Osmoregulation of Vasopressin Secretion via Activation of Neurohypophysial Nerve Terminals Glycine Receptors by Glial Taurine

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The Journal of Neuroscience, September 15, 2001, 21(18):7110-7116

Osmoregulation of Vasopressin Secretion via Activation of Neurohypophysial Nerve Terminals Glycine Receptors by Glial Taurine
Nicolas Hussy, Vanessa Brès, Marjorie Rochette, Anne Duvoid, Gérard Alonso, Govindan Dayanithi, and Françoise C. Moos
Laboratoire de Biologie des Neurones Endocrines, Centre National de la Recherche Scientifique (CNRS) Unité Mixte de Recherche 5101, Centre CNRS-Institut National de la Santé et de la Recherche Médicale de Pharmacologie et d'Endocrinologie, 34094 Montpellier Cedex 5, France

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Osmotic regulation of supraoptic nucleus (SON) neuron activity depends in part on activation of neuronal glycine receptors(GlyRs), most probably by taurine released from adjacent astrocytes.In the neurohypophysis in which the axons of SON neurons terminate,taurine is also concentrated in and osmo-dependently releasedby pituicytes, the specialized glial cells ensheathing nerve terminals.We now show that taurine release from isolated neurohypophysesis enhanced by hypo-osmotic and decreased by hyper-osmotic stimulation.The high osmosensitivity is shown by the significant increaseon only 3.3% reduction in osmolarity. Inhibition of taurine releaseby 5-nitro-2-(3-phenylpropylamino)benzoic acid, niflumic acid,and 4,4'-diisothiocyanatostilbene-2,2'-disulfonic acid suggeststhe involvement of volume-sensitive anion channels. On purifiedneurohypophysial nerve endings, activation of strychnine-sensitiveGlyRs by taurine or glycine primarily inhibits the high K⁺-induced rise in [Ca²⁺]_i and subsequent release of vasopressin. Expression of GlyRsin vasopressin and oxytocin terminals is confirmed by immunohistochemistry.Their implication in the osmoregulation of neurohormone secretionwas assessed on isolated whole neurohypophyses. A 6.6% hypo-osmoticstimulus reduces by half the depolarization-evoked vasopressinsecretion, an inhibition totally prevented by strychnine. Mostimportantly, depletion of taurine by a taurine transport inhibitoralso abolishes the osmo-dependent inhibition of vasopressin release.Therefore, in the neurohypophysis, an osmoregulatory system involvingpituicytes, taurine, and GlyRs is operating to control Ca²⁺ influx in and neurohormone release from nerve terminals. Thiselucidates the functional role of glial taurine in the neurohypophysis,reveals the expression of GlyRs on axon terminals, and furtherdefines the role of glial cells in the regulation of neuroendocrinefunction.

Key words: glycine receptors; taurine; vasopressin; oxytocin; osmoregulation; glial cells; pituicytes; volume-sensitive Cl channels; supraoptic nucleus; neurohypophysis; neurohormone secretion

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Vasopressin (VP) and oxytocin (OT) are synthesized by hypothalamic neuroendocrine cells localized in the supraoptic nucleus(SON) and the paraventricular nucleus (PVN). The axons of theseneurons terminate in the neurohypophysis in which the neurohormonesare secreted into the blood circulation. VP and to a lesser extentOT are involved in the regulation of the body water balance. Accordingly,their release is regulated by the osmotic pressure of extracellularfluid through modulation of the electrical activity of OT andVP neurons (Bourque et al., 1994; Bourque and Oliet, 1997; Hussyet al., 2000). Osmoregulation of these neurons is complex, comingfrom both osmosensory afferent inputs and their intrinsic osmosensitivity.The latter results in part from the presence of stretch-inactivatedcationic channels in their membrane, which depolarize and hyperpolarizethe neurons exposed to hyper-osmotic and hypo-osmotic medium,respectively (Bourque et al., 1994). We recently provided evidencefor an additional mechanism of SON neuron osmosensitivity, whichinvolves glial cells as osmosensory elements (Hussy et al., 2000).SON astrocytes specifically concentrate the amino acid taurine(Decavel and Hatton, 1995) and release it in an osmo-dependentmanner through volume-sensitive anion channels (Deleuze et al.,1998; Brès et al., 2000). Taurine is an agonist of strychnine-sensitiveglycine receptors (GlyRs) (Betz et al., 1999), expressed at highlevel on the soma and proximal dendrites of SON neurons (Hussyet al., 1997). Activation of these ligand-gated Cl channels mediates part of the in vivo hypo-osmotic inhibitionof VP neuron activity (Hussy et al., 1997). Although direct evidencefor glial taurine being the actual endogenous agonist of thesereceptors is still missing, a number of convergent observationsstrongly argue in favor of this hypothesis. These include theproperties of taurine release (Deleuze et al., 1998), its specificityrelative to that of the other potential GlyR agonists (Hussy etal., 1997), as well as the apparent absence of glycinergic afferentinput to these neurons (Wuarin and Dudek, 1993; Rampon et al.,1996). This points to a peculiar role of SON astrocytes in theosmoregulation of neuronal activity and of GlyRs that would serveanother function than mediating neuronal fast synaptictransmission.

In the neurohypophysis, taurine is also selectively accumulated in the pituicytes, the specialized astrocytes surroundingSON and PVN neuron axon terminals, and released during hypo-osmoticstimulation (Pow, 1993; Miyata et al., 1997). Numerous factorsare known to modulate hormone release at the level of nerve terminals,which express a variety of neurotransmitter and neuropeptide receptors(Hatton, 1990, 1999; Zhang and Jackson, 1995; Rusin et al., 1997;Sheikh et al., 1998; Troadec et al., 1998; Wilke et al., 1998).However, the effect of taurine on neurohormone secretion has notbeen studied, and it is not known whether local osmotic regulationof VP or OT release takes place in the neurohypophysis. We reporthere the hypo-osmotic regulation of depolarization-evoked VP secretionin the neurohypophysis, resulting from the osmo-dependent releaseof taurine from pituicytes, which activates strychnine-sensitiveGlyRs on the nerve terminals to inhibit Ca²⁺ influx and hormonerelease.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Measurement of taurine release. Neurohypophyses were isolated from adult male Wistar rats killed by decapitation, put in acold (4°C) oxygenated Locke's solution [in mM: 137 NaCl, 5 KCl,2 CaCl₂, 2 MgCl₂, 1.2 KH₂PO₄, 10 HEPES, and 10 glucose, pH 7.4(300 mOsm/l)], and carefully isolated from the pars intermedia.Tissues were incubated for 40 min in a Locke's medium supplementedwith 500 nM [³H]taurine (Amersham Pharmacia Biotech, Orsay, France) at 35°C,rinsed three times, placed in perfusion chambers (250 µl, oneneurohypophysis per chamber) at 35°C, and perfused at a rate of250 µl/min with oxygenated Locke's solution. After 20 min rest,perfusate was collected every 2 min with a sample collector (modelFC204; Gilson France, Villiers-le-Bel, France). [³H]Taurine release was estimated by scintillation counting. Hypo-osmoticmedia were Locke's solutions, to which the appropriate amountof NaCl was omitted. The respective control iso-osmotic mediawere the same solutions to which sucrose was added up to an osmolarityof 300 mOsm/l. Basal release of taurine in iso-osmotic mediumwas fitted with a monoexponential function, and data were normalizedto this fit to express release as percentage of basal release(Deleuze et al., 1998, 2000). Two chambers were systematicallyused as control, and the effects of the various drugs were alwayscompared with the controls of the same set of experiments. Allexperiments were realized on at least two different preparations.Analysis was performed with Origin 5.0 software (Microcal Software,Inc., Northampton, MA). Data are given as means ±SEM.

Measurements of[Ca²⁺]_i. Neurohypophyses freed from the pars intermedia were homogenized at 37°C [in 100 µl of a solution containing(in mM): 270 sucrose, 0.1 or 2 EGTA, and 20 HEPES, pH 7.2] andspun at 100 × g for 1 min, and the supernatant was further spunat 2400 × g for 4 min. The final pellet containing highly purifiednerve terminals (Cazalis et al., 1987) was resuspended in Locke'ssolution. Isolated nerve terminals were seeded onto glass coverslips and incubated in Locke's solution containing fura-2 AM (2.5µM; Molecular Probes, Europe, Leiden, The Netherlands) and 0.01%pluronic acid at room temperature for 1 hr. After washing, nerveterminals were perfused at a rate of 100 µl/min with Locke's orhigh (25 mM) K⁺ solution (Locke's solution with KCl replacing NaCl). Fluorescencemeasurements of [Ca²⁺]_i were performed with a Zeiss Microscope Photometer System (FFP;Zeiss, Oberkochen, Germany), based on an inverted microscope (Axiovert100; Zeiss) equipped for epifluorescence (objective, Plan-Neofluar100×/1.30 numerical aperture oil immersion). With fluorescencevalues corrected for background and dark current, [Ca²⁺]_i was calculated from the ratio between 340 and 380 nm recordings,after fura-2 calibration performed as described previously (Dayanithiet al., 1996).

Immunohistochemistry. After deep anesthesia with pentobarbital (300 mg/kg), animals were perfused through the ascending aortawith 100 ml of PBS, pH 7.4, followed by 500 ml of 4% paraformaldehydein 0.1 M phosphate buffer, pH 7.4. The neurointermediate hypophysiallobe and a portion of the spinal cord were dissected and immersedin the same fixative for 8 hr. Tissues were cut with a vibratomeinto 40-µm-thick sections and rinsed in PBS. Sections were incubatedfor 48 hr at 4°C with a monoclonal antibody against GlyR thatrecognizes all subunits (mAb4a, diluted 1:200; Alexis Corp., Läufelfingen,Switzerland), either alone or in combination with a second antibodyagainst either VP (guinea pig polyclonal antibody GHC8103, diluted1:500; Peninsula Laboratories, Belmont, CA) or OT [rabbit polyclonalantibody obtained from G. Alonso, diluted 1:2000]. After rinsingin PBS, sections were incubated for 1 hr with secondary antibodiesagainst mouse IgG conjugated with Cy3 (diluted 1:1000; JacksonImmunoResearch, West Grove, PA) and rabbit or guinea pig IgG conjugatedwith Alexa 488 (diluted 1:1000; Molecular Probes). After rinsing,sections were mounted in Mowiol (Calbiochem, La Jolla, CA) andobserved under a Bio-Rad (Hercules, CA) MRC 1024 confocal laserscanning microscope equipped with a krypton-argon mixed gas laser.Two laser lines emitting at 488 and 568 nm were used to excitethe Alexa 488- and Cy3-conjugated secondary antibodies, respectively.The background noise of each confocal image was reduced by averagingfive image inputs. Immunostained structures were studied on singleconfocal images of 1-2 µm thick. Unaltered digitized images weretransferred to a personal computer, and Photoshop (Adobe Systems,San Jose, CA) was used to prepare and print final figures. Nofluorescent labeling was detected when omitting to apply the primaryantibodies.

Radioimmunoassay. Either purified isolated neurohypophysial nerve terminals obtained as described above (terminals from one-halfneurohypophysis per chamber), or isolated whole neurointermediatelobes (one per chamber) were placed in 60 µl perfusion chambersat 35°C and perfused at a rate of 100 µl/min with oxygenated Locke'ssolution containing 0.01% BSA and bacitracin (170 µM) to preventVP degradation (Sladek and Armstrong, 1987). After 1 hr rest,2.5 min perfusate samples were collected in iced tubes containing10 µl of acetic acid and rapidly frozen. Iso- and hypo-osmoticsolutions were prepared as described for taurine release. HighK⁺ solutions (25-50 mM) were obtained by replacing NaCl by KCl.One hundred microliters (isolated terminals) or 10 µl (whole neurohypophyses)of each sample were incubated for 24 hr at 4°C with a VP polyclonalantibody [kindly supplied by Dr. John Bicknell (Babraham Institute,Cambridge, UK)] used at a 1:133,000 dilution in a buffer saline(BS) (140 mM NaCl, 10 mM HEPES, and 2 gm/l BSA, pH 7.3) and thenfor 31 hr at 4°C with 12.5 pM iodinated VP (Amersham PharmaciaBiotech). Bound and free [¹²⁵I]VP were separated by 15 min centrifugation at 4000 × g in BSsupplemented with 0.5% activated charcoal and 0.05% dextran (Sigma,St. Quentin, France). Radioactivity was measured in the pelletby gamma counter and converted to VP concentration according toa standard curve systematically established inparallel.

Drugs. Taurine, glycine, strychnine, Arg-vasopressin, niflumic acid, 4,4'-diisothiocyanatostilbene-2,2'-disulfonic acid (DIDS),tamoxifen, 4-bromophenacyl bromide (pBPB), and ATP-Na were fromSigma. Gabazine, N- phenylanthranylic acid (DPC), and 5-nitro-2-(3-phenyl-propylamino)benzoicacid (NPPB) were from Research Biochemicals (Natick, MA). Guanidinoethylsulfonate (GES) was from Toronto Research Chemicals, and mibefradilwas a gift from E. Bourinet (Centre National de la Recherche Scientifique,Montpellier,France).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Osmo-dependent release of taurine in the neurohypophysis

The osmo-dependent release of taurine from neurohypophysial pituicytes was estimated on perfused acutely isolated whole neurohypophysesfrom adult rats, using tritiated taurine as a tracer. Under isotonicconditions (300 mOsm/l), neurohypophyses displayed a low sustainedrelease of taurine, which was reversibly increased by applicationof hypo-osmotic solutions ranging from 290 to 260 mOsm/l and decreasedby hyper-osmotic stimulation (330 mOsm/l) (Fig. 1). These effectswere attributable to variations in osmotic pressure because onlythe concentration of sucrose was changed in the perfusing solutions,with the ion concentrations being kept constant (see Materialsand Methods). The increase in taurine release induced by hypo-osmolaritywas dependent on the intensity of the stimulus, with a very highsensitivity: a consistent increase in release (26 ± 5% increase;n = 5) was already observed for a 10 mOsm/l decrease in osmolarity,corresponding to a 3.3% change in osmotic pressure (Fig. 1). Thistype of sensitivity was reminiscent of that of taurine releasefrom SON astrocytes (Deleuze et al., 1998, 2000). Release evokedby greater osmotic changes showed a transient component that hasbeen shown in other systems to reflect cell volume regulation(Pasantes-Morales and Shousboe, 1997).

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Figure 1. Osmo-dependent release of taurine from the neurohypophysis. A, Release of [³H]taurine from isolated neurohypophyses was modulated by both hypo-osmotic and hyper-osmotic stimuli. Each trace is the average of 5-12 measurements from at least three different experiments. Note the sustained release induced by small stimulus. B, Relationship between the peak of taurine release and the osmolarity of the perfusing solution, showing the high osmosensitivity of release. Error bars are shown when exceeding the size of the symbols. Solid line is a Boltzmann fit of the data.

Basal release was strongly enhanced in the presence of 300 µM of the taurine transporter inhibitor GES (from 219 ± 14 to 468± 44 dpm; n = 6 each), indicative of a constant reuptake of taurine,but GES did not prevent release evoked by a 280 mOsm/l hypo-osmoticstimulus (39 ± 6 vs 33 ± 2% increase in the absence and presenceof GES, respectively; n = 6 each; data not shown). Therefore,the taurine transporter does not mediate release of taurine. Thepharmacological properties of taurine release were then studiedin the continuous presence of GES to increase the sensitivityof the measurements of drug effects. Both basal and hypotonicityevoked-release were inhibited by classical blockers of anion channels,such as NPPB, niflumic acid, DIDS, and high concentrations ofextracellular ATP (Fig. 2), arguing for the involvement of volume-sensitiveanion channels, as seen in the SON (Deleuze et al., 1998; Brèset al., 2000). Blockade of evoked release reached 52 ± 11 (50µM NPPB), 47 ± 8 (100 µM niflumic acid), 70 ± 4 (1 mM DIDS), and34 ± 5% (10 mM ATP) (Fig. 2C). On the other hand, release of taurinewas totally insensitive to a variety of compounds that block volume-activatedanion channels in other preparations (Nilius et al., 1997a,b),such as tamoxifen (30 µM), pBPB (50 µM), mibefradil (30 µM), orDPC (300 µM) (Fig. 2C). This pharmacological profile is similar,although not identical, to that reported in the SON. The maindifferences are the lower sensitivity to ATP and the total absenceof blockade by DPC in the neurohypophysis, the latter inhibitingtaurine release in the SON with an IC₅₀ of 280 µM (Brès et al.,2000). Such a difference was seen in parallel experiments on SONand neurohypophysis using the same batch of DPC.

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Figure 2. Pharmacological properties of taurine release. A, B, Both basal release and that evoked by a hypotonic stimulus are blocked by the anion channel antagonists DIDS (A) and NPPB (B). C, Pharmacological profile of taurine release evoked by a 250 mOsm/l hypotonic stimulus. Inhibition was estimated as described previously (Brès et al., 2000). Number of observations are indicated above the bars.

Taurine-activated GlyRs on neurohypophysial nerve terminals

To check for a possible action of taurine on nerve terminals, those were isolated from neurohypophysis using a differentialcentrifugation method (Cazalis et al., 1987), and their activitywas monitored by spectrofluorimetry using the Ca²⁺ indicator fura-2. Because an inhibitory effect may be manifestonly when the terminals are formerly excited, the effect of taurinewas tested both in resting conditions and on the Ca²⁺ entry through voltage-activated Ca²⁺ channels evoked by a depolarizing high K⁺ solution (Brethes et al., 1987). A moderate concentration ofK⁺ (25 mM) was chosen to allow inhibitory currents to modulate Ca²⁺ channel activation. A 10 sec application of this high K⁺ solution induced a transient increase in intracellular Ca²⁺ concentration ([Ca²⁺]_i) that went from 154 ± 10 to 631 ± 37 nM (n = 28). Applicationof taurine (0.5 mM) did not affect resting [Ca²⁺]_i level but strongly and reversibly inhibited the increase in[Ca²⁺]_i evoked by depolarization (Fig. 3A). On average, inhibitionby taurine was 65 ± 5% (Fig. 3C). The effect of taurine was inhibitedby 69 ± 11% (n = 6) when it was coapplied with the GlyR antagoniststrychnine (1 µM) (Fig. 3A,C). Because taurine can also activateGABA_A receptors, albeit with a lower potency (Hussy et al., 1997),and because these receptors are expressed on neurohypophysialnerve terminals (Zhang and Jackson, 1995), we tested the effectof the GABA_A receptor antagonist gabazine. Gabazine (3 µM) wasunable to prevent the inhibitory effect of taurine (Fig. 3B,C).Preapplication of 20 µM glycine also inhibited the depolarization-induced[Ca²⁺]_i rise (76 ± 3% inhibition) (Fig. 3D,E), and this effect wassensitive to 1 µM strychnine, with a 71 ± 13% block of glycineaction (n = 4) (Fig. 3D,E). Therefore, taurine and glycine activateGlyRs on neurohypophysial nerve terminals to reduce the depolarization-evokedCa²⁺ influx.

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Figure 3. Taurine activates GlyRs on acutely isolated neurohypophysial nerve terminals. A, The [Ca²⁺]_i rise induced by a 10 sec application of a high K⁺ solution is inhibited in a strychnine-sensitive manner by taurine (preapplied for 30 sec and coapplied with high K⁺). B, The GABA_A receptor antagonist gabazine does not prevent the inhibitory action of taurine. C, Mean values of the inhibitory effect of taurine (left), its blockade by strychnine (middle), and lack of effect of gabazine (right). Numbers of observations are indicated above the bars. D, Glycine also inhibits high K⁺-induced [Ca²⁺]_i transients, and this effect is blocked by strychnine. E, Mean values of the inhibitory effect of glycine (left) and its blockade by strychnine (right).

Inhibition of Ca²⁺ influx should result in inhibition of hormone secretion (Cazalis et al., 1987; Stuenkel and Nordmann, 1993).This was verified by measuring VP release from purified isolatedneurohypophysial nerve terminals, using radioimmunoassay. Releasecould be evoked consistently by a 5 min application of 25 mM K⁺, which increased basal release 2.5-fold to 3.5-fold (Fig. 4),going on average from 40 ± 2 to 107 ± 3 pg/min (n = 16). A 5 minpreincubation with 0.5 mM taurine strongly inhibited high K⁺-evoked release, with a peak release in the presence of taurineof only 48 ± 3 pg/min (n = 6) (Fig. 4B), corresponding to an 82%inhibition. This inhibitory effect of taurine was primarily preventedwhen it was coapplied with 1 µM strychnine, with evoked releasereaching then 99 ± 6 pg/min (n = 6) (Fig. 4C).

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Figure 4. Taurine inhibits VP release on isolated neurohypophysial nerve terminals via activation of GlyRs. A 5 min application of a high K⁺ solution evokes an increase in VP release (top; n = 4), which is strongly inhibited in the presence of taurine (preapplied for 5 min and coapplied with high K⁺; middle; n = 6). Taurine-induced inhibition is prevented in the presence of strychnine (bottom; n = 6).

Immunohistochemical visualization of GlyRs in the neurohypophysis

The presence of GlyRs in the neurohypophysis was confirmed by immunohistochemistry, using a monoclonal antibody recognizingall subunits of GlyR (mAb4a). Intense GlyR immunostaining wasdetected both within the gray matter regions of spinal cord (datanot shown) and throughout the neurohypophysis (Fig. 5A). Examinationof double-immunostained sections under confocal microscopy furtherindicated that, within the neurohypophysis, the large majorityof GlyR immunostaining was associated with VP- or OT-immunopositiveaxonal structures of various size (Fig. 5C-H), including smallaxonal endings and large preterminal dilatations (also known asHerring bodies) (Hatton, 1999). Noteworthy is the observationthat, in contrast to VP terminals, some OT-immunopositive nerveendings were not labeled with the GlyR antibody.

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Figure 5. Immunohistochemical detection of GlyRs in the neuro-intermediate lobe. A, Intense immunostaining for the GlyR antibody mAb4a is associated with axon-like structures localized in the neurohypophysis, both the small axon terminals and the large preterminal swellings called Herring bodies (arrows). Note the absence of staining in the intermediate lobe (IL). B, No labeling is detected when the primary antibody is omitted. C-H, Double immunostaining for GlyR (C, F) and either VP (D) or OT (G), with superimposed images shown in E and H. The majority of GlyR immunostaining in the neurohypophysis colocalizes with axon terminals and Herring bodies (arrows) immunolabeled for either VP or OT (colocalization appears in yellow in E and H). Note that, in contrast to VP axons, a number of OT axons are devoid of GlyR immunostaining (red structures in H). V, Blood vessels. Scale bars (shown in B): A, B, 150 µm; (shown in H) C-H, 75 µm.

Taurine- and GlyR-dependent osmoregulation of VP release in the neurohypophysis

The results described above suggested that glial taurine and GlyRs could be involved in the osmotic regulation of neurohormonerelease. This was investigated by measuring VP release by radioimmunoassayfrom isolated whole neurohypophyses, in which glial-axon contactsshould still be functional. To prevent depletion of intracellulartaurine, a low concentration of taurine (1 µM, lower than normalblood concentration) (Huxtable, 1992) was added to all extracellularsolutions. VP release was evoked by a depolarizing high K⁺ solution (50 mM). This concentration of K⁺ evoked a consistent, robust increase in VP release from neurohypophysis(from 237 ± 18 to 726 ± 150 pg/min, corresponding to a threefoldincrease; n = 7) (Fig. 6) but was still primarily smaller thanthe ninefold maximal stimulation observed with 100 mM K⁺ (data not shown), thus allowing to study the effects of modulatoryfactors. Basal VP release was not affected by a 20 min applicationof a 20 mOsm/l hypo-osmotic solution, corresponding to a 6.6%decrease in osmolarity (216 ± 21 pg/min; n = 9) (Fig. 6A). Toquantify and compare evoked release, we considered the amountof VP released during 5 min taken in the middle of the applicationof the high K⁺ solution and normalized it to basal release measured during anequivalent period before stimulation. High K⁺-evoked release was significantly inhibited by preapplicationof the hypo-osmotic medium, decreasing from 306 ± 26 to 191 ±19% of basal release (n = 9; p < 0.005, unpaired Student's t test),which corresponded to a 56% inhibition (Fig. 6). Inhibition byhypo-osmolarity was completely prevented when 1 µM strychninewas added to the hypo-osmotic solution (305 ± 32% of basal; p< 0.01) (Fig. 6). Therefore, the inhibitory effect of the hypo-osmoticstimulus on the depolarization-evoked release of VP mainly involvesactivation of GlyRs.

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Figure 6. Hypo-osmotic regulation of VP release from isolated neurohypophysis involves GlyRs and requires the presence of taurine. A, Release evoked by high K⁺ (10 min), but not basal release, is antagonized by a 20 mOsm/l hypotonic stimulus (preapplied for 20 min and coapplied with high K⁺). Each curve is the mean of seven to nine measurements. This inhibition is blocked in the presence of strychnine. Taurine (1 µM) was added to all media to preserve the intracellular taurine level. B, Mean values of evoked release of VP and strychnine-sensitive blockade by hypotonic stimulus in the presence of 1 µM extracellular taurine (left). A 2.5 hr pretreatment with 1 mM GES in the absence of extracellular taurine to deplete taurine from the tissue totally prevents the inhibitory effect of the hypotonic stimulus (right).

To verify that taurine is indeed the endogenous agonist of GlyRs in hypotonic conditions, neurohypophyses were perfused for2.5 hr in the absence of extracellular taurine and the presenceof 1 mM of the taurine transport inhibitor GES. Such treatmentwas performed to partially deplete intracellular taurine frompituicytes (Morán et al., 1994). GES was then washed out for30 min to prevent any direct action of GES on VP release, andthe effect of hypo-osmotic stimulus was tested. In these conditions,VP release evoked by high K⁺ (395 ± 44% of basal) was no longer inhibited by the hypo-osmoticsolution (411 ± 69% of basal) (Fig. 6B). Therefore, the strychnine-dependentinhibition of evoked VP release requires a high level of intracellulartaurine, identifying the endogenous activator ofGlyRs.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We demonstrate here that neurohormone secretion within the neurohypophysis is subject to local osmo-dependent regulation.This regulatory process involves the release of glial taurineduring hypo-osmotic stimulation through volume-sensitive anionchannels. Taurine then inhibits evoked hormone secretion via theactivation of GlyRs present on neurohypophysial nerve terminals.This mechanism is strikingly similar to that hypothesized previouslyin the SON and as so validates and extends this model of osmoregulation(Hussy et al., 2000). Taurine- and GlyR-dependent osmoregulationof neuroendocrine activity therefore occurs both at the levelof the soma and dendrites of magnocellular neurons, in the SON,and at the level of their axon terminals, in the neurohypophysis.Moreover, this report constitutes the first description of thefunctional expression of GlyRs on an axon terminal, which servesthe atypical function of mediating a slow, nonsynaptic, glia-to-neurontransmission. The high osmosensitivity of taurine and VP releasesconstitutes a strong indication that such a process actually takesplace during physiological variations of osmoticpressure.

Taurine release

We showed that release of taurine is induced by hypo-osmotic stimulus in the neurohypophysis. Because taurine is selectivelyconcentrated in the pituicytes that ensheathe the nerve terminals(Pow, 1993; Miyata et al., 1997), release likely comes from thisglial compartment. In the SON, selective accumulation of taurineby astrocytes (Decavel and Hatton, 1995) has been correlated clearlyto a pure glial origin of released taurine (Deleuze et al., 1998).Release of taurine in the neurohypophysis is highly sensitiveto even small changes in osmotic pressure. Decrease of releaseby hyper-osmotic stimulus indicates a sustained osmo-dependentrelease in isotonic conditions. Release was not antagonized bythe taurine transporter inhibitor GES but was blocked by variousCl channel blockers, indicative of the implication of volume-sensitiveanion channels, as seen in most cell preparations (Strange andJackson, 1995; Nilius et al., 1997a; Pasantes-Morales and Schousboe,1997). The properties of taurine release in the neurohypophysisare mostly similar to those described in the SON (Deleuze et al.,1998; Brès et al., 2000). One difference is the lower sensitivityto ATP in the neural lobe, but this could be attributable to agreater degradation of ATP. Indeed, whereas SON astrocytes arereadily accessible to applied drugs because of their locationat the ventral side of the nucleus (Hatton, 1999), ATP will haveto penetrate the complex structure of the neurohypophysis to accessthe pituicytes, being then more exposed to ectonucleotidases.More striking is the absence of effect of DPC in the neurohypophysis,although this compound blocks efficiently release in the SON (Brèset al., 2000). This could mean that SON astrocytes and neurohypophysialpituicytes express a different subtype of volume-sensitive anionchannels, but for a clear conclusion to be drawn, we will haveto wait for the knowledge of the exact site of action of the blocker(Ballatori et al., 1995).

GlyRs on neurohypophysial nerve terminals

Taurine activates strychnine-sensitive GlyRs on nerve terminals isolated from neurohypophysis. Large expression of GlyRs inboth VP and OT terminals (although possibly larger in VP thanOT terminals) was confirmed by immunohistochemistry. Activationof these receptors leads to opening of Cl channels and results in an inhibition of the depolarization-evoked[Ca²⁺]_i rise, which has been shown previously to depend exclusivelyon Ca²⁺ entry through voltage-activated Ca²⁺ channels (Brethes et al., 1987). As expected from the close relationshipbetween Ca²⁺ entry and neurohormone release (Cazalis et al., 1987; Stuenkeland Nordmann, 1993), GlyR activation by taurine also blocks depolarization-evokedrelease of VP from purified nerve terminals. The Cl concentration in neurohypophysial terminals in situ has beenestimated to be 20 mM from measurements of GABA_A receptor responses(Zhang and Jackson, 1995), yielding an equilibrium potential forCl ions (E_Cl of $-$ 48 mV) slightly more depolarized than the restingpotential of the terminals (Zhang and Jackson, 1995; Branshawet al., 1998). Activation of a Cl conductance will thus depolarize the terminals but not sufficientlyto activate voltage-dependent Na⁺ or Ca²⁺ currents. Despite this depolarizing influence, it will resultin an inhibition of the terminal excitability. In the case ofhigh K⁺-evoked Ca²⁺ entry in isolated terminals, activation of Ca²⁺ channels is the mere consequence of the depolarizing action ofhigh K⁺, because it is not blocked by inhibition of Na⁺ channels by TTX (G. Dayanithi, unpublished observation). Becauseactivation of the GlyR Cl current will lower the depolarization evoked by high K⁺ by pulling the membrane potential toward E_Cl, it will reducethe level of activation of Ca²⁺ channels, thus accounting for the inhibition of Ca²⁺ entry. The mechanism of inhibition in situ is, however, different,as shown for GABA_A receptors, which activation inhibits Na⁺-dependent spike propagation into neurohypophysial nerve terminalsmainly through the voltage-dependent inactivation of axonal Na⁺ channels consecutive to the Cl current-induced depolarization (Zhang and Jackson, 1995; Branshawet al., 1998). A similar consequence of GlyR activation can reasonablybeexpected.

Implication of GlyR and taurine in the osmoregulation of VP release

Finally, we showed the inhibition of neurohypophysial VP release by moderate hypo-osmotic stimulus. This effect depends onactivation of GlyRs, further implying the receptors in the osmoregulationof neurosecretory activity. Therefore, inhibition of VP secretionby a hypo-osmotic stimulus probably results from the decreasedCa²⁺ influx induced by activation of GlyR Cl currents. Because GlyRs can be visualized in both VP and OT terminalsin situ and because all isolated terminals express functionalGlyRs, such regulation likely applies to OT release as well. However,the detection of some OT terminals not labeled with the GlyR antibodymay suggest a lower impact on OT release. Basal, nonstimulatedVP secretion is unaffected by hypotonic stimulus or by the blockadeof GlyRs by strychnine, despite the increased release of taurine.This observation can be explained by the activity independenceof basal hormone release from nerve endings, which is not blockedby removal of external Ca²⁺ (Cazalis et al., 1987), by chelating intracellular Ca²⁺ with BAPTA (Stuenkel and Nordmann, 1993) or by blocking Na⁺ channels with TTX (G. Dayanithi, unpublished observation). Therefore,basal release should not be affected by changes in membrane potentialor resistance and thus by activation of the Clconductance.

Removal of this regulatory mechanism by depletion of taurine clearly identifies glial taurine as the endogenous activatorof GlyRs, in agreement with the lack of detection of glycine inthe neurohypophysis (Pow, 1993) and our previous inference fromdata on the osmoregulation of SON neuron activity (Hussy et al.,2000). Taurine is thus released by glial cells under such osmoticconditions in a sufficient amount to activate GlyRs, as hypothesizedpreviously (Hussy et al., 1997, 2000; Hatton, 1999) based on thehigh concentration gradient for taurine (a few tens of millimolarinside cells vs at most a few tens of micromolar in the extracellularfluid) (Kimelberg et al., 1990; Huxtable, 1992; Martin, 1992),the reduced extracellular space by hypo-osmolarity-induced cellswelling, and the apparent affinity of GlyRs for taurine (EC₅₀of ~400 µM in SON neurons) (Hussy et al., 1997). Pituicytes andSON astrocytes therefore act as sensory elements, releasing inan osmo-dependent manner a glia-to-neuron transmitter, taurine.The role of GlyRs as receptors for slow transmission of glialinformation is quite uncommon for ionotropic receptors. However,this peculiar function may not be restricted to the hypothalamo-neurohypophysialsystem and could explain the failure to detect glycinergic synaptictransmission in some brain neurons expressing GlyRs (Kaneda etal., 1995). Extrasynaptic activation of GlyRs by endogenous taurinehas also been reported in developing cortical neurons (Flint etal., 1998). Whether the implication of GlyRs in the osmoregulationof neuronal electrical and secretory activities is a common mechanismor is specifically related to the particular involvement of SONneurons in the regulation of water balance has still to bedetermined.

Osmoregulation of neuroendocrine function is a highly complex process, which was known to result from the integration of theosmotic information coming from multiple osmoreceptors locatedboth inside and outside the nervous system, as well as from theosmosensitivity of magnocellular neurons within the SON and PVN(Bourque et al., 1994; Hussy et al., 2000). Our data show thatosmoregulation also takes place in the neurohypophysis, actingat the last stage of the hypothalamo-neurohypophysial system,the axon terminals, to directly modulate secretion of neurohormones.Osmoregulation of SON neuron activity involves both neuronal mechanoreceptorsand the glial taurine-GlyR system (Hussy et al., 2000). It willbe of interest to know whether mechanoreceptors are also presenton neurohypophysial nerve terminals to complement regulation byGlyRs in a manner similar to that observed in theSON.

  FOOTNOTES

Received Feb. 22, 2001; revised July 2, 2001; accepted July 5, 2001.

This work was supported in part by Centre National d'Etudes Spatiales Grant 98/7346/793. We thank C. Deleuze, V. Chevaleyre,A. Rabié, and M. G. Desarménien for critical reading of thismanuscript and E. Bourinet for kindly providingmibefradil.
Correspondence should be addressed to Nicolas Hussy, Centre National de la Recherche Scientifique Unité Mixte de Recherche5101, CCIPE, 141 rue de la Cardonille, 34094 Montpellier Cedex5, France. E-mail: hussy{at}bacchus.montp.inserm.fr.

V. Brès's present address: Centre National de la Recherche Scientifique Unité Propre de Recherche 1142, Institut de GénétiqueHumaine, 141 rue de la Cardonille, 34396 Montpellier Cedex 5,France.

M. Rochette's present address: Mayo Clinic, Birdsall Building, 4500 San Pablo Road, Jacksonville, FL32224.

G. Dayanithi's present address: Institut National de la Santé et de la Recherche Médicale U432, Université MontpellierII, Place E. Bataillon, 34095 Montpellier Cedex 5,France.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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