Inhibition of Synaptic Transmission by Neuropeptide Y in Rat Hippocampal Area CA1: Modulation of Presynaptic Ca2+ Entry

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Volume 17, Number 21, Issue of November 1, 1997 pp. 8169-8177
Copyright ©1997 Society for Neuroscience

Inhibition of Synaptic Transmission by Neuropeptide Y in Rat Hippocampal Area CA1: Modulation of Presynaptic Ca²⁺ Entry

Jing Qian¹, William F. Colmers², and Peter Saggau¹
¹ Division of Neuroscience, Baylor College of Medicine, Houston, Texas 77030, and ² Department of Pharmacology, University of Alberta, Edmonton, Canada T6G 2H7

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Neuropeptide Y (NPY) agonists inhibit glutamate release by a presynaptic action at the CA3-CA1 synapse of rat hippocampus.We have examined the relationship between [Ca_pre]_t via presynaptic,voltage-dependent calcium channels (VDCCs), measured opticallyby using the fluorescent calcium indicator fura-2, and transmitterrelease, measured electrophysiologically. Activation of presynapticNPY Y₂ receptors reduced [Ca_pre]_t and thereby inhibited synaptictransmission. Multiple calcium channels are involved in synaptictransmission at this synapse. Activation of Y₂ receptors inhibitsN-type, P/Q-type, and unidentified presynaptic VDCCs. The inhibitionof each of these calcium channel types contributes to the reductionof [Ca_pre]_t by Y₂ receptors. Activation of adenosine receptorsfully occluded the inhibition of presynaptic calcium influx byY₂ receptors but not the inhibition by GABA_B receptors, suggestinga convergent action for Y₂ and adenosine receptors, probably bycoupling to the same G-protein.
Key words: hippocampus; presynaptic calcium; synaptic transmission; neuropeptide Y; Y₂ receptor; fura-2

INTRODUCTION

Neuropeptide Y (NPY) is expressed in interneurons in the rat hippocampus (Milner and Veznedaroglu, 1992; Pickel et al., 1995),and its receptors are concentrated in this region (Dumont et al.,1993). Application of NPY selectively inhibits excitatory synaptictransmission in area CA1 of rat hippocampus in vitro (Colmerset al., 1987, 1988; Klapstein and Colmers, 1992). The site ofaction is presumably presynaptic, because not the postsynapticmembrane properties, the postsynaptic response to exogenouslyapplied glutamate, nor the excitability of presynaptic fibersis affected by NPY (Colmers et al., 1987, 1988; McQuiston andColmers, 1996). Consistent with this, NPY inhibits the frequencyof spontaneous (i.e., Ca²⁺-dependent) but not miniature (Ca²⁺-independent) synaptic currents in rat CA3 pyramidal neurons ofhippocampal slices from adult rats (McQuiston and Colmers, 1996),suggesting indirectly that NPY also may reduce Ca²⁺ in presynaptic terminals of this region.

In the rat hippocampus, the involvement of at least two types of high-threshold voltage-dependent calcium channels (VDCC)in synaptic transmission has been demonstrated (Wheeler et al.,1994a; Dunlap et al., 1995). These are $omega$ -conotoxin GVIA-sensitive(N-type) and $omega$ -agatoxin-IVA-sensitive (P/Q-type) VDCCs, respectively.N- and P/Q-type VDCCs in neuronal somata are inhibited by theactivation of G-protein-coupled receptors for numerous neurotransmitters(Campbell et al., 1995). Measurements of Ca²⁺ influx into presynaptic terminals of sympathetic neurons filledwith a Ca²⁺ indicator by means of a patch pipette revealed that the presynapticaction of NPY in this system was attributable entirely to theinhibition of Ca²⁺ entry through N-type channels at these terminals (Toth et al.,1993). Inhibitory modulation of presynaptic VDCCs by neurotransmittersalso was observed at presynaptic terminals from CNS, includingcerebellar parallel fibers (Dittman and Regehr, 1996), hippocampalCA3 to CA1 axons (Wu and Saggau, 1994a, 1995; Qian and Saggau,1997), and the giant calyx of Held in the medial nucleus of thetrapezoid body (Takahashi et al., 1996). We hypothesize that theactivation of presynaptic NPY receptors directly inhibits presynapticVDCCs, thereby reducing synaptic transmission at the CA3-CA1 synapseof hippocampus.

However, the activation of presynaptic K⁺ conductances, also a well established response to neurotransmitters (Nicoll, 1988),also could result in presynaptic inhibition. Hyperpolarizationof presynaptic terminals because of increased K⁺ conductance would shorten action potentials, resulting in a decreasedpresynaptic calcium influx and consequent reduction of synaptictransmission.

At the CA3-CA1 pyramidal cell synapse in adult rat hippocampus, receptors for at least five different neurotransmitters caninhibit synaptic transmission (for review, see Thompson et al.,1993; Wu and Saggau, 1997). Of these, NPY is the only transmitterwith no postsynaptic action to complicate the interpretation ofchanges in synaptic responses (Colmers et al., 1988; Thompsonet al., 1993). Here, we have taken advantage of this to test thehypothesis that NPY acts by presynaptic inhibition of VDCCs.

MATERIALS AND METHODS
Recording of the field EPSP (fEPSP) and the presynaptic [Ca_pre]_t in hippocampal slices. Transverse hippocampal slices (300-350µm) were prepared from male Sprague Dawley rats (4 weeks of age)and incubated at 30°C in artificial cerebrospinal fluid composedof (in mM): 124 NaCl, 3 KCl, 2.5 CaCl₂, 2 MgCl₂, 22 NaHCO₃, 1.25NaH₂PO₄, and 10 D-glucose, gassed with 95% O₂/5% CO₂ to maintaina constant pH of 7.4. The dentate gyrus and part of CA3 were removedroutinely. The procedure for loading calcium indicator into presynapticterminals of CA3-CA1 synapses has been described in detail elsewhere(Wu and Saggau, 1994a). Briefly, a small amount of 1 mM fura-2AM or furaptra AM (Molecular Probes, Eugene, OR) dissolved inDMSO solution (80% DMSO plus 20% pluronic acid) was pressure-injectedinto brain slices in the stratum radiatum (SR) of area CA1, whereit was taken up locally into CA3 axons (see Fig. 1A). Approximately2 hr after injection, an area with a diameter of 200 µm in SR,~800 µm away from the injection site, was illuminated at a singleexcitation wavelength (380 nm). Fluorescence was collected bya 50× objective lens (numerical aperture, 0.9), filtered by along-pass filter (495 nm), and converted into an electrical signalby a single photodiode.
Fig. 1. A nonlinear relationship exists between [Ca_pre]_t and fEPSP. A, Schematic diagram for loading calcium indicators into presynapticterminals. Esterified (membrane-permeant) forms of fura-2 or furaptrawere pressure-injected into stratum radiatum (SR), where theywere taken up into CA3 axons, trapped by the action of esterases,and diffused into the remote presynaptic terminals onto CA1 neurons.Typical traces of the electrically recorded field EPSP (fEPSP),normalized transients of calcium indicator-related fluorescence(Fura), and their first derivative are shown under control conditionsand during blocked synaptic transmission (CNQX+APV). B, Comparisonbetween the peak of $Delta$ F/F and the peak of the first derivativeof $Delta$ F/F. C, Semi-log plot of normalized synaptic transmissionand [Ca_pre]_tversus extracellular calcium concentration, [Ca²⁺]_o. [Ca_pre]_t was a logarithmic function of [Ca²⁺]_o. D, Double-log plot of normalized fEPSP versus [Ca_pre]_t foreach tested [Ca²⁺]_o. The regression line has a slope of m = 4.2 (r² = 0.99) for fura-2 measurement and 3.8 (r² = 0.99) for furaptra, respectively.
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A bipolar tungsten electrode was positioned in SR of area CA1 to stimulate afferent inputs to CA1 neurons. An extracellularglass microelectrode (1-5 M $Omega$ , filled with 2 M NaCl) was used torecord fEPSPs in SR of area CA1. Slices were stimulated every20 sec to elicit a submaximal response, and stimulation-inducedpresynaptic calcium transient ([Ca_pre]_t) and fEPSPs were sampledsimultaneously at 10 kHz. Three successive traces were averagedto improve signal-to-noise ratio. The amplitude of calcium transients( $Delta$ F) was measured as the difference between peak and resting fluorescence(F). Signals were corrected for dye bleaching and diffusion byforming the ratio $Delta$ F/F. [Ca_pre]_t is assumed to be proportionalto the normalized change in fluorescence of the Ca²⁺ indicator, $Delta$ F/F. Autofluorescence of the brain slice was measuredand subtracted from the total fluorescence signal. When testingfor changes in presynaptic resting [Ca²⁺], we performed ratio measurements at excitation wavelengths of360 and 380 nm. The selective presynaptic loading of the Ca²⁺ indicator was verified by applying the ionotropic glutamate receptorantagonists 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX; 10 µM)and D-amino-phosphonovalerate (D-APV; 25 µM), which did not alter $Delta$ F/F while completely blocking the fEPSP (Fig. 1A). The maximalslope of the fEPSP was taken as the measure of synaptic transmission.

In those experiments in which $omega$ -Aga IVA was used, slices were cut at 300 µm, and 0.1% cytochrome c was added to the bath solutionto reduce nonspecific binding of the toxin. An active C-terminalfragment of human PYY (hPYY_3-36, a potent agonist at theNPY Y₂ receptor; Dumont et al., 1996) was dissolved in water andstocked at 1 mM. Data in each experiment were normalized to baselinebefore any drug application and then pooled and expressed as themean ± SD.

Drugs. PYY was a gift from Dr. Yvan Dumont (Children's Hospital Center, Verdun, Québec, Canada); CNQX and D-APV were purchasedfrom Tocris Cookson (Bristol, UK); $omega$ -CgTx GVIA and $omega$ -CgTx MVIICwere purchased from Bachem (Torrance, CA); $omega$ -Aga IVA was a giftfrom Pfizer (Groton, CT).

RESULTS

A nonlinear relationship exists between presynaptic calcium influx and synaptic transmission
The Ca²⁺ indicators, fura-2 and furaptra, were loaded selectively into the presynaptic terminals of the CA3-CA1 synapse at hippocampus,as described by Wu and Saggau (1994b) (Fig. 1A). This allowedus to record optically the presynaptic Ca²⁺ influx ([Ca_pre]_t), represented by the ratio $Delta$ F/F or the firstderivative of this ratio (d( $Delta$ F/F)/dt). The stimulation-evoked[Ca_pre]_t was detected simultaneously with the corresponding fEPSP.The extracellular Ca²⁺ concentration ([Ca²⁺]_o) was reduced systematically from 2.5 mM (control) to 0.5 mM,whereas the [Mg²⁺]_o was kept constant. No significant changes in the presynapticfiber volley were observed. [Ca_pre]_t and fEPSP slope from individualexperiments were normalized and used to calculate the relationshipbetween presynaptic Ca²⁺ influx and synaptic transmission in different [Ca²⁺]_o. Figure 1 compares measurements of [Ca_pre]_t obtained with theCa²⁺ indicators fura-2 and furaptra. In both cases, the peak of $Delta$ F/Fwas found to maintain a linear relationship with the peak of d( $Delta$ F/F)/dt,as shown in Figure 1B (slope = 0.98). Therefore, the peak of $Delta$ F/Fwas chosen as the measure of [Ca_pre]_t, because it is less noisythan the first derivative of $Delta$ F/F. As indicated by Figure 1C,[Ca_pre]_t was not proportional to [Ca²⁺]_o but was fairly linear with the logarithm of [Ca²⁺]_o. The nonlinearity between [Ca_pre]_t and [Ca²⁺]_o is not attributable to the saturation of Ca²⁺ indicators, because even in those experiments in which furaptra,an indicator with much lower Ca²⁺ affinity (K_D = 50 µM) than fura-2 (K_D = 200 nM), was loaded intoterminals, [Ca_pre]_t also showed a similar relationship with [Ca²⁺]_o. The mean reduction of [Ca_pre]_t measured with fura-2 was slightlyless than that with furaptra for the same [Ca²⁺]_o. This might be attributable to slight saturation of the fura-2signal. However, a major advantage of fura-2 signals was theirmuch higher signal-to-noise ratio, as compared with those obtainedwith furaptra; therefore, we used fura-2 for all further experiments,except where indicated.

Synaptic transmission also was shown to be steeply dependent on [Ca_pre]_t, revealing close to a fourth power relationship betweenpresynaptic Ca²⁺ influx and transmitter release in both fura-2 and furaptra measurements.The calculated power numbers were 3.9 ± 0.5 (n = 8), 4.1 ± 0.5(n = 8), and 4.3 ± 0.5 (n = 8) for 1.5, 1.0, and 0.5 mM [Ca²⁺]_o, respectively, in the experiments with fura-2. With furaptra,the power numbers were 3.2 ± 0.6 (n = 10), 3.7 ± 0.4 (n = 10),and 4.0 ± 0.6 (n = 10) for 1.5, 1.0, and 0.5 mM [Ca²⁺]_o, respectively. The average power numbers 4.2 (fura-2) and 3.8(furaptra) were estimated from the slope of the regression lines,as revealed in a double logarithmic plot (Fig. 1D). Synaptic transmissionwas not significantly different between fura-2 and furaptra measurements,suggesting at most a minor interference of the Ca²⁺ indicators with the release process under our conditions. Itis interesting to note that, with 0.5 mM [Ca²⁺]_o, synaptic transmission was eliminated almost completely, whereasa residual [Ca_pre]_t, ~50% of control, still could be detected(Fig. 1C).

Neuropeptide Y presynaptically inhibits synaptic transmission at the CA3-CA1 synapse
Application of hPYY_3-36 (a C-terminal fragment of human PYY, which is a potent agonist at NPY Y₂ receptors, abbreviatedas PYY throughout) at 1 µM inhibited both [Ca_pre]_t and synaptictransmission. Figure 2A shows the time course of both [Ca_pre]_tand the fEPSP of five experiments. On average, the [Ca_pre]_t wasinhibited by 20.1 ± 1.5% (n = 8), whereas the corresponding fEPSPslope was reduced by 58.3 ± 4.4%. NPY (1 µM) produced similar,but slightly less potent, effects than PYY (data not shown). Thepower number calculated from the peak effects of PYY on [Ca_pre]_tand fEPSP was m = 3.9 ± 0.5 (n = 8; Fig. 2D). There was no significantchange in either the size of the presynaptic fiber volley (Fig.2C) or resting calcium concentration during the application ofPYY (data not shown). The similarity in power numbers obtainedby applying PYY or reducing [Ca]_o are consistent with the hypothesisthat inhibition of synaptic transmission by PYY is attributablemainly to a reduction of [Ca_pre]_t.
Fig. 2. The activation of presynaptic Y₂ receptors inhibits [Ca_pre]_t and fEPSP. A, Group data (n = 5) showing the time course of normalized[Ca_pre]_t and fEPSP during the application of 1 µM PYY. Sampletraces taken at control and during maximal action of PYY are shownin the inset. B, Summary data for eight experiments. Approximately20% of [Ca_pre]_t was inhibited by application of 1 µM PYY. Thesynaptic transmission was reduced by ~60%. C, The presynapticvolley did not show a significant change during the applicationof PYY. D, Double-log plot of normalized fEPSP and [Ca_pre]_t duringthe peak action of PYY. Estimated power number for the inhibitionof synaptic transmission by PYY was 3.9 ± 0.5 (n = 8). Similarpower numbers were observed in this preparation for the actionof PYY and the reduction of [Ca²⁺]_o.
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Effects of calcium channel toxins on the inhibition of [Ca_pre]_t by PYY
To determine which types of calcium channels are inhibited by Y₂ receptors, we used $omega$ -CgTx GVIA (N-type channel toxin) and $omega$ -Aga IVA (P/Q-type channel toxin). If Y₂ receptors act exclusivelyon N-type or P/Q-type calcium channels, these toxins would occludethe effects of PYY completely. Figure 3A shows grouped data forsix experiments. On average, 1 µM $omega$ -CgTx GVIA inhibited [Ca_pre]_tand fEPSP to 79.5 ± 1.2% and 44.4 ± 2.5% of baseline, respectively(n = 7). The calculated power number for the inhibition of synaptictransmission by $omega$ -CgTx GVIA was m = 3.5 ± 0.3. After preapplicationof the toxin, PYY further reduced [Ca_pre]_t and fEPSP to 64.6 ±2.3% and 18.5 ± 4.5% of baseline, respectively (n = 7). The powernumber for the combination of $omega$ -CgTx GVIA and PYY was m = 3.9± 0.4 (Fig. 3C). Compared with the inhibition of [Ca_pre]_t undercontrol conditions (20.1%), 14.9% (79.5 $-$ 64.6%) of baseline [Ca_pre]_twas inhibited by PYY after preapplication of $omega$ -CgTx GVIA. Thus,~5.2% (20.1 $-$ 14.9%) inhibition of [Ca_pre]_t by PYY was occludedby $omega$ -CgTx GVIA. Normalized by the fraction of presynaptic N-typechannels, the relative inhibition of N-type VDCCs by PYY was ~25%(5.2%/20.5%).
Fig. 3. $omega$ -CgTx GVIA does not abolish the effects of PYY. A, Group data (n = 6) showing the time course of normalized [Ca_pre]_t andfEPSP during the application of $omega$ -CgTx GVIA (1 µM) and PYY (1µM). Sample traces taken at control, after application of $omega$ -CgTxGVIA, and during the peak effect of PYY are shown in the inset.B, Summary data for seven experiments. After preapplication of $omega$ -CgTx GVIA, PYY could still inhibit [Ca_pre]_t but to a lesserextent (~15% of control [Ca_pre]_t), whereas fEPSP was decreasedto 80% of control. C, Double-log plot of normalized fEPSP and[Ca_pre]_t during application of $omega$ -CgTx GVIA and $omega$ -CgTx GVIA+PYY.Estimated power numbers were m = 3.5 ± 0.3 (n = 7) for the inhibitionby $omega$ -CgTx GVIA alone and m = 3.9 ± 0.4 (n = 7) for the combinationof $omega$ -CgTx GVIA and PYY. The peak responses of $omega$ -CgTx GVIA andPYY were used to calculate the power numbers.
[View Larger Version of this Image (19K GIF file)]

Similarly, $omega$ -Aga IVA was applied to test the possible involvement of P/Q-type calcium channels in the modulation of synaptictransmission by PYY. $omega$ -Aga IVA (500 nM) reduced [Ca_pre]_t and fEPSPto 66.6 ± 1.8% and 18.1 ± 1.6% of control, respectively (n = 2),which resulted in a power number of m = 4.2 ± 0.1. Like $omega$ -CgTxGVIA, $omega$ -Aga IVA could not block the effect of PYY fully. Afterblockade of P/Q-type calcium channels, application of PYY stillproduced an inhibition of ~15.2 ± 1.7% of control [Ca_pre]_t (n= 2; Fig. 4A,C). Therefore, the percentage of inhibition of P/Q-typechannels was estimated to be ~15% [(20.1 $-$ 15.2%)/33.4%].
Fig. 4. $omega$ -Aga IVA and $omega$ -CgTx MVIIC do not abolish the effects of PYY. A, Group data showing the time course of normalized [Ca_pre]_tand fEPSP during the action of $omega$ -Aga IVA (500 nM) alone and togetherwith 1 µM PYY. Sample traces taken at control, after applicationof the calcium channel toxin, and during the peak effect of PYYare shown in the inset. B, Group data showing the time courseof normalized [Ca_pre]_t and fEPSP during the action of PYY togetherwith $omega$ -CgTx MVIIC (1 µM). Sample traces taken at control, afterapplication of calcium channel toxins, and during peak effectof PYY are shown in the inset. C, Summary data for A. [Ca_pre]_tand synaptic transmission were reduced irreversibly by ~34 and80%, respectively, after application of $omega$ -Aga IVA. PYY still inhibited[Ca_pre]_t by ~15% of control [Ca_pre]_t after blockade of P/Q-typecalcium channels, and synaptic transmission also was decreasedfurther. D, Approximately 11% inhibition of [Ca_pre]_t was observedeven after application of $omega$ -CgTx MVIIC to stop synaptic transmissionalmost completely.
[View Larger Version of this Image (32K GIF file)]

Neither $omega$ -CgTx GVIA nor $omega$ -Aga IVA alone fully blocked the inhibition of [Ca_pre]_t by PYY. This indicates that PYY did not selectivelyaffect either N-type or P/Q-type channels and suggests that multipletypes of VDCCs were involved. To confirm this, we used anotherconotoxin, MVIIC, to block both N- and P/Q-type channels (Turneret al., 1995) to test whether this occluded the inhibition of[Ca_pre]_t by PYY. $omega$ -CgTx MVIIC (1 µM) almost completely abolishedsynaptic transmission, whereas [Ca_pre]_t was reduced to ~56% ofcontrol (n = 2; Fig. 4B). Application of PYY after $omega$ -CgTx MVIICelicited ~11.1% inhibition of the total [Ca_pre]_t. Thus, $omega$ -CgTxMVIIC occluded the inhibition of [Ca_pre]_t by PYY (9% = 20.1 $-$ 11.1%) more than the application of either $omega$ -CgTx GVIA (5.2% =20.1 $-$ 14.9%) or $omega$ -Aga IVA (4.9% = 20.1 $-$ 15.2%). This is consistentwith an inhibition of both N- and P/Q-type calcium channels byactivation of presynaptic NPY receptors.

It should be noted that the effect of $omega$ -CgTx MVIIC might not have reached steady-state. This toxin should block both N-type(20.5%) and P/Q-type (33.4%) VDCCs and reduce the [Ca_pre]_t by~54% (20.5% + 33.4%). However, $omega$ -CgTx MVIIC blocked only 44% ofthe [Ca_pre]_t, leaving ~10% of the total [Ca_pre]_t, mediated byN- and P/Q-type, unblocked. This unblocked fraction potentiallycould contribute to the effect of PYY we observed with $omega$ -CgTxMVIIC. Because the relative percentage of inhibition of N- andP/Q-type channels by PYY was estimated to be ~25 and 15%, respectively,it is unreasonable to assume that the remaining 11.1% inhibitionof total [Ca_pre]_t by PYY after application of $omega$ -CgTx MVIIC wasentirely attributable to the inhibition of unblocked N- and P/Q-typeVDCCs. Instead, the inhibition of Ca²⁺ channels other than N- and P/Q-type significantly contributedto the reduction of [Ca_pre]_t by PYY after the application of $omega$ -CgTxMVIIC.

Actions of Y₂ and adenosine receptors occlude one another in the inhibition of [Ca_pre]_t
Similar to the effects of other neuromodulators, activation of NPY receptors has been shown to inhibit the [Ca_pre]_t. We havereported previously that adenosine and the muscarinic receptoragonist carbachol (CCh) mutually occlude one another in the inhibitionof [Ca_pre]_t at this synapse (Qian and Saggau, 1997), suggestinga convergent action of different neuromodulators. A common typeof G-protein may be the point of convergence in the inhibitorypathway from adenosine and muscarinic receptors to presynapticVDCCs. We were interested to learn whether NPY receptors sharedthe same presynaptic transduction pathway as do receptors of otherneuromodulators such as adenosine. We choose adenosine for thispurpose because its inhibition of presynaptic calcium channelshas been demonstrated at both the parallel fiber synapse of cerebellum(Dittman and Regehr, 1996) and the CA3-CA1 synapse of hippocampus,the present experimental preparation (Wu and Saggau, 1994a). Anotheradvantage of using adenosine is its rapid and complete washout,which allows for multiple application of the drug. Results ofexperiments with coapplication of adenosine and PYY are shownin Figure 5, A and B. PYY partially occluded the effect of adenosinein the inhibition of [Ca_pre]_t, regardless of the adenosine concentration.The inhibition of [Ca_pre]_t by adenosine and PYY was not additive.The occluding effect became more prominent when high does of adenosinewere used: PYY had no detectable effect on [Ca_pre]_t in the presenceof a saturating concentration (100 µM) of adenosine (Fig. 5B).Such a complete occlusion strongly suggests convergence of theNPY pathway with the adenosine pathway. However, when baclofen,a GABA_B receptor agonist, was coapplied with 100 µM adenosine,only a partial occlusion of [Ca_pre]_t inhibition was observed (Fig.5C,D). Because a saturating concentration of adenosine did notocclude the effect of baclofen completely, this indicates thatonly a partially shared pathway for these two neuromodulatorsexists at this synapse.
Fig. 5. Activation of Y₂ receptors occludes the inhibition of [Ca_pre]_t by adenosine. A, Time course of normalized [Ca_pre]_t and fEPSPillustrates the occlusion of inhibition of [Ca_pre]_t between activationof Y₂ and adenosine (AD) receptors. The inhibition of [Ca_pre]_tby adenosine in the presence of PYY (1 µM) was always smallerthan that without activation of Y₂ receptors, regardless of theconcentrations of adenosine (5, 10, or 100 µM). B, A saturatingconcentration of AD (100 µM) completely abolished the inhibitionof [Ca_pre]_t by PYY. C, D, Time course of normalized [Ca_pre]_t andfEPSP illustrates the partial occlusion between the activationof AD receptors and the activation of GABA_B receptors by baclofen(50 µM).
[View Larger Version of this Image (37K GIF file)]

However, if the activation of Y₂ receptors were to inhibit calcium channels via an unknown mechanism that depended on Ca²⁺ influx for its effect, then the reduction in Ca²⁺ influx caused by the activation of adenosine receptors in theabove experiments also might prevent a further inhibition of [Ca_pre]_tby PYY. To rule out this possibility, we applied PYY after reducing[Ca_pre]_t by lowering [Ca]_o to mimic the reduction in presynapticCa²⁺ influx caused by adenosine in the occlusion experiments above.The application of PYY in reduced [Ca²⁺]_o elicited a similar percentage of inhibition of [Ca_pre]_t asin control conditions (23.5%; Fig. 6), although presynaptic calciuminflux was reduced to ~56% of control. This is inconsistent withthe Ca²⁺-dependent mechanism postulated.
Fig. 6. PYY inhibits the same percentage of [Ca_pre]_t in reduced [Ca²⁺]_o. Shown is the time course of normalized [Ca_pre]_t and fEPSP inreduced [Ca²⁺]_o (0.7 mM). Application of PYY still elicited a 23.5% inhibitionof [Ca_pre]_t under these conditions. The inset shows the sampletraces taken under control conditions (2.5 mM [Ca²⁺]_o), in the presence of 0.7 mM [Ca²⁺]_o, and during the peak effect of PYY.
[View Larger Version of this Image (13K GIF file)]

DISCUSSION

Nonlinear relationship between presynaptic [Ca_pre]_t and synaptic transmission
Synaptic transmission is a nonlinear function of presynaptic calcium influx. This has been observed in many preparations,including the squid giant synapse (Katz and Miledi, 1970; Augustineand Charlton, 1986), the guinea pig hippocampal CA3-CA1 synapse(Wu and Saggau, 1994b), the cerebellar parallel fiber synapse(Mintz et al., 1995) and the calyx of Held (Borst et al., 1996).Postsynaptic responses can be described best by a power functionof measured [Ca_pre]_t. A power number of 4 has been observed inmost cases, whereas a power number of 2.5 has been reported atthe parallel fiber synapse of rat cerebellum (Mintz et al., 1995)and a retinotectal synapse in the frog (Feller et al., 1996).This estimated power number indicates that the release of neurotransmitteris a process that involves multiple calcium ions. Whether or notthe estimated apparent power number can be inferred to the numberof calcium binding sites depends on how precisely the calciumconcentration near the release sites is proportional to the totalcalcium influx into the presynaptic terminal that leads to themeasured [Ca_pre]_t. The relative location of calcium channels tothe calcium sensor of release machinery can greatly influencethe apparent power number that was measured. This might be thereason for the reported difference in power number between N-and P/Q-type channels in the cerebellum (Mintz et al., 1995).Comparative experimental and modeling studies at the same synapseindicate that the difference in the affinity of the calcium indicatorused to measure [Ca_pre]_t cannot explain the large difference inapparent power numbers found at the above synapses (Sinha et al.,1997). The present observations from the rat CA3-CA1 synapse confirmedthose results, although furaptra gave a slightly smaller powernumber than fura-2 (see Fig. 1D). Although the [Ca_pre]_t measuredby Ca²⁺ indicators represents a population average in our preparation,a power number of ~4 still was observed when [Ca_pre]_t was variedby the reduction of [Ca²⁺]_o, the application of calcium channel toxins, or the activationof Y₂ receptors. This is similar to the effects of activatingpresynaptic adenosine, GABA_B, or muscarinic receptors, as reportedearlier (Wu and Saggau, 1994a, 1995; Qian and Saggau, 1997) (forreview, see Wu and Saggau, 1997).

Multiple types of calcium channels are involved in the synaptic transmission at the CA3-CA1 synapse of hippocampus
$omega$ -CgTx GVIA-sensitive (N-type) and $omega$ -Aga IVA-sensitive (P/Q-type) calcium channels are involved in synaptic transmission atthe CA3-CA1 synapse (Wheeler et al., 1994b; Wu and Saggau, 1994c).Based on the observation of their supra-additive block of synaptictransmission, a presynaptic colocalization of N- and P/Q-typecalcium channels was proposed (Wu and Saggau, 1994c). Our resultsare consistent with those observations and also suggest that,besides N- and P/Q-type channels, unidentified types of calciumchannels, resistant to both $omega$ -CgTx GVIA and $omega$ -Aga IVA, also aresignificantly involved in the process of transmitter release.We observed a fourth power relationship between [Ca_pre]_t and fEPSPby reducing [Ca²⁺]_o, which decreases calcium influx equally for all channel types(N-, P/Q-, and those resistant to toxins). If the toxin-resistanttypes were not involved in transmitter release, then the powernumbers for both N- and P/Q-type would be significantly lowerthan 4. On the other hand, 0.5 mM [Ca²⁺]_o practically abolished transmitter release, while ~50% [Ca_pre]_tremained. A similar amount of [Ca_pre]_t (56%) remained after theapplication of $omega$ -CgTx MVIIC, which completely inhibited transmitterrelease, although the toxin specifically blocks only N- and P/Q-typechannels. Moreover, we show here that the inhibition of transmitterrelease by PYY is attributable to the reduction of [Ca_pre]_t, andPYY also was shown to inhibit $omega$ -CgTx MVIIC-insensitive Ca²⁺ channels. This suggests that $omega$ -CgTx MVIIC-insensitive Ca²⁺ channels also are involved in triggering transmitter release.

The hypothesis that other types of calcium channels are involved in triggering transmitter release, besides the N- and P/Q-types,cannot be tested directly, because channel blockers specific forthose $omega$ -CgTx GVIA- and $omega$ -Aga IVA-resistant VDCCs are not available.The K⁺-channel blocker, 4-AP, which is presumed to prolong the presynapticaction potential and thus to increase [Ca_pre]_t, recently was usedto assess this hypothesis indirectly (Wheeler et al., 1996). Inthese experiments 4-AP was shown to potentiate synaptic transmissionand to shift the transmission curve in the direction of a reduced[Ca²⁺]_o, i.e., lower [Ca²⁺]_o is required to maintain the same amount of transmitter releasein the presence of 4-AP. The effective blockade of synaptic transmissionby the combined application of $omega$ -CgTx GVIA and $omega$ -Aga IVA evenin the presence of 4-AP led these authors to the conclusion thatthe possible involvement of VDCCs other than N- and P/Q-type toplay a role in triggering transmitter release is restricted andthat crucial tests have to wait until better tools become availableto study these toxin-insensitive channel types separately. Ourfindings, however, suggest that a simple linear extrapolationof [Ca_pre]_t from [Ca²⁺]_o might overestimate the amount of increase in [Ca_pre]_t becauseof the nonlinear relationship between [Ca_pre]_t and [Ca²⁺]_o, especially under the conditions of high [Ca²⁺]_o (see Fig. 1C). Thus, it is necessary to measure the [Ca_pre]_tdirectly to prove that 4-AP can compensate sufficiently for thereduction of [Ca_pre]_t caused by the blockade of N- and P/Q-typechannels. If 4-AP could not compensate for this reduction of [Ca_pre]_tto values above threshold for transmitter release, then a blockof synaptic transmission by the combination of $omega$ -CgTx GVIA and $omega$ -Aga IVA would be anticipated, even in the presence of 4-AP.

Modulation of calcium channels by activation of presynaptic Y₂ receptors
Activation of presynaptic Y₂ receptors reduced both [Ca_pre]_t and synaptic transmission. During application of PYY the powerrelationship between [Ca_pre]_t and fEPSP was 3.9, compared with4.2 when [Ca²⁺]_o was reduced. This suggests that the inhibition of synaptictransmission by PYY is attributable mainly to the reduction of[Ca_pre]_t, and there is no evidence to support the involvementof an additional mechanism downstream of Ca²⁺ entry. Were the latter the case, then the power number observedwould be greater than that obtained by manipulating [Ca_pre]_t.Not $omega$ -CgTx GVIA, $omega$ -Aga IVA, nor $omega$ -CgTx MVIIC could abolish fullythe inhibition of [Ca_pre]_t by PYY. The sum of the inhibitionsby PYY after application of $omega$ -CgTx GVIA and $omega$ -Aga IVA, respectively,was larger than the inhibition of [Ca_pre]_t by PYY observed withoutany toxins. These data suggest that other types of VDCCs besidesN-type and P/Q-type contribute to the inhibition of [Ca_pre]_t byPYY. The estimated percentages of inhibitions are 25, 15, and21% for N-type, P/Q-type, and unidentified calcium channels, respectively.

Several lines of evidence suggest that PYY inhibits calcium channels rather than activates K⁺ channels in presynaptic terminals. First, the presynaptic fibervolley did not change significantly during application of PYY.Second, the differential inhibition for different types of calciumchannels observed in our experiments is inconsistent with a reductionin duration of the presynaptic action potential that would accompanyan activation of K⁺ channels. Such a shortening of the depolarization of presynapticterminals would be expected to affect all types of VDCCs equally(Wheeler et al., 1996). Third, the occlusion of PYY-induced inhibitionby adenosine that we observed is also inconsistent with an involvementof K⁺ channels. Furthermore, if activation of Y₂ receptors were toopen K⁺ channels and thus shorten the action potential, this should reducethe [Ca_pre]_t regardless of the type or number of VDCCs inhibitedby the previous application of adenosine. This was not observedwhen a saturating concentration of adenosine was used. Previousstudies revealed no evidence for adenosine action on presynapticK⁺ channels at this synapse (Wu and Saggau, 1994a). Finally, theinvolvement of K⁺ channels in the modulation of synaptic transmission by NPY wastested previously at this synapse by Klapstein and Colmers (1992).Their observation that 4-AP could not reduce the inhibition ofsynaptic transmission by NPY is consistent with our conclusionthat PYY acts on calcium channels and not on K⁺ channels.

A common G-protein may be the convergent point of inhibition of [Ca_pre]_t by Y² and adenosine receptors
Y₂ and adenosine receptors occlude each other's inhibition of [Ca_pre]_t, as shown in Figure 5. A similar mutual occlusion betweenactivation of muscarinic and adenosine receptors also has beenobserved at this synapse (Qian and Saggau, 1997). In sympatheticneurons it has been proposed that adenosine, NPY, and muscarinicreceptors all act convergently on the same G-protein, G_o, to inhibitN-type calcium channels in these cells (Hille, 1994). The mutualocclusion of their inhibition of [Ca_pre]_t that we observed atthe CA3-CA1 synapse would be consistent with this hypothesis andfurther suggests that a similar mechanism may underlie the inhibitionof presynaptic VDCCs by adenosine and muscarinic and NPY receptorsin the CNS. This is in contrast to baclofen, a GABA_B receptoragonist, which, when applied at a saturating concentration togetherwith a saturating concentration of adenosine, resulted in a nonoccludinginhibition of [Ca_pre]_t (Fig. 5C,D). This indicates that the completeocclusion of inhibition of [Ca_pre]_t among adenosine, NPY, andmuscarinic receptors is not attributable to either a limitationof experimental methods or a saturation of the inhibitory processat the presynaptic terminal (such as insufficient available G-proteins).Rather, it suggests that inhibition of presynaptic VDCCs by GABA_Breceptors is attributable at least in part to a mechanism differentfrom the one activated by adenosine and muscarinic and NPY receptors.

Studies of presynaptic inhibition by NPY and the other neuromodulators suggest that modulation of presynaptic Ca²⁺ channels by G-protein-coupled receptors acts as a fast, short-termmechanism to control transmitter release. Our results supportthe hypothesis that a common mechanism underlies the inhibitoryeffect of different neuromodulators at the presynaptic site. Sucha common mechanism would greatly improve the efficiency of intracellularsignaling pathway in controlling transmitter release.

FOOTNOTES

Received May 9, 1997; revised Aug. 11, 1997; accepted Aug. 15, 1997.

This work was supported by National Institutes of Health Grant NS-33147 to P.S. and Medical Research Council (Canada) GrantMT-10520 to W.F.C. We acknowledge Dr. Yvan Dumont for the giftof PYY. We also thank Dr. N. A. Saccomano at Pfizer Incorporated,Groton, CT, for generously supplying samples of $omega$ -Aga IVA. Thecomputer software for data acquisition and analysis was developedby Dr. S. S. Patel. We thank S. Sinha for critical and helpfulcomments on this manuscript.

Correspondence should be addressed to Dr. Peter Saggau, Baylor College of Medicine, One Baylor Plaza, Houston, TX 77030.

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Volume 17, Number 21, Issue of November 1, 1997 pp. 8169-8177 Copyright ©1997 Society for Neuroscience

Inhibition of Synaptic Transmission by Neuropeptide Y in Rat Hippocampal Area CA1: Modulation of Presynaptic Ca2+ Entry

Copyright ©1997 Society for Neuroscience 0270-6474/1997/178169-09$05.00/0

Volume 17, Number 21, Issue of November 1, 1997 pp. 8169-8177
Copyright ©1997 Society for Neuroscience

Inhibition of Synaptic Transmission by Neuropeptide Y in Rat Hippocampal Area CA1: Modulation of Presynaptic Ca²⁺ Entry