Role of Ca2+ in the Synchronization of Transmitter Release at Calyceal Synapses in the Auditory System of Rat

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Role of Ca²⁺ in the Synchronization of Transmitter Release at Calyceal Synapses in the Auditory System of Rat

Nao Chuhma and Harunori Ohmori

Department of Physiology, Faculty of Medicine, Kyoto University, Kyoto 606-8501, Japan

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Chuhma, Nao and Harunori Ohmori. Role of Ca²⁺ in the Synchronization of Transmitter Release at Calyceal Synapses in the Auditory System of Rat. J. Neurophysiol. 87: 222-228, 2002. The synchronization of transmitter release in the synapse of the medial nucleus of the trapezoid body (MNTB) is achieved duringearly postnatal development as a consequence of elimination ofdelayed asynchronous releases and appears to reflect changes inthe dynamics of Ca²⁺ entry and clearance. To examine the role of Ca²⁺ in regulating synchronization of transmitter release in the maturesynapse (after postnatal day 9, P9), we perturbed Ca²⁺ dynamics systematically. Replacement of external Ca²⁺ (2 mM) with Sr²⁺ induced delayed asynchronous release following the major EPSC.We tried to reproduce asynchronous releases without using Sr²⁺ and instead by manipulating the time course and the size of Ca²⁺ transient in the presynaptic terminal, under the assumption thatreplacement of external Na⁺ with Li⁺ or application of eosin-Y would prolong the lifetime of Ca²⁺ transient by reducing the rate of Ca²⁺ extrusion from the terminal. With application of Li⁺, Ca²⁺ transient in the terminal was prolonged, the EPSC decay timecourse was prolonged, and the EPSC amplitude increased. However,these EPSCs were not followed by delayed asynchronous release.When Ca²⁺ influx was reduced, either by partial Ca²⁺ channel blockade with a low concentration of Cd²⁺ or $omega$ -agatoxin IVA, a marked asynchronous release resulted. Thiswas further enhanced by the combined application of Li⁺ or eosin-Y. These results suggest that cooperative increasesof both Ca²⁺ influx and Ca²⁺ clearance capacities leading to a sharper Ca²⁺ spike in the presynaptic terminal underlie synchronized transmitterrelease in the presynaptic terminal of theMNTB.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The medial nucleus of the trapezoid body (MNTB) synapse mediates fast, high-fidelity transmission that is crucial for auditoryprocessing (Goldberg and Brown 1968; Guinan and Li 1990; Oertel1999). Synchronized release develops during early postnatal life.At postnatal days 4-5 (P4-5), when the calyx-like structure ofthe presynaptic terminal begins to form (Kandler and Friauf 1993),the excitatory postsynaptic current (EPSC) is followed by manyminiature EPSC (mEPSC)-like currents (Chuhma and Ohmori 1998).These mEPSC-like currents are a part of the evoked response, asthey do not arise spontaneously, appearing only following evokedEPSCs (Chuhma et al. 2001). They disappear after P9 (Chuhma andOhmori 1998). Synchronization of transmitter release progressesin parallel with maturation of Ca²⁺ extrusion and Ca²⁺ buffering capacities in the presynaptic terminal (Chuhma et al.2001), which are likely to reduce the lifetime of Ca²⁺ transients in the presynaptic terminal (Mironov et al. 1993;Roberts 1994; Reuter and Porzig 1995). Sequential expressionsof some Ca²⁺ binding proteins were observed in these postnatal days in thebrain stem auditory nuclei (Friauf 1993; Lohmann and Friauf 1996).

If the nature of Ca²⁺ extrusion and buffering capacities are essential for synchronized transmitter release, then manipulationsto prolong the lifetime of Ca²⁺ transients should desynchronize transmitter release in the MNTBsynapse (after P9). In agreement with this hypothesis, Sr²⁺ is known to produce delayed asynchronous release (Goda and Stevens1994) and is reported to have a long lifetime in the presynapticterminal (Xu-Friedman and Regehr 2000). In this report, we testedthis hypothesis with inhibitors of Ca²⁺ clearance to modulate Ca²⁺ lifetime in theterminal.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Preparations of brain slices

Most experiments were performed in brain-stem slices containing the MNTB prepared from P9-12 Wister rats as described previously(Chuhma and Ohmori 1998). A part of the records shown in Fig.1 was obtained from P4-5 rats. Briefly, rats were deeply anesthetizedwith ether and decapitated. Brain-stem slices were cut 200-300µM thick using a vibratome (DTK-2000; Dosaka, Kyoto, Japan). Afterincubation at 36°C for 1 h in high-glucose artificial cerebrospinalfluid (high-glucose ACSF; concentrations in mM as follows unlessotherwise noted: 75 NaCl, 2.5 KCl, 26 NaHCO₃, 1.25 NaH₂PO₄, 0.7CaCl₂, 2 MgCl₂, and 100 glucose, pH 7.4) saturated with 95% O₂-5%CO₂, slices were maintained in the same high-glucose ACSF at roomtemperature until they were used. Experiments were performed atroom temperature (20-25°C).

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Fig. 1. Sr²⁺-generated delayed releases in the medial nucleus of the trapezoid body (MNTB) synapse. A: evoked excitatory postsynaptic current (EPSCs) (P11). Six traces are superimposed in each panel. Insets indicate 10-20 trace-averaged miniature EPSCs (mEPSCs). In this and subsequent figures, EPSCs and mEPSCs were recorded from neurons voltage-clamped at $-$ 70 mV. a: P11 EPSC in control. b: P11 EPSC after replacement of external Ca²⁺ with Sr²⁺ recorded from the same synapse as in a. c: immature P5 EPSC in control. B: event time histograms made from 30 consecutive traces (in a, b) or 50 consecutive traces (in c) of EPSC. Each histogram was made from the same EPSC traces as indicated in A. C: asynchronicity indexes of P11 EPSC in control (open bar), after replacement with Sr²⁺ (hatched bar) and immature P5 EPSC (filled bar).

Recordings of EPSCs

As described previously (Chuhma and Ohmori 1998), EPSCs were recorded from MNTB principal neurons superfused with ACSF (125NaCl, 2.5 KCl, 26 NaHCO₃, 1.25 NaH₂PO₄, 2 CaCl₂, 1 MgCl₂, and17 glucose, pH 7.4, saturated with 95% O₂-5% CO₂) and supplementedwith 20 µM strychnine (Sigma), 10 µM bicuculline (Sigma), and50 µM D-2-amino-5-phosphonovalerate (APV; Tocris). The pipettesolution was Cs⁺-based (136 Cs-glucuronate, 14 CsCl, 10 HEPES, 5 EGTA, pH 7.4)with the addition of 5 mM N-(2,6-dimethylphenylcarbamoylmethyl)triethylammonium bromide (QX-314; Alomone Labs, Jerusalem, Israel).In some experiments, CaCl₂ was replaced with SrCl₂ (2 mM) (Sr²⁺-ACSF).

Neurons were voltage clamped at $-$ 70 mV (Axopatch 200A; Axon Instruments). Corrections were made for the liquid junction potential(approximately $-$ 10 mV). Pipette resistances were approximately2-5 M $Omega$ . Series resistances were 9-20 M $Omega$ and compensated by 70-80%.Presynaptic nerve fibers were electrically stimulated (0.5-8V,100-µs duration) every 5 s using bipolar tungstenelectrode.

Ca²⁺ overloading

Ca²⁺ clearance was reduced in the presynaptic terminal by several procedures: 1) replacement of external Na⁺ with Li⁺, 2) bath application of eosin Y (0.2 mM, Sigma), 3) La³⁺ (1 mM), 4) thapsigargin (10 µM, Sigma), 5) carbonyl cyanide m-chlorophenylhydrazone (CCCP, 2-10 µM, Sigma), and 6) tetraphenyl phosphonium(TPP, 100 µM, Sigma). When Na⁺ was replaced with Li⁺, Li⁺-ACSF was used (125 LiCl, 2.5 KCl, 26 NaHCO₃, 1.25 NaH₂PO₄, 2CaCl₂, 1 MgCl₂, 17 glucose pH 7.4). La³⁺ was added to HEPES-buffered external solution (138 NaCl, 2.5KCl, 10 HEPES, 2 CaCl₂, 1 MgCl₂, 17 glucose, pH 7.4, saturatedwith 100% O₂).

Partial block of Ca²⁺ channels

Cd²⁺ (3 µM) or $omega$ -Agatoxin IVA (50 nM, Peptide Institute, Osaka, Japan) was applied to block a fraction of presynaptic Ca²⁺ channels. Cd²⁺ reduced the size of EPSCs with a K_d of 1.77 µM and a cooperativityof 1.76 (Chuhma et al. 2001). These concentrations of Cd²⁺ or $omega$ -Agatoxin reduced the EPSC size to 20-30% of thecontrol.

Measurement of presynaptic [Ca²⁺]_i with fura-2 and Mg-fura2

The Ca²⁺ transient and basal Ca²⁺ level in the presynaptic terminal were monitored with a high-affinity Ca²⁺ indicator fura-2 (K_d 145 nM) or a low-affinity indicator Mg-fura-2(K_d 25 µM) loaded directly through the patch electrode. Pipettesolution was K⁺-based (120 K-gluconate, 20 KCl, 10 HEPES, pH 7.4) with 0.1 mMfura-2 pentapotassium salt (fura-2-5K, Molecular Probes), 5 Mg-ATP,5 creatine phosphate. When [Ca²⁺]_i was measured with Mg-fura-2, the same pipette solution wasused but with 0.4 mM Mg-fura-2-4K (Molecular Probes) in the placeof fura-2. Ca²⁺ transients measured with fura-2 were induced by a train of fiveaction potentials to improve the signal-to-noise ratio or by asingle action potential (see Fig. 3 and Chuhma et al. 2001), withdepolarizing current injection through the patch electrode byusing EPC-7 (List). In measurements with Mg-fura-2, Ca²⁺ transients were induced by a train of 20 action potentials becausefluorescence changes were small and <1% by a single action potential(see Helmchen et al. 1997). Membrane potential was maintainedat approximately $-$ 70 mV. Pipette resistances were 5-10 M $Omega$ . Becauseof the limitation of the current clamp speed of EPC-7 (Magestrettiet al. 1996), the time course of the presynaptic action potential,which was recorded during the fluorescence measurement (Fig. 3A),was slightly slower than those published (half-amplitude widthof 0.5 ms in Borst et al. 1995). A wavelength pair of 340 and380 nm alternately excited fura-2 or Mg-fura-2, and fluorescences(f340 and f380) were sampled by a photomultiplier (OSP-3, Olympus)through a 500-nm-long pass filter. The fluorescence ratio (R =f340/f380) of the presynaptic terminal area was calculated on-linewithout background subtraction. The time resolution was 100-200ms. The ratio was converted to [Ca²⁺]_i by the equation determined through in situ calibration doneon MNTB neurons as described in Neher (1989): for fura-2, [Ca²⁺]_i = 2.7(R $-$ 0.7)/(5.3 - R), and for Mg-fura-2, [Ca²⁺]_i = 12.4(R $-$ 0.47)/(0.71 $-$ R). The decay time constant ( $tau$ _decay)of Ca²⁺ transients was determined by fitting a single exponential functionto the data. Because a train of five action potentials for fura-2and 20 action potentials for Mg-fura-2 was used to induce theCa²⁺ transient, the decay time course was likely prolonged more thanthe case generated by a single action potential (Chuhma and Ohmori2001). However, the time constant of decay we observed at roomtemperature (1 s for fura-2 and 0.4 s for Mg-fura-2) was withinthe range reported by using fura-2 (0.1 mM; Helmchen et al. 1997)and the low-affinity Ca²⁺ indicator dyes (0.4 mM Mg-fura-2 or 0.2 mM Calcium Green-5N;Borst et al. 1995; Helmchen et al. 1997).

Data analysis

Data were stored and analyzed as described previously (Chuhma and Ohmori 1998). The occurrence time of mEPSC-like currentswas determined off-line by registering visually identified peaksand scored in a histogram (event time histogram). The frequencyof mEPSC-like currents was quantified as an asynchronicity index,obtained by dividing the total counts of mEPSC-like currents duringa 60-ms time window (from 20 to 80 ms in 100-ms records) by thenumber of traces (30-50 traces). Data are given as the mean ±SE (number of cells) unless otherwisenoted.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Sr²⁺ desynchronized transmitter release

In the mature (P9-P12) synapse, delayed mEPSC-like currents were rarely observed (Fig. 1Aa). We have scored the occurrencetime of EPSC or mEPSC-like currents from 10 ms before stimulationof the presynaptic fiber to 100 ms after (Fig. 1B). In the controlevent time histogram, a large peak corresponding to the main EPSCwas seen (Fig. 1Ba), and the asynchronicity index (defined inMETHODS) was 0.07 ± 0.03 (n = 3). In Sr²⁺-ACSF, many mEPSC-like currents followed the EPSC (Fig. 1Ab) andthe amplitude of EPSC was reduced to 24.8 ± 6.4% (n = 4) of thecontrol. The event time histogram showed many late counts reflectingmEPSC-like currents (Fig. 1Bb) and the asynchronicity index was1.03 ± 0.16 (n = 3, P < 0.05, paired t-test, Fig. 1C). In theimmature P4-5 synapse, similar delayed mEPSC-like currents wereobserved in the control ACSF (Fig. 1, Ac and Bc). The asynchronicityindex was 1.34 ± 0.21 (n = 11, Fig. 1C). The amplitude and thedecay time constant of the mEPSC-like currents were almost thesame for all conditions [P = 0.70 for amplitude; P = 0.14 fordecay time constant, analysis of variance (ANOVA)] as follows:P4-5 synapse (30.9 ± 1.8 pA, 1.48 ± 0.10 ms, n = 3), P9-12 synapsein Sr²⁺-ACSF (29.4 ± 2.5 pA, 1.76 ± 0.02 ms, n = 3), or in 5 mM Ba²⁺-enriched ACSF (26.6 ± 0.5 pA, 1.70 ± 0.11 ms, n =3).

Effects of reduced Ca²⁺ clearance capacities

During the early stage of postnatal development (P4-9), the delayed mEPSC-like currents disappeared and presynaptic Ca²⁺ currents increased twofold (Chuhma and Ohmori 1998); at the sametime, both presynaptic Ca²⁺ buffering and Ca²⁺ clearance capacities were increased (Chuhma et al. 2001). Delayedasynchronous transmitter release observed in Sr²⁺-ACSF seems to have a close relation to the prolonged lifetimeof Sr²⁺ in the presynaptic terminal (Xu-Friedman and Regehr 2000). Theseobservations about Ca²⁺ dynamics and Sr²⁺ effects suggest a close relationship between delayed asynchronousrelease in immature MNTB synapses and the slow decay time courseof Ca²⁺ transients in the presynaptic terminal. To test this hypothesis,we first prolonged the lifetime of the Ca²⁺ transient in the synapse after P9. Of the two major factors thatdetermine the lifetime of the Ca²⁺ transient, it is practically impossible to reduce the Ca²⁺ binding capacity of soluble Ca²⁺ binding proteins in the presynaptic terminal, so we chose toreduce Ca²⁺clearance.

1) Replacement of Na⁺ in ACSF with Li⁺ is expected to reduce Ca²⁺ extrusion through the Na⁺-Ca²⁺ exchanger. When [Na⁺]_o was reduced by replacement with Li⁺, the amplitude of the evoked EPSC increased and the decay timecourse was slowed (Fig. 2A). The decay time course of the matureEPSC was well-fit by a combination of three exponential functionsin the control and in Li⁺-ACSF (Fig. 2B). We are not certain what caused each of the threecomponents of decay (see Otis et al. 1996 for one possibilityfor delayed clearance of transmitter). However, in Li⁺-ACSF, the relative amplitude of the third (slowest) componentwas reduced (2.1 ± 1.3%) from that in the control (5.0 ± 1.3%,n = 5), and the decay was nearly fit by a combination of onlytwo exponentials (Fig. 2B, c and d). Both the first (fastest)and the second (intermediate) decay time constants were increasedin Li⁺-ACSF, but the relative amplitude of each component was not significantlydifferent from the control (Table 1). These effects of Li⁺ could be reversed by washing, implying that these effects werenot due to deterioration of the synapse. The amplitude and decaytime constant of mEPSC recorded in Li⁺-ACSF were the same as those in the control (Fig. 2A, insets;27.3 ± 2.8 pA, 1.5 ± 0.1 ms in control and 24.9 ± 3.0 pA, 1.6± 0.2 ms in Li⁺-ACSF, n = 4, P = 0.57 and 0.88, at $-$ 70 mV). However, delayedmEPSC-like currents were not observed in Li⁺-ACSF (Fig. 2A).

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Fig. 2. Effects of external Li⁺ in MNTB synapse. A: evoked EPSCs (P11) recorded in the control (a) and after replacement of external Na⁺ with Li⁺ (b). Five traces are superimposed. Broken lines indicate baselines. Ten to twenty trace-averaged mEPSCs are indicated in insets. B: two-exponential fits (a, c) and three-exponential fits (b, d) of the decay phase of the ensemble-averaged EPSC in control (a, b) and in Li⁺-ACSF (c, d). Open circles indicate the averaged EPSC of 10 traces from the same records shown in A. Smooth lines are the fitted curves. The time constants of the fitted exponentials are indicated in each panel.

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Table 1. Effects of inhibitors of Ca^2⁺ extrusion on excitatory postsynaptic current (EPSC)

The lifetime of the Ca²⁺ transient in the presynaptic terminal was prolonged in Li⁺-ACSF. The Ca²⁺ transient measured by fura-2 rose quickly and decayed exponentially(Fig. 3B). The decay time constant was 1.2 ± 0.1 s (n = 5) inthe control, 4.2 ± 1.0 s (n = 5) in Li⁺-ACSF, and 1.8 ± 0.2 s (n = 3) after washing. When an action potentialwas generated every 5 s in the control solution, a small Ca²⁺ transient was generated (Fig. 3C) and basal [Ca²⁺]_i was increased slightly (approximately 20 nM). After replacementof Na⁺ with Li⁺, the basal Ca²⁺ level was increased by 0.1 µM (0.14 ± 0.05 µM, n = 4, Fig. 3C)and remained about 50 nM higher than the control. During exposureto Li⁺-ACSF, the half-amplitude width of the presynaptic action potentialwas not affected significantly (1.3 ± 0.1 ms in control, 1.4 ±0.1 ms in Li⁺, n = 3 cells, Fig. 3A). When Ca²⁺ transients were measured with a low-affinity Ca²⁺ indicator Mg-fura-2, the decay time constant was faster thanit was when measured by fura-2; however, the same threefold increasein the time constant was seen in Li⁺-ACSF (0.40 ± 0.02 s in control, 1.25 ± 0.20 s in Li⁺, n = 3 cells).

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Fig. 3. Effects of replacement of external Na⁺ by Li⁺ on [Ca²⁺]_i in the presynaptic terminal. A: trains of presynaptic action potentials to induce Ca²⁺ transients in B. Resting potential was maintained near $-$ 66 mV. B: Ca²⁺ transients under control condition (left), after replacement with Li⁺ (middle), and after washing (right) in P11 presynaptic terminals. Decay time constant of each trace is indicated. C: time course of change of presynaptic basal [Ca²⁺]_i after solution change to Li⁺-ACSF. Noisy signals starting at 40 s are due to Ca²⁺ transients induced by individual action potentials.

2) We then examined the effects of eosin Y, an inhibitor of the plasma membrane Ca²⁺-ATPase (Gatto and Milanick 1993). Application of eosin Y (0.2mM) to the external solution increased the peak amplitude andthe first and the second decay time constants of the EPSC (Table1). The amplitude (27.1 ± 1.9 pA in control vs. 24.6 ± 1.9 pAin eosin Y, P = 0.46) and decay time constant (1.9 ± 0.3 ms incontrol vs. 1.9 ± 0.3 ms in eosin Y, P = 0.37) of the mEPSC werenot significantly affected (n = 4). Delayed mEPSC-like currentswere not observed. We could not visualize the expected increasein presynaptic [Ca²⁺]_i after eosin Y because of its fluorescence. La³⁺ is reported to inhibit plasma membrane Ca²⁺-ATPase (Carafoli 1991; Zenisek and Matthews 2000). However, 1mM La³⁺ progressively reduced EPSC amplitude until it blocked transmissioncompletely (n = 3 cells). When the first and second decay timeconstants and the asynchronicity index were compared between controland during the course of block, when the EPSC was reduced to 20%,there was no change in the EPSC parameters [1st decay time constant0.93 ± 0.16 ms in control, 0.77 ± 0.17 ms at 20% amplitude (P< 0.01); 2nd decay time constant 3.67 ± 0.56 ms in control, 3.99± 1.18 ms at 20% amplitude (P = 0.75); asynchronicity index 0.06± 0.03 in control, 0.25 ± 0.12 at 20% amplitude (P = 0.18); n= 3 cells]. Lower concentrations of La³⁺ (100 and 10 µM) had no effect on EPSC (n = 3cells).

3) We then tested thapsigargin (10 µM, n = 4), an inhibitor of Ca²⁺ uptake by the endoplasmic reticulum (ER; Jackson et al. 1988).There was no effect on the EPSC even after 30 min incubation (Table1).

4) We examined two agents affecting mitochondrial Ca²⁺ dynamics: CCCP (Gunter and Pfeiffer 1990; Herrington et al. 1996) andTPP (Tang and Zucker 1997). Both 2-10 µM CCCP and 100 µM TPP progressivelyreduced the EPSC amplitude until it was blocked completely. Thetime course of the effect of 100 µM TPP on the EPSC is shown inFig. 4. When the peak amplitude of the EPSC was reduced to 20%of that of the control, there was no difference in the first andsecond decay time constants or the asynchronicity index [1st decaytime constant 1.34 ± 0.40 ms in control, 1.24 ± 0.36 ms at 20%amplitude (P = 0.74); 2nd decay time constant 4.34 ± 0.83 ms incontrol, 4.52 ± 1.30 ms at 20% amplitude (P = 0.81); asynchronicityindex 0.03 ± 0.02 in control, 0.05 ± 0.03 at 20% amplitude (P= 0.48); n = 3 cells]. However, in two cells, many spontaneousmEPSC-like currents appeared after complete block of the evokedEPSC (Fig. 4Ad). This suggests that TPP increased the basal Ca²⁺ level. TPP effects on evoked EPSC were probably masked by itsinhibitory effects on ATP production (Nguyen et al. 1997). CCCP(2-10 µM) gradually blocked synaptic transmission similarly. Thedecay time constants and the asynchronicity index were not differentfrom the control when EPSC amplitude was reduced to 20% [1st decaytime constant 1.43 ± 0.18 ms in control, 2.25 ± 0.89 ms at 20%amplitude (P = 0.42); 2nd decay time constant 5.01 ± 1.11 ms incontrol, 5.94 ± 2.21 ms at 20% amplitude (P = 0.78); asynchronicityindex 0.03 ± 0.02 in control, 0.01 ± 0.01 at 20% amplitude (P= 0.42); n = 5 cells].

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Fig. 4. Effects of tetraphenyl phosphonium (TPP) on synaptic transmission. A: sample traces of EPSC (P12) at the points indicated in B. Five traces are superimposed in each panel. a: control. b, c, d: after application of 100 µM TPP. The arrow in d indicates stimulus artifact. B: time course of effects of TPP on the peak amplitude of EPSC. The hatched bar indicates the period TPP was applied.

Li⁺ reduced presynaptic Ca²⁺ influx and generated delayed mEPSC-like currents

MEPSC-like currents were not observed in the late phase of EPSCs even though the lifetime of Ca²⁺ transient was prolonged (Fig. 2A). Since Ca²⁺ currents were smaller in immature P5-6 terminals than in thesynapse after P10 (Chuhma and Ohmori 1998), we examined the combinedeffects of reduced Ca²⁺ influx and prolonging the Ca²⁺transient.

After reducing Ca²⁺ influx with $omega$ -Agatoxin IVA (50 nM), mEPSC-like currents started to appear following the EPSC, but the asynchronicityindex was still small (0.23 ± 0.09, n = 5), as previously reported(Chuhma et al. 2001 and Fig. 5Ab). When external Na⁺ was replaced with Li⁺ in the presence of 50 nM $omega$ -Agatoxin, the frequency of mEPSC-likecurrents was further increased, and many late counts emerged inthe event time histogram (Fig. 5Ac). The asynchronicity indexwas 1.22 ± 0.31 (n = 5, Fig. 5Ba) and was significantly differentfrom the control (P < 0.05). This level of the asynchronicityindex was close to that of the immature synapse (1.34 ± 0.21,n = 11). The induction of delayed mEPSC-like currents by a combinationof reduced Ca²⁺ influx and replacement of ACSF with Li⁺-ACSF did not depend on the method of reducing Ca²⁺ influx (Fig. 5B). Cd²⁺ (3 µM) induced delayed mEPSC-like currents (Fig. 5Bb), and thefrequency markedly increased after addition of Li⁺ (1.22 ± 0.31, n = 5, P < 0.01). When [Ca²⁺]_o was reduced from 2 to 0.7 mM, the asynchronicity index wasnot increased. However, in Li⁺-ACSF with reduced [Ca²⁺]_o, the asynchronicity index was markedly increased (0.79 ± 0.18,n = 3, P = 0.085; Fig. 5Bc). The delayed mEPSC-like currents disappearedafter returning to control solution.

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Fig. 5. Combination of reduced Ca²⁺ extrusion and reduced Ca²⁺ influx generated asynchronous release. A: effects of replacement of Na⁺ with Li⁺ after partial block of Ca²⁺ channels with $omega$ -Agatoxin 50 nM (P9). Sample traces are shown; control (a), after application of $omega$ -Agatoxin (b), and after replacement of external Na⁺ with Li⁺ in the presence of $omega$ -Agatoxin (c). All traces were obtained from a single neuron sequentially. Six traces are superimposed. Insets indicate the event time histograms made from 30 consecutively recorded traces. B: asynchronicity indexes after combined reduction of Ca²⁺ influx and Ca²⁺ extrusion. The indexes were calculated from 30 EPSC traces in P9-12 synapses. a-c: Ca²⁺ extrusion was reduced by replacement of Na⁺ with Li⁺. Ca²⁺ influx was reduced 3 ways: application of 50 nM $omega$ -Agatoxin (a, n = 5), of 3 µM Cd²⁺ (b, n = 4), and reduction of [Ca²⁺]_o to 0.7 mM (c, n = 3). d: Ca²⁺ influx was reduced by 50 nM $omega$ -Agatoxin, and Ca²⁺ extrusion was reduced by application of 0.2 mM eosin Y. Each panel shows the index in the control (open bar) in reduced Ca²⁺ influx (hatched bar) and in reduced Ca²⁺ extrusion combined with reduced Ca²⁺ influx (filled bar).

Instead of Li⁺ replacement, we asked whether adding eosin Y to reduce Ca²⁺ extrusion would affect the EPSC. We found that the combinationof eosin Y with $omega$ -Agatoxin increased mEPSC-like currents (theasynchronicity index was increased from 0.11 ± 0.02 in $omega$ -Agatoxinto 0.72 ± 0.17 in $omega$ -Agatoxin and eosin Y, n = 3, P < 0.05, pairedt-test, Fig. 4Bd).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Synchronization of transmitter release at the MNTB synapse depends on a rapid and robust Ca²⁺ influx, which is quickly removed by active extrusion. Solelyreduced Ca²⁺ influx, when Ca²⁺ channels were partially blocked, produced only a slight increaseof asynchronous delayed release (Fig. 5B). Similarly, reducedCa²⁺ extrusion alone prolonged the decay phase of EPSC, but asynchronousdelayed releases were not observed (Figs. 2 and 3). This indicatesthat cooperative increase of both Ca²⁺ influx and Ca²⁺ clearance capacities in the presynaptic terminal are requiredto make a sharper Ca²⁺ spike for synchronized transmitter release at the MNTB synapse.Sharpening of presynaptic action potentials during developmentin MNTB is compatible with this idea (Taschenberger and von Gersdorff2000).

Ca²⁺ clearance mechanisms in the presynaptic terminal

Presynaptic [Ca²⁺]_i is reduced by uptake by the ER and mitochondria, or extrusion by the Na⁺-Ca²⁺ exchanger or the plasma membrane Ca²⁺-ATPase (Rosenberger and Triggle 1978). In the MNTB synapse, replacementof external Na⁺ with Li⁺ prolonged the lifetime of the Ca²⁺ transient and increased EPSC amplitude and decay time constants(Figs. 2 and 3). Eosin Y, an inhibitor of the plasma membraneCa²⁺-ATPase (Gatto and Milanick 1993), had similar effects. AlthoughLa³⁺, another inhibitor of plasma membrane Ca²⁺-ATPase (Carafoli 1991; Zenisek and Matthews 2000), blocked synaptictransmission completely, this is probably due to the effect ofCa²⁺ channel block by La³⁺ (Hagiwara and Takahashi 1967). Thapsigargin, an inhibitor ofCa²⁺ uptake to ER (Jackson et al. 1988), had little effect on theCa²⁺ transient and EPSCs (Table 1). TPP and CCCP, both inhibitorsof Ca²⁺ uptake by mitochondria (Gunter and Pfeiffer 1990; Herringtonet al. 1996; Tang and Zucker 1997), blocked EPSCs (Fig. 4). Thisis probably a consequence of the inhibition of ATP productionby these agents (Parsons et al. 1995; Rothman 1994). From theseresults, it is suggested that Ca²⁺ extrusion to the outside of the terminal may be more importantthan Ca²⁺ uptake and storage within organelles. A similar conclusion wasalso reached for hippocampal presynaptic boutons (Reuter and Porzig1995) and for retinal bipolar cells (Kobayashi and Tachibana 1995),and was suggested for the presynaptic terminal of the MNTB synapse(Helmchen et al. 1997).

Our results on TPP and CCCP are different from observations by others. In the crayfish neuromuscular junction, Tang and Zucker(1997) reported that inhibition of mitochondrial Ca²⁺ uptake with either TPP or CCCP enhanced the elevation of [Ca²⁺]_i induced by tetanus and increased the amplitude of excitatoryjunctional potential within 10 min after application. Similarresults were observed in the terminal of the ribbon synapse ofthe bipolar cell in the goldfish retina (Zenisek and Matthews2000); furthermore, these authors reported that the contributionof Na⁺-Ca²⁺ exchanger to the terminal Ca²⁺ clearance was negligible. In our experiments with MNTB presynapticterminals, these inhibitors blocked synaptic transmission (Fig.4). We did not see any increase in the amplitude nor prolongationof the EPSC preceding the block. However, in some experimentsof TPP, the frequency of occurrence of mEPSC-like currents wasincreased after the block of evoked synaptic responses (Fig. 4Ad).This suggests mitochondrial Ca²⁺ uptake may still have some contribution to keep the basal Ca²⁺ level low in theterminal.

Effects of Li⁺

Li⁺ is a popular substitute of Na⁺ to reduce Ca²⁺ extrusion through the Na⁺-Ca²⁺ exchanger while maintaining the excitability of nerve fibers.When external Na⁺ was replaced with Li⁺ without reducing Ca²⁺ influx, the first and the second decay time constants of theEPSC were prolonged (Fig. 2B). These prolongations might be expectedfrom the increased asynchronous release; however, mEPSC-like currentswere not seen. This is probably because individual mEPSC-likecurrents were buried in the large number of delayed release events,so we could not detect them. There is also the possibility thatLi⁺ might have affected the desensitization of postsynaptic AMPAreceptors (Karakanias and Papke 1999). Cyclothiazide (CTZ) hada Li⁺-like effect on the EPSC. Both Li⁺ (Fig. 2A) and 100 µM CTZ (Barnes-Davies and Forsythe 1995) increasedthe evoked EPSC amplitude and prolonged the decay time course.However, it is unlikely that the effects on desensitization werethe major Li⁺ effects in this synapse, because Li⁺ did not affect the amplitude nor the decay time course of themEPSC (Fig. 2A, insets).

Li⁺ has other activities, such as reducing PI turnover (Berridge and Irvine 1989) and inhibition of the glutamate transporter(Dixon and Hokin 1998). Both suppression of Ca²⁺ extrusion through the Na⁺-Ca²⁺ exchanger and suspension of PI turnover should increase intracellularCa²⁺ concentrations. Inhibition of the glutamate transporter withLi⁺ was, if anything, minor, because application of 200 µM D,L-threo- $beta$ -hydroxyasparticacid (THA), a glutamate transporter inhibitor, did not affectsynaptic transmission during a 1 h application (unpublished observation).There is the further possibility that suspension of PI turnovermight affect transmitter release via synaptotagmin (Mikoshibaet al. 1999), which we cannot exclude as a possibility. However,we believe that the asynchronous release induced by Li⁺-ACSF with reduced presynaptic Ca²⁺ influx is a consequence of the prolonged lifetime of the Ca²⁺ transient, because eosin Y, the other inhibitor of Ca²⁺ extrusion, also induced robust asynchronous release under similarconditions (Fig. 4Bd). In summary, both the rapid rise of theCa²⁺ transient and the subsequent clearance of Ca²⁺ appear to underlie synchronous transmitter release at the MNTBsynapse.

	ACKNOWLEDGMENTS

We thank Drs. Lou Byerly, Stephen Rayport, and Professor Y. Kang for reading this manuscript and making helpful comments.We further thank Professor Y. Kang for technical assistance andM. Fukao for excellentmachining.

This work was supported by Grants-in-Aid from the Ministry of Education Japan to N. Chuhma (PD8936) and H. Ohmori(12053233).

Present address of N. Chuhma: Dept. of Psychiatry, Anatomy and Cell Biology, Columbia University, New York, NY10032.

	FOOTNOTES

Address for reprint requests: H. Ohmori (E-mail: ohmori{at}nbiol.med.kyoto-u.ac.jp).

Received 22 March 2001; accepted in final form 3 October 2001.

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