Neuromodulators Enhance Transmitter Release by Two Separate Mechanisms at the Inhibitor of Crayfish Opener Muscle

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The Journal of Neuroscience, July 15, 1998, 18(14):5160-5169

Neuromodulators Enhance Transmitter Release by Two Separate Mechanisms at the Inhibitor of Crayfish Opener Muscle
Andrey Vyshedskiy¹, Kerry R. Delaney², and Jen-Wei Lin¹
¹ Department of Biology, Boston University, Boston, Massachusetts 02215, and ² Department of Biological Sciences, Simon Fraser University, Burnaby, British Columbia, V5A 156 Canada

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

A presynaptic voltage control method has been used to investigate the modulatory effects of serotonin (5-HT) and okadaic acid(OA) on the inhibitory junction of the crayfish opener muscle.Instead of using action potentials, we used 20 msec pulses depolarizedto 0 mV to activate transmitter release. This approach allowedus to monitor two separate physiological parameters related tothe release process. The first parameter, transmitter releasekinetics, is characterized as the delay when inhibitory postsynapticconductance reaches its half-maximum (IPSG₅₀). The second parameter,the total area of IPSG (IPSG_area), estimates total transmitteroutput. We have reported previously that the F2 component of synapticfacilitation is associated with a decrease in IPSG₅₀ but withouta change in IPSG_area. These results raised the possibility thatIPSG₅₀ and IPSG_area could be mediated by separate mechanisms thatwere modulated independently. To explore this possibility, weinvestigated the effects of 5-HT (100-200 nM) and OA (2.5 µM)on the two parameters. 5-HT and OA enhanced IPSG neither by changingthe sensitivity of postsynaptic receptors, as tested by iontophoreticallyejected GABA, nor by elevating resting and action potential-activatedpresynaptic free calcium, as monitored by fura-2 imaging. 5-HTand OA decreased IPSG₅₀ by 3.0 ± 1.4 and 3.6 ± 1.1 msec, respectively,and increased IPSG_area by 50 ± 21 and 37 ± 6%, respectively. Theability of F2 facilitation to accelerate release kinetics wasreduced in the presence of the modulators, suggesting that themechanism underlying the accelerated release kinetics was sharedby the two modes of synaptic enhancement. This report demonstratesthat the acceleration in release kinetics and the increase intotal release are two separate mechanisms for enhancing transmitteroutput and that these two mechanisms can be activated withoutchanges in presynaptic calcium dynamics.

Key words: IPSG; GABA; synaptic transmission; modulators; transmitter release; serotonin; okadaic acid

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The strength of synaptic transmission can be regulated by either activity-dependent or modulator-mediated processes. Activity-dependentsynaptic enhancement includes both short- and long-term synapticenhancement. Four distinct components of short-term synaptic enhancementhave been identified, F1 and F2 components of facilitation, augmentation,and post-tetanic potentiation (Magleby, 1987). Although it generallyis agreed that an increase in intracellular free Ca concentration([Ca²⁺]_i) is the main driving element for short-term synaptic enhancement,specific molecular processes that are activated by an increasein [Ca²⁺]_i have not yet been identified (Zucker, 1996). Modulator-mediatedprocesses represent a more diverse collection of processes. Modulatorshave been shown to increase transmitter release by regulatingpresynaptic calcium influx (McGehee et al., 1995; Byrne and Kandel,1996; Dittman and Regehr, 1996; Huang et al., 1996) or by directlymodulating the release machinery (Atwood et al., 1989; Man-Son-Hinget al., 1989; Dale and Kandel, 1990; Malgaroli and Tsien, 1992;Scanziani et al., 1992; Scholz and Miller, 1992; Klein, 1994;Dittman and Regehr, 1996; Trudeau et al., 1996). The fact thatthere are so many examples showing direct modulation of the releasemachinery suggests that more than one process may be involvedin this type of presynaptic mechanism. The separation and isolationof individual mechanisms at the physiological level are urgentlyneeded for further investigation of their molecular counterparts.

The excitatory junction of the crayfish claw opener has been used as a model system to study both activity-dependent and modulator-mediatedsynaptic plasticity. It has been demonstrated that this junctionexhibits both short- and long-term activity-dependent plasticity(Bittner, 1989; Dixon and Atwood, 1989a). The crayfish excitoralso has been used for in-depth investigation of modulator-mediatedsynaptic enhancement (Fischer and Florey, 1983; Dixon and Atwood,1985; Swain et al., 1991). Specific second messenger pathwaysunderlying the effects of serotonin have been identified (Dixonand Atwood, 1989b,c). Furthermore, it has been shown that serotoninincreases transmitter output without increasing presynaptic calciuminflux or the resting calcium level (Delaney et al., 1991). Therefore,there appear to be both calcium-driven and calcium-independentprocesses that can enhance transmitter output. To dissect thevarious presynaptic mechanisms, one usually relies on binomialanalysis (Zucker, 1973; Mclachlan, 1978), pharmacological manipulationsthat reveal presynaptic release probability (Hessler et al., 1993;Rosenmund et al., 1993), or the use of controlled presynapticpulses (Hochner et al., 1986a,b; Klein, 1994). This last approachsimplifies the analysis of presynaptic plasticity by controllingfor the class of mechanism mediated by potassium channel modulation.We have implemented a presynaptic voltage control method (Vyshedskiyand Lin, 1997a) at the inhibitory junction of the crayfish neuromuscularsynapse. Using 20 msec presynaptic steps as test pulses, we haverevealed that the F2 component of synaptic facilitation was associatedwith an acceleration in transmitter release kinetics (Vyshedskiyand Lin, 1997c). [F1 and F2 components of synaptic facilitationat the crayfish inhibitor are characterized by their decay timeconstants of 19 and 520 msec, respectively (Vyshedskiy and Lin,1997b)]. In addition, the total amount of transmitter release(total release) was not changed during F2 facilitation. If oneassumes that release kinetics and total release represent twoseparate mechanisms, the facilitation process would be presumedto use only one of them. To explore this possibility further,we believed it was essential to show that both parameters couldbe modulated. In this report we show that 5-HT and OA enhancetransmitter release at the inhibitor not by modulating calciuminflux but by simultaneously accelerating transmitter releasekinetics and increasing the total amount of transmitter release.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals and preparations. Crayfish, Procambarus clarkii, were obtained from Carolina Biological (Burlington, NC). Animalswere maintained at 23°C until use. Experiments using the voltagecontrol method as well as ratiometric calcium measurements wereperformed at 15°C (Vyshedskiy and Lin, 1997a). Experiments performedat room temperature (23°C) are specified in the figure legends.The typical size of the animals was ~3.8 cm, head to tail. Theopener muscle of the first walking leg was used for all experiments.Details of the experimental setup have been described before (Vyshedskiyand Lin, 1997a). Briefly, a presynaptic voltage electrode penetrateda secondary axon near a branch point where a tertiary branch emerged.A presynaptic current electrode penetrated the main branch pointof the inhibitor. The distance between the two presynaptic electrodeswas between 100 and 150 µm. A two-electrode voltage clamp amplifier(GeneClamp 500, Axon Instruments, Foster City, CA) was used tocontrol presynaptic potential. Two postsynaptic electrodes penetrateda muscle fiber near the presynaptic voltage electrode. One electrodewas used to inject current, and the second electrode recordedmembrane potential. This arrangement allowed us to monitor chlorideequilibrium potential (E_Cl), input resistance (R_m), and the timeconstant ( $tau$ _m) of the muscle fiber under study.

Experiments involving action potentials were conducted in a control saline (in mM): 195 NaCl, 5.4 KCl, 13.5 CaCl₂, 2.6 MgCl₂,and 10 sodium Na-HEPES, pH 7.4. In voltage control experimentsthe control saline was replaced by experimental solution (in mM):155 NaCl, 40 tetraethylammonium (TEA) chloride, 5.4 KCl, 10 CaCl₂,6.1 MgCl₂, 10 Na-HEPES, and 1 4-aminopyridine plus 300 nM tetrodotoxin,pH 7.4. All chemicals were purchased from Sigma (St. Louis, MO),except OA, which was ordered from Research Biochemicals (Natick,MA). Morphological examination of the terminal branches that innervatedthe recorded muscle fiber was performed after each experiment,by sketching or photography (Vyshedskiy and Lin, 1997a).

Modulator applications. The concentration of 5-HT used in all experiments was 100-200 nM. Previous studies of excitatory junctionshave used higher concentrations, from 1 to ~10 µM (Dixon and Atwood,1985). This was not practical for us because the infusion of high-level5-HT induced muscle contraction in the presence of K⁺ channel blockers. The introduction of 5-HT was achieved by increasingthe perfusion rate for 3-5 min to allow an exchange of five recordingchamber volumes, ~20 ml. Then the perfusion rate was returnedto the control level. This procedure created a transient increasein temperature, which returned to its control value within 5 minafter the perfusion rate was reduced to control level, 1 ml/min.

The effects of okadaic acid were studied in the absence of perfusion. Stock solution, 300 µl of 30 µM OA (okadaic acid ammonium)in experimental solution, was added to the recording chamber,~3.6 ml, to yield a final concentration of 2.5 µM. Control datawere collected for 40 min, in the absence of perfusion, beforeOA application. Stopping the perfusion did not affect transmitterrelease for as long as 2 hr (see Fig. 1B₂, for example).

Iontophoretic application of GABA. The effects of 5-HT and OA on postsynaptic GABA receptors were investigated by iontophoreticallyapplied GABA. The GABA-delivering pipette had a resistance of30 M $Omega$ , with 1 M GABA titrated to pH 4 with HCl. GABA was deliverediontophoretically by current pulses of ~1 µA and 5-20 msec. Long-termstability of GABA ejection was best achieved by using (1) sharpGABA electrodes with a short shank and (2) a retention currentof 5 nA to decrease the leakage of GABA. The placement of theGABA pipette, however, depended on experimental conditions. Inthe study of OA the GABA-containing pipette was placed as closeto a "hot spot" on the muscle fiber as possible. The pipette touchedthe muscle fiber, and the extent to which GABA was diluted atthe pipette tip appeared to be minimal.

With the GABA pipette positioned on a hot spot, application of 5-HT invariably led to a decrease in amplitude, and an increasein rise time, of the GABA-evoked response. These changes, withthe concurrent instability of muscle membrane potential, suggestthat the introduction of 5-HT triggered a small muscle contraction(n = 8). It has been shown that a small displacement, in the rangeof 5 µm, between the GABA pipette and a "hot spot" may lead toa 50% decrease in GABA-evoked responses (Takeuchi and Takeuchi,1965). To minimize the impact of small movements on the GABA-activatedpotential change, we positioned the GABA-containing electrodeat some distance from the muscle surface, ~10 µm. In this configurationthe GABA-evoked response slowly decreased over time (see Fig.2A₁), presumably because of the continuous dilution of the GABAsolution at the tip of electrode. The statistical analysis ofexperiments involving 5-HT application was performed after theslow decline was corrected for by linear extrapolation.

Presynaptic calcium imaging. Calcium concentration in presynaptic terminals was measured as previously described (Delaneyet al., 1989). An Olympus Quartz 60×, 0.8 numerical aperture waterimmersion objective and a cooled CCD camera (Photometrics CH250)were used to image the fluorescence from individual terminals.Presynaptic axons were filled with fura-2 by iontophoresis toa concentration of <200 µM. Selective stimulation of the inhibitoraxon at a frequency of 8-10 Hz for 30 sec was used to elevate[Ca²⁺]_i to a plateau level to assess the effect of 5-HT or OA on actionpotential-mediated calcium influx. The change in [Ca²⁺]_i was calculated as the difference between pretetanus [Ca²⁺]_i and the [Ca²⁺]_i at the end of each tetanus after [Ca²⁺]_i reached a plateau (Tank et al., 1995). The change in [Ca²⁺]_i during exposure to 5-HT or OA, 30-45 min after the modulatorswere applied, was compared with the average of three control trainsdelivered before the application of modulators. To ensure thatthe modulators were accessing the terminals and having an effecton synaptic transmission, we monitored in several experimentsthe IPSPs from proximal muscle fibers simultaneously with calcium-imagingmeasurements. The modulators were always effective when we checkedthe enhancement of transmitter release in calcium-imaging experiments.

Data analysis. The application of the voltage control method is valid only if the space constant of the inhibitor is not affectedby 5-HT and OA. It was shown previously that the quality of spatialcontrol correlates well with the shape of the depolarization-release(D-R) coupling plot of IPSPs activated by 5 msec presynaptic pulses(Vyshedskiy and Lin, 1997a). In a spatially well controlled terminal,suppression of the IPSP can be achieved when the presynaptic terminalis depolarized beyond 0 mV. To examine the possible effects of5-HT and OA on the presynaptic space constant, we compared themaximal point of the D-R coupling plot before and after the modulatorswere applied. The maximal point occurred at $-$ 5.0 ± 5.0 and at $-$ 1.0 ± 1.4 mV, respectively, before and after 5-HT application(n = 4). The control and experimental maximal points in OA experimentswere 4.4 ± 6.5 and 6.4 ± 5.7 mV (n = 5), respectively. The smalldifferences in the maximal points were not statistically significant.In addition, the modulators did not alter the shape of the D-Rcoupling curves, further suggesting that the presynaptic spaceclamp characteristics remained unchanged.

The use of chloride-containing electrodes in postsynaptic recordings increased the intramuscular chloride concentration, whichresulted in depolarizing IPSP. Signal-to-noise ratio considerationsprohibited us from performing simultaneous pre- and postsynapticvoltage clamp. To take into account the nonlinear summation ofIPSP, we routinely used the two postsynaptic electrodes to measureE_Cl, R_m, and $tau$ _m of the muscle fiber under investigation. The chloridedriving force ( $Delta$ E_Cl), which is defined as the difference betweenresting membrane potential and E_Cl, and the values of R_m and $tau$ _mallowed us to reconstruct inhibitory postsynaptic conductance(IPSG) from IPSP (Vyshedskiy and Lin, 1997a). The validity ofthis conversion has been verified previously by comparing thetime course of an IPSC calculated from IPSG with that of an IPSCmeasured with the use of two-electrode voltage clamp. $Delta$ E_Cl, R_m,and $tau$ _m of individual experiments are listed in the figure legends.All of the statistical data shown in this report are presentedin the form of mean ± SD, with sample size (n) that representsthe number of preparations. Student's t test was used in all statisticalanalyses.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

5-HT and OA enhance inhibitory synapses of the crayfish opener muscle

In the absence of previously published data, we first investigated the effects of 5-HT and OA on the crayfish inhibitor. Actionpotential-activated IPSPs were compared before and after the modulatorswere introduced. To control for factors that may affect IPSP amplitude,such as drifting E_Cl or nonlinear summation of IPSP amplitudes,we converted IPSP peak amplitudes to IPSG for quantitative analysis.Figure 1A₁ shows that 100 nM 5-HT initially increases IPSG amplitudeto 340% of control level. The enhancement then slowly decays to250%. The inset shows averaged IPSPs obtained in control saline(dashed line) and at 40-60 min after 5-HT application (solid line).The time course of IPSG enhancement averaged from 12 preparationsis shown in Figure 1B₁. There was a large variation in the magnitudeof initial enhancement. The maximal level, measured within 20min of 5-HT application, ranged from 210 to 892%. The enhancementthen settled into a phase of slow decline for the next hour. Datacollected between 40 and 60 min after 5-HT application were consideredto be in a steady state. The average value of the steady-stateenhancement was 304 ± 88%.

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Figure 1. 5-HT and OA enhance action potential-mediated transmitter release of the inhibitor. A, Time courses of peak IPSGs enhanced by 100 nM 5-HT (A₁) and 2.5 µM OA (A₂). Peak IPSGs were normalized to the average IPSG measured 5 min before the modulators were applied. Insets in A₁ and A₂, Control (1 and dashed line) and enhanced (2 and solid line) IPSPs that represent the averages of 60 and 75 trials, respectively. $Delta$ E_Cl and R_m measured before and after 5-HT was applied were 9 mV, 0.45 M $Omega$ and 8.3 mV, 0.4 M $Omega$ , respectively. $Delta$ E_Cl and R_m measured before and after OA was applied were 10 mV, 0.6 M $Omega$ and 10 mV, 0.7 M $Omega$ , respectively. B, Averaged time courses showing the effects of 5-HT (n = 12) and OA (n = 5) on IPSG amplitude. Open triangles in B₂ represent averaged results (n = 5) from control experiments in which perfusion was stopped but in which no OA was added. All experiments were performed at 23°C.

Figure 1A₂ shows that 2.5 µM OA induced an increase in IPSG that rose gradually and reached a plateau. The inset shows averagedIPSP recorded in control saline (dashed line) and at 40-60 minafter OA application (solid line). The time course and amplitudeof transmitter release enhancement mediated by OA were very similarto those observed at the crayfish excitor (Swain et al., 1991).Averaged results from five preparations are shown in Figure 1B₂( $open circle$ ), in which the steady-state level of OA-induced enhancementwas 412 ± 65% of control level. The strength of synaptic transmissionremained unchanged in control experiments ( $Delta$ ) in which perfusionwas stopped but no OA was introduced (n = 5). The enhancementof transmitter release mediated by both modulators remained stablethroughout the period of investigation. In the remaining partof this report we focus on the effects of 5-HT and OA during thesteady state.

5-HT and OA-mediated synaptic enhancement is not attributable to an increase in GABA receptor sensitivity

Although previous studies have established that 5-HT and OA enhance transmitter release by presynaptic mechanisms at the excitor(Fischer and Florey, 1983; Swain et al., 1991), no such evidenceis available for the inhibitor. Because of the small driving forcefor IPSPs, it is not possible to evaluate the postsynaptic effectsof these modulators by miniature IPSPs. We therefore examinedthis issue by investigating the GABA-mediated conductance change(g_GABA) activated by iontophoretically applied GABA. Figure 2,A₁ and A₂, shows that neither 5-HT nor OA affected GABA-activatedconductance, although action potential-activated IPSGs were enhancedby the modulators (Fig. 2B₁,B₂). Traces in the insets illustratethe membrane potential changes activated by iontophoreticallyapplied GABA before (dashed line) and after (solid line) the modulatorswere applied. These experiments were repeated in five preparationsfor each modulator in which g_GABA measured 1 hr after applying5-HT and OA was 95 ± 5 and 95 ± 9% of control levels, respectively.(The statistical analysis of the 5-HT effect was performed afterthe declining trend had been corrected for by linear extrapolation;see Materials and Methods).

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Figure 2. 5-HT and OA have no effect on GABA receptors of muscle fibers. A, 5-HT (A₁) and OA (A₂) do not change g_GABA. g_GABA amplitudes were calculated from membrane potential changes in a muscle fiber activated by iontophoretically applied GABA. Insets, GABA-activated membrane potential changes before (1 and dashed line) and after (2 and solid line) modulator application. The traces represent the averages of 38 trials. B, IPSGs calculated from action potential-activated IPSPs in the same muscle fibers. Both 5-HT (B₁) and OA (B₂) increase the IPSG amplitude. $Delta$ E_Cl and R_m measured before and after 5-HT application were 7.5 mV, 0.21 M $Omega$ and 7.5 mV, 0.21 M $Omega$ , respectively. The same parameters measured before and after OA application were 8.8 mV, 0.29 M $Omega$ and 9 mV, 0.3 M $Omega$ , respectively. All experiments were performed at 23°C.

5-HT and OA-mediated synaptic enhancement is not attributed to increased presynaptic calcium influx

To understand the mechanisms underlying 5-HT and OA-activated synaptic enhancement in the inhibitor, we examined the effectsof these modulators on resting and action potential-activated[Ca²⁺]_i. A previous study has demonstrated that 5-HT does not enhancetransmitter output by increasing [Ca²⁺]_i in the excitor (Delaney et al., 1991). Experiments performedin the inhibitor are shown here. The example shown in Figure 3A₁indicates that the level of resting and action potential-activated[Ca²⁺]_i was not increased by 200 nM 5-HT. In three preparations theresting [Ca²⁺]_i level changed <50 nM during the first 30 min after 5-HT addition.Small changes like these cannot be resolved confidently by fura-2imaging over the time scale studied here (Delaney et al., 1989;Tank et al., 1995). Although exposure to 1-2 µM 5-HT has beenreported to reduce slightly the accumulation of [Ca²⁺]_i during repetitive stimulation in the excitor (Delaney et al.,1991), application of 200 nM 5-HT to the inhibitor, in three preparations,changed the action potential-activated [Ca²⁺]_i increase by 2.1 ± 3.9%, which is not statistically differentfrom zero. The resting level of [Ca²⁺]_i also was not affected consistently by 2.5 µM OA, whereas actionpotential-activated [Ca²⁺]_i was decreased slightly. Figure 3B is an example of a typicalexperiment in which a slight downward shift in resting [Ca²⁺]_i was seen before the addition of OA, and this trend was notaffected by the addition or washout of OA. In six preparationsa small but significant decrease, 10.7 ± 5.6%, in the accumulationof [Ca²⁺]_i during trains of action potentials was observed between 30and 60 min after the addition of OA. The small decrease in actionpotential-elevated [Ca²⁺]_i can be attributed to a slight narrowing of presynaptic actionpotential duration (data not shown; see also Swain et al., 1991).Therefore, 5-HT and OA do not mediate synaptic enhancement byincreasing presynaptic calcium influx.

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Figure 3. Effects of 5-HT and OA on [Ca²⁺]_i level. Resting [Ca²⁺]_i levels are not changed by 5-HT (A) or OA (B). Activity-dependent calcium influx was activated by a train of 10 Hz action potentials for 30 sec. 5-HT (200 nM) did not create any detectable change in the [Ca²⁺]_i increase activated by the action potential train (A). OA (2.5 µM) application caused a small but significant decrease in the [Ca²⁺]_i increase activated by the same stimulation as in A (B).

5-HT and OA enhance synaptic transmission by accelerating release kinetics and increasing the total release

Because 5-HT and OA enhance synaptic transmission without altering the sensitivity of postsynaptic GABA receptors or increasingpresynaptic calcium influx, it was possible that these modulatorsenhanced transmitter output by regulating the release machinerydirectly. To investigate this possibility, we used the voltagecontrol method to examine the effects of these modulators on thekinetics of transmitter release and total release mediated by20 msec presynaptic steps. Figure 4, A₁ and A₂, shows examplesof pre- (lower traces) and postsynaptic (upper traces) recordingsobtained before (dashed line) and after (solid line) the modulatorswere applied. The waveforms of presynaptic voltage steps werenot altered by the modulators. However, transmitter release wasenhanced, as indicated by the larger IPSP amplitudes. In a totalof 14 experiments, seven for 5-HT and seven for OA, the shapesof presynaptic voltage steps recorded before and after applyingthe modulators were superimposable.

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Figure 4. 5-HT and OA accelerate release kinetics and increase IPSG_area. A, Pre- (lower) and postsynaptic (upper) potentials recorded 5 min before (dashed line) and ~50 min after (solid line) 100 nM 5-HT (A₁) and 2.5 µM OA (A₂) were applied. Presynaptic steps were 20 msec in duration and depolarized to 0 mV. A₁ and A₂ share the same time scale. B, IPSGs converted from IPSPs shown in A. 5-HT (B₁) and OA (B₂) increase IPSG_area significantly. The kinetics of IPSG is quantified by measuring the interval between the beginning of the pulse and the half-maximum point of IPSG ( $open circle$ ). B₁ and B₂ share the same time scale. C, Changes of IPSG₅₀ over time after 5-HT (C₁) and OA (C₂) application. Y-scales are identical on both graphs. Averaged results, with SD, are shown at the end (see Results). D, Time course of change in IPSG_area in response to 5-HT (D₁) and OA (D₂) application. Y-scales are identical on both graphs. Averaged results, with SD, are shown at the end (see Results). $Delta$ E_Cl, R_m, and $tau$ _m of the muscle fiber measured before and after 5-HT application were 10.1 mV, 0.47 M $Omega$ , 9.2 msec and 10.3 mV, 0.47 M $Omega$ , 8.9 msec, respectively. The membrane characteristics of the muscle fiber used in the OA experiment were 5.6 mV, 0.66 M $Omega$ , 13.8 msec and 6.2 mV, 0.75 M $Omega$ , 17.0 msec, respectively.

To analyze transmitter release quantitatively, we converted IPSPs into IPSG (Vyshedskiy and Lin, 1997a,c). Figure 4, B₁ andB₂, illustrates IPSGs converted from IPSPs shown in Figure 4,A₁ and A₂. Transmitter release kinetics was characterized as thetime when IPSG reaches half-maximum (IPSG₅₀) (Fig. 4B₁, $open circle$ ). Both5-HT and OA decreased IPSG₅₀. This effect is best visualized byscaling control IPSG to the height of enhanced IPSG (Fig. 4B₁,B₂,dotted line). The effect of the modulators on IPSG₅₀ over timeare plotted in Figure 4, C₁ and C₂, where IPSG₅₀ was reduced by22% (2.2 msec) in 100 nM 5-HT and by 37% (3.9 msec) in 2.5 µMOA. On average, 5-HT accelerated the release kinetics by 27 ±10% (3.0 ± 1.4 msec) of control IPSG₅₀ (n = 6). OA decreased IPSG₅₀by 36 ± 12% (3.6 ± 1.1 msec) of control value (n = 7). Finally,as in our analysis of F2 facilitation (Vyshedskiy and Lin, 1997c),we were not able to demonstrate conclusively a change in minimalsynaptic delay during 5-HT and OA-mediated synaptic enhancement.

The area of IPSG (IPSG_area) reflects the transmitter content of the early component of continuous transmitter release (Vyshedskiyand Lin, 1997c). The early component was defined as an initialtransient component of transmitter release, with a duration of~15 msec, which is followed by a steady-state, or late, componentthat persists for several seconds. Both 5-HT and OA increasedIPSG_area. The time course of the change in IPSG_area after eachof the modulators was applied is illustrated in Figure 4, D₁ andD₂. On average, 5-HT increased IPSG_area by 50 ± 21% (n = 6) andOA increased IPSG_area by 37 ± 6% (n = 7). This observation markedlydiffers from the activity-induced F2 facilitation, which doesnot change IPSG_area (Vyshedskiy and Lin, 1997c) (also see below).[There was an apparent difference in the time course of IPSG₅₀(Fig. 4C₁) and IPSG_area (Fig. 4D₁) after 5-HT application. Thisdifference was attributable mainly to changes in bath temperatureassociated with rapid solution exchange. Control experiments inwhich 5-HT was introduced slowly, and without disturbing bathtemperature, revealed a similar time course for IPSG₅₀ and IPSG_area(data not shown).]

Interaction between F2 facilitation and modulator-mediated synaptic enhancement

To investigate whether the accelerated release kinetics could be a mechanism shared by modulator-mediated synaptic enhancementand activity-dependent plasticity, we investigated the interactionbetween these two types of synaptic enhancement. The magnitudeof F2 facilitation was compared before and after the modulatorswere introduced. F2 facilitation was activated by a burst of eightsubthreshold conditioning pulses, a conditioning stimulus knownto activate a near-maximal level of facilitation without triggeringsignificant transmitter release (Vyshedskiy and Lin, 1997b). Themagnitude of F2 facilitation, measured 150 msec after the conditioningstimulus, was quantitated by measuring the difference betweencontrol and facilitated IPSG₅₀ ( $Delta$ IPSG₅₀ or release shift). Thisdifference has been shown to be related linearly to the magnitudeof F2 facilitation estimated from IPSG amplitudes (Vyshedskiyand Lin, 1997c). (To avoid confusion, we have referred to theincrease in synaptic strength associated with F2 facilitationas facilitation, whereas we have referred to the increase mediatedby the modulators as enhancement.)

Figure 5, A₁ and A₂, illustrates the effects of 5-HT and OA on control ( $open circle$ ) and facilitated ( $bullet$ ) IPSG₅₀. As in the example shownin Figure 4, 5-HT and OA decreased control IPSG₅₀. IPSG₅₀ measuredfrom facilitated responses also was reduced by 5-HT and OA. $Delta$ IPSG₅₀,which reflects the magnitude of F2 facilitation, was reduced significantlyby the modulators (Fig. 5B₁,B₂). On average, 5-HT decreased therelease shift by 39 ± 10% (1.5 ± 0.5 msec, n = 6), whereas OAdecreased the release shift by 76 ± 12% (2.4 ± 0.8 msec, n = 7).The observation that the release shift was reduced in the presenceof modulators suggests that F2 facilitation and the modulatorsmay share a common pathway that leads to accelerated release kinetics.

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Figure 5. Interaction between synaptic enhancement mediated by F2 facilitation and modulators. A, IPSG₅₀ measured from both control ( $open circle$ ) and facilitated ( $bullet$ ) IPSGs is decreased by 100 nM 5-HT (A₁) and 2.5 µM OA (A₂). The dotted lines are used to highlight the fact that 5-HT did not decrease IPSG₅₀ beyond the level achieved by F2 facilitation, whereas OA was able to reduce IPSG₅₀ beyond that level. B, The effect of F2 facilitation is quantified by calculating the difference between control and facilitated IPSG₅₀ ( $Delta$ IPSG₅₀). Both 5-HT (B₁) and OA (B₂) decrease $Delta$ IPSG₅₀. The averaged percentage change in $Delta$ IPSG₅₀ is shown also, with SD (see Results). Membrane characteristics of the muscle fiber used in the 5-HT experiment were 10.4 mV, 0.89 M $Omega$ , 13.5 msec and 10.4 mV, 0.88 M $Omega$ , 13.3 msec. The same parameters measured from the OA experiment were 6.6 mV, 0.38 M $Omega$ , 9.0 msec and 6.8 mV, 0.39 M $Omega$ , 9.3 msec.

It has been shown that F2 facilitation does not affect IPSG_area (Vyshedskiy and Lin, 1997c). This observation remains truein the presence of 5-HT and OA. The normalized change in IPSG_areais defined as:

where IPSG_cnt(area) and IPSG_test(area) represent control and facilitated IPSG_area, respectively. $Delta$ IPSG_area was 1.3 ± 5.5%(n = 13) in control saline and was $-$ 2.0 ± 5.4% (n = 6) and 4.1± 5.2% (n = 7) in 5-HT and OA, respectively. None of these valuesis statistically different from zero. Therefore, the presenceof modulators does not change one of the main characteristicsof F2 facilitation, i.e., IPSG_area remains constant.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

We have demonstrated that 5-HT and OA enhance transmitter output by presynaptic mechanisms that do not involve an increasein the level of resting or action potential-activated [Ca²⁺]_i. These modulators enhance transmitter output by acceleratingrelease kinetics and by increasing the total amount of transmitterrelease. Together with the finding that the release kinetics canbe modulated without changing the amount of total release by F2facilitation, the results reported here provide strong supportfor the hypothesis that there exist at least two separate mechanismsfor enhanced transmitter release that are independent of calciuminflux or resting [Ca²⁺]_i. Furthermore, the presynaptic voltage control method allowsus to monitor directly the two mechanisms physiologically.

Additional support for the above-mentioned hypothesis can be derived from the results of the interaction between the two modulatorsand F2 facilitation. Plots in Figure 5A show that, during thesteady state, 5-HT was not able to decrease IPSG₅₀ to the levelmediated by F2 facilitation, whereas OA decreased IPSG₅₀ beyondthat level (dotted lines in Fig. 5A₁, A₂). This was a consistentobservation, n = 6 for 5-HT and n = 6 for OA. Although one couldattribute this difference to the relatively low concentrationof 5-HT used in this report, concurrent comparison of the effectsof the two modulators on IPSG_area suggests that this interpretationis too simplistic. Specifically, despite the effectiveness ofOA in accelerating release kinetics, its ability to increase IPSG_areais lower than that of 5-HT (see Fig. 4D). Therefore, OA is moreeffective in accelerating kinetics than 5-HT, whereas the abilityof OA to increase IPSG_area is weaker than that of 5-HT at 100nM. This observation provides further support for the hypothesisthat transmitter release kinetics and total release representtwo separate mechanisms that can be modulated separately or differentially.

Because the modulators and F2 facilitation appear to share a common mechanism underlying the accelerated release kinetics,one would expect the magnitude of F2 facilitation to be reducedin 5-HT and OA. This prediction is consistent with the findingthat 5 µM OA effectively reduces facilitation (Swain et al., 1991).It has been shown that 5-HT reduces the magnitude of facilitationat 25 µM but has no effect at 25 nM (Fischer and Florey, 1983).Our results suggest a clear interaction between 100 nM 5-HT andF2 facilitation. Our results and those of Fischer and Florey (1983)are consistent if one assumes that release kinetics is modulatedby 5-HT in a concentration-dependent manner.

Despite rigorous pursuit it had not been possible previously to demonstrate changes in release kinetics, during facilitation,with transmitter release activated by action potentials or briefpresynaptic depolarization (Datyner and Gage, 1980; Parnas etal., 1989). The presynaptic voltage control method is able toprovide a clear demonstration of changes in release kinetics.The success of this method can be explained by comparing actionpotential-based studies and studies using the presynaptic controlmethod (Fig. 6A). The increase in transmitter release could beattributable to an increase in the total amount of transmittercontent (dashed line and V $up-arrow$ ) and/or attributable to an accelerationin release kinetics without changing transmitter content (wide-spaceddotted line and $alpha$ $up-arrow$ ). The differentiation between the two mechanismsis obvious when the duration of presynaptic depolarization is20 msec (Fig. 6A, lower trace, solid line). In contrast, an actionpotential with a duration of 2.5 msec only allows for a narrowwindow of observation (Fig. 6A, lower trace, dashed line and doublearrows). With such a short period of observation, the only significantchange in the postsynaptic response is in its amplitude. Kineticchanges would be difficult to resolve unless there was a clearshift in synaptic delay. Therefore, prolonged presynaptic depolarizationprovides a simple way to visualize directly certain mechanismsunderlying the increase in transmitter output.

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Figure 6. Multiple mechanisms for enhancement transmitter release. A, A schematic drawing to illustrate the two mechanisms that can enhance transmitter release. The solid curve in the upper panel represents the time course of vesicular release activated by a 20 msec presynaptic pulse (lower trace, solid line). Transmitter release can be increased by accelerating release kinetics (wide-spaced dotted line and $alpha$ $up-arrow$ ) and/or by increasing the total number of vesicles released without altering release kinetics (dashed line and V $up-arrow$ ). A brief presynaptic depolarization with a duration of 2.5 msec (lower trace, dashed line) allows one to observe only the beginning of transmitter release and therefore does not provide sufficient resolution to observe the mechanisms underlying release (double arrows). Inset, The transmitter release process is modeled according to a simple reaction in which V represents the concentration of available vesicles and R represents release; the secretion step has a forward reaction rate of $alpha$ , which is modulated by calcium ions. B, Block diagram illustrating different mechanisms that could increase transmitter output and the relationship between activity-dependent and modulator-mediated synaptic enhancement. 5-HT and OA are both able to increase protein phosphorylation. Physiological effects of protein phosphorylation include an acceleration in release kinetics and an increase in total release. Both mechanisms result in an increase in action potential-activated release. Facilitation processes have access only to the kinetic branch of the flow chart. It remains unclear whether the increase in [Ca⁺²]_i associated with F2 facilitation accelerates release kinetics by way of protein phosphorylation (dotted arrow) or processes further downstream (dashed arrow).

Mechanisms of 5-HT and OA effects

Second messenger pathways involved in 5-HT-mediated synaptic enhancement have been studied in detail at the crayfish excitor.A brief application of 5-HT evoked two distinct components ofsynaptic enhancement, a transient and a persistent component (Dixonand Atwood, 1985). It was suggested that the early and transientcomponent is mediated by the IP₃/protein kinase C pathway, whereasthe late and persistent component is mediated by the protein kinaseA pathway (Dixon and Atwood, 1989b,c). Assuming that the actionsof 5-HT on the inhibitor are identical to those on the excitor,it is reasonable to suggest that both the release kinetics andtotal release can be modulated by protein phosphorylation. Asa result, the qualitative similarities between the effects of5-HT and OA are not surprising, because OA also can enhance proteinphosphorylation by retarding the dephosphorylation process (Bialojanand Takai, 1988; Cohen et al., 1990). A summary of the effectsof these two modulators is illustrated in the form of a blockdiagram in Figure 6B. Possible targets of the phosphorylationprocess under our experimental conditions remain undefined. Effectsof protein phosphorylation on the transmitter secretion processalso have been implicated in the sensory-motor synapses of Aplysia(Hochner et al., 1986a; Byrne and Kandel, 1996), the squid giantsynapse (Lin et al., 1990; Llinás et al., 1991), and transgenicmice (Rosahl et al., 1995).

Acceleration in release kinetics

Kinetic description of the transmitter secretion process traditionally has been modeled as a chemical reaction in which freecalcium ions act as a catalyst (Fig. 6A, inset). To increase transmitterrelease (R), one could (1) increase [Ca²⁺]_i, (2) increase the concentration of available vesicles (V),or (3) increase the forward reaction rate ( $alpha$ ). Our results suggestthat 5-HT and OA do not increase [Ca²⁺]_i. The two physiological parameters analyzed here, release kineticsand total release, are conceptually equivalent to the forwardreaction rate and the concentration of available vesicles, respectively.

It would be too simplistic to take the acceleration in release kinetics literally and to try to construct a quantitative modelby increasing the forward reaction rate. Here, we discuss theaccelerated release conceptually in the context of two observations.First, there is no detectable change in minimal synaptic delayduring F2 facilitation (Vyshedskiy and Lin, 1997c) or modulator-mediatedsynaptic enhancement. Second, there is a decrease in apparentcalcium cooperativity during F2 facilitation (Stanley, 1986; Vyshedskiyand Lin, 1997b). We propose that the accelerated release is attributableto a redistribution in the states of synaptic vesicles. Specifically,available vesicles are assumed to be in various states of readinessfor release. Highly ready vesicles will be released first andless ready vesicles will be released later (Fig. 6A, upper trace,solid line), if calcium influx continues during a 20 msec presynapticdepolarization (Fig. 6A, lower trace, solid line). Both the facilitationprocess and modulators increase the fraction of vesicles thatare in a highly ready state. If the minimal synaptic delay isdetermined by the presence of vesicles in the highly ready state,an increase in the fraction of these vesicles should not changethe detection of the minimal delay.

The precise definition of the vesicular states remains a matter of speculation. For example, different vesicular states maycorrespond to various stages of assembly of the docking complexthat includes, but is not limited to, synaptobrevin, syntaxin,SNAP-25, synaptotagmin, and calcium channels (for review, seeSollner and Rothman, 1996). Alternatively, different vesicularstates may correspond to various levels of phosphorylation ofthe docking complex proteins (Fujita et al., 1996; Hirling andScheller, 1996; Shimazaki et al., 1996; Yokoyama et al., 1997).The physiological significance of these biochemically definedstates is not completely understood. An alternative definitionof various states of readiness could be made at a physiologicallevel. Specifically, they may reflect the state of calcium bindingsites associated with the secretion machinery. It has been proposedthat facilitation is attributable to the filling of high-affinitycalcium binding sites of the secretion machinery (Stanley, 1986;Yamada and Zucker, 1992; Winslow et al., 1994; Bertram et al.,1996). This definition theoretically could generate a detectablechange in release kinetics during prolonged release and representsa direct modulation of elevated [Ca²⁺]_i on vesicular states (Fig. 6B, dashed arrow). In addition, thismodel fits well with the finding that calcium cooperativity isdecreased during facilitation. Therefore, known kinetic propertiesof F2 facilitation are well accounted for by this model.

However, this line of logic cannot explain the finding that the modulators and F2 facilitation share the same pathway leadingto an acceleration in release kinetics. How can 5-HT and OA acceleraterelease kinetics by filling the high-affinity calcium bindingsites when neither of the modulators increases [Ca²⁺]_i? One way to resolve this controversy would be to assume thatprotein phosphorylation may "activate" one of the calcium bindingsites such that the calcium binding of that site would not benecessary for secretion. (Alternatively, the affinity of the calciumbinding sites could be increased by phosphorylation such thatsome of the sites would be occupied at the resting level of [Ca²⁺]_i.) Supporting evidence for this hypothesis comes from the Drosophiladnc mutant in which the cellular cAMP-dependent phosphorylationlevel is elevated (Byers et al., 1981). The calcium cooperativityof transmitter release in this mutant is 3, rather than 4 as observedin wild-type animals, which suggests the possibility that proteinphosphorylation could modulate calcium cooperativity (Zhong andWu, 1991). However, there is also evidence indicating no changein calcium cooperativity in 5-HT (Glusman and Kravitz, 1982).The second way to resolve this controversy would be to proposethat F2 facilitation also passes through protein phosphorylation(Fig. 6B, dotted arrow). Because it is well documented that elevatedintracellular free calcium is the main driving element for synapticfacilitation, it is conceivable that calcium/calmodulin-dependentprotein kinase pathways could underlie synaptic facilitation.Pharmacological studies, however, have failed to substantiatea role for the CAM kinase II pathway in F2 facilitation in theinhibitor. [We have tested calmidasolium (up to 50 µM), n = 2;KN-62 (up to 100 µM), n = 3; KN-93 (up to 50 µM), n = 2; and K-252a(up to 5 µM), n = 2. None of the drugs significantly altered F2facilitation. See also Kamiya and Zucker (1994) for experimentsin the excitor.] Therefore, further study is needed to understandmolecular mechanisms for the modulator-mediated acceleration inrelease kinetics.

Regulation of total release

Results reported here demonstrate that 5-HT and OA are able to increase the total amount of transmitter release mediated bya 20 msec pulse. A 20 msec step depolarized to 0 mV releases upto 90% of the transmitter content of an early component of continuoustransmitter release (Vyshedskiy and Lin, 1997c). The specificmechanism that underlies this early component is unknown. An obviouspossibility is that this component reflects a pool of availablevesicles, which includes vesicles in various states of readiness.The modulation of the size of this pool by 5-HT and OA then couldbe considered in terms of vesicular mobilization resulting ina larger number of available vesicles. Because of our limitedunderstanding in the dynamics of vesicular mobilization duringcontinuous transmitter release, it is difficult to discuss theconcept of available vesicles in more specific terms.

Factors other than a vesicular pool with vesicles in various states of readiness also can shape the transmitter release timecourse and create an "apparent" available pool. For example, inactivationof calcium current (Wright et al., 1996a,b), adaptation of therelease process (Hsu et al., 1996), calcium sequestration duringthe 20 msec pulse (Herrington et al., 1996), or a combinationof GABA receptor desensitization and increased GABA reuptake duringthe 20 msec pulse may all create a transient component duringcontinuous release. Because 5-HT and OA increase neither the restingnor the action potential-activated [Ca²⁺]_i, a decrease in calcium current inactivation or a decrease incalcium sequestration, during 20 msec pulses, can be ruled outas possible pathways by which the modulators could increase totalrelease. In addition, because responses evoked by iontophoreticallyapplied GABA were not changed by the modulators, the possibilitythat postsynaptic modulation creates an apparent increase in totalrelease can be ruled out also. The adaptation process has beendescribed in the squid giant synapse where transmitter secretionis prematurely terminated, in the presence of high [Ca²⁺]_i, and in the absence of vesicle depletion. This process hasnot been studied in the crayfish neuromuscular junctions and cannotbe ruled out as a possible target for the modulation of totalrelease. Consequently, 5-HT and OA may increase total releaseby slowing or blocking the adaptation process or by increasingthe number of available vesicles in the early component.

In conclusion, this report demonstrates the presence of at least two separate mechanisms for the enhancement of transmitterrelease. The separation of these mechanisms by distinct physiologicalparameters should facilitate future studies of the molecular basisfor these mechanisms.

  FOOTNOTES

Received Jan. 14, 1998; revised April 24, 1998; accepted April 28, 1998.

This work was supported by National Institutes of Health Grant NS31707 (to J.W.L.) and by the Natural Sciences and EngineeringResearch Council Canada (OG 0121698 to K.D.). We thank Nicky Schweitzerfor correcting our English.
Correspondence should be addressed to Dr. Jen-Wei Lin, Department of Biology, Boston University, 5 Cummington Street, Boston,MA 02215.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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