Synchronized Paroxysmal Activity in the Developing Thalamocortical Network Mediated by Corticothalamic Projections and "Silent" Synapses

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The Journal of Neuroscience, April 15, 1999, 19(8):2865-2875

Synchronized Paroxysmal Activity in the Developing Thalamocortical Network Mediated by Corticothalamic Projections and "Silent" Synapses
Peyman Golshani and Edward G. Jones
Center for Neuroscience, University of California, Davis, California 95616

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In mouse thalamocortical slices in vitro, the potassium channel blocker 4-AP and GABA_A receptor antagonist bicuculline togetherinduced spontaneous prolonged depolarizations in layer VI neuronsfrom postnatal day 2 (P2), in ventroposterior nucleus neurons(VP) from P7, and in reticular nucleus neurons (RTN) from P8.Dual whole-cell recordings revealed that prolonged bursts weresynchronized in layer VI, VP, and RTN. Bursts were present incortex isolated from thalamus, but not in thalamus isolated fromcortex, indicating that bursts originated in cortex and propagatedto thalamus. Prolonged bursts were synchronized in layer VI whenvertical cuts extended from pia mater through layers IV or V,but were no longer synchronized when cuts extended through layerVI and whitematter.
In voltage-clamp recordings before P10, burst conductance of all three neuronal populations was dominated by the NMDA receptor-mediatedconductance, and therefore synapses were "silent". In cortex andRTN, after P10, bursts were associated with strong AMPA/kainatereceptor-mediated conductances, and synapses had become "functional";silent synapses persisted in a large proportion of VP cells afterP10.
Before P9, the NMDA receptor antagonist APV or the non-NMDA receptor antagonist CNQX blocked the prolonged bursts. After P9,CNQX continued to block the prolonged bursts, but APV merely shortenedtheirduration.
Thus, NMDA receptor-based silent synapses are essential for paroxysmal corticothalamic activity during early postnatal development,and connections between layer VI neurons are sufficient for horizontalcorticalsynchronization.

Key words: ventroposterior nucleus; reticular nucleus; somatosensory cortex; NMDA receptor; cortical oscillations; paroxysmal activity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Synchronous oscillatory activity of large populations of forebrain neurons is a concomitant of changes in conscious stateduring arousal and sleep (Steriade et al., 1993). Synchronizationof large ensembles of cortical and thalamic cells during state-dependentchanges in rhythmic activities of the forebrain is dependent onthe corticothalamic projection (Contreras et al., 1996). The developmentof low- and medium-frequency, state-dependent oscillations inthe thalamocortical network is delayed until maturation of theintrinsic membrane properties of thalamic cells (Warren and Jones,1997). Until these properties mature, certain forms of seizureactivity, notably the absence seizures of childhood, are uncommon.Nevertheless, in both the immature and adult nervous system, smallperturbations of inhibitory or excitatory systems lead to highlysynchronized, paroxysmal activity that can propagate across largedistances.

Recently, the existence of silent synapses has been revealed in the developing optic tectum of Xenopus and in the hippocampusand layer IV of the cerebral cortex of mammals (Crair and Malenka,1995; Durand et al., 1996; Wu et al., 1996; Isaac et al., 1997).These synapses are called silent because they induce excitatorypostsynaptic conductances that are mediated solely by the NMDAreceptor, and hence do not conduct current at the resting membranepotential of the cell. Silent synapses can be converted into functionalsynapses, i.e., synapses that induce both NMDA and AMPA/kainate-mediatedEPSCs, by pairing presynaptic activation with postsynaptic depolarization.The selective transformation of silent synapses into functionalsynapses has been hypothesized to underlie the Hebbian, activity-dependentshaping of retinotectal (Wu et al., 1996) and thalamocortical(Isaac et al., 1997) circuitry and may determine the selectivestabilization or retraction of synapses duringdevelopment.

Although the existence of silent thalamocortical synapses during early development has been a topic of considerable discussion(Isaac et al., 1997; Malenka and Nicoll, 1997), there has beenlittle consideration of the potential existence of silent corticocorticaland corticothalamic synapses or of how they may support synchronizedoscillatory or paroxysmal activity. It is well known that theneonatal brain is especially susceptible to induction of epileptiformactivity (Blom et al., 1978; Ellenberg et al., 1984), but therehas been little study of the mechanisms of seizure induction andpropagation in immature corticalcircuits.

Most in vitro studies of epileptiform activity in the cortex have been performed on isolated cortical slices that eliminatethe corticothalamocortical loop. Although intrinsic cortical circuitryis rich in recurrent excitatory connections and can support theexistence of epileptiform activity on its own, paroxysmal activityin vivo undoubtedly involves the integration of activity at bothcortical and thalamic levels (Neckelmann et al., 1998, Steriadeet al., 1998; Steriade and Contreras, 1998; Timofeev et al., 1998).In this study, using an in vitro slice preparation that maintainsthalamocortical and corticothalamic connectivity (Agmon and Connors,1991), we demonstrate that the corticothalamocortical circuitdominated by silent synapses can support the existence of synchronizedparoxysmal activity and that connections between layer VI cellsare sufficient for the propagation of paroxysmalactivity.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Postnatal day 0 (P0)-P17 ICR mice (Harlan Sprague Dawley, Indianapolis, IN) mice were anesthetized by hypothermia (P0-P4)or with ether (P5-P17) and decapitated. The brain was quicklyremoved and put in chilled artificial CSF (ACSF) containing inmM: NaCl 126, KCl 3, NaH₂PO₄ 1.25, MgSO₄ 1.3, CaCl₂ 2.5, NaHCO₃26, and dextrose 20, pH 7.4 when bubbled with 95% O₂ and 5% CO₂,osmolarity 300-315 mOsm. Slices (400-µm-thick) containing thesomatosensory cortex, reticular nucleus (RTN), and ventroposteriornucleus (VP) were cut at an angle that preserves corticothalamicand thalamocortical connectivity (Agmon and Connors, 1991); inthree experiments, the thalamus and cortex were disconnected bycuts through the internal capsule and striatum. In one experiment,a vertical cut extending from the pia mater to the superficialwhite matter was made in the cortex. In two other experiments,vertical cuts extending from the pia to the layer IV/layer V border,or to the layer V/layer VI border were made in slices in whichthe cortex was disconnected from the thalamus. Cuts were madewith a thin steel blade while slices were immersed in chilledACSF. Slices were transferred to a submersion-type chamber, superfusedwith ACSF aerated with 95% O₂ and 5% CO₂, and allowed to recoverfor at least 1 hr before recording. Fourteen cells were recordedat 35°C, and the remaining 377 cells were recorded at room temperature(22-25°C). Because prolonged bursts were present at similar frequenciesand were indistinguishable at both temperatures, results fromthe two sets of experiments have been pooled. All voltage-clampdata were recorded at roomtemperature.

Whole-cell recording pipettes were pulled from borosilicate glass on a Narishige PP-83 two-stage puller and had resistancesof 2-5 M $Omega$ . Internal solutions (in mM) included: either (1) potassiumgluconate 120, HEPES 10, EGTA 1, MgCl₂ 2, CaCl₂ 0.1, NaCl 20,Na₂ATP 2, NaGTP 0.5, pH adjusted to 7.2-7.4 with KOH; or (2) CsOH120, D-gluconic acid 120, HEPES 10, EGTA 1.1, MgCl₂ 2, CaCl₂ 0.1,NaCl 20, Na₂ATP 2, NaGTP 0.5, QX-314 3, pH adjusted to 7.2-7.4with CsOH. Osmolarity was adjusted to 290-300 mOsm. Biocytin 0.5%was present in the internal solution during most recordings. Current-clamprecordings were performed with an Axoclamp-2A amplifier (AxonInstruments, Foster City, CA) and occasionally with an Axopatch200B (Axon Instruments). During current-clamp recordings, seriesresistance was typically 5-25 M $Omega$ and never >50 M $Omega$ , and was compensatedin bridge mode. Voltage-clamp recordings were always performedwith the Axopatch 200B. During voltage-clamp recordings, seriesresistance was 5-25 M $Omega$ , was monitored regularly, and was compensatedby 70-80%. Extracellular field recordings were performed withwhole-cell recording pipettes filled with ACSF. Data were digitizedvia a CED 1401plus interface (Cambridge Electronic Design, Cambridge,UK) at 150 Hz for the first nine current-clamp recordings andat 5000 Hz for the remainingrecordings.

Drugs used included (in µM): 4-aminopyridine (4-AP) 70, bicuculline methchloride (BMC) 10, D-2-amino-5-phosphonovaleric acid(APV) 50, and 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) 20.BMC and CNQX were purchased from Research Biochemicals (Natick,MA). APV was purchased from Research Biochemicals and from Sigma(St. Louis, MO). 4-AP was purchased from Tocris Cookson (Ballwin,MO). All drugs were applied in thebath.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study is based on data collected during whole-cell recordings from 181 neurons in the VP nucleus of the thalamus, from162 in layer VI of the somatosensory cortex, and from 48 neuronsin the RTN at P2-P17. These data include dual whole-cell recordingsfrom 20 VP neuron-cortical neuron pairs, 12 cortical neuron-corticalneuron pairs, 15 VP neuron-VP neuron pairs, 1 cortical neuron-RTNneuron pair, 1 RTN neuron-RTN neuron pair, and 1 RTN neuron-VPneuron pair. All cells recorded with a potassium gluconate-basedsolution in the pipette had membrane potentials more negativethan $-$ 60 mV and fired overshooting action potentials in responseto depolarizing current pulses or over-riding spontaneous EPSPs.Field potentials were recorded in layer VI simultaneously withwhole-cell recordings from 5 VP neurons. Membrane potentials werecorrected for a 10 mV junctionpotential.

Induction of synchronized prolonged bursts in cortical, VP, and RTN neurons by 4-AP and bicuculline

Current-clamp recordings were obtained with pipettes filled with a potassium gluconate-based internal solution from 101 VP,81 layer VI, and 7 RTN neurons in thalamocortical slices fromP2-P16 mice. From P2 in layer VI, P7 in VP, and P8 in RTN, jointapplication of 4-AP and bicuculline elicited prolonged depolarizationscrested with trains of action potentials (Fig. 1A-F). In VP andRTN, these prolonged bursts were present only in a subset of cells(50-100%) at all postnatal stages. Between P2 and P9, prolongedbursts were present in 20 of 56 (36%) layer VI cortical neuronsand in all but one layer VI cell after P9. The duration of prolongedbursts (0.5-85.9 sec) and the intervals separating the prolongedbursts (0.8-454.0 sec) could remain relatively constant duringthe recording, but usually varied considerably. Bursts longerthan 20 sec in duration were only recorded very rarely. Linearregression analysis demonstrated that the mean interval betweenthe bursts decreased during postnatal development (data not shown).Furthermore, the duration of a bursts was often related to theinterval of time separating it from the previous burst; burstsafter a prolonged silence were usually but not invariably longerin duration than those after a short silent period.

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Figure 1. Paired whole-cell recordings from a layer VI-layer VI neuron pair (A), a layer VI-VP neuron pair (B), a layer VI-RTN neuron pair (C), a VP-VP neuron pair (D), an RTN-RTN neuron pair (E), and a VP-RTN neuron pair (F) reveal that prolonged bursts are synchronized in layer VI, VP, and RTN. Schematic drawings illustrate the location of the paired recordings in each experiment.

In addition to eliciting prolonged bursts, 4-AP and BMC elicited short bursts in VP and RTN neurons (Figs. 1E, 2A). Shortbursts were typically <0.5 sec in duration and had characteristicsthat distinguished them from the prolonged bursts that were 5-1000times longer in duration. In voltage clamp, the short bursts appearedas giant EPSCs characterized by a fast rise and smooth decay andreversing near 0 mV (data not shown). Because short bursts wereabsent from cortical neurons and did not occur synchronously withinVP and RTN, they were not studied further.

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Figure 2. A, Paired whole-cell recordings from two VP neurons in an isolated thalamic slice. Note the absence of prolonged bursts. Also note that short bursts are still present in thalamus isolated from cortex but do not appear synchronously. B, Paired whole-cell recordings from two layer VI neurons in cortex isolated from thalamus. Note that prolonged bursts are still present in cortex isolated from thalamus and are synchronized. C, Paired whole-cell recordings from two layer VI cortical neurons on either side of a vertical cut extending from the pia mater through layer IV; note that the prolonged bursts are present in both recordings and are still synchronized. D, Paired whole-cell recordings of two layer VI neurons on either side of a vertical cut extending from the pia mater through layer V; note that the prolonged bursts are present in both recordings and are still synchronized. E, Paired whole-cell recordings of two layer VI neurons on either sides of a cut extending from the pia mater through layer VI and white matter; note that the prolonged bursts are present in both recordings but are no longer synchronized.

Burst synchronization

To determine whether prolonged bursts in cortical cells were synchronized within the cortex, whole-cell recordings of pairsof layer VI cortical neurons were performed (n = 6 pairs). Inall recordings in which prolonged bursts were present (n = 5),bursts appeared synchronously in the two cortical neurons (Fig.1A), even when the cortical neurons were separated by 3-4 mm.The lag time between the beginning of a prolonged burst in onecortical neuron and the beginning of the synchronous bursts inthe second cortical neuron was between 0 and 40 msec (n = 3 pairs)when the cortical neurons were separated by 100-500 µm, but was100-300 msec when the cortical neurons were separated by 3-4 mm.The order in which the prolonged bursts were detected in the pairedcells varied even within the same pair of cells, suggesting thata prolonged burst traveled as a propagating wave of activity acrossthe cortex and that the location from which the wave started wasrandom.

To determine whether prolonged bursts in VP cells were synchronized with prolonged bursts in the cortex, whole-cell recordingswere performed in VP simultaneously with field potential recordingsin deep layers of the cortex (n = 5) (data not shown). In allcases, prolonged bursts in VP neurons were synchronized with fieldpotentials in the cortex. In addition, dual whole-cell recordingswere obtained from pairs of cells in VP and layer VI of the cortex(n = 20 pairs). None of the cell pairs were monosynaptically coupled,as determined by the fact that action potentials elicited by theinjection of depolarizing current pulses into either the thalamicor cortical neuron could not evoke EPSPs in the other recordedneuron. In all cases in which prolonged bursts were present inVP neurons, they were synchronized with prolonged bursts in thecortex (n = 11 pairs) (Fig. 1B). In one case, prolonged burstsin the cortex were synchronized with barrages of subthresholdEPSPs in the VP neuron. The onset delay between the beginningof the prolonged burst in a cortical neuron and the beginningof the synchronous prolonged burst in the paired thalamic neuronvaried between 5 and 100 msec. Bursts could appear first in thecortex or first in VP and, as in the cortex, the order in whichthe burst appeared varied even within the same pair of cells.However, in 85% (202 of 239) of the total number of burst pairs,the prolonged burst was first detected in the corticalcell.

To determine whether prolonged bursts in RTN were synchronized with prolonged bursts in the cortex, dual whole-cell recordingswere performed in layer VI of the cortex and RTN (n = 1). Thepair of cells was not monosynaptically coupled. Prolonged burstsin the layer VI cortical cell occurred synchronously with prolongedbursts in the RTN neuron (Fig. 1C).

To determine whether prolonged bursts were synchronized within VP, dual whole-cell recordings were performed in VP (n = 13pairs). In all cases in which prolonged bursts were present inboth VP neurons, they were always synchronized (n = 10 pairs)(Fig. 1D). In one case, prolonged bursts present in one VP neuronwere synchronized with barrages of 2-4 mV EPSPs in the other VPneuron.

Dual whole-cell recordings from one RTN-VP pair and one RTN-RTN pair also revealed that prolonged bursts appeared synchronously(Fig. 1E,F).

We attempted to define the site of origin of the prolonged bursts by completely cutting the cortex away from the thalamus.Whole-cell recordings of layer VI cortical neurons in the isolatedcortex revealed that prolonged bursts were present in all neuronsexamined (n = 4). Paired recordings from layer VI neurons locatedin adjacent cortical columns revealed that the prolonged burstsremained synchronized in the isolated cortical preparation (n= 1 pair) (Fig. 2B). In contrast, prolonged bursts were neverdetected in whole-cell recordings of VP neurons in the isolatedthalamus (n = 4), although short bursts were recorded in all cells(Fig. 2A). Paired whole-cell recordings in VP revealed that shortbursts were not synchronized (n = 2pairs).

To determine whether intracortical connections were critical for synchronizing prolonged bursts within the cortex, cuts extendingfrom the pia mater to the superficial white matter were made inthe cortex, and paired whole-cell recordings were performed inlayer VI of the cortex on both sides of the cut. These recordingsites were separated by 500-1000 µm, a range that matches thedistances separating the recording sites in control experiments.In all three pairs of cells examined, prolonged bursts were presentin all recordings, but bursts in the cell pairs were no longersynchronized, confirming that horizontal cortical connectionssynchronized the prolonged bursts in the cortex (Fig. 2E). Todetermine which cortical layers were critical for the horizontalspread of the prolonged bursts, partial vertical cuts were madein cortex isolated from the thalamus, and paired whole-cell recordingswere performed in layer VI on either side of the cut. Cuts extendingfrom the pial surface to the layer IV/layer V border did not disruptthe synchrony of the prolonged bursts (n = 4 pairs) (Fig. 2C).Similarly, cuts extending from the pial surface to the layer V/layerVI border did not disrupt the synchrony of the prolonged bursts(n = 2 pairs) (Fig. 2D), suggesting that axons traversing layerVI and the white matter are sufficient for the synchronizationof the prolongedbursts.

Voltage-clamp analysis of prolonged bursts

Prolonged synchronized corticothalamic bursts were further studied in voltage clamp in 80 VP neurons, 81 layer VI neurons,and 38 RTN neurons. Recordings were performed with pipettes filledwith a cesium gluconate-based internal solution supplemented withQX-314 to reduce voltage-dependent potassium currents and blockvoltage-dependent Na⁺ currents and GABA_B-mediated currents. Prolonged bursts were typicallyrecorded at seven different holding potentials between $-$ 90 and+30 mV. At all postnatal ages, in all three cell populations,prolonged burst currents were recorded as compound inward currentsat hyperpolarized membrane potentials and reversed to outwardcurrents near 0 mV (layer VI neurons, $-$ 0.44 ± 4.38 mV; RTN neurons,+0.06 ± 4.53 mV; VP neurons, +1.07 ± 4.73 mV) (Fig. 3). Therewere no developmental changes in the reversal potentials in anyof the three cell populations. There was a dramatic developmentalshift in the voltage dependence of the peak conductance and chargetransfer of the burst currents (Fig. 3). Between P2 and P10, atholding membrane potentials close to the resting membrane potentialof the cell (around $-$ 70 mV), burst currents were relatively smallin amplitude. Hyperpolarization of the membrane typically resultedin a further reduction of the peak current amplitude and chargetransfer, whereas depolarization of the membrane potential ledto a marked increase in the peak amplitude and charge transfer.Plotting the peak burst current amplitude versus the membranepotential made evident the strong voltage dependence of the burstpeak conductance in all three cell populations and also revealeda region of negative conductance between $-$ 70 and $-$ 30 mV, typicalof NMDA receptor-mediated conductances.

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Figure 3. Voltage-clamp traces and current-voltage plots of synaptic currents underlying the prolonged bursts in layer VI (A), RTN (B), and VP (C) neurons at P7-P8 and P14. Note that at P7-P8 burst conductances show strong voltage dependence at the peak of the current, but that at P14, they show little or no voltage dependence.

After P12, at membrane potentials near the resting membrane potential of the cell, burst currents recorded from layer VI andRTN cells were very large in peak amplitude (up to several nanoamps)and displayed large charge transfer. Hyperpolarization of themembrane typically resulted in an increase, whereas depolarizationresulted in a decrease of the peak amplitude and charge transferof the burst currents. Current versus voltage plots typicallyrevealed a linear or near-linear relationship between holdingmembrane potential and peak current amplitude typical of non-NMDAreceptor-mediated conductances. After P12, burst currents recordedfrom a large proportion of VP neurons (25 of 31) still displayedstrong voltage dependence, whereas the burst currents recordedfrom the remaining 6 VP neurons displayed linear or near linearcurrent-voltagerelationships.

To further quantify the change in voltage dependence in burst current peak amplitude during development, the ratio of thepeak amplitude recorded at $-$ 90 mV to the peak amplitude recordedat +30 mV was calculated and plotted versus the age of the animals(Fig. 4). Linear correlation analysis revealed a significant developmentalshift in the voltage dependence of the peak burst current amplitudein layer VI (n = 56; R² = 0.342; p < 0.0001) and RTN neurons (n = 28; R² = 0.443; p = 0.0001). Changes were not proven to be linear. InVP, where a large number of cells did not show a decrease in thevoltage dependence of the peak burst conductance (Fig. 4C), therewas no statistically significant shift in the voltage dependenceof the response (n = 41; R² = 0.023; p > 0.1), although a few VP cells after P14 did showdecreases in voltage dependence of burst currents. The strongvoltage dependence of the peak conductance of the burst currentsbefore P12 suggests that NMDA receptor-mediated currents are thedominant contributors to the total burst current during the earlypostnatal period. The lack of voltage dependence of the peak conductanceof the burst currents in layer VI and RTN cells after P12 suggeststhat non-NMDA receptors, which typically show little voltage dependenceat peak conductance, make a large contribution to the total burstcurrent during more mature postnatal stages.

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Figure 4. Scatter plot and linear regression analysis of the ratio of the peak burst current recorded at $-$ 90 mV to the peak burst current recorded at +30 mV versus developmental stage in layer VI (A), RTN (B), and VP (C) neurons. Note the increase in the ratio of the current at later developmental stages in layer VI and RTN neurons confirming that current-voltage relationships show voltage dependence at early stages but little or no voltage dependence at later developmental stages. In VP neurons, a large proportion of the neurons still show strong voltage dependence at later developmental stages.

Pharmacological analysis of prolonged corticothalamic bursts

The NMDA receptor antagonist APV and the non-NMDA glutamate receptor antagonist CNQX were applied together in the bath (n= 4 layer VI neurons, 1 VP neuron, and 1 RTN neuron). Applicationof APV and CNQX together always reversibly blocked the prolongedbursts, indicating that ionotropic glutamate receptors are essentialfor the genesis of the prolonged bursts (data notshown).

To determine which ionotropic glutamate receptor is essential for the genesis of the prolonged bursts at early and late developmentaltime points, CNQX and APV were applied separately to layer VIneurons, RTN neurons, and VP neurons at all postnatal ages examined.Application of CNQX alone reversibly blocked the prolonged burstsat all postnatal ages examined (P6-P15) (n = 2 VP neurons, 3 layerVI neurons), indicating that at both early and late postnatalstages non-NMDA ionotropic glutamate receptors are involved inthe maintenance of the prolonged bursts (Fig. 5). The NMDA receptorantagonist APV, however, had developmentally specific effectson the synchronized corticothalamic bursts. APV reversibly blockedthe prolonged bursts only when it was applied before postnatalday 8 (n = 2 of 2 cells) in layer VI cells and before postnatalday 10 in VP cells (n = 3 of 3 cells) (Fig. 6A,C). APV reversiblyblocked the prolonged bursts in two of three RTN cells beforeP10 and reduced the peak conductance in the third cell to <10%of the control value (data not shown). After P8 in cortical cells,and after P10 in VP and RTN cells, APV never blocked the prolongedbursts, only reducing the peak conductance of burst currents whenrecorded in voltage clamp (Fig. 6B,D).

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Figure 5. Prolonged bursts recorded from P6 (A) and P14 (B) layer VI neurons before, during, and after application of CNQX. Note that CNQX blocks the prolonged bursts at both early and late postnatal ages.

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Figure 6. A, Whole-cell voltage-clamp recordings showing prolonged burst currents recorded from P9 layer VI neuron before, during, and after application of APV. Note that APV reversibly blocks the prolonged burst currents at this age. B, Whole-cell voltage-clamp recordings of prolonged burst currents recorded from a P13 layer VI neuron before, during, and after application of APV, and APV and CNQX. Note that APV no longer completely blocks the bursts but reduces the duration of the currents. Further addition of CNQX reversibly blocks the bursts. C, Whole-cell voltage-clamp recording of prolonged burst currents recorded from a P8 VP neuron before, during, and after application of APV. Note that APV reversibly blocks the burst currents at this age. D, Whole-cell voltage-clamp recording of prolonged burst currents recorded from a P15 VP neuron. Note that APV no longer blocks the burst currents and only reduces their duration.

To quantify further the developmentally specific effects of APV on the prolonged bursts, the proportion of the peak burstconductance remaining after APV application was plotted againstthe age of the animal. Linear correlation analysis revealed asignificant decrease with increasing age in the proportion ofthe peak conductance blocked by APV in layer VI (n = 13; R² = 0.536; p < 0.005), RTN (n = 7; R² = 0.881; p < 0.005), and VP (n = 5; R² = 0.865, p < 0.05), demonstrating that NMDA receptor-mediatedcurrents are much more prominent in early postnatal developmentand are essential for the generation of the prolonged bursts duringthe early postnatal period (Fig. 7). During later postnatal ages,the APV-insensitive current typically displayed a linear peakcurrent versus voltage relationship, again suggesting that thestrong nonlinearities in the current-voltage relationships observedin slices from animals before P8-P10, resulted from the relativelylarge contribution of NMDA receptor-mediated conductances to thetotal burst conductance.

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Figure 7. Scatter plots and linear regression analysis of percentage of the total peak conductance of the burst currents remaining after application of APV versus age in layer VI (A), RTN (B), and VP (C) neurons. Note that the percentage of the total peak conductance remaining after application of APV increases with increasing age of the animal in all three cell populations.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Induction of prolonged corticothalamic bursts by 4-AP and bicuculline

Application of 4-AP and bicuculline elicited prolonged bursts in layer VI, RTN, and VP neurons in P2-P16 thalamocortical slices.Paired whole-cell recordings demonstrated that the prolonged burstsappeared synchronously in the cortex, RTN, and VP. Synchronizedprolonged bursts were still observed in cortex isolated from thalamusbut were never observed in thalamus isolated from cortex, demonstratingthat the prolonged bursts were generated in the cortex and propagatedto RTN and VP via the corticothalamic projection. Because RTNneurons also receive strong excitatory input from collateralsof thalamocortical fibers, prolonged bursts could also have propagatedfrom VP toRTN.

Paired whole-cell recordings in cortex demonstrated that even in the same pair of cells, there was a great deal of variabilityin the sequence of onset of the bursts. This suggests that prolongedbursts originated in different cortical loci with each burst andpropagated through the two recording sites in a variable manner.Similar variability in the origin of spontaneous synchronizedactivity has been observed in the neocortex and hippocampus usingvoltage dye-imaging techniques (Colom and Saggau, 1994; Sutoret al., 1994). In a minority of cases, the onset of the prolongedburst was first observed in VP and then in the cortex. In thesecases, synchronized activity probably propagated from an initialsite in the cortex to the recording site in the thalamus beforepropagating to the recording site in thecortex.

Paired whole-cell recordings separated by vertical cuts of various depths through the cortex demonstrated that prolonged burstsremained synchronized in the recordings if the cut extended fromthe pia mater to the deep aspect of layer V but that prolongedbursts were no longer synchronized when cuts extended into layerVI and the white matter. This suggests that horizontal connectionsprobably arising from layer VI cells are sufficient for the propagationof the prolonged bursts across the cortical slice. A subset oflayer VI neurons possesses extensive horizontal collaterals restrictedto infragranular layers (Ojima et al., 1992); excitation of thesecells may play a cardinal role in the propagation of synchronizedactivity in thecortex.

The induction of synchronized activity by 4-AP and/or GABA_A receptor antagonists has been studied extensively in the hippocampusand neocortex (Gutnick et al., 1982; Traub and Wong, 1983; Connors,1984; Hablitz, 1984; Voskuyl and Albus, 1985; Rutecki et al.,1989; Ives and Jeffreys, 1990; Hwa and Avoli, 1991; Lee and Hablitz,1991a,b; Muller and Misgeld, 1991; Avoli et al., 1993, 1996a,b;Traub et al., 1993; Burke and Hablitz, 1994; Colom and Saggau,1994; Scharfman, 1994a,b; Sutor et al., 1994; Bianchi and Wong,1995; Hoffman and Prince, 1995; Bijak and Misgeld, 1996; Psarropoulouand Avoli, 1996; Barbarosie and Avoli, 1997; Benardo, 1997; Fortiet al., 1997; Golomb and Amitai, 1997; Siniscalchi et al., 1997;Lopantsev and Avoli, 1998), but there has been little or no studyof the propagation of paroxysmal activity from the cortex to thethalamus. At the low doses used in this study (70 µM), 4-AP isthought to selectively block the D-type potassium current (Wuand Barish, 1992). Suppression of the D current in axons or axonterminals prolongs the action potential and the period of calciumentry at the terminal and consequently increases transmitter release(Barish et al., 1996; Wheeler et al., 1996). Increased strengthof excitatory transmission in a neocortical circuit rich in recurrentexcitatory connections, accompanied by increases in the frequencyof ectopic action potentials (Traub et al., 1995), leads to generationof spontaneous synchronous propagating discharges. In the presentstudy, we blocked GABA_A receptors to best study the developmentof excitatory circuitry in the corticothalamocortical loop, furtherpromoting the generation and propagation of synchronized discharges.A recent study demonstrated that the GABA_A receptor antagonistused in this study, bicuculline methchloride, also directly blocksthe afterhyperpolarization terminating the low-threshold spikeburst in thalamic cells (Debarbieux et al., 1998). This effectcould contribute to the generation of paroxysmal activity in thisstudy.

In slices cut in an ideal plane, where both thalamocortical and corticothalamic connections are preserved, there are likelyto be re-entrant loops of activity whereby a prolonged burst initiatedin the cortex propagates to the thalamus through excitation ofcorticothalamic cells in layer V and VI and then backpropagatesto cortex via the thalamocortical projection. Although the creationof corticothalamocortical "strong-loops" has been hypothesizedto lead to epileptiform activity (Crick and Koch, 1998), thalamocorticalactivation of an already epileptic cortex may in fact act to disruptthe synchrony of corticalcells.

Voltage-clamp and pharmacological analysis of corticothalamic prolonged bursts

Voltage-clamp analysis of prolonged bursts in the layer VI, VP, and RTN cells demonstrated considerable developmental changesin the excitatory postsynaptic conductances underlying the prolongedbursts. The peak burst conductance was highly voltage-dependentduring the early postnatal stages in all three types of neurons,but became nonvoltage-dependent or nearly so in most corticaland RTN neurons and in some VP neurons; a large proportion ofVP cells still showed voltage-dependent burst conductances atlater ages. These changes can be attributed to changes in therelative contributions of non-NMDA and NMDA receptors to the totalburst conductance, because non-NMDA receptor-mediated conductancesusually show little voltage dependence, whereas NMDA receptorsshow strong voltage dependence (Nowak et al., 1984; Mayer andWestbrook, 1987; Ascher and Nowak, 1988). This suggests that duringthe first 8-9 d of postnatal development, a very large majorityof synapses activated during the prolonged bursts in layer VI,RTN, and VP are silent synapses, i.e., synapses in which onlyNMDA receptor-mediated currents can be evoked. Later in development,prolonged bursts activate functional synapses, i.e., synapsesat which both AMPA and NMDA receptors areactivated.

Pharmacological analysis further confirmed that the voltage-dependent conductance recorded during early postnatal times wasan NMDA receptor-mediated conductance. APV reversibly blockedprolonged bursts only when it was applied before postnatal day8 in layer VI cells and before postnatal day 10 in VP. In RTNcells, before P10, APV reversibly blocked prolonged bursts orreduced the peak conductance to <10% of the control value. Laterin development, APV only reduced the amplitude and duration ofburst currents and eliminated any voltage dependence in the current-voltagerelation. The non-NMDA receptor antagonist CNQX, however, blockedthe prolonged bursts at all ages examined. This indicates thatactivation of NMDA receptors at silent synapses was necessarybut not sufficient for the existence of prolonged bursts at earlypostnatal ages. During the early developmental period, the relativelysmall contribution of non-NMDA receptors is critical for the genesisof the bursts, probably by causing an initial depolarization intothe voltage range in which NMDA receptors can be activated. Duringlater postnatal ages, activation of NMDA receptors was neithernecessary nor sufficient for bursts, but activation of non-NMDAreceptors was both necessary and sufficient. The larger proportionof synapses with active non-NMDA receptors after P9 is enoughto cause recurrent excitation and propagation of thebursts.

Silent synapses have been demonstrated in developing Xenopus tectal neurons, in hippocampal CA1 neurons, and in cortical layerIV neurons (Crair and Malenka, 1995; Durand et al., 1996; Wu etal., 1996; Isaac et al., 1997). In all these neurons, silent synapsescan be converted to functional synapses by pairing presynapticactivity with postsynaptic depolarization, suggesting that calciumentry through NMDA receptors can enter the postsynaptic cell andactivate AMPA receptors through activation of signal transductionintermediates. EPSCs at developing corticothalamic synapses arealso dominated by NMDA receptor-mediated currents (Golshani etal., 1998). It will be interesting to determine whether sustainedsynchronous bursts can convert silent synapses between layer VIcortical neurons, VP neurons, and RTN neurons into functionalsynapses.

In the adult hippocampus, prolonged synchronized bursts that originate in CA3 and propagate to CA1 and are recorded in thepresence of 4-AP, GABA_A, and ionotropic glutamate receptor blockers,are mediated by activation of metabotropic glutamate receptors(mGluRs) (Bianchi and Wong, 1995). mGluR activation alone wasincapable of sustaining the prolonged corticothalamic bursts recordedin our preparation (our unpublished observations), suggestinga higher density of recurrent excitatory connections containingmGluRs in CA3 compared with thecortex.

Silent synapses and neuronal synchronization: implications for juvenile epilepsies

We observed paroxysmal activity in the cortex as early as postnatal day 2, at a stage when only layers V and VI have formed,and synaptogenesis is only beginning. Spontaneous synaptic currentshave been recorded in neocortical slices in very early postnatalstages (Blanton and Kriegstein 1991; Kim et al., 1995), but ithas generally been assumed that synaptic connectivity at thesestages is incomplete or insufficiently dense to maintain synchronizednetwork or paroxysmal activity. By suppressing inhibition andincreasing transmitter release, we have shown that very earlypostnatal cortical circuitry can indeed support the existenceof synchronized activity, mainly through activation of silentsynapses. Because synchronized presynaptic and postsynaptic activitycan transform silent synapses into functional synapses, synchronousparoxysmal activity in time may transform a large number of silentsynapses into functional synapses, thereby strengthening recurrentexcitatory loops and promoting epileptogenesis. Synchronized paroxysmalactivity may also interfere with activity-dependent formationof cortical, thalamocortical, and subcortical circuits and adverselyaffect the normal maturation of sensory, motor, and cognitivecenters.

  FOOTNOTES

Received Dec. 10, 1998; revised Jan. 25, 1999; accepted Jan. 28, 1999.

This study was supported by Grants NS21377 and NS30109 from the National Institutes of Health, United States Public HealthService. P.G. is an MD/PhD student and was supported by AmericanHeart Association under Grant 96005020. We thank Dr. Richard Warrenfor a critical reading of this manuscript, Drs. Diane O'Dowd,Ivan Soltesz, Alberto Muñoz, and Greg Hollrigel for practicaland theoretical advice during the experiments, and Vu Nguyen,Hyle Park, Phong Nguyen, and Hao Truong for technicalassistance.
Correspondence should be addressed to Dr. Edward Jones, Center for Neuroscience, 1544 Newton Court, Davis, CA 95616.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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