Cortical Slow Oscillatory Activity Is Reflected in the Membrane Potential and Spike Trains of Striatal Neurons in Rats with Chronic Nigrostriatal Lesions

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The Journal of Neuroscience, August 15, 2001, 21(16):6430-6439

Cortical Slow Oscillatory Activity Is Reflected in the Membrane Potential and Spike Trains of Striatal Neurons in Rats with Chronic Nigrostriatal Lesions
Kuei Y. Tseng, Fernando Kasanetz, Lucila Kargieman, Luis A. Riquelme, and M. Gustavo Murer
Departamento de Fisiología, Facultad de Medicina, Universidad de Buenos Aires, Paraguay 2155, Buenos Aires 1121, Argentina

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurons in the basal ganglia output nuclei display rhythmic burst firing after chronic nigrostriatal lesions. The thalamocorticalnetwork is a strong endogenous generator of oscillatory activity,and the striatum receives a massive projection from the cerebralcortex. Actually, the membrane potential of striatal projectionneurons displays periodic shifts between a very negative restingpotential (down state) and depolarizing plateaus (up states) duringwhich they can fire action potentials. We hypothesized that anincreased excitability of striatal neurons may allow transmissionof cortical slow rhythms through the striatum to the remainingbasal ganglia in experimental parkinsonism. In vivo intracellularrecordings revealed that striatal projection neurons from ratswith chronic nigrostriatal lesions had a more depolarized membranepotential during both the down and up states and an increasedfiring probability during the up events. Furthermore, lesionedrats had significantly fewer silent neurons than control rats.Simultaneous recordings of the frontal electrocorticogram andmembrane potential of striatal projection neurons revealed thatthe signals were oscillating synchronously in the frequency range0.4-2 Hz, both in control rats and rats with chronic nigrostriatallesions. Spreading of the slow cortical rhythm is limited by thevery low firing probability of control rat neurons, but a slowoscillation is well reflected in spike trains of ~60% of lesionedrat neurons. These findings provide in vivo evidence for a roleof dopamine in controlling the flow of cortical activity throughthe striatum and may be of outstanding relevance for understandingthe pathophysiology of Parkinson'sdisease.

Key words: striatum; cerebral cortex; dopamine; in vivo intracellular recording; Parkinson's disease; neuronal firing patterns

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It is conventionally accepted that a substantial part of the influence of dopamine (DA) on sensorimotor and cognitive functionsis related to its modulatory effects on striatal processing ofcortical input (Albin et al., 1989; Hollerman et al., 2000). Dopamineinputs from the substantia nigra converge with glutamatergic inputsfrom the cerebral cortex at the dendrites of striatal projectionneurons (Smith et al., 1998), which are called "medium spiny neurons"(MSNs). In vivo intracellular recordings from MSNs revealed thattheir membrane potential alternates between two steady-state values.A very polarized resting potential ("down state") is interruptedby periods of sustained depolarization ("up states") lasting afew hundred milliseconds (Wilson and Groves, 1981; Calabresi etal., 1990; Wilson, 1993). There is evidence supporting the theorythat the up events are driven by excitatory inputs from the cerebralcortex and thalamus (Wilson et al., 1983; Wilson 1993; Plenz andAertsen, 1996). In vitro studies indicate that the ionic conductancesshaping the fluctuating membrane potential of MSNs are modulatedby DA (Nicola et al., 2000). The up events are currently perceivedas "enabling states," during which synchronously depolarized MSNstranslate afferent activity into sequences of action potentials,allowing transmission of information to structures receiving striatalprojections (Wilson, 1993; O'Donnell and Grace, 1995).

Extracellular single unit recordings established that after nigrostriatal system lesions, the firing pattern of neurons innuclei receiving strong striatal innervation, like the globuspallidus (GP) and substantia nigra pars reticulata (SNpr), shiftsfrom a regular pattern to a rhythmic burst firing mode (Pan andWalters, 1988; MacLeod et al., 1990; Murer et al., 1997; Ni etal., 2000). Recent studies from our laboratory indicate that asmuch as 40% of SNpr units recorded from 6-hydroxydopamine (6-OHDA)-lesionedrats display rhythmic ~1 Hz firing rate modulations (Tseng etal., 2001). Our findings showing a strong modulatory effect ofintrastriatally administered DA receptor agonists on the firingpattern of SNpr units in 6-OHDA-lesioned rats support a role ofthe striatum in the genesis of this phenomenon (Tseng et al.,2000). Interestingly, it has been reported that the membrane potentialfluctuations of MSNs display a weak periodicity, also with a frequencyof ~1 Hz (Stern et al., 1997). In slow wave sleep and anesthesia,rhythmic modulations of firing rate occur in neurons throughoutthe cerebral cortex and thalamus. Rhythmic activity of the thalamocorticalnetwork is reflected in the electroencephalogram (EEG) of animalsand humans as oscillations of different frequencies (includinga slow ~1 Hz oscillation) that are synchronized over widespreadareas of the cerebral cortex (Steriade, 1999). Therefore, we hypothesizedthat an altered functional state of striatal projection neuronsmay facilitate the transmission of slow cortical rhythms to thebasal ganglia output nuclei in experimental parkinsonism. In thismanuscript, we report the existence of a strong correlation betweencortical slow rhythmic activity and membrane potential fluctuationsof striatal neurons. Furthermore, we describe modifications inthe membrane potential of striatal neurons from 6-OHDA-lesionedrats that may allow transmission of slow cortical rhythms towardbasal ganglia output nuclei in experimentalparkinsonism.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Male adult Sprague Dawley rats, weighing 190-220 gm, were randomly assigned to receive a 6-OHDA lesion or a sham lesion. Theanimals were maintained on a 12 hr light/dark cycle with foodand tap water available ad libitum until the time of the experiment.In vivo intracellular recordings of striatal neurons were performed6-10 weeks after thelesion.

Lesions. A severe unilateral lesion of mesencephalic dopaminergic neurons was obtained with the neurotoxin 6-OHDA hydrobromide(Sigma, St. Louis, MO), as reported previously (Murer et al.,1997). Briefly, the rats were anesthetized with pentobarbital(50 mg/kg, i.p.), and with the aid of a stereotaxic instrument(David Kopf Instruments, Tujunga, CA), they were injected withthe neurotoxin (8 µg free base in 4 µl of 0.1% ascorbic acid)at the medial forebrain bundle (stereotaxic coordinates: anterior(A), $-$ 4.3 from bregma; lateral (L), 1.6; H, 8.3 below the corticalsurface) (Paxinos and Watson, 1997). The control group receivedonly the ascorbic acid solution. The effectiveness of the lesionwas evaluated with the stepping test (Olsson et al., 1995; Changet al., 1999) and further confirmed postmortem by means of immunohistochemistry(Murer et al., 1997). The stepping test was repeated three timesbetween days 15 and 20 after surgery in all the rats. Only those6-OHDA-lesioned rats that showed less than two adjusting stepswith the forelimb contralateral to the lesion during each trialwere selected for the experiments (see Fig. 1).

Electrophysiological recordings. The rats were anesthetized with urethane (1.2 gm/kg, i.p.), treated with a local anestheticon the scalp and pressure points, and secured to the stereotaxicframe. Temperature was maintained between 36 and 37°C with a heatingpad. Additional urethane was administered throughout the experimentas necessary to maintain a constant level of anesthesia, as determinedby testing the hindlimb compression reflex, and electrocorticographicrecordings when available (customarily, supplements of 0.4 gm/kg,s.c., every 3-4hr).

A concentric bipolar stimulating electrode (SNE-100; Better Hospital Equipment, Rockville Centre, NY) was placed in the frontalcortex (A, 3 mm anterior to the bregma; L, 1.5 mm; and H, 2.5mm below the cortical surface) (Paxinos and Watson, 1997) to allowdelivery of 300 µsec square wave pulses, 300-500 µA in amplitude(10-15 pulses at 0.5 Hz). In many experiments, an additional concentricbipolar electrode was located 1 mm lateral to the stimulatingelectrode, with the tip inserted ~1.5 mm below the cortical surface,to obtain a differential recording of the electrocorticogram (ECoG).The cortical signal was filtered (0.1-300 Hz), amplified (ER-98;NeuroData, Delaware Water Gap, PA), and sent to an A/D converter(DigiData 1200; Axon Instruments, Foster City,CA).

Intracellular recordings were obtained from a striatal region located 1.0 mm anterior to bregma, 2.5-3.0 mm lateral to themidline, and 3.0-5.0 mm below the cortical surface (Paxinos andWatson, 1997). The microelectrodes were pulled (Rhema-Labortechnikmicroelectrode puller; Campden Instruments, Loughborough, UK)from 1.2 mm outer diameter borosilicate glass capillaries (WPI,Sarasota, FL) and filled with 2 M K-acetate and 2% Neurobiotin(Research Biochemicals, Natick, MA); they had resistances rangingfrom 60 to 130 M $Omega$ . The recorded signal was sent to a conventionalbridge amplifier (IR-283; NeuroData) and to the A/D converter.The microelectrode was advanced with a hydraulic micromanipulatorthrough the cortex up to the striatum (2.5-3 mm below the corticalsurface), while continuously measuring electrode resistance bypassing 0.5 nA, 100 msec current pulses. The microelectrode wasleft in place for 20-30 min and then slowly advanced through thestriatum until a neuron was impaled. Recordings had to fulfillall of the following criteria to be included in the study: (1)resting membrane potential of at least $-$ 55 mV; (2) action potentialamplitude >45 mV measured from threshold and duration inferiorto 1 msec measured at half maximal amplitude; and (3) input resistance>20 M $Omega$ . All of these parameters had to remain stable for at least10 min (without any hyperpolarizing current). Input resistancewas estimated from the membrane potential measured 80-90 msecafter the onset of small amplitude hyperpolarizing or depolarizing(subthreshold) current pulses. Ordinarily, several epochs of spontaneousactivity lasting 1-2 min could be recorded, and the activity evokedby cortical stimulation could be evaluated at least twice at intervalsof 5-10 min. All signals were acquired with Axoscope 1.1 (AxonInstruments) at a sampling rate of 10kHz.

After completion of the experimental manipulations, we attempted to label the neurons with Neurobiotin by passing 1 nA, 300msec positive current pulses at a frequency of 2 Hz for at least20 min (Kita and Armstrong, 1991). The rats were transcardiallyperfused with cold saline, followed by 4% paraformaldehyde inPBS. The brain was removed, stored overnight in the same fixative,and then incubated in PBS containing 15% sucrose for 24hr.

Tissue processing. Serial 40-µm-thick coronal sections were obtained from the entire forebrain and mesencephalon. The localizationof the extracellular recording sites was determined from Nissl-stainedsections. Neurobiotin was revealed after a slightly modified versionof the protocol of Kita and Armstrong (1991). Briefly, the sectionswere incubated for 4 hr in 0.1 M PBS containing an avidin-biotin-peroxidasecomplex (1/100, Vectastain Elite ABC kit; Vector Laboratories,Burlingame, CA) and 0.3% Triton X-100, washed in 0.1 M PBS, andincubated for 5-10 min in 0.05 M sodium acetate containing 0.5mg/ml 3,3'-diaminobenzidine (Sigma), 0.8 mg/ml ammonium nickelsulfate, and 0.2 µl/ml H₂O₂. Tyrosine-hydroxylase (TH) immunohistochemistrywas performed on free-floating sections following a publishedprotocol (Murer et al., 1997).

Analysis of membrane potential fluctuations and firing pattern of striatal neurons. For all the neurons included in the study,at least two 1 min signal segments of basal activity were analyzed.Sampling was reduced to 1000 Hz by using the substitute averagemodule of Axoscope. The signal was browsed to select epochs showinga clear two-state membrane potential. These epochs were used toconstruct histograms displaying the amount of time spent at anygiven membrane potential (all-points histograms, pClamp 6; AxonInstruments). For most recorded neurons, the histogram showeda clear bimodal profile fitting to a dual-Gaussian function (seeFig. 2). Fitting was performed with the Levenberg-Marquart methodof nonlinear least squares (pClamp 6; Axon Instruments) (Sternet al., 1997). The voltage corresponding to the minimum reachedby the function amid its peaks was used to estimate the time ofstate transitions in the signal. The time spent in the up anddown states was estimated with custom-made software that recordsa state each time that voltage remains for >100 msec below orabove the selected transitional value. This approach was preferredto the alternative of estimating time spent in the lower and uppervoltage ranges of the distribution directly from the histogram,because the duration of individual states probably influencesdistinctively the activity of voltage-sensitive ionic conductancesand firing probability (Nicola et al., 2000). The mode insideeach of the two resulting series of voltage values was consideredto represent the steady state reached during the down and upstates.

Spectral analysis was used to characterize the periodic components in the membrane potential of striatal neurons. Spectrawere computed from 1 min segments of signal (down-sampled to 1000Hz), yielding a spectral resolution of 0.017 Hz. For the spontaneouslyactive neurons, smoothing with a 20 points moving average wasused to truncate the action potentials before performing the fastFourier transform (FFT). Spectral densities were obtained usinga Hamming window (width, 5). Relative power was calculated bynormalization to the total power within the frequency range 0.017-10Hz (the power of frequencies above 10 Hz was negligible). Peaksexceeding the 95% confidence interval of the mean relative spectralpower were consideredsignificant.

Neurons that did not spontaneously fire any action potential during the recording period were considered "silent." For thespiking neurons, the number of up states yielding at least oneaction potential was determined. Interspike interval (ISI) streamswere obtained from the intracellular recordings by means of amplitudediscrimination. Autocorrelograms were computed from 1 min segmentsof signal using 10 msec bins over 1000 bins (yielding a totallag of 10 sec). The autocorrelograms were smoothed using a movingaverage method and then subjected to an FFT, yielding power spectrawith 0.1 Hz resolution. Because the purpose of the analysis wasto determine whether an ~1 Hz rhythm can be retrieved from thespike trains of individual striatal neurons, this analysis wasonly performed on cells firing at rates >1Hz.

Several measures were performed on the responses induced by cortical stimulation, including the time from the beginning ofthe stimulus artifact to the peak of the fast depolarizing postsynapticpotential (dPSP), the voltage at the peak of the fast dPSP, andthe duration and amplitude of the long-lasting hyperpolarizingand depolarizing changes that follow the fast dPSP (Wilson, 1993).The same rationale that was applied to the analysis of naturallyoccurring fluctuations in membrane potential was used to examinethe long-lasting changes evoked by cortical stimulation. The voltagechosen to establish the occurrence of spontaneous state transitionsin the signal was used to define the beginning and end of thelong-lasting changes that were evoked by cortical stimulation.The segments of signal including the long-lasting responses werecut off and used to construct histograms of the frequencies distributionof membrane potential, which showed bimodal profiles. The modeinside each part of the frequencies distribution of voltage valueswas considered to represent the steady state that was reachedduring the long-lasting hyperpolarizing and depolarizing phasesof theresponse.

Analysis of the simultaneously acquired ECoG and striatal recordings. For each ECoG-intracellular recording pair, at leastthree disjoined 30 sec epochs (typically 4-6) were studied. Samplingwas reduced to 1000 Hz as described above, and the signals werestandardized. Cross-correlograms were computed for delays of 3sec with a resolution of 3 msec. Peaks exceeding three correlatedwhite noise SEs were considered significant. Cross-correlationanalysis allowed estimation of the phase shift between the signals(time lag of the highest peak) and the frequency of the dominantcoincident oscillatory activity (the reciprocal of the time betweentwo successive peaks) (Lopes da Silva et al., 1989). The similarityin the oscillatory frequency content of the signals was furtherevaluated using spectral analysis and coherence estimation (Lopesda Silva et al., 1989). Power spectra were computed as describedabove (resolution for 30 sec signal segments = 0.033 Hz). Coherencewas calculated from the cross-spectral density between the twosignals normalized by the spectral density of each signal. Coherenceattains its highest value when the phase shift and ratio betweenthe amplitudes of the two waveforms remains constant. A significantcoherence (>0.75 in at least three disjoined 30 sec signal segments)(Rosenberg et al., 1989) at the dominant frequency of the cross-spectrum,was accepted as an indication of a high probability of oscillatorysynchronization and allowed estimation of the phase relationshipbetween the signals. Phase lags were calculated from portionsof the phase spectrum encompassing the frequencies showing a significantcoherence and a linear phase relationship between the signals(Lopes da Silva et al., 1989). Time series analysis was performedusing Statistica 4.2 (Statsoft Inc., Tulsa, OK). Because the ECoGwas high-pass filtered at 0.1 Hz, the time lags were correctedusing a series of coefficients that were derived from measurementsof the phase lag introduced by the filter to digitally generatedsinusoidal waveforms (with a 0.1 Hzresolution).

Statistical comparisons. The Fisher exact probability test was used to evaluate the relationship between two dichotomous variables.The Student's t test was used for two-group comparisons involvinga single continuous variable. If the data were not normally distributed,or had unequal variances, the Mann-Whitney U test was used insteadof the t test. Normality was assessed with the Kolmogorov-Smirnovtest, and homogeneity of variances was assessed with Levene'stest. To compare sham-lesioned and 6-OHDA-lesioned rats alongtwo or more variables, ANOVA was used. The Kruskal-Wallis ANOVAby ranks was preferred for multiple comparisons involving interrelatedproportions.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effects of 6-OHDA-induced lesions on the membrane potential of striatal neurons

In vivo intracellular recordings were obtained from 27 striatal neurons from 21 sham-lesioned rats and 31 striatal neuronsfrom 24 6-OHDA-lesioned rats. All neurons successfully injectedwith Neurobiotin were identified as MSNs (Fig. 1). Among the sevensuccessful Neurobiotin injections performed in control rats, allled to the labeling of a single spiny neuron. In contrast, 7 amongthe 11 successful Neurobiotin injections performed in 6-OHDA-lesionedrats revealed two labeled spiny neurons (p = 0.013, Fisher exacttest). An increased probability of labeling more than one striatalneuron after a single intracellular Neurobiotin injection in ratswith chronic nigrostriatal lesions has been reported by others(Cepeda et al., 1989; Onn and Grace, 1999) and was suggested toreflect increased "coupling" via gap junctions. Neurons recordedfrom control and 6-OHDA-lesioned rats did not differ in some oftheir basic electrophysiological parameters, like input resistance,firing threshold, and action potential duration and amplitude(Table 1).

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Figure 1. A, B, Coronal sections of the forebrain immunolabeled with antibodies directed against tyrosine hydroxylase. The microphotographs depict the typical aspect of the striatum in sham-lesioned (A) and 6-OHDA-lesioned (B) rats. Scale bar, 1.5 mm. C, The behavioral effect of the lesion was evaluated with the "stepping test." The 6-OHDA-lesioned rats had a significant impairment in the test (p < 0.001; main group effect in a two-way ANOVA) involving both the contralateral forelimb (** p < 0.05; Tukey's test) and, although in a smaller degree, the ipsilateral forelimb (* p < 0.05; Tukey's test). D, Schematic diagram showing the placement of the concentric bipolar electrodes used to record the electrocorticogram (lateral electrode) and to stimulate the frontal cortex (medial electrode). Scale bar, 1.2 mm. E, F, All the neurons that were successfully injected with Neurobiotin had the typical morphology of striatal medium spiny neurons. In sham-lesioned rats, all injections yielded a single labeled cell (E), whereas in 6-OHDA-lesioned rats, ~60% of the injections yielded two neurons (F). Insets, Segments of dendrites showing spines. Scale bar, 25 µm. ECoG, Electrocorticogram; FCx-S, frontal cortex stimulation; C, contralateral; I, ipsilateral.


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Table 1. Electrophysiological properties of intracellularly recorded striatal neurons in control and 6-hydroxydopamine-lesioned rats

Twenty-two neurons in the control group and 23 in the 6-OHDA-lesioned group showed a fluctuating membrane potential (Fig.2). The membrane potential fluctuations differed between groups(Table 1) (Fig. 3). The voltage during both the down and up stateswas significantly more depolarized in 6-OHDA-lesioned rats thancontrol rats. Considering that up events are perceived as enablingstates during which MSNs can fire action potentials (Wilson, 1993;O'Donnell and Grace, 1995), the above described alterations probablyunderlie the increased firing rates reported for striatal singleunits in 6-OHDA-lesioned rats (Arbuthnott, 1974; Schultz, 1982;Nisenbaum et al., 1986). Actually, for the spontaneously activeneurons, the probability of firing at least one action potentialduring an up state was significantly higher in 6-OHDA-lesionedthan control rats (Fig. 4). Furthermore, striatal neurons from6-OHDA-lesioned rats spent significantly less time in the downstate and required more time to shift from one state to the other(Fig. 3). The contrast between the experimental groups is furtheremphasized by the finding that control rats had a significantlyhigher proportion of silent neurons than 6-OHDA-lesioned rats(Table 1).

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Figure 2. Representative recordings of striatal neurons from sham-lesioned rats (top trace) and 6-OHDA-lesioned rats (bottom trace). In both experimental groups, most neurons had a fluctuating membrane potential. Histograms depicting the time spent at any given membrane potential typically had bimodal profiles with the distributions fitting dual-Gaussian functions.

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Figure 3. Sham-lesioned and 6-OHDA-lesioned rats differed in several measurements related to their two-state membrane potential. Top, The membrane potential was more depolarized during both the down states (*p = 0.027) and up states (*p = 0.004; two-tailed Student's t test) in rats with nigrostriatal lesions. The box-plots include data from both silent and active neurons. Median (black line), 25th and 75th percentiles (bar limits), 10th and 90th percentiles (error bars), and outliers (black circles) are shown. Bottom left, Down states were shorter in 6-OHDA-lesioned rats (*p < 0.001; two-tailed Student's t test). The duration of the up events was not significantly different between groups. Bottom right, In a given time window, neurons from 6-OHDA-lesioned rats spent a smaller proportion of time in the down state (*p = 0.0044; ANOVA by ranks) and a higher proportion of time shifting from one state to the next (fluctuating around the transitional voltage or reaching short-lived steady states) (NUD) (*p = 0.011, ANOVA by ranks). There was a trend toward an increased proportion of time spent in the up state that did not reach statistical significance (*p = 0.10; ANOVA by ranks).

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Figure 4. Box-plots summarizing information regarding the firing rate and firing probability of striatal neurons. Median (black line), 25th and 75th percentiles (bar limits), 10th and 90th percentiles (error bars), and outliers (black circles) are shown. Left, Seventy-five percent of the spontaneously active neurons recorded from 6-OHDA-lesioned rats had firing rates >3 Hz, whereas 75% of the spontaneously active neurons recorded from control rats had rates <3 Hz (*p = 0.002; Mann-Whitney U test). Right, The spontaneously active neurons recorded from control rats had a significantly lower probability of firing at least one spike during an up event than those recorded from rats with nigrostriatal lesions (*p = 0.011; Mann-Whitney U test).

Spectral analysis of the membrane potential of bistable-like neurons revealed that >90% of the spectral power was concentratedin the frequency range comprised between 0.4-2 Hz (Table 2; seeFigs. 6 and 7). All two-state neurons had peaks within this frequencyrange that largely exceeded the 95% confidence interval of themean relative spectral power. Note that for spontaneously activeneurons the action potentials have been truncated before performingthe FFT. Consequently, spectral profiles reflect true membranepotential frequency components. State transitions probably explainmost of the spectral power within this frequency range (Sternet al., 1997). The frequency of state transitions, as estimatedfrom counts performed on the same signal segments, was 0.95 ±0.05 in control rats and 1.03 ± 0.07 in 6-OHDA-lesioned rats (p= 0.34, two-tailed t test).


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Table 2. Characterization of the response of intracellularly recorded striatal neurons to cortical stimulation in control and 6-hydroxydopamine-lesioned rats

For five neurons in the control group and eight in the 6-OHDA-lesion group, it was not possible to ascertain the existenceof a two-state membrane potential. The small number of this kindof recordings in our sample prevented the investigation of betweengroupsdifferences.

Response of striatal neurons to cortical stimulation

As reported previously (for review, see Wilson, 1993), cortical stimulation evoked a short latency dPSP, followed by a sequenceconsisting of a prolonged hyperpolarization and a plateau depolarization.The latter sequence closely resembled the spontaneous membranepotential shifts of striatal neurons (Fig. 5). Although the shortlatency dPSP is probably produced by activation of a small volumeof cortical tissue around the electrode tip, the hyperpolarization-depolarizationsequence is probably driven by a hypersynchronous cortical oscillatorycycle that indicates resumption of the endogenously generatedrhythm (Wilson, 1993). After a single pulse applied to a corticalarea, neighbor cortical neurons display a short latency dPSP,followed by a long-lasting inhibition and a postinhibitory depolarizingplateau (Amzica and Steriade, 1998); the shape and time courseof this response closely resembles that of striatal neurons.

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Figure 5. Typical examples of the response evoked by cortical stimulation in sham-lesioned (top) and 6-OHDA-lesioned rats (bottom). Several events were superimposed in each graphic. Note the shorter latency of the depolarizing plateau and the more depolarized membrane potential during the hyperpolarizing phase of the response in the 6-OHDA-lesioned rats.

The shape of the response of striatal neurons to cortical stimulation, time to the peak of the fast dPSP, and peak amplitudeof the fast dPSP were similar in both experimental groups (Table2). In agreement with the results reported above regarding naturallyoccurring state transitions in the signal, the long-lasting hyperpolarizationwas shorter and had a more depolarized potential in 6-OHDA-lesionedrats than in control rats (Fig. 5). The plateau depolarizationhad a significantly reduced latency and reached a slightly moredepolarized potential (the difference between groups was not significant)in 6-OHDA-lesioned rats (Table 2).

A low-frequency oscillation is encoded in spike trains of striatal neurons

Most striatal neurons show very low mean firing rates (many are silent) in control rats, but in 6-OHDA-lesioned rats theirfiring rates are significantly increased (Arbuthnott, 1974; Schultz,1982; Nisenbaum et al., 1986) (Fig. 4). Because striatal neuronsfire action potentials during the up states, and the probabilityof firing at least one spike during an up state is increased in6-OHDA-lesioned rats, it seemed likely that the slow membranepotential fluctuation would be transmitted more effectively tostriatal target nuclei in rats with nigrostriatal lesions. Toprovide evidence in support of this hypothesis, we sought forlow-frequency oscillations in spike trains of striatal neuronsrecorded from control and 6-OHDA-lesioned rats. Only those cellshaving firing rates higher than 1 spike per second were analyzed(Fig. 4). A significant ~1 Hz periodic frequency component couldbe retrieved from 4 of 22 control rat recordings (14.8% of thesampled neurons) and from 15 of 23 6-OHDA-lesioned rat recordings(67.7% of the sample) (p = 0.0023, Fisher exact test) (see Fig.7).

Correlation between the ECoG and the membrane potential of striatal neurons

Intracellular recordings of two-state striatal neurons were obtained simultaneously with the frontal cortex ECoG in 14 instancesfrom 12 control rats, and in 16 instances from 13 6-OHDA-lesionedrats. For 13 signal pairs in the control group and 12 in the 6-OHDA-lesionedgroup, clear signs of synchronized oscillation were found. Inboth experimental groups, the power spectra of the signals revealedthat the ECoG and the membrane potential of the simultaneouslyrecorded striatal neuron had the highest relative power at a closelysimilar frequency, usually in the 0.4-2 Hz range (Figs. 6, 7).The signals had a very strong coherence at the dominant spectralfrequency, suggesting that the waveforms were oscillating synchronously.The experimental groups did not differ in the mean coherence atthe dominant frequency or in the phase relationship between theECoG and intracellular recording (Table 3). Phase lags, estimatedat the coherent frequency, ranged from $-$ 155 to +72 msec (negativemeans that the ECoG precedes the striatal recording), with theECoG anteceding the intracellular signal in 15 of 25 instances(Table 3). Similarly, the cross-correlograms revealed a strongcorrelation between the ECoG and membrane potential fluctuationsof striatal neurons (Fig. 6). Lags between the signals, estimatedfrom the cross-correlograms, were consistent with those calculatedfrom the phase spectra (Table 3). The close relationship betweenthe signals was consistently retained over time, as indicatedby the analysis of several nonoverlapping 30 sec epochs withintime windows spanning several minutes (Fig. 6). For the remainingfive signal pairs, a close relationship between the ECoG and intracellularrecording could not be evidenced, i.e., they correlated weaklyand showed low coherence.

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Figure 6. Visual inspection of simultaneous recordings of the frontal electrocorticogram and the membrane potential of striatal neurons indicated that the two waveforms were oscillating synchronously at ~1 Hz. The signals are displayed as they were recorded, but note that they were down-sampled, smoothed, and standardized before analysis. The belief that the signals were synchronized was substantiated through the analysis of cross-correlograms and by means of coherence analysis. Each row of graphics shows the cross-correlogram, cross-spectrum, coherence spectrum, and phase-spectrum corresponding to the signal pairs displayed in the upper part of the figure (top row of graphics, sham-lesioned rat; bottom row of graphics, rat with nigrostriatal lesion). In each graphic, the results of the analysis of several 30 sec epochs from the same signal pair were superimposed. The four disjoined 30 sec epochs depicted for the sham-lesioned rat were chosen from a recording session elapsing 15 min. A 12 min recording session from a 6-OHDA-lesioned rat provided the three 30 sec epochs that were chosen for the bottom row of graphics. Both signal pairs showed strong correlations. The cross-spectra revealed a powerful common frequency component of ~0.7 Hz (SHAM) or ~0.9 Hz (6-OHDA), and the signals displayed a very high coherence and a lineal phase relationship at the dominant frequency.

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Figure 7. Each column depicts the power spectra of the electrocorticogram (ECoG), membrane potential (Vm), and spike trains of all the well correlated signal pairs recorded from sham (n = 13) and 6-OHDA-lesioned (n = 12) rats. The insets are averages of all the spectra contained in the corresponding graphic. Only one neuron in the pairs recorded from sham-lesioned rats displayed enough spontaneous discharge (>1 Hz) to compute its spike train spectrum. For 6-OHDA-lesioned rats, ~70% of these recordings showed firing rates higher than ~1 Hz.


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Table 3. Summary of the analysis of simultaneous recordings from the membrane potential of striatal neurons and frontal cortex electrocorticogram

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Membrane potential fluctuations of striatal neurons are correlated with slow oscillatory activity in the frontal cortex electrocorticogram

In slow wave sleep and anesthesia, the EEG of animals and humans displays synchronized oscillations of different frequencies.A slow oscillation (~1 Hz), which is generated intracortically,seems to be responsible for the grouping of delta waves and spindles,and is a major determinant of the shape of the EEG waveform (Steriade,1999). In vivo intracellular recordings revealed that the membranepotential of cortical neurons shows rhythmic depolarizing andhyperpolarizing shifts that are strongly correlated with the EEGslow oscillatory activity (Amzica and Steriade, 1995). Duringthe depolarizing phase of the membrane potential fluctuation,cortical neurons discharge bursts of action potentials that grantspreading of the rhythm through the cortex and thalamus (Steriade1999). Our simultaneous recordings of striatal neurons and thefrontal ECoG indicate that membrane potential fluctuations reflectspreading of cortical slow rhythms to the striatum. This conclusionis supported by previous findings indicating that up states instriatal neurons are driven by inputs from the cerebral cortex:(1) up states are abolished by decortication (Wilson 1993); (2)striatal neurons do not show up events in slices, but displayup states in chronic organotypic cortex-striatum cocultures (Plenzand Aertsen, 1996); (3) corticostriatal neurons display membranepotential fluctuations that resemble those of striatal neuronsin many aspects, including the presence of common low-frequencycomponents in the power spectra (Stern et al., 1997). Studieson the origin of state transitions in nucleus accumbens spinyneurons are consistent with our results. In the nucleus accumbens,up events are driven by excitatory hippocampal input (O'Donnelland Grace, 1995), and membrane potential fluctuations are correlatedwith shifts in hippocampal field potential (Goto and O'Donnell,2001). Finally, a report by Mahon et al. (2001) indicates thatslow waves in the EEG are correlated with depolarizing statesboth in corticostriatal and striatal neurons under a variety ofanesthetic conditions. It is likely that spreading of slow corticalrhythms to the striatum occurs via the massive corticostriatalpathway. In the present study, the mean time lag between corticaland striatal signals was similar to the latency of the fast dPSPthat was evoked in striatal neurons by corticalstimulation.

Chronic nigrostriatal lesions alter the membrane potential of striatal neurons, allowing transmission of slow cortical oscillations to the basal ganglia output nuclei

Spreading of slow cortical rhythms to striatal target nuclei seems to be limited in healthy animals. Neurons of the GP andSNpr display tonic regular firing during natural slow wave sleep(Datta et al., 1991; Urbain et al., 2000) and anesthesia (Panand Walters, 1988; MacLeod et al., 1990; Murer et al., 1997; Niet al., 2000). After chronic nigrostriatal lesions, SNpr unitsdisplay rhythmic burst firing (MacLeod et al., 1990; Tseng etal., 2000) that is strongly modulated by intrastriatal administrationof DA receptor agonists (Murer et al., 1997; Tseng et al., 2000).The capability of MSNs to transmit slow cortical rhythms to theirtarget nuclei is constrained by their very low firing probabilityin control animals. Our results suggest that after chronic nigrostriatallesions, an increased excitability of striatal neurons allowstransmission of slow cortical rhythms to striatal target nuclei(Figs. 7, 8).

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Figure 8. Postulated mechanism for the generation of rhythmic modulations of firing rate in the basal ganglia output nuclei. The ~1 Hz cortical rhythm is propagated to the striatum, where it produces a rhythmic fluctuation in the membrane potential of striatal projection neurons. During the depolarizing phase of the membrane potential fluctuation, striatal neurons are very close to threshold, but they only rarely discharge action potentials when the nigrostriatal system is intact (left). In animals having chronic nigrostriatal lesions, striatal projection neurons show a more depolarized up state and an increased firing probability (right). These changes may allow transmission of a coarse representation of the cortical rhythm to the striatal target nuclei.

Changes in the shape of the fluctuating membrane potential seem to underlie the increased firing probability of striatal neuronsin 6-OHDA-lesioned rats. Striatal neurons recorded from rats withnigrostriatal lesions displayed a more depolarized membrane potential,during both the down and up states, and spent less time in thedown state. The mechanisms leading to these changes remain tobe determined. Current knowledge suggests that they may be multipleand complex. Dopamine increases potassium currents that keep theresting potential near the potassium equilibrium potential (Pacheco-Canoet al., 1996; Waszczak et al., 1998). A reduced activity of thesecurrents may partly explain the more depolarized membrane potentialand shorter duration of the down state in rats with nigrostriatallesions. Dopamine receptors also modulate in a complex way currentsthat are active within the voltage range reached during the upevents. For example, D2 receptor stimulation suppresses currentsthrough L-type calcium channels and consequently, reduces striatalneuron excitability (Hernández-López et al., 2000). There isin vivo evidence demonstrating that L-type calcium channel blockersreduce glutamate-induced bursts in nucleus accumbens neurons (Cooperand White, 2000). Increased currents through L-type calcium channelsmay have yielded to a more depolarized potential during the upstates, and an increased firing probability, in rats with chronicnigrostriatal lesions. In addition, in vitro evidence supportsthat corticostriatal transmission is increased in slices from6-OHDA-lesioned rats. Striatal neurons do not show spontaneousfiring in control or in DA-depleted slices, but the number andamplitude of spontaneous dPSPs is increased in the DA-denervatedstriatum (Galarraga et al., 1987; Calabresi et al., 1993). Bothpresynaptic and postsynaptic mechanisms (Brown and Arbuthnott,1983; Cepeda et al., 1993; Umemiya and Raymond, 1997) may accountfor the increase in spontaneous corticostriatal transmission afterchronic nigrostriatallesions.

It may be argued that an increased susceptibility to damage induced by the intracellular recording electrode might have producedthe differences in striatal neuronal activity between sham- and6-OHDA-lesioned rats. This possibility seems unlikely, however,because: (1) reports based on extracellular single unit recordingshave demonstrated an increased firing rate of striatal units in6-OHDA-lesioned rats (Arbuthnott, 1974; Schultz, 1982; Nisenbaumet al., 1986); (2) action potential amplitude and duration, inputresistance, and the duration of recordings were not differentbetween control and 6-OHDA-lesioned rats (Table 1); (3) preliminaryresults indicate that the changes in membrane potential inducedby 6-OHDA lesions can be reversed by systemic administration ofdopamine receptor agonists, but not by vehicle injections (ourunpublishedobservations).

Multiple pathways may be involved in the transmission of slow cortical rhythms to the globus pallidus and basal ganglia output nuclei

The striatum is probably not the only structure involved in transmission of slow cortical rhythms to the remaining basal ganglia.Recent work by Magill et al. (2000) demonstrated that slow corticalrhythms are reflected in spike trains of subthalamic nucleus (STN)and GP neurons in ketamine-anesthetized nonlesioned rats and suggestedthat cortical rhythms are propagated via cortico-STN-GP connections.Most GP neurons show tonic regular firing in natural slow wavesleep (Urbain et al., 2000), as well as under the influence ofother anesthetics (Pan and Walters, 1988; Magill et al., 2000;Ni et al., 2000) and in paralyzed animals (Pan and Walters, 1988),however, suggesting that ketamine may propitiate the propagationof slow cortical rhythms through the basal ganglia. After chronicnigrostriatal lesions, GP neurons display rhythmic burst firingin any condition tested (Pan and Walters, 1988; Ni et al., 2000).A role for the STN in spreading cortical rhythms through the basalganglia in the parkinsonian condition is supported by previousreports showing that the proportion of SNpr units displaying rhythmicbursting is reduced to half (Tseng et al., 2000), and rhythmicbursting in the GP is almost abolished (Ni et al., 2000) afterSTN lesions in 6-OHDA-lesionedrats.

Implications for Parkinson's disease

In the awake monkey, basal ganglia output nuclei neurons display nonoscillatory firing patterns. However, after methyl-phenyl-tetrahydropyridine-inducedlesions, a significant proportion of units in the STN and basalganglia output nuclei exhibit an oscillatory pattern of actionpotential firing (Bergman et al., 1994; Nini et al., 1995; Wichmannet al., 1999; Raz et al., 2000). It is becoming increasingly evidentthat a substantial proportion of units in the STN and GP exhibitoscillatory firing in individuals with Parkinson's disease (Hurtadoet al., 1999; Levy et al. 2000; Magnin et al., 2000). The oscillatorybasal ganglia output is supposed to give rise to tremor, one ofthe cardinal signs of the illness. Furthermore, it has been postulatedthat an oscillatory basal ganglia output may disrupt corticalinformation processing by promoting the recruitment of thalamocorticalcircuits in rhythmic firing patterns (Brown and Marsden, 1998).Although the phenomenon resembles what happens in rats after 6-OHDA-inducedlesions, the main frequency of oscillatory activity in behavingparkinsonian primates (3-20 Hz) is higher than that found in anesthetized6-OHDA-lesioned rats (0.4-2 Hz). If abnormal spreading of corticalslow rhythms through the striatum and STN underlies the rhythmicfiring pattern of output nuclei neurons in parkinsonism, the differentoscillatory periods observed in awake parkinsonian primates andanesthetized 6-OHDA-lesioned rats may merely reflect the distinctdominant EEG frequencies that characterize each behavioral state.It seems possible that a population of more excitable striatalneurons will be prone to transfer high-frequency cortical rhythms(like those observed in the cortex during quiet waking) to striataltargets. The reduced latency of the plateau depolarization thatwas evoked by cortical stimulation in 6-OHDA-lesioned rats suggeststhat more excitable striatal neurons can be driven easily to adepolarized (enabling) state. We are not aware of studies aimedat characterizing the oscillatory behavior of basal ganglia neuronsin parkinsonian monkeys during slow wave sleep, nor those of awake6-OHDA-lesioned rats. Undoubtedly, this issue will be clarifiedin the nearfuture.

  FOOTNOTES

Received March 30, 2001; revised May 17, 2001; accepted May 31, 2001.

This work was supported by the Ministerio de Salud y Acción Social de la Nación (Beca Carrillo-Oñativia), Fundación Antorchas,Consejo Nacional de Investigaciones Científicas y Técnicas,y Universidad de Buenos Aires (Argentina). We thank Dr. PatricioO'Donnell for helpful comments on an earlier version of this manuscript,Dr. José L. Ferrán for excellent assistance with microphotographyand artwork, and Departamento de Ciencias Biológicas, Facultadde Ciencias Exactas y Naturales, Universidad de Buenos Aires,for their help with time seriesanalysis.
Correspondence should be addressed to Kuei Y. Tseng, Departamento de Fisiología, Facultad de Medicina, Universidad de BuenosAires, Paraguay 2155, Buenos Aires (1121), Argentina. E-mail:neurofis{at}fmed.uba.ar.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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