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The Journal of Neuroscience, December 15, 2000, 20(24):9162-9173
Fine-Tuning an Auditory Synapse for Speed and Fidelity:
Developmental Changes in Presynaptic Waveform, EPSC Kinetics, and
Synaptic Plasticity
Holger
Taschenberger and
Henrique
von Gersdorff
The Vollum Institute, Oregon Health Sciences University, Portland,
Oregon 97201
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ABSTRACT |
Fast, precise, and sustained synaptic transmission at high
frequency is thought to be crucial for the task of sound localization in the auditory brainstem. However, recordings from the calyx of Held
synapse have revealed severe frequency-dependent synaptic depression,
which tends to degrade the exact timing of postsynaptic spikes. Here we
investigate the functional changes occurring throughout the critical
period of synapse refinement from immature calyx terminal [postnatal
day 5 (P5)] to after the onset of hearing (P12-P14). Surprisingly,
for recordings near physiological temperature (35°C), we find that
P14 synapses are already able to follow extremely high input rates of
up to 800 Hz. This ability stems in part from a remarkable shortening
of presynaptic action potentials, which may lead to a lowering of
release probability and decrease in synaptic delays during development.
In addition, AMPA receptor-mediated EPSCs as well as quantal synaptic
currents acquired progressively faster kinetics, although their mean
amplitudes did not change significantly. NMDA receptor-mediated EPSCs,
however, diminished with age, as indicated by a 50% reduction in mean
amplitude and faster decay kinetics. Finally, the degree of synaptic
depression was greatly attenuated with age, presumably because of a
2.5-fold or larger increase in the releasable pool of vesicles, which
together with a decreasing release probability produces a fairly
constant EPSC amplitude. This finely tuned orchestra of developmental
changes thus simultaneously promotes speed while preventing premature vesicle pool depletion during prolonged bouts of firing. A few critical
days in postnatal development can thus have a large impact on synaptic function.
Key words:
development; MNTB; calyx of Held; AMPA and NMDA EPSCs; quantal and mEPSCs; short-term synaptic depression; patch-clamp; neuronal reliability
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INTRODUCTION |
Auditory brainstem circuits can
express unusually thick axons and giant, axo-somatic presynaptic
terminals with multiple active zones. The calyx of Held synapse in the
medial nucleus of the trapezoid body (MNTB) is a pivotal relay station
that is involved in sound localization (Guinan and Li, 1990 ; Oertel,
1999). The binaural cue used is the difference in sound intensity
received by the two cochleas. Contralateral inhibitory input via the
MNTB and excitatory input from the ipsilateral cochlear nucleus are received by neurons in the lateral superior olive, where the two signals are first integrated (Sanes, 1990; Park et al., 1997). It is
thought that microsecond differences in the arrival of action potentials (APs) are then used to pinpoint the locus of high-frequency sounds. Accordingly, in vivo (Rhode and Smith, 1986; Spirou
et al., 1990) and brain slice recordings (Oertel, 1983; Banks and Smith, 1992) have established that the adult calyx of Held receives and
follows high-input frequencies (e.g., 667 Hz at 34°C; Wu and Kelly,
1993). Young rats [postnatal day 8 (P8)-P11], however, can only
follow discharge rates up to 200 Hz (Borst et al., 1995; Brew and
Forsythe, 1995). Several studies at end-bulb (Wu and Oertel, 1987;
Zhang and Trussell, 1994a; Bellingham and Walmsley, 1999) and calyceal
synapses (Forsythe et al., 1998; Wang and Kaczmarek, 1998) have also
shown severe synaptic depression during stimulus trains. The reduced
EPSP size will then degrade postsynaptic AP timing (Reyes et al.,
1996).
Recent patch-clamp recordings have concentrated mostly on juvenile rats
from P8 to P11 (Forsythe, 1994; Borst et al., 1995; Chuhma and Ohmori,
1998). However, the onset of hearing in rats occurs at P12 (Blatchley
et al., 1987), and from P12 to P14 the rat cochlea undergoes its most
dramatic postnatal changes (Puel and Uziel, 1987; Oliver and Fakler,
1999), and the tonotopic map of the MNTB reaches adult properties by
P14 (Friauf, 1992). The adult calyx morphology is also reached by P14
(Kandler and Friauf, 1993). Furthermore, several developmental shifts
in expression levels of presynaptic Ca channels (Iwasaki and Takahashi,
1998), Ca-binding proteins (Lohmann and Friauf, 1996), metabotropic
(Elezgarai et al., 1999), and ionotropic (Caicedo and Eybalin, 1999)
glutamate receptors are completed by P14. The age from hearing onset to eye opening (P14) thus seems like a particularly interesting period in
which to study developmental changes in synaptic strength and plasticity.
Here we present recordings from a single synapse as it matures during
this critical developmental period. We find that presynaptic APs in
P12-P14 calyxes are 66% briefer compared with P5-P7. Synaptic delays, as well as EPSC rise times and half-widths, diminished with
increasing age, whereas EPSC amplitudes did not change significantly. Furthermore, P12-P14 synapses lacked the severe depression
characteristic of P5-P7. Finally, increasing temperature to 35°C
allowed some P14 synapses to reliably follow stimuli up to 800 Hz. The
ability to faithfully follow such high frequencies is thus because of parallel changes in both presynaptic and postsynaptic properties, which
together facilitate the precise firing of this pivotal brainstem synapse.
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MATERIALS AND METHODS |
Slice preparation. Brainstem slices were obtained
from P5 to P14 Sprague-Dawley rats. After decapitation, the brainstem
was immersed in ice-cold low-calcium artificial CSF (aCSF)
containing (in mM): NaCl (125), KCl (2.5),
MgCl2 (3.0), CaCl2 (0.1),
glucose (25), NaHCO3 (25),
NaH2PO4 (1.25), ascorbic
acid (0.4), myo-inositol (3), and Na-pyruvate (2), pH 7.3, when bubbled
with carbogen (95% O2 and
CO2 5%). The brainstem was glued onto the stage
of a vibratome slicer, and 180- to 200-µm-thick transverse slices
were cut proceeding from a caudal to rostral direction. Slices were
rapidly transferred to an incubation chamber containing normal aCSF
bubbled with carbogen and maintained at 36°C for 30 min, and
thereafter at room temperature. The normal aCSF was the same as the
low-calcium aCSF except that 1.0 mM
MgCl2 and 2.0 mM
CaCl2 were used.
Electrophysiology. Whole-cell patch-clamp recordings
were performed in normal aCSF at room temperature (RT; 21-23°C) or
at 35°C (Warner Instruments Heater system). The standard patch
pipette solution consisted of (in mM):
K-gluconate (75), KCl (75), Na2-phosphocreatine (2), HEPES (10), EGTA (5), and ATP-Mg (4), pH 7.3, with KOH. To record
NMDAR-mediated currents CsCl was substituted for K-gluconate and KCl,
and 10 mM TEA was added. During experiments
slices were continuously perfused with normal aCSF solution and
visualized by IR-DIC microscopy through a 40× water-immersion
objective (Axioskop, Zeiss, Germany) coupled to a 2× pre-magnification
(Optovart; Zeiss, Oberkochen, Germany) and a CCD camera (C79;
Hamamatsu, Tokyo, Japan). A bipolar stimulation electrode was
placed on the brainstem midline. Visualized recordings from slices
older than P11 were greatly hampered by the extensive myelinization of
the brainstem. Cells were thus patched in a "semiblind" approach,
after preselection of connected cells with extracellular AP recordings
(Guinan and Li, 1990; Borst et al., 1995). Only cells that showed
extracellular presynaptic and postsynaptic APs were chosen for
whole-cell patch-clamp recordings.
Patch pipettes were pulled from soft thin-walled glass (World Precision
Instruments, Sarasota, FL) using a Narishige (Tokyo, Japan)
puller (PP-830). Patch pipettes had an open tip resistance of 1.5-2.5
M . Access resistance (Rs) ranged
from 2.2 to 4.8 M (mean, 3.6 ± 0.2 M) with CsCl-filled
electrodes and slightly higher with K-gluconate-based internal
solution. This low uncompensated Rs
was essential for voltage-clamp recordings of the large EPSC amplitudes. Rs compensation was set to
75-90% (10 µsec delay) depending on the initial uncompensated
Rs value, producing an effective
Rs < 0.5 M. Under these
conditions, EPSC amplitudes <20 nA produced a clamp-voltage error of
<10 mV. For voltage-clamp recordings, the time constant was estimated
to be <18 µsec (Cslow capacitance < 36 pF; effective
Rs < 0.5 M). The accuracy of
voltage clamp was tested in a few cells with large EPSC amplitudes
by comparing the waveforms of control EPSCs with greatly reduced current responses obtained during application of 10-20
µM 6-7-dinitroquinoxaline-2,3-dione (DNQX)
[in the presence of 50 µM
D,L-2-amino-5-phosphonovaleric acid
(D,L-APV)]. After normalizing, the
kinetics of both EPSCs was virtually indistinguishable (data not
shown). Whole-cell leak currents were <300 pA at  70 mV in the data
set accepted for analysis. Principal cells were voltage-clamped at a
holding potential of 70 mV if not stated otherwise. No corrections
were made for liquid junction potentials.
Presynaptic and postsynaptic APs were recorded in the fast
current-clamp mode of the EPC-9 after adjusting the fast-capacitance cancellation while in cell-attached mode. After break-in, the Rs value was checked in the
voltage-clamped cell at 70 or 80 mV. Current-clamp recordings were
continued only if the initial uncompensated
Rs was <6 M. With a residual
uncompensated capacitance of ~2 pF in the EPC-9 fast
current-clamp mode (F. Sigworth, personal communication;
Sigworth et al., 1995), the time constant of the current-clamp
recordings was estimated to be <12 µsec.
Stimulation pulses were applied through a Master-8 stimulator
(AMPI, Jerusalem, Israel) and had a duration of 100 µsec and amplitudes of 2-15 V. Stimulation pulses were controlled using "Pulse" software (Heka, Lambrecht, Germany), and signals were recorded via a double EPC-9 (Heka) patch-clamp amplifier. Sampling intervals and filter settings were 10-25 µsec and 5 kHz, and 50 µsec and 3.3 kHz for AMPA- and NMDA-receptor mediated EPSCs,
respectively. D,L-APV and DNQX were from Tocris Cookson
(Bristol, UK). All other salts and chemicals were from Sigma. Offline
analysis was done with "IgorPro" software (Wavemetrics, Lake
Oswego, OR). Average data are reported as mean ± SE values.
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RESULTS |
Presynaptic and Postsynaptic APs: changes in waveform and
timing precision
The calyx of Held synapse consists of a single, large terminal
that contacts the soma of one principal cell of the MNTB. During postnatal development, the presynaptic terminal undergoes extensive morphological changes (Kandler and Friauf, 1993) reaching an adult-like morphology at P14. We first investigated whether this morphological reorganization was accompanied by functional changes in the presynaptic AP waveform. For this purpose we recorded presynaptic APs evoked by
afferent fiber stimulation at various stimulation frequencies (10-800
Hz). These are physiologically relevant frequencies because spontaneous
rates recorded in single afferent fibers of the trapezoid body range
from 10 to 80 Hz (Spirou et al., 1990). Moreover, rates driven by sound
stimulation can range from 100 to 700 Hz in adult cats (Rhode and
Smith, 1986; Spirou et al., 1990; Smith et al., 1998). Whole-cell
recordings were confirmed to be presynaptic by the following three
criteria: first, afferent stimulation evoked short-latency all-or-none
APs or "action currents", under current-clamp or voltage-clamp
conditions, respectively (Forsythe, 1994). These were followed by
characteristic small, postsynaptic potentials (elicited by APs in the
capacitatively coupled postsynaptic cells), which increased in latency
after high-frequency stimulation. Second, the recording exhibited a
complete absence of spontaneous miniature EPSCs. Finally, presynaptic
terminals had higher input resistance and more negative resting
membrane potential (approximately 80 mV). Examples of presynaptic AP
waveforms for P7, P10, and P14 slices are illustrated in Figure
1A. Mean AP amplitudes
were similar throughout development (P5-P7, 117 ± 2 mV,
n = 7; P8-P11, 120 ± 2 mV, n = 8; P12-P14, 126 ± 2 mV, n = 4;
Vr, 80 mV). However, the AP
half-width was reduced by approximately two-thirds for P12-P14 calyxes
(P5-P7, 564 ± 40 µsec; P8-P11, 334 ± 26 µsec; P12-P14, 191 ± 8 µsec), and the maximum rate of rise had
almost doubled at P12-P14 (P5-P7, 630 ± 50 mV/msec; P8-P11,
820 ± 40 mV/msec; P12-P14: 1108 ± 10 mV/msec). By
comparison, cerebellar granule cell presynaptic APs have a half-width
of 1.5 msec at RT (Sabatini and Regehr, 1997). Extremely narrow APs
(half-width of 0.25 msec at 37°C) are also observed in the rat nodes
of Ranvier, which contain a very high density of
Na+ channels (Schwarz and Eikhof,
1987).
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Figure 1.
Developmental changes in waveform and timing of
presynaptic and postsynaptic APs at the calyx of Held synapse.
A, Current-clamp whole-cell recordings of presynaptic
APs in brainstem slices at P7, P10, and P14. APs were evoked by
afferent fiber stimulation. Note the faster kinetics and shorter
duration of the APs and the presence of a fast afterhyperpolarization
in older calyxes. B, Presynaptic AP waveform for two
different P6 calyxes. One calyx was dialyzed with 0.2 mM
EGTA, whereas the other was dialyzed with 5 mM EGTA.
C, Consecutive responses to a train of afferent stimuli
(10 Hz) recorded in a presynaptic terminal at P7 (same neuron as in
A, first 10 responses). D, Comparison of
AP waveforms in postsynaptic MNTB neurons in P6 and P13 slices.
E, F, Consecutive responses to afferent stimulation at
10 Hz (same neurons as in D, first 10 responses).
G, Latency distribution of APs elicited at 10 Hz. Pooled
data from P5-P7 (n = 6) and P12-P14
(n = 4) slices. Latency was calculated as the time
from negative peak of the prepotential to the peak of the postsynaptic
APs. During development, the latency between presynaptic and
postsynaptic APs decreased and the jitter in AP timing was reduced.
Mean latency was 2.09 ± 0.24 and 0.64 ± 0.03 msec
for P5-P7 and P12-P14 slices, respectively. Latency distribution of
the presynaptic APs is shown for comparison (same neuron as in
C). K-gluconate-filled electrodes were used and
experiments were done at room temperature. The resting membrane
potential (Vr) was 80 and 70 mV
for presynaptic and postsynaptic neurons, respectively. Stimulus
artifacts were blanked for clarity.
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Presynaptic P12-P14 APs also had a more pronounced
afterhyperpolarization followed by a small afterdepolarization. The
slow afterdepolarization was previously suggested to originate from the
charging of the electrical capacitance of the large-diameter axon
(Borst et al., 1995). It is conceivable that the myelinization starting
at P8 in rat MNTB (K. Kandler and E. Friauf, personal communication), may reduce the capacitance of the axon. However, as shown in Figure 1A, we did not observe a
significant change in the presynaptic AP afterdepolarization with age.
Presynaptic whole-cell current-clamp recordings illustrated in Figure
1A were obtained with 5 mM EGTA
in the patch pipette. To clarify whether this concentration of mobile
Ca2+ buffer could uncouple
Ca2+-activated
K+ conductances and thereby slow the time
course of the presynaptic AP, we conducted additional experiments with
a lower EGTA concentration in the internal solution (0.2 mM; Borst and Sakmann, 1996). As shown in Figure
2B, this 25-fold lower
Ca2+ buffer concentration did not affect
the presynaptic AP waveform. Using 0.2 instead of 5 mM EGTA in the pipette solution, we obtained similar average values for AP amplitude (P5-P7, 115 ± 2 mV,
n = 5; P8-P11, 124 ± 3 mV, n = 4), half-width (P5-P7, 504 ± 27 µsec; P8-P11, 323 ± 25 µsec), and rate of rise (P5-P7, 668 ± 17 mV/msec; P8-P11,
894 ± 32 mV/msec) (p > 0.05, two-tailed
Student's t test).
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Figure 2.
The capacity for high-frequency transmission is
fully established by the end of the second postnatal week. A,
B, Postsynaptic APs in response to trains of 15 stimuli (100 Hz) recorded in P5 (A) and P14
(B) brainstem slices at room temperature. At P5,
usually only the first two to three EPSPs were suprathreshold and
generated APs in the postsynaptic neuron. Note the strong AP adaptation
and large plateau depolarization at P5, which are both absent at P14.
C, D, Current-clamp recordings at near physiological
temperature (35°C). In P12-P14 slices, reliable synaptic
transmission was generally possible at frequencies up to 600 Hz under
these conditions (50 stimuli; C). Occasionally,
postsynaptic neurons were able to respond to afferent stimulation up to
800 Hz without failures of AP generation (15 stimuli;
D). K-gluconate-filled electrodes.
Vr was approximately 70 mV. Notice
that for the 800 Hz frequency the exact timing of the APs late in the
train becomes less precise, as evidenced by the stimulus artifact
falling progressively further into the down stroke phase of the
preceding spike (D).
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An example of P7 APs elicited by afferent fiber stimulation at 10 Hz is
illustrated in Figure 1C. At all ages, the fluctuation in
the exact timing of the AP peak ("jitter") was <50 µsec at this
stimulation frequency. At RT, AP generation in presynaptic calyxes
could follow stimulation frequencies up to 200-300 Hz, but failed at
400 Hz or higher in P5-P7 slices. In contrast, frequencies up to 500 Hz (RT) or up to 800 Hz (35°C) were faithfully followed in P12-P14
calyxes (data not illustrated).
Examples of individual postsynaptic APs for P6 and P13 are shown in
Figure 1D. Compared with calyceal APs, postsynaptic
APs were generally smaller in amplitude and had a slower time course. In addition, similarly to the presynaptic terminal we also observed a
shortening of the AP waveforms in the postsynaptic neuron during development, whereas AP amplitudes did not significantly change [Fig.
1D; average values at P5-P7 (n = 11)
versus P12-P14 (n = 10) for AP amplitudes, 100 ± 2 mV versus 104 ± 2 mV; half-width, 980 ± 72 µsec versus
457 ± 15 µsec, maximum rate of rise, 377 ± 23 mV/msec
versus 582 ± 31 mV/msec; Vr
approximately 70 mV]. However, the timing pattern of postsynaptic
APs during repetitive stimulation was profoundly different for both
ages. For example, the P6 synapse of Figure 1E had a
latency between the presynaptic prepotential (defined below) and the
peak of postsynaptic APs that ranged from 1 to >4 msec (mean latency
of 2.90 msec). This occurred despite the fact that presynaptic APs at
P5-P7 had a jitter in peak timing of <50 µs (Fig.
1C). By contrast, the P13 synapse illustrated in Figure
1F had a mean latency of 0.58 msec (range, 0.42-0.66
msec). In Figure 1G, latency histograms obtained from pooled
data of 6 (P5-P7) and 4 (P12-P14) principal cells are shown. For each
neuron, the timing of the presynaptic AP was estimated from the
prepotential in the respective voltage-clamp recording. The
distributions are strikingly different and do not overlap. For
comparison, the latency distribution for the calyceal APs shown in
Figure 1C is given (normalized to time 0). It is evident
that the fidelity by which timing information is being transmitted has
greatly increased from P5 to P7 and from P12 to P14. This agrees well
with previous recordings that tested 0.2 Hz stimulation frequencies in
P4 and P9-P10 rats (Chuhma and Ohmori, 1998).
We next tested at various stages of development whether afferent fiber
stimulation at high frequencies (>100 Hz) could reliably evoke
postsynaptic APs. Figure 2, A and B, illustrates
current-clamp recordings after afferent fiber stimulation with 100 Hz
trains for P5 and P14 postsynaptic neurons. Both experiments were
performed at RT. At P5 typically only the first two or three EPSPs were suprathreshold. A pronounced AP adaptation and large plateau
depolarization was observed. In contrast, the same 100 Hz stimulation
triggered well timed and large postsynaptic APs during the whole train
without a decline in AP amplitude in the P14 neuron. Furthermore, the large plateau depolarization, presumably because of a summation of slow
NMDAR-mediated EPSPs (see below), was significantly reduced at P14
(Forsythe and Barnes-Davies, 1993; Zhang and Trussell, 1994a). In fact,
at RT this same P14 neuron could reliably generate APs for stimulation
frequencies of up to 400 Hz throughout the stimulus train. When the
bath temperature was increased to more physiological values (35°C),
the frequency range for reliable synaptic transmission was greatly
expanded. At 35°C principal cells followed input frequencies of up to
600 Hz for long tetanic stimulation (50 stimuli, Fig. 2C;
n = 5 cells) and up to 700-800 Hz for shorter trains
(15 stimuli, Fig. 2D; n = 3 cells).
Decrease in NMDAR-mediated EPSC amplitudes
We next characterized the underlying synaptic currents responsible
for triggering the postsynaptic APs of Figures 1 and 2. Afferent
stimulation evokes dual-component EPSCs in principal cells of the MNTB
(Forsythe and Barnes-Davies, 1993). In many glutamatergic synapses the
ratio of slow NMDAR-mediated (INMDA) to fast AMPAR-mediated (IAMPA) EPSC
component decreases with development (Hestrin, 1992; Shi et al., 1997;
Bellingham et al., 1998). We therefore investigated whether the size of
synaptic NMDAR current changed from P5 to P14 at the calyx of Held
synapse. Both EPSC components were isolated by measuring their peak
amplitudes at 75 mV and at +50 mV for
IAMPA and
INMDA, respectively. Figure 3, A and B,
illustrates families of EPSCs recorded from P6 (Fig. 3A) and
P14 (Fig. 3B) at various holding potentials. Although EPSC
peak amplitudes at Vh = 75 mV were
comparable for both ages, amplitudes of
INMDA were largely reduced at P14. In
addition, the NMDAR-mediated EPSC decayed faster for P14 compared with
P6 as is evident from Figure 3C, showing both current
responses normalized and superimposed. This faster decay of NMDA EPSCs
is indicative of a developmental change from NMDA receptor channels
containing NR2B subunits to those containing NR2A subunits with age
(Flint et al., 1997). As summarized in Figure 3D, mean
amplitudes of AMPA EPSC did not change significantly with development
(Table 1), whereas NMDA EPSCs were on
average reduced by ~50% (15.4 ± 2.9 vs 7.8 ± 1.1 nA)
from P5-P7 (n = 5) to P12-P14 (n = 8). Thus, the ratio
INMDA:IAMPA
decreased considerably in older slices (Table 1).
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Figure 3.
During postnatal development, NMDA
receptor-mediated EPSCs decreased in amplitude and acquired faster
kinetics. A, B, Families of evoked EPSCs were recorded
at various holding potentials (Vh, as
indicated) in P6 (A) and P14
(B) brainstem slices. At P14, amplitudes of
INMDA were largely reduced, whereas
IAMPA remained approximately constant
throughout development. C, Same neurons as depicted in
A and B. To facilitate comparison, EPSCs
evoked at Vh = +50 mV are shown
superimposed. Current responses were normalized and aligned at their
peak amplitudes of INMDA. D,
Summary data of five and eight different cells for P5-P7 and P12-P14,
respectively. Mean amplitudes of peak IAMPA
were 13.76 ± 1.36 and 12.96 ± 1.25 nA
(Vh = 75 mV), and mean amplitudes of
peak INMDA were 15.4 ± 2.92 and
7.8 ± 1.06 nA (Vh = +50 mV) for
P5-P7 and P12-P14, respectively. E, F, Current-clamp
recordings of postsynaptic APs evoked by afferent fiber stimuli (100 Hz) under control conditions and during application of 50 µM D,L-APV
(Vr = 70 mV). E, At P6
(n = 6 cells), APV strongly reduced the large plateau
depolarization but had no effect on the number of APs generated during
the stimulus train. Inset, Voltage-clamp recordings
(Vh = 30 mV) from the same cell; AMPA
EPSCs truncated for clarity. F, At P14, 50 µM D,L-APV had little effect on postsynaptic
responses. CsCl and K-gluconate-based internal solutions were used in
the experiments illustrated in A-D and E
and F, respectively.
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Table 1.
Developmental changes in synaptic delay, EPSC kinetics, and
short-term plasticity at the calyx of Held synapse
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In current-clamp recordings, high-frequency (>100 Hz) afferent
stimulation produced a long-lasting depolarization in postsynaptic MNTB
neurons that was especially pronounced in P5-P7 slices (Fig. 2A). Presumably this was caused by summation of slow
NMDA receptor-mediated EPSPs during the trains. Given the large
amplitude of INMDA in P5-P7 animals,
it is conceivable that this prolonged depolarization could
progressively inactivate Na channels and thereby prevent repetitive AP
generation. We therefore asked whether blocking NMDA receptor
activation affects the number of APs generated during a stimulus train.
Figure 3E illustrates a P6 synapse stimulated at 100 Hz in
the absence and presence of 50 µM
D,L-APV, a specific blocker of
INMDA (Fig. 3E, inset).
Although APV greatly reduced the plateau depolarization, blocking
INMDA did not affect the number of APs
generated during afferent fiber stimulation. However, the same neuron
was able to generate trains of APs after injection of depolarizing
current pulses (100 Hz, 1 msec pulses of 1nA; data not shown).
Nevertheless, it is conceivable that Na channel inactivation caused by
the slow plateau depolarization may contribute to the reduction in AP
amplitude as seen in Figures 2A and 3E. By
contrast, in P14 animals, APV caused only a small reduction in the
plateau depolarization (Fig. 3F). This suggests that
although there is still a significant amount of
INMDA at P14, it plays a gradually
diminishing role during the first 2 weeks of postnatal development.
Shortening of synaptic delays and faster kinetics of
AMPAR-mediated EPSC
The timing of the postsynaptic APs is primarily determined by the
synaptic delay as well as the amplitude and kinetics of the fast
AMPAR-mediated EPSC. We therefore measured synaptic delays and
quantified changes in kinetics of
IAMPA as a function of age. The
synaptic delay was determined from the negative peak of the prepotential to the beginning of the EPSC (20% rise time point). The
prepotential is a biphasic reflection of the calyx AP, and can usually
be clearly detected in postsynaptic voltage-clamp recordings. Its
negative peak coincides with the maximum rate of rise of the
presynaptic AP (Borst et al., 1995). Figure
4, A and B,
exemplifies EPSCs for P7 and P14 and illustrates the shortening of
synaptic delays from P7 to P14 cells. Both traces were aligned at the
lower peak of the prepotential that is marked with a dashed line. On
average, the synaptic delay was reduced by 291 µsec from P5-P7 to
P12-P14 (Table 1). To facilitate comparison of their waveforms, the
EPSCs were aligned at their initial rise and normalized in Figure
4B. Notice that both rise time and decay of the EPSCs
were faster for P14 than for P7. In Figure 4, the 20-80% rise times
(C), half-widths (D), and EPSC
amplitudes (E) of our full data set are plotted as a
function of age. Measured rise times and half widths ranged from 107 to
259 µsec (mean, 162 ± 3 µsec; n = 155) and
from 251 to 1694 µsec (mean,758 ± 27 µsec; n = 155). Although there was some cell to cell variability, a highly
significant developmental trend toward shorter rise times and
half-widths is evident (see also Table 1 for comparison of P5-P7 to
P12-P14). EPSC amplitudes ranged from 1.3 to 19.7 nA (mean,
9.1 ± 0.3 nA; n = 155) and exhibited a large
variability at all ages. The small increase in mean EPSC amplitudes
with age was not significant.
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Figure 4.
Developmental changes in synaptic
current kinetics for AMPA receptor-mediated EPSCs. A,
Sample EPSCs recorded in P7 and P14 brainstem slices
(Vh = 70 mV). Current responses were
aligned at the negative peak of the prepotential (dotted
line). Note the shorter synaptic delay and faster time course
at P14. B, Same responses as depicted in
A. To facilitate comparison, amplitudes were normalized,
and EPSCs were aligned at their onsets. C-E, Pooled
data for EPSC rise times (C), half widths
(D), and peak amplitudes
(E) from a total of >130 cells plotted versus
postnatal age. Solid and dotted lines
indicate linear regression and 99% confidence limits, respectively.
Regression coefficients and number of cells as indicated at each panel.
Both EPSC rise times and half widths decreased significantly
(p < 0.0001) during development. In
contrast, only little increase in EPSC peak amplitudes was observed
(p > 0.05).
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Changes in kinetics and latencies of evoked quantal EPSCs
In addition to channel kinetics, the waveform of evoked EPSCs at
different synapses is shaped by asynchronous release of individual quanta (Katz and Miledi, 1965; Diamond and Jahr, 1995; Isaacson and
Walmsley, 1995). At the calyx of Held synapse a single EPSC is composed
of ~200 quantal events (Borst and Sakmann, 1996). A variable degree
of asynchrony in the presynaptic release process could thus have a profound impact on the EPSCs
kinetics. Indeed, a large amount of jitter in the timing of EPSCs has
been reported for very young (P4) rats (Chuhma and Ohmori, 1998).
To estimate the contribution of asynchronous release to differences in
EPSC kinetics, we recorded miniature EPSCs (mEPSCs) and also evoked
quantal EPSCs under conditions of strongly reduced probability of
release (50 µM Cd2+ added to
the external solution; Isaacson and Walmsley, 1995). Under these
conditions maximum EPSC amplitudes evoked by afferent fiber stimulation
were <200 pA, and many stimuli failed to evoke a response (average
failure rate 30%). However, the prepotentials were unaffected by 50 µM Cd2+, indicating that
failures of glutamate release were not caused by failures of
presynaptic AP propagation or excitability. Moreover, 100 µM Cd2+ does not affect the
presynaptic AP waveform (Borst et al., 1995). We preferred to analyze
evoked quantal EPSCs as opposed to spontaneous mEPSCs, because
principal cells of the MNTB receive numerous non-calyceal excitatory
inputs (Banks and Smith, 1992; Forsythe and Barnes-Davies, 1993; Smith
et al., 1998). Excitatory inputs that could be identified as
non-calyceal by their much longer latencies and slower kinetics were
noticed in several recordings, especially from more mature slices (data
not shown). By recording evoked calyceal quantal EPSCs we thus excluded
these events generated from bouton-type terminals from our analysis.
Examples of mEPSCs and evoked quantal EPSCs for P5 and P14 are shown in
Figure 5A-D. Notice the large
variability in amplitude at both ages but the much faster current
kinetics at P14. Because we were interested in determining the exact
kinetics and latency of quantal responses, events with amplitudes >20
pA were selected, and rarely occurring EPSCs >150 pA were discarded.
This amplitude range corresponded to that observed for spontaneous
mEPSCs (Fig. 5A,C). Moreover, these evoked quantal events
had clearly defined monotonic rise times, with relatively little
contamination from baseline noise. Similarly to control EPSCs (Fig.
4A), evoked quantal EPSCs had shorter synaptic delays
for P14 compared with P5 (Fig. 5B,C). However, at both ages,
individual quantal events occurred stochastically within a comparably
narrow time window. Furthermore, evoked quantal EPSCs had much faster
rise and decay at P14 compared with P7. Figure 5E shows the
average quantal EPSC obtained from unaligned (solid line) and
aligned (at their 50% rise point, dotted line)
evoked events. For the P5 cell shown in Figure 5E, mean peak
amplitude, 20-80% rise time, and the half-width were 62 pA, 221 µsec, 1406 µsec, and 59 pA, 310 µsec, and 1477 µsec for aligned and unaligned events, respectively. The corresponding values
for the P14 cell amounted to 72 pA, 127 µsec, 441 µsec, and 62
pA, 176 µsec, and 541 µsec for aligned and unaligned events, respectively. For both ages, average EPSC waveforms obtained from aligned quantal events thus rose and decayed more quickly than those
computed from unaligned quantal events, as expected from previous
findings for P8-P10 rats (Borst and Sakmann, 1996).
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Figure 5.
Asynchronous transmitter release does not account
for slower EPSC waveforms in P5-P7 slices. A, C,
Spontaneous miniature EPSCs recorded at P5 (A)
and P14 (C) are superimposed and aligned at their
peak amplitude. B, D, Evoked quantal EPSCs recorded at
greatly reduced probability of release (50 µM
CdCl2 included in the bath solution) at P5
(B) and P14 (D).
Occasionally occurring EPSCs with amplitudes >150 pA were discarded.
The events in A-D are from four different cells, and 15 sample traces are shown superimposed. mEPSCs were collected under the
same recording conditions (with 50 µM
CdCl2) from 10 to 200 msec after the stimulus. Note
the difference in synaptic delays and EPSC kinetics in B
and D. Stimulus frequency for evoked quantal events was
1-2 Hz. E, Average waveforms of quantal EPSCs were
obtained either with (dotted lines) or without
(solid lines) previous aligning of individual EPSCs at
their 50% rise points. 170 and 125 responses were averaged for P5 and
P14, respectively. At both ages, aligned EPSC gave rise to slightly
faster kinetics of the averaged EPSC waveform. 20-80% rise times were
221 versus 310 µsec (P5) and 128 versus 176 µsec (P14) for the
aligned and unaligned EPSCs, respectively. Half widths were 1406 versus
1477 µsec (P5) and 441 versus 541 µsec (P14) for waveforms obtained
from aligned and unaligned EPSC, respectively. F,
Latency distribution of quantal EPSC. Latency was calculated as the
time difference between negative peak of the prepotential and 20% rise
point of the EPSCs. Pooled data obtained from four different cells in
each age group.
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To compare the variability of synaptic delays at both ages, synaptic
latencies were obtained for a total of four cells (>100 quantal
events/cell) in each age group. Latency histograms of the pooled data
are shown in Figure 5F (Barrett and Stevens, 1972). The two
histograms were temporally shifted by the difference in average
synaptic delay, and when they were superimposed, the P5-P7 histogram
was slightly wider than the P12-P14 histogram. The mean variance of
the synaptic delays was smaller for P12-14 (0.019 ± 0.006 msec2; n = 4) compared
with P5-P7 (0.037 ± 0.005 msec2;
n = 4) (p = 0.003; Student's
t test). This suggests that a smaller degree of asynchrony
in glutamate release may additionally contribute to the faster EPSC
kinetics in older animals.
Reduced synaptic depression and larger vesicle pool size
We next studied the developmental changes in frequency-dependent
depression of EPSCs. Recordings with similar initial peak amplitude
from P6 and P14 slices are shown in Figure
6. For P6 robust synaptic depression was
induced already at 10 Hz stimulation, and steady-state depression was
>95% for 100 Hz (Fig. 6A,B). In contrast, the
degree of depression was greatly reduced at P14 at the same stimulation
frequencies (Fig. 6C,D). At this age, the synapses were
generally capable of transmitting at high stimulus frequencies of 300 Hz in RT (Fig. 6E) and sometimes up to 500 Hz (Fig.
6F). The P14 EPSC of Figure 6C, for
example, had an initial peak amplitude of 13.3 nA. After 15 stimuli in
a 100 Hz train, the last EPSC still had a large amplitude of 5.4 nA. By
contrast, the P6 cell at 100 Hz (Fig. 6B) started
with a comparable amplitude of 14 nA, but was reduced to 0.21 nA by the
fourth EPSC in the train. The degree of steady-state depression
elicited by high-frequency stimulation was thus greatly reduced with
age. Nevertheless, for sufficiently high frequencies (e.g., 500 Hz,
Fig. 6F), a severe synaptic depression could still be
induced even in P14 synapses.
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Figure 6.
Frequency-dependent short-term depression at the
calyx of Held synapse during development. A-D, EPSC
trains evoked by afferent stimulation at 10 Hz (25 stimuli;
A, C) and 100 Hz (15 stimuli;
B, D). Data from two different cells
(A, B, P6; C,
D, P14) with similar peak amplitudes of the initial
EPSCs are shown. Vh = 70 mV.
E, F, Same neuron as depicted in C and
D. Stimulation frequency was 300 Hz
(E) and 500 Hz (F). For
A-F, mean amplitudes of depressed EPSCs (last five
EPSCs during a train) amounted to 1.91 nA (10 Hz), 0.32 nA (100 Hz),
and 6.45 nA (10 Hz), 5.41 nA (100 Hz), 2.98 nA (300 Hz), and 1.95 nA
(500 Hz) for P6 and P14, respectively.
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Average data for 115 different cells tested at 10 Hz between postnatal
days 5 and 14 are illustrated in Figure
7A. Although the degree of
synaptic depression was variable at any given stage of development,
there was a clear developmental trend toward less depression. This
trend was statistically highly significant. On average, the depression
measured at 10 Hz decreased from 84% (P5) to 56% (P14). With regard
to the variability of depression portrayed in Figure 7A, it
is noteworthy that the MNTB is not a homogeneous nucleus of cells, but
in fact has a tonotopically organized map of best frequency cells
(Friauf, 1992).
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Figure 7.
Synaptic depression and vesicle pool size during
postnatal development. A, Synaptic depression at 10 Hz.
The ratio between the initial EPSC over the mean steady-state depressed
EPSC (last five stimuli) after 25 stimuli was calculated for each cell
and expressed as a percentage. Pooled data for a total of 115 cells
plotted versus postnatal age. Solid and dotted
lines indicate linear regression and 99% confidence limits,
respectively. B, Average data of synaptic depression for
various stimulation frequencies in P5-P7 (open symbols)
and P12-P14 (filled symbols) slices. Three
frequencies (10, 100, and 300 Hz; n = 25 cells) were tested
for each age group. For P5-P7, depression obtained with 100 and 300 Hz
was similar, and therefore only the 100 Hz data points were included.
Solid lines represent single exponential fits to the
data points ( values for 10 and 100 Hz were 69.2 and 6.1 msec for
P5-P7 vs 233.3 and 23.2 msec for P12-P14, respectively). Note that a
30 times higher stimulation frequency was necessary to obtain a similar
amount of depression in P12-P14 slices as seen with 10 Hz at P5-P7.
C, Cumulative EPSC amplitudes obtained by adding EPSC
amplitudes during the 100 and 300 Hz trains (same symbols as in
B) to estimate change in vesicle pool sizes.
Dotted lines represent linear fits to the last five EPSC
amplitudes during the train back-extrapolated to 0 to estimate the
cumulative EPSC amplitudes before steady-state depression. At P12-P14,
the estimated pool size was 2.5-3× larger than P5-P7.
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In a subset of cells, we further tested depression for stimulus
frequencies of 100 and 300 Hz. Average data of these experiments are
illustrated in Figure 7B. At P5-P7, steady-state depression was already reached with the fifth stimuli at 10 and 100 Hz, whereas at
P12-P14 at least 10 stimuli were needed to reach steady state at 300 Hz. At this age, a 30× higher stimulation frequency was necessary to
achieve a comparable degree of steady-state depression as seen with 10 Hz at P5-P7. The degree of steady-state depression is thus strongly
regulated during development.
Assuming that vesicle pool depletion accounts for most of the severe
depression at 100 Hz for P6, and the strong depression at 300 Hz for
P14, we next estimated the size of the readily releasable pool of
synaptic vesicles for the two age groups. As an index of vesicle pool
size we used the cumulative EPSC amplitude (Schneggenburger et al.,
1999). The results of this analysis are shown in Figure 7C.
The summed P5-P7 EPSC amplitudes (represented by open triangles; same
data as in Fig. 7B) quickly reached a plateau value. A
linear fit over the last points during the train was then
back-extrapolated to yield an estimate for the initial pool size
proportional to 12 nA. A similar analysis for 100 Hz (solid triangles)
and 300 Hz (solid circles) gives values of 25 and 30 nA, respectively, for the pool size. This is a 2.1 and 2.5× larger pool size estimate for P12-P14 than for P5-P7. Because the 300 Hz train was presumably more depleting than 100 Hz, we estimate that the average pool size at
P12-P14 is probably closer to 30 nA. In fact, for some P14 cells
(e.g., the cell shown in Fig. 6F), the cumulative
EPSC, or pool size, was 40 nA. Moreover, because this analysis does not
take into account AMPA receptor saturation or desensitization, this
number is only a lower bound (Wu and Borst, 1999). The pool size could
in fact be larger, especially considering that desensitization may be
more pronounced at higher frequencies (Trussell, 1999). We thus
conclude that the readily releasable pool size probably increased on
average by a factor of at least 2.5-fold from P5-7 to
P12-P14.
Effects of temperature on single EPSCs and EPSC trains
We next studied the effects of temperature on EPSC kinetics
and synaptic depression. High temperature had striking effects on
single EPSCs and EPSC trains. We first noticed a marked decrease in the
synaptic delay as temperature was increased from RT (21-23°C) to
35°C (Fig. 8A,B). In
younger animals we observed a larger decrease in synaptic delay than in
older ones. At P5-P7 the synaptic delay decrease by 495 ± 33 µsec (n = 7), whereas at P12-P14 the reduction was
only 244 ± 48 µsec (n = 6). This difference was
statistically significant (t test; p < 0.001). Figure 8C shows an expanded view of the prepotential
and initial rise of the EPSC for a P6 cell. Previous observations in
P8-P10 rats indicated a decrease in delay of 500 µsec (Borst et al.,
1995). EPSC peak amplitudes also clearly increased at higher
temperature, and both rise time and decay were faster (Fig.
8A,B; Zhang and Trussell, 1994b). Finally, the amplitude of the steady state depressed EPSC in a train was also increased by raising the temperature from RT to 35°C (Fig.
8D; Brenowitz et al., 1998). These effects will all
clearly aid the synapse in its capacity to transmit at higher
frequencies.
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Figure 8.
Temperature dependence of synaptic delay,
EPSC time course, and synaptic depression. A, B,
Comparison of EPSC waveforms at RT and 35°C for P6
(A) and P14 (B) brainstem
slices. The 20-80% rise times were 220 and 136 msec (P6)
and 122 and 95 msec (P14) for RT and 35°C, respectively.
C, Temperature-dependent shift of prepotential and EPSC
onset in another P6 neuron shown at a faster time scale.
D, Comparison of EPSCs evoked by high-frequency afferent
stimulation (100 Hz) at room temperature (blue trace)
and 35°C (red trace). Same neuron as shown in
B. In this neuron, synaptic depression was reduced from
77% at room temperature to 65% at 35°C. In these examples, the
temperature was raised from RT (21-23°C) to 35°C in <5 min, and
all effects were fully reversible.
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DISCUSSION |
Our results indicate that the calyx of Held synapse undergoes
major presynaptic and postsynaptic developmental changes that progressively lead to its capacity to follow near kilohertz frequencies of stimulation by the end of the second postnatal week.
Presynaptic developmental changes
Presynaptic APs were >60% more brief for P12-P14 rats compared
with P5-P7. Our P5-P7 calyx APs had amplitudes and half-widths similar to those reported previously for P8-P10 (Borst et al., 1995;
Schneggenburger et al., 1999). However, the small
afterhyperpolarization described for some P8-P10 APs (Borst et al.,
1995), which was also present in our recordings from P12-P14 calyxes,
was not seen at P5-P7. Interestingly, the calyx of Held undergoes a
dramatic morphological transition from a spoon-like, amoebae-shaped
structure with fine appendages to a digitiform, floral-like structure
during this period (Kandler and Friauf, 1993). Changes in presynaptic activity may further influence neuronal morphology (Pasic et
al., 1994). Our results suggest that ion channel
densities, kinetics, and/or repertoire (Tan and Llano, 1999) also
change in parallel, leading to a briefer AP. We speculate that the
faster AP kinetics may be caused by a higher density of
Na+ and K+
channels with age (Wang et al., 1998).
Mechanisms for reducing synaptic delay and depression
A corollary effect of a shorter calyx AP is a briefer presynaptic
Ca current. This will have important consequences. First, the earlier
down stroke of the AP will trigger an earlier Ca current and thus
shorten synaptic delay (Llinás, 1999). Interestingly, the average
synaptic delay was reduced by 291 µsec from P5-P7 to P12-P14,
whereas the average reduction in presynaptic AP half-width was 373 µsec (see also Wu and Oertel, 1987). Thus, a large part of the
reduction in synaptic delay may be related to the decrease in AP width
with age. Second, the faster up and down stroke of the AP will open and
close presynaptic Ca channels more quickly producing a more phasic and
confined period of transmitter release. Indeed, we observed however
only a slight sharpening of the quantal EPSC latency histogram (Fig.
5F). Finally, the briefer Ca current may reduce the
probability of release. Accordingly, broader presynaptic APs are
usually associated with larger EPSCs (Augustine, 1990; Wheeler et al.,
1996; Wang and Kaczmarek, 1998; Borst and Sakmann, 1999). However, we
did not observe a decrease in the initial EPSC amplitude with age. On
the other hand, we did observed a decrease in the amount of
paired-pulse depression when calculated from the first two EPSCs during
a 10 Hz stimulus train (Fig. 6A,C), which again
suggests a reduction in release probability (Stevens and Wang, 1995).
The similar EPSC amplitudes in both age groups may thus be because of
antagonistic effects of a decrease in release probability and an
increase in vesicle pool size. The shortening of presynaptic APs may
represent a possible general mechanism underlying the decrease in
release probability typically observed at different CNS synapses during
development (Bolshakov and Siegelbaum, 1995; Pouzat and Hestrin,
1997).
Another factor that consistently reduces synaptic delays is increasing
temperature, which also leads to shorter presynaptic APs (Sabatini and
Regehr, 1996; Llinás, 1999). Indeed, at 36°C the calyx AP
half-width is only 250 µsec for P8-P10 rats (Borst and Sakmann,
1998). At mammalian physiological temperatures the adult calyx AP could
last for only 100 µsec, and would thus be well suited for
high-frequency transmission. The small variability in synaptic delays
throughout development may be related to the calyceal geometry of the
terminal that allows the invading AP to synchronously open a large
number of Ca channels in spatially separated active zones.
Interestingly, the mean synaptic delay of evoked quantal responses in
the presence of 50 µM Cd was increased by ~180 µsec
compared with the synaptic delay of the control EPSC (Table 1). This
could be because of the greatly reduced presynaptic Ca current
amplitude with Cd.
It has previously been suggested for this synapse that synaptic
depression induced at frequencies of 10-100 Hz is mainly caused by a
reduction in glutamate release rather than postsynaptic receptor desensitization (von Gersdorff et al., 1997; Wang and Kaczmarek, 1998).
Here we greatly extended the range of stimulation frequencies and found
a remarkable reduction in the degree of depression during development.
Presumably, young calyxes quickly exhaust their pool of readily
releasable vesicles and are not able to replenish it fast enough. In
fact, even at 10 Hz P5-P7 synapses undergo severe depression. On the
other hand, much higher stimulation frequencies (300-500 Hz) were
necessary to observe a similar amount of depression at P14. At this
age, the terminal may have a larger initial vesicle pool and/or a more
efficient capacity to replenish the depleted pool (Wang and Kaczmarek,
1998). Disregarding desensitization and assuming that the quantal size
does not change significantly with development, as suggested by Figure
5C (Chuhma and Ohmori, 1998), we roughly estimated an at
least 2.5-fold increase in pool size (12-30 nA). With a mean quantal
amplitude of 32 pA (Chuhma and Ohmori, 1998; Schneggenburger et al.,
1999) this could correspond to an average increase in pool size from
~375 to 940 vesicles. For P8-PP10 calyxes the estimated pool size is
proportional to 18 nA (~600 vesicles; Schneggenburger et al., 1999).
Thus, there may be a progressive increase in vesicle pool size as the
active zones mature during development.
Postsynaptic changes that aid in high-frequency transmission
The faster EPSC kinetics at P12-P14 could have presynaptic
origins, such as less jitter in glutamate release. This could be caused
by a developmental increase in the Ca+2
channel density (Chuhma and Ohmori, 1998). Alternatively, postsynaptic mechanisms could account for more rapid EPSC kinetics if the underlying AMPA receptors acquired a faster kinetics with age. Here we report that
the kinetics of evoked quantal responses was similar to control EPSCs
throughout development. The faster EPSC waveform at P12-P14 thus
probably has a mostly postsynaptic origin, perhaps stemming from the
expression of different AMPA receptors during development (Lawrence and
Trussell, 2000). Interestingly, a recent developmental study of AMPA
receptor subtype expression in the rat MNTB has revealed an increase in
GluRD expression after P8 (Caicedo and Eybalin, 1999). AMPA receptors
composed of this subunit have the fastest activation and deactivation
kinetics (Geiger et al., 1995). We also emphasize that the average EPSC
rise time of 127 µsec measured for P12-P14 may have undergone
significant filtering (Silver et al., 1992; Stiles et al., 1999). The
unfiltered 20-80% rise time is likely to be <100 µsec in adult
animals. Such fast rise times may be particularly suitable for
registering the exact onset of stimuli.
In addition, we also observed a reduction in amplitudes and faster
decays of NMDA EPSCs with development, as reported previously at other
CNS synapses (Hestrin, 1992; Zhou and Parks, 1992; Shi et al., 1997).
This may aid the synapse at high-frequency transmission by avoiding a
large depolarizing plateau. Finally, we observed a progressive
shortening of postsynaptic APs with age (Kandler and Friauf, 1995).
Similarly, a shortening of somatic APs during development, because of
an increase in delayed rectifier K+
channel density, was observed in developing Xenopus neurons
(Spitzer and Ribera, 1998), which also undergo a developmental shift
from NMDA to AMPA receptor expression (Wu et al., 1996).
Comparison with previous studies and other synapses
A previous study (Chuhma and Ohmori, 1998) of developmental
changes in EPSCs at the calyx of Held focused on P4 to P11 rats and did
not address changes in short-term plasticity during repetitive stimulation. We confirm their finding that postsynaptic APs jitter more
in young rats, however we did not observe their large degree of EPSC
asynchrony at P5-P7. Also, in contrast to this previous study, we
observed a progressive decrease in EPSC rise times and no significant
change in EPSC amplitudes from P5 to P14. In addition, we found
significantly faster EPSC kinetics for mEPSC and evoked quantal
responses at P12-P14. These differences may be attributable in part to
the different ages used for comparisons and other methodological differences. Interestingly, at the end-bulb synapse of the rat cochlear
nucleus, both EPSC quantal size and quantal content increased with age
(Bellingham et al., 1998).
Reliable transmission occurred in P14 calyx of Held synapses at
frequencies up to 800 Hz. How does this compare to other synapses? In
the neocortex, for example, synaptic depression can be already quite
severe at 20-50 Hz (Galarreta and Hestrin, 1998; Varela et al., 1999).
In the cochlear nucleus, however, octopus cells can follow inputs of up
to 1000 Hz, but accomplish this by receiving multiple synapses from
distinct auditory nerve fibers (Rhode and Smith, 1986; Oertel, 1999).
Thus, at a single synapse level, the calyx of Held synapse, with its
multiple active zones, appears to be among the fastest and most
reliable of CNS synapses in its ability to follow prolonged
high-frequency input. As previously suspected from its unique
morphology, the calyx of Held synapse thus seems specifically designed
to operate at extreme speed, in a sustained manner, without succumbing
to severe synaptic fatigue or depression.
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FOOTNOTES |
Received Aug. 23, 2000; revised Oct. 2, 2000; accepted Oct. 6, 2000.
This work was supported by a Pew Biomedical Research Scholar Award, an
Alfred P. Sloan Neuroscience Scholar Award, and a National Institutes
of Health RO1 grant. H.T. was supported by the Human Frontier Science
Program. We thank Drs. C. E. Jahr and G. D. Pollack for valuable
discussions and Drs. J. G. G. Borst, E. McCleskey, and L. Trussell for helpful comments on this manuscript.
Correspondence should be addressed to Henrique von Gersdorff, The
Vollum Institute, Oregon Health Sciences University, 3181 SW Sam
Jackson Park Road, Portland, OR 97201. E-mail: vongersd{at}ohsu.edu.
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M. J. Fedchyshyn and L.-Y. Wang
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R. M. Leao, C. Kushmerick, R. Pinaud, R. Renden, G.-L. Li, H. Taschenberger, G. Spirou, S. R. Levinson, and H. von Gersdorff
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G. B. Awatramani, R. Turecek, and L. O. Trussell
Staggered Development of GABAergic and Glycinergic Transmission in the MNTB
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M. Koike-Tani, N. Saitoh, and T. Takahashi
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P. Wasling, E. Hanse, and B. Gustafsson
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T. N. Allana and J.-W. Lin
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T. Watano, J. A. Calvert, C. Vial, I. D. Forsythe, and R. J. Evans
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C. Kushmerick, G. D. Price, H. Taschenberger, N. Puente, R. Renden, J. I. Wadiche, R. M. Duvoisin, P. Grandes, and H. von Gersdorff
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G. B. Awatramani, R. Turecek, and L. O. Trussell
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M. Kimura, N. Saitoh, and T. Takahashi
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F. Mori-Kawakami, K. Kobayashi, and T. Takahashi
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T. Ishikawa, Y. Nakamura, N. Saitoh, W.-B. Li, S. Iwasaki, and T. Takahashi
Distinct Roles of Kv1 and Kv3 Potassium Channels at the Calyx of Held Presynaptic Terminal
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A. Y. C. Wong, B. P. Graham, B. Billups, and I. D. Forsythe
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T. Yamashita, T. Ishikawa, and T. Takahashi
Developmental Increase in Vesicular Glutamate Content Does Not Cause Saturation of AMPA Receptors at the Calyx of Held Synapse
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C. J Meinrenken, J G. G Borst, and B. Sakmann
Local routes revisited: the space and time dependence of the Ca2+ signal for phasic transmitter release at the rat calyx of Held
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C. M. Macica, C. A. A. von Hehn, L.-Y. Wang, C.-S. Ho, S. Yokoyama, R. H. Joho, and L. K. Kaczmarek
Modulation of the Kv3.1b Potassium Channel Isoform Adjusts the Fidelity of the Firing Pattern of Auditory Neurons
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P. D. Dodson, M. C. Barker, and I. D. Forsythe
Two Heteromeric Kv1 Potassium Channels Differentially Regulate Action Potential Firing
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August 15, 2002;
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Auditory Response Properties in the Superior Paraolivary Nucleus of the Gerbil
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R. M. Leao and H. Von Gersdorff
Noradrenaline Increases High-Frequency Firing at the Calyx of Held Synapse During Development by Inhibiting Glutamate Release
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T. Tsujimoto, A. Jeromin, N. Saitoh, J. C. Roder, and T. Takahashi
Neuronal Calcium Sensor 1 and Activity-Dependent Facilitation of P/Q-Type Calcium Currents at Presynaptic Nerve Terminals
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Maturation of Synaptic Transmission at End-Bulb Synapses of the Cochlear Nucleus
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A. C. Meyer, E. Neher, and R. Schneggenburger
Estimation of Quantal Size and Number of Functional Active Zones at the Calyx of Held Synapse by Nonstationary EPSC Variance Analysis
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S. Iwasaki and T. Takahashi
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S. J. Pyott and C. Rosenmund
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TOP
ABSTRACT
INTRODUCTION
