Enhanced Synchrony among Primary Motor Cortex Neurons in the 1-Methyl-4-Phenyl-1,2,3,6-Tetrahydropyridine Primate Model of Parkinson's Disease

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The Journal of Neuroscience, June 1, 2002, 22(11):4639-4653

Enhanced Synchrony among Primary Motor Cortex Neurons in the 1-Methyl-4-Phenyl-1,2,3,6-Tetrahydropyridine Primate Model of Parkinson's Disease
Joshua A. Goldberg¹, Thomas Boraud¹, Sharon Maraton¹, Suzanne N. Haber², Eilon Vaadia¹, and Hagai Bergman¹
¹ Department of Physiology, The Hebrew University-Hadassah Medical School, and the Interdisciplinary Center for Neural Computation, The Hebrew University, Jerusalem 91120, Israel, and ² Department of Neurobiology and Anatomy, University of Rochester, Rochester, New York 14642

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Primary motor cortex (MI) neurons discharge vigorously during voluntary movement. A cardinal symptom of Parkinson's disease(PD) is poverty of movement (akinesia). Current models of PD thushypothesize that increased inhibitory pallidal output reducesfiring rates in frontal cortex, including MI, resulting in akinesiaand muscle rigidity. We recorded the simultaneous spontaneousdischarge of several neurons in the arm-related area of MI oftwo monkeys and in the globus pallidus (GP) of one of the two.Accelerometers were fastened to the forelimbs to detect movement,and surface electromyograms were recorded from the contralateralarm of one monkey. The recordings were conducted before and aftersystemic treatment with 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine(MPTP), rendering the animals severely akinetic and rigid withlittle or no tremor. The mean spontaneous MI rates during periodsof immobility (four to five spikes/sec) did not change after MPTP;however, in this parkinsonian state, MI neurons discharged inlong bursts (sometimes >2 sec long). These bursts were synchronizedacross many cells but failed to elicit detectable movement, indicatingthat even robust synchronous MI discharge need not result in movement.These synchronized population bursts were absent from the GP andwere on a larger timescale than oscillatory synchrony found inthe GP of tremulous MPTP primates, suggesting that MI parkinsoniansynchrony arises independently of basal ganglia dynamics. AfterMPTP, MI neurons responded more vigorously and with less specificityto passive limb movement. Abnormal MI firing patterns and synchronization,rather than reduced firing rates, may underlie PD akinesia andpersistent musclerigidity.

Key words: correlations; neuronal synchronization; EMG; firing patterns; intracortical microstimulation; monkey; striatum; globus pallidus; kinesthetic; oscillations

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The normal execution of voluntary movement is correlated with an increase in the synchronous discharge of primary motor cortex(MI) neurons (Evarts, 1965; Porter and Lemon, 1993; Ohara et al.,2001). Many Parkinson's disease (PD) patients suffer from a deficitof voluntary movement, termed akinesia, as well as increased musclerigidity. These facts have been incorporated succinctly into currentphysiological models of PD (Albin et al., 1989; DeLong, 1990).They hypothesize that the loss of midbrain dopaminergic cellsleads to changes in firing rates throughout the basal ganglia(BG) that ultimately decrease motor cortical output, resultingin akinesia and rigidity. It follows that the predicted suppressionof motor cortical discharge should be evident in MI, because itis the area of frontal cortex that is most closely related tospinal cord output and to the final execution of movement (Asanuma,1989; Porter and Lemon, 1993).

Evidence from various human studies, including regional cerebral blood flow (Playford et al., 1992; Rascol et al., 1994),functional magnetic resonance imaging (fMRI) (Sabatini et al.,2000; Haslinger et al., 2001), and transcranial magnetic stimulation(Ridding et al., 1995; Kleine et al., 2001), fails to supportthe notion that MI activation or excitability is decreased inPD. Similarly, direct measurement of single-unit discharge (Doudetet al., 1990; Watts and Mandir, 1992) and cerebral metabolic studies(Porrino et al., 1987; Schwartzman et al., 1988) in primates renderedparkinsonian by 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine (MPTP)lesions have shown no evidence of a lasting decrease in MI activity.However, most of these studies focused on task- or movement-relateddischarge, and the animal studies were conducted on mildly affectedor recovered animals. The enduring symptoms of severe akinesiaand rigidity suggest that the presumed suppression of firing ratesshould be present in the spontaneous activity of MI neurons (i.e.,during periods ofimmobility).

Physiological studies in tremulous parkinsonian subjects have found prominent changes in neuronal discharge patterns and insynchronization between neurons throughout the BG (Nini et al.,1995; Levy et al., 2000; Raz et al., 2000). This increased synchronizationin the BG is accompanied by a loss of neuronal specificity inthe globus pallidus (GP) in response to passive joint manipulation(Filion et al., 1988; Boraud et al., 2000) and striatal microstimulation(Tremblay et al., 1989). Because BG circuits are closely tiedto the cortex (Gerfen and Wilson, 1996; Hoover and Strick, 1999;Bolam et al., 2000), it is likely that changes in neuronal synchronizationand specificity will arise in the cortex aswell.

The aims of this study were (1) to directly test the hypothesis that the mean spontaneous discharge in MI is reduced afterMPTP treatment; (2) to characterize the population activity ofMI neurons as revealed by the multiple electrode recording techniqueand compare it with the population activity of BG neurons; (3)to test whether MPTP treatment induces changes in the specificityof joint representation in MI; and (4) to determine whether MImicro-excitability is altered by MPTP treatment, as reflectedin the responses to intracortical microstimulation(ICMS).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experimental design. Two monkeys (monkey S: Cercopithecus aethiops aethiops, female, weight 3.5 kg; monkey Z: Macaca fascicularis,female, 2 kg) were trained to perform a self-initiated button-pressingtask with their dominant hand. With each monkey we used a slightlydifferent design to address the issue of spontaneous MI activity.Monkey S performed the task throughout the whole recording sessionin the normal state. In this monkey, the spontaneous activitywas defined as the neuronal activity during periods of the monkey'simmobility determined by use of accelerometry (see below). Theaverage duration of the periods of immobility was on the orderof a few seconds long. In contrast, monkey Z was trained to sitquietly until given a liquid reward that signaled it to commencethe motor task. Thus, in this monkey we were able to record spontaneousactivity for several (~15) minutes while the monkey was at rest.Nevertheless, we again used accelerometry to exclude segmentsof data that included movements. Both monkeys were rendered parkinsonianby systemic treatment with the MPTP neurotoxin (see below). Inthe MPTP-treated state, the monkeys were akinetic and did notperform the task. Throughout the whole recording sessions in bothstates, the examiners verified regularly that the monkeys wereawake. An additional monkey (monkey G: Macaca mulatta, female,3.5 kg) that participated in another study and was not treatedwith MPTP was used as control for thehistology.

The monkeys' health was monitored by a veterinarian, and their fluid consumption, diet, and weight were monitored daily. Themonkeys' care and surgical procedures were in accordance withthe NIH Guide for the Care and Use of Laboratory Animals (1996)and the Hebrew University guidelines for the use and care of laboratoryanimals in research, supervised by the institutional committeefor animal care anduse.

Surgical and neuronal recording procedures. After training, a square recording chamber with a 27 mm (inner) side was attachedto the skull under deep ketamine-xylazine anesthesia in asepticconditions. Location of the chamber was determined with the aidof MRI (Biospec Bruker 4.7 tesla animal system; fast-spin echosequence; effective echo time = 80 msec and repetition time =2.5 sec; 13 coronal slices, 2 mm wide). The sides of the chamberwere aligned with the coronal and sagittal planes. The chamberwas placed such that its center lay in the stereotactic A10 plane.Thus the central and arcuate sulci were within the chamber, and,in monkey S, good access to striatum and GP was available in theanterior part of the chamber. In this monkey, the recording chamberwas tilted 45° laterally in the coronal plane to optimize accessto GP. In each recording day, eight glass-coated tungsten (0.2-1.2M $Omega$ at 1 kHz) electrodes, confined to a 1.65 mm inner diameterguide tube, were inserted into the brain in the following manner.For cortical penetrations (Fig. 1), the electrodes were firstlowered manually to ~3 mm above the dura mater. Then a mechanicalmicro-drive (EPS 1.28, Alpha-Omega Engineering, Nazareth, Israel)was used to lower each electrode individually through the durato the cortex while tracking its depth. All recording sites werewithin a 6 mm (mediolateral) by 5 mm (anteroposterior) regionof the precentral gyrus in both monkeys. For GP penetrations,the guide tube with the eight electrodes was advanced ~9 mm intothe brain, and then each electrode was individually driven throughthe striatum to the vicinity of GP cells. Striatal neurons wereoften encountered during the GP sessions and were recorded aswell. The output of the electrodes was amplified ×10⁴, bandpass filtered (0.3-6 kHz, four-pole Butterworth filter),and fed to a template-matching device to isolate the extracellularactivity of 1-3 units per electrode. The timing of the detectedspikes was sampled at 12 kHz (MCP+, MSD2.1, AlphaMap 4.8, Alpha-OmegaEngineering). Neurons were selected by isolation quality and recordingstability only. The number of recording sessions (and days) usedfor the analysis is listed in Table 1.

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Figure 1. Experimental setup: simultaneous recording of multiple electrodes, accelerometers, and surface EMGs. Monkeys were trained to execute a self-initiated button-pressing task. Eight electrodes were lowered to the brain (cortical penetrations depicted). Accelerometers were fastened to both wrists (contralateral working hand depicted) to detect movement. In monkey Z, surface EMG was recorded from the biceps and triceps of the working arm.


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Table 1. The neuronal database

Somatosensory examination and intracortical microstimulation. Somatosensory examination and ICMS were used to verify the locationof the electrodes within the arm area of MI. At the end of everyrecording day we assessed the responsiveness of each recordingsite to passive manipulation of six joints in the contralaterallimbs (shoulder, elbow, wrist, hip, knee, and ankle). The strengthof responsiveness of a site was graded according to the multiunitactivity it elicited: 0 = no response; ? = questionable response;1 = background/hash response; 2 = response of cells at foreground.In cortical sessions, after somatosensory examination, we injected100 msec, 300 Hz trains of 0.2 msec cathodic current pulses withamplitudes ranging from 5 to 40 µA through each of the recordingelectrodes. Two to three examiners visually monitored the monkeysand determined the threshold current for eliciting movement ofthe contralateral arm. This protocol (using one to two electrodes)was used also during standard mapping sessions conducted beforethe commencement of the recording sessions to determine the locationof the arm area of MI within the recording chamber. In monkeyS, mapping sessions (including somatosensory examination) wereconducted to localize GP within the chamber aswell.

MPTP treatment. MPTP-HCl (Sigma, St. Louis, MO) was injected systemically five times over a period of 4 d (0.4 mg/kg per injection,i.m.) under mild ketamine anesthesia. After the first MPTP injection,both monkeys were clinically assessed on a regular basis usingthe Hoehn and Yahr (1967) clinical staging scale (0-5). MonkeyZ was also clinically rated using a primate rating scale (Benazzouzet al., 1995) with the following items: tremor (0-3), body posture(0-3), general activity (0-3), vocalization (0-2), freezing (0-2)rigidity (0-3 for each side), and frequency of arm movement (0-3for each upper limb). The maximum disability score is 25. Thethreshold for severe parkinsonism is defined at 15 (Imbert etal., 2000).

Accelerometer and Electromyogram data collection and analysis. Two uni-axial accelerometers (8630C5, Kistler, Amherst, NY)were fastened to the wrists of each of the monkeys (Fig. 1). Inmonkey S, two additional accelerometers were attached to the ankles.The output of the accelerometers was sampled at 0.8 kHz. Duringthe recording sessions in the MPTP state, the monkeys were generallyimmobile and did not perform the task. Therefore, to make a validcomparison between the normal and MPTP states, it was necessaryto discriminate between periods of limb movements ("active periods")and periods of immobility ("immobile periods") in the normal state.We used the accelerometer on the contralateral (working) arm tomake this classification. The output of the accelerometers waszero-phase bandpass filtered (1-30 Hz) and a root mean square(rms) version of the signal was calculated (averages were estimatedover running windows of 0.8 sec). When a segment of the rms signalfrom the contralateral wrist exceeded a predetermined thresholdof 0.05 g (=25 cm × sec²) it was defined as an active period. Visual inspection of theother accelerometer traces proved that the output of this singleaccelerometer was a reliable measure of whether the monkey wasactive. The comparison between the normal and the MPTP stateswas conducted only for the periods ofimmobility.

In monkey Z, surface EMG electrodes were attached to the bellies of the triceps and biceps of the contralateral arm (Fig.1). The electromyogram (EMG) was amplified and rectified, andits rms was sampled at 0.8kHz.

Neuronal data analysis. Only spike trains judged during the real-time sorting to be emitted by a single cell were subjectedto rate stability analysis. In the rate stability analysis, asmoothed estimate of the instantaneous rate of a neuron as a functionof time was displayed for the whole period of recording. Thenthe largest segment of data for which the following criteria weremet was kept for further analysis: (1) the statistics of the rateof the unit within the segment were judged visually to be stationary(e.g., no abrupt changes or trends in instantaneous rate), and(2) the interspike interval (ISI) histogram of the unit calculatedover this segment was judged visually to increase monotonicallyfrom zero at bin zero [indicating that the unit displays a refractoryperiod and hence is well isolated (Fee et al., 1996)]. Table 1lists the median number of units per session that were originallydetected, followed by those that met the above criteria. It alsoindicates the duration of recording from these stable and wellisolatedunits.

After stability analysis, the firing rates, autocorrelograms (ACs), and pairwise cross-correlograms (CCs) of the cells werecalculated. The CCs were calculated only for pairs of cells recordedby different electrodes to avoid artifacts caused by sorting shading(Bar-Gad et al., 2001). The correlograms were calculated as follows:coincidence histograms at 1 msec resolution were estimated overperiods of immobility that were at least 2 sec long (twice themaximum lag-shift). A smoothed coincidence histogram (SCH) wascreated using a K = 81 bin (msec) moving average and was thennormalized to units of rate (spikes per second) to generate thecorrelograms (the zero lag of the ACs was set to zero before smoothing).The ACs were calculated only for cells with segments of stablerecording and isolation that contained at least 400 spikes. Similarly,CCs were calculated only for pairs in which each cell fired atleast 400 spikes during their joint period of stable recordingand isolation. We estimated the SD of the SCH at lag shift t by:

where HSCH is a heavily smoothed version of the coincidence histogram (using a 251 bin moving average). SD(·) thus accountsfor the local variability of the SCH(·). Confidence intervalsfor the correlograms were set to 4.5 SDs normalized to units ofrate around the expected value of the CC(·) estimated at the flanks(absolute lag shift >900 msec). This conservative threshold wasused because it efficiently removed what were visually judgedto be spurious excursions of the correlograms. However, performingthe analysis with less conservative confidence intervals did notchange theresults.

To quantify the strength of the association between neurons, we defined for each pair an association index (AI) as the relativeincrease in the number of spikes fired as a result of the associationbetween the cells. The AI is defined as follows:

where CC(t) is the cross-correlogram value at lag shift t in spikes per second, [t1,t2] is the range of lag shifts wherethe CC exceeds its upper confidence level, and R is the expectedvalue of CC(·) estimated at the flanks of the CCs. Thus AI isthe percentage of additional spikes (relative to the expectednumber) fired by one cell because of its association with theother and is independent of which of the two cells is tagged asthe reference cell [this is essentially the same as the "meanpercent increase" used by Murthy and Fetz (1996)]. The auto-associationindex (AAI) of a single neuron was defined in the same mannerwith CC(·) replaced by AC(·). When a correlogram did not exceedthe upper confidence level at any lag shift, the AI or AAI wasset to zero percent. When the AI value exceeded 50% we definedthe pair of cells as "stronglysynchronized."

To further quantify the degree of "burstiness" at the single-unit level in the MPTP versus the normal state, we used a testmotivated by the Kaneoke-Vitek algorithm (Kaneoke and Vitek, 1996).For a given spike train we first calculated the duration of itsmean ISI and then rebinned the spike train into segments of thisduration. We thus create a stochastic process of the number ofspikes per bin, denoted by P_t. The mean of this process is unity,by construction. We used the following statistic L to quantifythe degree of burstiness of a spike train: L is the number ofdistinct values taken on by the rebinned process P_t. If a cellis bursty its P_t will attain large values (many spikes per meanISI). To test whether there is a change in burstiness in MI afterMPTP we compared the distribution of L between the normal immobileand the MPTP states. We preferred to use the L statistic ratherthan the range of values taken on by P_t, because the former isinsensitive to outliers. However, using the range statistic gavethe same statistical results. Obviously, the value of both thesestatistics depends on the duration of the recording. However,in monkey S the mean duration was longer in the normal state,and in monkey Z the mean duration was longer in the MPTP state(see Table 1), so a consistent result across monkeys regardingthese statistics would indicate that it is not an artifact causedby the duration ofrecordings.

Histology. After the last recording session (days 57 and 22 from last injection to monkeys S and Z, respectively), the monkeyswere deeply anesthetized with a lethal dose of pentobarbital andkilled by perfusion through the heart with saline followed bya 4% paraformaldehyde solution in 0.1 M phosphate buffer, pH 7.4.The brains were removed and cryoprotected in increasing gradientsof sucrose (10, 20, and finally 30%). Serial sections of 50 µmwere cut on a freezing microtome, and every eighth section wasprocessed for either immunocytochemistry for tyrosine hydroxylase(TH) or a Nisslstain.

Tissue processed for TH immunocytochemistry was incubated with antisera to TH (1:20,000; Eugene Tech, Inc.) in 0.1 M phosphatebuffer with 0.3% Triton X-100 and 10% normal goat serum (Incstar)for four nights at 4°C and further processed using the avidin-biotinmethod (rabbit Elite Vectastain ABC Kit, Vector Labs). Sectionswere rinsed first in PBS and then in Tris buffer (0.05 M, pH 7.6)and preincubated in a filtered 0.05% 3,3'-diaminobenzidine tetra-hydrochloridesolution in Tris buffer for 10 min, before adding 0.01% H₂O₂.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Clinical and histological effects of the MPTP treatment

Systemic MPTP treatment rendered the monkeys severely akinetic and rigid with abnormal flexed posture. The parkinsonian symptomsstabilized in both monkeys 8 d after the first MPTP injectionand remained stable up to the conclusion of the experiment. Examinationof the output of the accelerometers showed that the monkeys displayedno (monkey S) or very infrequent (monkey Z) episodes of tremorafter MPTP treatment. Both monkeys rated stage 5 on the Hoehnand Yahr Scale (Hoehn and Yahr, 1967). Monkey Z rated 17.3 ± 1.0(mean ± SD; n = 7 d) on the primate rating scale (Benazzouz etal., 1995; Imbert et al., 2000).

In the control animal, there was dense TH immunoreactivity throughout the striatum (Fig. 2, rows 1 and 2). The intensity ofstaining for TH immunoreactivity was heterogeneous, with a patchyand uneven pattern. Consistent with the behavioral deficits, bothMPTP-treated animals showed an almost complete loss of TH stainingthroughout the caudate nucleus and the putamen. In contrast tothe lack of staining in the dorsal striatum, there were patchesof TH immunoreactivity in the ventral striatum. In particular,the shell of the nucleus accumbens remained TH positive (Fig.2, row 1). There are two groups of midbrain dopamine cells, adorsal tier (ventral tegmental area and the retrorubral group)and a ventral tier (substantia nigra, pars compacta), that havedifferent vulnerabilities to the toxic effects of MPTP (Lavoieand Parent, 1991; Song and Haber, 2000) and different projectionpatterns (Lynd and Haber, 1994). The dorsal tier is less vulnerableto toxic insult and projects to the ventral striatum, whereasthe ventral tier is more vulnerable to toxic insult and projectsto the dorsal striatum. The pattern of striatal loss of TH immunoreactivityin monkeys S and Z is consistent with these characteristics ofthe dorsal and ventral tier midbrain dopamine cells. The TH cellloss was concentrated in the ventral tier, whereas in the dorsaltier the cells were selectively spared (Fig. 2, rows 3 and 4).The Nissl-stained sections further demonstrate the loss of neuronsin the ventral tier, compared with control. Instead, a massivemicroglia reaction infiltrates the area previously occupied byneurons (Fig. 2, row 5).

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Figure 2. Photomicrographs of tyrosine hydroxylase (TH) (rows 1-4) and Nissl staining (row 5) through the striatum and midbrain of a normal control (A) and the two MPTP-treated animals (B-C); rostral striatum (row 1); central striatum (row 2); and midbrain (rows 3 and 4). Row 5 depicts the adjacent sections stained for Nissl. The asterisks in rows 4 and 5 mark corresponding blood vessels. Note the lack of TH-positive staining throughout most of the striatum in the MPTP-treated animals. The shell region of the ventral striatum, however, is selectively spared (rows 1 and 2). TH-positive cells are selectively lost in the ventral tier (vt, 3A, in white). In contrast, cells in the dorsal tier (dt) are selectively spared (row 3). Row 4 depicts the magnified views of the boxed areas in row 3. Each region is taken at the border between TH-positive cells and the lack of cells. The photomicrographs from the MPTP-treated animals are taken at a more dorsal level, at the junction between the dorsal and ventral tier cells. The photomicrograph from the normal control animal was taken at the junction between the ventral tier cells and the pars reticulata. The Nissl-stained sections (row 5) demonstrate the lack of neurons in the ventral tier of the MPTP-treated animals. Although in the control animal Nissl-stained neurons are clearly evident, in the MPTP-treated animals a massive glial infiltration has largely replaced the compacta cells.

Effects of MPTP as reflected in the EMG and accelerometer traces

In monkey Z, the EMG recordings in the normal state often exhibited the characteristic tri-phasic pattern of muscle activation(agonist-antagonist-agonist) (Basmajian and De Luca, 1985) duringmovement (Fig. 3A). In contrast, the accelerometer and EMG tracesshowed very little modulation throughout the MPTP sessions andfailed to show any obvious temporal relationship to the neuronalbursts (Fig. 4B). On the rare occasions when sporadic movementswere detected in the MPTP state, the EMG revealed coactivationof the antagonistic muscles (Fig. 3B) (Doudet et al., 1990; Benazzouzet al., 1992).

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Figure 3. Activation patterns of antagonistic muscles in the normal and MPTP states of Monkey Z. A, Normal; B, MPTP. Top, Output of accelerometer attached to the wrist of the working arm. Bottom, EMG recording from biceps and triceps of the working arm. Calibration: horizontal, 1 sec; vertical (accelerometer traces), 0.5 g (=490 cm × sec²). Scale of EMG is arbitrary. Note the tri-phasic pattern of muscle activation (biceps leading) in the normal voluntary movement, in contrast to the completely overlapping co-contraction in the MPTP movements.

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Figure 4. Neuronal discharge in the arm area of MI and contralateral arm movements in the normal and MPTP states of Monkey S. A, Normal; B, MPTP. A, B, Top traces, Extracellular activity recorded from eight electrodes simultaneously. Bottom, Output of accelerometer attached to the contralateral wrist. Bars below the accelerometer trace in A represent active periods of the monkey. Calibration: horizontal, 1 sec; vertical (accelerometer traces), 1 g.

To quantify the paucity of movement, we calculated the percentage of time that the accelerometers spent above the 0.05 g thresholdduring the MI recording sessions (Table 1). The total durationof these active periods decreased significantly after MPTP. Inmonkey S it decreased from 40.0 ± 5.2% (mean ± SEM) in the normalstate to 5.4 ± 1.6% (p < 10⁴) after MPTP, and in monkey Z it decreased from 12.7 ± 2.3% to2.5 ± 0.8% (p < 10³; two-sided two-sample t test). The difference between the monkeysin the normal state results from the different experimental designsused in the two animals. In monkey S the periods of immobilitywere interleaved among the self-initiated movements, whereas inmonkey Z they were taken from the ~15 min period before the animalbegan the motortask.

Effects of MPTP on firing rates of single MI cells

In the normal state, increases in MI firing rates that covary among neurons were typically confined to periods of movement(Fig. 4A). In contrast, in the MPTP state, MI cells exhibitedlong volleys (sometimes >2 sec long) of synchronized bursts recordedacross most electrodes, although no movement could be detected(Fig. 4B, raw data; 5, raster plots).

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Figure 5. Raster plots of simultaneous spontaneous discharge of 9 units in the normal (A) and MPTP (B) states of monkey Z. In each panel 2 contiguous minutes of data (12 rows of 10 sec each) are depicted. Each tick is a spike of one cell. Nine cells are depicted in each row. In A, the 2 min are from a period at the beginning of the session wherein the normal monkey sat restfully before the commencement of the behavioral task. In B, data are shown from the akinetic MPTP-treated monkey. Long population bursts (sometimes >2 sec long) separated by relatively quiescent periods are evident in the MPTP state. Calibration: 2 sec.

Parsing the MI data from the normal state into active and immobile periods revealed, as expected, that the firing rates weresignificantly higher in the active periods than in the immobileones (Table 2A). Comparison of overall mean firing rates betweenthe normal immobile and MPTP states revealed no significant difference(Table 2A, Fig. 6). Figure 5 demonstrates how this is possible.Although monkey Z sat restfully in the normal state, the cellshad a rather constant firing rate; however, after MPTP treatment,several cells seem to fire in clusters separated by extended periodsof silence (see also Fig. 4B).


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Table 2. Firing rates and synchronization of neurons in the arm area of MI in the normal and MPTP states

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Figure 6. Frequency distributions of the mean spontaneous firing rates of MI neurons in the normal immobile (A, C) and the MPTP (B, D) states. A, B, Monkey S; C, D, Monkey Z. Abscissa, spikes per second; ordinate, percentage; n, number of neurons; mean, mean ± SEM of firing rates in spikes per second. There is no significant difference in the population mean spontaneous rate between the normal immobile and the MPTP states (two-sided two-sample t test; p > 0.45, monkey S; p > 0.5, monkey Z).

Effects of MPTP on firing patterns of MI cells

The appearance of bursts in the MPTP state is reflected in the autocorrelograms of the cells. As illustrated in Figure 7,the autocorrelograms in the MPTP state tend to have larger andwider peaks, indicative of the increase in bursting dischargein this state compared with the immobile periods in the normalstate. To quantify this increase, we calculated the AAI of eachcell. There was a significant shift in the distribution of AAIstoward larger values in the MPTP state relative to the normalimmobile state (Fig. 8A,B). Similarly, the mean value of the AAIwas significantly larger in the MPTP state (Table 2B). The Lstatistic [based on the Kaneoke-Vitek algorithm (Kaneoke and Vitek,1996)] was also shifted significantly toward larger values, indicatinga stronger tendency to burst after MPTP (Fig. 8C,D). This tendencywas evident throughout all recording sessions and was not confinedto certain penetration depths. Finally, no periodicities (in the2-500 Hz range) were observed in any of the MI auto-coincidencehistograms after MPTP.

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Figure 7. Autocorrelograms of spontaneous discharge of MI neurons in the normal immobile and MPTP states. Solid line, Estimate of the auto-intensity function; dashed line, confidence intervals. Abscissa, Lag shift in milliseconds; range, ±1000 msec; ordinate, conditional discharge rate in spikes per second. The absence of the typical refractory period around time 0 is attributable to the smoothing used.

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Figure 8. Spontaneous neuronal bursting in MI in the normal immobile and MPTP states. A, C, Monkey S; B, D, Monkey Z. A, B, Cumulative frequency distribution of the auto-association index (AAI) of neurons with significant peaks in their autocorrelograms. Dashed line, Normal; solid line, MPTP (abscissa, AAI; ordinate: percentage). The distribution in the MPTP state is shifted to the right, indicating that the AAIs are stochastically greater in this state than in the normal immobile one (two-sided Wilcoxon rank-sum test; monkey S, normal: n = 65, MPTP: n = 119, p < 0.02; monkey Z, normal: n = 51, MPTP: n = 96, p < 10⁴). C, D, Cumulative frequency distribution of the L statistic. L is the size of the set of distinct values attained by the process of rebinning the spike train at its mean ISI. Dashed line, normal; solid line, MPTP (abscissa, L; ordinate, percentage). The distribution in the MPTP state is shifted to the right, indicating that the L values are stochastically greater in this state than in the normal immobile one (two-sided Wilcoxon rank-sum test; monkey S, normal: n = 71, MPTP: n = 125, p < 10⁴; monkey Z, normal: n = 57, MPTP: n = 106, p < 2 × 10³).

Effects of MPTP on the synchronization of MI cells

The level of synchrony in MI is reflected in the cross-correlograms of simultaneously recorded neurons (Fig. 9, monkey S;Fig. 10, monkey Z). Although the cross-correlograms were relativelyflat in the normal immobile state (Murthy and Fetz, 1996), theyhad broad (on the order of 1 sec long) pronounced peaks in theMPTP state. These peaks were centered on time 0 and were rathersymmetrical. An enhancement of synchronization on such a broadtimescale is more aptly described as a covariation of firing ratesamong neurons. The noisy character of the cross-coincidence histogramscalculated between MI pairs with low firing rates precluded detectionof a finer form of synchrony on the timescale of tens of milliseconds.The increase in the percentage of cross-correlograms with significantpeaks in the MPTP state was not significant (Table 2C), indicatingthat pairs of neurons in the normal immobile state were as likelyto be coupled as in the MPTP state. However, there was a significantshift in the distribution of AIs toward larger values (Fig. 11)in the MPTP state. Similarly, there was a significant increasein the mean AI and in the percentage of strongly synchronizedpairs in this state (Table 2C). This implies that the associationbetween pairs is larger in the MPTP state and that there is asignificantly larger subset of neuronal pairs that are abnormallycoupled in this state. The enhancement of synchronization wasevident in all recording sessions. As with the auto-coincidencehistograms, no periodicities were observed in the MI cross-coincidencehistograms after MPTP.

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Figure 9. Cross-correlograms of spontaneous discharge of five simultaneously recorded MI neurons in the normal immobile and MPTP states of monkey S. Above diagonal, Normal; below diagonal, MPTP. Solid line, Estimate of conditional rate of the reference cell; dashed line, confidence intervals. Numbers at top of each column, reference cell; numbers to the right of each row, trigger cell. Abscissa, Lag shift in milliseconds; range, ±1000 msec; ordinate, conditional discharge rate in spikes per second.

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Figure 10. Cross-correlograms of the spontaneous discharge of five simultaneously recorded MI neurons in the normal immobile and MPTP states of monkey Z. Format same as in Figure 9.

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Figure 11. Synchronization in arm area of MI in the normal immobile and MPTP states. A, Monkey S. B, Monkey Z. Shown is the cumulative frequency distribution of the association index (AI) of pairs of neurons with significant peaks in their cross-correlograms. Dashed line, Normal; solid line, MPTP (abscissa, AI; ordinate, percentage). The distribution in the MPTP state is shifted to the right, indicating that the AIs are stochastically greater in this state than in the normal immobile one (two-sided Wilcoxon rank-sum test; monkey S, normal: n = 67, MPTP: n = 246, p < 10⁴; monkey Z, normal: n = 40, MPTP: n = 135, p < 0.02).

Effects of MPTP on the discharge of pallidal and striatal cells

All pallidal cells recorded were encountered within a 2 mm depth from the border between striatum and GP. This along withthe typical firing patterns of the cells (DeLong, 1971) indicatesthat our pallidal sample was composed only of neurons from theexternal segment of the globus pallidus (GPe). The mean firingrates of GPe (n = 80) and striatal (n = 17) neurons in the normalstate of monkey S were not augmented during the monkeys' activeperiods relative to the immobile periods (p > 0.15; one-sidedpaired t test). There was no significant difference between themean spontaneous GPe firing rates before (36.1 ± 2.6 spikes/sec;mean ± SEM; n = 80) and after (32.5 ± 1.6 spikes/sec; n = 105)MPTP treatment, or between the mean spontaneous firing rates ofstriatal neurons before (5.2 ± 0.9 spikes/sec; n = 17) and after(6.8 ± 0.9 spikes/sec; n = 18) treatment (p > 0.2; two-sided two-samplet test). Interestingly, the cross-correlograms of GPe pairs werecompletely flat in both states (Fig. 12A). The AIs were identicallyzero for all pairs both before (n = 185) and after (n = 233) treatment.In contrast, 94% of cross-correlograms (15 of 16) among striatalneurons showed 10 Hz oscillatory synchronization after MPTP (Fig.12B). Judging by their electrophysiological properties, most striatalneurons we recorded both before and after MPTP treatment wereprobably tonically active neurons, although we did not verifytheir responsiveness to reward (Kimura et al., 1984; Graybielet al., 1994; Raz et al., 1996).

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Figure 12. Synchronization in the BG of monkey S in the normal immobile and MPTP states. Format same as in Figure 9. A, Examples of cross-correlograms from the GPe. All cross-correlograms, both before and after MPTP, are flat. B, Examples of cross-correlograms from the striatum. Note the 10 Hz oscillatory associations after MPTP (the oscillatory coincidence histograms were smoothed by a 21 msec moving average).

Somatosensory examination and intracortical microstimulation

The results of somatosensory examination and ICMS are summarized in Table 3. There was no significant difference betweenthe normal and the MPTP state in the percentage of MI penetrationsites whose stimulation elicited movement of the contralateralarm. The mean threshold for eliciting movement did not differsignificantly after MPTP treatment in monkey S but did significantlyincrease in monkey Z (Table 3A). However, even in monkey Z afterMPTP, ICMS often elicited strong responses and the threshold currentsometimes reached as low as 5 µA, which is in the lower rangeof normal MI micro-excitability (Murthy and Fetz, 1996; Tokunoand Nambu, 2000).


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Table 3. Excitability and responsiveness to passive movement of the arm area of MI in the normal and MPTP states

Analysis of the responses from MI recording sites to the passive manipulation of the three contralateral arm joints revealsthat the specificity of motor representation in MI significantlydecreased after MPTP. The number of positive responses increased(Table 3B), and there was a shift toward stronger responses,i.e., relatively more responses included cells in the foregroundand relatively less were composed of hash only (Fig. 13). The mediannumber of joints whose passive manipulation elicited multiunitactivity in MI recording sites increased significantly after MPTPtreatment (Table 3C). In GPe we discerned no significant differencein neuronal specificity between the normal and the MPTP states.

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Figure 13. Frequency distribution of the pooled responses to passive manipulation of the contralateral shoulder, elbow, or wrist as recorded at all cortical penetration sites. A, Monkey S. B, Monkey Z. White bars, Normal. Black bars, MPTP. Neuronal responses were graded as follows: 0 = no response; ? = questionable response; 1 = background/hash response; 2 = response of cells at foreground. There is a significant shift of the frequency histograms to the right, indicating an increase in the positive responses to passive manipulation and that more responses involved strongly activated single units ( $chi$ ²; monkey S, normal: n = 213, MPTP: n = 168, p < 10⁴; monkey Z, normal: n = 222, MPTP: n = 183, p < 0.01).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We recorded the spontaneous discharge of several neurons in the arm area of the primate MI before and after systemic MPTPtreatment. We chose to first study the effects of MPTP on MI,because it is the cortical structure whose activity is classicallyconsidered to be most closely related to muscle activation andthe final execution of movement (Evarts, 1965; Porter and Lemon,1993). After MPTP treatment the monkeys became severely akinetic,with enhanced muscle rigidity. Tremor was either absent or minimal.Our results show that these clinical effects were not accompaniedby a change in the mean spontaneous firing rates of the MI neurons,which remained in the normal range of four to five spikes persecond. However, there were marked changes in firing patternsof single cells and in synchronization among cells. Typically,the neurons discharged in long volleys of spikes (bursts, sometimes>2 sec long). Moreover, the bursts of different neurons occurredin synchrony. The synchronous bursts were observed at all depthsalong the recording tracts. Interestingly, these MI populationbursts in the MPTP state failed to elicit transient muscle activationor armmovement.

Comparison with physiological and imaging studies of the parkinsonian MI

Previous single-electrode studies in parkinsonian primates have demonstrated that mean task- or movement-related MI firingrates do not change after electrolytic or MPTP nigral lesions(Gross et al., 1983; Doudet et al., 1990; Watts and Mandir, 1992).Doudet et al. (1990) also reported no significant change in thespontaneous (non-task-related) mean firing rate of MI neurons.However, their monkeys underwent a rapid and almost complete behavioralrecovery after MPTP and were able to perform trained and self-initiatedmovements. In contrast, our monkeys were severely affected duringthe period of recordings. Previous studies of MPTP-recovered catshave shown that all electrophysiological measures of neuronaldischarge in BG returned to levels resembling those seen in normalanimals (Rothblat and Schneider, 1993; Rothblat and Schneider,1995). Thus, our study that focused on spontaneous MI discharge(in the absence of movement) demonstrates that the mean spontaneousfiring rates remain unchanged even in severely akineticprimates.

Experimental methods that indirectly measure MI activity in the parkinsonian state have yielded contradictory results. Brownand collaborators (Brown et al., 1998; Brown and Marsden, 1999;Wang et al., 1999; Brown, 2000) have studied the spectra of macroscopiccortical signals and EMG to demonstrate differences between PDpatients and healthy controls during the execution of voluntarymovements. Studies of 2-[¹⁴C]deoxyglucose metabolism in MPTP primates have found transientchanges in glucose utilization in MI (Porrino et al., 1987; Schwartzmanet al., 1988). Emission tomography studies of MI in PD patientshave shown that the metabolic activity remains mostly unchangedrelative to controls during both rest and movement (Playford etal., 1992; Rascol et al., 1994; Jahanshahi et al., 1995; Samuelet al., 1997a). There is no consensus regarding the effect onMI activity of (1) pallidal inactivation during rest (Eidelberget al., 1996; Henselmans et al., 2000; Fukuda et al., 2001) ormovement (Ceballos-Baumann et al., 1994; Grafton et al., 1995;Samuel et al., 1997b), (2) subthalamic nucleus stimulation (Limousinet al., 1997; Ceballos-Baumann et al., 1999), or (3) levodopatherapy (Rascol et al., 1994). In contrast, fMRI studies haveconsistently shown increased task-related blood-oxygen-level-dependent(BOLD) responses in MI relative to controls (Sabatini et al.,2000; Haslinger et al., 2001) and return to normal levels afterlevodopa (Haslinger et al., 2001).

What aspects of neuronal activity are reflected in these indirect measures of cortical metabolism is still under debate (Jueptnerand Weiller, 1995; Heeger et al., 2000; Logothetis et al., 2001).Some of these studies may be more sensitive to mean firing rates,whereas others may reflect the level of population synchrony.For example, it has been proposed that the fMRI BOLD signal mayreflect changes in neuronal firing patterns and synchrony (Arthursand Boniface, 2002). Our demonstration of an enhanced burstingsynchrony in MI may explain why the fMRI studies of PD patientsshow an enhanced BOLDsignal.

Changes in mean firing rates in the cortical-BG circuits

The above-mentioned studies alongside our results fail to demonstrate that MI is deactivated in PD as hypothesized by thecurrent model of the BG. How can these data be reconciled withthe observed changes in pallidal firing rates in parkinsonism(Miller and DeLong, 1987; Filion and Tremblay, 1991; Boraud etal., 1998) that presumably inhibit frontal cortex? Perhaps thepallidal receiving areas in the ventrolateral thalamus or frontalcortex possess compensatory mechanisms that regulate the overallmean firing rates in MI (Sabatini et al., 2000; Thobois et al.,2000). Alternatively, this inhibition may differentially affectdifferent subclasses of cortical neurons (Bauswein et al., 1989;Gur et al., 1999; Turner and DeLong, 2000). However, the changesin MI firing patterns and synchronization at various depths alongthe penetration tracts indicate that these changes are not confinedto any specific cortical layer. Finally, we found no change inthe mean firing rate of GPe neurons after MPTP. This result joinsgrowing evidence that pallidal firing rates do not change in allmonkeys as described in the current model of PD (Bergman et al.,1994; Bezard et al., 1999; Wichmann et al., 1999; Raz et al.,2000; Boraud et al., 2001). It thus appears that what underliesparkinsonian akinesia is not necessarily the hypothesized changesin firing rates in the cortical-BG circuits (Boraud et al., 2002).

Changes in synchrony in the cortical-BG circuits

Studies of the cortico-BG circuitry have shown its propensity to oscillate synchronously (Plenz and Kitai, 1999; Magill etal., 2000). Several studies of parkinsonism have shown an increasein synchronization within the cortico-BG circuitry (Bergman etal., 1998; Hurtado et al., 1999; Levy et al., 2000; Raz et al.,2000; Brown et al., 2001; Marsden et al., 2001). Collectively,these studies suggest a loss of functional segregation among parallelcorticobasal ganglia circuits (Alexander et al., 1986; DeLong,1990), leading to loss of neuronal specificity in response topassive joint manipulation (Filion et al., 1988; Boraud et al.,2000). We too found a decrease in MI specificity after MPTP inboth the number and strength of the responses to passive arm manipulation;however, we failed to reveal a loss of specificity in GPe. Ourability to detect the changes only in MI but not in GPe probablyhad to do with the weaker modulation of pallidal activity in responseto passive limb movements relative toMI.

Previous multiple-electrode primate studies found abnormal oscillatory synchronization among the tonically active neuronsof the striatum (Raz et al., 1996) and among pallidal neurons(Nini et al., 1995; Raz et al., 2000). The temporal width of thispathological synchronization is on the order of tens to hundredsof milliseconds, similar to what we observed among the striatalneurons of monkey S (Fig. 12B); however, we did not find such synchronousoscillations in our pallidal recording. The salient differencebetween the animals of the previous studies and monkey S is thatthe latter exhibited no tremor. Thus, it is possible that oscillatorycorrelation in GP appears only in tremulous primates. This suggestionis in line with a recent study of the subthalamic nucleus in PDpatients that found oscillatory activity and high-frequency synchronizationonly among neurons of tremulous patients and not among those ofnontremulous ones (Levy et al., 2000). Still, we see that evenin akinetic monkey S striatal neurons display oscillatory synchronizationafter MPTP, indicating that enhanced synchrony and loss of neuronalspecificity in cortico-BG circuits is not only a property of tremuloussubjects (Brown et al., 2001; Marsden et al., 2001). In summary,our findings that (1) the pathological MI synchrony is on a largertimescale than that found in the BG and that (2) GPe neurons inmonkey S remain uncorrelated after MPTP indicate that corticalsynchrony cannot result simply from BG dynamics. It thereforeseems that parkinsonian MI synchrony represents an intrinsic reorganizationof cortical dynamics in response to the MPTP insult. The depletionof dopamine in frontal cortex or in the thalamus (Freeman et al.,2001) in response to this insult may play a role in thisreorganization.

The relationship between MI activity and movement

Surface EMG detects transient changes in muscle activation; however, during the MI bursts in the MPTP state, we found no suchtransients in the EMG recording from monkey Z. Similarly, theaccelerometer traces from both monkeys indicated that these burstselicited no movement. This is surprising because similar populationbursts in the normal monkeys usually appeared with movement (Fig.4). A faulty corticospinal transmission, as may be indicated bythe increased mean ICMS threshold current in monkey Z, could resolvethis paradox. However, because ICMS threshold currents were oftenquite low (well below 50 µA) (Murthy and Fetz, 1996; Tokuno andNambu, 2000) in the MPTP state of monkey Z and because in monkeyS there was no change in ICMS threshold currents, our opinionis that cortical micro-excitability was not dramatically affectedby the MPTP. This is in line with human studies showing that thecorticospinal motor pathway remains intact in parkinsonism (Dicket al., 1984; Ridding et al., 1995; Rothwell, 1999; Kleine etal., 2001). The ability of EMG to detect changes in "baseline"muscle tone (in contrast to transient activations) is questionable.Still, we hypothesize that the excessive MI synchronization mayunderlie muscle rigidity by causing a persistent co-contractionof antagonistic muscles that may result in the observed rigidity(Goldberg et al., 2002). Alternatively, changes in BG activityin parkinsonism may induce changes in the activity of descendingpathway structures, such as the pedunculopontine nucleus (Munro-Davieset al., 1999; Pahapill and Lozano, 2000), whose influence on thespinal cord may shunt the corticalbursts.

A possible decoupling of MI discharge and movement has been described in previous single-unit studies (Evarts, 1964; Muirand Lemon, 1983; Carpenter et al., 1999). It was suggested thatthis decoupling may result from insufficient synchronous activityin MI (Phillips and Porter, 1977). Our multiple electrode resultsdemonstrate that even robust synchronous activation of MI neednot result inmovement.

Clinical implications

Although the current physiological model of the basal ganglia circuitry has been invaluable for the development of neurosurgicaltherapies of PD (Gross et al., 1999), it has become the targetof much criticism (Marsden and Obeso, 1994; Obeso et al., 2000;Vitek and Giroux, 2000). Our findings reveal yet another oversightof the model regarding motor cortical involvement in parkinsonism.However, they raise the possibility that noninvasive transcranialtherapies aimed at the disruption of pathological synchronizationin MI could some day ameliorate PDsymptoms.

  FOOTNOTES

Received Jan. 16, 2002; revised March 5, 2002; accepted March 5, 2002.

This research was supported in part by the Israel Science Foundation, which was founded by the Israel Academy of Sciencesand Humanities, and by the United States-Israel Binational ScienceFoundation. J.A.G. is supported by the Yeshaya Horowitz Association.T.B. is supported by the European Community Marie Curie fellowship.V. Sharkansky provided technical support. We thank G. Goelmanfor conducting the MRI, M. Abeles and T. Wichmann for their criticalreading of a previous version of this manuscript, and D. Jaegerfor his helpfulsuggestions.

Correspondence should be addressed to Joshua A. Goldberg, Department of Physiology, The Hebrew University-Hadassah MedicalSchool, P.O. 12272, Jerusalem 91120, Israel. E-mail: joshg{at}md.huji.ac.il.

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MATERIALS AND METHODS
RESULTS
DISCUSSION
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