Synaptic Mechanisms Regulating the Activation of a Ca2+-Mediated Plateau Potential in Developing Relay Cells of the LGN

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Synaptic Mechanisms Regulating the Activation of a Ca²⁺-Mediated Plateau Potential in Developing Relay Cells of the LGN

Fu-Sun Lo, Jokubas Ziburkus, and William Guido

Department of Cell Biology and Anatomy and the Neuroscience Center of Excellence, Louisiana State Health Sciences Center, New Orleans, Louisiana 70112

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Lo, Fu-Sun, Jokubas Ziburkus, and William Guido. Synaptic Mechanisms Regulating the Activation of a Ca²⁺-Mediated Plateau Potential in Developing Relay Cells of the LGN. J. Neurophysiol. 87: 1175-1185, 2002. Using intracellular recordings in an isolated (in vitro) rat brain stem preparation, we examined the synaptic responses ofdeveloping relay neurons in the dorsal lateral geniculate nucleus(LGN). In newborn rats, strong stimulation of the optic tract(OT) evoked excitatory postsynaptic potentials (EPSPs) that gaverise to a sustained (300-1,300 ms), slow-decaying (<0.01 mV/s),depolarization (25-40 mV). Riding atop this response was a trainof spikes of variable amplitude. We refer to this synapticallyevoked event as a plateau potential. Pharmacology experimentsindicate the plateau potential was mediated by the activationof high-threshold L-type Ca²⁺ channels. Synaptic activation of the plateau potential reliedon N-methyl-D-aspartate (NMDA) receptor-mediated activity andthe spatial and/or temporal summation of retinally evoked EPSPs.Inhibitory postsynaptic responses (IPSPs) did not prevent theexpression of the plateau potential. However, GABA_A receptor activitymodulated the intensity of optic tract stimulation needed to evokethe plateau potential, while GABA_B receptor activity affectedits duration. Expression of the plateau potential was developmentallyregulated, showing a much higher incidence at P1-2 (90%) thanat P19-20 (1%). This was in part due to the fact that developingrelay cells show a greater degree of spatial summation than theirmature counterparts, receiving input from as many as 7-12 retinalganglion cells. Early spontaneous retinal activity is also likelyto trigger the plateau potential. Repetitive stimulation of optictract in a manner that approximated the high-frequency dischargeof retinal ganglion cells led to a massive temporal summationof EPSPs and the activation of a sustained depolarization (>1min) that was blocked by L-type Ca²⁺ channel antagonists. These age-related changes in Ca²⁺ signaling may contribute to the activity-dependent refinementof retinogeniculateconnections.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Many aspects of neuronal development depend on the sequestration of intracellular Ca²⁺ (Ghosh and Greenberg 1995). A major source is acquired via theactivation of ligand-gated N-methyl-D-aspartate (NMDA) channelsthat allow for the influx of Ca²⁺ in an activity-dependent manner (Constantine-Paton et al. 1990).However, NMDA receptors need not be the sole source of Ca²⁺. For example, in sensory thalamic nuclei like the lateral geniculatenucleus (LGN), relay neurons possess a variety of voltage-gatedCa²⁺ channels. Most notable in the LGN are the low-threshold (T-type)and high-threshold (L- and N-type) Ca²⁺ currents (Coulter et al. 1989; Hernandez and Pape 1989; Huguenard1996). The low-threshold Ca²⁺ current that underlies burst firing has been the subject of extensiveinvestigation and found to play a major role in the state-dependentmodulation of retinogeniculate transmission (McCormick and Bal1997; Steriade et al. 1993). By comparison, high-threshold Ca²⁺ channels have received far less attention. While these have beenwell characterized in dissociated cell preparations (Budde etal. 1998; Kammermeier and Jones 1997), their interplay with synapticresponses has yet to be explored. The paucity of such informationmay in part be due to technical reasons. Such study requires apreparation that allows for intracellular access and intact synapticcircuitry, conditions not found in either dissociated cell orconventional slice preparations. Therefore we used a unique isolatedbrain stem preparation (Hu 1993) to examine the nature of synaptictransmission in the developing LGN. This preparation is especiallysuited for the study of retinogeniculate transmission. Unlikea conventional thalamic slice preparation, in the isolated brainstem preparation, a large segment of the optic tract (OT) as wellas the intrinsic circuitry of the LGN remain intact. The isolatedbrain stem is readily maintained in vitro and has been used successfullyto examine the synaptic activity in a number of CNS structuresincluding thalamus (Hu 1993; Xia and Lo 1996), hypothalamus (Huand Bourque 1992), and superior colliculus (Lo and Mize 2000).Our results indicate the synaptic responses of developing LGNcells exhibit a large and sustained synaptically evoked Ca²⁺-mediated depolarization. This event provides LGN cells with arich source of Ca²⁺ during strong postsynapticdepolarization.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Sprague-Dawley rat pups ranging in age from postnatal day 1 (P1) to P24 were anesthetized with Halothane and killed by decapitation.The brain was excised and placed in a bubbled (95% O₂-5% CO₂)solution of artificial cerebrospinal fluid (ACSF, see followingtext). The brain was cut in half along the midline axis, gluedto a silver plate, and placed into a well of a temperature-controlledrecording chamber. Separate recordings were done on each hemisphere.With the aid of a dissecting microscope positioned above the chamber,the lateral surface of the thalamus and midbrain were exposedby gently removing the forebrain. The isolated brain stem wasthen submerged and perfused continuously (4-5 ml/min) with warmed(28-33°C) ACSF [which contained (in mM) 124 NaCl, 2.5 KCl, 1.25NaH₂PO₄, 1.0 MgSO₄, 26 NaHCO₃, 10 dextrose, and 2 CaCl₂, saturatedwith 95% O₂-5% CO₂, pH = 7.4]. Recordings began 1-3 h after incubationand were done at a depth of 50-200 µm below the pialsurface.

For whole cell intracellular recording, patch electrodes were pulled horizontally in two stages from borosillicate glass andfilled with a solution containing (in mM) 140 K gluconate, 10HEPES, 1.1 EGTA-Na, 0.1 CaCl₂, 2 MgCl₂, 2 ATP-Mg, and 0.2 GTP-Na,pH = 7.2 to a final tip resistance of 5-7 M $Omega$ . Whole cell patchrecordings were done in current-clamp mode with an Axoclamp 2Bamplifier using the techniques described by Blanton et al. (1989).Briefly, the formation of the whole cell configuration was indicatedby a sudden drop in seal resistance and a DC drop of $-$ 60 mV ormore. After breaking in, the series resistance was completelycompensated with bridge balance of the Axoclamp-2B amplifier.The junction potential was left uncorrected. Only those cellsthat exhibited a resting membrane level more negative than $-$ 55mV, an input resistance >300 M $Omega$ , and overshooting action potentialswere included in the study. In some instances (n = 8), we switchedthe recording mode from current clamp to single continuous voltageclamp (SEVC) to record postsynaptic currents at a holding potentialof $-$ 60 mV. We also conducted extracellular single-unit recordings(n = 20). For these we used patch electrodes filled with 1 M NaCl(1-3 M $Omega$ ). All neuronal activity was displayed on a storage oscilloscope,digitized at 10-20 kHz, and stored directly oncomputer.

To evoke synaptic activity in LGN, single square-wave pulses (0.1-0.5 ms, 0.1-1.0 mA) were delivered at a rate of 0.20-1.0Hz through a pair of thin gauged Ir wires (WPI) placed on thesurface of the OT. To examine the extent to which EPSPs summatespatially we adjusted current intensity in 1, 2, 5, or 10% increments(12-15 steps) above a stimulus level that elicited a thresholdresponse. We then constructed amplitude by stimulus intensityplots (Figs. 7 and 8), and these were used to estimate the numberof retinal inputs converging onto a single LGN cell (Chen andRegehr 2000). To examine the extent to which EPSPs summate temporally,optic tract was stimulated repetitively at 20 Hz for 0.1 s (Fig.10, A and B) or at 50 Hz for 1 s (Fig. 10C).

Various ligand-gated antagonists were bath applied to ascertain the pharmacology underlying EPSP [NMDA: D( $-$ )-2-amino-5-phosphonopentanoicacid (APV), 100 µM] and IPSP (GABA_A: bicuculline 10 µM and GABA_B:2-hydro-saclofen 100 µM) activity. The dihydropyridine, nitrendipine,was also used (10-20 µM) to determine whether L-type Ca²⁺ channels contributed to synaptically evoked depolarizations.Unless otherwise stated, a single preparation was used for eachdrugapplication.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We studied the synaptic responses evoked by OT stimulation of 311 LGN cells in rats that were 1-24 days old. Of these, 20responses were recorded extracellularly and 291 using intracellulartechniques. For the latter, cells exhibited a resting membranelevel of $-$ 60 to $-$ 65 mV, an input resistance of 300-500 M $Omega$ , actionpotentials >60 mV, and near-threshold synaptic responses >3mV.

Single-unit extracellular recordings indicated that developing LGN cells exhibit three distinct firing modes in response toOT stimulation. Examples of these modes are shown in Fig. 1A.At relatively low stimulus intensities (0.1-0.3 mA), OT stimulationevoked a single action potential. This is the typical responseobserved in the adult (Burke and Sefton 1966; Lo and Sherman 1991)and one that we consistently observed between P10 and 24 (n =8), even when higher stimulus intensities were employed. However,at ages earlier than P10 (n = 12), higher levels of stimulationelicited two additional firing patterns. A moderate increase instimulus intensity (2-5 times above threshold), gave rise to ashort train of spikes that was 100-300 ms in duration. Higherlevels of stimulation (5-10 times above threshold) produced asustained discharge (300-1,000 ms) composed of spikes with variableamplitude. Intracellular whole cell recordings shown in Fig. 1Bdepict the underlying synaptic events that correspond to eachof these response modes. Note the striking similarity in the extracellularresponses of Fig. 1A with the intracellular ones of Fig. 1B. Weaklevels of stimulation produced a conventional EPSP that had asingle spike riding its peak. Moderate levels of stimulation produceda somewhat longer depolarization that gave way to a short trainof spikes. Higher levels of stimulation elicited a long-lasting(300-1,300 ms), slow decaying (<0.01 mV/ms) depolarization (25-40mV). Riding the crest of this response was a train of spikes ofvariable amplitude. We refer to this response profile as the plateaupotential. In close to half of all cells tested between P1 and24 (139/291, 48%), suprathreshold levels of OT stimulation evokeda plateau potential. Representative examples of plateau potentialsare shown in Figs. 3-7 and 10. However, as shown in Fig. 2, the incidenceof the plateau potential declined with age. At P1-2, 90.6% ofthe encountered cells (29 of 32 cells) exhibited a synapticallyevoked plateau potential. By P13-14, the incidence dropped to43.5% (20 of 46 cells) and by P20 to <1% (1 of 12 cells). Althoughthe incidence declined with age, we did not detect any systematicchanges with age in either the duration or amplitude of the plateaupotential. These parameters varied considerably within and betweencells and were influenced by several factors including, membranelevel (Fig. 3), the nature of EPSP and IPSP activity (Figs. 4and 5), stimulus intensity (Figs. 6-8), and the degree of spatialand temporal summation present (Figs. 6-8 and 10). These factorsand the manner in which they influenced the plateau potentialare described in detail in the following text.

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Fig. 1. Synaptic transmission in developing lateral geniculate nucleus (LGN) cells. A: extracellular recordings from a single LGN cell at P2. Electrical stimulation of optic tract (OT) evokes 3 different response patterns. Left: at stimulus threshold, OT stimulation evokes a single spike. Middle: moderate intensity levels (2-5 times greater than value in left trace) elicits a short train of spikes. Right: stronger levels of stimulation (5-10 times greater than value in left trace) gives rise to a sustained discharge pattern that contains spikes of varying amplitude. B: whole cell voltage recordings showing the synaptic responses of a P3 LGN cell obtained under a similar stimulation protocol. Left: at or near threshold, OT stimulation evokes an excitatory postsynaptic potential (EPSP) that has a single spike riding its peak. Middle: moderate stimulus levels; gives rise to a large EPSP that has 3 spikes riding its peak. Right: at strong stimulus levels, OT activation elicits a high-amplitude (>30 mV), long-lasting (>300 ms) depolarization (plateau potential) that contains a long train of spikes.

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Fig. 2. Incidence of the plateau potential as a function of age. Each point shows the percentage of cells exhibiting a plateau potential at various postnatal ages. Between 12 and 46 cells were recorded at each age.

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Fig. 3. Pharmacology and voltage dependency of the plateau potential. A: control responses showing postsynaptic activity at 2 different membrane levels. At $-$ 65 mV, strong stimulation of OT evoked a plateau potential. At more hyperpolarized level of $-$ 93 mV, the same level of stimulation evoked a large postsynaptic potential. B: recordings from the same cell after drop application (10 µM) of nitrendipine. At $-$ 65 mV, this L-type Ca²⁺ antagonist abolishes the plateau potential while leaving the underlying EPSP/IPSP intact. The EPSP has a short early peak (20 mV) that is followed by 2 IPSPs, an early short-lasting hyperpolarization and a late long-lasting one. At $-$ 105 mV, a large postsynaptic potential is present that is comparable in amplitude (45 mV) to the potential recorded under control conditions at $-$ 93 mV.

Pharmacological experiments indicate the plateau potential was mediated by the activation of high-threshold L-type Ca²⁺ channels. In each of 13 cells tested, the L-type Ca²⁺ channel antagonist, nitrendipine blocked the expression of theplateau potential (Figs. 3, 4A, and 7B). Cells treated with nitrendipinestill maintained robust EPSP activity. For example, at membranelevels of $-$ 60 to $-$ 65 mV and at stimulus intensities strong enoughto evoke a plateau potential, EPSPs had peak amplitudes between12 and 23 mV. Figure 3 depicts a cell in which nitrendipine blockeda plateau potential. At a resting level of $-$ 65 mV, strong stimulationof OT evoked a large plateau potential. When the membrane levelwas hyperpolarized to $-$ 93 mV (Fig. 3A), the underlying EPSP, whilequite large (40 mV), was unable to trigger a plateau potential.Figure 3B shows the application of nitrendipine abolished theplateau potential but left the underlying EPSP/IPSP event intact.At $-$ 65 mV, this EPSP has a peak amplitude of 20 mV but a relativelyshort duration (20 ms). The duration of the EPSP was curtailedby the presence of IPSP activity (see also Fig. 5A). It was alsopossible to evoke a large EPSP at a hyperpolarized membrane potentialof $-$ 105 mV (Fig. 3B) during nitrendipine application. This EPSPwas comparable in amplitude and duration to those evoked undercontrol conditions (Fig. 3A). These results indicate the plateaupotential is mediated by L-type Ca²⁺ channels and that EPSP-induced depolarizations are needed toactivate this channelactivity.

The example in Fig. 3A also underscores the voltage dependency of plateau potential activation. At a resting membrane level $-$ 65 mV, strong stimulation of OT evoked a large plateau potential.However, when the membrane was hyperpolarized to $-$ 93 mV, the samelevel of stimulation was not sufficient to evoke a plateau potential.Instead, OT stimulation evoked a conventional EPSP. Typically,we found at resting levels of $-$ 60 to $-$ 65 mV, EPSPs >20-25 mV (therebydriving the membrane potential above $-$ 40 mV) was sufficient toactivate plateaupotentials.

Another critical factor in determining the activation of the plateau potential was EPSP duration. As shown in Fig. 4A, nitrendipinecompletely abolished the plateau potential while leaving the underlyingEPSP intact. This EPSP, like those of all thalamic relay cells,contained two overlapping components, an early fast one that relieson non-NMDA receptor activity and a slower, longer voltage-dependentone that is mediated by NMDA receptor activity (Scharfman et al.1990). We found that EPSPs recorded in the presence of nitrendipine(Fig. 4A), or those evoked at relatively low levels of stimulation(Fig. 4B), contained an APV-sensitive NMDA component. In eachof 12 cells tested, when the NMDA antagonist APV was applied toblock the late excitatory component, EPSPs were no longer sufficientin duration to activate a plateau potential. A representativeexample is shown in Fig. 4C. Under control conditions, strongstimulation evoked a large plateau potential (Fig. 4C, trace 1).However, in the presence of APV, the same level of stimulationwas not sufficient to evoke a plateau potential (Fig. 4C, trace2). These results also indicate the remaining non-NMDA componentof the underlying EPSP was not sufficient in duration to activatethe plateau potential. This was true whether high-intensity, singleshocks (Fig. 4C) or repetitive shocks (3 pulses at 20 Hz) wereemployed (n = 3).

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Fig. 4. Excitatory postsynaptic events underlying the activation of the plateau potential. A: synaptic responses recorded in same cell before (1) and after (2) the application of nitrendipine (10 µM). The L-type Ca ²⁺ channel antagonist abolishes the plateau potential while leaving the underlying EPSP intact. B: synaptic responses evoked at a relatively weak stimulus intensity before (1) and after (2) APV (100 µM) application. APV reduces the overall amplitude and duration of EPSP, blocking the slow-rising late, NMDA component and preventing spike discharge. C: synaptic responses evoked before (1) and after (2) the application of APV. In the control response (1), the EPSP evokes a plateau potential. Application of APV (2) blocks the NMDA component of EPSP that prevents the activation of the plateau potential. The non-NMDA receptor component persists but fails to activate the plateau potential.

We also examined how inhibitory synaptic activity influenced the plateau potential. Even at early postnatal ages (P0-10),many synaptic responses were composed of EPSP/IPSP pairs (Crunelliet al. 1988; Lo and Sherman 1991). A typical example is shownin Fig. 5A. IPSP activity evoked at low levels of stimulation(i.e., below the level required to activate plateau potentials)often times contained both an early short-duration and a latelong-lasting hyperpolarization (Fig. 5A, top). The former is mediatedby GABA_A and the latter by GABA_B receptor activation (Crunelliet al. 1988). Both components have reversal potentials at membranelevels more negative than $-$ 90 mV (Fig. 5A, bottom). Figure 5Bshows the pattern of EPSP/IPSP activity at low, moderate, andstrong levels of OT stimulation. Weak OT stimulation (Fig. 5B,trace 1) evoked a response profile similar to that shown in Fig.5A. At moderate and strong levels of stimulation, these inhibitoryresponses become more difficult to see (Fig. 5B, traces 2 and3) because of the activation of a plateau potential. Evidencefor an early inhibitory response appears as a notch that precedesthe plateau potential (see Fig. 5B, *). However, the late inhibitorycomponent cannot be delineated because it is masked by the slow-decayof the plateau potential. To better understand the manner in whichinhibitory activity modulates the expression of the plateau potential,we recorded synaptic responses after the application of selectiveGABA antagonists (n = 9). Figure 5C shows that GABA_A activityaffected the stimulus threshold required for the activation ofthe plateau potential. Weak levels of stimulation evoked an EPSP/IPSPpair (Fig. 5C, trace 1). After GABA_A blockade with bicuculline(Fig. 5C, trace 2), the same stimulus evoked a plateau potential(n = 5). These results suggest that GABA_A activity affects theintensity of OT stimulation needed to evoke the plateau potential,perhaps by truncating the amplitude and/or duration of the underlyingEPSP (Crunelli et al. 1988; Ramoa and McCormick 1994) (see alsoFigs. 5A and 3B). Figure 5D shows that GABA_B activity modulatedthe duration of plateau potential. Strong stimulation of OT evokeda large but relatively brief plateau potential (Fig. 5D, trace1). The application of the GABA_B antagonist, 2-hydroxysaclofen,increased the duration of the plateau potential by ~40% (n = 4),largely by slowing down its rate of decay (Fig. 5D, trace 2).

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Fig. 5. Inhibitory postsynaptic events underlying the activation of the plateau potential. A: example of EPSP/IPSP pair evoked by weak levels of OT stimulation. Top: at resting levels, IPSP activity is composed of an early fast event that immediately procedes the EPSP and a slower longer event that follows the early IPSP. Bottom: IPSPs reverse at membrane levels more of $-$ 110 mV. B: 3 responses at progressively larger stimulus levels depicting the nature of GABA activity in relation to the plateau potential. Low level of stimulation evokes an EPSP/IPSP pair (1). The IPSP contains an early, short (GABA_A) and long-lasting (GABA_B) hyperpolarization. At higher levels of stimulation, the early IPSP is still apparent (see *), but the late one is masked by the plateau potential. C: synaptic response evoked by weak stimulation, before (1) and after (2) GABA_A receptor blockade by bicuculline (10 µM). Weak stimulation (1) evokes an EPSP/IPSP pair. After GABA_A blockade with bicuculline (2), the same weak stimulus evokes a plateau potential. D: plateau potentials evoked at high-intensity levels before (1) and after (2) GABA_B blockade with 2-hydrosaclofen (100 µM). Blockade of GABA_B increases the duration of the plateau potential.

In summary, the expression of the plateau potential relied on excitatory synaptic responses that result in a strong and sustainedmembrane depolarization, whereas inhibitory responses influencedthe intensity of OT stimulation needed to evoke the plateau potential(GABA_A activity) or the duration of the plateau potential (GABA_Bactivity).

At young postnatal ages, increased membrane depolarization was readily accomplished by the spatial (Figs. 6 and 7) and temporalsummation of EPSPs (Fig. 10). The extent to which EPSPs summatespatially are best illustrated by examining synaptic responsesat different stimulus intensities (Allen et al. 1977; Bartlettand Smith 1999; Chen and Regehr 2000; Mariani and Changeux 1981;Mock et al. 1997; O'Brien et al. 1978). In developing LGN cells,a systematic increase in stimulus intensity above threshold ledto incremental increases in EPSP amplitude and the subsequentactivation of a plateau potential. Representative examples areshown in Fig. 6, A and B. Numbered traces depict a series of responsesevoked by progressively larger stimulus intensities (range, 0-1.0mA, 0.9- to 1.2-mA steps). EPSP amplitude grew incrementally,and when amplitudes in excess of 30 mV were reached, plateau potentialsoften emerged. These discrete increases in EPSP amplitude in responseto elevations in stimulus intensity are taken to reflect the successiverecruitment of active inputs innervating a single cell (Allenet al. 1977; Bartlett and Smith 1999; Chen and Regehr 2000; Marianiand Changeux 1981; Mock et al. 1997; O'Brien et al. 1978). WhenEPSP amplitude is measured and plotted as a function of stimulusintensity, it can be used to obtain estimates in the number ofretinal inputs converging on a single LGN cell (Chen and Regehr2000; see also Bartlett and Smith 1999; Mock et al. 1997). Examplesof such plots and corresponding responses at different ages areshown in Figs. 7 and 8. At early ages, such as P3 and P8, a systematicelevation in stimulus threshold led to a step-wise increase inEPSP or EPSC amplitude, and as shown in Fig. 7A, the activationof a plateau potential. The graded steps in amplitude are betterillustrated when the plateau potential is blocked pharmacologically(Fig. 7B) or prevented by voltage clamping (Fig. 7C). Taken together,the steps evident in the amplitude by stimulus plots of Fig. 7show these cells received input from 7 to 10 retinal ganglioncells. By contrast, the responses from older animals revealedthis feature of retinogeniculate connectivity was transient. Figure8 shows that at P18 and P19, cells had fewer inputs (1-4). Asa result, they showed less spatial summation and lacked plateaupotentials.

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Fig. 6. Spatial summation of EPSPs evokes the plateau potential. A and B: records from 2 cells showing responses (superimposed) to an increase in stimulus intensity. A progressive increase in stimulus intensity (range, 0-1.0 mA, 0.9- to 1.2-mA steps) leads to a step-wise increase in EPSP amplitude. At high stimulus intensities, inputs summate and evoke plateau potentials. Numbered traces correspond to responses evoked at progressively higher levels of stimulation.

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Fig. 7. Synaptic responses to incremental increases in stimulus intensity at P3 and P8. Left: representative responses over the range of stimulus intensities tested. Numbered traces represent responses at successively higher levels of stimulation. The superimposition of responses underscores the successive recruitment of additional retinal fibers with increasing levels of stimulus intensity. Right: plots showing peak EPSP (A and B) or EPSC (C) amplitude as a function of stimulus intensity. A progressive increase in stimulus intensity produces a step-wise increase in EPSP amplitude. Each interval reflects the activation of an additional input. The steps evident in the amplitude by stimulus plots suggest these cells received input from 7 to 10 retinal ganglion cells. A: current-clamp recording showing that at high levels of stimulation EPSPs summate and evoke a plateau potential. B: current-clamp recording during bath application of nitrendipine. C: 2 examples of voltage-clamp recordings at holding potentials of $-$ 60 mV.

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Fig. 8. Synaptic responses to incremental increases in stimulus intensity at P18 and 19. Responses were obtained during the bath application of bicuculline (10 µM). Cells recorded at older ages exhibited fewer inputs.

Estimates of retinal convergence for 72 cells tested at different stimulus intensities (see preceding text) are summarizedin the scatterplot of Fig. 9. We found a significant reductionin retinal convergence with age (r = $-$ 0.64, P < 0.001). BeforeP7 we estimated that LGN cells receive input from as many as 7-12retinal ganglion cells (see also Chen and Regehr 2000). By P14,LGN cells begin to resemble their adult counterparts and receivefar fewer (between 1 and 4) inputs. Comparing the scatterplotof Fig. 9 with the plot of Fig. 2 reveals the loss of inputs atolder ages is accompanied by a reduced incidence in the plateaupotential. These results suggest the high degree of retinal convergenceoccurring at early ages provides a greater opportunity for spatialsummation, thereby increasing the probability that synaptic responseswill lead to the activation of the plateau potential.

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Fig. 9. Scatterplot showing the number of retinal inputs an LGN cell receives as a function of age. Each point represents a single cell.

, cells that shared the same number of inputs. $---$ , a significant reduction in inputs with increasing age (r = $-$ 0.64, P < 0.001).

The repetitive activation of optic tract reveals that the plateau potential could be evoked by the temporal summation of EPSPs.Figure 10A depicts the responses of an LGN cell to a 20-Hz trainof three stimulus pulses delivered at a constant stimulus intensity.The response to the initial first shock (Fig. 10A, trace 1) evokeda singular EPSP, while those generated by subsequent shocks (Fig.10A, traces 2 and 3) gave rise to plateau potentials. Figure 10Breveals the plateau potential could also be evoked by a combinationof spatial and temporal summation. A 20-Hz train of three stimuluspulses delivered at relatively low stimulus intensities (i.e.,levels that were unable to evoke a plateau potential when singleshock was employed) readily evoked a plateau potential. As statedin the preceding text, the plateau potential was most prevalentprior to eye opening, at times when spontaneous retinal activitytakes the form of periodic high-frequency burst discharges (Galli-Restaand Maffei 1990; Meister et al. 1991; Wong et al. 1993). To determinewhether such activity is sufficient for activating the plateaupotential, we recorded the synaptic activity evoked by a tetanusprotocol (50-Hz train for 1 s) designed to mimic early intrinsicretinal activity (n = 8). Figure 10C (top) shows this form of high-frequencystimulation led to a massive summation of EPSPs and evoked a long-lastingdepolarization (>1 min). Moreover, this tetanus-induced depolarizationwas mediated largely by L-type Ca²⁺ channel activation. Figure 10D (bottom) shows that nitrendipinegreatly reduced the amplitude and duration of this large depolarization(n = 3).

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Fig. 10. Temporal summation of synaptic responses evokes plateau potentials. A: repetitive shocks of a constant stimulus intensity delivered at 20 Hz produce a temporal summation of EPSPs. The response to the 1st shock (1) evokes an EPSP, while those evoked by subsequent shocks (2 and 3) gives rise to a plateau potential. B: a train of 3 stimulus pulses delivered at 20 Hz at progressively larger stimulus levels produces both the spatial and temporal summation of EPSPs. C: high-frequency stimulation (50 Hz, 1 s) evokes a long-lasting (~1 min) plateau potential. D: another example showing that a plateau potential evoked by tetanus is blocked by nitrendipine (20 µM). In C and D, the insets depict expanded traces taken during tetanus (see *) and Na²⁺ spikes are filtered for clarity.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Thalamic relay cells possess both low (T-type) and high (L- and N-type, and two $omega$ -conotoxin MVIIC-sensitive ones) thresholdCa²⁺ channels (Coulter et al. 1989; Hernandez-Cruz and Pape 1989;Huguenard 1996; Kammermeier and Jones 1997). At membrane levelsmore negative than $-$ 65 mV, depolarization activates a T-type currentthat leads to a large Ca²⁺-mediated triangular depolarization and burst firing (Jahnsenand Llinas 1984). The burst firing mode of relay cells has beenstudied extensively, serving as the primary basis for oscillatoryactivity during different behavioral (sleep) or pathological states(absence seizures) (McCormick and Bal 1997; Steriade et al. 1993).Prominent among the family of high-threshold Ca²⁺ channels for thalamic relay cells is the L-type (Budde et al.1998; Kammermeier and Jones 1997). These are activated at membranelevels that generally exceed $-$ 40 mV and result in a high-amplitudedepolarization that shoulders the Na⁺ spike. L-type Ca²⁺ channels are believed to regulate cell excitability, perhapshelping to support a tonic firing mode in relay cells (Budde etal. 1998, 2000). However, a more specific role during retinogeniculatesignal transmission has not been fully explored. Recent imagingstudies suggest they may play an important role in the modulationof synaptic responses. Although high-threshold Ca²⁺ channels generally reside on the soma (Munsch et al. 1997; Zhouet al. 1997), the L-type channel in particular tends to clusterat the base of dendrites (Budde et al. 1998), thereby puttingthem in close proximity to retinal terminals (Wilson et al. 1984).This arrangement puts them in an ideal position to affect thegain of retinally mediated activity (Budde et al. 1998). Indeed,we found that EPSP activity evoked by strong stimulation of theoptic tract activates L-type Ca²⁺ channels. Their activation triggers a high-amplitude, slow-decaying,sustained depolarization that rides atop the EPSP. We refer tothis event as a plateau potential. This event is virtually identicalto the synaptically evoked plateau potential recorded in neuronsof the developing rodent superior colliculus (Lo and Mize 2000)and shares some similarities to those reported in developing structuresof the brain stem (Rekling and Feldman 1997) and spinal cord (Morissetand Nagy 1999).

In some central synapses, L-type Ca²⁺ channels facilitate synaptic transmission by regulating transmitter release from presynapticterminals (e.g., Bonici et al. 1999; Jensen et al. 1999). However,we saw no evidence for such a role in LGN. The blockade of L-typeCa²⁺ activity with nitrendipine abolished the plateau potential butleft underlying postsynaptic events intact. The fact that EPSPsas well as IPSPs were not compromised by nitrendipine indicatesL-type Ca²⁺ channels modulate retinogeniculate transmission at postsynapticsites rather than at presynaptic ones (Budde et al. 1998, 2000;Munsch et al. 1997; Zhou et al. 1997).

To evoke the plateau potential, EPSPs were required to produce a strong and sustained membrane depolarization. Neither Na²⁺ spikes nor the early, fast AMPA component of EPSPs could triggerthe plateau potential. This suggests the synaptic activation ofthe plateau is both voltage and time dependent. We found at leastthree ways in which EPSP activity led to heightened membrane depolarizationand the activation of the plateau potential. These included NMDAreceptor activation, and the spatial and/or temporal summationof EPSPs. Interestingly, these events prevail during early postnatallife, a time when retinal afferents are actively sorting intoeye specific domains (Jeffery 1984). The timing of these eventsmay also explain why the plateau potential was developmentallyregulated, showing a high incidence at P1-7. For example, at earlypostnatal ages relay cells possess a prominent NMDA current withchannel kinetics that favor long open times and slower decay rates(Chen and Regehr 2000; Ramoa and McCormick 1994; Ramoa and Prusky1997, but see Hohnke et al. 2000). In rodents, these featuresof excitatory transmission are transient. By the time of naturaleye opening (P14-16) excitatory events are faster and shorter,in part because they have a larger AMPA-to-NMDA current ratioas well as faster NMDA decay times (Chen and Regehr 2000). Wealso found at young ages (<P7), relay cells receive input fromseveral (7-12) retinal ganglion cells. In fact, our estimatesseem conservative. Others report that developing LGN cells areinnervated by as many as 20 retinal ganglion cells (Chen and Regehr2000). This contrasts the adult state, where LGN cells are reportedto receive input from just one or a few retinal ganglion cells(Chen and Regehr 2000; Cleland et al. 1971; Hamos et al. 1987;Mastronarde 1987; Ursey et al. 1999). Such remodeling happensquickly during development. Between P14 and 24, we found morethan a threefold reduction in the number of retinal inputs innervatinga single LGN cell. It is conceivable that a change in electrotoniccompactness due to an increase in dendritic complexity led toa failure to detect weak synaptic inputs in mature cells. However,our estimates are in accord with other electrophysiological studiesshowing the receptive field properties of LGN cells are dominatedby one or a few retinal ganglion cells (Cleland et al. 1971; Mastronarde1987; Ursey et al. 1999). Moreover, retinal terminals form synapseson proximal regions of relay cell dendrites (Hamos et al. 1987;Wilson et al. 1984), thereby minimizing potential space clampproblems.

The high degree of retinal convergence coupled with heightened NMDA activity observed at early ages would certainly favorthe spatial (and temporal) summation of EPSPs and greatly increasethe likelihood that synaptic responses will lead to the activationof the plateau potential. The high degree of summation at earlydevelopmental ages may also minimize the influence of GABA-mediatedinhibition (Guyon and Leresche 1992), which we found to affectboth the threshold and duration of the plateaupotential.

The age-related decrease in the incidence of the plateau potential could also be due to nonsynaptic factors such as a developmentaldifference in the density of L-type Ca²⁺ channels or an inherent difference in channel kinetics betweenimmature and mature LGN cells. However, this possibility seemsunlikely. Both Ca²⁺-imaging and -electrophysiological studies indicate that maturerelay cells possess a high density of active L-type Ca²⁺ channels (Budde et al. 1998, 2000; Coulter et al. 1989; Hernandez-Cruzand Pape 1989; Huguenard 1996; Munsch et al. 1997; Zhou et al.1997).

Although in the present study we used electrical stimulation to evoke the plateau potential, it is reasonable to assume thatsuch activation occurs endogenously at early postnatal ages. Priorto eye opening, retinal ganglion cells exhibit a high degree ofspontaneous activity in the form of synchronous bursts that traverseacross the retina in a wave-like fashion (Galli-Resta and Maffei1990; Meister et al. 1991; Wong et al. 1993). This patterned retinalactivity is also capable of driving LGN cells to fire prolongedbursts of action potentials (Mooney et al. 1996). Such early spontaneousretinal activity also seems capable of activating the plateaupotential. Repetitive activation of OT fibers or the use of atetanus protocol that approximated the intrinsic activity of retinalganglion cells evoked a large and long-lasting depolarizationthat was mediated by L-type channel activation. The sustainednature of this Ca²⁺-mediated depolarization also suggests that early retinal activitycan support long-term changes in synaptic efficacy. Indeed, inboth LGN (Ziburkus and Guido 1999) and superior colliculus (Loand Mize 2000), L-type Ca²⁺ activity was necessary for the induction of tetanus induced changesin synaptic strength. Such associative changes are believed torepresent the "Hebbian" substrate for synapse stabilization andthe activity-dependent remodeling of retinofugal connections (Constantine-Patonet al. 1990; Cramer and Sur 1995).

Taken together, these results underscore the idea that the functional state of the developing retinogeniculate synapse iswell suited for the activity-dependent sequestration of Ca²⁺. Moreover, the activation of NMDA receptors need not be the solesource of Ca²⁺ during synaptic transmission, but a much larger and longer influxcan occur via the activation of L-type Ca²⁺ channels. The Ca²⁺ influx associated with the synaptically evoked plateau potentialcould play an important role in the experience-dependent modificationof the visual system, triggering a cascade of signal transductionpathways that lead to the maturation and stabilization of retinogeniculateconnections.

	ACKNOWLEDGMENTS

This study was supported by grants from the Whitehall Foundation and the National Eye Institute (RO1 12716-01A2) to W.Guido.

	FOOTNOTES

Address for reprint requests: W. Guido, Dept. of Cell Biology and Anatomy, LSU Health Sciences Center, 1901 Perdido St., NewOrleans, LA 70112 (E-mail: wguido{at}lsumc.edu).

Received 23 August 1999; accepted in final form 29 October 2001.

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Synaptic Mechanisms Regulating the Activation of a Ca2+-Mediated Plateau Potential in Developing Relay Cells of the LGN

0022-3077/02 $5.00 Copyright © 2002 The American Physiological Society

Synaptic Mechanisms Regulating the Activation of a Ca²⁺-Mediated Plateau Potential in Developing Relay Cells of the LGN