Peptidergic Modulation of Synaptic Transmission in the Parabrachial Nucleus In Vitro: Importance of Degradative Enzymes in Regulating Synaptic Efficacy

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Volume 16, Number 19, Issue of October 1, 1996 pp. 6046-6055
Copyright ©1996 Society for Neuroscience

Peptidergic Modulation of Synaptic Transmission in the Parabrachial Nucleus In Vitro: Importance of Degradative Enzymes in Regulating Synaptic Efficacy

Tarek M. Saleh¹, Samuel B. Kombian¹, Jeffrey A. Zidichouski¹^,², and Quentin J. Pittman¹
¹ Neuroscience Research Group, University of Calgary, and ² Ciba-Geigy Canada Limited, Calgary, Alberta, Canada T2N 4N1

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

This study examined the effects of substance P (SP) and calcitonin gene-related peptide (CGRP) on synaptic transmission in a pontine slice containing the parabrachial nucleus (PBN). Stimulation of the ventral, external lateral portion of the PBN elicited glutamate-mediated EPSCs in cells recorded using the nystatin perforated-patch recording technique in the external lateral, external medial, and central lateral subnuclei of the PBN. Bath application of SP or CGRP dose-dependently and reversibly attenuated the evoked EPSC. The attenuation of the EPSC induced by both of these peptides was not accompanied by changes in input resistance of PBN cells over a wide voltage range, nor did these peptides alter the inward current induced by a brief bath application of AMPA. The combined application of subthreshold concentrations of these peptides revealed a synergistic interaction in reducing the evoked EPSC. The substance P neurokinin-1 receptor antagonist CGP49823 completely and reversibly blocked both the SP- and the CGRP-induced attenuation of the EPSC. However, the rat CGRP receptor antagonist human-CGRP_8-37 did not block the actions of CGRP or SP on the EPSC. Using a metabolically stable analog of SP, SP(5-11), or an endopeptidase inhibitor, phosphoramidon, we were able to demonstrate that CGRP enhances the SP effect by inhibiting an SP endopeptidase. Application of phosphoramidon also revealed an endogenous SP ``tone'' apparently made effective by blockade of the endopeptidase. These results suggest that SP (and CGRP indirectly through an inhibition of the SP endopeptidase) acts on presynaptic NK-1 receptors to cause an inhibition of excitatory transmission in the PBN. These results indicate an important role of endopeptidases in regulating synaptic modulation by peptides.
Key words: visceral afferent pathway; CGP49823; synergism; presynaptic modulation; nystatin-patch recording; endopeptidase; phosphoramidon; substance P; calcitonin gene-related peptide

INTRODUCTION
Visceral afferent information is known to reach the CNS via the vagus nerve, which projects to an important brainstem nucleus, the nucleus of the solitary tract (NTS). The NTS, in turn, relays this information via a direct projection to the parabrachial nucleus (PBN), which is also an obligatory synapse between the NTS and the thalamus (Saleh and Cechetto, 1994) in the relay of visceral information destined for the sensory cortex. Although synaptic transmission through the PBN appears to be glutamatergic in nature (Zidichouski and Jhamandas, 1993; Saleh and Cechetto, 1994; Zidichouski et al., 1996), previous work in vivo has also revealed peptidergic modulation of visceral information passing through the PBN en route to the thalamus (Saleh and Cechetto, 1993). In studies involving the microinjection of SP and CGRP into the PBN while recording the vagally evoked neuronal response in the thalamus, both SP and CGRP were shown to act synergistically to inhibit the flow of glutamatergic transmission through the PBN in vivo (Saleh and Cechetto, 1993, 1995). Also, Mantyh and Hunt (1985) demonstrated substance P (SP)- and calcitonin gene-related peptide (CGRP)-immunoreactive fibers and terminals located in nuclei along the visceral afferent pathway. Similarly, binding sites for both of these peptides have been localized to the PBN (SP, Quirion et al., 1983; CGRP, Kruger et al., 1988).
Peptidergic modulation of visceral afferent transmission in the PBN may provide a means for selectively controlling the flow of modality-specific visceral information in the CNS. In fact, immunohistochemical evidence has demonstrated that the intensity of SP and CGRP staining in subnuclei of the PBN is changed significantly in response to loading and unloading of the aortic baroreceptors but not to gastrointestinal stimulation (Saleh and Cechetto, 1996). In light of the critical role of the PBN in controlling the flow of visceral information to higher central areas, as well as a variety of studies pointing to the possible role of this nucleus in modifying response patterns to visceral stimuli (Saleh and Cechetto, 1993), the present investigation was performed to determine directly the electrophysiological effects of SP and CGRP on excitatory synaptic transmission in the PBN. Specifically, we sought to determine the identity of the receptor subtypes involved, whether the site of action was pre- or postsynaptic, and to examine more closely the synergistic action of SP and CGRP using the perforated-patch recording technique in an in vitro slice preparation.

MATERIALS AND METHODS
Slice preparation. Sprague Dawley rats (25-40 d old) were anesthetized with halothane and decapitated. The brain was quickly removed and placed in ice-cold, carbogenated (95% CO₂/5% O₂) artificial CSF (ACSF; pH 7.3-7.4). Coronal slices (400 µm thick) were cut with a vibratome from a block of tissue containing the parabrachial nucleus, in cold (4°C), carbogenated ACSF. Pontine slices (bregma $-$ 9.1 to $-$ 9.8 mm; Paxinos and Watson, 1986) containing the PBN were then taken and hemisected along the midline and incubated in ACSF at room temperature (22°C) for at least 1 hr before recording. A slice was then transferred into a 500 µl recording chamber where it was submerged and continuously perfused with prewarmed ACSF (27-29°C) at a rate of 2-3 ml/min. The composition of the ACSF was (in mM): NaCl 126, KCl 2.5, NaH₂PO₄ 1.2, MgCl₂ 1.2, CaCl₂ 2.4, NaHCO₃ 18, glucose 11. To evoke synaptic responses, a bipolar stimulating electrode connected to a stimulus isolation unit was placed ventral-lateral to the PBN, close to the ventral tip of the superior cerebellar peduncle. To examine the spontaneous, miniature EPSCs, bath application of sucrose (30 mM) and TTX (1 µM) was used to enhance and isolate spontaneous, presynaptic events (Bekkers and Stevens, 1989).
Nystatin-patch recording. The perforated (nystatin)-patch whole-cell recording technique was used in this study to avoid the problems of ``washout'' and rundown of responses typically encountered with whole-cell patch recording (Blanton et al., 1989; Hamill et al., 1989; Korn and Horn, 1989). The nystatin-patch recording technique has been shown to provide access to the cell and a low signal-to-noise ratio comparable to that observed with whole-cell recording (Korn et al., 1991; Rae et al., 1991; Meriney et al., 1994). Nystatin-patch recordings from PBN neurons were made with glass micropipettes (Garner Glass; tip resistance 4-8 M $Omega$ ) filled with a solution containing (in mM): K-acetate 120, HEPES 40, MgCl₂ 5, EGTA 10, and 450 µg/ml nystatin in dimethyl sulfoxide (DMSO) and Pluronic F127. High-resistance seals (1-3 G $Omega$ ) were made using an Axopatch 2A patch-clamp amplifier in current-clamp mode (Axon Instruments, Foster City, CA). The amplifier was then placed in the voltage-clamp mode and a $-$ 20 mV step (100 msec duration) was applied to monitor the partitioning of nystatin into the membrane. Access to the cell (series resistance 15-25 M $Omega$ ) was attained in 1-15 min after seal formation.

Data acquisition and analysis. After attaining access to the cell, the amplifier was switched back to the current-clamp mode and the resting membrane potential was recorded. Action potentials were generated by continuous current injection (+10 to +50 pA) and were sampled using pClamp programs (Axon Instruments) to characterize the cells. All cells that satisfied the established criterion of having an action potential amplitude exceeding 90 mV (from peak to trough) were then voltage-clamped at $-$ 65 mV (V_h). All current responses were filtered at 1 or 3 kHz; because currents were small and of slow duration, no compensation for series resistance was done. Synaptic currents were evoked by applying single pulses via bipolar stimulating electrodes ( $<=$ 10 V, 10-20 µsec), and a stimulus intensity that yielded a response 50-60% of the maximum response was used for the remainder of the experiment. Three successive synaptic samples were taken 10 sec apart, digitally averaged, and stored for analysis. In all synaptic current experiments, a $-$ 20 mV, 50 msec square pulse was applied 100 msec after synaptic stimulation to monitor input and series/access resistance. Current-voltage relationships (I-V curves) were generated by applying 200 msec step, square voltage pulses from V_h to $-$ 120 through to $-$ 20 mV (in 10 mV increments) or by applying slow voltage ramps and recording the corresponding steady-state current. To produce the ramp I-V curve, the voltage was gradually ramped to $-$ 120 mV over a 2 sec period, then ramped (over ~18 sec) to $-$ 5 mV and then back to $-$ 65 mV (V_h). In addition to the computer-assisted pClamp data acquisition, continuous records of membrane potentials and currents were made on a pen chart recorder (Gould 2400S).

All acquired data were analyzed off-line using pClamp programs and a 386 PC. All data were corrected for any electrode offset observed at the end of each recording session. Input resistances for all cells were estimated from the step I-V protocol by determining the difference of the steady-state current (measured at ~150 msec into the pulse) at $-$ 70 and $-$ 50 mV. The amplitude of the EPSC was taken as a measure of the magnitude of synaptic strength. Data are expressed either as means of actual currents or as mean percentage change from control values ± SEM. Cells served as their own controls, and only cells that showed significant recovery (>85%) from any drug effect (except in TTX experiments) were included in the analysis. Statistical comparisons were performed on raw data using the Student's t test or one-way ANOVA (p $<=$ 0.05 was considered significant).

All drugs were bath-applied by perfusion with ACSF containing the final concentration of the drug. Appropriate stocks were made and diluted with ACSF just before application. Drugs used were 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX), AMPA hydrobromide (both from RBI); SP(5-11), CGRP, and HCGRP (rat CGRP receptor antagonist) (from Bachem); CGP49823 (NK-1; SP receptor antagonist) was a kind gift from Dr. Felix Brugger (Ciba-Geigy Limited); Pluronic F127 was from BASF Wyandotte, and bicuculline, TTX, nystatin, phosphoramidon, and all of the salts in the ACSF were obtained from Sigma (St Louis, MO). Stock solutions of CNQX, AMPA, SP, CGRP, and the NK-1 and CGRP antagonists were aliquoted and then frozen at $-$ 20°C.

RESULTS
All neuronal recordings obtained in this study (n = 79) were located in the dorsal, central, and external lateral aspect of the PBN. All cell characteristics recorded in the present study were comparable to those described previously by Zidichouski and Jhamandas (1993). Resting membrane potentials were $-$ 53 to $-$ 73 mV (mean $-$ 63 ± 3.5 mV), and estimated input resistances were 494-775 M $Omega$ (635 ± 38 M $Omega$ , n = 58). Stimulus intensity-dependent EPSCs could be evoked in 79% of cells; this EPSC was mediated predominantly by the non-NMDA receptor subtype, because CNQX (10 µM) reduced it by 93 ± 2% (n = 12). All EPSCs were abolished by bath application of TTX (1 µM; reduced by 96.5 ± 0.2%; n = 22). All experiments were performed in the presence of bicuculline (25 µM) to eliminate the possibility of GABA_A-mediated IPSC contamination, even though only glutamate-mediated EPSCs were recorded at V_h because bicuculline (25 µM; n = 8) had little effect on the amplitude of the EPSC (reducing it by 5 ± 1%).
Substance P- and CGRP-related peptide reduce the amplitude of the EPSC
In experiments on 19 different cells, bath application of SP (0.03-10 µM) in voltage clamp caused a reversible, concentration-dependent decrease in the evoked EPSC with an estimated EC₅₀ of 0.75 µM and a maximal effect at 5 µM (Fig. 1A1,A2). Figure 1A1 shows a typical example of an EPSC recorded in control and in the presence of 5 µM SP and the recovery after a 10 min washout. The onset of this effect was observed ~1 min after application of SP to the bath, with a peak effect observed after 2-3 min. This SP-induced (10 µM) blockade of the EPSC was repeatable using multiple applications in the same cell (there was no evidence of desensitization). Similarly, bath application of CGRP (2.5-10 µM; n = 16) in voltage clamp caused a reversible, concentration-dependent decrease in the evoked EPSC with an estimated EC₅₀ of 6.25 µM and a maximal effect observed at 10 µM (Fig. 1B1,B2). Figure 1B1 shows a typical example of an EPSC recorded in control, in the presence of 10 µM CGRP and the recovery after 10 min washout. The time taken to observe the onset and peak effects was similar to that for SP and, again, there was no evidence of desensitization with multiple application of CGRP.
Fig. 1. Effects of the peptides substance P (SP) and calcitonin gene-related peptide (CGRP) on EPSC responses in the PBN. In this and all subsequent figures, stimulus intensities were in the range of 0.2-2.0 V, intensities that yielded EPSC responses 50-60% of maximum. A1, The synaptic response of a PBN neuron in voltage-clamp experiments (V_h = $-$ 65 mV). SP (5 µM) attenuated the evoked EPSC with no change in input resistance as monitored by a 20 mV, 50 msec hyperpolarizing pulse. A2, Dose-dependent attenuations in the EPSC amplitude with an estimated EC₅₀ of 0.75 µM (n = 4-9 cells at each dose). B1, In the same cell (V_h = $-$ 65 mV), CGRP (10 µM) attenuated the EPSC with no change in input resistance as monitored by a 20 mV, 50 msec hyperpolarizing pulse. B2, Dose-dependent attenuations in the EPSC amplitude with an estimated EC₅₀ of 6.25 µM (n = 4-9 cells at each dose).
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Attenuation of the EPSC is not postsynaptic
Under voltage clamp, steady-state I-V curves were generated and showed that those taken in control (TTX only) were superimposable on those taken in the additional presence of SP (1-10 µM) or CGRP (10 µM) over the voltage ramp tested ( $-$ 120 to $-$ 5 mV; n = 6 for each peptide; data not shown). The possible postsynaptic action of the peptides was also investigated by bath application of AMPA (2.5 µM in TTX for 20 sec) alone or in combination with 10 µM SP or CGRP. The magnitude of the AMPA response was not changed significantly in the presence of SP (8 ± 3% from control; n = 4) or CGRP (6 ± 2% from control; n = 4). Taken together, these results suggest that the effect of SP on synaptic transmission is not postsynaptically mediated.
SP and CGRP effects are not polysynaptic
To rule out possible polysynaptic pathways in the actions of the peptides, we decided to test whether either of these peptides affected the appearance of mEPSCs in voltage clamp. In 4 cells voltage-clamped at $-$ 65 mV and bathed in sucrose (30 mM) and TTX (1 µM) to eliminate action potential-driven EPSCs, bath application of either SP or CGRP reduced, in a reversible manner, the frequency of mEPSCs (by 69 ± 6 and 65 ± 5%, respectively; cutoff 8 pA). At the end of each experiment, we verified that the mEPSCs were non-NMDA receptor-mediated by completely blocking them with CNQX (20 µM).
The CGRP-induced effects on the EPSC are not mediated by a classical CGRP receptor
To characterize further the CGRP-induced effect on the EPSC, the selective and reversible rat CGRP receptor antagonist HCGRP (Mimeault et al., 1991) was bath-applied in the presence of CGRP. HCGRP (100 µM) alone had no effect on the evoked EPSC or on the membrane conductance [Fig. 2 (1)], nor did it block the CGRP-induced (5 µM) attenuation of the evoked EPSC [n = 4; Fig. 2 (2, 3)].
Fig. 2. Effect of the CGRP receptor antagonist human-CGRP_8-37 (HCGRP) on CGRP actions. 1, Application of HCGRP alone does not affect the size of the evoked EPSC. 2, The reduction in the amplitude of the EPSC produced by application of an EC₅₀ dose of CGRP (5 µM), which is not significantly affected by the CGRP receptor antagonist (HCGRP; 100 µM; 3).
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The SP- and CGRP-induced synaptic depression is blocked by the NK-1 receptor antagonist
Because SP has been shown to act at NK-1 receptors, we examined the effect of a selective and reversible NK-1 receptor antagonist, CGP49823 (5-100 µM), on the SP-induced attenuation of the EPSC. Bath application of CGP49823 (n = 12) alone had no effect on the evoked EPSC or on the membrane conductance because no change in resting current at V_h was observed (data not shown). The SP-induced (1 µM) attenuation of the EPSC was completely abolished in the presence of CGP49823 at concentrations of >20 µM [n = 4 at each concentration; Fig. 3A1-A4 (left), B].
Fig. 3. Blockade of SP- and CGRP-induced synaptic depression with the NK-1 receptor antagonist CGP49823. CGP49823 attenuated and, at higher concentrations, blocked the inhibition of the evoked EPSC induced by SP (1 µM, left) and CGRP (5 µM, right) in the same cell (A1-A4, B). Application of CGP49823 (5-100 µM) alone had no observable effect on the EPSC (data not shown). B, A graph illustrating that the inhibitory effects of SP (1 µM) or CGRP (5 µM) are blocked in an identical manner by CGP49823 at all concentrations used (n = 4 at each concentration for each peptide). Bars represent mean ± SEM.
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In testing the selectivity of CGP49823 for the SP NK-1 receptor, we examined whether it would affect the CGRP response. Surprisingly, the CGRP (5 µM)-induced blockade of the EPSC was completely, and reversibly, attenuated by coapplication of CGP49823 at concentrations of >20 µM [n = 4 at each concentration; Fig. 3A1-A4 (right), B] in a manner identical to that seen with SP. However, in the converse experiment, application of HCGRP did not significantly change the SP-induced attenuation (1 µM) of the EPSC (data not shown).

We tested the specificity of the NK-1 receptor antagonist for the NK-1 receptor in blocking the SP- or CGRP-induced decrease of the EPSC. In voltage-clamp experiments (n = 8), dose- response curves for SP and CGRP were generated alone and in the additional presence of the NK-1 receptor antagonist at three concentrations (10, 25, and 50 µM; Fig. 4A1,B1). In the presence of the NK-1 receptor antagonist, the SP dose-response curves were shifted to the right (Fig. 4A1). Using the estimated ED₅₀ of each dose-response curve, we constructed Schild plots for each peptide using the equation log(dr $-$ 1) = log[B] $-$ log K_B (Kenakin, 1987). The slope of the Schild plot is ~1.1 for SP, which indicates that CGP49823 is a competitive antagonist of the SP NK-1 receptor (Fig. 4A2). In contrast, the slope of the Schild plot constructed for CGRP is ~0.65, which is significantly different from 1.0; this indicates that CGP49823 may interact in a noncompetitive manner with CGRP at the NK-1 receptor (Fig. 4B2) or that CGRP is acting on a heterogeneous receptor population.
Fig. 4. The CGP49823 block of the SP- and CGRP-induced effects show different pharmacological profiles. A1, Dose-response curves for SP alone and in the presence of CGP 49823 at three concentrations (10, 25, and 50 µM). The ED₅₀ values of all curves were estimated and used to calculate the dose ratio that was used for Schild plots. A2 shows the Schild plots obtained from these estimates with a slope of 1.1, indicating competitive antagonism between SP and CGP49823 at the NK-1 receptor. B1, CGRP dose-response curves in control (CGRP alone) and in the presence of CGP 49823 under the same conditions as in A. B2 shows the Schild plot obtained for the CGRP-CGP49823 interaction. The slope of 0.65 indicates a noncompetitive antagonism.
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SP and CGRP interaction
Bath application of a threshold dose of SP (0.05 µM) reduced the magnitude of the EPSC by only 5 ± 2% (n = 9; Fig. 5B,E). Similarly, in the same cells, bath application of a threshold concentration of CGRP (0.1 µM) reduced the magnitude of the EPSC by only 2 ± 2% (n = 9; Fig. 5A,E). However, coapplication of SP and CGRP at their respective threshold concentrations reduced the amplitude of the EPSC by 27 ± 9% (n = 4; Fig. 5C,E). Furthermore, this synergistic reduction in the EPSC amplitude was reversibly blocked by the NK-1 antagonist CGP49823 [10 µM (n = 5; data not shown) or 100 µM (n = 4); Fig. 5D]. In addition, this synergism with a subthreshold concentration of CGRP (0.1 µM) was observed along the entire dose range of SP used (0.05-10 µM; Fig. 5E; n = 4).
Fig. 5. Synergistic interaction between SP and CGRP on the magnitude of the EPSC. A and B illustrate the effect of subthreshold doses of CGRP (0.1 µM) and SP (0.05 µM), respectively, on the evoked EPSC. C, Combined application of both peptides at these concentrations resulted in an attenuation of the EPSC amplitude. D, This synergistic interaction on the evoked EPSC by coapplication of SP and CGRP was reversibly blocked by CGP49823 (100 µM). E, The synergism between SP and CGRP can be seen at all doses along the dose-response curve for SP (n = 4 at each dose).
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An interesting mechanism of interaction for SP and CGRP is suggested by in vitro observations that CGRP competes for the neutral endopeptidase responsible for SP degradation (Le Greves et al., 1985). Therefore, to determine whether this was a possible mechanism for the interaction between SP and CGRP in our study, we used the metabolically stable methylester analog of SP, SP(5-11) (Urban et al., 1994). Bath application of SP(5-11) produced a dose-response curve that had an estimated ED₅₀ of 0.1 µM (Fig. 6A; ~10-fold more potent than SP; n = 4). This curve, in contrast to the SP dose-response curve, was not affected by the additional presence of CGRP (0.1 µM) along the entire concentration range of SP(5-11) used (Fig. 6A; n = 4).
Fig. 6. CGRP reduces the EPSC by inhibiting an SP endopeptidase. A, Dose-response curve generated by application of several doses of the metabolically stable methylester analog of SP, SP(5-11). This dose-response curve is unaffected by coapplication of CGRP (0.1 µM; n = 3 or 4 cells for each point). B1, Addition of the SP endopeptidase inhibitor phosphoramidon (10 µM) attenuates the amplitude of the EPSC by 89 ± 3% (peak effect). B2, This phosphoramidon-induced effect on the EPSC is blocked by the NK-1 antagonist. B3, Addition of phosphoramidon (5 µM) attenuates the amplitude of the EPSC by 68 ± 3% (peak effect), and the addition of CGRP (1 µM) enhances this effect by 14 ± 5% (peak effect; n = 3 to 4 for each point). B4, Bar graph summarizing the effects of the NK-1 receptor antagonist and CGRP (1 µM) in the presence of phosphoramidon (10 and 5 µM) on the magnitude of the EPSC.
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A second way to test the hypothesis that CGRP was interacting with an SP endopeptidase was to bath-apply a neutral endopeptidase inhibitor, phosphoramidon (10 µM; Fig. 6B) (Chiba and Misawa, 1995) to the slice, which reduced the amplitude of the EPSC by 89 ± 3% (n = 4; Fig. 6B1). The phosphoramidon-induced synaptic depression was blocked by the NK-1 receptor antagonist CGP49823 (100 µM; Fig. 6B2; n = 4), suggesting a tonic release of SP. Coapplication of CGRP (0.1 µM) with phosphoramidon (10 µM) did not further enhance the phosphoramidon-induced attenuation of the EPSC (n = 4; Fig. 6B3,B4). However, when the phosphoramidon concentration was lowered to 5 µM, the EPSC was attenuated (68 ± 3%; n = 4; Fig. 6B3), and this attenuation in the EPSC was reduced further by CGRP (by 14 ± 5%; giving a combined attenuation of 82 ± 5%; Fig. 6B3,B4).

DISCUSSION
The results of this study demonstrate that the peptides SP and CGRP reversibly depress excitatory synaptic transmission in the PBN in a dose-dependent manner in vitro. The data presented here are consistent with the conclusion that the inhibitory effects of SP occur via presynaptically located NK-1 receptors. The mechanism of the CGRP-induced attenuation of the EPSC appears to be through a novel mechanism involving competition for an SP degrading enzyme, the neutral endopeptidase, to increase the availability of SP.
SP and CGRP act presynaptically to reduce EPSCs
The dose-dependent, potent actions of SP and CGRP on the evoked EPSC most likely have a presynaptic locus of action. These peptides had no postsynaptic actions on input resistance, on holding current at $-$ 65 mV, or on currents generated by a voltage ramp between $-$ 120 and $-$ 5 mV. An interaction with the postsynaptic AMPA receptors underlying excitatory transmission in the area (Zidichouski et al., 1996) also appears unlikely, because currents elicited by exogenously applied AMPA were unaffected in the presence of maximal concentrations of the peptides. Thus, although we cannot rule out additional postsynaptic actions, evidence supports a presynaptic locus. This is consistent with observations in other brain areas of a presynaptic action of SP (Shapiro and Hille, 1993; Len et al., 1994; Tremblay et al., 1994) and CGRP (Schworer et al., 1991; Nuki et al., 1994). Additional anatomical evidence supporting a presynaptic action would be the localization of receptors on presynaptic terminals in the PBN; although autoradiographic studies have identified receptors for both SP (Quirion et al., 1983) and CGRP (Kruger et al., 1988) in the PBN, the cellular locus for them has not been identified. Such a localization on a presynaptic terminal would also eliminate the possibility that these peptides are acting on interneurons that, via release of another transmitter, presynaptically inhibit glutamate release from the excitatory afferents activated in this experiment. However, it is unlikely that there is a GABAergic intermediary because bath application of SP(5 µM) caused an equal attenuation in the size of the EPSC as that reported in this paper, even in the additional presence of the GABA_B receptor antagonist CGP36742 (data not shown).
Do SP and CGRP act at the same receptor?
Dose-response studies of the peptide effects on the EPSC revealed classical sigmoid-shaped curves for both peptides. It was interesting that the EC₅₀ for SP was ~10-fold lower than that for CGRP, raising the possibility that the CGRP has a much lower affinity for its receptor than does SP. To investigate more thoroughly the receptors mediating the effects on the EPSC, we used receptor antagonists to block the peptide actions. SP is thought to act on the NK-1 receptor, and when the slice was pretreated with the NK-1 receptor antagonist, we found that it displaced the dose-response curve for SP to the right in a dose-dependent manner. Based on these data, we constructed a Schild plot, which enabled us to conclude that the shift was attributable to a competitive action by the antagonist at the NK-1 receptor.
In contrast to what was seen with SP, CGRP action on the EPSC was not antagonized by the specific rat CGRP antagonist HCGRP. Because there is evidence in the literature for another, yet unidentified CGRP receptor (Dennis et al., 1990), such a receptor could be mediating or contributing to the inhibitory effects of CGRP on synaptic transmission.

The observation that the CGRP-induced inhibition of the evoked EPSC was completely and reversibly blocked by the NK-1 receptor antagonist CGP49823, but not a by specific CGRP receptor antagonist, raises the alternate possibility that the CGRP effect may involve SP which, in turn, acts at NK-1 receptors to inhibit neurotransmitter release. This is supported by the observation that the blockade of CGRP effect by CGP49823 was identical to that of SP at each of six concentrations of the antagonist tested. Nonetheless, when Schild plots were carried out on the CGRP-NK-1 antagonist interaction, the slope of the line was significantly less than 1, indicating that something other than a competitive interaction with only this NK-1 receptor underlies this antagonism. The complexity of the CGRP-CGP49823 interaction is underlined further by the fact that the pA₂ value (estimated as the x-axis intercept from Shild plots in Fig. 5) for the antagonist is different from that calculated for an SP-CGP49823 interaction. We cannot at present fully explain this difference, but it does raise the possibility that there are additional subtypes of receptors responsive to these peptides in the PBN.

SP-CGRP interactions
Additional evidence that the action of CGRP may involve an SP-dependent mechanism comes from our results indicating that the SP inhibitory action on the EPSC can be potentiated by a subthreshold dose of CGRP. Because this action of CGRP potentiating SP can be blocked by the NK-1 antagonist, how might it be working? One possibility is that CGRP stimulates the release of SP by acting at a novel CGRP receptor not susceptible to antagonism by the CGRP antagonist HCGRP. A second possibility is that CGRP may not be acting via a ``classical receptor,'' and a mechanism for its action is suggested by previous findings (Le Greves et al., 1985; Schaible et al., 1992) that CGRP can interfere with SP degradation by competing with SP for the endopeptidase. This would make more SP available for binding to its receptor and thereby ``potentiate '' its action. If this, indeed, were the case, the action of CGRP would be dependent on an endogenous, tonic SP release in this nucleus. Our observations that the SP receptor antagonist alone had no effect on the size of the EPSC does not provide any evidence for this scenario. However, an endogenous SP release could still be present but not unmasked by the NK-1 antagonist if a very effective endopeptidase action was constantly removing SP from the synapse. This scenario is supported by our experiments using the endopeptidase inhibitor phosphoramidon. Phosphoramidon (10 µM) reduced the amplitude of the EPSC by 89 ± 3%, an effect that was reversed by the NK-1 receptor antagonist. This indicates that SP is tonically released. Furthermore, in these experiments, CGRP was ineffective in enhancing this effect on the EPSC, indicating that phosphoramidon occluded the CGRP effect. However, when the phosphoramidon concentration was lowered to 5 µM and the resulting attenuation of the EPSC was 68 ± 3%, CGRP was able to enhance the synaptic depression by another 14 ± 5%. This result strongly suggests that CGRP requires sufficient functional endopeptidase to affect the EPSC on its own or to enhance the SP effect.
Functional considerations
At the cellular level, we have uncovered evidence for an endogenous release of SP that appears to be functionally ineffective because of the presence of a highly active endopeptidase. If these findings in slice are representative of what is seen in the intact brain, one might question why this seemingly ineffective release of SP should occur. An answer may be found in an understanding of the localization of SP in afferents in the PBN. In the brain and spinal cord, it appears that SP is colocalized with glutamate (Penny et al., 1986; De Biasi and Rustioni, 1988; Copray et al., 1990). While recognizing that release characteristics for amino acids and peptides could be different (Iverfeldt et al., 1989), it is possible that some SP is released concurrently with glutamate. Under basal conditions, it can be appreciated that one might want fidelity of transmission at the glutamergic synapse; concurrent activation of presynaptic SP receptors would interfere with this by reducing the quantity of glutamate released. A highly efficient endopeptidase would prevent this by inactivating the SP coreleased with glutamate (Fig. 7, left). This situation could be different if the afferents are activated at very high frequency, for example, during intense visceral activation; experiments in vivo suggest that under such situations, NMDA receptors underlie the excitatory transmission in the PBN (Saleh and Cechetto, 1994). Given the possible excitotoxic effects of large amounts of glutamate acting at these receptors, it would be advantageous for the coreleased SP to reduce the amount of glutamate released. This could happen if sufficient SP is released to overwhelm the endopeptidase (Fig. 7, right) and thereby permitting SP to bind to the presynaptic receptor. Although such a scenario is speculative, it is open to experimental verification using dialysis monitoring of extracellular glutamate.
Fig. 7. Schematic diagram illustrating the possible actions of SP and CGRP within the PBN. Left, Under basal conditions, the SP coreleased with glutamate is degraded by an efficient (endo)peptidase, preventing it from reaching its presynaptic NK-1 receptor. Thus, sufficient glutamate is released to produce a postsynaptic response (lower trace). Right, Under conditions of excessive afferent input, sufficient SP is released to overwhelm the peptidase, resulting in activation of its receptor. In addition, CGRP similarly released under conditions of high afferent activity increases the availability of SP by competing with it for sites on the endopeptidase. Thus, glutamate release is more profoundly inhibited, and the postsynaptic response is attenuated (lower trace).
[View Larger Version of this Image (23K GIF file)]

The participation of CGRP in this scenario could also be related to a protective action of SP. Cell bodies giving rise to the CGRP-positive afferents in the PBN are thought to lie in the central nucleus of the amygdala (Honkaniemi et al., 1990). There is a population of neurons in the amygdala that are activated under conditions of intense visceral activation (Anton et al., 1991; McKitrick et al., 1993); if there were CGRP-positive cells in this population, release of CGRP in the PBN would add to the effectiveness of the SP in this nucleus by competing for the endopeptidase (Fig. 7, right). Whatever the relevance of this interaction to the physiological state, it points to the care that must be taken in interpreting the action of certain peptides on cellular responses.

FOOTNOTES

Received April 3, 1996; revised June 14, 1996; accepted July 18, 1996.

This work was supported by the Heart and Stroke Foundation of Canada. T.M.S. was supported by postdoctoral fellowships from the Alberta Heritage Foundation for Medical Research (AHFMR), S.B.K. was supported by a Medical Research Council (MRC; Canada) Centennial Fellowship, and Q.J.P. was supported by an MRC and AHFMR Senior Scientist Award. We thank Ciba-Geigy Limited for the generous gift of the NK-1 receptor antagonist and Drs. Brian MacVicar and Morley Hollenberg for their comments on this manuscript.

Correspondence should be addressed to Tarek M. Saleh, Neuroscience Research Group, Faculty of Medicine, University of Calgary, Calgary, Alberta, Canada, T2N 4N1.

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