Electrical Synapses in the Thalamic Reticular Nucleus

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The Journal of Neuroscience, February 1, 2002, 22(3):1002-1009

Electrical Synapses in the Thalamic Reticular Nucleus
Carole E. Landisman¹, Michael A. Long¹, Michael Beierlein¹, Michael R. Deans², David L. Paul², and Barry W. Connors¹
¹ Department of Neuroscience, Division of Biology and Medicine, Brown University, Providence, Rhode Island 02912, and ² Department of Neurobiology, Harvard Medical School, Boston, Massachusetts 02115

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurons of the thalamic reticular nucleus (TRN) provide inhibitory input to thalamic relay cells and generate synchronizedactivity during sleep and seizures. It is widely assumed thatTRN cells interact only via chemical synaptic connections. However,we show that many neighboring pairs of TRN neurons in rats andmice are electrically coupled. In paired-cell recordings, electricalsynapses were able to mediate close correlations between actionpotentials when the coupling was strong; they could modulate burst-firingstates even when the coupling strength was more modest. Electricalsynapses between TRN neurons were absent in mice with a null mutationfor the connexin36 (Cx36) gene. Surprisingly, inhibitory chemicalsynaptic connections between pairs of neurons were not observed,although strong extracellular stimuli could evoke inhibition insingle TRN neurons. We conclude that Cx36-dependent gap junctionsplay an important role in the regulation of neural firing patternswithin the TRN. When combined with recent observations from thecerebral cortex, our results imply that electrical synapses area common mechanism for generating synchrony within networks ofinhibitory neurons in the mammalianforebrain.

Key words: thalamus; reticular nucleus; gap junctions; electrical coupling; connexin36; rat; mouse; inhibition; synchrony

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The thalamic reticular nucleus (TRN) is a thin layer of inhibitory neurons that borders relay nuclei of the dorsal thalamus(Steriade et al., 1997). Excitatory inputs to TRN neurons comefrom topographically aligned collaterals of both thalamocorticaland corticothalamic axons. Neurons of the TRN are exclusivelyGABA containing (Houser et al., 1980; Spreafico et al., 1991),and the primary targets of inhibitory TRN axon terminals are thethalamic relay neurons (Ohara, 1988; Pinault and Deschenes, 1998).Thus, the anatomy of the TRN suggests that the bidirectional excitatoryactivity between the thalamus and the neocortex generates, inparallel, an inhibitory regulation of the relay neurons (Kim etal., 1997).

A wide range of functions has been proposed for the TRN; all of them depend on the nature of its intrinsic circuitry (Wangand Rinzel, 1993; Destexhe et al., 1994; Ulrich and Huguenard,1996). Anatomical and physiological investigations of the TRNhave concluded that its neurons interact via chemical synapticconnections (Ohara, 1988; Bal et al., 1995b; Ulrich and Huguenard,1996; Sanchez-Vives et al., 1997; Huntsman et al., 1999; Sohalet al., 2000). Several studies describe local axon collateralswithin the TRN (Scheibel and Scheibel, 1966; De Biasi et al.,1988; Cox et al., 1996; Liu and Jones, 1999); electron microscopyshows that these axons form axosomatic and axodendritic chemicalsynapses on TRN cells (Williamson et al., 1994; Liu and Jones,1999). However, some analyses of the somatosensory thalamus inrats suggest that intrinsic TRN axons are relatively sparse orabsent (Pinault et al., 1995) and that TRN neurons interact throughdendrodendritic (presumably GABAergic) synapses (Deschenes etal., 1985; Yen et al., 1985). Whatever their precise morphologicalsubstrate, there has been nearly universal agreement that GABA-mediatedinhibitory synapses are the mechanism by which neurons withinthe TRN network interact (but see Warren et al., 1994).

There are also hints that TRN neurons may communicate using mechanisms other than GABAergic chemical synapses. The dendritesof TRN cells often bundle tightly together (Scheibel and Scheibel,1966; Steriade et al., 1997), and puncta adherentia, which aresmall, specialized intercellular junctions, sometimes form atdendrodendritic appositions (Ohara and Lieberman, 1985; Pinaultet al., 1997). Unfortunately, the functions of puncta adherentiaareunknown.

Recent work on GABAergic neurons in the neocortex (Galarreta and Hestrin, 1999; Gibson et al., 1999) and several other partsof the mammalian brain (Galarreta and Hestrin, 2001) suggeststhat electrical coupling may be a common feature of networks ofinhibitory neurons. Gap junctions are the ultrastructural substrateof electrical synapses (Bennett, 1977), and connexins are theproteins that comprise gap junction channels. In situ hybridizationshows that the mRNA for connexin36 (Cx36) (Condorelli et al.,1998), a connexin subtype that is most often associated with neuronalgap junctions (Rash et al., 2000), is strongly expressed in theTRN (Condorelli et al., 2000). Here we show that Cx36-dependentelectrical synapses exist in the TRN of rats and mice, and wedescribe their functionalproperties.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Thalamocortical slices, 300- to 400-µm-thick, were prepared as described previously (Gibson et al., 1999) from either SpragueDawley rats [postnatal day 14 (P14) to P21] or Cx36 wild-type(WT) or knockout (KO) littermate mice (P14-P18) and were constructedas described previously (Deans et al., 2001). Slices were visualizedusing either an Olympus Optical (Tokyo, Japan) BX50WI or a Zeiss(Oberkochen, Germany) Axioskop microscope and a Hamamatsu (HamamatsuCity, Japan) CCD camera using infrared-differential interferencecontrast (IR-DIC) in a submerged recording chamber at 32°C. Thebathing solution [artificial CSF (ACSF)] contained (in mM): 126NaCl, 3 KCl, 1.25 NaH₂PO₄, 26 NaHCO₃, 2 CaCl₂, 10 dextrose, andeither 1 or 2 MgCl₂. Micropipettes were filled with (in mM): 130K-gluconate, 0.2 EGTA, 4 KCl, 2 NaCl, 10 HEPES, 20 sucrose, 4ATP-Mg, 0.3 GTP-Tris, and 14 phosphocreatine-Tris, pH 7.25-7.5,(280-293 mOsm). Recordings were performed in current clamp usingAxoprobe amplifiers (Axon Instruments, Foster City, CA). In somecases, neurobiotin (4 mg/ml) was added to the electrode fillingsolution to test for dye coupling. The technique for developingthe tissue has been described previously (Gibson et al., 1999).

Extracellular stimuli were delivered using bipolar stimulating electrodes, monopolar tungsten electrodes, and ACSF-filledglass electrodes. Data were collected and analyzed using a digital-to-analogboard and Labview software (National Instruments, Austin, TX)on a personal computer (Dell Computer Company, Round Rock, TX).To test for the presence of chemical synapses, five spikes wereelicited in each neuron of a pair at 40 Hz while observing thepostsynaptic membrane potential at high gain. To estimate thestrength of coupling, a small hyperpolarizing current step (600msec duration) was injected into one cell while measuring thevoltage deflection in that cell ( $Delta$ V₁) and the coupled cell ( $Delta$ V₂)(see Fig. 2A); the coupling coefficient was defined as $Delta$ V₂/ $Delta$ V₁.The coupling coefficients for each cell are derived from the averageof 10-20 trials obtained from current steps applied to each cellof a pair; they did not depend on which cell of each pair wasstimulated. For estimates of the frequency dependence of coupling,resting membrane potentials were polarized to between $-$ 70 and $-$ 80 mV to prevent spiking, and sinusoidal currents were appliedto one neuron (1-100 Hz, with amplitudes sufficient to generatepeak-to-peak voltage deflections of 20-25 mV in the injectedcell).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrical synapses between neurons in the TRN

To test for the presence of electrical and chemical synapses, we recorded from pairs of TRN neurons in slices of rat or mousethalamus. Recordings were made along the full extent of the nucleus(Fig. 1A). However, most recorded pairs were in the dorsal capbecause its relatively low myelination allowed better visualizationof somata. We did not detect any difference in the electricalcoupling of cells recorded at different locations within the TRN.The intrinsic firing properties of TRN cells in both mice andrats were similar to previous descriptions (Steriade et al., 1997).The input resistance of the TRN neurons in rats was 166 ± 54 M $Omega$ (all reported data are means ± SD), and the time constant was13.1 ± 3.7 msec (n = 45). The properties of the mouse cells arereported below. Cell pairs were spaced <35 µm apart (Fig. 1B).Four TRN cells were injected with neurobiotin, and their morphologywas reconstructed. In all cases, only a single stained neuronwas recovered (Fig. 1C). Each cell had an ovoid soma and a longprimary axon that emanated dorsolaterally and coursed for severalhundred micrometers. The axons made very few collaterals withinthe TRN and traveled 0.5-1 mm into adjacent relay nuclei beforebranching extensively; in some cases, they formed terminal tufts.

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Figure 1. Structure of the TRN slice and its neurons. A, Low-power IR-DIC image of the thalamic region of a living slice. Str, Striatum; IC, internal capsule. B, Higher-power view of a pair of TRN cells with adjoining somata (left). This pair was not electrically coupled. The right shows a pair of TRN cells with nonadjoining somata. These cells were strongly coupled (coupling coefficient of 0.1). Thus, the somata of cell pairs need not touch to be electrically coupled, and many pairs that do have adjacent somata are not coupled. C, Reconstruction of a neurobiotin-filled TRN neuron. Three major axonal branches leave the nucleus.

The chemical synaptic connections between pairs of neurons were tested by evoking single or short trains of action potentialsin one cell and measuring spike-triggered voltage changes in theother cell while depolarizing by ~10-15 mV to maximize the visibilityof IPSPs. Surprisingly, no evidence of chemical synapses was observed(rats, n = 56 pairs; mice, n = 34). The absence of IPSPs was probablynot attributable to the "washout" of postsynaptic receptor function,because we were able to evoke IPSPs by stimulating extracellularlywithin the nucleus (data not shown). As described in previousstudies (Ulrich and Huguenard, 1996; Zhang et al., 1997; Huntsmanet al., 1999), the current required to evoke even a minimal IPSPwas quite high (400-500 µA evoked a 0.5 mV IPSP at rest when stimulating10-20 µm away), suggesting that chemical synaptic connectionswithin the TRN are sparse (Ohara and Lieberman, 1985; Liu andJones, 1999).

In contrast to chemical synapses, electrical synapses were commonly observed between pairs of TRN cells. Electrical connectionswere tested by applying current in steps of varying duration,strength, and polarity to one cell while searching for appropriatelytimed and scaled voltage deflections in the second cell. Approximately31% (28 of 90) of paired neurons from the TRN of rats clearlyshowed electrical coupling (Fig. 2A). The strength of each electricalconnection was quantified by calculating a coupling coefficient,which averaged 0.032 ± 0.027 (range, 0.01-0.13; n = 28) for low-frequency,or steady-state, voltage deflections. Electrical coupling wassymmetric [signals passed equally well in both directions (Fig.2A)] and was independent of transjunctional voltage over a rangeof at least ±20 mV.

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Figure 2. Electrical coupling between rat TRN neurons. A, Intracellular current steps (±200 pA) to evoke responses in cell 1 induced attenuated voltage changes in cell 2 (left traces) (coupling coefficient of 0.1). Tracings on the right are from the same cell pair, but, in this case, current steps were delivered to cell 2. B, Close-up of a single presynaptic spike and the averaged spikelet it induced in the soma of a coupled neighboring cell. C, Close-up of the rebound burst generated by cell 2 in A (right) and the coupling potential corresponding to it in cell 1.

Electrical synapses had strong low-pass filtering characteristics. Single action potentials generated a small but rapidlyrising electrical postsynaptic potential in some electricallycoupled cells, and such spikelets had an average rise time of0.43 msec (Fig. 2B); the mean coupling coefficient for actionpotentials in these pairs was 0.007 ± 0.002. However, in mostpairs in which electrical coupling was clearly evident for relativelyslow signals, action potential-evoked events were not visible;only six pairs in both rats and mice had visible spikelets (n= 39 coupled pairs). Neurons of the TRN readily generated low-thresholdspikes and spike bursts after hyperpolarization (Fig. 2A) (Baland McCormick, 1993). The relatively slow envelope of depolarizationunderlying each low-threshold burst evoked a depolarization incoupled postsynaptic neurons, with a magnitude well predictedby the low-frequency coupling coefficient of the pair (Fig. 2C);fast action potentials generated much smaller postsynaptic eventsproportionally. In another TRN pair (data not shown), which hada coupling coefficient of 0.03 (i.e., near the population average),the 10 mV envelopes of low-threshold spikes evoked postsynapticdepolarizations of ~320 µV; fast action potentials did not generatemeasurable postsynaptic events in this pair. To investigate thefrequency dependence of coupling more systematically, subthresholdsinusoidal currents were injected into single cells while recordingthe induced voltage deflections in those cells and the cells coupledto them. The attenuation of the signals recorded in the noninjectedneurons increased rapidly at stimulus frequencies $>=$ 10 Hz (Fig.3A,B).

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Figure 3. Frequency dependence of signal transfer between coupled neurons. A, Subthreshold sinusoidal currents were injected into one cell of a coupled pair, and membrane voltage deflections were recorded from the injected cell (top traces) and the cell coupled to it (bottom traces). Stimulus frequencies were 1 Hz (left traces) and 100 Hz (right traces). Note the differences in voltage gain between the traces of cell 1 (low gain) and cell 2 (high gain). B, Attenuation of sinusoidal signals across electrical synapses as a function of signal frequency. Data were obtained as described in A, and attenuation was defined as the ratio of peak-to-peak amplitudes in the noninjected compared with the injected cell, normalized to the 1 Hz attenuation and expressed as a percentage. Data points are the means ± SEM of measurements from four neuron pairs.

Electrical synapses can regulate firing patterns

Electrical coupling was strong enough for the activity of one TRN cell to influence the firing patterns of another. This couldbe demonstrated in several ways. Figure 4A shows recordings froma cell pair with a moderate coupling coefficient of 0.04. Whencell 1 was depolarized with 600 msec steps of 100 pA, it generateda train of action potentials (left traces). When cell 1 receivedthe same stimulus but cell 2 concurrently received a $-$ 300 pA currentstep, both the duration of spiking and its rate were decreasedin cell 1 (right traces). In addition, an electrical synapse couldsometimes synchronize the action potentials of two simultaneouslyfiring neurons. The cell pair shown in B was strongly coupled.Application of simultaneous current stimuli evoked tonic firingin each cell. The cross-correlogram from the spiking in this pairhas a strong peak centered on 0 msec, with a half-width of only4 msec (C), indicating that the firing patterns of the cells wereclosely synchronized. This form of spike synchrony could be demonstratedonly in the most strongly coupled pairs (i.e., coupling coefficients~0.1).

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Figure 4. Electrical synapses can regulate spiking. A, Simultaneous recordings from a coupled TRN cell pair. Traces on the left show repetitive firing in cell 1 as it received a 100 pA pulse of depolarizing current; cell 2 received no current. Traces on the right show how a hyperpolarizing current step of $-$ 300 pA delivered to cell 2 reduced the duration and frequency of spiking induced by the same 100 pA stimulus to cell 1. B, Simultaneous current steps applied to a coupled pair (coupling coefficient of 0.1) evoked repetitive firing in both. Note the small spikelets in cell 2 during intervals of spike silence; each spikelet coincided with a spike in cell 1. C, Cross-correlogram of the spiking in the pair shown in B shows a sharp, narrow peak centered on 0 msec.

Relatively low-frequency fluctuations of membrane potential were particularly effective at entraining the firing of coupledneurons. Figure 5A shows data from a pair in which steady depolarizingcurrent was injected to hold cell 2 close to the spiking threshold.When sinusoidal stimuli (1 Hz) sufficient to generate one spikeper cycle were applied to cell 1, the spiking of cell 2 was entrainedto the stimulus as well, at two spikes per cycle. Electrical couplingcould also switch TRN cells between bursting and tonically spikingmodes. Sinusoidal (1 Hz) current stimuli were first applied tocell 1 only (Fig. 5B) and adjusted so that a low-threshold burstfired near the peak of each stimulus cycle. Next, similar sinusoidalstimuli with the same phase were applied to both cells. The in-phasestimuli, interacting through the electrical synapse, reinforcedthe spiking of cell 1 and forced it to generate a burst plus twotonic spikes on each cycle. On the other hand, when the sinusoidalstimuli to the two cells were subsequently switched to anti-phase,the bursting in both cells was suppressed, and each fired onlyone or two spikes at the peak of each cycle.

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Figure 5. Modulation of spiking patterns mediated by electrical synapses. A, A sine wave current stimulus (1 Hz) was applied to cell 1, with the amplitude adjusted to generate one spike per cycle. Cell 2, which was electrically coupled to cell 1, was depolarized with steady current to near threshold. Sine wave stimuli to cell 1 induced entrained spikes in cell 2. The traces below show expansion of the traces above. Spikes in these panels are truncated. B, In a different pair of electrically coupled cells (coupling coefficient of 0.04), a 1 Hz sine wave stimulus to cell 1 induced firing of a single burst of spikes on each cycle (left). When both cells were stimulated with similar currents in-phase, cell 1 generated a burst plus two tonic spikes on each cycle (middle). When the same stimuli were shifted to anti-phase (right), cell 1 fired only two tonic spikes per cycle, and cell 2 fired a single spike per cycle. The top row shows expanded regions of recordings from cell 1, as indicated. Spike amplitudes have been truncated in all traces.

Electrical synapses in the TRN require Cx36

Cx36 appears to be the predominant type of connexin expressed in central neurons (Condorelli et al., 1998; Rash et al., 2000;Venance et al., 2000). We tested the importance of Cx36 for electricalsynapses between TRN neurons by studying WT and littermate micethat were homozygous for a null mutation of the Cx36 gene (KOmice). KO mice were constructed so that histochemical reporterswere expressed in place of the Cx36 protein (Deans et al., 2001).The thalamic expression pattern of one reporter, $beta$ -galactosidase( $beta$ -gal), is shown in a 200-µm-thick vibratome section that wascut in the same oblique plane as the slices used for electrophysiology(Fig. 6A). Staining was very strong throughout the TRN, but itwas notably sparse or absent in the relay nuclei of the dorsalthalamus. In this example, the reaction was strongly developedto reveal staining within relay nuclei. As a result, cellulardetail in the TRN is obscured by the signal intensity. To revealthe cellular distribution of staining, 14-µm-thick frozen sectionswere prepared, and the timing of the histochemical reaction wasoptimized for the TRN. As shown in Figure 6B, intense stainingis evident, but it is restricted to a subset of TRN cell bodies.A substantial number of cells are completely devoid of the reactionproduct. Double labeling in companion sections for $beta$ -gal and forparvalbumin immunoreactivity (data not shown) confirmed that markerexpression is abundant in some TRN neurons but absent in others.A restriction in Cx36 expression could explain the relativelylow incidence of coupling between neurons in the TRN (31%) comparedwith specific inhibitory interneurons in somatosensory cortex(>60%) (Gibson et al., 1999; Deans et al., 2001). It is possiblethat, in the TRN, as in neocortex, inhibitory neurons are nothomogeneous and that electrical synapses are restricted to someundefined neuronal subtype.

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Figure 6. Electrical synapses in the TRN depend on Cx36. A, $beta$ -gal histochemistry of a section from a Cx36 KO mouse shows strong staining in the TRN but very weak staining in VB. The section was cut in the oblique plane used for electrophysiology (see Materials and Methods), and the reaction was strongly developed in an attempt to reveal staining in VB. B, Higher-power view of $beta$ -gal-reacted TRN, showing that some neurons stain strongly, whereas others are apparently unstained. In this case, the section was cut in the coronal plane, and the reaction time was optimized for the TRN. C, Moderate electrical coupling between a representative pair of TRN cells from a WT mouse (left); coupling was absent from almost all pairs of TRN cells from KO mice (right).

Paired recordings from TRN neurons of WT and heterozygous mice revealed that electrical coupling and other electrophysiologicalproperties were very similar to those of TRN neurons from rats.Electrical coupling occurred in 32% of tested pairs (11 of 34pairs; two of four of these pairs were in heterozygotes) (Fig.6C, left). The mean coupling coefficient between coupled mousepairs was 0.032 ± 0.03 (range, 0.01-0.13). In contrast, electricalcoupling between TRN cells in KO tissue was all but absent (Fig.6C, right). Only one of 38 pairs had measurable coupling, andthat single coupled KO pair had an exceptionally low couplingcoefficient (~0.002). Thus, TRN neurons from WT mice exhibitedsignificantly more electrical coupling than the neurons of KOmice (p < 0.001; Fisher's exact test). Neither the input resistance(WT, 130 ± 40 M $Omega$ , n = 46; KO, 157 ± 104 M $Omega$ , n = 85) nor the membranetime constant (WT, 10.3 ± 3.4 msec; KO. 9.9 ± 5.4 msec) of TRNcells varied with genotype. Intrinsic firing patterns of WT andKO neurons were not obviously different. These results suggestthat virtually all electrical coupling between TRN neurons requiresgap junctions containingCx36.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrical synapses between TRN neurons

Our central conclusion is that many of the neurons in the TRN of rodents are interconnected by electrical synapses. At leastone author speculated as early as the 1960s that electrical synapsesmight play a role in thalamic circuitry (Bennett, 1966), but thepossibility was never given much credence nor had it been testedexperimentally. Our most direct evidence comes from paired recordingsof TRN neurons: changes of the transmembrane potential inducedin one cell cause appropriate changes of potential in the adjacentcell. The properties of these electrical interactions are similarto most electrical synapses that have been studied in vertebratenervous systems (Bennett, 1977; Galarreta and Hestrin, 2001):(1) coupling is symmetric, and current passes equally well inboth directions; (2) there is no obvious rapid gating of the couplingconductance that depends on transjunctional voltage; (3) electricalsignals are attenuated and low-pass filtered as they pass fromthe first cell to the second cell; and (4) coupling depends onthe expression of a connexin protein. No other known form of electricalinteraction between neurons is consistent with all of theseproperties.

Gap junctions are the morphological hallmark of electrical synapses (Bennett, 1977), but they are often small and are notoriouslydifficult to detect by transmission electron microscopy. The literatureon the ultrastructure of gap junctions seems to lack any descriptionof them between neurons of the TRN (Deschenes et al., 1985; Oharaand Lieberman, 1985; Ohara, 1988; Liu and Jones, 1999). In theneocortex, in which electrical synapses between GABAergic neuronsare very common (Galarreta and Hestrin, 1999; Gibson et al., 1999)and for which innumerable ultrastructural studies have been done,descriptions of gap junctions have nevertheless been quite rare(Sloper and Powell, 1978; Tamas et al., 2000).

Surprisingly, we never detected chemical synaptic interactions in our TRN paired-cell recordings. It is unlikely that technicalartifacts obscured them, because strong extracellular stimulievoked IPSPs in single TRN cells. We frequently observed unitaryIPSPs when using the same paired-cell recording methods in theneocortex (Gibson et al., 1999; Deans et al., 2001). Indeed, Zhanget al. (1997) described shock-evoked, as well as miniature IPSCs,in TRN cells of rodents; IPSPs can also be triggered in the cellsof the ferret perigeniculate nucleus (which is part of the TRN)by applying glutamate to neighboring cells (Sanchez-Vives et al.,1997). There are at least two hypotheses with regard to why wedid not observe paired-cell IPSPs. First, it may be that TRN neuronsmake very sparse connections with each other. This is consistentwith the report that the size of spontaneous and miniature IPSCsin the cells of TRN and ventrobasal nucleus (VB) are similar,yet the peak amplitude of evoked IPSCs is four times larger inVB cells compared with TRN cells when using equivalent stimuli(Zhang et al., 1997). Second, it is possible that the probabilityof neurotransmitter release is very low at intra-TRN synapses;consistent with this, the frequency of miniature IPSCs was muchsmaller in TRN than in VB neurons (Zhang et al., 1997). Our limitedtesting protocol may have missed synaptic events of low probability.Both sparse connections and low-release probability are consistentwith the very large stimulus currents we needed to evoke IPSPs.Anatomical results favor the hypothesis of sparse connections,because relatively small numbers of symmetric (Ohara, 1988) andGABA-immunoreactive (Liu and Jones, 1999) axosomatic and axodendriticsynapses are observed within the TRN. It appears that intrinsicaxonal arbors of rat TRN are short and spare (Cox et al., 1996;Liu and Jones, 1999) or, indeed, absent entirely (Pinault et al.,1995; Pinault and Deschenes, 1998). Some GABAergic synapses ontoTRN cells also arise from extrinsic sources (Ohara and Lieberman,1985; De Biasi et al., 1988), which could be activated with extracellularstimuli but would not be evident in paired-cell recordings. Ina study that combined single-cell reconstruction with serial sectionelectron microscopy, Pinault et al. (1997) suggested that dendrodendriticsynapses might be the sole type of GABAergic interconnection inthe TRN of rodents. However, not all studies have supported thisconclusion (Ohara and Lieberman, 1985; Liu and Jones, 1999).

It seems very likely that inhibitory synaptic connections within the TRN exist, but additional studies will be needed to resolvetheir properties. Our recordings show that at least a subset ofTRN cells are also coupled by electrical synapses. The circuitdiagram in Figure 7 illustrates the general pattern of chemicaland electrical synaptic connections within the TRN.

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Figure 7. Synaptic circuitry of the TRN. Rectangular terminals, Excitatory chemical synapses; circular terminals, inhibitory chemical synapses; zigzagged lines, electrical synapses. The dashed line representing the intra-TRN chemical synaptic connection indicates uncertainty about its structural basis.

Role of Cx36 in the TRN

We found that mice with a null mutation for Cx36 were nearly devoid of electrical synapses in the TRN. This suggests thatCx36 is an essential component of functional gap junctions betweenmost TRN neurons. Cx36 may also be sufficient for this purpose,because it is the only one of >16 connexin subtypes that is preferentiallyexpressed by central neurons (Condorelli et al., 1998). Studiesthat combine freeze fracture electron microscopy with immunocytochemistryhave concluded that Cx36, but not Cx43 and Cx32, is found withingap junctions that interconnect neurons in a variety of mammalianbrain regions (Rash et al., 2000, 2001). The anatomical localizationof Cx36 is also consistent with our physiological results. ThemRNA for Cx36 is densely expressed in the TRN, in stark contrastto most thalamic relay nuclei, which are "completely devoid ofhybridization grains" (Condorelli et al., 2000). Our $beta$ -gal stainingpatterns are similar to these in situ hybridization patterns (Fig.6A). The restricted expression of $beta$ -gal among TRN cells is consistentwith the relatively modest incidence of electrical coupling; itsuggests that electrical synapses selectively interconnect subsetsof TRNneurons.

The intercellular channels formed by Cx36 have interesting properties that distinguish them from other connexins. Cx36 channelshave the weakest voltage-dependent gating and the smallest single-channelconductance of any tested connexin; they are only slightly permeableto some organic dyes that permeate other connexin channels easily(Srinivas et al., 1999; Teubner et al., 2000). This is consistentwith the absence of dye coupling between electrically coupledTRN cells (in this study) and neocortical interneurons (Gibsonet al., 1999).

Recent studies have shown that GABAergic neurons of the neocortex (Galarreta and Hestrin, 1999; Gibson et al., 1999; Tamaset al., 2000) and hippocampus (Venance et al., 2000) are alsoelectrically coupled and that the coupling is severely deficientin Cx36 KO mice (Deans et al., 2001; Hormuzdi et al., 2001). Thisraises the possibility that Cx36 expression is necessary for thelarge majority of electrical coupling between inhibitory neuronsof the mammalian forebrain. Such molecular specificity shouldbe very helpful for studies of the functional role of electricalsynapses, because there are powerful methods potentially availableto manipulate the timing and location of Cx36 expression patternsselectively.

Functions of electrical synapses in the TRN

Understanding the role of electrical synapses in the TRN is complicated by uncertainty about the functions of the TRN itself.This nucleus has been implicated in, among other things, mechanismsof sensory processing (Yingling and Skinner, 1976; Lee et al.,1994; Hartings et al., 2000), attention (Crick, 1984; Guilleryet al., 1998), the generation of synchronous, rhythmic activityduring slow-wave sleep and certain seizure states (Steriade etal., 1987; Bal and McCormick, 1993; Kim et al., 1995; Avanziniet al., 2000), and the development of connections between thethalamus and the neocortex (Mitrofanis and Guillery, 1993). Thesediverse functions undoubtedly require myriad cellular mechanisms,but one feature that could be common to all of them is some degreeof synchronized neuronal activity. This converges nicely withthe well known ability of electrical synapses to synchronize neuronsacross a range of temporal scales (Bennett, 1966, 1977). Our studiesof interactions between paired neurons show clearly that electricalsynapses can synchronize neurons in the TRN. Our results implythat the relatively strong filtering properties of electricalconnections between TRN cells favor the synchronization of low-frequencyevents, such as low-threshold calcium spikes and even slower fluctuations,and preclude spike-to-spike synchrony in all but the most stronglycoupled groups of neurons. In comparison, the electrical synapsesbetween neocortical interneurons are frequently able to mediatea temporally close (±1 msec) synchrony of spikes (Galarreta andHestrin, 1999; Gibson et al., 1999).

Studies of synchrony in the TRN have emphasized the roles of chemical synapses. For example, spindle rhythms apparently arisefrom an alternation between excitatory cortical and thalamic inputsonto TRN cells on the one hand, and inhibitory TRN inputs backto thalamic relay and cortical cells on the other (Bal et al.,1995a,b; Cox et al., 1997; Sanchez-Vives and McCormick, 1997).The GABAergic synaptic connections within the TRN of rodents maymediate sustained, rhythmic, propagating activity during sleep(Bazhenov et al., 1999), but there is also evidence that theyserve to desynchronize certain forms of rhythmic activity andrestrict them spatially (Huntsman et al., 1999; Sohal et al.,2000). However, all of these studies assume strong and extensivelocal chemical connections, which is not consistent with our findings.Studies in ferret perigeniculate nucleus also support the roleof TRN cells in desynchronizing spindle oscillations (Bal et al.,1995b; Sanchez-Vives et al., 1997). Perhaps within the TRN network,electrical and chemical synapses serve opposing roles, with chemicalsynapses desynchronizing relatively high-frequency activity (e.g.,7-14 Hz sleep spindles) and electrical synapses synchronizingrelatively low-frequency activity (e.g., $<=$ 1 Hz delta rhythms),as they do in neocortex (Beierlein et al., 2000). Electrical couplingbetween TRN neurons may also be important during certain pathologicalstates, especially seizures. For example, the 3 Hz paroxysms thatcharacterize spike-wave seizures are accompanied by periodic,synchronized excitation of TRN neurons by corticothalamic synapses(Steriade and Contreras, 1995). The excited TRN neurons generatefeedforward waves of inhibition in thalamic relay cells, synchronized,perhaps, by the influence of electrical synapses within theTRN.

  FOOTNOTES

Received Sept. 20, 2001; revised Nov. 8, 2001; accepted Nov. 9, 2001.

This work was supported by the Helen Hay Whitney Foundation (C.E.L.) and by the Burroughs-Wellcome Trust (M.B.). This workwas also funded by National Institutes of Health Grants NS25983and NS27248 to B.W.C. and GM37751 and GM18974 to D.L.P. We thankJay Gibson for developing the data acquisition and analysis softwareand Saundy Patrick and Caterina Sellitto for excellent technicalassistance.
Correspondence should be addressed to Barry W. Connors, Box 1953, Department of Neuroscience, Brown University, Providence,RI 02912. E-mail: bwc{at}brown.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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