Maturation of Synaptic Transmission at End-Bulb Synapses of the Cochlear Nucleus

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The Journal of Neuroscience, December 1, 2001, 21(23):9487-9498

Maturation of Synaptic Transmission at End-Bulb Synapses of the Cochlear Nucleus
Stephan Brenowitz¹^,² and Laurence O. Trussell²
¹ Neuroscience Training Program, University of Wisconsin, Madison, Wisconsin 53706, and ² Oregon Hearing Research Center and Vollum Institute, Oregon Health Sciences University, Portland, Oregon 97201

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurons of the avian nucleus magnocellularis transmit phase-locked action potentials of the auditory nerve in a pathway thatcontributes to sound localization based on interaural timing differences.We studied developmental changes in synaptic transmission thatenable the end-bulb synapse to function as a synaptic relay. Inchick, although the auditory system begins to function early inembryonic development, maturation of audition around the timeof hatching suggested that synaptic transmission in the cochlearnucleus of young chicks may undergo further developmental changes.Synaptic physiology was investigated via patch-clamp recordingsfrom bushy cells in brainstem slices during stimulation of auditorynerve fibers at 35°C. Compared with embryonic synapses (embryonicday 18), post-hatch chicks (post-hatch days 1-11) exhibited highprobability of firing a well timed postsynaptic action potentialduring high-frequency stimulation of the auditory nerve. Improvementsin reliability and timing of postsynaptic spikes were accompaniedby a developmental increase in steady-state EPSCs during stimulustrains and a decline in the extent of synaptic depression. Synchronyof EPSCs during stimulus trains improved with age. An increasedpool of synaptic vesicles, lower release probability, larger andfaster transmitter quanta, and reduced AMPA receptor desensitizationcontributed to these changes. Together, these factors improvethe ability of cochlear nucleus magnocellularis neurons to faithfullytransmit timing information encoded by the auditorynerve.

Key words: short-term depression; AMPA receptors; cochlear nucleus; end-bulb synapse; auditory; development

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Localization of sound based on differences in phase or arrival time of sounds at the two ears requires accurate preservationof timing information by neurons of the auditory system. In thechick, such temporal resolution necessitates accurate and reliabletransmission of auditory nerve activity by the end-bulb synapsein the cochlear nucleus magnocellularis (nMag). Preservation oftiming information by specialized auditory synapses results fromphysiological and anatomical specializations (Oertel, 1999; Trussell,1999). In the chick, such features appear early in development.Initial formation of the nMag end-bulb synapse occurs by embryonicday (E) 11 when responses in nMag neurons to auditory nerve stimulation(Jackson et al., 1982) or sound (Saunders et al., 1973) firstarise. Retraction of dendrites (Jhaveri and Morest, 1982), synapseelimination (Jackson and Parks, 1982), and maturation of end-bulbmorphology (Jhaveri and Morest, 1982; Rubel and Parks, 1988) appearcomplete by E18. Tuning properties of auditory nerve fibers achievemature values before hatching (Rebillard and Rubel, 1981; Manleyet al., 1991). EPSCs in nMag at late embryonic stages have largeamplitudes and rapid kinetics but also exhibit strong synapticdepression during stimulation at frequencies expected of the auditorynerve in vivo. Such EPSPs fall subthreshold after several stimuliat frequencies of 200 Hz (Brenowitz et al., 1998). Although activationof presynaptic GABA_B receptors on auditory nerve terminals improvedreliability of signaling during short bursts of activity, theprobability of spike firing after the 10th stimulus of a 200 Hztrain remained low (<50%).

Such findings in embryos, however, are not consistent with in vivo recordings from older animals that indicate sustained activityat higher rates. In post-hatch day 10-28 (P10-28) chicks, in vivofiring rates of nMag neurons caused by spontaneous auditory nerveactivity alone were 31-231 Hz and increased to 110-480 Hz withacoustic stimulation (Warchol and Dallos, 1990). Improvementsin high-frequency responses in auditory neurons between P4 andP14 have also been reported in rat and mouse medial nucleus ofthe trapezoid body (MNTB) (Chuhma and Ohmori, 1998; Taschenbergerand von Gersdorff, 2000; Futai et al., 2001) and mouse cochlearnucleus (Wu and Oertel, 1987). Thus, it might be expected thatreliability of signal transfer at the nMag end-bulb synapse improvessignificantly afterhatching.

Developmental changes in patterns and levels of activity in the auditory system further predict that maturation of transmissionin nMag occurs around the time of hatching. Sound-evoked responsethresholds in the auditory nerve and cochlear nucleus declineand reach adult values between E19 and P1, resulting from clearanceof middle ear fluids and improved transduction by the cochlea(Saunders et al., 1973; Rebillard and Rubel, 1981). Behavioralstudies indicate a decline in auditory thresholds between hatchingand P4 (Gray and Rubel, 1985). Patterns of spontaneous auditorynerve firing change around E19, when rhythmic bursts of actionpotentials are replaced by the sustained Poisson-like firing observedin adults (Lippe, 1994; Jones and Jones, 2000). Spontaneous activityis thought to play an important role in synaptic modificationduring development of sensory systems (Katz and Shatz, 1996).Thus, increased spontaneous and sound-evoked auditory nerve activityoccurring around the time of hatching may be a driving force forfurther maturation of synaptic function innMag.

In this study, by comparing transmission in late embryos (E18) and young hatchlings (P1 through P11), we examined developmentalchanges in transmission at a morphologically mature synapse thatis experiencing increased activity levels. During this time, synapsesexhibited marked improvements in their ability to reliably generatewell timed postsynaptic action potentials during trains of high-frequencyauditory nerve stimulation. Experiments were conducted to determinethe mechanisms underlying this developmentaltransition.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Physiology. Brainstem slices (250-300 µm) were prepared from E18 and P1-11 chicks. Dissections were performed in ice-coldoxygenated saline containing (in mM): 140 NaCl, 20 glucose, 10HEPES, 5 KCl, 3 CaCl₂, 1 MgCl₂, pH 7.35. Slices were then maintainedat 34°C for 30 min. During recordings (34-36°C) slices were perfusedat 2-4 ml/min in a 1 ml chamber. Neurons were viewed with a ZeissAxioskop and Olympus 60× water immersion lens using differentialinterference contrast optics and infrared illumination. For measurementof AMPA-mediated EPSCs, saline was supplemented with (in µM):100 DL-2-amino-5-phosphonovalerate (APV), 10 7-Cl-kynurenate,10 SR-95531, and 2 strychnine. In some experiments, GYKI-52466(20 µM), a noncompetitive AMPA receptor antagonist, was addedto bath solutions to reduce EPSC conductance. Neurons were voltageclamped with an Axopatch 200B amplifier (Axon Instruments, FosterCity, CA) at $-$ 30 mV (for recording AMPA receptor-mediated EPSCs)or $-$ 60 mV [for recording miniature EPSCs (mEPSCs)]. Electrodeseries resistance (2-8 M $Omega$ ) was compensated 80-95%. Pipettes werefilled with an intracellular solution containing (in mM): 125Cs-methanesulfonate, 15 CsCl, 10 HEPES, 5 BAPTA, 1 MgCl₂, pH 7.25.During current-clamp experiments, pipettes contained (in mM):140 K-gluconate, 5 NaCl, 1 MgCl₂, 10 HEPES, 1 EGTA, pH 7.3. Synapticresponses were obtained by positioning a stimulus electrode (1.5-3M $Omega$ ) onto nearby myelinated fibers 20-100 µm from the postsynapticcell body. Individual afferent auditory nerve axons were stimulatedby 100-200 µsec, 5-50 V pulses delivered via an isolated stimulusunit (AMPI Iso-flex). Currents were filtered at 5-10 kHz and sampledat 20-50 kHz. Aniracetam stocks (0.5 M, 100×) were prepared inDMSO and added to extracellular solutions immediately before use.The final working concentration of aniracetam was 5 mM, and aniracetam-containingsolutions included 1% (v/v) DMSO. For all experiments using aniracetam,control extracellular solutions were also supplemented with 1%DMSO. Means are reported as ± SE. Chemicals and drugs were obtainedfrom Sigma (St. Louis, MO), RBI (Natick, MA), and Tocris Cookson(Ballwin,MO).

To assess the quality of voltage clamp, the current-voltage relationship of EPSC amplitudes was measured at holding potentialsranging from $-$ 40 to +20 mV. The relationship obtained was linear(r = 0.99; n = 4 neurons), suggesting minimal voltage error. However,bath application of 20 µM GYKI-52466, a noncompetitive AMPA receptorantagonist, sufficient to block EPSCs by 64 ± 2% (n = 14), causeda small but consistent increase in paired-pulse depression, asexpected if large EPSCs are limited by clamp error. The ratioof EPSC₂/EPSC₁ (with a 5 msec interval) was 0.40 ± 0.07 and 0.36± 0.06 (n = 6) in control and 20 µM GYKI, respectively (p < 0.05;t test). Although this effect was small, GYKI was added to bathsolutions in some experiments to maximize voltagecontrol.

Measurement of mEPSCs. Spontaneous mEPSCs were obtained at a holding potential of $-$ 60 mV. Currents were filtered at 10 kHzand sampled at 50 kHz. Events were detected using a template detectionalgorithm implemented in Axograph software (Axon Instruments).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Action potentials during synaptic trains

In embryos, depression at the nMag end-bulb synapse caused synaptic responses to become subthreshold during high-frequencytrains (Brenowitz et al., 1998). To determine reliability of signaltransfer in nMag in young hatchlings, we recorded EPSPs and actionpotentials in current-clamp configuration during stimulation ofpresynaptic auditory nerve fibers (Fig. 1A). The criterion forspike detection was the biphasic rising phase of a differentiatedtrace (Fig. 1B). In response to 100 and 200 Hz stimulation, neuronsconsistently fired spikes throughout stimulus trains of 20-40stimuli. For P2-3 synapses, mean spike probability for stimuli16-20 was 1.0, 1.0, and 0.81, at 100, 200, and 333 Hz, respectively(Fig. 1C), compared with probabilities of 0.69, 0.02, and 0 forE18 synapses (Brenowitz et al., 1998). Thus, developmental changesoccurring around the time of hatching greatly enhance reliabilityof signal transmission at the end-bulb synapse.

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Figure 1. Improved suprathreshold transmission in post-hatch synapses. A, Trains of 20 stimuli delivered at 200 Hz to an E18 (left trace) and a P4 synapse (right trace). At 200 Hz, action potential failures were not observed in P4 synapses. B, Action potentials were defined as responses showing an inflection (arrow, top traces) that was determined by the presence of a biphasic rise in the differentiated trace (arrow, bottom traces). C, Probabilities of action potential firing during stimulus trains was measured as the fraction of suprathreshold EPSPs for each stimulus during 10 repetitions delivered at 30 sec intervals. Data shown are for P2-4 synapses (circles; n = 6 neurons) and E18 synapses (squares; n = 4-7 neurons).

Improvement in spike timing during trains

Because temporally accurate transmission of auditory nerve activity by the cochlear nucleus is essential for detection ofinteraural timing differences used in sound localization, we comparedtemporal jitter in postsynaptic action potentials during stimulustrains in embryos and young hatchlings. Stimulus trains at 100Hz were repeated 10 times at 20-30 sec intervals, and SDs of thetime of action potential peaks were determined for each responseof the train. A frequency of 100 Hz was chosen so that actionpotentials were reliably generated in embryos (Brenowitz et al.,1998). Stimuli that produced subthreshold responses were not analyzed.Figure 2, A and B, shows the 1st and 10th responses from an E18and P3 synapse. The first response is well timed at both ages.During the train, depression of EPSPs in the E18 synapse causesvariability in the time at which threshold is reached, producingjitter in the timing of the action potential (Chuhma and Ohmori,1998; Taschenberger and von Gersdorff, 2000). In embryos, theSD in the time of the action potential peak increased from 18± 3 µsec for the first stimulus to 83 ± 8 µsec (average of lastfive stimuli of the train). In P2-3 synapses, temporal jitterincreased from 19 ± 2 µsec on the first stimulus to 24 ± 2 µsec(average of last five action potentials) during 100 Hz stimulustrains. These values are similar to those reported by Goldinget al. (1995), who reported temporal jitter of 20 µsec in auditorynerve-evoked action potentials in octopus cells of mature mousecochlear nucleus. These results indicate that changes in transmissionat the end-bulb synapse around the time of hatching allow moreaccurate temporal coding of auditory nerve activity by the cochlearnucleus.

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Figure 2. Improvement in action potential timing with older synapses. A, First and 10th responses are shown for 10 repetitions of a 100 Hz train in an E18 synapse. Action potentials show temporal jitter during the 10th stimulus. B, First and 10th responses for 10 repetitions of a 100 Hz train in a P3 synapse. Timing of action potentials during the 10th stimulus is improved. C, SD of peaks of action potentials were calculated for each stimulus of 100 Hz trains in E18 (squares; n = 9) and P2-3 (circles; n = 5) synapses. Progressive increase in variation of action potential timing seen in embryos is not present in P2-3 hatchlings.

Reduction in synaptic depression with age

Further experiments were performed to examine the mechanisms that account for improvements in the reliability and temporalprecision of high-frequency transmission. Under voltage clamp,transmission at the embryonic synapse in nMag is characterizedby strong depression of synaptic currents (Zhang and Trussell,1994a; Brenowitz et al., 1998). Therefore, we examined depressionof EPSCs during stimulus trains at different ages. Trains of EPSCswere recorded during stimulation of single auditory nerve fibersat a holding potential of $-$ 30 mV. Responses to 200 Hz stimulationin E18, P2, and P10 synapses are shown in Figure 3A. A progressivereduction in the amount of synaptic depression and an increasein steady-state EPSCs during trains are apparent during this developmentalperiod. Average EPSC amplitudes during stimulus trains deliveredat 100, 200, and 333 Hz are shown in Figure 3B. Trains of 20 stimuliwere delivered in post-hatch synapses. Shorter trains of 10 stimuliwere routinely delivered in embryonic synapses because greaterdepression made EPSC measurements unreliable during longer high-frequencytrains. Data from post-hatch synapses were combined in two agegroups of P2-3 and P6-11. At these three frequencies, averagesteady-state EPSC amplitudes (EPSC_SS; the average of the lastthree EPSCs in trains of 10 or 20 stimuli) showed progressiveand significant increases in the age groups tested (ANOVA; p <0.001; Tukey post hoc comparison). For example, at 200 Hz, EPSC_SSwas 0.52 ± 0.02, 2.53 ± 0.02, and 3.49 ± 0.04 nA at ages E18,P2-3, and P6-11, respectively (Fig. 3B). Between E18 and P6-11,EPSC_SS increased 4.0-, 6.7-, and 6.8-fold at 100, 200, and 333Hz, respectively.

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Figure 3. Reduction of synaptic depression during development. A, Trains of 20 EPSCs were evoked at 200 Hz in brain slices obtained from animals at different ages. Top trace, E18; middle trace, P2; bottom trace, P10. Averages of three to five traces are shown. V_m = $-$ 30 mV. B, Absolute amplitudes during 200 Hz stimulus trains. Trains of 10 and 20 stimuli were delivered to embryos and hatchlings, respectively. Summarized data from E18 (n = 12), P2-3 (n = 15), and P6-11 (n = 10) are shown. C, Depression during 200 Hz trains was compared by normalizing each EPSC to the first EPSC of each train. Data in B and C are from the same cells. Asterisks indicate a slow phase of depression present in embryos.

Synaptic depression was also examined after normalization of the initial EPSC amplitude of each train (Fig. 3C). Normalizeddepression declined progressively in the three age groups. Paired-pulsedepression (PPD; EPSC₂/EPSC₁) with a 5 msec interval changed from0.25 ± 0.03 to 0.36 ± 0.03 to 0.61 ± 0.06 at ages E18, P2-3, andP6-11. The decline in synaptic depression was most apparent atthe highest frequencies tested (333 Hz). Also, a slow phase ofdepression in E18 synapses that was apparent after two to threestimuli was reduced in older chicks (Fig. 3C, asterisk).

Developmental changes in EPSC size and shape

Amplitude and time course of EPSCs were compared in synapses from three age groups: E18, P2-3, and P6-11 (Fig. 4A,C). BetweenE18 and P2-3, EPSC amplitudes increased 68%, from 8.4 ± 0.9 to14.1 ± 0.9 nA (p < 0.001; ANOVA; Tukey post hoc comparison). MeanEPSC amplitude for P6-11 synapses was 12.3 ± 1.1 nA, not significantlydifferent from for P2-3 synapses. Changes in EPSC time courseare illustrated by scaling and superimposing EPSCs from synapsesof different ages (Fig. 4B). Rise times (10-90%) became fasterbetween E18 and P2-3 but did not change significantly betweenP2-3 and P6-11. Fits of double-exponential functions to the decayphase of EPSCs indicated that the fast exponential component becamefaster by 50% between ages E18 and P6-11, causing a reductionof 41% in EPSC half-widths during this time (Fig. 4B,C). The observedincrease in the overall amplitude of EPSCs therefore could explainpart of the increase in synaptic strength during trains (Fig.1) but cannot account for the dramatic reduction in synaptic depressionwith age (Fig. 3).

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Figure 4. Developmental changes in EPSC kinetics. A, EPSCs at indicated ages were recorded at a holding potential of $-$ 30 mV. Averages of five traces are shown. Stimulus artifacts have been removed. B, Traces from A are superimposed and scaled to illustrate developmental changes in EPSC kinetics. C, Summarized data from E18 (n = 12 neurons), P2-3 (n = 12 neurons), and P6-11 (n = 7 neurons). Different letters above bars indicate statistically significant differences (p < 0.01; ANOVA; Tukey post hoc comparison).

Time course of EPSCs during trains

Rapidly rising and decaying synaptic conductance serves an important function in nMag (Trussell, 1999). Brief EPSCs are necessaryfor accurately timed postsynaptic action potentials that enablesound localization. Indeed, the presence of a low-threshold potassiumconductance makes rapidly rising synaptic conductance necessaryfor generation of spikes (Brew and Forsythe, 1995; Rathouz andTrussell, 1998). We therefore investigated developmental changesin time course of EPSCs during repetitive stimulation (Fig. 5).Rise times and half-widths of EPSCs were determined during 200Hz trains at different ages (E18, P2-3, and P6-11). Rise timesof EPSCs in E18 synapses increased progressively during 10-stimulustrains by 66%, from 0.20 ± 0.01 to 0.33 ± 0.03 msec (Fig. 5A).In post-hatch synapses, rise times increased by a much smalleramount (Fig. 5B). At ages P2-3, increase in rise time during 20stimulus trains was 28%, and at ages P6-11 a 24% increase wasmeasured (Fig. 5C). Notably, EPSC rise times in P6-11 hatchlingsafter 20 stimuli at 200 Hz in P6-11 synapses are as fast (0.19± 0.01 msec) as rise times of the first EPSCs of trains at ageE18 (0.20 ± 0.01 msec).

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Figure 5. EPSC kinetics during trains stabilize with age. A, EPSCs from an E18 synapse during 200 Hz stimulation were superimposed to illustrate changes in rise times and half-widths. B, Superimposed EPSCs from a P2 synapse during 200 Hz stimulation. C, Progressive increase in 10-90% rise times of EPSCs during trains is reduced with age. D, Half-widths of EPSCs increase during trains in embryos but remain stable in post-hatch synapses.

Progressive broadening of EPSCs during trains also declined with age (Fig. 5D). A large decrease in EPSC half-width was alwaysseen between the first two EPSCs of a train associated with amplitudedepression, so comparisons were made between the second and lastEPSCs. The broader first EPSC is a result of its larger quantalcontent and consequent delayed clearance of transmitter from thesynaptic cleft (Otis and Trussell, 1996). In E18 synapses, half-widthsincreased 33%, from 0.59 ± 0.02 to 0.79 ± 0.05 msec. In P2-3 hatchlings,half-widths increased from 0.40 ± 0.01 to 0.49 ± 0.02 msec, anincrease of 22%. In P6-11 hatchlings, half-widths increased byonly 8%, from 0.42 ± 0.02 to 0.45 ± 0.02 msec. Thus, not onlyare EPSCs at older synapses larger, but the time course of signalingremains more stable during high-frequencyactivity.

Changes in mEPSCs with age

To account for developmental changes in EPSCs and synaptic depression, further experiments were performed to measure quantalsize (q), vesicle pool size (N), transmitter release probability(P_R), and the time course of recovery from synaptic depression( $tau$ _REC). First, we recorded spontaneous mEPSCs in embryos and hatchlingsto determine the contribution of changes in quantal size and kineticsto the changes we observed in evoked EPSCs. Average mEPSCs froman E18 neuron (average of 277 events) and a P3 neuron (averageof 421 events) are illustrated in Figure 6A. Double-exponentialfunctions were fit to the decay phase of the mEPSC and are superimposedon the averaged events in Figure 6A. Data from eight embryos (E18)and 11 hatchlings (P2-3) were analyzed (Fig. 6B). Amplitudes weresignificantly larger, and rise times and $tau$ _FAST were significantlyfaster at P2-3 compared with E18 (p < 0.01; Student's t test).The increase in mEPSC amplitude between E18 and P2-3 was 34%,sufficient to account for part, but not all, of the developmentalincrease in EPSC amplitudes (Fig. 4). mEPSCs in P2-3 hatchlingswere strikingly rapid, with a major exponential decay time constantof 0.120 msec. No significant differences in any parameters wereseen in a comparison between mEPSCs obtained at P2-3 (n = 11)and P6-11 (n = 6). Thus, developmental changes in quanta are responsiblein part for developmental changes in evoked EPSCs.

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Figure 6. Increase in quantal size with development. A, Spontaneous mEPSCs were recorded in an E18 and a P3 neuron. Double exponential fits are superimposed on the decay of each averaged trace (gray lines). B, Averaged results from E18 (n = 8) and P2-3 (n = 12) neurons. Between 75 and 2148 events were averaged from each cell. Asterisks indicate statistically significant differences (p < 0.01; Student's t test).

We next compared in hatchlings and embryos the effects on mEPSCs of aniracetam, a modulator of AMPA receptors that reducesdesensitization (Vyklicky et al., 1991; Raman and Trussell, 1995;Partin et al., 1996). In addition to providing information aboutquantal size in the presence of aniracetam for vesicle pool measurements(see below), assaying sensitivity of mEPSCs to aniracetam couldprovide evidence for changes in AMPA receptor subunit compositionduring development (Partin et al., 1996). However, no significantdifferences with respect to changes in amplitude or decay timecourse were seen in the effect of aniracetam on mEPSCs in E18versus P2-3 synapses (data notshown).

Reduction of AMPA receptor desensitization in hatchlings during trains

To determine the contribution of desensitization to synaptic depression in hatchlings, trains of EPSCs were recorded in controlconditions and in the presence of aniracetam. Individual EPSCswere increased by aniracetam (5 mM) from 12.4 ± 1.1 to 14.9 ±0.6 nA (n = 9), an increase of 25 ± 8% (data not shown). Thiseffect of aniracetam on EPSC amplitudes at age P2-3 was not significantlydifferent from the effect seen at age E18 (35 ± 5%; n =18).

To determine the effect of aniracetam on synaptic depression, trains of EPSCs were normalized to the amplitude of the firstpeak (Fig. 7A). After normalization, depression was reduced inthe presence of aniracetam compared with controls, an effect attributableto relief of desensitization. Normalized EPSC_SS (average of thelast five EPSCs of trains) were larger in aniracetam at 100, 200,and 333 Hz (Fig. 7B) (p < 0.0001; Mann-Whitney U test). At 100,200, and 333 Hz, respectively, aniracetam enhanced EPSC_SS by 26± 3, 38 ± 4, and 73 ± 10%, respectively [calculated as 100 × (EPSC_ANI $-$ EPSC_CON)/EPSC_CON]. Thus, the amount of desensitization is dependenton stimulus frequency (Fig. 7C). Enhancement of EPSC_SS by 38%indicates that 28% of synaptic AMPA receptors are desensitizedduring 200 Hz trains. By contrast, aniracetam enhancement of EPSCsin E18 synapses was 104 ± 1% at 200 Hz (Brenowitz and Trussell,2001), indicating that 51% of AMPA receptors are desensitized.Thus, the contribution of desensitization to synaptic depressionduring trains declines with age. Aniracetam does not completelyblock desensitization to a long pulse of a high concentrationof glutamate (Raman and Trussell, 1995). However, it was mostlikely effective here, because the estimate of maximal desensitizationin E18 synapses (51%) made using aniracetam was similar to thatprovided through direct measurement of depression of quantal size(Brenowitz and Trussell, 2001).

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Figure 7. Effects of aniracetam on synaptic depression. A, Stimulus train delivered at 333 Hz in control conditions and with 5 mM aniracetam. Traces were normalized to the amplitudes of the first peak in each train. Averages of three to five traces are shown. Inset shows EPSCs 14-17 of the stimulus train. B, Normalized peak amplitudes during stimulus trains delivered at 100 Hz (n = 9 neurons), 200 Hz (n = 8), and 333 Hz (n = 4) Circles, Control (con); triangles, aniracetam (ani). Depression was significantly reduced by aniracetam for stimulus 2 through 20 of trains. C, Relative enhancement of EPSC amplitudes by aniracetam throughout stimulus trains at 100 Hz (triangles), 200 Hz (circles), and 333 Hz (squares), calculated as 100% · (EPSC_ANI $-$ EPSC_CON)/EPSC_CON.

Measurements of vesicle pools and release probability

To investigate presynaptic mechanisms that may contribute to the observed developmental changes in synaptic depression duringstimulus trains, estimates of vesicle pool size and P_R were madeat ages E18 and P2-3. This approach relied on a plot of the cumulativeEPSC as a function of stimulus number during high-frequency trains(Schneggenburger et al., 1999; Wu and Borst, 1999; Bollmann etal., 2000). Because desensitization contributes to depressionof EPSCs during trains (Fig. 7), pool size measurements were madein the presence of aniracetam. In some experiments on P2-3 hatchlings,15-20 µM GYKI-52466, a noncompetitive AMPA receptor antagonist,was added to improve voltage clamp by reduction of EPSCs (seeMaterials and Methods). No effects of GYKI were seen on pool sizemeasurements or on estimates of release probability, so pool sizedata from 12 neurons in aniracetam and 12 neurons in aniracetamand GYKI were combined for analysis. Quantal content of EPSCswas determined by dividing the peak synaptic currents by the quantalsize. Quantal size was measured in the presence of 5 mM aniracetamin E18 and P2-3 synapses at $-$ 60 mV and corrected for a holdingpotential of $-$ 30 mV at which EPSCs were recorded. At $-$ 60 mV, mEPSCamplitudes in 5 mM aniracetam for E18 and P2-3 synapses, respectively,were 129 ± 9 pA (n = 8) and 180 ± 14 pA (n = 11). To determinequantal size in 20 µM GYKI, these values were further scaled by64%, the effect of 20 µM GYKI on EPSC amplitudes. Using the steady-stateregion of the cumulative EPSC plot to extrapolate back to time0 (stimulus 1), the initial size of the vesicle pool can be determined,under the assumption that EPSC recovery rates are uniform duringthe train (see below). With this method we find that the sizeof vesicle pools increased 44%, from 209 ± 14 to 291 ± 19 betweenages E18 and P2-3 (data not shown). This change was highly significant(p < 0.001; Student's t test). Release probability was determinedby calculating the ratio between the quantal content of the firstEPSC of the train and the total pool size. P_R declined 17%, from0.69 ± 0.01 to 0.53 ± 0.03 during this developmental period (p< 0.001; Mann-Whitney Utest).

Using a related method based on a plot of the relationship between quantal content of the EPSC and cumulative quantal contentof the train (Elmqvist and Quastel, 1965; Christensen and Martin,1970; Lu and Trussell, 2000), similar results were obtained (datanot shown). Although both methods use similar approaches, relyingon extrapolation of plots based on EPSC trains, the regions ofthe trains used for extrapolation differ between the two methods.Unlike the cumulative EPSC plot used above, the method of Christensenand Martin (1970) relies on data points during the initial (pre-steady-state)portion of the stimulus trains and is insensitive to effects ofa slow phase of depression (Fig. 3C, asterisk). Using this approach,the estimated increase in the vesicle pool size was 69%, and releaseprobability declined by 26%. These changes were highly significant(p < 0.001; Mann-Whitney U test for P_R, Student's t test for poolsize). Increased vesicle pool size and reduced P_R are expectedto reduce synaptic depression and thereby improve sustained high-frequencytransmission at the nMag end-bulbsynapse.

The developmental decline in P_R suggests that transmitter release should become more sensitive to decreases in extracellularcalcium (i.e., a rightward shift in the dose-response relationshipbetween calcium and release). Therefore we predicted that loweringextracellular calcium should cause a larger reduction of EPSCamplitudes in hatchlings compared with embryos. Consistent withthis hypothesis, we found that lowering bath calcium from 3 to1.5 mM had a greater effect in hatchlings, reducing EPSCs by 26± 4% in E18 synapses (n = 3) and by 37 ± 2% in hatchlings (n =11; p < 0.05; Student's ttest).

Developmental changes in quantal parameters are summarized in Table 1. Quantal sizes were scaled for a holding potentialof $-$ 30 mV. Values of N and P_R were obtained from the cumulativeEPSC plots (Fig. 7A-C). EPSC amplitudes were determined in a populationof 8 embryos (E18) and 11 hatchlings (P2-3) from which mEPSCswere also recorded.


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Table 1. Developmental changes in EPSC parameters

Close agreement was observed between EPSC amplitudes predicted by the product N · P_R · q and experimentally measuredvalues.

Recovery from synaptic depression

An additional factor that determines the amplitudes of synaptic responses during repetitive stimulation is the rate of recoveryfrom synaptic depression (O'Donovan and Rinzel, 1997; Dittmanand Regehr, 1998). Therefore we performed a series of experimentsto monitor recovery rates (determined by recovery of EPSC amplitudes),under different conditions. These experiments were designed toinvestigate developmental changes, as well as effects of conditioningstimuli and calcium on rates of recovery from synapticdepression.

Recovery from single conditioning stimuli was compared in E18 and P2-3 synapses (Fig. 8). To determine the amount and timecourse of desensitization after a single conditioning stimulus,these experiments were conducted in the absence and presence ofaniracetam. In the continuous presence of GYKI-52466 (see Materialsand Methods), recovery was monitored between 5 msec and 5 sec.Recovery from 5 to 50 msec is shown for E18 and P2 synapses inFigure 8, A and B, respectively. EPSCs recorded in control conditionsand in aniracetam were normalized and superimposed. Average recoverydata for E18 and P2-3 synapses is shown in Figure 8, C and D,respectively. Recovery for E18 and P2-3 synapses is superimposedfor comparison in Figure 8E,F. The EPSC₂/EPSC₁ ratio in GYKI-52466at a 5 msec stimulus interval was 0.12 ± 0.02 at E18 and 0.37± 0.04 at P2-3. Thus, paired-pulse depression with a 5 msec stimulusinterval was reduced by a factor of 3 in P2-3 versus E18 synapses.

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Figure 8. Time course of recovery from synaptic depression after a single stimulus. A, Recovery was monitored by test pulses at intervals of 5 msec to 5 sec after one conditioning stimulus in an E18 synapse. Traces showing recovery in the presence GYKI (peaks indicated by dots) and in GYKI + aniracetam were normalized and superimposed. For these experiments, 20 µM GYKI was used to improve voltage clamp. B, Recovery in GYKI (indicated by dots) and GYKI + aniracetam is shown for a P2 synapse. C, Summary of recovery data for E18 synapses (n = 10), in GYKI (squares) and GYKI + aniracetam (circles). Data points were fit with double-exponential functions. Inset shows recovery from 5 to 100 msec on an expanded time scale. For recovery of E18 synapses in GYKI, $tau$ _fast = 26 msec, $tau$ _slow = 1.5 sec, and %fast = 65%. For recovery of E18 synapses in GYKI + aniracetam, $tau$ _fast = 33 msec, $tau$ _slow = 1.4 sec, and %fast = 59%. D, Recovery in P2-3 synapses (n = 11) in GYKI (squares) and GYKI + aniracetam (circles). Inset shows recovery from 5 to 100 msec on an expanded time scale. For recovery of P2-3 synapses in GYKI, $tau$ _fast = 35 msec, $tau$ _slow = 1.8 sec, and %fast = 47%. For recovery of P2-3 synapses in GYKI + aniracetam, $tau$ _fast = 35 msec, $tau$ _slow = 1.5 sec, and %fast = 36%. E, Comparison of depression and recovery in E18 and P2-3 synapses in GYKI. With a 5 msec recovery interval, EPSC₂/EPSC₁ ratio was 0.12 ± 0.02 and 0.37 ± 0.04 at ages E18 and P2-3, respectively. F, Comparison of recovery in E18 and P2-3 synapses in GYKI + aniracetam. With a 5 msec recovery interval, EPSC₂/EPSC₁ ratio was 0.31 ± 0.05 and 0.48 ± 0.04 at ages E18 and P2-3, respectively. G, Relative enhancement of EPSCs by aniracetam is plotted versus recovery interval. Enhancement is calculated as (EPSC_GYKI-ANI/EPSC_GYKI)/EPSC_GYKI.

When recovery was monitored in the presence of aniracetam, a large difference in the amount of desensitization between embryosand hatchlings became apparent (Fig. 8C,D, insets), in agreementwith previous results using train stimulation (Fig. 7). In E18synapses (Fig. 8C) aniracetam significantly reduced depressionat intervals of 5-30 msec (p < 0.006; Wilcoxon signed rank test),but with stimulus intervals >30 msec, depression in control andaniracetam were not significantly different. In P2-3 synapses,significant effects of aniracetam on depression persisted throughthe 5 and 10 msec recovery intervals, but with a 20 msec interval,PPD was not affected by aniracetam (Fig. 8D). Thus desensitizationis greater and more persistent in embryos than in hatchlings.At both ages, recovery from desensitization contributed to thefast component of EPSC recovery but did not affect the slow component.However, the effect of aniracetam on the fast component was greatestin embryos (Fig. 8C,D). Reduced desensitization after hatchingis consistent with our earlier measurement of lower P_R becausewe have shown previously that desensitization is minimal whenrelease probability is lowered (Brenowitz and Trussell, 2001).Recovery from desensitization, measured as decay in the enhancementof EPSC₂/EPSC₁ by aniracetam, is shown in Figure 8G. At near-physiologicalrecording temperatures (34-36°C), recovery from effects of aniracetamproceeded with a time course of <10 msec in E18 and P2-3 synapses,suggesting rapid unbinding and clearance ofglutamate.

Figure 8E illustrates recovery from synaptic depression that consists of both presynaptic and postsynaptic components. Byblocking desensitization with aniracetam, presynaptic componentsof recovery could be observed in isolation (Fig. 8F). A fast componentof presynaptic recovery persisted in hatchlings and embryos. Therate and amplitude of slow recovery components and the rate ofthe fast component did not change appreciably with age (Fig. 8,see legend). The main developmental change in recovery after asingle stimulus was the magnitude of the fast recovery component,which decreased from 59 to 36% between E18 and P2-3 (Fig. 8E,F).The remaining fast component of recovery in the presence of 5mM aniracetam is unlikely to result from residual desensitizationthat is resistant to aniracetam, because in a group of four hatchlingneurons that did not show any effects of aniracetam on depression("nondesensitizing"), a fast component of recovery was still present(data not shown). Moreover, the rate of this component (~35 msec)is more than threefold slower than recovery of aniracetam-sensitivedepression (Fig. 8G). The multiple components of recovery mayindicate the presence of multiple vesicle pools or multiple kineticsteps involved in replenishment of a releasable pool. Mechanismsof depression other than depletion, such as refractoriness ofrelease, may also contribute to recoveryrates.

Recovery of EPSCs after multiple conditioning stimuli

Because the auditory nerve exhibits both spontaneous and acoustically driven activity, we examined recovery from multipleconditioning stimuli to determine how ongoing activity may affectrecovery rates. After 10 stimuli at 200 Hz, test EPSCs were evokedat recovery intervals ranging from 5 msec to 5 sec. Data froma P3 neuron are shown in Figure 9A. In P2-3 synapses, althoughthe total amount of depression was increased threefold by theconditioning train, the time course of recovery was not affected,as indicated by superposition of scaled recovery curves (Fig.9E). However, in E18 synapses the conditioning train caused atwofold slowing of the fast component of recovery, from 26 to53 msec (Fig. 9D). A small increase in the contribution of thefast component to recovery was also seen (Fig. 9F).

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Figure 9. Recovery from synaptic depression after trains of stimuli. A, Recovery was monitored after conditioning by 1 (left) or 10 (right) stimuli delivered at 200 Hz. Stimuli delivered to monitor recovery are indicated by dots above traces. B, Summary of recovery from 1 stimulus (circles; n = 16 neurons) and 10 stimuli (squares; n = 15 neurons) in GYKI, from 5 msec to 5 sec in P2-3 hatchlings. For recovery after 10 stimuli in GYKI, parameters of a double-exponential fit to the data points were $tau$ _fast = 46 msec, $tau$ _slow = 1.9, and %fast = 48%. For recovery after 10 stimuli in GYKI + aniracetam, parameters were $tau$ _fast = 39 msec, $tau$ _slow = 1.5, and %fast = 43%. C, Data from B on an expanded time scale. Also shown is recovery from 10 stimuli in GYKI + aniracetam (triangles; n = 5 neurons). D, Recovery from depression in E18 synapses after 1 (squares; n = 10) and 10 stimuli (circles; n = 7) at 200 Hz. For recovery of E18 synapses after 10 stimuli in GYKI, double-exponential fit parameters were $tau$ _fast = 53 msec, $tau$ _slow = 2.1, and %fast = 71%. E, Double-exponential fits of hatchling recovery data from B were normalized and superimposed to illustrate that relative time course of recovery did not change. F, Double-exponential fits of embryo recovery data from D were scaled and superimposed to illustrate that trains increased and slowed the fast component of depression. Dashed line in E and F indicates recovery after trains. Solid line in E and F indicates recovery after single stimulus.

To summarize, EPSC recovery after trains was bi-exponential and exhibited a fast (<100 msec) component at both ages. Thisfast recovery component resulted from both presynaptic recoveryand recovery from AMPA receptor desensitization. Improved high-frequencytransmission in hatchlings is thus achieved in part by acquisitionof "stable" recovery rates that do not exhibit activity-dependentslowing during repetitive stimulation. In embryonic synapses,a slowing of $tau$ _FAST caused by activity is predicted to underliethe slow phase of depression (Fig. 3C, asterisk). In addition,the contribution of desensitization to the fast component of depressionand recovery declines withage.

Recovery in reduced extracellular calcium

Calcium entry into the presynaptic terminal has been shown to affect rates of vesicle cycling in other synapses (Dittman andRegehr, 1998; Wang and Kaczmarek, 1998; Wang and Zucker, 1998),suggesting that the fast phase of recovery seen at the nMag synapsemay be induced by elevated presynaptic calcium. If so, we predictedthat recovery would be slowed if extracellular calcium were reduced.However, when we measured recovery from depression in low extracellular(1.5 mM) calcium after conditioning trains of 1, 5, and 16 stimulidelivered at 333 Hz (data not shown), a fast component of recoveryremained. The time constant of recovery after conditioning trainsof 1, 5 and 16 stimuli was 22, 24, and 27 msec, respectively.The contribution of the fast component to recovery (percentagefast) after 1, 5, and 16 conditioning stimuli was 39, 58, and59%. Thus, fast recovery persisted under the lowest levels ofpresynaptic calcium influx that weretested.

Membrane properties of post-hatch neurons

Current-clamp experiments were conducted to examine responses of post-hatch nMag neurons to current steps. The membrane responsein hatchlings is very similar to that in embryos, being characterizedby generation of a single spike and strong outward rectification(Reyes et al., 1994; Zhang and Trussell, 1994b). The current-voltagerelationship was measured for a group of eight neurons of agesP2-3 (data not shown). Our results indicate that input resistanceof nMag neurons in P2-6 neurons declined threefold compared withE18 neurons (Zhang and Trussell, 1994b). Membrane capacitancealso increased with development. C_M increased from 11.9 ± 0.5pF at E18 (n = 31) to 14.8 ± 0.7 pF in P2-11 hatchlings (n = 31),a change of 24% (p < 0.001; Student's ttest).

Action potential generation required larger current injections in post-hatch nMag neurons. Threshold was reached with currentinjections of 1.05 ± 0.06 nA (n = 20; data not shown), comparedwith 0.43 ± 0.12 nA in embryos (Zhang and Trussell, 1994b). Thissuggests that larger synaptic conductances would be required foraction potential generation in older animals. Thus, despite theincrease in spike threshold and shorter duration of synaptic currents(Fig. 4), developmental increases in EPSC_SS during trains enablesustained high-frequencytransmission.

Effects of GABA_B receptors on synaptic transmission in hatchlings

Previously we demonstrated in embryonic nMag that GABA_B receptors enhance EPSC amplitudes during high-frequency trains (Brenowitzet al., 1998), attributable to relief of AMPA receptor desensitization(Brenowitz and Trussell, 2001). Because desensitization was reducedin hatchlings compared with embryos, we performed experimentsto examine effects of GABA_B receptor activation on synaptic depressionin hatchlings during trains (Fig. 10). EPSCs were recorded undercontrol conditions and in the presence of a saturating concentrationof baclofen (100 µM), a GABA_B receptor agonist. Single EPSCs werereduced by 84 ± 3% in E18 synapses (n = 6) (Brenowitz and Trussell,2001) and by 76 ± 6% in P3-6 synapses (n = 6). These effects ofbaclofen on embryos versus hatchlings were not significantly different(p > 0.05; Mann-Whitney U test).

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Figure 10. Effects of GABA_B receptor activation on synaptic depression in P3-6 neurons. A, Top traces, Stimulus trains were delivered to a P6 synapse at 200 Hz in the absence (con) or presence (bac) of 100 µM baclofen. Bottom traces, EPSCs 11-20 were superimposed and displayed on an expanded time scale to illustrate convergence of steady-state EPSC amplitudes. B, Top traces, Trains at 333 Hz in control (con) and baclofen (bac). Bottom traces, EPSCs 11-20 are superimposed and displayed on an expanded time scale to illustrate enhancement of EPSC amplitudes by baclofen at 333 Hz. C, Ratios of EPSCs in baclofen versus control (bac_N/con_N) for each stimulus of trains delivered at 100 Hz (triangles), 200 Hz (squares), and 333 Hz (circles) in P3-6 neurons (n = 6). At steady state, bac_N/con_N was 0.66, 1.0, and 1.45 at 100, 200, and 333 Hz, respectively. D, Comparison of (bac_N/con_N) ratio at 200 Hz at P3-6 and E18. For E18 synapses, the steady-state value of bac_N/con_N (average of last 3 stimuli) at 200 Hz was 2.0 ± 0.2 (n = 8). E, Rise times (10-90%) of EPSCs during 200 Hz stimulus trains in P3-6 neurons in control conditions (con, triangles) and in the presence of baclofen (bac, squares). Rise times remain faster during trains in the presence of baclofen. F, Half-widths of EPSCs during 200 Hz trains are narrower in baclofen (squares) compared with control (triangles).

Next, we delivered trains of stimuli at 200 Hz to P3-6 synapses in control conditions and in baclofen (Fig. 10A). Amplitudesof EPSCs recorded in both conditions converged on the same steady-statevalue after two to three stimuli (Fig. 10A,C), and amplitudes maintainedthe same values for the remainder of the 20-stimulus trains, suggestingequivalent levels of AMPA receptor desensitization in baclofenand control conditions. When stimulus rates were increased to333 Hz, however, EPSCs in baclofen became larger than controlEPSCs after two to three stimuli and remained larger for the durationof the train (Fig. 10B,C). By contrast, baclofen enhanced by morethan twofold EPSCs evoked at 200 Hz in E18 synapses (Fig. 10D).

Because enhancement of synaptic strength by GABA_B receptor activation was observed in post-hatch synapses only at high frequenciesthat are in the upper range of chick auditory nerve firing rates,we investigated alternative roles of GABA_B receptors in auditorysignal processing. Because deterioration of rapid EPSC kineticsduring trains will limit temporal accuracy and maximum rates ofpostsynaptic action potential firing, we examined effects of baclofenon EPSC rise times and half-widths during 200 Hz trains (Fig.10E,F). Rise times were significantly faster in baclofen comparedwith control for stimuli 2-20 of trains (p < 0.05; paired t tests).Half-widths of EPSCs were also significantly reduced by baclofen(p < 0.01; paired t tests). Thus, GABA_B receptors at the nMagend-bulb synapse in hatchlings may accelerate the time courseof the EPSC during high-frequency repetitive firing. At frequenciesapproaching the maximum reported firing rates for avian auditorynerve fibers (200-300 Hz) (Manley et al., 1991; Salvi et al.,1992), GABA_B receptor activation will also serve to enhance synapticstrength and promote suprathresholdtransmission.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this work we have described physiological changes at the nMag end-bulb synapse that occur around the time of hatching andresult in dramatic improvement in reliability and timing of high-frequencysynaptic transmission. These changes include an increase in EPSCamplitude, faster rise and decay kinetics of EPSCs, reduced synapticdepression during stimulus trains, and lower input resistance.Contributing to these changes are larger and faster mEPSCs, alarger pool of transmitter vesicles, lowered probability of transmitterrelease, and reduced AMPA receptor desensitization during trains,as summarized in Table 1. Rates of recovery from synaptic depressionduring repetitive stimulation are also more stable in older synapses.The improved reliability and timing of postsynaptic action potentialsduring stimulus trains promote suprathreshold transmission atfrequencies reaching the upper limit of auditory nerveactivity.

Improvements in high-frequency transmission during development have been observed at other synapses of the auditory pathway.In rodents, the onset of hearing occurs between P10 and P14 (Mikaelianand Ruben, 1964), but auditory nerve responses do not appear adult-likeuntil P18-36 (Sanes and Constantine-Paton, 1985; Blatchley etal., 1987).

Various changes at auditory synapses have been described that accompany the onset of neural activity in the auditory system.Wu and Oertel (1987) reported a developmental decrease in inputresistance and improved responses to repetitive stimulation betweenP7 and P22 in the mouse cochlear nucleus, consistent with findingsof this study. Bellingham and Walmsley (1997) report increasedmEPSC and evoked EPSC amplitudes in the rat cochlear nucleus betweenP4 and P18, also consistent with our results. In contrast, nochanges in mEPSC or evoked EPSC amplitudes were found in rat MNTB(Taschenberger and von Gersdorff, 2000; Iwasaki and Takahashi,2001). However, at the mouse calyx of Held, Futai et al. (2001)report a severalfold increase in EPSC amplitudes between P5 andP27. Acceleration of EPSC kinetics at auditory synapses duringdevelopment has also been reported by Taschenberger and von Gersdorff(2000), Futai et al. (2001), and Iwasaki and Takahashi (2001).Acquisition of rapid AMPA-mediated EPSC kinetics may result frompostsynaptic alterations in receptor subunit composition (Lawrenceand Trussell, 2000) and faster presynaptic action potential waveforms(Taschenberger and von Gersdorff, 2000). In the embryonic aviannMag, NMDA receptors do not contribute substantially to synapticsignaling (Zhang and Trussell, 1994b) and were not investigatedin this study. Larger vesicle pools and reduced P_R also contributeto maturation of transmission at the calyx of Held (Taschenbergerand von Gersdorff, 2000; Iwasaki and Takahashi, 2001). In hippocampus,reduced P_R also occurs during development (Chavis and Westbrook,2001). Acquisition of rapid EPSC kinetics and stable high-frequencytransmission as auditory activity increases during developmentappear to be common features of auditory synapses. Recent work(Lawrence and Trussell, 2000; Futai et al., 2001) provides evidencethat these changes may result from intrinsic developmental processesas well as from increased synapticactivity.

Developmental changes in recovery from synaptic depression included a decline in the overall magnitude of depression and adecrease in the relative amount of the fast recovery component.Thus, changes in recovery time course were apparent only at intervalsup to 50 msec. This suggests that a developmental decline in theamount of synaptic depression should be present with high stimulusrates but should not be apparent during low-frequency stimulation(less than ~20 Hz). In fact, such an effect was apparent in ourresults (Fig. 3C), which indicate that the decline in synapticdepression between E18 and P6-11 was more pronounced at 333 Hzthan at 100 Hz. Because P_R is higher in embryos, such findingsmay indicate a population of vesicles that is more "releasable"and recovers more readily but declines in size with age. The dramaticreduction in synaptic depression (Fig. 3) and trend toward smallerEPSCs (Fig. 4) between P2-3 and P6-11 suggest that further changesin P_R and vesicle recovery rates may occur between these ages.In this study recovery was not examined in older (P6-11)hatchlings.

Although a fast component of recovery from depression (<100 msec) was present in nMag, at the rat calyx of Held in the MNTB(P8-10) only a slow phase of recovery was apparent (Schneggenburgeret al., 1999; Wu and Borst, 1999). In mouse (P12-15), Wang andKaczmarek (1998) also report a single, slow recovery time constant(5.0 sec at room temperature) after 100 Hz stimulation. However,when stimulus rates were increased to 300 Hz, elevated calciumlevels in the presynaptic terminal induced a fast (84 msec atroom temperature, 43% fast) phase of recovery. A calcium-dependentfast component of recovery (100 msec at room temperature, 44 msecat 34°C) after a single stimulus was also present at the climbingfiber-Purkinje cell synapse, but in low (1 mM) calcium, recoverywas monoexponential with a time course of 3.6 sec at room temperature(Dittman and Regehr, 1998). Recently, Iwasaki and Takahashi (2001)reported in rat MNTB that no developmental change occurs in thetime course of recovery from depression after 10 Hz stimulation.However, with low-frequency stimulation, fast components of recoveryare not apparent at the calyx of Held (Wang and Kaczmarek, 1998).Our findings indicate a developmental decrease in the fast componentof recovery after both single stimuli andtrains.

Recovery in nMag differs from these examples in that a fast component of recovery was present after single or multiple conditioningstimuli in standard (3 mM) or reduced (1.5 mM) calcium. The persistenceof a fast recovery component in 1.5 mM calcium suggests that acalcium-dependent recovery mechanism may be saturated by low levelsof presynaptic calcium and therefore may not influence recoverywith realistic activity rates. Mechanisms for fast recovery, whetherconstitutively active or calcium dependent, may be a common featureof auditory synapses, enabling sustained and rapidsignaling.

The values obtained in this study for quantal parameters N, P_R, and q, as well as the rate of recovery from synaptic depression,allow comparison between experimentally measured EPSCs and predictionsof a depletion model of synaptic depression (Dittman and Regehr,1998; Weis et al., 1999; Brenowitz and Trussell, 2001). As shownin Table 1, both E18 and P2-3 synapses show agreement betweenmeasured EPSCs and predicted amplitudes on the basis of parametersobtained in this study. Moreover, experimentally measured PPDagrees closely with predictions based on a depletion model, asdescribed in Brenowitz et al. (2001). For P2-3 synapses, PPD inaniracetam with a 5 msec stimulus interval was 0.44 ± 0.05 (Fig.7) compared with a prediction of 0.46 when parameters from thisstudy were used. Close agreement between observed and predictedEPSCs and PPD was also seen with embryonic synapses. However,experimentally measured steady-state EPSCs during trains wereconsistently larger than predictions of a depletion model (Brenowitzand Trussell, 2001), using recovery rates measured in this study,by a factor of 2. The developmental increase in observed steady-stateEPSC amplitudes can be attributed to lower P_R, less desensitization,and disappearance of a persistent slow component of depressionseen in embryos (Fig. 3B,C) (Brenowitz and Trussell, 2001, theirFig. 4). Discrepancies between the predicted and observed amplitudesmay indicate that activity-dependent recovery mechanisms are presentbut were not revealed when recovery was monitored with singletest pulses (Fig. 9). Previous studies at the calyx of Held (Weiset al., 1999) also indicated that measured recovery rates predictsmaller EPSCs than observed experimentally, and these authorsalso failed to observe evidence for calcium-dependence of recovery.Such findings may demonstrate shortcomings of using depletionmodels to describe synaptic transmission (Kraushaar and Jonas,2000; Matveev and Wang, 2000). Alternatively, these observationsmay provide evidence for activity-dependent enhancement of recoveryfrom synaptic depression that operates by a calcium-independentmechanism.

  FOOTNOTES

Received July 16, 2001; revised Sept. 17, 2001; accepted Sept. 18, 2001.

This work was supported by National Institutes of Health Grants DC02004, NS28901, and GM07507. We thank Drs. G. Awatramani,E. Chapman, R. Fettiplace, D. Oertel, T. Otis, R. Pearce, andH. von Gersdorff for helpful comments anddiscussion.
Correspondence should be addressed to Laurence O. Trussell, Auditory Neuroscience L-335A, Oregon Health Sciences University,3181 SW Sam Jackson Park Road, Portland OR, 97201. E-mail: trussell{at}ohsu.edu.

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