Ca2+-Permeable AMPA Receptors and Spontaneous Presynaptic Transmitter Release at Developing Excitatory Spinal Synapses

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The Journal of Neuroscience, October 1, 1999, 19(19):8528-8541

Ca²⁺-Permeable AMPA Receptors and Spontaneous Presynaptic Transmitter Release at Developing Excitatory Spinal Synapses
Jeffrey Rohrbough and Nicholas C. Spitzer
Department of Biology and Center for Molecular Genetics, University of California, San Diego, La Jolla, California 92093

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

At many mature vertebrate glutamatergic synapses, excitatory transmission strength and plasticity are regulated by AMPA andNMDA receptor (AMPA-R and NMDA-R) activation and by patterns ofpresynaptic transmitter release. Both receptors potentially directneuronal differentiation by mediating postsynaptic Ca²⁺ influx during early development. However, the development ofsynaptic receptor expression and colocalization has been examineddevelopmentally in only a few systems, and changes in releaseproperties at neuronal synapses have not been characterized extensively.We recorded miniature EPSCs (mEPSCs) from spinal interneuronsin Xenopus embryos and larvae. In mature 5-8 d larvae, ~70% ofmEPSCs in Mg²⁺-free saline are composed of both a fast AMPA-R-mediated componentand a slower NMDA-R-mediated decay, indicating receptor colocalizationat most synapses. By contrast, in 39-40 hr embryos ~65% of mEPSCsare exclusively fast, suggesting that these synapses initiallyexpress predominantly AMPA-R. In a physiological Mg²⁺ concentration (1 mM), mEPSCs throughout development are mainlyAMPA-R-mediated at negative potentials. Embryonic synaptic AMPA-Rare highly Ca²⁺-permeable, mEPSC amplitude is over twofold larger than at maturesynapses, and mEPSCs frequently occur in bursts consistent withasynchronous multiquantal release. AMPA-R function in this motorpathway thus appears to be independent of previous NMDA-R activation,unlike other regions of the developing nervous system, ensuringa greater reliability for embryonic excitatory transmission. Earlyspontaneous excitatory activity is specialized to promote AMPA-R-mediatedsynaptic Ca²⁺ influx, which likely has significant roles in neuronaldevelopment.

Key words: Ca²⁺-permeable AMPA receptors; NMDA receptors; developing excitatory synapses; spontaneous transmitter release; mEPSCs; receptor colocalization; presynaptic mEPSC bursts

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

AMPA and NMDA glutamate receptor subtypes (AMPA-R and NMDA-R) are colocalized postsynaptically at many mature central glutamatergicsynapses and are activated concurrently by synaptic transmitterrelease (Nicoll et al., 1990). AMPA-R are used for fast excitatorysignaling, whereas NMDA-R-mediated Ca²⁺ influx is believed to underlie multiple forms of developmentaland activity-dependent synaptic plasticity, including long-termpotentiation (LTP). Because NMDA-R are usually not functionaluntil the postsynaptic membrane is depolarized by AMPA-R activation,the proximity and degree of coactivation of both receptors atindividual excitatory synapses have important implications forfunction and plasticity at both developing and maturesynapses.

A number of developmental studies support a predominant role for NMDA-R in initial glutamatergic transmission (Constantine-Patonand Cline, 1998; Feldman and Knudsen, 1998). NMDA-R are detectedfirst at developing excitatory synapses in mammalian hippocampus(Durand et al., 1996; Liao et al., 1998), sensory cortex (Crairand Malenka, 1995; Isaac et al., 1997) and spinal cord (Ziskind-Conhaim,1990), and in Xenopus optic tectum (Wu et al., 1996). NMDA-R synapticcurrents are also more prolonged initially than at later stages(Carmignoto and Vicini, 1992; Hestrin, 1992), and NMDA-R-mediatedCa²⁺ influx may serve multiple roles in synaptic development (Sheetzand Constantine-Paton, 1994; Sheetz et al., 1997; Constantine-Patonand Cline, 1998). Functional AMPA-R expression may be inducedat initially "silent" synapses by NMDA-R activation (Malenka andNicoll, 1997). However, it remains unclear how NMDA-R providethis induction signal because transmission at immature, pure NMDA-Rsynapses usually is revealed only at depolarized potentials orin Mg²⁺-free saline. Depolarizing GABA responses may have such a rolein some immature neurons (Ben-Ari et al., 1997; Constantine-Patonand Cline, 1998).

Alternatively, Ca²⁺-permeable AMPA-R may mediate Ca²⁺-dependent developmental and plastic synaptic changes independently of NMDA-R.Ca²⁺-permeable AMPA-R are expressed first on cultured rat hypothalamicand Xenopus spinal neurons (van den Pol et al., 1995; Gleasonand Spitzer, 1998) and underlie mature excitatory transmissionin chick cochlear nucleus (Otis et al., 1995). Synaptic AMPA-Rfunction can be modulated directly by postsynaptic AMPA-R-mediatedCa²⁺ entry (Gu et al., 1996; Jia et al., 1996; Mahanty and Sah, 1998),but little is known about the developmental appearance of Ca²⁺-permeable AMPA-R at embryonic synapses in vivo. Additionally,few studies have examined changes in patterns of presynaptic transmitterrelease (Gao et al., 1998; Wall and Usowicz, 1998) that may influencethe contribution of AMPA-R and NMDA-R to developing synapticresponses.

We use whole-cell recordings of spontaneous mEPSCs to analyze functional properties of glutamate receptors at developing excitatoryspinal synapses in Xenopus embryos and larvae. We find that bothAMPA-R and NMDA-R are colocalized at most mature larval synapses.At embryonic stages, mEPSCs are mediated almost entirely by AMPA-Rat negative membrane potentials, have larger amplitudes, and frequentlyoccur in bursts, differing from mEPSC activity at mature stages.Furthermore, AMPA-R are permeable to Ca²⁺ from their earliest detection, suggesting that AMPA-R activationprovides a pathway for Ca²⁺ influx that may serve an important role in the plasticity ofdeveloping spinalsynapses.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Spinal cord preparations. Experiments were performed on Xenopus laevis embryos and larvae at developmental stages between39 hr after fertilization and 8 d of age. Animals were stagedby standard morphological criteria (Nieuwkoop and Faber, 1967),and the results are grouped into three developmental categoriesthat we refer to as embryonic, early larval, and mature larvalstages. The embryonic stage is 39-40 hr after fertilization (morphologicalstage 31/32), which precedes hatching by ~15 hr. The early larvalstage (~54 hr; stage 37/38) corresponds to the stage of hatchingand the beginning of free swimming (Sillar and Roberts, 1988).Mature larvae were 5-8 d ofage.

Spinal cords were dissected and secured for recording by using methods similar to those reported previously (Rohrbough andSpitzer, 1996). Larvae were decapitated in recording solutioncontaining 0.1 µg/ml TTX (see below) and pinned into small Sylgard(Dow Corning, Midland, MI) wells in 35 mm culture dishes. Trunkskin and dorsal tail muscle were removed with the aid of an electrolyticallysharpened tungsten needle and fine forceps. Then the needle wasused to lightly score the meningeal membranes along the dorsalmidline of the spinal cord to expose the cell bodies of dorsaland dorsolateral neurons. Embryos were removed from their jellymembranes in recording solution containing TTX and 50 µM d-tubocurareto inhibit muscle movement, and the spinal cord was transectedwith forceps just caudal to the hindbrain. Trunk skin was removedwith needle and forceps, and gut tissue was cut away to the ventraledge of the myotomal muscle. Preparations were pinned throughthe muscle and notochord into a Sylgard well and, in most cases,exposed for 5-10 min to collagenase B (0.1 mg/ml; Boehringer Mannheim,Indianapolis, IN), which facilitated the dissection of dorsalmyotomal muscle from the spinal cord. Collagenase-containing solutionthen was replaced with fresh recording solution. We did not observeany differences in mEPSC properties in collagenase-treated versusuntreatedpreparations.

Electrophysiological recordings. Preparations were visualized at 500× magnification with interference contrast optics on anupright Zeiss microscope and superfused continuously with recordingsaline (~2 ml/min) in a bath volume maintained at ~0.5 ml. Whole-cellvoltage-clamp recordings (Hamill et al., 1981) of spontaneousminiature synaptic currents (mEPSCs) and kainate-evoked whole-cellcurrents were made with a Dagan 8900 amplifier (Dagan, Minneapolis,MN). Recording pipettes were pulled from 100 µl capillaries (DrummondScientific, Broomall, PA) with a Flaming/Brown electrode puller(model P-87, Sutter Instruments, Novato, CA) and had 3-5 M $Omega$ resistanceswhen filled with pipette solution. Seals were formed on exposedand clearly visualized cell bodies (10-20 µm diameter) by applyinggentle suction to the pipette, followed by a manual suction pulseto achieve whole-cell configuration. All recordings were obtainedfrom neurons positioned in the dorsal quarter of the spinal cordjust lateral to Rohon-Beard sensory neurons. These neurons aremost likely either dorsolateral commissural or dorsolateral ascendinginterneurons (Roberts and Clarke, 1982; Clarke and Roberts, 1984;Roberts et al., 1988; Sillar and Roberts, 1988; Sillar and Simmers,1994). By previous convention (Sillar and Simmers, 1994; Rohrboughand Spitzer, 1996) they are denoted here as dorsolateral interneurons(DLi).

DLi receive excitatory glutamatergic input from Rohon-Beard neurons as well as inhibitory input from other interneurons (Dale,1995). In initial recordings from mature larvae in standard externalsaline (see below) containing no added drugs, several classesof spontaneous synaptic currents were observed consistently. Themost frequent class of currents reversed near the expected Cl equilibrium potential, had monoexponential decay time constantsof ~10 msec, and were abolished by 1 µM strychnine, indicatingthat they were glycinergic mIPSCs. To unambiguously isolate glutamatergicmEPSCs, we made all recordings that were analyzed for this studyin the presence of 0.1 µg/ml TTX, 1 µM strychnine, and 50 µM bicucullineto block action potential-evoked synaptic currents and mIPSCsmediated by glycine or GABA, respectively. mEPSCs were recordedat holding potentials between $-$ 70 and +60 mV. Series resistance(R_S) estimated from current transients (digitized at 50 kHz) generatedby a 10 mV depolarizing step from $-$ 70 mV was typically 4-10 M $Omega$ .Because the maximum amplitude of mEPSCs was several hundred picoamps,electronic compensation for R_S was usually not applied. Whole-cellaccess was monitored at regular intervals during recordings, anddata were discarded if R_S was not stable. Whole-cell responsesto kainate were evoked by focal pressure application (100-200msec, ~3 psi) of 500 µM kainic acid in external saline, usinga patch pipette positioned 30-40 µM from thecell.

Data acquisition and analysis. Continuous amplified current signals were filtered at 1 kHz and stored on videotape (Neurocordermodel DR-390, Neuro Data Instruments, New York, NY). Selectedportions were digitized later at 5 kHz by using DMA TL-1 interfacehardware and pClamp Fetchex 5.5 software (Axon Instruments, FosterCity, CA). mEPSC detection and sorting were performed with analysissoftware (ACSPLOUF) written and generously provided by Dr. PierreVincent (University of California, San Diego), described elsewhere(Vincent and Marty, 1993). Briefly, a user-defined detection windowcaptured current transitions when they exceeded a threshold abovebaseline within a specified interval of three to four digitizedpoints (0.6-0.8 msec). The detection threshold typically was setat 6-7 pA. Peak amplitude and time-to-peak for each event weredetermined relative to the preceding portion (2-5 msec) of thewindow, which was averaged and assigned as baseline. Each detectedevent was displayed on a computer monitor along with its idealizedamplitude and rise time and visually reviewed so that noise, superimposedevents, and obvious artifacts could be rejected. In most cases,>100 mEPSCs were collected under control conditions as well asfor each pharmacological condition that was assayed, except forAMPA-R antagonists. Cells for which <50 mEPSCs were recorded incontrol saline (usually embryonic neurons) were excluded fromanalysis. For recordings in Mg²⁺-free saline, the set of accepted events for each record thenwas reviewed and sorted further into several kinetic categories(i.e., fast, dual, slow). The individual events assigned to eachcategory, numbering from between 5 and 10 to several hundred events,were aligned on the rising phase and averaged to generate a meanmEPSC. The rise time, peak amplitude, and decay kinetics of themean mEPSC reliably reflected the properties of individual mEPSCsand provided a convenient method for illustrating overall amplitudeand kinetic properties of mEPSCs during development. Peak amplitudesand decay time constants of mean mEPSCs were measured with Clampfit6 analysis software (Axon Instruments). For recordings in 1 mMMg²⁺, mEPSC kinetic properties were nearly homogeneous, and mean amplitudetherefore was determined by averaging the amplitudes of all mEPSCsin the record. In a subset of these recordings, mEPSCs also weredivided into fast and dual categories. Dendritic filtering didnot appear to contribute significantly to mEPSC variability, becauseboth small- and large-amplitude fast mEPSCs had similar rise timesand decaykinetics.

For a subset of recordings (eight embryonic neurons and nine mature neurons) made at $-$ 70 mV in 1 mM Mg²⁺, a modified event-detection protocol was applied to analyze propertiesof mEPSC bursts, in which successive events were separated bybrief intervals. The width of the event detection window was reducedto four digitized points (0.8 msec), with the baseline for eachevent determined by a single point preceding the threshold crossing.Using these parameters, we reliably detected and measured successivepeaks and interpeak intervals as brief as 0.8-1.0 msec. Rare mEPSCsseparated by briefer intervals or those with nearly superimposedrising phases were not resolved as distinct events. No correctionwas made for underestimated peak amplitudes of mEPSCs occurringon the falling phase of the preceding event. However, becausefast mEPSC lifetime was <2 msec (~0.4 msec rise times and ~1 msecdecay constants), amplitude errors were limited to those eventspreceded by intervals <2 msec. These mEPSCs represented only asmall fraction of all events occurring in bursts, which we arbitrarilydefined as mEPSCs separated by <20msec.

Kainate-evoked whole-cell currents were recorded at potentials from $-$ 90 to +60 mV, digitized directly to disk at 1 kHz, andanalyzed withpClamp6.

Reversal potential measurements and determination of calcium permeabilities. Estimations of relative Ca²⁺ permeability of AMPA receptors were made by using the Goldman-Hodgkin-Katzequation extended to accommodate divalent cations, with the assumptionthat Cs⁺, K⁺, and Na⁺ are equally permeant (Mayer and Westbrook, 1987; Gilbertson etal., 1991). Ionic activity estimates rather than concentrationswere used for these calculations, using activity coefficientsof 0.8 for Cs⁺, K⁺, and Na⁺ and 0.5 for Ca²⁺ (Jahr and Stevens, 1993). Liquid junction potentials were measured(Neher, 1992) between the pipette and bath solutions for eachcombination of solutions used in reversal potential experimentsand varied between $-$ 5 and $-$ 9 mV. Corrections for liquid junctionpotentials and R_S errors were applied to measured reversalpotentials.

Solutions and drugs. The standard external recording solution contained (in mM): 125 NaCl, 3 KCl, 2 CaCl₂, and 5 HEPES, pH7.4, as well as TTX (0.1 µg/ml), bicuculline (50 µM), strychnine(1 µM), and d-tubocurare (50 µM). MgCl₂ (1 mM) was added for recordingsin the presence of Mg²⁺. Glycine (10 µM), a required co-agonist for NMDA-R activation,was included in the external solution in some experiments. Solutionswere changed by manually switching a four-way stopcock valve (Hamilton,Reno, NV). The time to exchange the bath was estimated to be 40-60sec by measuring changes in liquid junction potential with anopen recording pipette while exchanging test solutions. To ensurecomplete exchange during mEPSC recordings, we allowed ~2 min foreach solution change. In experiments that used the selective antagonistsGYKI 53655 and APV, complete blockade usually was achieved afterseveral minutes of drug perfusion, but much longer periods (>10min) of washing were necessary for complete or nearly completereversal, particularly for GYKI (see Fig. 3). It also was difficultto reverse the effects of Mg²⁺, which blocks NMDA-R in Xenopus spinal neurons with a K_D of ~20µM (Zhang and Auerbach, 1995), even after extensive washing insaline with no added Mg²⁺. Therefore, once these antagonizing agents had been applied,we avoided making recordings in standard saline from a secondcell in the samepreparation.

mEPSC reversal potential measurements were made in external salines containing 1 or 20 mM Ca²⁺. The 1 mM Ca²⁺ solution contained (in mM): 95 NaCl, 3 KCl, 1 CaCl₂, 1 MgCl₂,30 N-methyl-D-glucamine-Cl (NMG-Cl), 50 µM APV, and 5 HEPES, pH7.4. In the 20 mM Ca²⁺ solution, NMG-Cl was replaced with 20 mM CaCl₂ to maintain aninvariant concentration of permeable monovalent cations. CdCl₂(100 µM) was included to reduce current noise at depolarized voltagescaused by Ca²⁺ conductances, improving the resolution of mEPSCs near the reversalpotential. In cultured spinal neurons 200 µM Cd²⁺ has no detectable effect on NMDA receptor current amplitude andreduces AMPA receptor current by no more than 13% (Gleason andSpitzer, 1998). Kainate reversal potentials were recorded in 0-Na⁺ external saline containing (in mM): 95 NMG-Cl, 20 CaCl₂, 3 KCl,1 MgCl₂, and 5 HEPES, pH 7.4.

Standard pipette solution contained (in mM): 120 CsCl, 5 EGTA, 2 Mg-ATP, and 10 HEPES, pH 7.4. KCl was substituted for CsClin the patch solution in some recordings; no differences in mEPSCproperties were observed between these two solutions. NaCl, KCl,MgCl₂, and CaCl₂ were obtained from Fisher Scientific (Tustin,CA) and HEPES from Research Organics (Cleveland, OH). Kainate,CNQX, and APV (2-amino-5-phosphonovaleric acid) were obtainedfrom Research Biochemicals (Natick, MA). GYKI 53655 is a 2,3-benzodiazepinecompound that is a highly selective noncompetitive antagonistof AMPA-preferring receptors without effect on kainate-preferringreceptors (Donevan and Rogawski, 1993; Zorumski et al., 1993;Paternain et al., 1995). GYKI was a generous gift of Dr. D. Leander(Lilly Research Laboratories, Indianapolis, IN). Other chemicalsand drugs were obtained from Sigma (St. Louis,MO).

Statistics. The two-tailed Student's t test was used for statistical analysis, and p values $<=$ 0.05 were taken to be significant.Variability in mEPSC amplitudes recorded in each neuron is reportedas SD. All other data, including mean SDs, are reported as mean±SEM.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Three classes of spontaneous mEPSCs are evident in dorsolateral interneurons of mature larvae in the absence of Mg²⁺

Whole-cell recordings of spontaneous mEPSCs were made from cell bodies of visually identified neurons in the dorsolateralspinal cord (Fig. 1). These DLi (Sillar and Simmers, 1994; Rohrboughand Spitzer, 1996) are likely either dorsolateral commissuralor ascending interneurons (Roberts and Clarke, 1982; Clarke andRoberts, 1984; Sillar and Roberts, 1988).

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Figure 1. Excitatory synapses on dorsolateral interneurons (DLi) are examined in intact Xenopus embryonic and larval spinal cords. A schematic representation of neurons in the early larval spinal cord is shown. Glutamatergic mEPSCs described in this study originate from Rohon-Beard cells. The DLi also receive inhibitory input from other interneurons (data not shown) and make excitatory connections onto motoneurons. Whole-cell recordings were made between developmental stages 31 (39 hr after fertilization) and 48 (7-8 d) from interneurons identified by the superficial location of their cell bodies in the dorsolateral spinal cord.

In mature (5-8 d) larvae three types of mEPSCs, distinguishable by their peak amplitudes and kinetic properties, are observedin most recordings from DLi held at $-$ 70 mV in Mg²⁺-free saline containing 0.1 µg/ml TTX (Fig. 2A,B). These mEPSCsare categorized as "fast," "slow," or "dual" (dual component).Dual mEPSCs are most common, constituting 71 ± 2% of all mEPSCs(range, 62-82%; n = 16; Table 1). Dual mEPSCs are composed ofan initial fast component with a rapid rise time (mean rise time<300 µsec) and decay time constant of ~1 msec, followed by a smallerand much slower component of variable duration, in which singlechannel current transitions of $-$ 4 to $-$ 5 pA occasionally can beresolved (Fig. 2B). A minority (21 ± 2%; range, 10-38%) of mEPSCshaving only a fast current component also is observed in nearlyall (15 of 16) cells. Fast mEPSCs and the fast component of dualmEPSCs have mean peak amplitudes of $-$ 28 ± 2 and $-$ 34 ± 3 pA, respectively,and are kinetically indistinguishable (Fig. 2B,C, Table 1). mEPSCrise times and peak amplitudes exhibit only a slight, positivecorrelation (data not shown), indicating that they are not influencedsignificantly by electrotonic filtering. Both fast and dual mEPSCsalso are recorded at strongly depolarized potentials (+60 mV;Fig. 2C). In addition, a third class of slow, noisy mEPSCs resemblingthe slow component of dual mEPSCs is observed with a low incidence(8 ± 2%; range, 0-23%; n = 16) in most records (Fig. 2B1). SlowmEPSCs are initiated by the approximately synchronous openingof two to three individual channels of $-$ 4 to $-$ 5 pA amplitude.In addition, individual single channel openings by the same classof receptors (see below) can be resolved in many recordings. Becauseit was impossible to discern whether this channel activity resultsfrom synaptic receptor activation or from the diffusion of transmitterto nonsynaptic receptors, it is not included in mEPSC analyses.

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Figure 2. mEPSCs recorded from mature excitatory synapses are predominantly dual component in Mg²⁺-free saline. A, Continuous traces of mEPSCs recorded at $-$ 70 mV (bottom trace) and +60 mV (top trace). All recordings in this and subsequent figures were made in the presence of TTX (0.1 µg/ml), strychnine (1 µM), and bicuculline (50 µM) to block action potentials and mIPSCs. B, C, Examples of dual-component (dual mEPSCs), fast, and slow mEPSCs recorded at $-$ 70 mV (B1) and dual and fast mEPSCs recorded at +60 mV (C1). Dual mEPSCs, consisting of a fast initial current component followed by a variable slow decay, predominated at both potentials. B2, C2, Mean dual-component (n = 113, $-$ 70 mV; n = 49, +60 mV) and fast mEPSCs (n = 34, $-$ 70 mV; n = 3, +60 mV); slow mEPSCs were too infrequent to construct an average. Single-exponential (fast mEPSCs) and double-exponential (dual mEPSCs) fits are superimposed on the mean mEPSC traces. D, Distribution of fast, dual-component, and slow mEPSCs at both potentials. All data are from a single DLi in a 6 d larva.


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Table 1. Developmental changes in amplitudes and kinetics of mEPSCs recorded at $-$ 70 mV in Mg²⁺-free and 1 mM Mg²⁺-containing salines

To better quantify the properties of these three populations of mEPSCs at mature larval synapses, we constructed mean mEPSCsby averaging dual, fast, and slow mEPSCs recorded from each neuron(Fig. 2B2,C2). Mean dual mEPSCs in most cases are well fit bytwo exponentials, having fast time constants of 1.1 ± 0.1 msec(n = 16). The slow time constant of dual mEPSCs is 10-50 timeslonger at $-$ 70 mV (mean, 26.8 ± 5.4 msec; n = 16; Table 1), andis prolonged two- to threefold by depolarization to +60 mV (Fig.2B,C; n = 4). Although the slow current component of dual mEPSCsaverages only $-$ 8 to $-$ 10 pA in amplitude, it constitutes ~90% ofthe current area of the mean dual mEPSC. Mean fast mEPSCs arefit adequately in most cases by a single time constant (Fig. 2B,C)that does not differ significantly at $-$ 70 mV (0.8 ± 0.1 msec;n = 16) from the fast time constant of dual mEPSCs (Table 1).Because slow mEPSCs occur rarely and vary substantially in durationat $-$ 70 mV, their kinetic properties were notquantified.

mEPSCs at mature synapses are mediated by both AMPA-R and NMDA-R

To determine which glutamate receptor subtypes underlie mEPSCs at DLi synapses in mature larvae, we studied the effects ofspecific AMPA-R and NMDA-R antagonists. GYKI 53655 (25-50 µM),a highly selective noncompetitive antagonist of AMPA-R (Donevanand Rogawski, 1993; Zorumski et al., 1993; Paternain et al., 1995),completely and selectively abolishes both fast mEPSCs and thefast component of dual mEPSCs after several minutes of exposure,while sparing the slow current component (Fig. 3A,B; n = 6). Inthe presence of GYKI, the addition of 1 mM Mg²⁺, a voltage-dependent blocker of NMDA-R channels, abolishes theremaining slow mEPSCs at $-$ 70 mV, revealing occasional bursts ofsingle channel openings. These channel events have an estimatedconductance of ~50 pS (assuming a reversal potential of 0 mV;n = 3), which is close to the expected size for NMDA-R channelsundergoing periodic relief of Mg²⁺ blockade (Zhang and Auerbach, 1995). At strongly depolarizedpotentials (+30 to +60 mV) expected to relieve the Mg²⁺ blockade of NMDA-R, slow mEPSCs are revealed (n = 3) with decayconstants several-fold longer than at $-$ 70 mV (Fig. 3B; also 2B,C),demonstrating a positive effect of voltage on NMDA-R synapticcurrent decay similar to that reported previously (Hestrin, 1992).

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Figure 3. mEPSCs at mature excitatory spinal synapses are mediated by both AMPA-R and NMDA-R. A, B, GYKI and Mg²⁺ selectively block the fast and slow mEPSC components, respectively. A, Continuous traces of mEPSCs recorded at $-$ 70 or +60 mV, as indicated. B, Mean mEPSCs are shown for each corresponding segment of the recording. a, Dual-component mEPSCs predominate in control 0-Mg²⁺ saline. b, GYKI blocks fast mEPSCs and the fast component of dual mEPSCs; the mean mEPSC has a slow decay constant comparable to the slow component of the mean dual mEPSC in a. c, In the continued presence of GYKI the addition of Mg²⁺ blocks all mEPSCs at $-$ 70 mV (lower trace), although occasional single channel openings of 4-5 pA are observed that may be attributable to synaptic NMDA-R. At depolarized potentials (+60 mV; upper trace), outward mEPSCs with prolonged decay constants are evident. These results indicate that fast mEPSC components are mediated by AMPA-R, and the slow component is mediated by NMDA-R. d, Both dual-component and fast mEPSCs are recorded after >8 min washout of GYKI and Mg²⁺. C, D, APV selectively abolishes the slow mEPSC component. Traces (C) and averaged mEPSCs (D) at $-$ 70 mV are illustrated as in A and B. a, Dual-component and fast mEPSCs recorded in control 0-Mg²⁺ saline. b, In the presence of APV and GYKI all mEPSCs are abolished. c, After the washout of GYKI in the continued presence of APV, only fast mEPSCs are observed, which are indistinguishable from fast mEPSCs observed in control saline. A, B and C, D were recorded from two cells in different mature 7 d larvae; the recording in A and B was made in the presence of 10 µM glycine, which did not change the distributions of mEPSCs significantly (n = 4). Mean fast mEPSCs are averages of 7-21 events; other mean mEPSCs are averages of >50 events.

APV (50-100 µM), a specific NMDA-R antagonist, selectively abolishes the slow component of mEPSCs as well as background singleNMDA-R channel openings within 2-3 min exposure (n = 5). The meanmEPSC remaining in APV is indistinguishable from the control fastmEPSC at both negative and positive potentials (Fig. 3C,D). Theseresults demonstrate that the fast and slow mEPSC components aremediated by AMPA-R and NMDA-R,respectively.

Glycine is a required co-agonist for NMDA-R activation (Johnson and Ascher, 1987). The addition of 10 µM glycine to the externalsaline in recordings from mature DLi does not change the distributionof mEPSCs significantly (n = 4; data not shown), suggesting thatin control recordings glycine is present at endogenous levelssufficient to permit NMDA-R activation. Larval DLi also receivestrong glycinergic inhibitory synaptic input (Dale, 1995). Inrecordings from mature larvae in drug-free standard saline (datanot shown), we consistently observed frequent mIPSCs that wereabolished after the addition of 1 µM strychnine; thus endogenousglycine may be supplied by spontaneous release at nearby inhibitorysynapses.

mEPSCs at embryonic synapses are mediated predominantly by AMPA-R

To study the involvement of AMPA-R and NMDA-R at excitatory synapses during their development, we examined the pharmacologicaland kinetic properties of mEPSCs in DLi in stage 31/32 embryos(39-40 hr). This stage is ~13 hr after reflex movements are firstdetectable, but it precedes hatching and the free-swimming larvalstage by 15 hr (Nieuwkoop and Faber, 1967). mEPSC frequency atthese early stages of development is highly variable, and in somecells too few events were recorded for statistically significantanalysis. However, at $-$ 70 mV in Mg²⁺-free saline, all neurons in which activity is recorded exhibitboth fast mEPSCs with rapid rise times and decays and dual mEPSCswith slower decay components (Fig. 4; n = 5). The fast and slowcomponents of embryonic mEPSCs are blocked selectively by GYKI(Fig. 4A,B; n = 4) and Mg²⁺ (n = 3) or APV (n = 2), respectively (Fig. 4C,D), indicatingthat, as at mature synapses, they are mediated by AMPA-R and NMDA-R.

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Figure 4. mEPSCs at embryonic excitatory spinal synapses are mediated primarily by AMPA-R. A, B, GYKI and Mg²⁺ selectively block the fast and slow embryonic mEPSC components, respectively. A, Continuous traces of mEPSCs recorded at $-$ 70 mV. B, Mean mEPSCs for each corresponding segment of the recording. a, Fast mEPSCs predominate in control 0-Mg²⁺ saline, and the slow component of dual mEPSCs is proportionately smaller and briefer than in mature mEPSCs (see Fig. 3B). b, The addition of Mg²⁺ reduces the incidence of dual mEPSCs to <10%. c, All mEPSCs are abolished in the presence of Mg²⁺plus GYKI. d, After the washout of GYKI, fast mEPSCs again predominate. C, D, APV reveals a minor NMDA-R-mediated component in embryonic dual mEPSCs. Continuous traces (C) and averaged mEPSCs (D) at $-$ 70 mV are illustrated as in A and B. a, The majority of mEPSCs recorded in control 0-Mg²⁺ saline are fast. b, In the presence of APV only fast mEPSCs remain, which are indistinguishable from the fast control mEPSCs. A, B and C, D were recorded from two cells in different stage 31/32 (39-40 hr) embryos. Mean mEPSCs are averages of $>=$ 49 events (fast) and $>=$ 18 events (dual).

Embryonic mEPSC distribution and peak amplitudes in Mg²⁺-free saline differ markedly from those at mature synapses, however(Fig. 5, Table 1). At $-$ 70 mV the majority (66 ± 6%; range, 47-78%;n = 5) of embryonic mEPSCs is exclusively fast, with peak amplitudestwofold larger than mature fast mEPSCs. Dual mEPSCs occur morerarely (32 ± 5%; range, 21-50%; n = 5) and also have peak amplitudesover twofold larger than in mature larvae. The rise times anddecay kinetics of fast mEPSC current components are indistinguishablefrom those at mature stages. However, the slow NMDA-R-mediatedcomponent of embryonic dual mEPSCs is less prominent and has asignificantly faster decay constant (8.2 ± 2.0 msec; n = 5) thanat mature synapses. Single channel activity resembling NMDA-Rchannel openings is also sometimes present, but slow mEPSCs areobserved only rarely (3 ± 2%; range, 1-9%; n = 5).

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Figure 5. The distribution of different classes of mEPSCs changes during embryonic and larval development. The mean percentages ± SEM of fast, dual, and slow mEPSCs recorded at $-$ 70 mV in Mg²⁺-free external saline are plotted for three developmental stages. The incidence of dual, AMPA-R- and NMDA-R-mediated, mEPSCs increases to >70% at mature synapses, and the incidence of fast AMPA-R-mediated mEPSC decreases. The percentage of dual mEPSCs in mature larvae (asterisk; 71 ± 2%; n = 12) is significantly greater than the values at both embryonic (38-40 hr; n = 5) and larval stages (54 hr; n = 6).

The predominance of fast mEPSCs at embryonic excitatory spinal synapses suggests that they differ in two possible respectsfrom mature larval synapses: (1) the majority of embryonic synapsesexpresses only AMPA-R; or (2) NMDA-R are present, but most arenonfunctional or blocked, even in the absence of added Mg²⁺. The large, predominantly fast AMPA-R-mediated mEPSCs presentat immature synapses gradually undergo a developmental transitionto smaller dual-component mEPSCs mediated by both AMPA-R and NMDA-Rin Mg²⁺-freesaline.

At an early larval stage (54 hr), mEPSC pharmacology is identical to that at embryonic and mature stages (n = 6; data notshown). Mean mEPSC amplitudes and the distribution of dual andfast mEPSCs at this stage are intermediate between embryonic andmature values (n = 6; Fig. 5, Table 1), indicating that theseproperties are changing gradually during development. By maturelarval stages, AMPA-R and NMDA-R are colocalized at most synapses,evidenced by the 71% incidence of dual-component mEPSCs (Fig.5). Depolarization to +60 mV slightly increases the incidenceof dual and slow mEPSCs (see Fig. 2D; n = 4), probably attributableto relief of a small amount of residual Mg²⁺ block of NMDA-R at $-$ 70 mV, and prolongs the decay constant ofthe NMDA-R component by two- to threefold. However, as noted above,fast mEPSCs are still observed even at +60 mV. These results indicatethat both AMPA-R and NMDA-R are colocalized at $>=$ 70% of matureexcitatory synapses, whereas most of the remaining synapses expressonly AMPA-R.

Early excitatory transmission at these spinal synapses thus is mediated principally by AMPA-R rather than by NMDA-R. Thisfinding contrasts with several studies in mammalian hippocampus(Durand et al., 1996; Liao and Malinow, 1996), sensory cortex(Crair and Malenka, 1995; Isaac et al., 1997) and spinal motoneurons(Ziskind-Conhaim, 1990), and in Xenopus optic tectum (Wu et al.,1996), where NMDA-R-mediated synaptic currents precede AMPA-R-mediatedsynaptic currents. Our finding is in agreement, however, witha recent developmental study of cultured Xenopus embryonic spinalneurons showing that AMPA-R expression precedes NMDA-R expressionand that AMPA-evoked currents are 10-fold larger than NMDA-evokedcurrents at 1 d in culture (~40 hr of embryonic development) (Gleasonand Spitzer, 1998).

mEPSCs at both embryonic and mature synapses are mediated essentially by AMPA-R in the presence of Mg²⁺

The addition of 1 mM Mg²⁺ to the external saline blocks nearly all of the NMDA-R-mediated synaptic current at $-$ 70 mV at embryonicas well as mature larval synapses, converting most dual mEPSCsto fast mEPSCs and eliminating slow mEPSCs. As a result, ~90%of both mature and embryonic mEPSCs in the presence of Mg²⁺ are exclusively fast, and the slow decay time constant in thefew remaining mature dual mEPSCs is shortened significantly to~5 msec (Table 1). Dual mEPSCs with prolonged slow current componentsare revealed only at strongly depolarized potentials (+30 to +60mV; n = 4). At negative potentials ( $-$ 30 to $-$ 70 mV) the mean mEPSCin Mg²⁺ is kinetically similar to the fast mEPSCs described above, witha decay constant of ~1 msec. Consistent with earlier results,embryonic mEPSCs in Mg²⁺ are over twice as large as mature mEPSCs (Table 1). Thus, overa broad range of negative potentials, synaptic NMDA-R are functionallyblocked in the presence of a physiological Mg²⁺ concentration. Under most normal conditions the excitatory currentat DLi synapses therefore must be mediated almost entirely byAMPA-R, even at mature synapses that express NMDA-R. This findingfurther strengthens the conclusion that initial excitatory transmissionin the embryonic spinal cord is mediated mainly by AMPA-R.

AMPA-R are permeable to Ca²⁺

AMPA-R in cultured embryonic Xenopus spinal neurons are permeable to Ca²⁺ (Gleason and Spitzer, 1998). Because transmission at excitatoryDLi synapses is mediated predominantly by AMPA-R, we investigatedthe Ca²⁺ permeability of these receptors. AMPA-R at embryonic synapsesare also permeable to Ca²⁺. The mEPSC reversal potential in the presence of APV and Mg²⁺ is shifted in the positive direction by 10 ± 1 mV (n = 5) whenexternal Ca²⁺ is raised from 1 to 20 mM (Fig. 6A). Using the Goldman-Hodgkin-Katzequation, we calculate a relative Ca²⁺ permeability (P_Ca/P_monocation) of 1.7 ± 0.3 (range, 1.0 to 2.5;n = 6) for embryonic synaptic AMPA-R, a value similar to thatfound for AMPA-R (relative P_Ca of 1.9) in cultured spinal neurons(Gleason and Spitzer, 1998).

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Figure 6. Embryonic synaptic AMPA-R and the total AMPA-R population in both embryonic and mature larval DLi are Ca²⁺-permeable. A, Top, Mean AMPA-R-mediated mEPSCs recorded in 1 and 20 mM external Ca²⁺ at three holding potentials from a DLi in a stage 31 (39 hr) embryo. Mg²⁺ (1 mM) and APV (50 µM) were present to isolate AMPA-R. Note that the mean mEPSCs at 0 mV have opposite polarity at the two Ca²⁺ concentrations. A, Bottom, mEPSC I-V relations in 1 and 20 mM Ca²⁺ for the same cell. The mEPSC reversal potential (determined by interpolation) in 20 mM Ca²⁺ is shifted by +10.5 mV, indicating a significant Ca²⁺ permeability for synaptic AMPA-R (estimated P_Ca of 1.8 relative to monovalent cations). B, Whole-cell responses to kainate (KA) in 0-Na⁺, 20 mM Ca²⁺ external saline support the conclusion that the AMPA-R population (synaptic plus nonsynaptic) is permeable to Ca²⁺. B, Top, Currents evoked by 500 µM KA focally applied with a pressure pipette (horizontal bar) in 0-Na⁺, 20 mM Ca²⁺ saline to a DLi in a stage 31 embryo. B, Bottom, The KA I-V in 0-Na⁺, 20 mM Ca²⁺ is shown for the same embryonic neuron (filled symbols); the KA reversal potential is $-$ 22 mV, and the estimated relative P_Ca for AMPA-R is 1.5. Open symbols show the KA I-V in 0-Na⁺, 20 mM Ca²⁺ for a DLi in a mature (7 d) larva; the reversal potential is $-$ 30 mV, and estimated relative P_Ca is 1.0.

As a second, independent test for AMPA-R Ca²⁺ permeability, we recorded whole-cell responses to puffer-applied 500 µM kainate(KA) in 0-Na⁺, 20 mM Ca²⁺ saline (Gu et al., 1996; Jia et al., 1996), which likely activatesboth synaptic and nonsynaptic AMPA-R populations. KA reversalpotentials for embryonic and mature larval DLi are $-$ 22 ± 4 mV(n = 4) and $-$ 30 ± 1 mV (n = 3), respectively (Fig. 6B), indicatingsignificant Ca²⁺ permeabilities for AMPA-R in both embryonic and mature neurons.For embryonic AMPA-R, relative P_Ca values determined from KA reversalpotentials (1.5 ± 0.1; n = 4) and mEPSC reversal potential experimentsdo not differ significantly, suggesting that Ca²⁺ permeabilities of both synaptic and nonsynaptic receptors aresimilar. For mature AMPA-R, relative P_Ca determined from KA reversalpotentials is 1.0 ± 0.1 (n = 3). This value is significantly lessthan that for embryonic receptors, but nevertheless it indicatesa substantial P_Ca for AMPA-R during the period of developmentthat was studied. The Ca²⁺ permeability of these AMPA-R raises the possibility that, inaddition to mediating excitatory transmission, they allow Ca²⁺ influx from the earliest stages of synaptic activity, which regulatesaspects of neuronal maturation and synapticplasticity.

Developmental changes in presynaptic activity patterns and mEPSC amplitude distributions

Spontaneous activity patterns and amplitudes of AMPA-R-mediated mEPSCs in 1 mM Mg²⁺-containing saline are strikingly different at embryonic and maturelarval synapses (Figs. 7, 8). At embryonic synapses a componentof spontaneous transmitter release occurs in a nonrandom manner,with a disproportionate number of mEPSCs occurring in bursts witha high incidence of activity, interspersed with periods of muchlower frequency (Figs. 7A, 9B). Bursts vary from pairs of mEPSCsto over a dozen closely spaced events and are observed in allembryonic recordings. They appear to result from brief episodesof heightened release probability at individual presynaptic inputs,because they occur even when overall mEPSC frequency is low (<1Hz). The average embryonic mEPSC frequency (2.1 ± 0.6 Hz; n =17) in the presence of these bursts is not significantly lessthan that in mature neurons (3.0 ± 0.9 Hz; n = 13).

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Figure 7. AMPA-R-mediated mEPSCs at embryonic synapses occur in spontaneous bursts and have large amplitudes, both of which are absent at mature synapses. A, B, Continuous records (top traces) of mEPSCs recorded at $-$ 70 mV in 1 mM Mg²⁺ from an embryonic neuron (A) and a mature neuron (B). Note the difference in amplitude scales. Portions of the continuous traces contained in the boxed regions are shown on an expanded time scale (bottom set of traces). Many mEPSCs at embryonic synapses occur in bursts separated by brief intervals (A, bottom trace) even when the overall frequency is low, whereas at mature synapses (B, bottom trace) such bursts are absent. C, D, Inter-mEPSC interval (IMI) distributions (left panels) and mEPSC amplitude distributions (right panels) for the cells illustrated in A and B. The proportion of brief IMIs (1-20 msec durations) is markedly greater at the embryonic synapse (C) than at the mature synapse (D) because of events occurring in bursts, although both cells had the same overall mEPSC frequency; note the different scale of ordinates. Insets show distributions of IMIs <50 msec in each cell in greater detail. All embryonic neurons had disproportionately greater numbers of brief IMIs. Embryonic mEPSCs have significantly greater amplitudes and variability than mature mEPSCs. Values above IMI distributions are overall frequency and number of events; values above amplitude distributions are mean amplitude ± SD.

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Figure 8. mEPSC amplitude and variability decrease with development. A, Histogram of mean mEPSC amplitudes recorded from embryonic and mature neurons ( $-$ 70 mV; 1 mM Mg²⁺). Mean mEPSC amplitudes at 13 mature synapses are tightly grouped (filled bars), with an average value of $-$ 30 ± 2 pA (n = 13). Embryonic mean mEPSC amplitudes appear to fall into two populations: a "low" group (n = 10; shaded bars) and a "high" group (n = 7; open bars), with an overall average amplitude of $-$ 74 ± 7 pA. B, Variability (SD) in mEPSC amplitude is plotted against the mean amplitude for 17 embryonic and 13 mature neurons. mEPSC variability is correlated strongly and positively with mean mEPSC amplitude; regression values in the panel inset were determined from straight line fits to the data. A much wider range of mEPSC amplitudes and variability is observed in embryonic neurons, which are plotted in two groups, as in A. Inset histograms show representative mEPSC amplitude distributions for a neuron from each group. C, Mean mEPSC amplitudes (left panel), variability in amplitude (SD, middle panel), and coefficients of variability ± SEM (CV; right panel) for the two embryonic groups and mature neurons shown in A and B. Mean mEPSC amplitude and variability are significantly larger in both embryonic groups than in mature mEPSCs, but there is no significant difference in CV during development.

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Figure 9. Ca²⁺-dependent unsynchronized multiquantal release underlies mEPSC bursts at embryonic synapses. A, B, mEPSC amplitude at embryonic and mature synapses is independent of spontaneous frequency. A, Scatter plot of mEPSC amplitudes versus mEPSC intervals (IMI, in log scale) preceding each event for two embryonic neurons from the "low" (a) and "high" amplitude groups (b) shown in Figure 8. Mean mEPSC amplitudes ± SD, number of events, and frequency in each neuron are shown above the plots. mEPSCs occurring during bursts are those preceded by brief duration IMIs (<20 msec). There is no correlation between mEPSC amplitude and IMI, demonstrating that mEPSCs within and outside of bursts have similar amplitudes; lines were fit to the data by linear regression (r = 0.008, a; r = $-$ 0.053, b). B, Left, The proportion of brief duration IMIs (<20 msec) is significantly larger for embryonic (28 ± 3%) than for mature (7 ± 2%) synapses. Mean mEPSC frequencies ± SEM for the data shown are 3.3 ± 1.1 Hz for embryonic neurons (range, 0.7-9.9 Hz; n = 8) and 3.3 ± 1.3 Hz for mature neurons (range, 0.7-13.4 Hz; n = 9). B, Right, mEPSC amplitudes (normalized to the mean value in each recording ± SEM) are plotted against IMI bins of increasing duration for embryonic (n = 8) and mature neurons (n = 9). There is no significant difference in mEPSC amplitudes over a 1000-fold range of IMI duration, indicating that amplitude is not affected by intrinsic release frequency. C, Reducing the probability of spontaneous release eliminates most spontaneous bursts but does not alter mEPSC amplitude and variability. mEPSC amplitude (left plots) and IMI distributions (right plots) are shown for an embryonic neuron (40 hr) in normal 2 mM Ca²⁺ (a) and 0-Ca²⁺ saline (b). Mean amplitudes ± SD, number of events, and frequency for both conditions are shown above the plots. mEPSC amplitude and variability are not significantly different in 0-Ca²⁺ saline, but mEPSC frequency is reduced to <10% of control, and bursts of >2 mEPSCs are eliminated. Examples of normal mEPSC bursts and rare doublets in 0-Ca²⁺ are inset above the IMI histograms.

To assay bursting behavior, we measured intervals between mEPSCs. The distribution of inter-mEPSC intervals (IMIs) is markedlydifferent between embryonic and mature synapses (Fig. 7B-D). Allembryonic IMI distributions exhibit a prominent component of briefintervals (<20 msec; Figs. 7C, 9A,B) regardless of overall mEPSCfrequency (range, 0.7-9.9 Hz; n = 8). By contrast, at mature synapseswith comparable frequencies (0.7-13.5 Hz; n = 9), brief intervals(<20 msec) are rare, and mature IMI histograms have approximatelysingle-exponential distributions consistent with the random occurrenceof mEPSCs (Fig. 7D).

In addition, both mEPSC mean amplitude and variability are significantly greater at embryonic synapses (Figs. 7C,D, 8). MaturemEPSCs have amplitude distributions skewed toward larger values,with mean amplitudes of $-$ 30 ± 2 pA and SDs of 20 ± 2 pA (n = 13).Embryonic mEPSCs have 2.5-fold larger mean amplitudes ( $-$ 74 ± 7pA) and SDs (51 ± 5 pA; n = 17). Interestingly, embryonic synapsesappear to fall into "low" and "high" subgroups on the basis ofmEPSC mean amplitude and variability, although both groups havesignificantly greater values than those of mature synapses (Fig.8A-C). The embryonic "low" group has a mean mEPSC amplitude of $-$ 53 ± 1 pA and broadly skewed amplitude distributions (SD, 38± 2 pA; n = 10) that usually have several wide peaks (Fig. 8B).The embryonic "high" group has significantly larger amplitudes( $-$ 104 ± 10 pA) and a much wider range in amplitude from cell tocell (Fig. 8A,B). mEPSC amplitude distributions for this lattergroup of neurons are broader (SD, 70 ± 7 pA; n = 7) and occasionallylack a predominant peak (Figs. 7C, 8B). Mean mEPSC amplitudesand SDs are strongly correlated during development as well aswithin each age group, suggesting a developmental reduction andrefinement in both mEPSC amplitude and variability (Fig. 8B).However, the coefficient of variability (CV) does not change significantlyand remains surprisingly large (~0.65) even in mature larvae (Fig.8C).

The larger amplitude and variability of mEPSCs at embryonic spinal synapses could be attributable to both pre- or postsynapticfactors thought to contribute to large synaptic current variabilityat other CNS synapses (Bekkers et al., 1990; Bekkers and Stevens,1995; Frerking et al., 1995; Nusser et al., 1997; Wall and Usowicz,1998). One possibility is that the simultaneous fusion of multipletransmitter vesicles occurs with a greater probability at embryonicpresynaptic boutons, possibly as a result of spontaneous Ca²⁺ influx at boutons with multiple release sites (Bennett et al.,1995; Frerking et al., 1997). This would be expected to generatebroad mEPSC amplitude distributions with multiple peaks, as weobserved for all 17 embryonic neurons that were analyzed. However,peak number differs greatly among different distributions andpeak intervals are highly inconsistent, thus providing no clearevidence for quantal modes of release (Figs. 7C, 8B, 9C), andinflections or notches on the rising phase of large mEPSCs indicativeof multivesicular events (Wall and Usowicz, 1998) arerare.

If large mEPSC amplitudes are generated by a Ca²⁺-dependent multiquantal release mechanism, then reducing the probability ofspontaneous release should result in a decrease of both mEPSCvariability and mean amplitude (Frerking et al., 1997; Wall andUsowicz, 1998). To test this possibility directly, we recordedembryonic mEPSCs in both normal 2 mM Ca²⁺ and in saline without added Ca²⁺ (0-Ca²⁺ saline). mEPSC frequency is greatly reduced (18 ± 4% of control;n = 4) in 0-Ca²⁺ saline, as expected, but mEPSC mean amplitude (99 ± 10% of control)and variability (96 ± 8% of control) are not significantly differentfrom those in 2 mM Ca²⁺ (Fig. 9C). These parameters are thus mainly Ca²⁺-independent and likely derive from factors other than multiquantalrelease, such as differences in quantal transmitter content (Frerkinget al., 1995), synaptic transmitter concentration (Kullmann andAsztely, 1998), and AMPA-R number or availability at differentrelease sites (Walmsley, 1995; Nusser et al., 1997; Walmsley etal., 1998).

In contrast, spontaneous multi-mEPSC bursts are eliminated in 0-Ca²⁺ saline, except for rare doublets (Fig. 9C; n = 4). This resultsuggests that the bursts of mEPSCs observed at all embryonic synapsesare triggered by spontaneous presynaptic Ca²⁺ entry, resulting in episodes of unsynchronized multiquantal releaseover a period of several milliseconds to tens of milliseconds.The mechanism generating bursts at embryonic synapses is thusdistinct from that underlying larger mEPSC amplitude and variability.Bursts are equally prominent in embryonic neurons in the "low"group, which have smaller mEPSC amplitudes and variability (Fig.9A,C). Moreover, for all of the neurons that were analyzed, themean amplitude of mEPSCs occurring within high-frequency bursts(<20 msec IMI) does not differ significantly from that of mEPSCsoccurring outside of bursts (Fig. 9B). At embryonic synapses inparticular, large mEPSC amplitudes coupled with the spontaneousbursting of presynaptic transmitter release underscore the possibilitythat AMPA-R are used as an important source of spontaneous postsynapticCa²⁺entry.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Early AMPA-R expression and later colocalization of NMDA-R and AMPA-R at excitatory spinal synapses

mEPSCs at embryonic Xenopus DLi spinal synapses are already dominated by fast, large-amplitude AMPA-R currents in Mg²⁺-free saline within 13 hr after reflex movements begin. Previously,intracellular mEPSP recordings from DLi in newly hatched (54 hr)larvae suggested that non-NMDA-R and NMDA-R were primarily segregatedat different postsynaptic sites (Sillar and Roberts, 1991). Incontrast, we show that NMDA-R and AMPA-R are colocalized progressivelyto >70% of individual synapses by mature larval stages, producingdistinct mEPSC components similar to those observed at other maturecentral synapses (Bekkers and Stevens, 1989; Hori and Endo, 1994;Isaacson and Walmsley, 1995; Wu et al., 1996; O'Brien et al.,1997). In parallel, AMPA-R mEPSC amplitudes decrease and NMDA-RmEPSC decay constants lengthen, increasing the relative NMDA-Rcontribution to mature synaptic currents. However, mEPSCs throughoutdevelopment are predominantly AMPA-R-mediated under normal physiologicalconditions (+Mg²⁺).

Properties of embryonic AMPA-R synapses: larger mEPSC amplitude and variability and asynchronous multiquantal release

AMPA-R-mediated mEPSCs at embryonic spinal synapses have unusually large amplitudes and variability in TTX and frequentlyoccur in unsynchronized bursts. mEPSC variability decreases withage, as observed at developing cerebellar (Wall and Usowicz, 1998)and hippocampal synapses (Hsia et al., 1998). However, our findingthat mEPSC amplitude decreases by ~60% contrasts strikingly withstudies at other developing central synapses (Wu et al., 1996;Gao et al., 1998; Hsia et al., 1998; Wall and Usowicz, 1998).Most embryonic mEPSCs are probably monoquantal, because theiramplitude and variability are unchanged after reducing the probabilityof synchronous multiquantal fusion with 0-Ca²⁺ saline. By contrast, the dependence of bursts on external Ca²⁺ suggests that they are triggered by spontaneous presynaptic Ca²⁺ influx, resulting in episodes of unsynchronized multiquantalrelease. mEPSCs have similar amplitude and variability whetherthey occur in bursts or in isolation, indicating that they occurat the same population of synapses. This form of multiquantalrelease, which has not been described previously at a developingcentral synapse, may serve to increase the frequency of immaturespontaneous synaptic currents to a functionally significantlevel.

Variability in miniature synaptic currents observed at many central synapses may derive from several factors, including intrinsicvariability at individual synapses, synaptic heterogeneity suchas different postsynaptic receptor densities, and multiquantalrelease (Bekkers et al., 1990; Borst et al., 1994; Bekkers andStevens, 1995; Frerking et al., 1995, 1997; Liu and Tsien, 1995;Walmsley, 1995; Isaacson and Walmsley, 1996; Auger et al., 1998;Wall and Usowicz, 1998). The simplest explanation for our resultsis that embryonic DLi synapses have both greater variability andnumber of postsynaptic AMPA-R (Liu and Tsien, 1995; Wall and Usowicz,1998) than at mature larval synapses. Postsynaptic AMPA-R andGABA_A receptor number, respectively, underlie activity-modulatedchanges in mEPSC amplitude in cultured rat spinal neurons (O'Brienet al., 1998) and large variation in mIPSC amplitude in mousecerebellar stellate cells (Nusser et al., 1997). However, embryonicAMPA-R that have greater conductance or are differently modulated(Benke et al., 1998) or differences in synaptic transmitter concentrations(Frerking et al., 1995; Kullmann and Asztely, 1998) also couldcontribute to mEPSC amplitude and variability. The large CV throughoutdevelopment suggests that some combination of these factors maintainsa large relative variability in quantal amplitude. Larval DLireceive excitatory input from up to three to four Rohon-Beardneurons, probably via en passant synaptic contacts, and have compactdendritic arbors (Soffe et al., 1984; Roberts et al., 1988; Sillarand Roberts, 1988). However, detailed synaptic structural featuresincluding synapse size, number, and distribution, which couldcorrelate to functional developmental changes (Bennett et al.,1995; Walmsley et al., 1998), have not been examined. Determiningwhether mIPSCs undergo similar changes will determine whethersimilar mechanisms exist at embryonic inhibitory spinalsynapses.

Ca²⁺ permeability of AMPA-R

Transmission mediated by Ca²⁺-permeable AMPA-R has been reported at several mature synapses (Otis et al., 1995; Mahanty andSah, 1998), but it is unclear how the expression of these receptorsis regulated developmentally or whether they have a role at developingexcitatory synapses in vivo. AMPA-R Ca²⁺ permeability in mammalian subunit coexpression studies is conferredby the lack of the edited GluR2 subunit isoform (for review, seeJonas and Burnashev, 1995). Relative Ca²⁺ permeabilities (P_Ca/P_monocation) from ~0.2 to ~2 reported fornative Ca²⁺-permeable AMPA-R, compared with values of 5-10 for NMDA-R (Mayerand Westbrook, 1987; Jahr and Stevens, 1993), presumably reflectdifferent levels of GluR2-containing receptors (Jonas and Burnashev,1995). AMPA-R in cultured embryonic Xenopus spinal neurons directlymediate Ca²⁺ influx (relative P_Ca ~1.9) as well as Ca²⁺ release from internal stores (Gleason and Spitzer, 1998). Weshow that Ca²⁺-permeable AMPA-R (relative P_Ca ~1.7) are present at embryonicexcitatory spinal synapses, as well as extrasynaptically. MatureDLi also express Ca²⁺-permeable AMPA-R, although relative P_Ca (~1.0) is decreased ascompared with embryonic DLi, potentially reflecting a change inAMPA-R subtype expression as synapsesmature.

Development of glutamatergic signaling at Xenopus excitatory spinal synapses contrasts with other developing central synapses

Many immature excitatory synapses in mammalian hippocampus (Durand et al., 1996; Liao and Malinow, 1996; Liao et al., 1998;Petralia et al., 1998), sensory cortex (Crair and Malenka, 1995;Isaac et al., 1997; Golshani et al., 1998), and spinal motoneurons(Ziskind-Conhaim, 1990), as well as in Xenopus optic tectum (Wuet al., 1996), appear to lack functional AMPA-R. Initial transmissionat these synapses is thus nearly or completely absent, exceptat strongly depolarized potentials or in Mg²⁺-free saline that reveals NMDA-R currents or after LTP-inducingstimulation paradigms that "unsilence" synaptic AMPA-R (Liao etal., 1995; Durand et al., 1996; Wu et al., 1996; Isaac et al.,1997). A postnatal increase in AMPA-R synaptic currents (Crairand Malenka, 1995; Wu et al., 1996; Isaac et al., 1997) and ashortening of NMDA-R currents (Carmignoto and Vicini, 1992; Hestrin,1992; Crair and Malenka, 1995) also occur at several mammaliancentral synapses. These studies support the view that NMDA-R activationis required for subsequent AMPA-R expression at most developingglutamatergic synapses (Constantine-Paton and Cline, 1998; Feldmanand Knudsen, 1998), although they have not resolved how NMDA-Rat immature silent synapses become sufficiently activated underphysiological conditions to induce thisexpression.

In contrast, we find that AMPA-R-mediated mEPSCs predominate at immature Xenopus DLi glutamatergic spinal synapses and observean opposite developmental transition in AMPA-R and NMDA-R currents.Why might these developing synapses depart from the above model?We propose that, at these and possibly other excitatory synapses,early expression of AMPA-R, particularly Ca²⁺-permeable receptors, offers several advantages. Unlike sensoryareas of the brain that undergo extensive synaptic integrationand plasticity during a critical postnatal period, early spinalreflex and sensory-motor circuitry may be mainly "hard-wired,"rendering initial NMDA-R activity less important than establishingfunctional motor output that enables early swimming and escapebehaviors. AMPA-R mediate faster, larger-amplitude synaptic currents,ensuring early transmission. EPSPs in spinal motoneurons and DLiin early Xenopus larvae have similarly prominent non-NMDA-R components(Clarke and Roberts, 1984; Dale and Roberts, 1985; Sillar andRoberts, 1988), indicating that AMPA-R are used preferentiallyat other embryonic excitatorysynapses.

Our finding that embryonic mEPSCs have amplitudes ~2.5-fold larger than mature mEPSCs furthermore suggests that AMPA-R numberis greater at immature synapses. AMPA-R density at cultured mammaliansynapses has been shown to vary inversely with synapse number(Liu and Tsien, 1995) and to be downregulated by increased neuronalactivity levels (Craig, 1998; O'Brien et al., 1998; Turrigianoet al., 1998). The developmental decrease in mEPSC amplitude thereforemay coincide with increased neuronal activity and the number ofsynaptic inputs, and with a corresponding decrease in postsynapticAMPA-Rnumber.

Moreover, Ca²⁺-permeable AMPA-R are likely to mediate postsynaptic Ca²⁺ signals at early stages when activity level and excitatory synapsenumber are probably low. Large mEPSCs occurring in spontaneousbursts provide a mechanism for amplifying and prolonging AMPA-R-mediatedCa²⁺ influx in the absence of action potentials. To our knowledge,functional Ca²⁺-permeable AMPA-R have not been reported previously at immatureglutamatergic synapses in vivo. However, Ca²⁺-permeable AMPA-R support several forms of Ca²⁺-dependent synaptic modulation independently of NMDA-R, includingLTP (Gu et al., 1996; Jia et al., 1996; Mahanty and Sah; 1998).Therefore, it is plausible that developing synapses could useCa²⁺-permeable AMPA-R both for functional transmission and for Ca²⁺-dependent modulatory processes usually dependent on NMDA-R.

These interpretations do not preclude a functional role for NMDA-R in the developing spinal cord. mEPSC distributions in Mg²⁺-free saline indicate that NMDA-R are present at ~35 and ~80%of embryonic and mature larval synapses, respectively. NMDA-R-mediatedEPSPs regulate interspike potential and the cycle period of postembryonicrhythmic swimming output (Dale, 1995), demonstrating that NMDA-Rcontribute to synaptic signaling under conditions that relievevoltage-dependent Mg²⁺ blockade. The postembryonic increase in the proportion of NMDA-R-expressingsynapses parallels the period during which NMDA-R predominateat tectal synapses and may coincide with a later period of plasticityin the spinal cord, supporting experience-dependent modificationof larval motor behavior. NMDA-R-mediated Ca²⁺ influx also may underlie chemotropic responses in developingXenopus spinal neurons (Zheng et al., 1996). NMDA-R channel eventsoften are recorded in embryonic as well as mature neurons evenin the presence of Mg²⁺, suggesting that NMDA-R activation by extrasynaptic glutamatediffusion (Kullmann and Asztely, 1998; Walmsley et al., 1998)may admit sufficient Ca²⁺ to serve such arole.

Our results suggest that different glutamatergic synapses meet developmental and functional requirements in different ways.Embryonic Xenopus excitatory spinal synapses are specialized toachieve functional transmission and generate postsynaptic Ca²⁺ signals via AMPA-R activation. Postsynaptically, embryonic AMPA-Rare highly Ca²⁺-permeable and mediate large-amplitude mEPSCs. Presynaptically,unsynchronized spontaneous multiquantal transmitter release prolongsreceptor action. Large, fast synaptic currents ensure transmissionand motor function beginning well before hatching, which may beimportant for the development of patterned swimming activity.AMPA-R-mediated Ca²⁺ signals are likely to have a role in synaptic differentiation,including the regulation of changes in postsynaptic receptor expressionand function. Ca²⁺-permeable AMPA-R thus may serve a primary role in transmissionfrom early stages as well as regulatory roles analogous to thosesuggested for NMDA-R.

  FOOTNOTES

Received Jan. 29, 1999; revised July 15, 1999; accepted July 15, 1999.

We thank Dr. E. L. Gleason for insightful comments on this manuscript, I. Hsieh and S. Watt for technical assistance, Dr.P. Vincent for providing analysis software, and Dr. D. Leanderof Lilly Research Laboratories, Indianapolis, IN, for the giftof GYKI53655.
Correspondence should be addressed to Dr. Nicholas C. Spitzer, Department of Biology, 0357, University of California, SanDiego, 9500 Gilman Drive, La Jolla, CA 92093-0357.

Dr. Rohrbough's present address: Department of Biology, University of Utah, 257 South 1400 East, Salt Lake City, UT 84112-0840.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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