Involvement of cGMP-Dependent Protein Kinase in Adrenergic Potentiation of Transmitter Release from the Calyx-Type Presynaptic Terminal

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The Journal of Neuroscience, July 1, 1999, 19(13):5293-5300

Involvement of cGMP-Dependent Protein Kinase in Adrenergic Potentiation of Transmitter Release from the Calyx-Type Presynaptic Terminal
Hiromu Yawo
Department of Neurophysiology, Tohoku University School of Medicine, Sendai 980-8575, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

I have previously reported that norepinephrine (NE) induces a sustained potentiation of transmitter release in the chick ciliaryganglion through a mechanism pharmacologically distinct from anyknown adrenergic receptors. Here I report that the adrenergicpotentiation of transmitter release was enhanced by a phosphodiesteraseinhibitor, 3-isobutyl-1-methylxanthine (IBMX) and by zaprinast,an inhibitor of cGMP-selective phosphodiesterase. Exogenous applicationof the membrane-permeable cGMP, 8-bromo-cGMP (8Br-cGMP), potentiatedthe quantal transmitter release, and after potentiation, the additionof NE was no longer effective. On the other hand, 8Br-cAMP neitherpotentiated the transmitter release nor occluded the NE-inducedpotentiation. The NE-induced potentiation was blocked by neithernitric oxide (NO) synthase inhibitor nor NO scavenger. The quantaltransmitter release was not potentiated by NO donors, e.g., sodiumnitroprusside. The NE-induced potentiation and its enhancementby IBMX was antagonized by two inhibitors of protein kinase G(PKG), Rp isomer of 8-(4-chlorophenylthio) guanosine-3',5'-cyclicmonophosphorothioate and KT5823. As with NE-induced potentiation,the effects of 8Br-cGMP on both the resting intraterminal [Ca²⁺] ([Ca²⁺]_i) and the action potential-dependent increment of [Ca²⁺]_i ( $Delta$ Ca) in the presynaptic terminal were negligible. The reductionof the paired pulse ratio of EPSC is consistent with the notionthat the NE- and cGMP-dependent potentiation of transmitter releasewas attributable mainly to an increase of the exocytotic fusionprobability. These results indicate that NE binds to a novel adrenergicreceptor that activates guanylyl cyclase and that accumulationof cGMP activates PKG, which may phosphorylate a target proteininvolved in the exocytosis of synapticvesicles.

Key words: adrenergic receptors; cGMP; protein kinase G; presynaptic terminal; synaptic plasticity; neurotransmitter release

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Norepinephrine (NE) and epinephrine are principal neuromodulators in the central and peripheral nervous systems (Moore andBloom, 1979; Kuba et al., 1981; Nicoll et al., 1990). The adrenergicresponses are characterized according to both the receptor subtypesand the intracellular signal transduction mechanisms (Nicoll etal., 1990; Bylund et al., 1994; Goldstein, 1998). For example,the $alpha$ ₁-adrenergic receptors usually couple with phospholipaseC and use IP₃ and diacylglycerol as second messengers (Nicollet al., 1990; Bylund et al., 1994). The $alpha$ ₂-adrenergic receptorspreferentially couple with G_i-group G-proteins and downregulateadenylyl cyclase or modulate K⁺ channels or Ca²⁺ channels through a membrane-delimited mechanism (Nicoll et al.,1990; Delcour and Tsien, 1993; Milligan, 1993; Bylund et al.,1994; MacKinnon et al., 1994). The $beta$ -adrenergic receptors aretypical of the G_s-coupled receptors, which upregulate adenylylcyclase (Nicoll et al., 1990; Milligan, 1993; Bylund et al., 1994).However, some adrenergic responses are resistant to conventionalantagonists of any present known adrenergic receptors (Hirst etal., 1982, 1992; Benham and Tsien, 1988). In the rat arterialsmooth muscle, NE causes a membrane depolarization that is resistantto $alpha$ and $beta$ blockade (Hirst et al., 1982). Similarly, the NE-dependentenhancement of the L-type Ca²⁺ current in the arterial smooth muscle was resistant to blockersof $alpha$ - and $beta$ -adrenergic receptors (Benham and Tsien, 1988). However,whether these responses are attributable to the activation ofa new class of adrenergic receptors remains unknown. I have previouslyreported that NE induces a sustained potentiation of transmitterrelease in the chick ciliary ganglion through a mechanism resistantto any known adrenergic receptor antagonists (Yawo, 1996). Moreover,no receptor-selective synthetic agonists induced the potentiationof transmitter release, and only NE, adrenaline, and dopamineinduced the potentiation (Yawo, 1996). Here, I report that theNE-induced presynaptic potentiation involves a nitric oxide (NO)-independentguanylyl cyclase and that an intraterminal increase of cGMP inducesthe potentiation of transmitter release by activating proteinkinase G (PKG). It is suggested that the potentiating adrenergicreceptor in the calyx-type presynaptic terminal is different fromany known adrenergic receptors in terms of the intracellular signaltransduction as well as pharmacologicalproperties.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation. The methods used here are the same as those described previously (Yawo, 1996, 1999). Chick embryos (White Leghorn;Aoki Egg Farm, Nasu, Japan) were incubated at a constant temperatureof 37°C. Day 14 embryos (stage 39-40; Hamburger and Hamilton,1951) were decapitated, and the ciliary ganglion was removed withthe presynaptic oculomotor nerve. A whole ganglion was mountedin a superfusing chamber (~1 ml); the oculomotor nerve was drawnto the stimulating electrode by suction; and the collagenous envelopewas enzymatically removed by focally applying a mixture of collagenase(type II, 2000 U/ml; Sigma-Aldrich, St. Louis, MO) and thermolysin(20 U/ml, Sigma-Aldrich) through a glass pipette (tip diameter,30 µm). The ganglion was superfused with standard saline (in mM:NaCl, 132; KCl, 5; CaCl₂, 1; MgCl₂, 1; HEPES, 10; NaOH, 4; andglucose 11, pH adjusted to 7.4 with NaOH). All experiments wereperformed at room temperature (25°C).

EPSC recordings. A conventional whole-cell patch-clamp recording was made from a postsynaptic ciliary neuron (Yawo, 1996,1999) using an EPC-7 patch-clamp amplifier (List Electronic, Darmstadt-Eberstadt,Germany). Patch pipettes (2.5-3 M $Omega$ , coated with silicon resinand fire-polished) were filled with an internal solution containing(in mM): CsCl, 130; MgCl₂, 1; Na₂-EGTA, 10; HEPES, 10; and MgATP,5, pH adjusted to 7.4 with NaOH. The series resistance was usually<10 M $Omega$ throughout the experiment. EPSC was measured at a holdingpotential of $-$ 60 mV. To ensure the stable recording of EPSC, thecapacitative transient was minimized by electrical circuitry,and the series resistance was compensated for by 50-70%. The whole-cellcurrents were low-pass-filtered at 3 kHz ( $-$ 3 dB, eight-pole Besselfilter, P-84P; NF Electronic Instruments, Yokohama, Japan), digitizedat 10-20 kHz (ADX-98E; Canopus, Kobe, Japan), and stored in acomputer (PC9801FA; NEC, Tokyo,Japan).

The quantal content (m) was estimated from the coefficient of variation (c.v.) based on Poisson statistics (Kuno and Weakly,1972). When the occurrence of failure transmission was moderate,m calculated from the occurrence of failure was almost identicalto that calculated from the c.v., indicating that the EPSC fluctuationapproximately followed the Poisson statistics (Martin and Pilar,1964a; Yawo and Chuhma, 1994). Therefore, [Ca²⁺]_o and [Mg²⁺]_o were adjusted so that the occurrence of transmission failurewas obvious at the beginning of the experiment. Because of theinfrequent occurrence of miniature EPSCs, the quantal size (q)was estimated as the mean EPSC divided by m.

Measurement of intraterminal Ca²⁺ concentration. The method of measuring intraterminal [Ca²⁺] ([Ca²⁺]_i) was almost the same as described previously (Yawo and Chuhma,1993; Yawo, 1996, 1999). The oculomotor nerve was cut at its exitfrom the orbital bone in Ca²⁺-free saline containing 1 mM EGTA. Crystals of fura-2-conjugateddextran (fura dextran, M_r 10,000; Molecular Probes, Eugene, OR)were applied to the distal stump. After 30 min of incubation at10°C, the ganglion was incubated at 37°C for 1.5 hr. Fura dextranwas transported anterogradely and accumulated in the calyx-typenerve terminals. Because of its large molecular size, fura dextranwas confined to the presynaptic axons and their terminals. A conventionalepifluorescence system equipped with a water-immersion objective(40×; numerical aperture, 0.7; Olympus, Tokyo, Japan) and xenonlamp (150 W) was used. Fluorescence was excited alternately atwavelengths of 340 and 380 nm. Because the microscope was focusedon the surface of the ganglion, the fluorescence from one to threeterminals was measured at a single spot with a diameter of 50µm by a photomultiplier tube (OSP-3, Olympus). Confocal pupilsat both excitation and emission light paths enable a reductionin the background fluorescence behind the focal plane. The signalwas integrated for 80 msec and sampled at 12.5 Hz by a computer(PC-9801RS, NEC) using software for measuring the intracellularCa²⁺ (MiCa, provided by Drs. K. Furuya and K. Enomoto, National Instituteof Physiological Science of Japan). Twenty records were averagedusing the computer-generated stimulating pulse as a trigger. The[Ca²⁺]_i was calculated from the ratio of fluorescence intensities atwavelengths of 340 and 380 nm (Grynkiewicz et al., 1985) usingthe dissociation constant determined by the manufacturer (216nM). The minimum ratio and the maximum fluorescence at 380 nmwere measured in a Ca²⁺-free solution containing 10 mM EGTA and 0.1 mM ionomycin (Calbiochem,La Jolla, CA). Thereafter, the solution was changed to one containing10 mM Ca²⁺, and the maximum ratio and the minimum fluorescence at 380 nmweremeasured.

Reagents. Pharmacological agents were usually bath-applied through a surperfusing line with a constant flow rate. The solutionin the chamber was completely replaced in <2 min. The agents usedin this study and their sources were as follows: L-NE (NacalaiTesque, Kyoto, Japan); phentolamine (Research Biochemicals International,Natick, MA); D,L-propranolol (Sigma-Aldrich); 3-isobutyl-1-methylxanthine(IBMX, Sigma-Aldrich); zaprinast (Sigma-Aldrich); Ro-20-1724 (BIOMOL">BiomolResearch Laboratories, Inc., Plymouth Meeting, PA); 8-bromo-cGMP(8Br-cGMP, Sigma-Aldrich); 8Br-cAMP (Sigma-Aldrich); N-nitro-L-arginine methyl ester (L-NAME, Sigma-Aldrich); hemoglobin(Sigma-Aldrich); sodium nitroprusside (SNP, Sigma-Aldrich); (±)-(E)-4-methyl-2-[(E)-hydroxyimino]-5-nitro-8-methoxy-3-hexenamide(NOR1; Dojin, Tabaru, Kumamoto, Japan); Rp isomer of 8-(4-chlorophenylthio)guanosine-3',5'-cyclic monophosphorothioate (Rp-8pCPT-cGMPS; BioLogLife Science Institute, Bremen, Germany); KT5823 (Calbiochem);phorbol 12-myristate 13-acetate (PMA; Wako, Osaka, Japan); andbisindolylmaleimide I (BIS, Calbiochem). The 10 mM stock solutionof NE was made with isomolar isoascorbic acid (Wako), and NE wasbath-applied with 10 µM isoascorbic acid, which has no effecton the synaptic transmission. All the experiments were done underyellow fluorescent light (wavelength, >520 nm; EL40SY-F; MatsushitaElectronic Co., Kadoma, Japan) to minimize the photodynamic oxidation.IBMX was dissolved as 100 mM in 0.1N NaOH. Zaprinast was dissolvedas 100 mM in 0.2 M N-methyl-D-glucamine (Sigma-Aldrich). Ro-20-1724,Rp-8pCPT-cGMPS, KT-5823, PMA, and BIS were dissolved in DMSO andthen diluted. The concentration of DMSO did not exceed 0.1% andby itself had no effect on the EPSC. To minimize the aberranteffects of the cyclic nucleotides on the A₁-adenosine autoreceptors(Yawo and Chuhma, 1993), the antagonist 8-cyclopentyl-1,3-dimetylxanthine(10 µM, Research Biochemicals International) was present throughouttheexperiment.

The values in the text and figures are mean ± SEM (number of experiments). Statistically significant differences between variousparameters were determined using Student's two-tailed t test forpaired data. Otherwise, Mann-Whitney's U test was used. Usually,p < 0.05 was consideredsignificant.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pharmacological properties of adrenergic presynaptic potentiation

The previous study (Yawo, 1996) revealed that NE increases the quantal transmitter release from calyx-type presynaptic terminalsof chick ciliary ganglion with a negligible change in the postsynapticacetylcholine sensitivity. As shown in Figure 1A, NE (10 µM) potentiatedthe average EPSC even in the presence of both an $alpha$ ₁- and $alpha$ ₂-adrenergicreceptor antagonist, phentolamine (10 µM), and a $beta$ -adrenergicreceptor antagonist, propranolol (10 µM). A fluctuation of theEPSC amplitude was observed in extracellular solution with lowCa²⁺ and high Mg²⁺ (Fig. 1B). Before the application of NE, the capacitative couplingresponse, which indicates the presynaptic invasion of the actionpotential (Yawo and Chuhma, 1994), occasionally accompanied anull EPSC response (synaptic failure). As indicated in the amplitudehistogram of control EPSCs before the application of NE (Fig.1C), the occurrence of failures was 7 in 100 consecutive trials.From the c.v., m and q were estimated to be 2.7 and 8.6 pA, respectively.Based on Poisson statistics (Martin and Pilar, 1964a; Yawo andChuhma, 1994), the expected occurrence of failure (Fig. 1C, arrow)is 7 in 100 trials, which is exactly identical to the observedoccurrence. In the presence of NE, no synaptic failures were observed,whereas instead the frequency of the occurrence of large EPSCswas increased (Fig. 1D); m and q were 10.6 and 9.0 pA, respectively.Therefore, NE increased m of the EPSC by 3.9-fold of the controlwith a negligible change in q in the presence of both phentolamineand propranolol. In all three experiments in the presence of bothphentolamine and propranolol, NE potentiated the EPSC by 1.6-to 3.6-fold of the control, which was the same as that in theabsence of adrenergic antagonists (range, 1.4- to 3.5-fold ofcontrol; n = 6; p > 0.1, Mann-Whitney's U test). Agonists selectivefor the $alpha$ ₁- or $beta$ -adrenergic receptors had no effect on the EPSC,and the $alpha$ ₂-adrenergic receptor agonist clonidine attenuated theEPSC (Yawo, 1996). Thus, the NE-dependent potentiation appearsto be mediated by a mechanism pharmacologically distinct fromany known adrenergic receptors.

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Figure 1. Adrenergic presynaptic potentiation in a chick ciliary ganglion. A, Representative experimental data showing the effect of 10 µM NE on the EPSC. The extracellular solution contained 1 mM [Ca²⁺]_o and 5 mM [Mg²⁺]_o. Phentolamine (10 µM) and propranolol (10 µM) were present throughout the experiment. The presynaptic oculomotor nerve was stimulated at 0.5 Hz by twin pulses with an interpulse interval of 40 msec. The biphasic current between the stimulus artifact and the EPSC is the capacitative coupling response indicating the invasion of the action potential into the presynaptic terminal. Top, Average EPSC of 100 consecutive records during control. The facilitation ratio was 2.3. Bottom, Average trace of 100 consecutive records during bath application of NE. The facilitation ratio was 1.8. B, Time-dependent plots of the EPSC amplitude of the experiment shown in A. NE (10 µM) was bath-applied during the indicated period (open bar). C, EPSC amplitude histogram of 100 consecutive records before the application of NE, the average of which was shown in A (top). The quantal content (m) and the quantal size (q) were estimated from c.v. and were 2.7 and 8.6 pA, respectively. The arrow on the left indicates the occurrence of failures expected from a Poisson distribution. D, EPSC amplitude histogram of 100 consecutive records during NE-induced potentiation, the average of which was shown in A (bottom). The m and the q were 10.6 and 9.0 pA, respectively.

Effects of phosphodiesterase inhibitors

The slow onset and the long-lasting nature of the NE-induced potentiation suggest the involvement of second messengers, e.g.,cyclic nucleotides. To test this notion, the effects of a phosphodiesterase(PDE) inhibitor, IBMX, were first investigated. A moderate EPSCpotentiation by 0.1 µM NE was further enhanced by IBMX (Fig. 2A),whereas IBMX alone had no effect (Fig. 2B). An increase in thedose of NE from 0.1 to 10 µM significantly increased the magnitudeof potentiation (p < 0.05, Mann-Whitney's U test), whereas thelevel of enhancement produced by IBMX remained virtually unchanged(p > 0.3, Mann-Whitney's U test; Fig. 2B). This suggests thatIBMX may inhibit the degradation of cyclic nucleotides, therebypotentiating the responsiveness to NE, and that this responsivenessto NE may be saturated in the presence of IBMX.

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Figure 2. Enhancement of NE-induced potentiation by inhibitors of cyclic nucleotide PDE. A, Time-dependent plots of the average EPSC amplitude in a representative experiment. NE (0.1 µM, open bar) and IBMX (100 µM, closed bar) were bath-applied during the indicated periods. Insets, Sample records of the EPSC of control (left), in the presence of NE (middle), and in the presence of both NE and IBMX (right). The small biphasic signal preceding the EPSC is the capacitative coupling response. Calibration: 10 msec, 0.5 nA. B, Summary of the effects of IBMX (100 µM) on the NE-dependent potentiation of EPSC. EPSCs were normalized to the mean EPSC in the absence of NE and IBMX. Each column is the mean of six or seven experiments. Error bars indicate SEM. Statistical significance was evaluated as indicated by paired t test. All differences between the groups with and without NE treatment were significant (p < 0.02, paired t test). C, Average effect of zaprinast (30 µM; n = 8) on NE-dependent potentiation of EPSC, which was normalized to that just before the application of NE (0.1 µM). Error bars indicate SEM. D, Summary (n = 7) of the effect of Ro-20-1724 (100 µM) on NE (0.1 µM)-dependent potentiation of EPSC. Each column is the mean of the value normalized to the control value in the absence of NE and Ro-20-1724; from left to right, the control, in the presence of NE, and in the presence of both NE and Ro-20-1724. The difference between the middle and the right columns is insignificant (p > 0.7, paired t test). Error bars indicate SEM.

The NE-dependent potentiation was also enhanced by zaprinast (Fig. 2C), an inhibitor of cGMP-selective PDE (PDE5). Zaprinastenhanced the NE (0.1 µM)-dependent potentiation by 1.77 ± 0.19-fold(n = 9; p < 0.02, paired t test between raw data), whereas zaprinastalone did not potentiate the EPSC (1.10 ± 0.04 of the control;n = 6; p > 0.1, paired t test between raw data). In contrast,Ro-20-1724, an inhibitor of cAMP-selective PDE (PDE4), had noeffect on the NE-induced EPSC potentiation (Fig. 2D). Therefore,cGMP rather than cAMP appears to be involved as the second messengerof the NE-induced potentiation of transmitterrelease.

Effects of cyclic nucleotide analogs

Next, the effect of the membrane-permeable cGMP analog 8Br-cGMP was examined. The EPSCs fluctuated in amplitude in the solutionwith low Ca²⁺ and high Mg²⁺ concentrations and often failed to elicit any response but, onaverage, were potentiated by 8Br-cGMP (30 µM) in a sustained manner(Fig. 3A,B). Synaptic failure occurred in 71 of 100 trials beforethe application of 8Br-cGMP (Fig. 3C). Bath application of 30µM 8Br-cGMP decreased the occurrence of synaptic failures to 18of 100 trials and increased the occurrence of large EPSCs (Fig.3B,D). Calculations based on these data (n = 6) revealed that8Br-cGMP (30 µM) increased the mean number of quanta in a singleEPSC (quantal content) by 2.23 ± 0.55-fold with a negligible changein the mean size of a single quanta (quantal size, 1.00 ± 0.14-fold),the difference being significant (p < 0.02, Mann-Whitney's U test).As summarized in Figure 3E, 8Br-cGMP potentiated the EPSC amplitudesignificantly, and no further potentiation was induced by theaddition of NE after potentiation by 8Br-cGMP. In contrast, thesame concentration of 8Br-cAMP did not potentiate the EPSC, andNE potentiated the EPSC in the presence of 8Br-cAMP to the sameextent as in its absence (Fig. 3E).

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Figure 3. Effects of membrane-permeable cyclic nucleotide analogs on the transmitter release. A, Representative experimental data showing the effect of 8Br-cGMP on the EPSC. The presynaptic oculomotor nerve was stimulated at 0.33 Hz by twin pulses with an interpulse interval of 40 msec. Top, Average trace of 100 consecutive records before the application of 8Br-cGMP. The facilitation ratio was 2.1. Bottom, Average trace of 100 consecutive records after 5 min treatment with 8Br-cGMP (30 µM). The facilitation ratio was 1.5. B, Time-dependent plot of the EPSC amplitudes of the same experiments as in A. 8Br-cGMP was bath-applied during the indicated period. C, Amplitude histogram of 100 consecutive EPSCs in B just before the application of 8Br-cGMP. The m was calculated from the occurrence of failure transmissions based on the Poisson statistics and was 0.342. The q was estimated as the mean EPSC divided by m and was 17.1 pA. D, Amplitude histogram of 100 consecutive EPSCs in B during potentiation by 8Br-cGMP. Note the reduction of the occurrence of failure responses. The m was 1.72, and the q was 14.0 pA. E, Effects of 8Br-cGMP on the EPSC and NE-induced potentiation were compared with those of 8Br-cAMP. Each column is the mean of the EPSC amplitude normalized to the mean EPSC amplitude before the application of the cyclic nucleotide analogs. Error bars indicate SEM. The three columns on the left are a summary of eight similar experiments of control, the effect of 100 µM 8Br-cGMP, and the effect of 100 µM 8Br-cGMP plus 10 µM NE. The two columns on the right are a summary of six similar experiments of the effect of 100 µM 8Br-cAMP and the effect of 100 µM 8Br-cAMP plus 10 µM NE. Statistical significance was tested as indicated (paired t test). The difference between the first and the fourth columns was insignificant (p > 0.3, paired t test between raw data).

The site of action of cGMP could be in either the presynaptic terminal or the postsynaptic cell. To distinguish between thesepossibilities, a high concentration of cGMP (0.3 mM) was injectedinto the postsynaptic cell through the recording electrode withan access resistance of <5 M $Omega$ . Ten minutes after the whole-cellconfiguration was established, NE (10 µM) still potentiated theEPSC amplitude by 2.0- to 5.0-fold of the control (n = 4; p >0.1, Mann-Whitney's U test), as was the case without cGMP (Fig.2B). Because the NE-induced potentiation is occluded by 8Br-cGMP(Fig. 3E), the site of action of cGMP appears to bepresynaptic.

Contribution of NO to NE-induced potentiation

These results suggest that NE selectively activates guanylyl cyclase. Two families of guanylyl cyclases have been reported:the soluble guanylyl cyclases, which are activated by NO, andthe particulate guanylyl cyclases, which are anchored to the membraneby a single transmembrane domain (Garbers, 1992). Is NO involvedin the NE-induced potentiation of transmitter release? Even inthe presence of NO synthase inhibitor L-NAME (100 µM, after pretreatmentfor 1-2 hr), NE (10 µM) again potentiated the EPSCs by 2.35 ±0.33-fold (n = 5), which is exactly the same extent as NE alone(p > 0.5, Mann-Whitney's U test). It is expected that extracellularNO scavengers would reduce the intracellular NO, because NO isfreely permeable through the membrane (Garthwaite, 1991). However,even in the presence of 30 µM hemoglobin, NE potentiated the EPSCby 1.5- to 10.8-fold (n = 3), which was the same as in the absenceof hemoglobin (p > 0.2, Mann-Whitney's U test). Does NO itselfpotentiate the transmitter release? To test this, the effectsof the NO donor SNP (100 µM) were examined. As exemplified inFigure 4A, SNP did not potentiate the EPSC even in the presenceof IBMX. The control EPSC was recorded in the presence of 100µM IBMX, and m and q were 2.7 and 10.1 pA, respectively (Fig.4B). The addition of 100 µM SNP did not cause an obvious distortionof the amplitude histogram (Fig. 4C), with m and q of 2.5 and10.6 pA, respectively. In a total of four similar experimentsin the presence of 100 µM SNP, the m was 0.93 ± 0.16 of the control(p > 0.5, paired t test between raw data), the q was 1.02 ± 0.01of the control (p > 0.2, paired t test between raw data), andthe average EPSC was 0.92 ± 0.15 of the control (p > 0.7, pairedt test between raw data). Another potent NO donor, NOR1 (20 µM),failed to potentiate the EPSC even in the presence of 100 µM IBMX(0.88 ± 0.14 of the control; n = 5; p > 0.3, paired t test betweenraw data).

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Figure 4. Effects of NO donor on the transmitter release. A, Time-dependent plot of EPSC amplitudes of a representative experiment. IBMX (100 µM) was present throughout the experiments. The presynaptic oculomotor nerve was stimulated at 0.33 Hz. SNP (100 µM) was bath-applied as indicated (closed bar). B, EPSC amplitude histogram of 100 consecutive records before the application of SNP. The m and the q were estimated from c.v. and were 2.7 and 10.1 pA, respectively. The arrow on the left indicates the occurrence of failures expected from a Poisson distribution. C, EPSC amplitude histogram of 100 consecutive records during the bath application of SNP. The m and the q were 2.5 and 10.6 pA, respectively. The arrow on the left indicates the occurrence of failures expected from a Poisson distribution.

Involvement of PKG

Four types of molecular targets that mediate the intracellular actions of cGMP are present: cGMP-gated channels (Zagotta andSiegelbaum, 1996), a cGMP-activated cAMP PDE (PDE2) (Polson andStrada, 1996), a cGMP-inhibited PDE (PDE3) (Polson and Strada,1996), and a cGMP-stimulated protein kinase (PKG) (Francis andCorbin, 1994). Because the effects of 8Br-cAMP on the transmitterrelease as well as on its potentiation by NE were negligible (Fig.3E), the indirect regulation of cAMP by cGMP is unlikely to bethe mechanism of the NE-induced potentiation. If the activationof cGMP-gated channels is involved in the potentiation of transmitterrelease, a change in the resting [Ca²⁺]_i or the nerve-evoked [Ca²⁺]_i increment ( $Delta$ Ca) would be expected. This notion was tested byexamining the effect of 8Br-cGMP on the Ca²⁺ influx into presynaptic terminals. As shown in Figure 5A, stimulationof the oculomotor nerve increased the intraterminal Ca²⁺ concentration ([Ca²⁺]_i). When eight pulses were applied at 100 Hz, $Delta$ Ca was accumulatedto approximately sevenfold of that by a single pulse (Fig. 5B).Calculations based on these data (n = 11) showed that the $Delta$ Caproduced by eight pulses at 100 Hz was 7.67 ± 0.08-fold of thatproduced by a single pulse, indicating that $Delta$ Ca was almost proportionalto the number of applied pulses in this range. Similarly, thereduction of [Ca²⁺]_o from 1 to 0.6 mM attenuated $Delta$ Ca to 0.63 ± 0.02 of the control(n = 10; Fig. 5C,D). Although [Ca²⁺]_i transients should be much larger and faster in the vicinityof Ca²⁺ channel clusters (Zucker, 1996; Neher, 1998), the volume-averagedfura-2 signal accurately reflects changes in the local concentration(Sinha et al., 1997). These results indicate that this is indeedthe case for the calyx-type terminal and that $Delta$ Ca appears to benearly proportional to the Ca²⁺ influx into the nerve terminal in this range of [Ca²⁺]_o (Yawo, 1999). If 8Br-cGMP increases the exocytotic fusion probabilityby increasing the Ca²⁺ influx during a presynaptic action potential, $Delta$ Ca would be expectedto increase to a value above the $Delta$ Ca at 0.6 mM [Ca²⁺]_o. Actually, 8Br-cGMP had no effect on $Delta$ Ca (Fig. 5C,D). The effectof 8Br-cGMP on the resting [Ca²⁺]_i was also negligible (Fig. 5C; 1.04 ± 0.01 of the control; n= 11; p > 0.2, paired t test between raw data).

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Figure 5. Effects of 8Br-cGMP on the intraterminal Ca²⁺ concentration ([Ca²⁺]_i) of a calyx-type presynaptic terminal of the chick ciliary ganglion. A, Sample record of the [Ca²⁺]_i in response to a single oculomotor nerve stimulation in a solution containing 1 mM [Ca²⁺]_o. The [Ca²⁺]_i was 36 nM before stimulation. B, The same presynaptic terminal was stimulated by eight pulses at 100 Hz in the same solution. The [Ca²⁺]_i was 46 nM before stimulation. C, Effects of 8Br-cGMP on the [Ca²⁺]_i. The same presynaptic terminal was stimulated by eight pulses at 100 Hz in a solution containing 0.6 mM [Ca²⁺]_o before (solid line) and after treatment with 8Br-cGMP (shaded line). During both conditions, the [Ca²⁺]_i was 42 nM before stimulation. D, Summary of the effects of 8Br-cGMP on the nerve-evoked increment of the [Ca²⁺]_i ( $Delta$ Ca). Each column represents the mean of the $Delta$ Ca normalized to that at 1 mM [Ca²⁺]_o before the application of the drugs. Error bars indicate SEM. The columns are summaries of eight series of similar experiments in which the extracellular solution was changed (from left to right) from the control with 1 mM [Ca²⁺]_o, to the 0.6 mM [Ca²⁺]_o solution, to the 0.6 mM [Ca²⁺]_o solution containing 100 µM 8Br-cGMP, to the 0.6 mM [Ca²⁺]_o solution containing 10 µM NE, and to the 0.6 mM [Ca²⁺]_o solution containing 10 µM NE plus 10 µM PA. Note that the effect of 8Br-cGMP was negligible (p > 0.8, paired t test), as was that of NE in the presence of PA (p > 0.7, paired t test), and that the difference was insignificant (p > 0.3, paired t test).

By exclusion, PKG appears to be the most likely candidate. A previous study has demonstrated the presence of PKG in embryonicchick ciliary ganglia (Lengyel et al., 1996). Pretreatment ofthe ganglion with the membrane-permeable PKG inhibitor Rp-8pCPT-cGMPS(100 µM) reduced both the NE-induced potentiation and its enhancementby IBMX (Fig. 6A). Another selective PKG inhibitor, KT5823 (1µM), which occupies the ATP-binding site of PKG (Kase et al.,1987), showed a tendency to suppress NE-induced potentiation.KT5823 evidently inhibited the enhanced adrenergic potentiationin the presence of IBMX (Fig. 6A). These observations indicatethat PKG-dependent phosphorylation of some presynaptic proteinsmust be the major mechanism of the NE-induced potentiation.

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Figure 6. Involvement of PKG-dependent phosphorylation in the NE-dependent potentiation of transmitter release. A, Average effects of PKG inhibitors on the NE-dependent potentiation of EPSC, which is normalized to that just before the application of NE (10 µM). Error bars indicate SEM. The period of application is indicated by an open horizontal bar. The period of application of IBMX (100 µM) is also indicated by a closed horizontal bar. Open circles, In the presence of 0.05% DMSO as control (n = 6); closed circles, in the presence of 1 µM KT5823 (n = 6); closed triangles, in the presence of 100 µM Rp-pCPT-cGMPS (n = 6). The inhibition of potentiation was statistically significant (*p < 0.05; Mann-Whitney's U test) as indicated. B, Comparison between NE-induced potentiation and PKC-dependent potentiation. Each column shows the mean of the relative effect on the EPSC amplitude of the test substances (from left to right): the effect of a phorbol ester (PMA, 0.1 µM, n = 7), the effect of NE (10 µM; n = 8), the effect of PMA in the presence of a PKC inhibitor, BIS (10 µM; n = 7), and the effect of NE in the presence of BIS (n = 7). Error bars indicate SEM. Statistical significance was tested as indicated (Mann-Whitney's U test). The difference between the first and the third columns was significant (p < 0.001, Mann-Whitney's U test), whereas the difference between the second and the fourth columns was insignificant (p > 0.2, Mann-Whitney's U test).

In this calyx-type presynaptic terminal the activation of protein kinase C (PKC) also potentiates transmitter release by upregulatingthe Ca²⁺ sensitivity of exocytosis with negligible effects on the Ca²⁺ dynamics (Yawo, 1999). Could NE potentiate transmitter releaseby activating PKC? As reported previously (Yawo, 1999), the EPSCwas potentiated by a phorbol ester (PMA, 0.1 µM) to a similarextent as by NE (Fig. 6B). The PMA-induced potentiation was completelysuppressed by the PKC-selective inhibitor BIS (10 µM), whereasthe NE-induced potentiation was not antagonized by BIS (Fig. 6B).Therefore, activation of PKC does not seem to be involved in theNE-inducedpotentiation.

Subcellular mechanisms of cGMP-induced potentiation

As previously reported (Yawo, 1996), NE significantly reduced the $Delta$ Ca (n = 8; p < 0.02; paired t test), and this effect wascompletely reversed by the $alpha$ ₁- and $alpha$ ₂-adrenergic receptor antagonistphentolamine (PA) (Fig. 5D) or by the $alpha$ ₂-adrenergic receptor antagonistyohimbine. This leads to the conclusion that NE upregulates theexocytotic mechanism other than Ca²⁺ influx or Ca²⁺ buffering and removal. Because 8Br-cGMP exhibited negligibleeffects on both the $Delta$ Ca and the resting [Ca²⁺]_i, it might potentiate EPSCs through the same mechanism as thatof NE. When the presynaptic oculomotor nerve was stimulated bytwin pulses at short intervals, the second EPSC was, on average,lager than the first EPSC (Figs. 1A, 3A). The mechanism of pairedpulse facilitation (Martin and Pilar, 1964b; Yawo, 1999) has beenattributed to the enhancement of the exocytotic fusion probabilityas a result of residual Ca²⁺ in the presynaptic terminal (Katz and Miledi, 1968; Zucker, 1996;Neher, 1998). In fact, the paired pulse facilitation was accompaniedby an increase in m with a negligible change in q (H. Yawo, unpublishedobservation). With a pulse interval of 40 msec, the ratio of thesecond EPSC amplitude to the first one (paired pulse ratio) was1.94 ± 0.12 at 1 mM [Ca²⁺]_o and 5 mM [Mg²⁺]_o (n = 5), whereas it was 1.07 ± 0.18 at 2 mM [Ca²⁺]_o and 4 mM [Mg²⁺]_o (n = 6). Because the size of the readily releasable pool ofsynaptic vesicles is limited, maneuvers that increase the probabilityof vesicular exocytosis would reduce the paired pulse ratio (Debanneet al., 1996; Schultz, 1997; Yawo, 1999). NE also reduced thefacilitation ratio with a time course similar to that of EPSCpotentiation (Fig. 1A). After the NE-induced potentiation, thepaired pulse ratio was 1.52 ± 0.16 at 1 mM [Ca²⁺]_o and 5 mM [Mg²⁺]_o (n = 5; p < 0.001, paired t test) and 0.74 ± 0.16 at 2 mM [Ca²⁺]_o and 4 mM [Mg²⁺]_o (n = 6; p < 0.01, paired t test). Because 8Br-cGMP also decreasedthe paired pulse ratio (Fig. 3A; 0.81 ± 0.06 of the control; n= 13; p < 0.005, paired t test between raw data), cGMP appearsto upregulate the exocytotic fusion probability of synaptic vesicles(Debanne et al., 1996; Schultz, 1997; Yawo, 1999). Therefore,with respect to the subcellular mechanism, the 8Br-cGMP-inducedpotentiation was indistinguishable from the NE-induced potentiation(Yawo, 1996).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Intracellular signal transduction mechanisms of the NE-induced potentiation of transmitter release

The data presented here revealed the following five main properties of the NE-induced potentiation: (1) NE potentiated thequantal transmitter release in a manner resistant to both $alpha$ ₁-, $alpha$ ₂- and $beta$ -adrenergic receptors (Fig. 1); (2) the NE-induced potentiationwas further enhanced by IBMX, a nonspecific PDE inhibitor or zaprinast,an inhibitor of cGMP-selective PDE, whereas it was unaffectedby Ro-20-1724, an inhibitor of cAMP-selective PDE (Fig. 2); (3)exogenously applied cGMP potentiated the quantal transmitter releaseand occluded the NE-induced potentiation, whereas the effectsof the cAMP analog were negligible (Fig. 3); (4) the NE-inducedpotentiation was resistant to both NO synthase inhibitor and NOscavenger, and the NO donors could not potentiate the transmitterrelease (Fig. 4); and (5) the NE-induced potentiation as wellas its enhancement by IBMX was antagonized by two PKG inhibitorswith different modes of action (Fig. 6). The negligible effectsof IBMX and zaprinast in the absence of NE indicate that theireffect was specific to PDE. Because the NE-induced potentiationwas not occluded by the intracellular injection of high cGMP intothe postsynaptic cell, cGMP appears to be generated in the presynapticterminal. The negligible effects of cAMP on the transmitter releaseindicate that the indirect regulation of cAMP by cGMP is unlikelyto be the mechanism of the NE-induced potentiation. Because bothNE-induced potentiation and cGMP-dependent potentiation were notaccompanied by a change in the resting [Ca²⁺]_i and $Delta$ Ca, the activation of cGMP-gated channels appears notto be the mechanism of the potentiation. Experiments using posthatchedchicks showed that LTP of the ciliary ganglion synapse was inhibitedby L-NAME (100 µM) and induced by SNP (100 µM) (Lin and Bennett,1994). It is unclear where this difference comesfrom.

In summary, all the present results indicate that NE drives the following series of reactions in the calyx-type presynapticterminals of embryonic chick ciliary ganglion: (1) NE binds tothe receptor, which activates NO-insensitive guanylyl cyclases;(2) accumulation of cGMP activates PKG; and (3) PKG phosphorylatesa target protein, which may be involved in the exocytosis of synapticvesicles. Therefore, the receptor involved in the presynapticpotentiation is different from any known catecholamine receptorsubtypes in terms of the signal transduction mechanisms as wellas the pharmacological properties. Although this receptor pharmacologicallyresembles the " $gamma$ -adrenergic receptor" reported in arterial smoothmuscle cells (Hirst et al., 1982; Benham and Tsien, 1988), themolecular identity is unclear. It also remains unknown how thisreceptor activates guanylylcyclases.

Mechanisms involved in NE-, cGMP-, and PKG-dependent potentiation

In many synapses including the chick calyx-type synapse, the magnitude of the paired pulse ratio is negatively correlatedwith m of the first response (Debanne et al., 1996; Schulz, 1997).The most plausible mechanism seems to be a depletion of dockedvesicles for the second release (Debanne et al., 1996; Doburunzand Stevens, 1997; O'Donovan and Rinzel, 1997; Yawo, 1999). Inthe present results, the NE-induced potentiation accompanied thereduction of the paired pulse ratio (Fig. 1A). It is likely thatNE increased the exocytotic fusion probability in the first presynapticrelease, depleting the available vesicles for the second release.The results of the paired pulse experiments are consistent withthe notion that NE enhances the Ca²⁺ sensitivity of the exocytotic fusion probability because it doesnot increase the Ca²⁺ influx (Yawo, 1996).

Because this report fills the missing link between NE and the potentiation of transmitter release, cGMP and PKG might upregulatethe Ca²⁺ sensitivity of exocytotic fusion probability. This notion isconsistent with the observation that the membrane-permeable cGMPanalog 8Br-cGMP enhanced m without increasing $Delta$ Ca (Fig. 5). Therefore,the cGMP-dependent potentiation was accompanied by no detectablechanges in net Ca²⁺ influx, buffering, or removal. In addition, the reduction ofthe paired pulse ratio by 8Br-cGMP strongly suggests that theexocytotic fusion probability was enhanced. The same mechanismappears to be upregulated by PKC, because NE was ineffective afterPKC-dependent potentiation and vice versa (H. Yawo, unpublishedobservation). Although the precise molecular target is unknown,this modulation might involve phosphorylation of the intracellularCa²⁺ sensor molecule itself or a molecule interacting with the Ca²⁺ sensor (Yawo, 1999).

  FOOTNOTES

Received Feb. 22, 1999; revised April 12, 1999; accepted April 20, 1999.

This work was supported by grants-in-aid from the Ministry of Education, Science and Culture of Japan and the Yamanouchi Foundationfor Research on Metabolic Disorders. I thank S. Sai for technicalsupport, Drs. T. Abe, K. Kawa, and M. Umemiya for comments onthis manuscript, and B. Bell for reading this manuscript. A reviewby Dr. M. Kuno is gratefullyacknowledged.
Correspondence should be addressed to Dr. Hiromu Yawo, Department of Neurophysiology, Tohoku University School of Medicine,Sendai 980-8575,Japan.

  REFERENCES

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MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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