the STN firing ratebut did not affect its firing pattern. GABA_A (but not GABA_B) antagonistsstrongly enhanced the STN mean discharge rate during all vigilancestates up to three to five times its basal activity. However,such applications did not change the typical W random pattern.When applied during SWS, GABA_A antagonists strongly reinforcedthe spontaneous bursty pattern into a particularly marked onewith instantaneous frequencies reaching 500-600 Hz. SWS-W transitionsoccurring during ongoing antagonist iontophoresis invariably disruptedthe bursty pattern into a random one. Thus GABA_A receptors playa critical, but not exclusive, role in regulating the excitatorySTN influence on basal gangliaoutputs.

Key words: subthalamic nucleus; GABA; bicuculline; gabazine; extracellular single-unit recordings; firing pattern; bursts of spikes; nonanesthetized animal; sleep-wake cycle; microiontophoresis

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The subthalamic nucleus (STN) plays a critical role in the control of movement by virtue of its glutamatergic projectionsto the basal ganglia output nuclei, which in turn innervate thethalamus and subcortical premotor areas (Albin et al., 1989; DeLong,1990). Indeed, previous studies have demonstrated that a largeproportion of STN neurons discharge high-frequency bursts relatedto movements (DeLong et al., 1985; Matsumura et al., 1992; Wichmannet al., 1994a; Cheruel et al., 1996). Furthermore, abnormal activityof the STN has been shown to be implicated in the parkinsonianmotor symptoms (Bergman et al., 1990; DeLong, 1990; Wichmann etal., 1994b) and in the generation of involuntary hemiballisticmovements (Hammond et al., 1979; Crossman et al., 1980, 1984;Beurrier et al., 1997). Several lines of evidence support an elevateddischarge rate and a preponderant bursty pattern of STN neuronsin experimental models of Parkinson's disease (PD; Bergman etal., 1994, 1998; Benazzouz et al., 1996; Hassani et al., 1996;Périer et al., 2000; Vila et al., 2000). Moreover, some STN cellsexhibit a rhythmic activity strictly correlated with tremor inlimbs of parkinsonian patients, suggesting that STN might be implicatedin the PD tremor (Rodriguez et al., 1998; Levy et al., 2000; Magariñoz-Asconeet al., 2000).

Although much progress has been made in understanding the intrinsic properties of STN neurons, the fact that in vitro theseneurons fire spontaneously with a tonic discharge of single spikesonly (Nakanishi et al., 1987; Overton and Greenfield, 1995; Bevanand Wilson, 1999; Bevan et al., 2002) (but see also Beurrier etal., 1999), whereas in vivo they exhibit a more or less regularor bursty pattern in anesthetized preparations (Hollerman andGrace, 1992; Ryan et al., 1992; Hassani et al., 1996; Kreiss etal., 1997; Magill et al., 2000), suggests that STN afferents playa crucial role in the modulation of its firingpattern.

Plenz and Kitai (1999), using a simplified culture system in vitro, proposed that reciprocally connected glutamatergic STNand GABAergic globus pallidus (GP) neurons form an oscillatingfeedback system that might act as the central tremor generatorin PD. By contrast, in vivo we have shown recently that STN neuronalactivity could spontaneously shift from a more or less regulardischarge in wakefulness (W) to a bursty pattern in slow-wavesleep (SWS) but without related changes in the GP firing pattern(Urbain et al., 2000). Nevertheless, the GP mean firing rate waslower in SWS than in W. Changes in the GP rate might thus resultin changes in the STN pattern, as suggested previously by lesionsthought to mimic increased or decreased levels of the GABAergicGP tone on STN neurons (Ryan et al., 1992). According to thishypothesis, we have tested, across the sleep-wake cycle, whetherit was possible to regularize bursty STN neurons by microiontophoresisof GABA agonists (to mimic an increased W-GP tone), or inverselyto induce bursts on more or less regular neurons by GABA antagonists(to mimic a decreased SWS-GPtone).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fixation of the head-restraining system. Male Sprague Dawley rats (280-320 gm; IFFA Credo, Arbresle, France) were anesthetizedwith chloral hydrate (400 mg/kg, i.p., supplemented with 120 mg· kg¹ · hr¹, i.p., via a perfusion pump) and positioned conventionally (i.e.,with ear and nose bars) in a stereotaxic apparatus (Unimécanique,Epinay-sur-Seine, France). Body temperature was monitored andmaintained at 37-38°C with an electric heating pad. The skullwas exposed and carefully cleaned with citric acid (5%, w/v).Three stainless steel screws were implanted over the parietalareas of the skull, and three steel flexible wires inserted intothe neck muscles for standard monitoring of the electroencephalogram(EEG) and electromyogram (EMG), respectively. The bone was thencovered with a thin layer of acrylic cement (Superbond; Sun MedicalCo., Moriyama, Shiga, Japan), except the region overlying theSTN and the bregma suture (stereotaxic reference point). A U-shapedpiece of aluminum, fixed to a flexible carriage (GFG Co., Pierre-Bénite,Rhône, France) fastened to the stereotaxic apparatus was positionedabove the STN. This U-shaped piece was then embedded in dentalcement with the EEG screws and EMG wires and their six-pin connector,leaving a well inside the U-shaped piece that was closed withbone wax, as described previously (Darracq et al., 1996; Gervasoniet al., 1998, 2000; Soulière et al., 2000). This U-shaped piecelater allowed painless head restraint of the rat. The animal wasthen removed from the stereotaxic apparatus and allowed to recoverfrom surgery and anesthesia for 48 hr before the habituation sessionsbegan. The U-shaped piece (~5 gm) was well tolerated by the rats,which were able to move, sleep, feed, and drink normally in theirhome cage. All experiments were performed with the approval ofthe Regional Animal Care Committee (Université Claude Bernard-Lyon1) and the French Ministry of Agriculture (legal authorizationnumber 03-505), in accordance with the appropriate European CommunitiesCouncil directive (86/609/EEC), and complied with rules set forthin the National Institutes of Health Guide for the Care and Useof Laboratory Animals (publication 80-23). All animals were housedin standard conditions (21 ± 1°C, food and water ad libitum),and all experiments were performed during the light part of thecycle (12 hr light/darkcycle).

Habituation of rats to the head-restraining frame. During 8-10 successive days, repetitive trials of increasing duration wereperformed to train the rats to stay in the restraining frame.Their heads were painlessly secured to the stereotaxic frame byscrewing the U-shaped piece, cemented to the rat's head, withits associated carriage; their bodies were lying comfortably ina hammock. At the end of the training period, they could staycalm for periods of 5-6 hr during which quiet W, SWS, and short-lastingparadoxical sleep (PS) episodes were typically observed, attestingthat the restraint was well tolerated, as described previously(Gervasoni et al., 1998, 2000; Soulière et al., 2000; Urbainet al., 2000).

Single-unit and polygraphic recordings. After the 8-10 d of habituation and before the first single-unit recording session,rats were anesthetized with chloral hydrate (320 mg/kg, i.p.,additional doses as needed, i.p.), and a 4 mm trephine hole wasdrilled over the STN. The dura matter was then removed, and thewell was closed as described above. After 1 d of recovery, dailyrecording sessions were typically performed over a maximum of7-10 d, each session lasting ~4-6 hr. The brain surface was cleanedunder local lidocaine anesthesia at the beginning of each dailyrecordingsession.

Extracellular recordings of STN neurons were performed using single-barrel glass micropipettes (external tip diameter, 2-3µm) filled with 2% pontamine sky blue in sodium acetate (0.5 M,pH 7.5). Electrode impedances measured at 10 Hz ranged between7 and 15 M $Omega$ . Filtered (AC, 0.3-10 kHz) and unfiltered (DC) electrodesignals were amplified (P16; Grass Instruments) and fed to storageoscilloscopes (5110 and 5111; Tektronix, Beverton, OR), a thermalarraycorder (WR7600; Graphtek, Tokyo, Japan), and an audio monitor.Single-unit activity (signal-to-noise ratio of at least 3:1) wasisolated with an amplitude spike discriminator (Centre d'Electroniqueet Microinformatique Institut National de la Santé et de la RechercheMedicale, Lyon, France) and collected on a personal computer viaa Cambridge Electronic Design (Cambridge, UK) interface usingthe Spike 2 software, in parallel with analog-to-digital samplingsof amplified (P55; Grass Instruments) polygraphic signals (EEGand EMG; sample rate, 100 or 200 Hz). STN neurons were identifiedon-line by their stereotaxic location relative to bregma (Paxinosand Watson, 1996), i.e., anteroposterior, $-$ 3.6 to $-$ 4.3 mm; lateral,2.0-3.0 mm; and ventral, 7.5-8.3 mm, as well as by their previouslydescribed extracellular biphasic spike waveform and their spontaneousactivity dependent on the vigilance states. We have shown previouslythat STN neurons typically shift from a random discharge in Wto a rhythmic bursty pattern in SWS without any change in theirmean firing rate. In contrast, PS episodes were characterizedby marked increases in the STN firing rate (Urbain et al., 2000).

Micropharmacology. To combine STN single-unit recordings with microiontophoresis, a seven-barrel micropipette (12-15 µm tipdiameter) was glued alongside a recording electrode, as describedpreviously (Akaoka et al., 1992). Four different barrels werefilled with one of the following solutions: GABA (400 mM, pH 4),bicuculline methiodide (GABA_A receptor antagonist, 25 mM, pH 4),gabazine (GABA_A antagonist, 5 mM, pH 4), baclofen (GABA_B agonist,50 mM, pH 4), and phaclofen (GABA_B antagonist, 50 mM, pH 4). Alldrugs were purchased from Sigma (L'Isle d'Abeau Chesnes, France),except gabazine (SR-95531; a gift from Sanofi Research, Montpellier,France), and were dissolved in distilled water. The remainingbarrels, filled with 145 mM NaCl, were used for automatic currentbalancing and current tests (Stone, 1985). To prevent drug diffusion,retaining currents (5-10 nA) were applied between periods of ejection.Analog signals proportional to the magnitudes of iontophoreticcurrents were collected on the computer via the Cambridge ElectronicDesign interface, in parallel to the single-unit and polygraphicrecordingssamplings.

Iontophoretic studies were typically conducted as follows. When a presumed STN unit was found, computer data collection wasstarted, and a period of ~5 min of spontaneous discharge was sampledbefore any drug application. When they had to be tested againsttheir respective antagonists, short-duration iontophoretic pulsesof GABA agonists were applied in a cyclic manner to induce regularand reproducible STN responses. Ejecting currents were chosenin such a way to induce a clear decrease in firing rate. Besides,prolonged low current GABA applications were invariably associatedwith a trend toward the total inhibition, leading to a nonstationaryfiring that avoided any correct quantitative analysis with thePoisson surprise method. Prolonged applications of GABA receptorantagonists led typically to a stable plateau of neuronal dischargeallowing further quantitative pattern analyses. Iontophoreticcurrents were adapted to each individual cell, and high currentswere generally avoided to limit the diffusional effect of thedrug and to allow the recovery to the baseline activity. However,in several neurons, antagonist currents were progressively increased(up to 500 nA) to examine STN responses to higher amounts ofdrugs.

Histological verification of recording sites. On the fourth, third, and second days preceding the last recording session,iontophoretic deposits of pontamine sky blue (50% duty, 20 seccycle for 30 min, $-$ 30 µA) were made 1500, 1000, and 500 µm, respectively,above the STN to avoid possible electrolytic lesions of STN areafor further recordings. On the last day of the experiment, theelectrode was left in place at the final recording site, and aclassical deposit of pontamine sky blue was performed ( $-$ 20 µAfor 10 min). Then the animal was given a lethal dose of pentobarbital,and its brain was removed and immediately frozen in cold isopentane( $-$ 20°C). Subsequent histological location of the four marked sitesand electrode track reconstruction were made on 25-µm-thick cresylviolet-stained frontalsections.

Data analysis. The three classical vigilance states described in the rat were discriminated on the basis of the cortical EEGand neck EMG. W was identified by a low-amplitude and desynchronizedEEG with sustained EMG activity. SWS was clearly distinguishedby high-voltage delta waves (0.5-5 Hz) and spindles associatedwith weak EMG activity, the animal being immobile and its eyesclosed. PS was characterized by a desynchronized EEG with a pronouncedtheta rhythm (5.5-8.5 Hz) and a complete loss of nuchal muscletone. Basal and drug-induced firing rates and patterns were comparedfor periods matching for the same vigilance state using polygraphiccriteria and EEG spectral analysis. Power spectra of the correspondingEEGs were calculated using the fast Fourier transform of the Spike2software.

Discharge rates of STN neurons were analyzed off-line for each vigilance state by the Spike 2 analysis software. Basal dischargerates of individual cells were typically determined for at leastthree separate 10 sec epochs in a given vigilance state out ofany drug ejection or recovery period. Drug-induced effects werecomputed during plateau periods induced by iontophoretic pulses.The latency of a drug-induced effect was defined as the intervalbetween the onset of iontophoretic application of a drug and afiring rate deviation of at least 25% from baseline activity.Likewise, the recovery was the interval between the offset ofthe iontophoretic ejection and a stationary firing within 25%of thebaseline.

For a given vigilance state, comparisons of basal and drug-induced firing rates of the same cells were performed using Student'st tests for paired data. Comparisons of absolute firing ratescomputed in each vigilance state were performed using ANOVA withthe vigilance state as a factor. Percent variations of drug-inducedfiring rates relative to baseline activity were compared withthe nonparametric Wilcoxon signed ranks test for paired data,i.e., neurons recorded during at least two vigilance states, orwith the nonparametric Kruskal-Wallis test for nonpaired data,e.g., comparisons between three vigilancestates.

Discharge pattern of STN neurons, in correspondence with vigilance states, iontophoretic drug applications, or both, wereanalyzed off-line with a burst detection method that uses thePoisson surprise concept (Legendy and Salcman, 1985). Althoughthe term "burst" is widely used, there has been no strict definitiongiven: bursts are commonly viewed as a period in a spike trainthat has a much higher discharge rate than surrounding periodsin the spike train (Kaneoke and Vitek, 1996), and no general methodof detection has been developed. Given the marked disparity betweenSWS spontaneous bursts (more or less discernible individually)and particularly clear-cut bursts under GABA_A antagonists application,the surprise method appeared well adapted to our data. Howeversome changes in the "surprise script" for the Cambridge ElectronicDesign Spike 2 software were required to detect with reasonableperformance both types of bursts with the same algorithm to makeappropriate statistical comparisons between treatments. We addedto the original script a moving 10 sec windowing of raw data andsettled the burst termination when 6 consecutive spikes failedto improve the calculated surprise or as soon as an interval twicethe mean interspike interval was encountered (Legendy and Salcman,1985). This greatly improved burst detection in our STN recordings.Figure 1 illustrates the overall satisfactory performance of thishome-modified version of the original algorithm, both for spontaneousand drug-induced bursts. This algorithm provided, over a givenperiod and for each neuron analyzed, the number of bursts, themean number of spikes per burst, the mean burst duration, themean interval between the beginnings of each burst (i.e., theperiodicity of bursts, in seconds), and the mean frequency withinbursts.

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Figure 1. Burst detection method applied on a typical STN neuron recording during SWS, in the control condition (A) and under a microiontophoretic application of a GABA_A antagonist (bicuculline; B). This automatic detection was performed by a home-modified version of the surprise script provided by Cambridge Electronic Design in the Spike 2 software library (see Materials and Methods). Detected bursts from the corresponding single-unit activity are illustrated by square pulses on the top. As illustrated, such detection was reasonably satisfactory when applied both on a more or less bursty period recorded in spontaneous SWS (A) and on a particularly identified bursty one during SWS under bicuculline (B), without any downgrading of its overall performance.

For all statistical analyses of firing rates and discharge patterns, the significance level was set at p < 0.05. All dataare expressed as mean ±SEM.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

One hundred seven neurons showing discharge properties characteristic of STN neurons were recorded during different vigilancestates in 14 rats. In this database, 97 were recorded both inSWS and W, 32 through an SWS to PS or a PS to SWS transition,and 30 during a PS to W transition. These cells were identifiedas presumed STN neurons on the basis of the short (~1 msec duration)and biphasic waveform of their extracellular spikes as well asthe particular spontaneous activity across the sleep-wake cyclethat we described recently (Urbain et al., 2000); they shiftedinvariably from a random discharge in W to a rhythmic bursty patternin SWS without any significant change in their mean firing rate(W, 14.7 ± 0.9 spikes/sec; n = 100; vs SWS, 16.9 ± 1.0 spikes/sec;n = 102). In addition, 33 of these neurons were also recordedduring a PS episode, during which they doubled their mean firingrate (35.5 ± 2.7 spikes/sec) relative to SWS and W (p < 0.001;ANOVA). The location in the STN of all these neurons was supportedby subsequent histologicalverifications.

Given the fact that, on this anesthetic-free preparation, animals exhibited spontaneous alternating of the three vigilancestates without forewarning the experimenter, and whatever theiontophoretic protocol used, it was not always possible to sampleboth the baseline and the drug-induced firing of a neuron duringthe same vigilance state. Consequently, only paired data obtainedduring a given vigilance state on a given cell, both in controlconditions and during drug applications, have been consideredbelow for appropriate statisticalanalyses.

Response of STN neurons to GABA agonists

Iontophoretic applications of GABA were performed on 34 STN neurons during W, SWS, or PS. As illustrated in Figure 2, ejectionsof GABA (68 ± 7 nA for 8 ± 1 s) led to a fast (typically 1-3 srange) and marked dose-dependent decrease of the STN firing ratewhatever the vigilance state (W, $-$ 68.2 ± 4.5%; p < 0.001;n = 20; SWS, $-$ 75.5 ± 3.1%; p < 0.001; n = 28; PS, $-$ 66.8 ± 11.8%;p < 0.01; n = 8). Recovery to baseline activity took only a fewseconds. This depression of the firing rate under GABA was notstatistically different among the three vigilance states (p =0.48; ANOVA). In all tested cells, these GABA-induced inhibitionswere antagonized by co-iontophoresis of the GABA_A antagonistsbicuculline (61 ± 9 nA; n = 10) (Fig. 2A) and gabazine (107 ±25 nA; n = 3) (Fig. 2B). Occasionally, we observed transient increasesin the firing rate during W, which were time-locked with briskmovements of the animal despite the potent iontophoretic GABA-inducedinhibitions on which they were superimposed.

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Figure 2. Typical inhibitions of STN neurons induced by iontophoretic applications of GABA along the spontaneous alternance of SWS and W and their blockade by the co-iontophoretic ejection of the GABA_A antagonists bicuculline (A) and gabazine (B). In each panel, below the polygraphic recordings (EMG and EEG), the horizontal black lines indicate ejection pulses for each compound with corresponding iontophoretic currents. The bottom part relates to the corresponding single-unit activity.

To examine the effect of GABA on the STN firing pattern, we also used moderate and prolonged GABA applications that inducedonly slight inhibitions (to be sure that GABA was going out ofthe pipette), although trends toward total inhibitions were obtainedwith sufficient amounts of GABA. As illustrated in Figure 3, STNneurons, that exhibited a bursty pattern in SWS, kept this burstypattern during clear GABA-induced inhibitions. Likewise, if appliedin W, when STN neurons showed a random discharge, GABA did notalter this pattern. Furthermore, a rebound burst-like patternwas never observed after the end of GABA applications.

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Figure 3. Illustration of the inability of iontophoretic GABA applications to clearly alter the spontaneous occurrence of a bursty pattern in STN neurons during a SWS episode. A, Below the EMG and EEG raw traces, the firing pattern of an STN neuron is summarized on a large time scale by plotting the mean instantaneous frequency (in hertz, mean of the inverse of intervals between events, computed at each event over a 0.5 sec period) versus time. Large variations of this index are indeed more indicative of marked nonstationary conditions (e.g., during bursting activity) than the classical discharge rate histogram (event counts over 2 sec periods, expressed in spikes per second) displayed immediately below. Although this GABA application induces a progressive decrease in the mean firing rate up to 50%, it is ineffective to dampen the variability in instantaneous frequencies. Note also that some transient increases in instantaneous frequencies were rather attributable to spontaneous microawakenings (see EMG trace). B, Single-unit activity on an expanded time scale; the length of the recording corresponds to the width of the boxed area in A. Note the persisting bursty pattern of this STN neuron as its mean firing rate starts to decrease.

Effects of iontophoretic applications of the specific GABA_B receptor agonist baclofen were examined on 28 neurons. Baclofen(113 ± 6 nA for 10 ± 1 s) typically induced a progressive andlong-lasting decrease of the STN firing rate (Fig. 4; W, $-$ 61.5± 6.6%; p < 0,001; n = 19; SWS, $-$ 63.5 ± 5.2%; p < 0.001; n = 18;PS, $-$ 21.5 ± 18.8%; p = 0.27; n = 5). This response started a fewseconds after the beginning of baclofen applications (7 ± 1 s;n = 28). However, in contrast with GABA-induced inhibition, itdeveloped slowly, and the recovery time was relatively longer(36 ± 10 sec; n = 23). In addition, only a few total inhibitionswere obtained (5 of 23). As observed with GABA, the firing patternof STN neurons across the sleep-wake cycle was not qualitativelyaltered by baclofen applications; i.e., STN neurons exhibiteda bursty pattern in SWS and a more or less regular one in W. Inall tested neurons (n = 16), co-iontophoresis of the GABA_B antagonistphaclofen antagonized the baclofen-induced inhibitions (Fig. 4)but not the GABA_A-induced ones.

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Figure 4. Example of baclofen-induced inhibitions and their blockade by co-iontophoresis of the GABA_B antagonist phaclofen. This STN neuron was recorded during an SWS period interrupted by short periods of W (microarousals indicated by stars). In each panel, below the polygraphic recordings (EMG, EEG), the horizontal black lines indicate ejection pulses for each compound with corresponding iontophoretic currents. The bottom part relates to the rate histogram (spike counts with a 2 sec bin width) and the corresponding single-unit activity of this STN neuron.

Response of STN neurons to GABA antagonists

Whatever the vigilance state, iontophoretic applications of the GABA_A antagonists bicuculline (61 ± 9 nA for 125 ± 43 sec;n = 36) on gabazine (107 ± 25 nA for 114 ± 47 sec; n = 9) induceda progressive and sustained increase of the firing rate of allneurons recorded in the STN. The latency of this effect was ~9sec, and firing rate was almost doubled across the first minuteof bicuculline or gabazine ejection (Fig. 5A). If applicationwas stopped, the recovery to baseline took typically several tensof seconds; otherwise, the neuronal mean firing rate increasedprogressively to a plateau whose level depended on the recordedcell and the current applied.

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Figure 5. Switch in the firing pattern of STN neurons during SWS-W transitions under iontophoretic applications of GABA_A antagonists. A, Mean instantaneous frequency (in hertz, computed at each event in 0.5 sec) versus time of an STN neuron before, during, and after the iontophoretic ejection of bicuculline (black horizontal bar) together with the corresponding polygraphic recordings (EMG, EEG, top). Note the progressive increase in frequency leading to a well established SWS bursty pattern ~30 sec after the onset of bicuculline application. Note also its dramatic decrease associated with the spontaneous appearance of a short W episode, as well as the progressive reappearance of a bursty pattern during the consecutive transient drowsiness period, which fully comes back during reinstallation of typical SWS. The total recovery to baseline activity in SWS took ~3 min after the offset of bicuculline application. B, Raw traces of polygraphic recordings and single-unit activity during the SWS-W transition of the STN neuron shown in A but with an expanded time scale corresponding to the shaded area in A. Superimposed deflections on the EMG trace correspond to the electrocardiogram of this animal, which can sometimes be recorded during particularly low muscular tone SWS episodes. The frequency spectra (relative power in the 0-15 Hz band, computed over 10 sec before and after the change in vigilance state indicated by a star) of the corresponding EEGs are shown on the right. They typically illustrate the high-voltage slow waves in the delta range (0.5-5 Hz) observed in SWS and the low-amplitude and desynchronized EEG in W. On the single-unit trace, spikes were unfortunately truncated in their negative part because of the settings of the Graphtek thermal printer. Note in particular that bicuculline-induced marked bursts in SWS suddenly vanished when the rat spontaneously woke up. Note also the increased discharge activity associated with brisk movements in quiet W (see EMG trace). C, Same representation as in B of another STN neuron during an SWS-W transition occurring during the ongoing iontophoresis of another GABA_A antagonist, gabazine.

In addition, we evaluated maximal firing abilities of STN neurons. On five STN neurons, particularly high currents (up to500 nA and 100 sec) of bicuculline were progressively appliedto follow the STN neuron response to the highest doses. Althoughthe mean firing rate of three of these five cells was slightlyincreased by such high currents, the mean firing rate of the twoother cells was not further enhanced. Likewise, the firing patternas well as the modifications of the discharge rate related tovigilance states were not further affected by high doses of bicucullinecompared with the lower ones; i.e., STN neurons shifted typicallyfrom a bursty pattern in SWS to a more regular one in W (see below).Moreover, no sign of depolarization blockade was observed at thehighest currents tested. Because increases of the firing rateinduced by high currents of bicuculline were similar to thoseinduced by lower ones, all data were pooled for this particularevaluation. Overall, STN activity was significantly enhanced bybicuculline application up to three to five times its basal activity,and maximal STN mean firing rates (computed as the highest meanfiring rate in 20 sec periods) were quite similar between thethree vigilance states (p = 0.45; ANOVA; W, 92.2 ± 12.5 spikes/sec;range, 31.8-184.3; SWS, 103.0 ± 10.6 spikes/sec; range, 26.8-184.1;PS, 124.1 ± 20.1 spikes/sec; range, 59.0-177.8).

Furthermore, dramatic alterations of the firing pattern were related to changes in the firing rate. When GABA_A antagonistapplications began during SWS episodes, a particularly robustbursty pattern developed in the majority of STN cells (Fig. 5B).Salient bursts started to occur several tens of seconds afterthe beginning of bicuculline (28 ± 4 sec; n = 18) or gabazine(25 ± 6 sec; n = 5) applications. Burst analysis of the correspondingsubsets of SWS-paired data for bicuculline and gabazine is summarizedin Table 1. In contrast, when antagonist applications began duringW episodes, such strong bursts only rarely occurred, but as soonas the rat fell asleep, they typically started to develop.


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Table 1. Quantitative parameters of the SWS burst-firing mode

During SWS, bicuculline or gabazine increased the frequency of occurrence of bursts and their duration, as well as the numberof spikes per bursts (Table 1). Such bursts were markedly differentfrom the spontaneous ones observed during SWS. This derived mainlyfrom the sustained high frequencies of spikes noticeable withineach burst (Fig. 6), thus delineating clearly isolated bursts.With both antagonists, almost all bursts started with few consecutivespikes speeding up to reach a brief episode of instantaneous frequenciestypically as high as 500-600 Hz, followed by a long series ofspikes slowing down toward the end of each burst (Fig. 7). Suchhigh mean or instantaneous frequencies within bursts were onlyrarely observed within control bursts appearing spontaneouslyduring SWS episodes (Table 1, Fig. 6), which were also neverso sustained for a long time.

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Figure 6. Histograms of the mean frequencies within all bursts of 2 groups of STN neurons (n = 17, top; n = 6, bottom) recorded both in control SWS (left column; 526 and 369 bursts, respectively) and during iontophoresis of the GABA_A antagonists in SWS (right column; bicuculline, SWS + BIC, 1767 bursts; gabazine, SWS + GBZ, 1359 bursts). Note that, for both groups, mean frequencies within bursts were distributed at ~100 Hz in typical SWS, whereas they were significantly increased during the same vigilance state to ~300 Hz by both GABA_A antagonists. Note also the shoulder on the right of the SWS + BIC histogram reflecting the somewhat higher frequencies within bicuculline-induced bursts compared with the gabazine-induced ones.

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Figure 7. Representation of the instantaneous frequencies computed for each consecutive interval making up typical bursts of STN neurons. Bursts were automatically detected by the Poisson surprise method during SWS episodes in a control condition (SWS) and under iontophoretic application of bicuculline (SWS + BIC) or gabazine (SWS + GBZ). Plot resolution does not permit discrimination of particularly timely close spikes.

This property of GABA_A antagonists to induce such a robust bursty pattern almost exclusively during SWS was largely confirmedon STN neurons recorded during both an ongoing antagonist applicationand a spontaneous SWS-W transition (n = 17) or an SWS-PS one (n= 5). Strikingly, these marked SWS bursts typically disappearedwhen rats woke up (Fig. 5) or were strongly modified during PSepisodes (Fig. 8). As illustrated in Figure 5B, although bicucullinewas still applied with the same iontophoretic parameters, theawakenings of the rat were typically associated with an immediateregularization of the bursty pattern. In addition, this shiftin the STN discharge was associated with a significant decreaseof the enhanced mean firing rate under bicuculline (from +277.0± 51.2% in SWS to +161.0 ± 49.7% in W; Wilcoxon test between SWSand W, p < 0.05). The same was observed for gabazine (Fig. 5C).In contrast, when spontaneous SWS-PS transitions occurred underbicuculline, the STN neuron firing rate was nonsignificantly affected(SWS, 113.2 ± 18.5 spikes/sec; vs PS, 134.8 ± 14.4 spikes/sec).Actually, strong PS bursts, similar to those observed in SWS,were still recorded during bicuculline or gabazine applications,but whereas they were isolated bursts occurring on a silent backgroundin SWS (Fig. 8, SWS), numerous single spikes randomly appearedbetween more or less clear bursts in PS (Fig. 8, PS).

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Figure 8. Illustration of changes in the STN neuronal discharge between SWS and PS episodes under ongoing iontophoresis of bicuculline (A) or gabazine (B). Raw traces of polygraphic recordings (EEG, EMG) and single-unit activity of two STN neurons are represented together with the Fourier spectra (relative power in the 0-15 Hz band) of the corresponding EEGs on the right. These periodograms typically illustrate the high-voltage slow waves in the delta range during SWS and the power highly concentrated in the theta band (5.5-8.5 Hz) during PS. A, The clear-cut bicuculline-induced bursts recorded on this STN neuron during SWS were replaced by a mixed pattern during a spontaneous PS episode. Single spike random activity was superimposed on strong bursts. The expanded time scale (250 msec) was chosen to permit the visual appreciation of single random spikes between bursts during PS. B, Same observations for another STN neuron recorded under ongoing gabazine iontophoresis during SWS and PS. Note that for B, the time scale (1 sec) is different from the one in A to illustrate the sustained high-frequency firing that can be observed within PS episodes.

In contrast to the GABA_A receptor antagonists, the specific GABA_B receptor antagonist phaclofen did not have marked or consistenteffects on the STN discharge activity. Iontophoretic applicationsof phaclofen (185 ± 7 nA for 157 ± 55 sec) during W and SWS wereperformed on 10 STN neurons. Neither the STN mean firing patternnor the firing rate was significantly altered by phaclofen applicationsduring W or SWS (W, +13.9 ± 17.2%; n = 7; SWS, +5.3 ± 12.0%; n= 9).

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To our knowledge, the present work is the first to describe the effects of iontophoretic applications of GABA agonists andantagonists on STN neurons in the rat free of any interferencewith anesthetic or immobilizing drugs. In agreement with studiesthat have described GABA_A and GABA_B receptors in the STN (Zhanget al., 1991; Wisden et al., 1992; Charara et al., 2000; Schwarzeret al., 2001), iontophoretic applications of GABA or the GABA_Bagonist baclofen decreased the STN firing rate, effects blockedby the selective antagonists bicuculline (or gabazine) and phaclofen,respectively. Bicuculline or gabazine alone altered STN activitywhatever the vigilance state, contrary to the GABA_B receptor antagonistphaclofen, which had no effect. This suggests that STN cells areunder a tonic GABAergic tone across the entire sleep-wake cycle,predominantly mediated via GABA_A receptors. We found also thatapplications of GABA_A antagonists promoted a robust bursty patternselectively during SWS, pointing out the critical but not exclusiverole of GABA in STN firing patternregulation.

The STN receives mainly GABAergic afferents from the GP (Albin et al., 1989; DeLong, 1990). The GP projection is massive (Vander Kooy and Kolb, 1985; Moriizumi and Hattori, 1992), distributedto the whole extent of the STN (Kitai and Kita, 1987; Canteraset al., 1990; Smith et al., 1990), and there is evidence thatGP cells may inhibit STN neurons (Rouzaire-Dubois et al., 1980;Kita et al., 1983; Smith et al., 1990). It is known that mostGP neurons are GABAergic (Smith et al., 1990; Kita, 1994; Bellet al., 1995). Moreover, the synaptic organization of the GP terminalsin STN suggests that the GP exerts a powerful GABAergic controlover the STN (Van der Kooy et al., 1981; Smith et al., 1990; Bevanet al., 1997).

Consequently, and as expected, we found that local GABAergic agonists were potent inhibitors of STN neurons and that GABA_Aantagonists easily induced their disinhibition, as described previouslyin the anesthetized rat (Rouzaire-Dubois et al., 1980; Fégeret al., 1991). At first glance, the GABA_A antagonist-induced burstypattern that we selectively observed in SWS does agree with ourprevious data (Urbain et al., 2000), according to which STN spontaneousbursts developing when the rat fell asleep were associated witha reduction in the GABAergic GP tone. It also agrees with theSTN rebound burst firing observed in vitro after removal of hyperpolarization(Nakanishi et al., 1987; Overton and Greenfield, 1995; Beurrieret al., 1999; Bevan et al., 2000), although we never observedsuch a phenomenon after the offset of GABA applications. The lackof effect of GABA to affect the STN random pattern in W may seemat variance with the tonic-bursting switch in discharge inducedby hyperpolarization in vitro (Beurrier et al., 1999), but wecannot exclude a preponderant membrane shunting effect by iontophoreticGABA_A receptor activation (Baufreton et al., 2001).

One of the most striking results of the present study is that GABA_A antagonists selectively reinforced the spontaneous SWSbursty pattern, leading to well delineated long bursts with intraburstinstantaneous frequencies as high as 500-600 Hz, only rarely observedin baseline conditions. Such bursts are likely related to GABA_Areceptor blockade, because they were evoked by both the GABA_Aantagonists bicuculline and gabazine (SR-95531; Heaulme et al.,1986; Michaud et al., 1986; Mienville and Vicini, 1987; Hamannet al., 1988; Yu and Ho, 1990; Rognan et al., 1992; Mestdagh andWulfert, 1999). The additional bicuculline-induced blockade ofcalcium-activated potassium currents (Johnson and Seutin, 1997;Seutin et al., 1997; Debarbieux et al., 1998; Khawaled et al.,1999; Mestdagh and Wulfert, 1999) or inhibition of acetylcholinesteraseactivity (Svenneby and Roberts, 1973; Miller and McLennan, 1974)might explain the somewhat longer burst duration evoked by thiscompound compared with gabazine (Table 1).

It must also be emphasized that this typical SWS bursty pattern emerged several tens of seconds after the onset of antagonistapplications. This delay might be linked to the requirement ofthe blockade of postsynaptic GABA_A receptors localized on distaldendrites. However, we cannot exclude the involvement of othercomplex interactions between particular STN intrinsic membraneproperties (Beurrier et al., 1999; Bevan et al., 2000) and presynapticmechanisms through various inputs distributed along the STN dendriticfield, involving, for example, glutamatergic afferents that makesynaptic contacts preferentially on distal dendrites (Bevan etal., 1995). More surprisingly, although GABA_A receptors were stillblocked by ongoing GABA_A antagonist applications, STN neuronssuddenly switched, as soon as rats woke up, from a robust high-frequencybursting pattern to a regular one. The intrinsic GABAergic toneappears then to be overridden by another phenomenon that regularizesSTN discharge inwakefulness.

In addition, clear disinhibitions or changes of firing pattern were not induced by GABA_B antagonist iontophoresis. This mightbe attributable to the recent description, in STN, of GABA_B receptorsnot only on postsynaptic targets but also on glutamatergic andGABAergic terminals. It must be underlined that most of theseanatomical studies have been performed on monkeys, with only twostudies in abstract form on the rat (Booth et al., 2000; Ng andYung, 2001). The lack of effects of GABA_B antagonist applicationsmight come from the result of a presynaptic blockade of GABA_B-inducedinhibition of glutamate but also GABA release, as suggested byShen and Johnson (2001).

In summary, it appears that, if the blockade of GABA_A receptors within STN favors the emergence of a particularly robust burstypattern, it is, however, not sufficient. These data also ruleout that the regularization of STN spontaneous activity in W mightresult solely from the related increase in the GP firing rate,as we have suggested recently (Urbain et al., 2000). Therefore,the switch of STN neurons between a tonic regular and bursty patternlikely involves other afferents than those of the simplified GP-STNnetwork proposed in vitro by Plenz and Kitai (1999), and mechanismsother than the strong inhibitory input from the GP are likelyable to shape the activity of STN cells (Mink and Thach, 1993;Albin et al., 1995; Hassani et al., 1996; Kreiss et al., 1996,1997; Nakao et al., 1998; Magill et al., 2000).

Actually, during SWS, thalamic and cortical cells oscillate in a low-frequency range (Steriade, 1993; Steriade et al., 1993;Contreras and Steriade, 1997a,b; McCormick and Bal, 1997). Becauseprojections from the cortex and parafascicular nucleus of thethalamus to STN cells are well documented (Kitai and Deniau, 1981;Afsharpour, 1985; Kitai and Kita, 1987; Fujimoto and Kita, 1993;Mouroux and Féger, 1993; Féger et al., 1994; Bevan et al., 1995;Mouroux et al., 1995, 1997), and because STN neurons are extremelysensitive to small changes in their excitatory inputs (Kitai andKita, 1987; Bevan and Wilson, 1999), such afferents are thereforein a position to efficiently shape the STN activity (Magill etal., 2000, 2001). Other mechanisms and afferents are also potentiallyin a position to modulate the STN neuronal activity, in particular,those linked to mesopontine and raphe nuclei inputs, both involvedin sleep-wake mechanisms (Hammond et al., 1983; Canteras et al.,1990; Bevan and Bolam, 1995).

Reduction of tonic pallidal inhibition, as it may result from a dopamine depletion in PD (DeLong, 1990), should have a profoundeffect by disinhibiting the STN. Indeed, a rhythmic bursting activityof STN neurons, phase-related to a resting tremor, has been evidencedin idiopathic and animal models of PD (Bergman et al., 1994, 1998;Wichmann et al., 1994b; Rodriguez et al., 1998; Levy et al., 2000;Magariñoz-Ascone et al., 2000). We found that STN disinhibitionby local GABA_A antagonists resulted in the emergence of robustburst discharges, as observed previously in the anesthetized rat(Féger et al., 1991). Moreover, GP lesions have been shown toincrease the degree of coordination of STN neuron activity andto enhance the neuronal response to motor cortex stimulation (Ryanand Clark, 1992; Ryan et al., 1992), and this may be related toour observation that, in SWS and during GABA_A antagonist applications,we could sometimes hear surrounding STN neurons firing in synchronizedbursts. These data suggest that GABA afferents might act as agating mechanism for the STN firing pattern, and blockade of suchafferents could decrease the selectivity of cortical control ofthe STN but increase STN responsiveness, thus leading to inappropriatemotorbehavior.

Clinical observations showed that most PD symptoms are alleviated by STN high-frequency stimulation (Benazzouz et al., 1993;Benabid et al., 1994; Limousin et al., 1995a,b). Nowadays, thepreponderant hypothesis is that such stimulation might act throughthe depolarization blockade of STN cell bodies (Burbaud et al.,1994; Benazzouz et al., 1995, 2000). However, as observed previouslyin vitro (Nakanishi et al., 1987; Bevan and Wilson, 1999; Wigmoreand Lacey, 2000), we found that disinhibited STN neurons wereable to fire in vivo at very high frequencies, up to 175-185 spikes/secfor mean frequencies and up to 600 spikes/sec for instantaneousfrequencies. In addition, as reported previously in the awakeprimate (Wichmann et al., 1994b), we never observed depolarizationblockade of STN neurons even under the highest amounts of bicucullinetested, in contrast with anesthetized rats (Féger et al., 1991).Taken together, our findings on a nonanesthetized preparationsuggest that STN cell bodies (but also axons; Nowak and Bullier,1998a,b) may easily follow frequencies considerably >130 Hz (clinicaleffective frequency). Although today there is no evidence thatsuch high firing rates can be maintained for a particularly longtime and whether it is possible to faithfully transmit increasesin glutamatergic firing to postsynaptic targets for an extendedperiod, these data nevertheless challenge somewhat the "depolarizationblock" hypothesis. These results might support alternative mechanismsfor deep brain stimulation in PD (Ashby et al., 1999, 2001; Windelset al., 2000), in particular the regularization of firing patternof STN targets, as suggested recently (Hashimoto et al., 2001).

  FOOTNOTES

Received Dec 5, 2001; revised June 27, 2002; accepted June 28, 2002.

This work was supported by grants from Institut National de la Santé et de la Recherche Médicale, Fondation pour la RechercheMédicale (FRM), Université Claude Bernard-Lyon 1, and ConseilRégional Rhône-Alpes. N.U. was the recipient of fellowshipsfrom the Région Rhône-Alpes and the FRM (Neuroscience Researchprograms). We thank Thierry Duffau for efficient computationalexpertise and Lydie Ferres, Margaret Pras, and Geneviève Deguilhemfor administrative assistance. We also thank Vincent Santuccifor providing SR-95531 and Christophe Dugast, Nathalie Javelle,Corinne Beurrier, and Constance Hammond for helpfulassistance.

Correspondence should be addressed to Guy Chouvet, Laboratoire de Neuropharmacologie et Neurochimie, Institut National dela Santé et de la Recherche Médicale U512, Université Claude-Bernard-Lyon1, 69373 Lyon, France. E-mail: gchouvet{at}rockefeller.univ-lyon1.fr.

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