Dynamic GABAA Receptor Subtype-Specific Modulation of the Synchrony and Duration of Thalamic Oscillations

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The Journal of Neuroscience, May 1, 2003, 23(9):3649

Dynamic GABA_A Receptor Subtype-Specific Modulation of the Synchrony and Duration of Thalamic Oscillations
Vikaas S. Sohal¹, Ruth Keist², Uwe Rudolph², and John R. Huguenard¹
¹ Department of Neurology and Neurological Sciences, Stanford University Medical Center, Stanford, California 94305-5122, and ² Institute of Pharmacology and Toxicology, University of Zürich, CH-8057 Zürich, Switzerland

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Networks of interconnected inhibitory neurons, such as the thalamic reticular nucleus (TRN), often regulate neural oscillations.Thalamic circuits generate sleep spindles and may contribute tosome forms of generalized absence epilepsy, yet the exact roleof inhibitory connections within the TRN remains controversial.Here, by using mutant mice in which the thalamic effects of theanti-absence drug clonazepam (CZP) are restricted to either relayor reticular nuclei, we show that the enhancement of intra-TRNinhibition is both necessary and sufficient for CZP to suppressevoked oscillations in thalamic slices. Extracellular and intracellularrecordings show that CZP specifically suppresses spikes that occurduring bursts of synchronous firing, and this suppression growsover the course of an oscillation, ultimately shortening thatoscillation. These results not only identify a particular anatomicaland molecular target for anti-absence drug design, but also elucidatea specific dynamic mechanism by which inhibitory networks controlneuraloscillations.

Key words: thalamus; generalized absence epilepsy; spike wave discharge; benzodiazepines; interneuronal network; inhibition

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Interconnected networks of inhibitory neurons regulate oscillations throughout the CNS. One such network, the thalamic reticularnucleus (TRN), participates in many thalamocortical oscillations,including 7-14 Hz sleep spindles and spike-wave seizures characteristicof generalized absence epilepsy. Spindles result from a well studiedcycle of events, in which TRN neurons inhibit thalamocortical(TC) relay neurons, eliciting rebound bursts mediated by T-typecalcium currents, and resulting in re-excitation of TRN (von Krosigket al., 1993). Similar mechanisms may contribute to absence epilepsy.Knocking out the T-type calcium channel gene $alpha$ _1g eliminates reboundbursts in TC neurons, and the resulting mice are resistant todrug-induced spike-wave discharges (Kim et al., 2001). BecauseTRN is the source of the hyperpolarizing input that deinactivatesT-current in TC neurons, this suggests that TRN may be necessaryfor absence seizures. Indeed, TRN lesions abolish spontaneousseizures in a genetic model (Avanzini et al., 1993) and suppressdrug-induced absence seizures (Banerjee and Snead, 1994). Notehowever that cortex alone supports some forms of spike-wave discharge(Steriade and Contreras, 1998).

Thus, intra-TRN inhibition may regulate different thalamic oscillations, and one hypothesis is that it suppresses epileptiformactivity. GABA_A receptor antagonists essentially eliminate intra-TRNinhibition and transform spindles into slower, more synchronizedepileptiform discharges in vitro (von Krosigk et al., 1993; Huguenardand Prince, 1994). A similar transformation follows knockout ofthe $beta$ ₃ subunit of the GABA_A receptor, which selectively disruptsintra-TRN inhibition (Huntsman et al., 1999). Alternatively, intra-TRNinhibition may spread (Bazhenov et al., 1999) or sustain thalamicoscillations (Steriade et al., 1987).

The anti-absence drug clonazepam (CZP) suppresses rhythmic activity in thalamic and thalamocortical slices (Huguenard andPrince, 1994; Zhang et al., 1996), but the locus for this suppressionis unclear, because CZP modulates IPSCs in TRN and TC neurons(Browne et al., 2001), and effects in thalamocortical slices mayreflect cortical actions (Oh et al., 1995). Here we use geneticmanipulations to locate the site of action of CZP and elucidatethe function of intra-TRN inhibition. Mutating one residue renders $alpha$ subunits of the GABA_A receptor insensitive to classical benzodiazepines,including CZP, without affecting their sensitivity to GABA (Wielandet al., 1992; Benson et al., 1998). Within the thalamus, $alpha$ ₁ and $alpha$ ₃ are selectively expressed in the relay and reticular nuclei,respectively (Wisden et al., 1992; Pirker et al., 2000). As aresult, in slices from mice with the $alpha$ ₁(H101R) mutation, 100 nMCZP selectively modulates IPSCs in TRN neurons without affectingTC neurons (Huntsman et al., 2000), whereas in $alpha$ ₃(H126R) mice,CZP selectively modulates IPSCs in TC neurons and has no effectin the TRN (Porcello et al., 2001).

By comparing effects of CZP on oscillations in wild-type (WT), $alpha$ ₁(H101R), and $alpha$ ₃(H126R) mice (Rudolph et al., 1999; Low etal., 2000), we demonstrate that CZP suppresses thalamic oscillationsby enhancing intra-TRN inhibition. CZP specifically suppressessynchronous spikes during rhythmic bursts of population activityand ultimately shortens the duration of oscillations. This identifiesa specific anatomical and molecular target for anti-absence drugdesign and suggests a mechanism for oscillatory control by inhibitorynetworks.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Slice preparation. All procedures involving animals were performed in accordance with protocols approved by the Stanford InstitutionalAnimal Care and Use Committee, and investigators adhered to theguidelines published in the NIH Guide for the Care and Use ofLaboratory Animals. Slices were made as described in Huguenardand Prince (1994). Slices were made from 11-13 d old Sprague Dawley(Simonsen) rat pups and 12-21 d old mouse pups. Animals were deeplyanesthetized with pentobarbital (50 mg/kg) and decapitated. Theirbrains were then rapidly removed and placed in chilled (4°C) slicingsolution consisting of (in mM): 234 sucrose, 11 glucose, 24 NaHCO₃,2.5 KCl, 1.25 NaH₂PO₄, 10 MgSO₄, and 0.5 CaCl, equilibrated witha 95% O₂, 5% CO₂ mixture. Horizontal slices (400 µm) were obtainedusing a Vibratome (TPI, St. Louis, MO). The slices were incubatedin 32°C oxygenated saline for at least 1 hr beforerecording.

Recording procedures. All recordings were made in an interface chamber at 34 ± 1°C. The superfusion solution consisted of(in mM): 126 NaCl, 26 NaHCO₃, 2.5 KCl, 1.25 NaH₂PO₄, 1 or 1.2MgCl₂, 2 CaCl, and 10 glucose. Electrical stimuli were deliveredto the internal capsule through a pair of 50-100 K $Omega$ tungsten electrodes(FHC, Bowdoinham, ME), with a separation of ~100 µm. Clonazepam(obtained from Sigma, St. Louis, MO) was dissolved in DMSO beforebeing added to the final solution, such that the final concentrationof DMSO in the superperfusion solution was $<=$ 0.03%. The concentrationof clonazepam used was always 100 nM, unless noted otherwise.Extracellular multiunit recordings, which also used 50-100 K $Omega$ tungsten electrodes, were normally bandpass filtered between 100Hz and 3kHz.

Intracellular recordings were made with sharp microelectrodes, which were pulled from borosilicate glass (1B100F-4, outerdiameter 1.0 mm, inner diameter 0.58 mm; WPI Inc., Sarasota, FL)using a Flaming Brown Micropipette Puller (P-80, Sutter Instruments,Novato, CA). Sharp electrodes had resistances between 80 and 120M $Omega$ when filled with 4 M KAc and 100 mM KCl. Recordings were amplifiedusing the AxoClamp 2A (Axon Instruments, Union City, CA). We reportresults from TRN neurons that had stable membrane potentials morenegative than $-$ 60mV.

Note that in this and all subsequent sections, we use the terms "oscillation" and "sweep" to refer to the response, recordedby one electrode, to a single stimulus, e.g., a set of spikesoccurring over 1-5 sec. In contrast, a "recording" is the entireset of oscillations recorded from one electrode in different conditions(control, drug application, and drug washout) over tens ofminutes.

Data analysis. To find spikes in extracellular multiunit recordings, we wrote software that detected sufficiently steep negativedeflections followed by sufficiently steep positive deflectionswithin a sufficiently short time window. The threshold for spikedetection was scaled by the root-mean-square of the backgroundnoise in each recording, and the other parameters were set inaccordance with the known properties of action potentials in TRNand TC neurons. Finally, in several cases, output from this spikedetection algorithm was cross-checked against manual inspectionof extracellular recordings to verify that the sensitivity andspecificity of the algorithm were both within reasonablebounds.

To ensure that our observations reflect experimental manipulations rather than nonspecific shifts in excitability, we excludedrecordings in which changes observed during drug application,e.g., shifts of >10% in the total number of spikes per evokedoscillation, did not reverse during the subsequentwash.

The period of an evoked oscillation, recorded from one electrode, was computed from the autocorrelogram of the multiunit spiketrain as follows. First, we counted spikes in 10-msec-wide binsto obtain the spike rate as a function of time (referred to asthe "ratemeter"). The first bin always began 50-100 msec afterthe stimulus to exclude stimulus artifacts and firing induceddirectly by the stimulus (rather than indirectly via intrathalamiccircuitry). Second, we computed the autocorrelogram, A( $tau$ ), ofthe ratemeter, r(t): A( $tau$ ) = $Sigma$ ₀ _t_N r(t+ $tau$ ) r(t),where N is the total number of bins. We excluded autocorrelogramsin which the second tallest peak (referred to as the "satellitepeak" to distinguish it from the tallest peak, which is locatedat $tau$ = 0) was not clearly distinguishable or was located at avalue of $tau$ > 250 msec. Then, we computed the period, T, as: T= $Sigma$ $tau$ [A( $tau$ ) $-$ A₀]/ $Sigma$ A( $tau$ ) $-$ A₀, where the sums are taken over valuesof $tau$ between the troughs on either side of the satellite peak,and A₀ is the mean of the levels of these two troughs. In thisformula, the period is determined from a weighted average takenover the entire area between the troughs on either side of thesatellite peak, rather than from just a single point at the satellitepeak.

We defined the duration of an oscillation as the time at which the last rhythmic burst occurred. A burst was defined as atleast five spikes in two adjoining, 10-msec-wide bins, and tobe classified as "rhythmic," a burst had to occur <400 msec afterthe preceding burst. A sample of durations determined by thisalgorithm were compared with those obtained via manual inspectionand found to besimilar.

We also compared the sizes and shapes of bursts during different conditions: control, CZP application, and CZP washout. Todo this, we first detected bursts during control oscillations.A burst was defined as a local maximum in the ratemeter that wasat least 80 msec after the preceding burst (before detecting maxima,we smoothed the ratemeter so that each point was an average ofthree consecutive 10-msec-wide bins). If we simply wanted to comparethe nth burst in control conditions with the nth burst duringCZP application, we could have detected bursts in this mannerfor each sweep in each different condition. However, on a givensweep, small bursts may or may not occur between larger bursts,making the exact timing of the nth burst highly variable. Suchvariability means that the fourth burst on one particular controlsweep might not really be comparable with the fourth burst ona particular CZP sweep. Therefore, to compare bursts in controlconditions with bursts that occurred at approximately the sametime during oscillations in CZP, we used the following approach.After detecting the nth burst in several consecutive control sweeps,we computed t_n, the average time of occurrence for the nth burst.Then, for each sweep in each condition, we found the local maximumin a 120-msec-wide window centered on t_n and then output the ratemetercentered around the time of this local maximum. We then averagedtogether the recentered ratemeters for all of the control sweepsto obtain a profile of a "control burst" and did the same thingfor CZP sweeps to obtain the "CZP burst,"etc.

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

CZP suppresses evoked thalamic oscillations

In rat thalamic slices, we recorded from TC neurons in the ventrobasal complex (VB) and TRN neurons. A single electrical shockto the internal capsule elicited spindle-like oscillations. Theseoscillations, which could extend across several electrodes inboth VB (22 recordings from nine slices) and TRN (16 recordingsfrom six slices), had frequencies between 4.7 and 8.2 Hz (mean= 6.0 Hz) and lasted 1-5 sec. Figure 1 shows evoked multiunitactivity in one slice (top three recordings from VB; bottom tworecordings from TRN). The evoked oscillation is shown in controlconditions (left), during the application of CZP (middle), andafter drug washout (right). CZP caused suppression of the oscillations,including a shortening of their duration, and this suppressionreversed after washing out CZP. Figure 3 (left) shows the averageamount of CZP-induced suppression in all recordings from rat slices,along with the degree of suppression at various time points duringthe drug washout. The number of spikes during each oscillationwas reduced by 32 ± 6% (mean ± SEM) in TRN (n = 16; p < 0.05)and 36 ± 4% in VB (n = 22; p < 0.001) (Table 1).

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Figure 1. Clonazepam (CZP) reversibly suppresses evoked oscillations in rat thalamic slices. Five simultaneous multiunit recordings from a rat thalamic slice in control conditions (left), during CZP application (middle), and after CZP washout (right). In each condition, the top three recordings are from thalamocortical neurons in the ventrobasal complex, and the bottom two recordings are from thalamic reticular neurons. In the top TRN trace, unit amplitude is small, so arrows point to the location of the last detected burst in each oscillation. The stimulus artifact is visible at the left of each recording. Calibration: 1 sec.


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Table 1. CZP effects in rats, WT mice, $alpha$ ₁(H101R) mice, and $alpha$ ₃(H126R) mice

$alpha$ ₁ mutants but not $alpha$ ₃ mutants retain CZP-mediated suppression

Having found that CZP suppresses evoked thalamic oscillations in rats, we looked for similar effects in WT and mutant mice.Because the CZP-mediated suppression is hypothesized to resultfrom the enhancement of inhibitory synapses between TRN neurons,we expect the CZP-mediated suppression of oscillations to be intactin $alpha$ ₁(H101R) mice, in which the effects of CZP are restrictedto TRN neurons. By the same argument, CZP should not suppressthalamic oscillations in $alpha$ ₃(H126R) mice, in which CZP modulatesIPSCs in relay neurons but not in TRN neurons. Indeed, CZP produceda reversible suppression of evoked oscillations in recordingsfrom the VB of WT and $alpha$ ₁(H101R) mice. Figure 2 shows multiunitactivity during two consecutive evoked oscillations in WT (top)and $alpha$ ₁(H101R) (middle) slices in control conditions (left), duringthe application of CZP (middle), and after CZP washout (right).In contrast, CZP had no noticeable effect on oscillations in recordingsfrom $alpha$ ₃(H126R) slices (Fig. 2, bottom). Figure 3 summarizes howthe average number of spikes during each oscillation changed duringCZP application and at various time points during the wash, forslices from rats, WT mice, $alpha$ ₁(H101R) mice, and $alpha$ ₃(H126R) mice.

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Figure 2. Clonazepam (CZP) reversibly suppresses evoked oscillations in thalamic slices from wild-type (WT, top) mice and mice with mutations in the $alpha$ ₁ subunit of the GABA_A receptor ( $alpha$ ₁(H101R), middle), but not in slices from mice with mutant $alpha$ ₃ subunits ( $alpha$ ₃(H126R), bottom). For each condition, control (left), CZP (middle), and washout (right), multiunit recordings from the same electrode during two consecutive evoked oscillations are shown. The stimulus artifact is visible at the left of each recording. Calibration: 500 msec.

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Figure 3. Comparison of the magnitude and washout of the clonazepam-mediated suppression of spikes during evoked oscillations in slices from rats, wild-type (WT) mice, $alpha$ ₁(H101R) mice, and $alpha$ ₃(H126R) mice. For each case, the total number of spikes in each evoked oscillation, relative to control, is plotted for various conditions (control, CZP application, and at 5 min intervals during drug washout). For rat slices, data from recordings in the ventrobasal complex (VB, $open circle$ ) and the thalamic reticular nucleus (TRN, $black-square$ ) are plotted separately. In mouse slices, all recordings were made in VB. CZP significantly reduces the number of spikes during evoked oscillations in rat TRN, rat VB, WT mice, and $alpha$ ₁ mutant mice but has no effect in $alpha$ ₃ mutant mice (*p < 0.05; ***p < 0.001). Error bars indicate ± 1 SEM.

In the following sections, we further characterize this CZP-mediated suppression. Because this suppression occurs in ratsas well as WT and $alpha$ ₁(H101R) mice, we will present data from ratsalongside those from mice. In most respects, the rat and mousedata are very similar; the differences are addressed inDiscussion.

CZP reduces the duration of thalamic oscillations

There are several independent mechanisms through which CZP might reduce the number of spikes per oscillation. These includereductions in the duration of each oscillation, the number ofspikes on each oscillatory cycle, and the oscillation frequency.For rats, we did not observe changes in the oscillation periodin either TRN (mean period in control = 170 ± 9 msec; mean periodin CZP = 177 ± 10 msec; n = 13; p = 0.23) or VB (mean period incontrol = 165 ± 5 msec; mean period in CZP = 169 ± 9 msec; n =12; p = 0.55). Similarly, CZP had no effect on the period in eitherWT (mean period in control = 139 ± 6 msec; mean period in CZP= 141 ± 7 msec; n = 13; p = 0.42) or $alpha$ ₁(H101R) mice (mean periodin control = 152 ± 4 msec; mean period in CZP = 146 ± 5 msec;n = 18; p = 0.09). However, as described below, the decrease inthe number of spikes per oscillation did result from both a lossof spikes during the early part of the oscillation and a reducedduration of thatoscillation.

For each set of oscillations recorded from one electrode, we divided the time span over which one oscillation occurred intofive domains. Each domain contained exactly one-fifth of the spikesin control conditions, e.g., if for one recording, an averageof 100 spikes occurred during each control oscillation, then the"first spike quintile" is the time interval from the occurrenceof the 1st spike until the occurrence of the 20th spike. We thencomputed the number of spikes that occurred within the same timeinterval after CZP application. We plotted the number of spikesthat occurred in each quintile in CZP, relative to the numberthat had occurred in the same quintile in control conditions.If CZP suppressed equal numbers of spikes during the early andlate portions of an oscillation, then the relative spike countshould be the same for each quintile. However, if the relativespike count was near one for early spike quintiles, but smallfor late spike quintiles, it would indicate that CZP only suppressedspikes late in the oscillation, i.e., CZP simply shortened theduration of the oscillation. In fact Figure 4a shows that, forrecordings from either rat TRN or rat VB, CZP suppresses spikesboth early and late in the oscillation, with a much larger suppression(~50%) occurring near the end of the oscillation (population datafrom n = 22 recordings in VB and n = 16 recordings in TRN). Figure4a also shows the relative spike count for WT mouse VB (n = 13)and $alpha$ ₁(H101R) VB (n = 21). In these cases, there is almost nosuppression (< 10%) in the early quintiles, but the amount ofsuppression increases steadily over the course of an oscillation.

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Figure 4. Clonazepam (CZP) both suppresses spikes throughout oscillations and shortens the duration of oscillations. a, The number of spikes suppressed by CZP increases over the course of an oscillation. Each oscillation is divided into five time intervals (quintiles), each of which represents a successively later portion of the oscillation and contains one-fifth of the spikes in control conditions. For each quintile, the number of spikes in CZP relative to that in control is shown. In the VB and TRN of rats, CZP suppresses some spikes (20-30%) early in the oscillation and a much greater fraction (~50%) late in the oscillation. In the VB of WT and $alpha$ ₁(H101R) mice, the CZP-mediated suppression is initially small but grows progressively over the course of the oscillation. b, CZP significantly shortens the duration of evoked oscillations in rat TRN, rat VB, WT mouse VB, and $alpha$ ₁(H101R) mouse VB (*p < 0.05; **p < 0.01), and this shortening reverses after CZP washout. In the VB of $alpha$ ₃(H126R) mice, CZP prolongs the duration, but this is not statistically significant.

Figure 4a shows that CZP suppresses some spikes during the early and intermediate parts of the oscillation and a much largernumber late in the oscillation. This suggests that the CZP-mediatedsuppression of total spike count derives in part from a shorterduration of oscillations in CZP. Indeed, as shown in Figure 4b,in rat VB and TRN, and in the VB of WT and $alpha$ 1(H101R) mice, CZPsignificantly reduces the duration of oscillations (rat TRN: 353± 109 msec reduction, n = 16, p < 0.01; rat VB: 417 ± 137 msecreduction, n = 22, p < 0.01; WT VB: 279 ± 95 msec reduction, n= 13, p < 0.05; $alpha$ ₁(H101R) VB: 276 ± 102 msec reduction, n = 22,p < 0.05). In contrast, CZP produces a nonsignificant prolongationof oscillations in the VB of $alpha$ ₃(H126R) mice (117 ± 99 msec prolongation;n = 18; p = 0.25). The lack of an effect on, or possible prolongationof, duration in $alpha$ ₃(H126R) slices is consistent with the fact thatin these slices, CZP actually increases the number of spikes latein the oscillation (Fig. 4a, right) (n = 18). Note, as illustratedby Figure 2, the duration varied considerably from recording torecording. Despite this variability, however, there were no systematicdifferences in duration among WT, $alpha$ ₁(H101R), and $alpha$ ₃(H126R) mice,and, as shown by Figure 4b, CZP consistently decreased the durationof oscillations in slices from WT and $alpha$ ₁(H101R)mice.

CZP suppresses synchronous spikes

Figure 3 shows that CZP suppresses spikes during thalamic oscillations in rats, WT mice, and $alpha$ ₁(H101R) mice, and Figure 4ashows which spikes are suppressed, on the time scale of an oscillation.On the finer time scale of individual bursts, however, it is stillnot clear which spikes are affected. As shown in Figures 1 and2, each cycle of an evoked oscillation consists of a populationburst, in which many neurons burst, followed by a period of relativequiescence. CZP may suppress spikes at the peaks of these bursts,at the beginning or end of the bursts, and/or in the intervalsbetween bursts. To elucidate exactly which spikes are suppressedon the time scale of bursts, we found the first, second, etc.bursts during oscillations in control conditions and comparedeach of these with bursts that occurred at approximately the sametime during oscillations in CZP or after CZP washout (see Materialsand Methods for details). Figure 5 shows the first through fourthbursts in control conditions in comparison with correspondingbursts in CZP and after CZP washout. It is clear that the majoreffect of CZP is to suppress synchronous spikes that occur atthe peaks of the population bursts. Although some spikes at othertimes are suppressed, this effect both is smaller and appearslater than the suppression of the peaks. For example, in rat VB,the peak is strongly suppressed on all four bursts, whereas spikesduring the interburst intervals are only modestly suppressed,and this suppression is evident only on the fourth burst. In wild-typeand $alpha$ ₁(H101R) mice, during the fourth burst, spikes within 25msec of the peak are significantly suppressed (WT: 25% suppression,n = 10, p < 0.001; $alpha$ ₁(H101R): 24% suppression, n = 19; p < 0.01),whereas spikes >60 msec from the peak are not affected (WT: 3%enhancement, n = 10, p = 0.77; $alpha$ ₁(H101R): 5% suppression, n =19; p = 0.64).

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Figure 5. Clonazepam (CZP) suppresses synchronous firing during evoked oscillations. We compared the bursts of synchronous population activity during oscillations in control conditions (solid black) with bursts at similar times during oscillations in CZP (gray) and after CZP washout (dotted black). Each burst shown here is an average computed from several sweeps from several experiments. In recordings from the TRN and VB of rats and from the VB of WT and $alpha$ ₁(H101R) mice, the main effect of CZP is to suppress spikes at the peaks of the bursts.

Figure 5 also reinforces the time course for the CZP-mediated suppression suggested by Figure 4. In rats, the CZP-mediatedsuppression is present from the very first burst. In contrast,in WT and $alpha$ ₁(H101R) mice, CZP has relatively small effects onthe first two bursts and larger effects on the third and fourthbursts. A straightforward interpretation of this observation isthat in mice, CZP does not appreciably suppress initial burstsbut does produce a suppression that grows as the oscillation progresses.However, because the bursts in Figure 5 are averages taken overseveral sweeps and several experiments, there is an alternativeto this "progressive suppression" interpretation. In particular,it is possible that the only effect of CZP is to accelerate theend of each oscillation in an abrupt, all-or-nothing manner. Ifthe degree of premature termination was variable, this effectwould manifest as a progressive decline in the amplitude of theaveraged bursts, although bursts in individual sweeps were suppressedeither completely or not at all. To verify the former progressivesuppression interpretation, we compared ratemeters on individualcontrol sweeps with those on individual CZP sweeps from the samerecording. Figure 6 shows binned spike counts (ratemeters) fromfour consecutive control sweeps alongside those obtained later,during CZP application, for a recording from a WT mouse slice.Comparing the two sets of ratemeters confirms that CZP progressivelysuppresses the bursts. Early in the oscillation, bursts are similarin control and CZP; however, soon thereafter, the bursts becomemarkedly smaller in CZP, and this leads to the premature end ofthe oscillation.

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Figure 6. Binned spike counts (ratemeters) during four consecutive evoked oscillations in control (left) and CZP (right) during a recording from WT mouse VB. A single shock to internal capsule elicits a sustained oscillation, consisting of a series of bursts of population firing. The amplitude of early bursts is similar in control and CZP, but the later bursts are strongly suppressed in CZP, so that in the latter condition, oscillations come to a premature end. Each bar (|) marks the center of a burst near the average time at which the third burst would occur during control oscillations in this recording. Calibration: horizontal, 500 msec; vertical, 5 spikes; bin width, 10 msec.

Figure 6 also demonstrates how our algorithm identifies "temporally corresponding" bursts for comparison. Above each ratemeter,a bar marks the burst that the algorithm selected as being closeto the time at which the third control burst usually occurred.In most cases (six of eight), the bar is clearly aligned withthe peak of the third burst. In the other two cases, however,the algorithm selected the fourth burst, because it searches forthe local maximum of the ratemeter (after it has been smoothed)in a time window centered on the average time at which the thirdburst occurred. Thus, the algorithm compares bursts that occurclose in time, rather than simply comparing the nth burst on differentsweeps (because these might occur at very differenttimes).

CZP reduces TRN neuron bursting in mice

The action of CZP to suppress evoked oscillations, shown in Figures 1-3, presumably results from effects on TRN neurons becauseit is present in $alpha$ ₁(H101R) but not $alpha$ ₃(H126R) mice. These effectsmay include a reduction in the number of TRN neuron bursts and/ora reduction in the number of spikes per TRN neuron burst. To clarifywhich of these mechanisms might be at work, we recorded intracellularlyfrom TRN neurons during evoked oscillations in WT and $alpha$ ₁(H101R)mice. In these recordings (two recordings from WT slices and onerecording from an $alpha$ ₁(H101R) slice), CZP always produced a significantreduction in the number of bursts, but we never observed a reductionin the number of spikes per burst, even for bursts immediatelyafter internal capsule stimulation (Table 2). Figure 7 showsthe activity of an $alpha$ ₁(H101R) TRN neuron in three different conditions:during application of 100 nM CZP (left), after washout with controlACSF (middle), and during the subsequent application of 300 nMCZP (right). For each condition, the activity during four consecutiveevoked oscillations is shown. Excluding the initial, stimulus-evokedburst (at left of each trace), this neuron consistently burststhree times in control ACSF, but only once or, rarely, twice inCZP. Each burst contains an average of 4.3 spikes in control conditionsand 5.6 spikes in 100 nM CZP. As in all of our recordings, theCZP-induced reduction in bursting was not accompanied by a tonichyperpolarization of the neuron. These observations are similarto those in a more thorough quantification of the effects of CZPon rat TRN neurons during evoked oscillations (Sohal and Huguenard,2001b). They also accord with multiunit recordings from TRN, whichclearly contain fewer TRN cell bursts after CZP application. Asshown in Figure 8, to the extent that bursts from individual neuronscould be discerned in multiunit recordings, they contained similarnumbers of spikes in control conditions and after the applicationof CZP.


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Table 2. CZP effects on intracellularly recorded RE cell bursts

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Figure 7. Clonazepam (CZP) reduces the number of bursts in reticular neurons. Intracellular recordings from a reticular neuron in an $alpha$ ₁ receptor mutant slice during evoked oscillations in three different conditions: application of 100 nM CZP (left), washout with control ACSF (middle), and subsequent application of 300 nM CZP (right). For each condition, the activity during four consecutive evoked oscillations is shown. Excluding the initial, stimulus-evoked burst (at left of each trace), this neuron consistently bursts three times in control ACSF, but only once or, rarely, twice in CZP. In the top three panels, bursts indicated by asterisks are shown on an expanded time scale in the insets to confirm that bursts consist of similar numbers of spikes in the three conditions: 100 nM CZP, wash, and 300 nM CZP.

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Figure 8. Clonazepam reduces the number of bursts, but not burst morphology, in multiunit activity recorded from TRN. Top, Multiunit recording from TRN in an $alpha$ ₁(H101R) mouse in control conditions and after the application of 100 nM CZP (calibration: 1 sec). a and b show a population burst in each of the two conditions on an expanded time scale (calibration: 25 msec). Note the spikes of varying amplitudes and high interspike frequency, suggesting that the population burst contains spikes from multiple bursting RE cells. The top traces together with a and b show that fewer RE cell bursts occur in CZP than in control conditions. c and d show a burst, likely from a single RE cell, in the two conditions (calibration: 10 msec). In this experiment, one to three bursts that had similar spike morphologies and overall burst pattern were discernable in each control sweep compared with at most one burst from this presumed unit that was visible in each CZP sweep (data not shown). In both conditions, these bursts contained four to five spikes, consistent with the idea that although CZP may decrease the number of RE cell bursts, the number of spikes in each burst by this RE cell does not change dramatically.

  Discussion

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

CZP suppresses thalamic oscillations by enhancing intra-TRN inhibition

We found that CZP suppresses evoked spindle-like oscillations in thalamic slices from rats, WT mice, and $alpha$ ₁(H101R) mice, butnot in slices from $alpha$ ₃(H126R) mice. In $alpha$ ₁(H101R) and $alpha$ ₃(H126R)mice, the effects of CZP are restricted to TRN or VB neurons,respectively (Huntsman et al., 2000; Porcello et al., 2001). Thus,enhancing inhibition between TRN neurons is both necessary andsufficient for CZP to suppress evoked thalamicoscillations.

The effects of CZP are dynamic over the course of an oscillation

How does enhancing intra-TRN inhibition suppress thalamic oscillations? First, the suppression is progressive: a relativelysmall reduction in spikes early on grows over the course of anoscillation, ultimately shortening the duration of that oscillation.Second, CZP does not suppress spikes indiscriminately. One largeburst of spikes occurs during each cycle of an oscillation, andCZP preferentially suppresses the "synchronous" spikes that occurduring the peaks of these population bursts. Third, in a limitednumber of intracellular recordings from TRN neurons in WT and $alpha$ ₁(H101R) slices, and in more extensive recordings in rat slices(Sohal and Huguenard, 2001b), CZP reduces the number of timesthat TRN neurons burst during anoscillation.

These observations suggest a possible mechanism by which CZP could suppress thalamic oscillations. CZP enhances intra-TRNinhibition, and as a result, fewer TRN neurons burst synchronouslyduring population bursts, reducing inhibitory output from TRN.Reduced TRN output elicits fewer or less intense rebound burstsin VB, attenuating synchronized bursts in TC neurons. ReducedTC activity would then recruit less TRN activity on the next cycleof the oscillation; this could explain how the effects of CZPgrow over the course of an oscillation (Fig. 4a).

Of course, the preceding mechanism may not be valid, because the effects of CZP, reduced TRN bursting, a progressive lossof synchronous spikes, and a reduction in the duration of theoscillation, may not be causally linked. Instead, a single factormight produce all three of these effects. For example, GABA_A receptoractivation could summate in TRN neurons over the course of anoscillation, so that the total GABA_A receptor-mediated conductance(g_GABA-A,TRN) grows. Early in the oscillation, a relatively smallg_GABA-A,TRN might have little effect. As the oscillation progressesand g_GABA-A,TRN grows, proportionately fewer spikes might occur.Ultimately, g_GABA-A,TRN might be large enough to bring the oscillationto a premature end. In such a scheme, changes in the early partof the oscillation do not affect later parts of the oscillation.However, thalamic oscillations are dynamic phenomenon in whichthe initial pattern of activity controls the form that the oscillationultimately takes [cf. colliding waves in vitro in Kim et al. (1995)and responses to differently sized stimuli in the simulationsof Sohal and Huguenard (2000)]. This dynamism supports a mechanismin which CZP produces effects early in the oscillation that leadto later effects, e.g., shortening of theduration.

The progressive nature of CZP effects (Figs. 4a, 5) suggests that ongoing intrathalamic activity is sufficient to recruitmeaningful levels of intra-TRN inhibition. An alternative wouldbe that only broad activation of TRN, which follows the stimulationof corticothalamic fibers to initiate an oscillation, is enoughto produce significant intra-TRN inhibition. In WT and $alpha$ ₁(H101R)mice, however, CZP has little effect on the early portion of theoscillation, which immediately follows stimulation of corticothalamicfibers, but later in the oscillation, after intrathalamic activityhas proceeded in the absence of corticothalamic stimulation, theCZP effect is muchlarger.

Role of intra-TRN inhibition

There are several hypothesized functions for intra-TRN inhibition. Our findings are consistent with studies suggesting thatinhibitory synapses between TRN neurons suppress thalamic oscillations(von Krosigk et al., 1993; Huguenard and Prince, 1994; Huntsmanet al., 1999; Sohal et al., 2000). One difference between ourstudies and those done in ferret slices (von Krosigk et al., 1993)is that the latter emphasized that blocking inhibition betweenneurons of perigeniculate nucleus (the visual analog of TRN) prolongedbursts. By contrast, data presented here (Fig. 7) and elsewhere(Sohal and Huguenard, 2001b) suggest that CZP may act by changingthe number of bursts peroscillation.

Bazhenov et al. (1999) have proposed that rather than suppressing oscillations, GABA_A receptor-mediated currents depolarizeTRN neurons, spreading activity through TRN and initiating spindles.It is difficult to predict, on the basis of this model, how CZPshould affect evoked spindles. One possibility is that by enhancingintra-TRN inhibition, CZP should spread activity. Alternatively,CZP might increase the amplitude or duration of IPSCs in TRN neuronsbeyond some critical value, so that these currents shunt, ratherthan elicit, bursts in TRN. We found that during evoked oscillations,CZP suppressed population bursts in multiunit recordings fromTRN and reduced the number of bursts in intracellular recordingsfrom TRN neurons. This suggests that if a regime exists withinwhich intra-TRN inhibition depolarizes TRN neurons and elicitsbursts, then during evoked oscillations, moderate augmentationof intra-TRN inhibition is sufficient to shift intra-TRN inhibitionto a primarily shunting and anti-oscillatoryrole.

A third hypothesis is that TRN is the "pacemaker" for spindle oscillations (Steriade et al., 1987; Destexhe et al., 1994),i.e., oscillations occur when TRN neurons burst and inhibit eachother, resulting in T-current deinactivation that elicits anothercycle of rebound bursts. In this scheme, intra-TRN inhibitionsustains and paces thalamic oscillations, so augmenting intra-TRNinhibition should enhance oscillations and alter their period.In contrast to this prediction, we not only observed marked suppressionof oscillations by CZP, but we also observed that CZP did notaffect the period of thalamicoscillations.

Synchrony in networks of inhibitory neurons

Weakening inhibition in interconnected inhibitory networks of the hippocampus disrupts population rhythmicity (Whittingtonet al., 1998). Here we studied an interconnected inhibitory networkin the thalamus and found that selectively strengthening of intra-TRNinhibition suppressed synchronous spikes that occur at the peaksof population bursts. Thus, networks of inhibitory neurons candesynchronize network oscillations, and as described above, thesuppression of synchronous activity might invoke dynamic mechanismsthat ultimately reshape an oscillation, e.g., reducing itsduration.

Why are synchronous spikes particularly affected by the strengthening of intra-TRN inhibition? Although modeling studies mayyield further insights, we offer the following possible explanation.In TRN, synchronous spikes occur, by definition, during timesof peak intra-TRN inhibition and thus are subject to increasedshunting in CZP. Reduced TRN output, resulting from CZP-mediatedenhancement of intra-TRN inhibition, may in turn elicit less intenserebound bursts from TC neurons. This translates into less activityat the peaks of population bursts. As long as many TC neuronsrebound burst at varying times, however, spikes will still occuroutside the peaks of the population bursts. Perhaps only laterin the oscillation, when the inhibitory output from TRN decreasessufficiently, does the number of bursting TC neurons decreaseso that spikes beyond the peaks of population bursts areaffected.

Differences between the effects of CZP in rats and mice

CZP suppressed evoked oscillations in thalamic slices from rats, WT mice, and a₁(H101R) mice. This suppression was much largerin rats than in mice, however, reflecting in large part the factthat CZP suppressed spikes throughout oscillations in rats, whereasin mice, CZP had a very small effect on early bursts. This differencemay reflect the different contributions made by GABA_B receptorsduring evoked thalamic oscillations in rats and mice. In intracellularrecordings from TC neurons during evoked oscillations in mice,blocking GABA_B receptors has no observable effect (Warren et al.,1994). By contrast, in rat TC neurons, the IPSP that immediatelyfollows internal capsule stimulation has a large GABA_B receptor-mediatedcomponent that is selectively suppressed by CZP (Huguenard andPrince, 1994). Thus, the strong suppression of the early partof an oscillation, which CZP produced in rats but not in mice,may reflect the effect of CZP to reduce GABA_B receptor activationin TC neurons by altering the excitability of TRNneurons.

Larger contributions from GABA_B receptors, which slow evoked thalamic oscillations (Jacobsen et al., 2001), may also explainwhy the period of oscillations was longer in rats than inmice.

Implications for anti-absence drug design

The same thalamic circuitry that generates spindles in vivo and spindle-like oscillations in vitro is hypothesized to contributeto the spike-wave discharges in absence epilepsy (Huguenard andPrince, 1997; Sohal and Huguenard, 2001a), and the effectivenessof CZP in treating absence epilepsy may derive from its abilityto dampen thalamic oscillations (Huguenard and Prince, 1994; Zhanget al., 1996). Our results suggest that the suppression of thalamicoscillations by CZP results exclusively from its action on $alpha$ ₃-containingGABA_A receptors in TRN. This suggests that drugs which selectivelyaugment currents mediated by $alpha$ ₃-containing GABA_A receptors, orare in other ways specific for GABA_A receptors in TRN, will sharethe therapeutic efficacy of CZP and may have fewer undesirableinteractions with other GABA_A receptors. Indeed, one major sideeffect of CZP is drowsiness, but when benzodiazepines and relateddrugs do not bind to $alpha$ ₁-containing GABA_A receptors, they are freeof sedative effects (Rudolph et al., 1999).

  FOOTNOTES

Received Nov. 4, 2002; revised Feb. 13, 2003; accepted Feb. 13, 2003.

This work was supported by National Institutes of Health Grants GM07365 from the National Institute of General Medical Sciencesand NS34774 from the National Institute of Neurological Disordersand Stroke, the Pimley Research Fund, and the Swiss National ScienceFoundation.

Correspondence should be addressed to J. R. Huguenard, Department of Neurology and Neurological Sciences, Stanford UniversityMedical Center, Stanford, CA 94305-5122. E-mail: john.huguenard{at}stanford.edu.

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