Protein Kinase C Increases the Apparent Affinity of the Release Machinery to Ca2+ by Enhancing the Release Machinery Downstream of the Ca2+ Sensor

Monoclonal Antibodies for Neuroscience Research

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (37)

Citing Articles via Google Scholar

Google Scholar

Articles by Wu, X.-S.

Articles by Wu, L.-G.

Search for Related Content

PubMed

PubMed Citation

Articles by Wu, X.-S.

Articles by Wu, L.-G.

Previous Article  |  Next Article

The Journal of Neuroscience, October 15, 2001, 21(20):7928-7936

Protein Kinase C Increases the Apparent Affinity of the Release Machinery to Ca²⁺ by Enhancing the Release Machinery Downstream of the Ca²⁺ Sensor
Xin-Sheng Wu and Ling-Gang Wu
Departments of Anesthesiology and Anatomy and Neurobiology, Washington University School of Medicine, St. Louis, Missouri 63110

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Modulation of the release probability of releasable vesicles in response to Ca²⁺ influx (Prob_Ca) is involved in mediating several forms of synapticplasticity, including short-term depression, short-term augmentation,and potentiation induced by protein kinases. Given such an importantrole, however, the mechanism underlying modulation of the Prob_Cais unclear. We addressed this question by investigating how theactivation of protein kinase C modulates the Prob_Ca at a calyx-typenerve terminal in rat brainstem. Various lengths of step depolarizationwere applied to the nerve terminal to evoke different amountsof Ca²⁺ currents and capacitance jumps, the latter of which reflect vesiclerelease. The relationship between the capacitance jump and theCa²⁺ current integral was sigmoidal and was fit well with a Hill function.The sigmoidal relationship was shifted significantly to the leftduring the application of the PKC activator 12-myristate 13-acetate(PMA), suggesting that PMA increases the apparent affinity ofthe release machinery to Ca²⁺. This effect was blocked in large part by the application ofthe PKC inhibitor bisindolylmaleimide, suggesting that the effectis mediated mainly by the activation of PKC. We also found thatPMA increased the rate of miniature EPSCs evoked by the applicationof hypertonic sucrose solution, which triggers release downstreamof the Ca²⁺ influx. Taken together, our results suggest that PKC enhancesthe apparent affinity of the release machinery to Ca²⁺ by a mechanism downstream of the binding between Ca²⁺ and its sensor. These results have provided the first exampleof the mechanisms underlying modulation of the Prob_Ca.

Key words: protein kinase C; calyx of Held; release probability; capacitance measurement; releasable pool; vesicle mobilization

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of protein kinase C (PKC) enhances synaptic transmission at a variety of synapses (Malenka et al., 1986; Shapiraet al., 1987; Minota et al., 1991; Bachoo et al., 1992; Capognaet al., 1995; Redman et al., 1997; Stevens and Sullivan, 1998;Hori et al., 1999; Yawo, 1999; Honda et al., 2000; Oleskevichand Walmsley, 2000) and may underlie certain forms of synapticplasticity (Byrne and Kandel, 1996; Son and Carpenter, 1996).Evidence suggests that the enhancement is mediated by an increaseof transmitter release (Malenka et al., 1987; Shapira et al.,1987; Capogna et al., 1995; Gillis et al., 1996; Redman et al.,1997). Although the increased transmitter release might be causedin part by modulation of voltage-gated ion channels leading toan increase of presynaptic Ca²⁺ influx during action potentials (Byrne and Kandel, 1996; Majewskiand Iannazzo, 1998; Honda et al., 2000), it is caused in largepart by mechanisms downstream of the Ca²⁺ influx at many synapses (Stevens and Sullivan, 1998; Hori etal., 1999; Yawo, 1999; Honda et al., 2000). After the Ca²⁺ influx, transmitter release depends on two factors, the sizeof a pool of vesicles immediately available for release (calledreleasable pool or readily releasable pool) and the averaged releaseprobability of vesicles in this pool in response to the Ca²⁺ influx (Prob_Ca). Which of these two factors is upregulated byPKC? By measurements of the membrane capacitance in chromaffincells, it was found that PKC enhances vesicle exocytosis by increasingthe releasable pool size (Gillis et al., 1996). A similar resultwas observed at cultured hippocampal synapses, in which the releasablepool size is defined as release evoked by 4-5 sec of hypertonicsucrose application (Stevens and Sullivan, 1998). In contrast,by an examination of EPSCs evoked by trains of electrical stimulationat calyx-type synapses, it was suggested that PKC may enhancetransmitter release by increasing the Prob_Ca (Yawo, 1999; Oleskevichand Walmsley, 2000). In these studies, however, the conclusionin large part was based on the result that the EPSC reached amaximum at a high extracellular Ca²⁺ solution and that PKC did not increase the EPSC further in thiscondition. Under high release conditions a maximal EPSC may bereached because postsynaptic receptors are saturated and desensitized(Sun and Wu, 2001). Thus it remains inconclusive whether PKC enhancestransmitter release by increasing the releasable pool size orthe Prob_Ca in these studies (Yawo, 1999; Oleskevich and Walmsley,2000).

In the present work we studied how PKC enhances synaptic transmission at a calyx-type synapse in the rat medial nucleus ofthe trapezoid body (MNTB). To study more directly how activationof PKC enhances transmitter release, we measured transmitter releaseby monitoring the change in the membrane capacitance at the nerveterminal (Sun and Wu, 2001), which is proportional to the surfacearea of the membrane and thus proportional to the number of vesiclesreleased (Albillos et al., 1997; Von Gersdorff et al., 1998; Sunand Wu, 2001). This approach avoids the complication of saturationand desensitization of postsynaptic receptors. With this approachwe found that activation of PKC enhanced release not by increasingthe releasable pool size but by increasing the Prob_Ca.

Modulation of the Prob_Ca is often a pathway by which synaptic strength is regulated. For example, modulation of the Prob_Cais involved in mediating short-term synaptic depression (Wu andBorst, 1999; Burrone and Lagnado, 2000), short-term synaptic augmentation(Stevens and Wesseling, 1999), and enhancement of transmitterrelease that is induced by the activation of protein kinase A(Trudeau et al., 1996). Although modulation of the Prob_Ca playsan important role in regulating synaptic strength, its underlyingmechanisms remain unclear. The present work was aimed at investigatingthe mechanisms underlying modulation of the Prob_Ca. Three potentialmechanisms may modulate the Prob_Ca: (1) modulation of the affinityof the Ca²⁺ sensor to Ca²⁺, (2) modulation of the number of Ca²⁺ ions required to bind the Ca²⁺ sensor and trigger release, and (3) modulation of any step atthe release machinery downstream of the Ca²⁺ sensor. By examining the relationship between the capacitancejump and the Ca²⁺ influx, we found that PKC increased the apparent affinity ofthe release machinery to Ca²⁺. By applying hypertonic sucrose solution to trigger release independentlyof the binding between Ca²⁺ and its sensor (Rosenmund and Stevens, 1996), we found that PKCenhanced transmitter release by a mechanism downstream of thebinding between Ca²⁺ and its sensor. These results suggest that enhancement of therelease machinery downstream of the Ca²⁺ sensor is involved in increasing the apparent affinity of therelease machinery to Ca²⁺ and thus the Prob_Ca.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recordings of presynaptic Ca²⁺ currents and capacitance. Wistar rats (8-12 d old) were decapitated. Parasagittal slices 200µm thick were cut from the auditory brainstem with a vibratome.Recordings were made at room temperature in a solution that pharmacologicallyisolated Ca²⁺ currents (Borst et al., 1995). This solution contained (in mM)105 NaCl, 20 TEA-Cl, 2.5 KCl, 1 MgCl₂, 2 CaCl₂, 25 NaHCO₃, 1.25NaH₂PO₄, 25 dextrose, 0.4 ascorbic acid, 3 myo-inositol, 2 sodiumpyruvate, 0.001 tetrodotoxin (TTX), and 0.1 3,4-diaminopyridine,pH 7.4, when bubbled with 95% O₂/5% CO₂. The presynaptic pipette(3.5-5 M $Omega$ ) solution contained (in mM) 125 Cs-gluconate, 20 CsCl,4 Mg-ATP, 10 Na₂-phosphocreatine, 0.3 GTP, 10 HEPES, and 0.05BAPTA, pH-adjusted to 7.2 with CsOH. Presynaptic whole-cell recordingswere made with an EPC-9 amplifier (HEKA Electronics, Lambrecht,Germany). The series resistance (<15 M $Omega$ ) was compensated by 60%.Holding potential was $-$ 80 mV, and the potential was correctedfor a liquid junction potential of $-$ 11 mV between the extracellularand the pipette solutions (also applies to postsynaptic recordings).Currents were low-pass filtered at 5 kHz and digitized at 20 kHz(also applies to postsynaptic recordings) with a 16 bit analog-to-digitalconverter (Instrutech, Great Neck,NY).

The selection of calyces and capacitance recordings has been described in detail in our recent study (Sun and Wu, 2001). Briefly,calyces that had a basal capacitance <22 pF and showed approximatelya single exponential decay in passive relaxation current, as judgedby eye, were used. The capacitance was measured with the EPC-9amplifier together with the software lock-in amplifier (PULSE,HEKA Electronics). A sinusoidal stimulus was applied in additionto the DC holding potential ( $-$ 80 mV). The peak-to-peak voltageof the sine wave was <60 mV to avoid activation of the Ca²⁺ currents (Borst et al., 1995; Wu et al., 1998). The resultingcurrent was processed via the Lindau-Neher technique (Lindau andNeher, 1988; Gillis, 1995) to give estimates of the membrane capacitance,membrane conductance, and the series conductance. The sine wavefrequency was 1000 Hz. The reversal potential of the measuredDC current was assumed to be 0 mV (Gillis, 1995). During stepdepolarization the capacitance was not measured. The capacitancejump was measured as the difference between the averaged capacitancevalue in 30-60 msec after stimulation and the baseline value.The capacitance jump returned to the baseline in a few secondsto tens of seconds (Sun and Wu, 2001). Therefore, measurementsof capacitance jumps were not affected by the relatively slowendocytosis. The interval between two voltage commands was atleast 30 sec to avoid short-term synaptic plasticity induced bythe previous voltage command. All capacitance traces shown inthe figures were taken from single recordings and were low-passfiltered at 100Hz.

Recordings of EPSCs and mEPSCs. Wistar rats (8-12 d old) were decapitated. Transverse slices 200 µm thick were cut from theauditory brainstem with a vibratome. Because the axon that connectsthe calyx is approximately parallel to the surface of the transverseslice, there are calyces connected with a longer axon that canbe stimulated electrically with a bipolar electrode positionedat the midline of the trapezoid body. Thus to induce an EPSC electrically(see Fig. 6), we applied a brief electrical stimulus (5-20 V,0.1 msec) to induce an action potential in the axon and thus anEPSC at the postsynaptic neuron. [For the method of identifyingsuch postsynaptic neurons, see Borst et al. (1995) and Wu et al.(1999).] To induce trains of mEPSCs with hypertonic solution,we positioned glass pipettes (1.5-2.5 M $Omega$ ) containing 2 M sucroseplus the bath solution described below close (<5 µm) to the surfaceof postsynaptic cells. The sucrose solution was pressure injected(0.2-10 sec, 5 psi) onto the surface of the synapse with a pneumaticpicopump (PV830, World Precision Instruments, Sarasota, FL). Theresulting mEPSCs were analyzed by a program (Jaejin Software,Leonia, NJ) with a threshold amplitude for detection set at 10pA.

Whole-cell voltage-clamp recordings of EPSCs and mEPSCs at postsynaptic neurons were made at room temperature in a bath solutioncontaining (in mM) 125 NaCl, 2.5 KCl, 1 MgCl₂, 2 CaCl₂, 25 NaHCO₃,1.25 NaH₂PO₄, 25 dextrose, 0.4 ascorbic acid, 3 myo-inositol,2 sodium pyruvate, 0.05 D-APV (NMDA receptor blocker), 0.01 bicuculline(GABA_A receptor blocker), and 0.01 strychnine (glycine receptorblocker), pH 7.4, when bubbled with 95% O₂/5% CO₂. The postsynapticpipette (2-3 M $Omega$ ) solution contained (in mM) 125 K-gluconate, 20KCl, 4 Mg-ATP, 10 Na₂-phosphocreatine, 0.3 GTP, 10 HEPES, and0.5 EGTA, pH-adjusted to 7.2 with KOH. Whole-cell recordings weremade with an Axopatch 200B amplifier (Axon Instruments, FosterCity, CA). The holding potential was $-$ 80 mV. The series resistance(<12 M $Omega$ ) was compensated by 95% (lag, 10 µsec).

Reagents and statistical tests. Phorbol 12-myristate 13-acetate (PMA) was purchased from Sigma (St. Louis, MO) and bisindolylmaleimide(BIS) from Calbiochem (La Jolla, CA). PMA and BIS were dissolvedfirst in DMSO and then diluted. The final concentration of DMSOdid not exceed 0.1% and by itself had no effect on the capacitancejump and the EPSC. Data were expressed as means ± SE. The statisticaltest for calculation of p values was the Student's ttest.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Measurement of the releasable pool size

We have found recently that a voltage step command of 10 msec from $-$ 80 to +10 mV evoked a maximal release the same as a 30msec step to +10 mV in an extracellular solution containing 2mM Ca²⁺ [Sun and Wu (2001), their Fig. 4]. This result suggests thata pool of releasable vesicles can be depleted in 10 msec. To confirmthis suggestion further, we determined whether release evokedby a 10 msec step to +10 mV was increased further when the extracellularCa²⁺ concentration was increased. The calyx of Held was whole-cellvoltage clamped in a bath solution that pharmacologically isolatesCa²⁺ currents. A step depolarization of 2 or 10 msec from the holdingpotential of $-$ 80 to +10 mV was applied alternately to the calyxto trigger vesicle release. Vesicle release was measured as thecapacitance jump after the step depolarization. When the extracellularCa²⁺ concentration was increased from 2 to 4 mM, the peak Ca²⁺ current at the end of a 2 or 10 msec step depolarization increasedby 27 ± 4 and 33 ± 3% (n = 4) (Fig. 1), respectively. The capacitancejump evoked by the 2 msec step depolarization increased by 74± 4%, whereas the capacitance jump evoked by the 10 msec stepdepolarization was increased only by 8 ± 4% (n = 4; p = 0.06).This result further supports our hypothesis that a 10 msec stepdepolarization in normal (2 mM) extracellular Ca²⁺ is sufficient to deplete the releasable pool.

View larger version (10K):
[in this window]
[in a new window]
Figure 1. The capacitance jumps recorded in different extracellular Ca²⁺ concentrations. A, The Ca²⁺ current (top) and the capacitance jump (bottom) evoked by a 2 msec step from $-$ 80 to +10 mV in extracellular solutions containing 2 mM (solid trace) and 4 mM (dotted trace) Ca²⁺. Both the Ca²⁺ current and the capacitance jump were increased significantly in 4 mM Ca²⁺. B, The Ca²⁺ current (top) and the capacitance jump (bottom) evoked by a 10 msec step from $-$ 80 to +10 mV in extracellular solutions containing 2 mM (solid trace) and 4 mM (dotted trace) Ca²⁺. Only the Ca²⁺ current, but not the capacitance jump, was increased significantly in 4 mM Ca²⁺. Data in A and B were obtained from the same calyx.

When the duration of the step depolarization was increased from 10 to 100-200 msec, the capacitance jump was increased by>50% (our unpublished results), suggesting that part of the releasablepool can be replenished rapidly in 100-200 msec (see also Fig.4). This result argues against the possibility that the similarcapacitance jumps observed during the 10-30 msec depolarization(Sun and Wu, 2001) or during a 10 msec depolarization in 2 and4 mM extracellular Ca²⁺ (Fig. 1) are caused by adaptation of the Ca²⁺ sensor (Hsu et al., 1996) or by an unknown mechanism that isturned on to inhibit the release machinery during prolonged stimulation.We conclude that the releasable pool size can be estimated asthe capacitance jump evoked by a 10 msec stepdepolarization.

A PKC activator PMA increases the apparent affinity of the release machinery to Ca²⁺

Bath application of the PKC activator PMA (100 nM) for 10 min increased the capacitance jump evoked by the 2 msec step depolarizationby 82 ± 18% (n = 6) (Fig. 2A). This effect reached the steadystate in a <10 min application of the drug (data not shown) (butsee Hori et al., 1999) and was not accompanied by any significantchange in the amplitude or the integral of the Ca²⁺ current (p > 0.4, t test; n = 6) (see Figs. 2A,B, 4A,B). In contrast,100 nM PMA did not increase significantly the capacitance jumpevoked by a 10 msec step depolarization (2 ± 2%; n = 6; p = 0.25,t test) (Fig. 2B). Thus PMA enhanced the transmitter release evokedduring a 2 msec step depolarization not by increasing the releasablepool size but by increasing the fraction of the releasable poolbeing released, i.e., the release probability of releasable vesicles.Because PMA did not affect the presynaptic Ca²⁺ current, the enhancement must occur downstream of the Ca²⁺ influx. In other words, PMA increased the Prob_Ca.

View larger version (16K):
[in this window]
[in a new window]
Figure 2. PMA increases the capacitance jump by increasing the apparent affinity of the release machinery to Ca²⁺, but not the releasable pool size. A, B, Sample traces of Ca²⁺ currents (top) and capacitance jumps (bottom) induced by a 2 msec (A) and a 10 msec (B) step depolarization from $-$ 80 to +10 mV before (left, solid trace) and during the application of 100 nM PMA for 10 min (middle, dotted trace). They are superimposed on the right for comparison. C, The relationship between the capacitance jump ( $Delta$ Cm) and the charge of the Ca²⁺ current (ICa) obtained before (Ctrl, circles) and during the application of PMA (triangles) for at least 10 min (n = 12 synapses). Before the data were pooled from different synapses, the data were normalized to the value obtained during the 10 msec step depolarization to +10 mV in the control condition. Both the data in control and in the presence of PMA were fit with a Hill equation (see Eq. 1 in Results). The application of PMA did not change two parameters in the equation, the RPS and the n, but decreased the EC₅₀ from 0.30 (solid curve, Ctrl_fit) to 0.16 (dotted curve, PMA_fit).

The increased Prob_Ca may be caused by either an increased apparent affinity of the release machinery to Ca²⁺ or a decrease in the number Ca²⁺ ions required to bind the Ca²⁺ sensor that triggers release. To identify which of these twomechanisms increases the Prob_Ca, we applied various lengths ofstep depolarizations to various voltages (0-20 mV) to the calyxto induce different amounts of Ca²⁺ influx and thus different amounts of vesicle release. The resultingcapacitance jumps were plotted versus the Ca²⁺ current integral (integrated for 10 msec) in the control condition(Fig. 2C, circles) and during the application of 100 nM PMA forat least 10 min (Fig. 2C, triangles). Before the data were pooledfrom different synapses into Figure 2C, the data were normalizedto the capacitance jump and the Ca²⁺ current evoked by the 10 msec step depolarization in controlat the same synapse. Both the data in control and in the presenceof PMA were fit with the Hill function:

(1)

where $Delta$ Cm is the normalized capacitance jump, RPS is the normalized releasable pool size or the maximal capacitance jump,ICa_integral is the integral of the Ca²⁺ current normalized to that evoked by a 10 msec step depolarizationin control at the same synapse, EC₅₀ is a value of ICa_integralat which $Delta$ Cm is 50% of RPS, and n is the Hill coefficient. Incontrol the RPS, EC₅₀, and n were 1.03, 0.30, and 2.4, respectively.In the presence of PMA these parameters were 1.02, 0.16, and 2.6,respectively. Evidently, PMA decreased the EC₅₀ to approximatelyone-half of the control value without significantly affectingthe Hill coefficient, the latter of which is interpreted widelyas the number of Ca²⁺ ions required to bind the Ca²⁺ sensor to trigger release (Reid et al., 1998; Schneggenburgeret al., 1999). Thus these results suggest that PMA enhanced transmitterrelease by increasing the apparent affinity of the release machineryto Ca²⁺, but not by modifying the number of Ca²⁺ ions required to bind the Ca²⁺ sensor to triggerrelease.

A PKC inhibitor in large part blocks the effect of PMA on the capacitance jump

Phorbol esters may enhance synaptic transmission via two mechanisms, one by the activation of PKC and the other by the interactionwith the synaptic protein Munc13-1 (Betz et al., 1998; Hori etal., 1999). Previous works at calyx-type synapses, including theMNTB synapse, indicate that phorbol esters (PMA and phorbol 1,2-dibutrate),but not their inactive forms (4 $alpha$ -PMA and 4 $alpha$ -phorbol 1,2-dibutrate),enhance the EPSC (Hori et al., 1999; Yawo, 1999; Oleskevich andWalmsley, 2000). The enhancement is blocked mainly or completelyby PKC inhibitors, such as BIS, sphingosine, calphostin C, anda PKC inhibitor peptide (Hori et al., 1999; Yawo, 1999; Oleskevichand Walmsley, 2000). These results indicate that phorbol estersenhance synaptic transmission in large part by the activationof PKC at calyx-typesynapses.

To confirm that PMA enhances the capacitance jump in large part by the activation of PKC, we applied a specific inhibitorof PKC, BIS (Toullec et al., 1991). The application of 1 µM BISfor 10 min slightly increased the $Delta$ Cm evoked by a 2 msec step(to +10 mV) by 10 ± 4% (n = 6; p = 0.04) (Fig. 3). The reasonfor the slight increase of the $Delta$ Cm is unclear.

View larger version (9K):
[in this window]
[in a new window]
Figure 3. A PKC antagonist BIS blocks in large part the effect of PMA on the capacitance jump. A, Sample recordings of presynaptic Ca²⁺ currents (ICa, top) and capacitance changes (Cm, bottom) evoked by a 2 msec presynaptic step from $-$ 80 to +10 mV in the control (left), in the presence of BIS (1 µM) for 10 min (middle left), and in the presence of BIS (1 µM) plus PMA (100 nM) for 10 min (middle right). These traces are superimposed on the right for comparison. B, Percentage of increase in the capacitance jump ( $Delta$ Cm) evoked by a 2 msec step depolarization to +10 mV during the application of 1 µM BIS (n = 6), 1 µM BIS plus 100 nM PMA (n = 6), and 100 nM PMA (n = 6). The percentages refer to the changes in capacitance jumps during the application of the drug or drugs normalized to the value obtained before any drug application at the same synapse. Data are expressed as means ± SE.

In the presence of 1 µM BIS the application of PMA increased the $Delta$ Cm evoked by a 2 msec step to +10 mV by 27 ± 5% (n = 6;p = 0.02) (Fig. 3) of the value obtained before the BIS application.This increase was significantly less than that (82 ± 18%; p =0.02) (Fig. 3) measured in the absence of BIS, suggesting thatPMA increases the capacitance jump in large part by the activationof PKC. This result is consistent with a recent study at MNTBsynapses showing that phorbol esters enhance the EPSC mainly bythe activation of PKC and partly by interaction with Munc13-1(Hori et al., 1999).

PMA does not affect the rate of vesicle mobilization

Phorbol esters have been suggested to enhance the releasable pool size and the rate of vesicle mobilization from the reservepool to the releasable pool at cultured hippocampal synapses andchromaffin cells (Stevens and Sullivan, 1998). Our results indicatedthat PMA did not increase the releasable pool size at the MNTBsynapse (Fig. 2). In the following we examined whether PMA increasesthe rate of mobilization. A pair of 10 msec steps to +10 mV withintervals that varied from 0.05 to 70 sec were applied to theterminal, and the resulting capacitance jumps were recorded (Fig.4A). The first step depleted the releasable pool, and the secondstep depleted the vesicles that have been mobilized to the releasablepool during the interval between the two steps. Thus the ratiobetween the second and the first capacitance jump indicates thefraction of the releasable pool being replenished. Such ratioswere plotted as a function of the interval and were fit well withthe sum of two exponential functions. In the control the timeconstants were 0.11 and 7.14 sec, respectively, and the weightsof the fast and the slow components were 48 and 52%, respectively(Fig. 4B). These results were consistent with the rate of mobilizationestimated with measurements of the EPSC at the same synapse (Wuand Borst, 1999). After the application of 100 nM PMA for 10 min,the time constants were 0.10 and 6.67 sec, respectively, and theweights of the fast and the slow components were 46 and 54%, respectively(Fig. 4B). The results obtained in the presence and the absenceof PMA were similar (Fig. 4), indicating that PMA did not affectthe rate of vesicle mobilization.

View larger version (17K):
[in this window]
[in a new window]
Figure 4. PMA does not affect the rate of vesicle mobilization. A, B, Sample recordings of Ca²⁺ currents (top) and capacitance jumps (bottom) induced by a pair of 10 msec step depolarizations (from $-$ 80 to +10 mV) with an interval of 400 msec before (A, Ctrl) and during (B) the application of 100 nM PMA. The labels and scales in A apply to B. C, The ratio between the second and the first $Delta$ Cm as a function of the paired pulse interval obtained in control and in the presence of PMA (100 nM). Data were obtained from experiments similar to those shown in A and B from 11 synapses. In control, the data were fit with a double-exponential function with time constants of 0.11 and 7.14 sec, respectively (solid curve). PMA does not affect these time constants and the relative contribution of these two components (dotted curve). The top and bottom panels show the same data in different scales.

PMA enhances transmitter release evoked by application of hypertonic sucrose solution

We have shown that PMA enhances transmitter release by increasing the apparent affinity of the release machinery to Ca²⁺ (Fig. 2). The increased apparent affinity may be caused by anincrease in the affinity of the Ca²⁺ sensor to Ca²⁺ and/or by an enhancement of the release machinery at a step downstreamof the Ca²⁺ sensor. To explore whether the latter mechanism is involved inmediating PMA-induced enhancement of the release, we applied hypertonicsucrose solution to trigger release. Release evoked by hypertonicsucrose solution is not affected when the voltage-dependent Ca²⁺ channels are blocked or when the Ca²⁺ buffer BAPTA is dialyzed to the nerve terminal to block effectivelythe action potential-evoked release (Rosenmund and Stevens, 1996).These results suggest that hypertonic sucrose solution triggersrelease independently of the binding between Ca²⁺ and its sensor (Rosenmund and Stevens, 1996). If PMA increasesthe release evoked by hypertonic solution, it suggests that PMAacts at a site downstream of the binding between Ca²⁺ and its sensor. Thus we determined whether PMA increases therelease evoked by the application of hypertonic solution. Fortwo reasons we monitored the release by measurements of the EPSCinstead of the presynaptic capacitance jump. First, we appliedthe sucrose solution by puff application (see below), which generatedan artifact in the capacitance recording that contaminated thecapacitance signal (data not shown). Second, release evoked bypuff application of hypertonic solution lasts for a few seconds(see below) during which significant endocytosis may occur (Stevensand Williams, 2000; Sun and Wu, 2001), which may result in a significantunderestimate of exocytosis (Smith and Betz, 1996).

Postsynaptic MNTB cells on the surface (<10 µm from the top) of the slice were whole-cell voltage clamped at $-$ 80 mV. A glasspipette containing 2 M sucrose plus the bath solution was positionedclose (<5 µm) to the cell. A pressure was applied for 0.2-10 secto puff the sucrose solution (<1 µl) to the MNTB synapse. Sucha puff induced a train of miniature EPSCs (mEPSCs) (Fig. 5A).Consistent with the previous study (Rosenmund and Stevens, 1996),the frequency of mEPSCs was not affected by adding the nonspecificCa²⁺ channel blocker CdCl₂ (200 µM) into the bath solution (n = 6)(Fig. 5B). The application of the AMPA receptor blocker CNQX (10µM) completely blocked the sucrose-induced mEPSCs (n = 4) (Fig.5C).

View larger version (16K):
[in this window]
[in a new window]
Figure 5. Hypertonic sucrose application evokes mEPSCs. A, Shown are the mEPSCs induced by a 1 sec puff application of hypertonic sucrose solution (2 M sucrose plus the bath solution in the pipette). The puff application time is marked in C. B, The Ca²⁺ channel blocker CdCl₂ (200 µM) did not block sucrose-induced mEPSCs. C, The non-NMDA glutamate receptor blocker CNQX (10 µM) blocked sucrose-induced mEPSCs. Calibration applies to all panels. Data in A-C were obtained from the same synapse.

The final concentration of sucrose at the synapse is unknown, because it depends on many factors such as the distance betweenthe puff pipette tip and the synapse, the pipette tip diameter,the duration of application, and the geometry of the synapse.Thus the same concentration of sucrose in the pipette may inducequite different responses at different synapses. However, theresults were repeatable at the same synapse (Fig. 5A,B). The mEPSCscontinued to occur for ~2-3 sec after puff application (Figs.5A,B, 6A,B), which may reflect the gradual decrease of sucroseconcentration caused by diffusion of sucrose away from the synapse.

View larger version (17K):
[in this window]
[in a new window]
Figure 6. Release evoked by hypertonic sucrose solution and nerve stimulation share the same vesicle pool. A, A train of nerve stimulations (20 V, 0.1 msec at 100 Hz for 200 msec) was applied, followed at 300 msec after the train by a puff application of sucrose solution (2 M in the pipette) for 500 msec. The EPSC evoked by the train was truncated to see the mEPSCs clearly. Calibration also applies to B. B, The EPSC is evoked by a puff the same as in A but without a conditioning train of stimulation. C, Shown are the EPSCs evoked by two identical electrical trains (20 V, 0.1 msec at 100 Hz for 200 msec) applied to the nerve with an interval of 1 sec (left). The EPSCs evoked by the second train (right, top) were smaller than those evoked by the first train (right, bottom). The stimulation artifacts were blanked.

Hypertonic sucrose solution and nerve stimulation trigger release from the same releasable vesicle pool at cultured hippocampalsynapses (Rosenmund and Stevens, 1996). To confirm this resultat MNTB synapses, we positioned a bipolar electrode at the midlineof the trapezoid body for stimulating the presynaptic axon. Atrain of nerve stimulations (20 V, 0.1 msec at 100 Hz for 200msec) was applied to induce a train of EPSCs, followed at 300msec after the end of the train by a puff application of hypertonicsucrose solution (2 M plus the bath solution) for 500 msec (Fig.6A). The same puff also was applied without the conditioning train(Fig. 6B). In control, the total number of mEPSCs in 3 sec duringand after sucrose application was 206 ± 32 (n = 6). After thetrain of nerve stimulations the number was decreased to 129 ±25 (or 63 ± 10%; p < 0.001; n = 6) (Fig. 6A), and the mean amplitudedid not change significantly (p = 0.47; n = 6). Similar resultswere observed in the presence of cyclothiazide that inhibits thedesensitization of AMPA receptors (n = 2; data not shown). Consistently,when two identical electrical trains (20 V, 0.1 msec at 100 Hzfor 200 msec) were applied to the nerve with an interval of 1sec, the EPSCs evoked by the second train were depressed significantly(Fig. 5C). The sum of the amplitude of the EPSC evoked by eachstimulus during the second train was 68 ± 9% (n = 4; p < 0.001)of that during the first train, similar to the decrease in thenumber of mEPSCs evoked by sucrose application. In addition, whenthe hypertonic sucrose solution (2 M in the pipette) was appliedfor 10 sec, the EPSC evoked by a single electrical stimulationor a train of stimulation (100 Hz for 200 msec) immediately aftersucrose application was <25% of that evoked in control (n = 4;data not shown). Consistent with the previous study (Rosenmundand Stevens, 1996), these results suggest that vesicles releasedby hypertonic sucrose application and the electrical train sharea common vesicle pool (Fig. 6) and that release evoked by hypertonicsucrose application is independent of the activation of voltage-gatedCa²⁺ channels (Fig. 5).

A 300 msec puff application of 2 M sucrose solution induced a train of ~30-100 mEPSCs that occurred in ~2-3 sec (Fig. 7A).The application of 100 nM PMA for 10 min increased the numberof mEPSCs (counted in 3 sec during and after puff application)by 154 ± 36% (p < 0.01; n = 5) (Fig. 7A) without significantlyaffecting the amplitude of the mEPSC (p = 0.39; n = 5). This resultsuggests that PKC enhances release by a mechanism downstream ofthe binding between Ca²⁺ and its sensor.

View larger version (23K):
[in this window]
[in a new window]
Figure 7. PMA enhances the rate of mEPSCs evoked by hypertonic sucrose solution. A, The mEPSCs evoked by a puff application of hypertonic sucrose solution (2 M) for 300 msec in the control (top), in the presence of 100 nM PMA (middle), and in the presence of 10 µM CNQX (bottom). B, The mEPSC evoked by a puff application of hypertonic sucrose solution (2 M) for 3 sec in the control (top), in the presence of 100 nM PMA (middle), and in the presence of 10 µM CNQX (bottom). The initial rise of the current is an artifact of the puff application because it was not blocked by CNQX (bottom trace). All data in this figure were obtained from the same synapse.

The percentage of increase in the number of mEPSCs decreased as the duration of the puff was prolonged. For example, a puffapplication of sucrose solution (2 M) for 3 sec induced a trainof mEPSCs that persisted for ~3 sec after the puff (Fig. 7B).The total number of mEPSCs that occurred during and 3 sec afterpuff application was increased by only 31 ± 9% (n = 5) (Fig. 7B),which is significantly lower than that (154 ± 36%; n = 5) obtainedwith a 300 msec puff application (p < 0.01). Because the frequencyof mEPSCs was high (50-200 Hz) during long puff application, thenumber of mEPSCs may be underestimated because of simultaneousmultiple quantal release. To avoid this potential problem, wecompared the charge of the EPSC (integrated for 5-6 sec duringand after sucrose application) before and after PMA application.A similar percentage of increase (36 ± 10%; n = 5) in the chargeof the EPSC was observed, confirming that PKC-induced enhancementof release evoked by a long puff application is significantlysmaller than that evoked by a brief puff application. These resultsare consistent with our finding that PMA enhanced release evokedby smaller stimulation to a larger extent than that evoked bylarger stimulation, because PMA increased the apparent affinityof the release machinery to Ca²⁺, but not the releasable pool size (Fig. 2).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Modulation of the Prob_Ca versus modulation of the releasable pool size

By monitoring transmitter release with presynaptic membrane capacitance measurements at MNTB synapses, we provided directevidence that PMA enhanced transmitter release at MNTB synapses.We found that PMA increased the Prob_Ca without affecting the releasablepool size (Fig. 2) or the rate of vesicle mobilization (Fig. 4).This result is consistent with a previous study at the cholinergicsynapse in the chick ciliary ganglion (Yawo, 1999), but it isin conflict with another study at hippocampal cultured synapsesin which phorbol esters were suggested to increase the releasablepool size (Stevens and Sullivan, 1998). The reason for this apparentdiscrepancy is unclear. Because Hori et al. (1999) found thatphorbol esters may enhance transmitter release by the activationof PKC and by interaction with another synaptic protein Munc13-1at the MNTB synapse (Hori et al., 1999), differential distributionof PKC and Munc13-1 in different tissues has been postulated toaccount for the discrepancy (Hilfiker and Augustine, 1999). Combinedwith the result obtained by Hori et al. (1999), our result thatPMA increased the Prob_Ca but not the releasable pool size at thesame MNTB synapse argues against this hypothesis. This does notnecessarily rule out the possibility that the discrepancy is attributableto a difference in synapses. However, as discussed below, thedifference in the method used to define and estimate the releasablepool size might account for thediscrepancy.

At cultured hippocampal synapses the releasable pool size is defined as the pool of vesicles released by a 4-5 sec applicationof hypertonic sucrose solution, subtracted by the number of vesiclesthat replenish the pool during sucrose application (Stevens andSullivan, 1998). Because more than one-half of the releasablepool can be replenished in 4-5 sec (Dittman and Regehr, 1998;Stevens and Sullivan, 1998; Stevens and Wesseling, 1998; Wangand Kaczmarek, 1998; Wu and Borst, 1999), an accurate estimateof the releasable pool size relies on the estimate of replenishment.Vesicles that newly replenish the releasable pool may have a muchlower release probability that takes >10 sec to recover (Wu andBorst, 1999; Burrone and Lagnado, 2000). In addition, in normalconditions the release probability of releasable vesicles is likelyto be inhomogeneous with a fraction of vesicles at low releaseprobability (Sakaba and Neher, 2001). It is possible that hypertonicsucrose application, which is far less efficient in triggeringrelease than a direct depolarization at the nerve terminal, preferentiallyreleases vesicles with a higher release probability. Activationof PKC may convert reluctant vesicles, such as vesicles with alow release probability in normal conditions and vesicles thatjust replenish the releasable pool during a 4-5 sec sucrose application,into vesicles ready for release by hypertonic solution, resultingin an apparent increase in the releasable pool size. For the samereason PKC may convert reluctant vesicles that have replenishedthe releasable pool during a pair of hypertonic shocks used toestimate the rate of mobilization, resulting in an apparent increasein the rate of mobilization. Our results suggest an approach totest whether PKC enhances the Prob_Ca at small synapses where theProb_Ca is difficult to measure. This approach is to determinewhether PKC increases release evoked by different intensitiesof hypertonic sucrose application to different degrees, as weshow in Figure 7 for MNTBsynapses.

Modulation of the Prob_Ca occurs at a step downstream of the binding between Ca²⁺ and its sensor

We found that PMA shifted the sigmoidal relationship between the capacitance jump and the Ca²⁺ current integral to the left (Fig. 2). When these sigmoidal curveswere fit with the Hill function (see Eq. 1), the EC₅₀ was reducedby approximately one-half by PMA (Fig. 2). These results suggestthat PMA increases the Prob_Ca by increasing the apparent affinityof the release machinery to Ca²⁺. If we assume a linear relationship between the local Ca²⁺ concentration that triggers transmitter release and the Ca²⁺ current integral, PMA would increase the affinity of the releasemachinery to Ca²⁺ to approximately two times the control value. However, whetherthis relationship is linear is currently unclear, making it difficultto estimate quantitatively the change in the apparent affinityof the release machinery to Ca²⁺. An alternative hypothesis that might account for the enhancementof the Prob_Ca is a rearrangement of Ca²⁺ channels such that a larger fraction of them is located physicallycloser to active zones where release occurs. This possibilityis highly unlikely because PMA enhanced transmitter release thatwas induced by hypertonic solution (Fig. 7), which triggered releaseindependently of activation of Ca²⁺ channels (Fig. 5) and the binding between Ca²⁺ and its sensor (Rosenmund and Stevens, 1996). In addition, releaseevoked by hypertonic sucrose solution shares a common pool ofvesicles releasable by nerve stimulation or activation of Ca²⁺ channels (Fig. 6) (Rosenmund and Stevens, 1996). We concludethat PMA increased the apparent affinity of the release machineryto Ca²⁺ and thus the Prob_Ca at least partly by a mechanism downstreamof the binding between Ca²⁺ and its sensor. Our results do not allow us to rule out completelythe possibility that an increase in the affinity of the Ca²⁺ sensor also contributes to the increase in the Prob_Ca. To ourknowledge this is the first example showing that modulation ofthe release machinery downstream of the Ca²⁺ sensor is involved in mediating modulation of the Prob_Ca andthus the synaptic strength. Such a mechanism may not be limitedonly to the PKC signaling pathway. Modulation of the Prob_Ca maybe a common pathway by which synaptic strength is regulated duringsynaptic modulation by neurotransmitters and neuromodulators (Thompsonet al., 1993; Wu and Saggau, 1997), during short-term synapticdepression (Wu and Borst, 1999; Burrone and Lagnado, 2000) andaugmentation (Stevens and Wesseling, 1999), and during activationof second messenger pathways involving protein kinase A (Trudeauet al., 1996) and G-proteins (Blackmer et al., 2001). Modulationof the Prob_Ca in these conditions may be achieved by regulationof the release machinery downstream of the Ca²⁺sensor.

Molecules that may be involved in modulation of the Prob_Ca

We found that the PKC inhibitor BIS inhibited in large part the PMA-induced enhancement of the capacitance jump (Fig. 3).This is consistent with previous works indicating that phorbolesters enhance synaptic transmission in large part by activationof PKC at calyx-type synapses (Hori et al., 1999; Yawo, 1999;Oleskevich and Walmsley, 2000). It would be of great interestto identify the substrate of PKC that is involved in modulationof the Prob_Ca. SNAP-25 and Munc18/nSec1 are two synaptic proteinsphosphorylated by PKC (Fujita et al., 1996; Shimazaki et al.,1996). Phosphorylation of them reduces their interaction withsyntaxin, which might enhance exocytosis by modifying dissociationor formation of SNARE complexes (Fujita et al., 1996; Shimazakiet al., 1996). Thus these two molecules are potential candidatesthat may mediate PKC-induced increase of the Prob_Ca, althoughit should be noted that there are many other transmitter release-relatedproteins that can be phosphorylated by PKC (Majewski and Iannazzo,1998).

Our results show that BIS did not block PMA-induced enhancement of the capacitance jump completely (Fig. 3). This is consistentwith a recent study at the same MNTB synapse showing that theenhancement of the EPSC by phorbol esters is blocked partly byhigh concentrations of PKC inhibitors, including BIS, calphostinC, and a PKC inhibitor peptide (Hori et al., 1999). In the samestudy (Hori et al., 1999) the enhancement also is blocked partlyby presynaptic loading of a synthetic peptide with the sequenceof the N-terminal domain of Doc2 $alpha$ interacting with Munc13-1. Thus,it is likely that the remaining effect of PMA on the capacitancejump in the presence of BIS (Fig. 3) involves interaction betweenDoc2 $alpha$ and Munc13-1. In other words, interaction between Doc2 $alpha$ and Munc13-1 may participate in regulation of the Prob_Ca.

  FOOTNOTES

Received June 6, 2001; revised July 31, 2001; accepted Aug. 2, 2001.

This work was supported by the National Science Foundation (IBN-0076091) and by the Mcdonnell Center for Cellular and MolecularNeurobiology (Washington University, St. Louis, MO). We thankDrs. Gong Chen, Steve Mennerick, and Jian-yuan Sun for criticalcomments on this manuscript and Dr. Jian-yuan Sun for his helpduring theexperiments.
Correspondence should be addressed to Ling-Gang Wu, Department of Anesthesiology, Campus Box 8054, Washington University Schoolof Medicine, 660 South Euclid Avenue, St. Louis, MO 63110. E-mail:wul{at}morpheus.wustl.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Albillos A, Dernick G, Horstmann H, Almers W, Alvarez de Toledo G, Lindau M (1997) The exocytotic event in chromaffin cells revealed by patch amperometry. Nature 389:509-512[Medline].
Bachoo M, Heppner T, Fiekers J, Polosa C (1992) A role for protein kinase C in long-term potentiation of nicotinic transmission in the superior cervical ganglion of the rat. Brain Res 585:299-302[Medline].
Betz A, Ashery U, Rickmann M, Augustin I, Neher E, Sudhof TC, Rettig J, Brose N (1998) Munc13-1 is a presynaptic phorbol ester receptor that enhances neurotransmitter release. Neuron 21:123-136[ISI][Medline].
Blackmer T, Larsen EC, Takahashi M, Martin TF, Alford S, Hamm HE (2001) G-protein $beta$ $gamma$ subunit-mediated presynaptic inhibition: regulation of exocytotic fusion downstream of Ca²⁺ entry. Science 292:293-297[Abstract/Free Full Text].
Borst JGG, Helmchen F, Sakmann B (1995) Pre- and postsynaptic whole-cell recordings in the medial nucleus of the trapezoid body of the rat. J Physiol (Lond) 489:825-840[Abstract/Free Full Text].
Burrone J, Lagnado L (2000) Synaptic depression and the kinetics of exocytosis in retinal bipolar cells. J Neurosci 20:568-578[Abstract/Free Full Text].
Byrne JH, Kandel ER (1996) Presynaptic facilitation revisited: state and time dependence. J Neurosci 16:425-435[Abstract/Free Full Text].
Capogna M, Gahwiler BH, Thompson SM (1995) Presynaptic enhancement of inhibitory synaptic transmission by protein kinases A and C in the rat hippocampus in vitro. J Neurosci 15:1249-1260[Abstract].
Dittman JS, Regehr WG (1998) Calcium dependence and recovery kinetics of presynaptic depression at the climbing fiber to Purkinje cell synapse. J Neurosci 18:6147-6162[Abstract/Free Full Text].
Fujita Y, Sasaki T, Fukui K, Kotani H, Kimura T, Hata Y, Sudhof TC, Scheller RH, Takai Y (1996) Phosphorylation of Munc-18/n-Sec1/rbSec1 by protein kinase C: its implication in regulating the interaction of Munc-18/n-Sec1/rbSec1 with syntaxin. J Biol Chem 271:7265-7268[Abstract/Free Full Text].
Gillis KD (1995) Techniques for membrane capacitance measurements. In: Single-channel recording (Sakmann B, Neher E, eds), pp 155-198. New York: Plenum.
Gillis KD, Mossner R, Neher E (1996) Protein kinase C enhances exocytosis from chromaffin cells by increasing the size of the readily releasable pool of secretory granules. Neuron 16:1209-1220[ISI][Medline].
Hilfiker S, Augustine GJ (1999) Regulation of synaptic vesicle fusion by protein kinase C. J Physiol (Lond) 515[Pt 1]:1[Abstract/Free Full Text].
Honda I, Kamiya H, Yawo H (2000) Re-evaluation of phorbol ester-induced potentiation of transmitter release from mossy fibre terminals of the mouse hippocampus. J Physiol (Lond) 529[Pt 3]:763-776[Abstract/Free Full Text].
Hori T, Takai Y, Takahashi T (1999) Presynaptic mechanism for phorbol ester-induced synaptic potentiation. J Neurosci 19:7262-7267[Abstract/Free Full Text].
Hsu S-F, Augustine GJ, Jackson MB (1996) Adaptation of Ca²⁺-triggered exocytosis in presynaptic terminals. Neuron 17:501-512[ISI][Medline].
Lindau M, Neher E (1988) Patch-clamp techniques for time-resolved capacitance measurements in single cells. Pflügers Arch 411:137-146[ISI][Medline].
Majewski H, Iannazzo L (1998) Protein kinase C: a physiological mediator of enhanced transmitter output. Prog Neurobiol 55:463-475[ISI][Medline].
Malenka RC, Madison DV, Nicoll RA (1986) Potentiation of synaptic transmission in the hippocampus by phorbol esters. Nature 321:175-177[Medline].
Malenka RC, Ayoub GS, Nicoll RA (1987) Phorbol esters enhance transmitter release in rat hippocampal slices. Brain Res 403:198-203[ISI][Medline].
Minota S, Kumamoto E, Kitakoga O, Kuba K (1991) Long-term potentiation induced by a sustained rise in the intra-terminal Ca²⁺ in bullfrog sympathetic ganglia. J Physiol (Lond) 435:421-438[Abstract/Free Full Text].
Oleskevich S, Walmsley B (2000) Phosphorylation regulates spontaneous and evoked transmitter release at a giant terminal in the rat auditory brainstem. J Physiol (Lond) 526:349-357[Abstract/Free Full Text].
Redman RS, Searl TJ, Hirsh JK, Silinsky EM (1997) Opposing effects of phorbol esters on transmitter release and calcium currents at frog motor nerve endings. J Physiol (Lond) 501[Pt 1]:41-48[ISI].
Reid CA, Bekkers JM, Clements JD (1998) N- and P/Q-type Ca²⁺ channels mediate transmitter release with a similar cooperativity at rat hippocampal autapses. J Neurosci 18:2849-2855[Abstract/Free Full Text].
Rosenmund C, Stevens CF (1996) Definition of the readily releasable pool of vesicles at hippocampal synapses. Neuron 16:1197-1207[ISI][Medline].
Sakaba T, Neher E (2001) Quantitative relationship between transmitter release and calcium current at the calyx of Held synapse. J Neurosci 21:462-476[Abstract/Free Full Text].
Schneggenburger R, Meyer AC, Neher E (1999) Released fraction and total size of a pool of immediately available transmitter quanta at a calyx synapse. Neuron 23:399-409[ISI][Medline].
Shapira R, Silberberg SD, Ginsburg S, Rahamimoff R (1987) Activation of protein kinase C augments evoked transmitter release. Nature 325:58-60[Medline].
Shimazaki Y, Nishiki T, Omori A, Sekiguchi M, Kamata Y, Kozaki S, Takahashi M (1996) Phosphorylation of 25 kDa synaptosome-associated protein. Possible involvement in protein kinase C-mediated regulation of neurotransmitter release. J Biol Chem 271:14548-14553[Abstract/Free Full Text].
Smith CB, Betz WJ (1996) Simultaneous independent measurement of endocytosis and exocytosis. Nature 380:531-534[Medline].
Son H, Carpenter DO (1996) Protein kinase C activation is necessary but not sufficient for induction of long-term potentiation at the synapse of mossy fiber-CA3 in the rat hippocampus. Neuroscience 72:1-13[Medline].
Stevens CF, Sullivan JM (1998) Regulation of the readily releasable vesicle pool by protein kinase C. Neuron 21:885-893[ISI][Medline].
Stevens CF, Wesseling JF (1998) Activity-dependent modulation of the rate at which synaptic vesicles become available to undergo exocytosis. Neuron 21:415-424[ISI][Medline].
Stevens CF, Wesseling JF (1999) Augmentation is a potentiation of the exocytotic process. Neuron 22:139-146[ISI][Medline].
Stevens CF, Williams JH (2000) "Kiss and run" exocytosis at hippocampal synapses. Proc Natl Acad Sci USA 97:12828-12833[Abstract/Free Full Text].
Sun JY, Wu LG (2001) Fast kinetics of exocytosis revealed by simultaneous measurements of presynaptic capacitance and postsynaptic currents at a central synapse. Neuron 30:171-182[ISI][Medline].
Thompson SM, Capogna M, Scanziani M (1993) Presynaptic inhibition in the hippocampus. Trends Neurosci 16:222-227[ISI][Medline].
Toullec D, Pianetti P, Coste H, Bellevergue P, Grand-Perret T, Ajakane M, Baudet V, Boissin P, Boursier E, Loriolle F (1991) The bisindolylmaleimide GF 109203X is a potent and selective inhibitor of protein kinase C. J Biol Chem 266:15771-15781[Abstract/Free Full Text].
Trudeau L-E, Emery DG, Haydon PG (1996) Direct modulation of the secretory machinery underlies PKA-dependent synaptic facilitation in hippocampal neurons. Neuron 17:789-797[ISI][Medline].
Von Gersdorff H, Sakaba T, Berglund K, Tachibana M (1998) Submillisecond kinetics of glutamate release from a sensory synapse. Neuron 21:1177-1188[ISI][Medline].
Wang L-Y, Kaczmarek LK (1998) High-frequency firing helps replenish the readily releasable pool of synaptic vesicles. Nature 394:384-388[Medline].
Wu LG, Borst JGG (1999) The reduced release probability of releasable vesicles during recovery from short-term synaptic depression. Neuron 23:821-832[ISI][Medline].
Wu LG, Saggau P (1997) Presynaptic inhibition of elicited neurotransmitter release. Trends Neurosci 20:204-212[ISI][Medline].
Wu LG, Borst JGG, Sakmann B (1998) R-type Ca²⁺ currents evoke transmitter release at a rat central synapse. Proc Natl Acad Sci USA 95:4720-4725[Abstract/Free Full Text].
Wu LG, Westenbroek RE, Borst JGG, Catterall WA, Sakmann B (1999) Calcium channel types with distinct presynaptic localization couple differentially to transmitter release in single calyx-type synapses. J Neurosci 19:726-736[Abstract/Free Full Text].
Yawo H (1999) Protein kinase C potentiates transmitter release from the chick ciliary presynaptic terminal by increasing the exocytotic fusion probability. J Physiol (Lond) 515:169-180[Abstract/Free Full Text].

Copyright © 2001 Society for Neuroscience 0270-6474/01/21207928-09$05.00/0

This article has been cited by other articles:

X. Lou, N. Korogod, N. Brose, and R. Schneggenburger
Phorbol Esters Modulate Spontaneous and Ca2+-Evoked Transmitter Release via Acting on Both Munc13 and Protein Kinase C
J. Neurosci., August 13, 2008; 28(33): 8257 - 8267.
[Abstract] [Full Text] [PDF]

G. Sharma, M. Grybko, and S. Vijayaraghavan
Action Potential-Independent and Nicotinic Receptor-Mediated Concerted Release of Multiple Quanta at Hippocampal CA3-Mossy Fiber Synapses
J. Neurosci., March 5, 2008; 28(10): 2563 - 2575.
[Abstract] [Full Text] [PDF]

Y. Shu, X. Liu, Y. Yang, M. Takahashi, and K. D. Gillis
Phosphorylation of SNAP-25 at Ser187 Mediates Enhancement of Exocytosis by a Phorbol Ester in INS-1 Cells
J. Neurosci., January 2, 2008; 28(1): 21 - 30.
[Abstract] [Full Text] [PDF]