Atrial Natriuretic Peptide Modulates Synaptic Transmission from Osmoreceptor Afferents to the Supraoptic Nucleus

QUICK SEARCH:

[advanced]

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

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (13)

Citing Articles via Google Scholar

Google Scholar

Articles by Richard, D.

Articles by Bourque, C. W.

Search for Related Content

PubMed

PubMed Citation

Articles by Richard, D.

Articles by Bourque, C. W.

Previous Article  |  Next Article

Volume 16, Number 23, Issue of December 1, 1996 pp. 7526-7532
Copyright ©1996 Society for Neuroscience

Atrial Natriuretic Peptide Modulates Synaptic Transmission from Osmoreceptor Afferents to the Supraoptic Nucleus

Dominique Richard and Charles W. Bourque
Centre for Research in Neuroscience, Montreal General Hospital Research Institute and McGill University, Montréal, Québec, Canada H3G 1A4

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Atrial natriuretic peptide (ANP) and its receptors are present in hypothalamic nuclei containing the magnocellular neurosecretorycells (MNCs), which release vasopressin and oxytocin. In the rat,intracerebroventricular injections of ANP inhibit the releaseof both hormones in response to hypertonicity. Although thesefindings suggest a role for endogenous ANP in the central controlof fluid balance, cellular mechanisms underlying the modulatoryactions of ANP are unknown. We therefore examined the effectsof ANP on the osmoresponsiveness of MNCs impaled in rat hypothalamicexplants. Applications of ANP (75-150 nM) over the supraopticnucleus did not affect depolarizing responses to local hypertonicity,but they reversibly abolished the synaptic excitation of MNCsafter hypertonic stimulation of the organum vasculosum laminaeterminalis (OVLT). These effects were associated with decreasedspontaneous EPSP (sEPSP) amplitude rather than with changes insEPSP frequency. Accordingly, application of ANP reduced the amplitudeof glutamatergic EPSPs evoked by electrical stimulation of theOVLT (IC₅₀ ~ 3 nM). The inhibitory effects of ANP on EPSP amplitudewere mimicked by application of 3 $'$ -5 $'$ -dibutyryl cGMP, consistentwith the guanylate cyclase activity of natriuretic peptide receptors.Although depolarizing responses of MNCs to ionotropic glutamatereceptor agonists were unaffected by ANP, the peptide reversiblyenhanced paired-pulse facilitation of electrically evoked EPSPs.These results indicate that centrally released ANP may inhibitosmotically evoked neurohypophysial hormone release through presynapticinhibition of glutamate release from osmoreceptor afferents derivedfrom the OVLT.
Key words: atrial natriuretic peptide; supraoptic nucleus; OVLT; organum vasculosum lamina terminalis; osmoregulation; vasopressin; oxytocin; osmoreceptor; presynaptic inhibition

INTRODUCTION

Atrial natriuretic peptide (ANP) is a 28 amino acid hormone that was first identified in heart myocytes (deBold, 1985). Systemicrelease of ANP by the atria, which follows expansion of extracellularfluid volume (Lang et al., 1985; Eskay et al., 1986), promotesrelaxation of the vascular smooth muscle as well as diuresis andnatriuresis at the level of the kidneys (Brenner et al., 1990).Circulating ANP, therefore, plays an important role in cardiovascularand body fluid homeostasis. Natriuretic peptides including ANPand brain natriuretic peptide (BNP) have also been detected inthe CNS (Imura et al., 1992). These peptides (Saper et al., 1985,1989; Standaert et al., 1986) and their receptors (Gibson et al.,1986) are particularly abundant in CNS regions that participatein the autonomic and neuroendocrine regulation of blood pressureand fluid balance. Moreover, intracerebroventricular injectionsof ANP interfere with hypertonically evoked changes in thirst(Antunes-Rodriguez et al., 1985; Nakamura et al., 1985; Katsuuraet al., 1986), salt appetite (Fitts et al., 1985; Antunes-Rodriguezet al., 1986), and diuresis (Itake et al., 1986; Poole et al.,1987; Samson et al., 1987; Manzanares et al., 1990). Althoughthese observations suggest a role for centrally released ANP inthe osmotic regulation of fluid balance, the cellular basis forits role as a neuromodulator remains unknown.

Central efferent pathways mediating the perception of thirst and salt appetite remain undefined, making it difficult to studythe cellular mechanisms by which such responses may be regulatedby neuromodulators and neurotransmitters. The osmotic controlof diuresis, however, is known to be achieved specifically throughchanges in the electrical activity of hypothalamic magnocellularneurosecretory cells (MNCs), which control the secretion of vasopressinfrom the neurohypophysis (Bourque et al., 1994). HypothalamicMNCs, therefore, offer an ideal opportunity to examine the cellularbasis underlying the modulatory actions of ANP in the CNS. Indeed,hypothalamic nuclei comprising MNCs are innervated by fibers containingANP (Standaert et al., 1986, 1987; Saper et al., 1989), and theyexpress binding sites for radiolabeled ANP (Gibson et al., 1986;Kurihara et al., 1987). Moreover, local application of natriureticpeptides reduces the basal electrical activity of MNCs in vivo(Standaert et al., 1987) and in vitro (Okuya and Yamashita, 1987;Yamamoto et al., 1991; Akamatsu et al., 1993; Oliet and Bourque,1993c). The mechanism by which ANP may modulate the osmoresponsivenessof these cells, however, is unknown.

The osmotic control of MNC firing is achieved both as a result of the intrinsic osmosensitivity of these cells (Mason, 1980;Bourque, 1989; Oliet and Bourque, 1993a,b) and by changes in thefrequency of spontaneous glutamatergic EPSPs they receive fromosmoreceptor afferents derived from the organum vasculosum laminaeterminalis (OVLT) (Richard and Bourque, 1995). In this study,therefore, we examined the modulatory effects of ANP on thesecomponents during intracellular recordings from MNCs in the ratsupraoptic nucleus (SON).

MATERIALS AND METHODS
Preparation of explants. Basal hypothalamic explants (8 × 8 × 2 mm) were prepared as described previously (Bourque, 1990),using the brains of male Long-Evans rats (200-300 gm) killed bydecapitation. The explants were pinned to the Sylgard base ofa temperature-controlled (32-34°C) recording chamber. The opticnerves were cut proximal to the optic chiasm to expose the OVLT,and the pial membranes overlying the SON and OVLT were removedusing fine forceps. The area of the SON was superfused (1.0 ml/min)with oxygenated (95% O₂/5% CO₂) artificial cerebrospinal fluid(ACSF; see below) delivered from a tube placed over the caudalend of the optic tract. The OVLT was superfused separately (0.3ml/min) via a second tube placed near the rostral tip of the opticchiasm (Richard and Bourque, 1995).

Solutions. The ACSF (295 ± 2 mOsm/kg), pH 7.4, comprised (in mM): 113 NaCl, 3 KCl, 1.3 MgCl₂, 25.9 NaHCO₃, 2 CaCl₂, and 10glucose. Hypertonic solutions were made by adding mannitol tothe ACSF. Hypertonic stimulation of the SON was achieved by infusinghypertonic solution via a small catheter inserted into the tubesuperfusing this area (Bourque, 1989). Hypertonic stimulationof the OVLT was achieved by bath-application of hypertonic solutionsthrough the main delivery tube superfusing the OVLT. The osmolalityof all solutions was verified using a freezing-point micro-osmometer(VWR Scientific, West Chester, PA). ANP (rat ANP 1-28; PeninsulaLaboratories, Belmont, CA), 3 $'$ -5 $'$ -dibutyryl cGMP (db-cGMP; Sigma,St. Louis, MO), 6-cyano-7-nitroquinoxaline-2,3,dione (CNQX; TocrisNeuramin, Bristol, UK) and D,L-2-amino-5-phosphonovalerate (APV;Sigma) were dissolved in ACSF and bath-applied over the SON. NMDA(Sigma) and AMPA (Sigma) were injected via a catheter insertedinto the tube superfusing the SON.

Electrophysiology. Pipettes were prepared by pulling glass capillary tubes (1.2 mm outer diameter) on a horizontal P-87 puller(Sutter Instruments, Novato, CA). The recording electrodes werefilled with 2 M potassium acetate (70-120 M $Omega$ ) and connected tothe headstage of an Axoclamp 2A amplifier (Axon Instruments, FosterCity, CA) via a Ag-AgCl wire. Each cell was impaled by advancingthe microelectrode in rapid steps (4 mM) with a piezoelectricdevice (Burleigh, Fishers, NY). Two copies of membrane voltage,one filtered at 0-5000 Hz and the other at 10-1000 Hz, were displayedon a chart recorder, digitized (44 kHz; Neuro Data Instruments,Delaware Water Gap, PA), and stored on videotape for off-lineanalysis. Electrical stimulation of the OVLT was achieved usinga bipolar platinum electrode (0.3 mm outer diameter; 40-200 µA;80-150 µsec) placed at the anteroventral midline wall of the thirdventricle, dorsal to the optic chiasm. In these experiments, bicucullinemethochloride (5-10 µM; Tocris Neuramin) was added to the ACSFto block the GABAergic IPSP component described previously (Yanget al., 1994). Consecutive trials ( $<=$ 0.5 Hz) were averaged (n $>=$ 4) to measure the amplitude of the evoked EPSP. Input conductance(G_in) was estimated as G_in = I/(V_rest $-$ V_ss), where V_rest andV_ss are the voltages at rest and during the steady-state phaseof the electrotonic response to the application of a fixed hyperpolarizingcurrent pulse (I), respectively. Percentage change in paired-pulsefacilitation ( $Delta$ PPF) was quantified as $Delta$ PPF = 100 × [(PPF_ANP $-$ PPF_CTR)/PPF_CTR], where PPF_ANP and PPF_CTR are the ratioed amplitudesof the second EPSP over the first, in the presence of ANP andduring control, respectively.

Spontaneous EPSP (sEPSP) analysis. The AC-coupled (10-1000 Hz) voltage signal was digitized (10 kHz) using a Labmaster interfaceand pCLAMP software (Axon Instruments). Individual sEPSPs weredetected manually using Fetchan 5.51, as described previously(Richard and Bourque, 1995). Changes in sEPSP frequency occurringin response to osmotic stimulation were analyzed by counting thenumber of events in 8 sec segments acquired 30 sec immediatelybefore and after the application of a stimulus. In five cells,the amplitudes of all manually detected sEPSPs observed during60 sec recording segments taken in ACSF and in the presence ofANP were measured as the difference between voltage at peak amplitude(average of 5-10 consecutive points) and baseline (average of20-200 points preceding each event). Events were binned accordingto size, and cumulative probability distributions were plotted.Changes in sEPSP amplitude were assessed as shifts in the medianamplitude of sEPSPs (amplitude at 0.5 probability). All data areexpressed as mean ± SEM. Statistical differences between groupswere evaluated using a paired t test and judged to be significantif p < 0.01.

RESULTS
The data presented below were obtained from 36 MNCs impaled in the SON of rat hypothalamic explants. The cells displayed restingmembrane potentials below $-$ 50 mV, input resistances >100 M $Omega$ , andtransient outward rectification during voltage responses to depolarizingcurrent pulses applied from holding potentials negative to $-$ 70mV. In addition, action potentials (amplitude >65 mV from baseline)evoked by depolarizing current pulses showed frequency-dependentspike broadening. Together, these features have been shown tobe characteristic of rat MNCs, but not of neighboring non-neuroendocrinecells, both in vivo (Bourque and Renaud, 1991; Dyball et al.,1991) and in vitro (Bourque and Renaud, 1990).

Effects of ANP on the osmotic excitation of MNCs
The osmotic control of MNC firing is determined both by intrinsically generated changes in membrane potential (Mason, 1980;Bourque, 1989; Oliet and Bourque, 1993a,b) and by changes in thefrequency of sEPSPs derived from osmoreceptor neurons in the OVLT(Richard and Bourque, 1995). We therefore examined the effectsof ANP on both components. The depolarizing response of MNCs tolocal hypertonic stimulation (+30 mOsm/kg) of the SON (5.8 ± 0.2mV) was not altered by bath-application of 75-150 nM ANP (5.8± 0.2 mV) in any of six cells tested (data not shown), indicatingthat the intrinsic osmosensitivity of MNCs is unaffected at theseconcentrations of the peptide. In contrast, bath-application ofANP (75-150 nM) over the SON consistently and reversibly abolishedthe excitation of MNCs that followed local hypertonic stimulationof the OVLT (+10-20 mOsm/kg) in each of five cells tested (Fig.1). This procedure did not significantly alter either basal sEPSPfrequency (Fig. 2A) or the increase in sEPSP frequency in responseto hypertonic stimulation (Fig. 2B). These findings indicate thatinhibition of presynaptic firing is not responsible for the blockadeof OVLT-mediated responses recorded under such conditions. Asillustrated in Figure 3, however, application of ANP reversiblyreduced the amplitude of sEPSPs to 76 ± 3% of control (p < 0.01;n = 5; see Materials and Methods), suggesting that the inhibitoryeffects of ANP are mediated by a reduction in the strength ofsynaptic transmission between the OVLT and MNCs of the SON.
Fig. 1. Effects of ANP on the osmoresponsiveness of MNCs impaled in the supraoptic nucleus (SON) of hypothalamic explants. A, Schematicdiagram of experimental setup illustrating the relative positionsof MNCs projecting to the posterior pituitary (PP) and of theirafferents from osmoreceptor neurons in the OVLT. OC, Optic chiasma.B, Chart recordings of voltage responses recorded in MNCs in responseto hypertonic stimulation of the OVLT (bar). Bath applicationof ANP (150 nM) reversibly blocked the excitatory response ofthe cell to the hypertonic stimulus. Initial membrane potentialwas $-$ 53 mV in each of the trials shown.
[View Larger Version of this Image (39K GIF file)]

Fig. 2. Effects of ANP on the frequency of sEPSPs recorded from MNCs in the SON. A, Bar histograms express the mean (±SEM) normalizedfrequencies at which sEPSPs occurred in MNCs under isotonic conditions.Note that addition of ANP (75-150 nM) to the solution superfusingthe SON did not significantly alter the basal frequency at whichsEPSPs were detected in MNCs (90 ± 3% of control; p > 0.05; n= 5). B, Bar histograms express mean (±SEM) normalized changesin sEPSP frequency ( $Delta$ sEPSP frequency), relative to the basalrate (% of control), evoked by hypertonic stimulation of the OVLT.Note that the increase in sEPSP frequency observed in ACSF (156± 12% of control) was not significantly affected by the inclusionof 75-150 nM ANP in the solution superfusing the SON (147 ± 8%;p > 0.05; n = 5).
[View Larger Version of this Image (20K GIF file)]

Fig. 3. Effects of ANP on the amplitude of sEPSPs. A, High-gain voltage excerpts of a recording obtained from a rat MNC in controlsolution (ACSF) and in the presence of ANP (75 nM). The membranepotential was $-$ 63 mV. B, The graph plots the cumulative probabilitydistributions of sEPSP amplitude measured from a different MNCduring 60 sec recording segments obtained in ACSF (899 events)and in the presence of 75 nM ANP (809 events). C, Bar histogramsplot the mean (±SEM) relative median amplitude (normalized amplitudeat 0.5 probability) of the sEPSPs observed in control solutions(ACSF; 100%) and in the presence of 75 nM ANP (the asterisk denotesp < 0.01; n = 5).
[View Larger Version of this Image (18K GIF file)]

Effects of ANP on EPSPs evoked by electrical stimulation of the OVLT
In agreement with an inhibitory effect on synaptic transmission, superfusion of ANP (1.5 to 500 nM) over the SON reversiblyattenuated the amplitude of EPSPs evoked by electrical stimulationof the OVLT (Fig. 4A). This effect was consistently observed ineach of 21 cells tested. Because vasopressin- and oxytocin-releasingMNCs occur in equal proportions in the rat SON (Vandersande andDierickx, 1975), it can be presumed that both types of MNCs aresubject to the inhibitory actions of ANP. As shown in Figure 4B,the effects of ANP on evoked EPSPs were dose-dependent (IC₅₀ ~3 nM), with maximal inhibition being observed at concentrations $>=$ 30 nM. Consistent with the intrinsic guanylate cyclase (GC) activityof receptors for ANP (Chinkers et al., 1989; Schultz et al., 1989),the effect of the peptide on evoked EPSP amplitude was mimickedby application of db-cGMP (0.5-1 mM; n = 3) (Fig. 5A). In thepresence of saturating concentrations of ANP, the amplitude ofevoked EPSPs was attenuated by 46 ± 2% (mean ± SEM; n = 9), avalue that coincides with the inhibitory effects of 1 mM db-cGMP(46%). As reported previously (Yang et al., 1994; Richard andBourque, 1995), the evoked EPSPs were reversibly abolished bythe application of CNQX and APV (20-40 µM each; n = 4) (Fig. 5B),confirming that the modulatory effects of ANP and db-cGMP areproduced at glutamatergic synapses.
Fig. 4. Effects of ANP on EPSPs evoked by electrical stimulation of the OVLT (arrows). A, Voltage traces showing the reversible decreasein EPSP amplitude in the presence of ANP (75 nM). B, The top graphplots the dose-dependency (dashed line shows IC₅₀ = 3 nM) of theeffects of ANP on the relative amplitude of EPSPs evoked by OVLTstimulation. The bottom graph plots the mean input conductance(G_in; relative to control) of cells bathed in the presence ofdifferent concentrations of ANP. Closed symbols are single measurements,whereas open symbols are mean values ± SEM; n $>=$ 3.
[View Larger Version of this Image (17K GIF file)]

Fig. 5. Effects of db-cGMP and glutamate receptor antagonists on EPSPs evoked by electrical stimulation of the OVLT (arrows). A, Superimposedtraces showing the EPSP recorded from a cell before (control),during (db-cGMP), and after (wash) bath application of 1 mM db-cGMP.B, Superimposed traces recorded from another MNC illustrate thereversible block of the evoked EPSP by application of CNQX andAPV (25 µM each).
[View Larger Version of this Image (14K GIF file)]

Effects of ANP on responses to ionotropic glutamate receptor agonists
Although the above observations demonstrate an inhibitory role for ANP on glutamatergic transmission, they do not indicatewhether modulation occurs pre- or postsynaptically. The bottompanel in Figure 4 reveals that the input conductance of MNCs wasunaffected by ANP under the present conditions. A postsynapticshunting effect, therefore, did not mediate the attenuation ofspontaneous and evoked EPSP amplitude observed in the presenceof ANP. We next examined whether ANP could modify the postsynapticresponses of MNCs to ionotropic glutamate receptor activation.As shown in Figure 6, depolarizing responses of MNCs to exogenouslyapplied NMDA (20-30 µM; n = 3) or AMPA (20-30 µM; n = 3) wereunaltered in the presence of the peptide (75-150 nM), indicatingthat the inhibitory effects of ANP are not attributable to a modulationof postsynaptic glutamate receptors.
Fig. 6. ANP does not affect the responsiveness of MNCs to glutamate receptor activation. A, Chart recordings of voltage responsesfrom a single supraoptic MNC to applications of 25 µM NMDA (bars;top traces) or 30 µM AMPA (bars; bottom traces), recorded in controlsolution (left panels) or in the presence of 75 nM ANP (rightpanels). Initial membrane potential was $-$ 60 mV in each trial.Action potentials are truncated in this figure. B, Bar histogramsplotting the mean ± SEM amplitude of depolarizing responses toNMDA (top) and AMPA (bottom) recorded from three cells.
[View Larger Version of this Image (25K GIF file)]

Effects of ANP on PPF
In response to pairs of electrical stimuli delivered to the OVLT (15-20 Hz), the amplitude of the second EPSP evoked in MNCswas increased compared with the first (Fig. 7A). This phenomenon,known as PPF, has been observed at many synapses, and it reflectsa selective enhancement of transmitter release (Zucker, 1989).Manipulations that decrease transmitter release enhance PPF (Mallartand Martin, 1967; Katz and Miledi, 1968). As illustrated in Figure7, PPF of OVLT-mediated EPSPs was enhanced in the presence ofANP (n = 8). At a concentration of 3 nM, which corresponds tothe IC₅₀ for ANP-mediated effects on EPSP amplitude, the mean(±SEM) enhancement in PPF was 25 ± 11% (n = 4). These observationssuggest that the effects of ANP on EPSPs result from a presynapticinhibition of glutamate release.
Fig. 7. Inhibitory effects of ANP are presynaptic. A, Voltage responses of an MNC to pairs of electrical stimuli delivered to theOVLT (arrows). In ACSF the amplitude of the second EPSP is enhancedrelative to the first, reflecting the occurrence of PPF. The traceon the right shows the response of the same cell to identicalstimuli delivered in the presence of 100 nM ANP. Note that theamplitude of the first EPSP recorded in ANP is attenuated comparedwith control but that PPF is enhanced. B, The traces shown inA are superimposed and scaled so that the amplitudes of the firstEPSPs match each other. Note the relative enhancement of the secondEPSP in the presence of ANP.
[View Larger Version of this Image (11K GIF file)]

DISCUSSION
Natriuretic peptides (Standaert et al., 1986, 1987; Saper et al., 1989) and receptors (Gibson et al., 1986; Kurihara et al.,1987) are present in hypothalamic nuclei comprising the MNCs,which release vasopressin and oxytocin into the systemic circulation(Bourque and Renaud, 1990). In the rat, intracerebroventricularinjections of ANP inhibit the release of both hormones in responseto rises in extracellular fluid osmolality (Itake et al., 1986;Poole et al., 1987; Samson et al., 1987; Manzanares et al., 1990).In this study, therefore, we examined the effects of ANP on theosmoresponsiveness of MNCs during intracellular recordings fromrat hypothalamic explants.

Inhibitory effects of ANP on the osmotic regulation of MNC firing
The osmotic control of MNC firing is achieved through changes in an intrinsic cationic conductance (Bourque, 1989; Oliet andBourque, 1993a,b) and by changes in the frequency of sEPSPs derivedfrom osmoreceptor neurons within the OVLT (Richard and Bourque,1995). Both of these components increase as a function of fluidosmolality from a threshold near 275 mOsm/kg (Bourque et al.,1994). Because this value corresponds to the osmotic pressureat which circulating neurohypophysial hormones become detectableby radioimmunoassay (Verbalis and Dohanics, 1991), it is likelythat both processes are important for the osmotic regulation ofhormone secretion in vivo. Consequently, both the intrinsic cationicconductance and the OVLT-mediated synaptic excitation representpotential targets through which centrally released ANP may modulatethis process. In the present experiments, application of ANP (75-150nM) over the SON inhibited the contribution of OVLT-derived excitatoryinputs, without altering the intrinsic osmosensitivity of MNCs.Our analysis revealed that ANP does not prevent increases in thefrequency of glutamatergic sEPSPs after hypertonic stimulationof the OVLT (Richard and Bourque, 1995). Rather, the inhibitoryactions of the peptide are associated with an attenuation of sEPSPamplitude. These observations suggest that endogenously releasedANP may impede the osmotic regulation of neurohypophysial hormonerelease by reducing the strength of the excitatory connectionbetween osmoreceptor neurons in the OVLT and MNCs in the SON.In agreement with this hypothesis, applications of ANP over theSON reversibly reduced the amplitude of glutamatergic EPSPs evokedby electrical stimulation of the OVLT.

The inhibitory effects of ANP are mediated by GC-A receptors
Receptors that transduce the biological actions of natriuretic peptides feature a single membrane-spanning domain, and theypossess an intrinsic GC as part of their cytoplasmic moiety. BothGC-A and GC-B have been cloned (Chinkers et al., 1989; Schultzet al., 1989), and in each case receptor activation has been shownto provoke increases in the concentration of intracellular cGMP.In our experiments, the attenuation of EPSP amplitude by ANP couldbe mimicked by application of db-cGMP. Furthermore, the maximalattenuation observed at saturating concentrations of ANP (46%)coincided with the largest inhibitory effects of db-cGMP (46%at 1 mM). These results suggest that the inhibitory effects ofANP on supraoptic MNCs are mediated through activation of theintrinsic GC of the receptors. In agreement with this hypothesis,bath-application of ANP has been reported to cause a three- tofourfold increase in the cGMP content of tissue slices containingthe SON (Akamatsu et al., 1993).

In COS-7 cells transfected with the gene encoding GC-A receptors, cGMP production resulting from exposure to ANP increaseswith a half-maximal concentration (EC₅₀) of 3 nM (Chinkers etal., 1989; Schultz et al., 1989). In contrast, cGMP productionin cells transfected with the gene coding for GC-B receptors increasesas a function of ANP with an EC₅₀ of 26 µM (Schultz et al., 1989).Because inhibition of OVLT-mediated EPSPs by ANP occurred withan EC₅₀ of 3 nM, activation of GC-A receptors presumably mediatedthe effects of the peptide in our experiments. Interestingly,BNP-like immunoreactivity has been detected in fibers within theSON (Saper et al., 1989), and BNP has been reported to serve asa selective agonist at GC-A receptors (EC₅₀ = 5 nM) rather thanat GC-B receptors (EC₅₀ = 6 µM) (Schultz et al., 1989). Althoughthe effects of BNP were not examined in the present study, GC-Areceptor activation by BNP, similar to that of ANP, would be expectedto cause attenuation in the amplitude of OVLT-mediated EPSPs.Future studies will be needed to determine whether GC-B receptorsalso play a role in the regulation of MNCs.

ANP causes presynaptic inhibition of glutamate release
The fast EPSP recorded in MNCs after electrical stimulation of the OVLT results from activation of the AMPA and NMDA subtypesof ionotropic glutamate receptors (Yang et al., 1994; Richardand Bourque, 1995). It is possible, therefore, that the effectsof ANP could be mediated through changes in the sensitivity orfunctional density of these receptors. The results presented hereshow that the depolarization and excitation of supraoptic MNCsinduced by exogenous applications of AMPA and NMDA were unaffectedby saturating concentrations of ANP (75-150 nM), suggesting thatmodulation of postsynaptic glutamatergic receptors does not mediatethe inhibitory effects of ANP acting at GC-A receptors. Previousstudies have shown that manipulations that decrease transmitterrelease at presynaptic terminals enhance PPF (Mallart and Martin,1967; Katz and Miledi, 1968; Zucker, 1989). Our experiments showedthat PPF of the OVLT-mediated EPSP recorded in MNCs is enhancedin the presence of ANP. Together, the observations presented heresuggest that ANP reduces glutamate release from axon terminalssynapsing onto supraoptic MNCs.

Presynaptic effects are associated with changes in the frequency of miniature EPSPs (mEPSPs) and not with variations in mEPSPamplitude (Del Castillo and Katz, 1954). Under our experimentalconditions, ANP reduced sEPSP amplitude without affecting therate at which these were observed under basal or osmotically stimulatedconditions. The majority of sEPSPs recorded in our study, however,were not mEPSPs but were synaptic events resulting from spikedischarge in afferent axons. Indeed, the frequency of spontaneoussynaptic events recorded in MNCs decreases dramatically on exposureto TTX (Wuarin and Dudek, 1993). Moreover, most of the sEPSPsrecorded from MNCs at rest are prevented by blocking spike dischargein OVLT neurons (Richard and Bourque, 1995). Under such conditions,changes in mEPSP frequency would not be expected to have a largeimpact on the frequency of sEPSPs, as was observed experimentally(Fig. 2). The reduction in sEPSP amplitude induced by ANP, therefore,presumably resulted from a decrease in mean quantal content ratherthan from a decrease in quantal size, in agreement with a presynapticeffect.

Although the mechanisms by which ANP inhibits glutamate release are unknown, the peptide reduces basal concentrations of intracellularcalcium ([Ca²⁺]_i) (Hassid, 1986) and inhibits the activity of voltage-gatedCa²⁺ channels (Hassid, 1986; Gisbert and Fishmeister, 1988) in vascularsmooth muscle and cardiac cells. The expression of either of thesemechanisms in neurons could potentially result in an attenuationof the amplitude of [Ca²⁺]_i transients occurring in response to spike discharge and reduceglutamate release from axon terminals. Moreover, a previous studyin GH₄C₁ cells has shown that ANP can enhance a voltage-sensitiveK⁺ conductance (White et al., 1993). By decreasing the durationof action potentials, the reduction of a repolarizing K⁺ current in neurons could also attenuate presynaptic [Ca²⁺]_i transients and reduce spike-evoked glutamate release. Additionalstudies will be required to determine which of these mechanisms,if any, underlies the inhibitory effects of ANP on glutamate release.

Functional implications
The results presented here provide a cellular mechanism for the inhibition of hypertonically evoked increases in vasopressinand oxytocin secretion by centrally administered ANP (Itake etal., 1986; Poole et al., 1987; Samson et al., 1987; Manzanareset al., 1990). As indicated earlier, the frequency of glutamatergicEPSPs derived from osmosensitive neurons within the OVLT increasesin MNCs as a function of fluid osmolality, from a threshold of275 mOsm/kg (Richard and Bourque, 1995). Because resting osmolalityin rats is near 295 mOsm/kg (Dunn et al., 1973), osmoreceptorneurons in the OVLT provide an excitatory drive to supraopticMNCs that is tonically active at rest (Richard and Bourque, 1995).Presynaptic inhibition of this input by ANP, therefore, mightbe expected to reduce basal firing rate as well as increases infiring evoked by hypertonic stimulation. Although the effectsof ANP on basal firing were not examined in the present experiments,previous recordings from MNCs in hypothalamic slices have revealedthat in a proportion of neurons, the inhibitory effects of ANPare lost under conditions blocking synaptic transmission (Okuyaand Yamashita, 1987), as would be expected for neurons in whichthe actions of ANP on basal firing were mediated presynaptically.Presynaptic inhibition of glutamate release from osmoreceptorafferents may underlie the effects of centrally administered ANPon other osmoregulatory mechanisms (Imura et al., 1992).

Postsynaptic effects of ANP
When recorded under conditions blocking synaptic transmission, a percentage of MNCs are inhibited by ANP (Okuya and Yamashita,1987), suggesting that receptors for ANP may also be expressedpostsynaptically. The existence of GC-A receptors on MNCs wasdemonstrated previously using whole-cell recordings from supraopticneurons isolated from adult rats (Oliet and Bourque, 1993c). Applicationof 1-20 nM ANP to these cells increased a voltage-insensitiveK⁺ conductance, resulting in membrane hyperpolarization. Surprisingly,consistent effects on input conductance were not observed on applicationof ANP to MNCs in hypothalamic explants (Fig. 4). The lack ofa postsynaptic effect in this case suggests that the target K⁺ channels, or components of the transduction system, may be activity-dependent.Indeed, in the present study the basal firing of spontaneouslyactive cells was suppressed by current injection to facilitatethe analysis of synaptic potentials. An interesting alternativeis that the postsynaptic mechanism might be expressed differentiallyunder different conditions. Additional studies will be requiredto resolve this issue.

FOOTNOTES

Received Aug. 25, 1996; revised Sept. 17, 1996; accepted Sept. 18, 1996.

This work was supported by an operating grant from the Medical Research Council (MRC) of Canada (C.W.B.), by a Heart and StrokeFoundation of Canada Studentship (D.R.), and by an MRC ScientistAward (C.W.B.). We thank S. H. R. Oliet, T. E. Fisher, and D.L. Voisin for their helpful criticism of an earlier version ofthis manuscript.

Correspondence should be addressed to Dr. Charles W. Bourque, Division of Neurology, Montréal General Hospital, 1650 CedarAvenue, Montréal, Québec, Canada H3G 1A4.

REFERENCES

Akamatsu N, Inenaga K, Yamashita H (1993) Inhibitory effects of natriuretic peptides on vasopressin neurons mediated through cGMP and cGMP-dependent protein kinase in vitro. J Neuroendocrinol 5:517-522 . [Web of Science][Medline]
Antunes-Rodrigues J, McCann SM, Rogers LC, Samson WK (1985) Atrial natriuretic factor inhibits dehydration- and angiotensin II-induced water intake in the conscious, unrestrained rat. Proc Natl Acad Sci USA 82:8720-8723 . [Abstract/Free Full Text]
Antunes-Rodrigues J, McCann SM, Samson WK (1986) Central administration of atrial natriuretic factor inhibits saline preference in the rat. Endocrinology 118:1726-1728 . [Abstract/Free Full Text]
Bourque CW (1989) Ionic basis for the intrinsic activation of rat supraoptic neurones by hyperosmotic stimuli. J Physiol (Lond) 417:263-277 . [Abstract/Free Full Text]
Bourque CW (1990) The isolated and perfused mammalian hypothalamus. In: Preparations of vertebrate central nervous system in vitro (Jahnsen, H, eds) , p. 203. Chichester, UK: Wiley.
Bourque CW, Renaud LP (1990) Electrophysiology of mammalian magnocellular vasopressin and oxytocin secreting neurons. Front Neuroendocrinol 11:183-212.
Bourque CW, Renaud LP (1991) Membrane properties of rat magnocellular neuroendocrine cells in vivo. Brain Res 540:349-352 . [Web of Science][Medline]
Bourque CW, Oliet SHR, Richard D (1994) Osmoreceptors, osmoreception, and osmoregulation. Front Neuroendocrinol 15:231-274 . [Web of Science][Medline]
Brenner BM, Ballermann BJ, Gunning ME, Zeidel ML (1990) Diverse biological actions of atrial natriuretic peptide. Physiol Rev 70:665-699 . [Free Full Text]
Chinkers M, Garbers DL, Chang M-S, Lowe DG, Chin H, Goeddel DV, Schultz S (1989) A membrane form of guanylate cyclase is an atrial natriuretic peptide receptor. Nature 338:78-83 . [Medline]
deBold AJ (1985) Atrial natriuretic factor: a hormone produced by the heart. Science 230:767-770. [Abstract/Free Full Text]
Del Castillo J, Katz B (1954) Quantal components of the end-plate potential. J Physiol (Lond) 124:560-573.
Dunn FL, Brennan TJ, Nelson AE, Robertson GL (1973) The role of blood osmolality and volume in regulating vasopressin secretion in the rat. J Clin Invest 52:3212-3219 .
Dyball REJ, Tasker J-G, Wuarin J-P, Dudek FE (1991) In vivo intracellular recordings of neurons in the supraoptic nucleus of the rat hypothalamus. J Neuroendocrinol 3:383-386. [Web of Science][Medline]
Eskay R, Zukowska-Grojec Z, Haass M, Dave JR, Zamir N (1986) Circulating atrial natriuretic peptides in conscious rats: regulation of release by multiple factors. Science 232:636-639 . [Abstract/Free Full Text]
Fitts DA, Thunhorst RL, Simpson JB (1985) Diuresis and reduction of salt appetite by lateral ventricular infusions of atriopeptin II. Brain Res 348:118-124 . [Web of Science][Medline]
Gibson TR, Wildey GM, Manaker S, Glembotski CC (1986) Autoradiographic localization and characterization of atrial natriuretic peptide binding sites in the rat central nervous system and adrenal gland. J Neurosci 6:2004-2011 . [Abstract]
Gisbert MP, Fishmeister R (1988) Atrial natriuretic factor regulates the calcium current in frog isolated cardiac cells. Circ Res 62:660-667 . [Abstract/Free Full Text]
Hassid A (1986) Atriopeptin II decreases cytosolic free Ca in cultured vascular smooth muscle cells. Am J Physiol 251:C681-C686 . [Abstract/Free Full Text]
Imura H, Nakao K, Itoh H (1992) The natriuretic peptide system in the brain: implications in the central control of cardiovascular and neuroendocrine functions. Front Neuroendocrinol 13:217-249 . [Web of Science][Medline]
Itake K, Share L, Crofton JT, Brooks DP, Ouchi Y, Blaine EH (1986) Central atrial natriuretic factor reduces vasopressin secretion in the rat. Endocrinology 119:438-440. [Abstract/Free Full Text]
Katsuura G, Nakamura M, Inoue K, Kono M, Nakao K, Imura H (1986) Regulatory role of atrial natriuretic polypeptide in water drinking in rats. Eur J Pharmacol 121:285-287 . [Web of Science][Medline]
Katz B, Miledi R (1968) The role of calcium in neuromuscular facilitation. J Physiol (Lond) 195:481-482 . [Abstract/Free Full Text]
Kurihara M, Saavedra JM, Shigematsu K (1987) Localization and characterization of atrial natriuretic peptide binding sites in discrete areas of rat brain and pituitary gland by quantitative autoradiography. Brain Res 408:31-39 . [Web of Science][Medline]
Lang RE, Tholken H, Ganten D, Luft FC, Ruskoaho H, Unger T (1985) Atrial natriuretic factor: a circulating hormone stimulated by volume loading. Nature 314:264-266 . [Medline]
Mallart A, Martin AR (1967) An analysis of facilitation of transmitter release at the neuromuscular junction of the frog. J Physiol (Lond) 193:679-694. [Web of Science][Medline]
Manzanares J, Lookingland KJ, Moore KE (1990) Atrial natriuretic peptide-induced suppression of basal and dehydration-induced vasopressin secretion is not mediated by hypothalamic tuberohypophysial or tuberoinfundibular dopaminergic neurons. Brain Res 527:103-108 . [Web of Science][Medline]
Mason WT (1980) Supraoptic neurones of rat hypothalamus are osmosensitive. Nature 287:154-157 . [Medline]
Nakamura M, Katsuura G, Nakao K, Imura I (1985) Antidipsogenic action of a human atrial natriuretic polypeptide administered intracerebroventricularly in rats. Neurosci Lett 58:1-6 . [Web of Science][Medline]
Okuya S, Yamashita H (1987) Effects of atrial natriuretic polypeptide on rat hypothalamic neurones in vitro. J Physiol (Lond) 389:717-728 . [Abstract/Free Full Text]
Oliet SHR, Bourque CW (1993a) Steady-state osmotic modulation of cationic conductance in neurons of the rat supraoptic nucleus. Am J Physiol 265:R1475-R1479. [Abstract/Free Full Text]
Oliet SHR, Bourque CW (1993b) Mechanosensitive channels transduce osmosensitivity in supraoptic neurons. Nature 364:341-343. [Medline]
Oliet SHR, Bourque CW (1993c) Inhibitory effects of atrial natriuretic factor (ANF) on supraoptic neurons isolated from the rat. Soc Neurosci Abstr 19:1794.
Poole CJM, Carter DA, Vallejo M, Lightman SL (1987) Atrial natriuretic factor inhibits the stimulated in vivo and in vitro release of vasopressin and oxytocin in the rat. J Endocrinol 112:97-102. [Abstract/Free Full Text]
Richard D, Bourque CW (1995) Synaptic control of rat supraoptic neurones during osmotic stimulation of the organum vasculosum lamina terminalis in vitro. J Physiol (Lond) 489.2:567-577. [Abstract/Free Full Text]
Samson WK, Aguila MC, Martinovic J, Antunes-Rodrigues J, Norris M (1987) Hypothalamic action of atrial natriuretic factor to inhibit vasopressin secretion. Peptides 8:449-454 . [Web of Science][Medline]
Saper CB, Standaert DG, Currie MG, Schwartz D, Geller DM, Needleman P (1985) Atriopeptin-immunoreactive neurons in the brain: presence in cardiovascular regulatory areas. Science 227:1047-1049 . [Abstract/Free Full Text]
Saper CB, Hurley KM, Moga MM, Holmes HR, Adams SA, Leahy KM, Needleman P (1989) Brain natriuretic peptides: differential localization of a new family of neuropeptides. Neurosci Lett 96:29-34 . [Web of Science][Medline]
Schultz S, Singh S, Bellet RA, Singh G, Tubb DJ, Chin H, Garbers DL (1989) The primary structure of a plasma membrane guanylate cyclase demonstrates diversity within this new receptor family. Cell 58:1155-1162. [Web of Science][Medline]
Standaert DG, Needleman P, Saper CB (1986) Organization of atriopeptin-like immunoreactive neurons in the central nervous system of the rat. J Comp Neurol 253:315-341 . [Web of Science][Medline]
Standaert DG, Cechetto DF, Needleman P, Saper CB (1987) Inhibition of the firing of vasopressin neurons by atriopeptin. Nature 329:151-153 . [Medline]
Vandersande F, Dierickx K (1975) Identification of the vasopressin and oxytocin producing neurons in the hypothalamic magnocellular neurosecretory system of the rat. Cell Tissue Res 164:153-162. [Web of Science][Medline]
Verbalis JG, Dohanics J (1991) Vasopressin and oxytocin secretion in chronically hypoosmolar rat. Am J Physiol 261:R1028-R1038 . [Abstract/Free Full Text]
White RE, Lee AB, Shcherbatko AD, Lincoln TM, Schonbrunn A, Armstrong DL (1993) Potassium channel stimulation by natriuretic peptides through cGMP-dependent dephosphorylation. Nature 361:263-266 . [Medline]
Wuarin J-P, Dudek FE (1993) Patch-clamp analysis of spontaneous synaptic currents in supraoptic neuroendocrine cells of the rat hypothalamus. J Neurosci 13:2323-2331 . [Abstract]
Yamamoto S, Inenaga K, Yamashita H (1991) Inhibition by brain natriuretic peptide of vasopressin neurons in the supraoptic nucleus and neurons in the region of the anteroventral third ventricle in rat hypothalamic slice preparations. J Neuroendocrinol 3:45-49.
Yang CR, Senatorov VV, Renaud LP (1994) Organum vasculosum lamina terminalis-evoked postsynaptic responses in rat supraoptic neurones in vitro. J Physiol (Lond) 477:59-74 . [Abstract/Free Full Text]
Zucker RS (1989) Short-term synaptic plasticity. Annu Rev Neurosci 12:13-31 . [Web of Science][Medline]

Copyright ©1996 Society for Neuroscience   0270-6474/1996/167526-07$05.00/0

This article has been cited by other articles:

J. ANTUNES-RODRIGUES, M. DE CASTRO, L. L. K. ELIAS, M. M. VALENCA, and S. M. McCANN
Neuroendocrine Control of Body Fluid Metabolism
Physiol Rev, January 1, 2004; 84(1): 169 - 208.
[Abstract] [Full Text] [PDF]

M Hirasawa, S B Kombian, and Q J Pittman
Oxytocin retrogradely inhibits evoked, but not miniature, EPSCs in the rat supraoptic nucleus: role of N- and P/Q-type calcium channels
J. Physiol., May 1, 2001; 532(3): 595 - 607.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (13)

Citing Articles via Google Scholar

Google Scholar

Articles by Richard, D.

Articles by Bourque, C. W.

Search for Related Content

PubMed

PubMed Citation

Articles by Richard, D.

Articles by Bourque, C. W.