Nitric Oxide and the Oxytocin System in Pregnancy

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NITRIC OXIDE
OXYTOCIN
VASOPRESSIN

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The Journal of Neuroscience, September 1, 2000, 20(17):6721-6727

Nitric Oxide and the Oxytocin System in Pregnancy
Rungrudee Srisawat, Mike Ludwig, Philip M. Bull, Alison J. Douglas, John A. Russell, and Gareth Leng
Department of Biomedical Sciences, University of Edinburgh Medical School, Edinburgh EH8 9XD, United Kingdom

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We examined the functional role of the nitric oxide (NO)-producing system in magnocellular neurons and how this changes atthe end of pregnancy, using a combination of blood sampling andoxytocin radioimmunoassay, electrophysiology, immunocytochemistryfor Fos expression, and in situ hybridization histochemistry.In urethane-anesthetized virgin rats, systemic administrationof NO synthase (NOS) inhibitors led to a facilitation of oxytocinrelease evoked by hyperosmotic stimulation. Direct applicationof the NO donor sodium nitroprusside to the supraoptic nucleusby in vivo microdialysis inhibited the electrical activity ofboth oxytocin neurons and vasopressin neurons, whereas directapplication of an NOS inhibitor increased electrical activity,indicating that endogenous NO acts within the supraoptic nucleusto inhibit neuronal activity. However, during late pregnancy,the influence of endogenous NO is dramatically downregulated,reflected by a reduced expression of neuronal NOS mRNA in theseneurons and a loss of efficacy of NOS inhibitors on stimulus-evokedoxytocin release. This downregulation may cause the oxytocin systemto become more excitable at term, resulting in the capacity forgreater release of oxytocin duringparturition.

Key words: supraoptic nucleus; microdialysis; osmotic stimulation; in situ hybridization; Fos expression; hypothalamus

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In pregnancy, stores of oxytocin in the posterior pituitary gland of the rat accumulate in anticipation of secretory demand.The pituitary content increases by ~50% from the beginning tothe end of pregnancy, and this accumulated excess will be releasedduring the 60-90 min of parturition and plays an important rolein promoting uterine contraction and birth (Russell and Leng,1998). Thus, relatively abruptly at the end of pregnancy, theoxytocin system switches from active restraint of secretion (toallow stores to accumulate) to hypersecretion. It is now clearthat a number of mechanisms actively contribute to this switchand that these particularly involve the actions of factors secretedfrom the oxytocin cells themselves. One of these factors, as wedescribe here, is nitric oxide(NO).

Neuronal nitric oxide synthase (nNOS) is expressed nowhere more densely than in the magnocellular neurosecretory neurons ofthe supraoptic nuclei (SON) and paraventricular nuclei (PVN).This expression is functionally regulated (Sagar and Ferriero,1987; Bredt et al., 1990; Pow, 1992; Vincent and Kimura, 1992);increases in nNOS mRNA expression and nicotinamide adenine dinucleotidephosphate (NADPH)-diaphorase staining (a NOS marker) in the SONand PVN (Kadowaki et al., 1994; Villar et al., 1994) and increasesin NO-forming activity in the posterior pituitary (Kadowaki etal., 1994) all accompany chronic saltloading.

Most reports suggest that NO is inhibitory to both oxytocin cells and vasopressin cells in the SON and PVN. In electrophysiologicalstudies in vitro, the NO donor sodium nitroprusside (SNP) andthe NO precursor L-arginine inhibit supraoptic neurons, whereasthe NOS inhibitor N-nitro-L-arginine methyl ester (L-NAME) and the NO scavenger hemoglobinenhance neuronal activity (Liu et al., 1997). Application of theNO donor S-nitroso-N-acetylpenicillamine increases the frequency,but not the amplitude, of spontaneous IPSCs recorded from supraopticneurons but has no effect on EPSCs (Ozaki et al., 2000). Thus,it has been hypothesized that NO inhibits supraoptic neurons byacting presynaptically at terminals of GABA neurons rather thanby a directeffect.

However, a recent report has suggested that NO may be functionally excitatory. Yang and Hatton (1999) report that SNP increasesdye-coupling among supraoptic neurons and that cGMP, via whichNO is thought to act, excites supraoptic neurons in vitro. Theseauthors speculate that NO may play a role in neuronal hyperexcitabilityunderlying the high-frequency burst firing that is displayed byoxytocin cells in response to suckling (Yang and Hatton, 1999).Such burst firing occurs during parturition and lactation butis never seen in virgin rats, and it is believed that the expressionof the ability to discharge in synchronized bursts requires a"remodeling" of the oxytocin cells in the SON and PVN and theirinputs, and that this remodeling is driven, indirectly, by thesteroid environment of pregnancy (Montagnese et al., 1990).

In this study, we examined the functional role of the NO-producing system in magnocellular neurons and how this changes atthe end ofpregnancy.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Age-matched female Sprague Dawley rats (250-300 gm) were housed under standard laboratory conditions (12 hr dark/light cycle;22 ± 1°C) with access to food and water ad libitum. Pregnant ratswere obtained by leaving virgin rats with stud males overnight;day 0 of pregnancy was determined by the appearance of a vaginalplug of semen shed into the mating cage. The rats were then housedindividually with food and water ad libitum. In these conditions,rats normally gave birth on the afternoon of day 22 ofpregnancy.

All studies were on rats anesthetized with urethane (ethyl carbamate, 1.2 gm/kg, i.p.) or, for studies of Fos expression,with sodium pentobarbitone (Sagatal; 50 mg/kg, i.p; Rhône Mérieux,Hertfordshire,UK).

Blood sampling. Blood samples of 0.3 ml were withdrawn from the left femoral artery via a polythene cannula and heparinized.The plasma was separated by centrifugation and stored at $-$ 20°C.The blood cells were resuspended in isotonic saline (0.15 M NaCl)at the same volume as the plasma taken and returned via the leftfemoral vein. Plasma [Na⁺] was determined using a Corning (Corning, NY) 455 flamephotometer.

Radioimmunoassay. On the day of assay, plasma samples were thawed and centrifuged. Oxytocin radioimmunoassay was performedusing the specific anti-oxytocin antiserum (Higuchi et al., 1985).All samples in each experiment were measured in a single assayto avoid interassayvariance.

Intravenous injections were administered via a cannula in the left femoral vein. All drugs were made up in isotonic saline,and control rats were given equivalent volumes of isotonic salinealone.

Effect of NOS inhibitors and SNP on oxytocin release. In experiment 1, virgin rats were injected intraperitoneally with eitherN-nitro-L-arginine (L-NNA) (10 mg/kg; Sigma, Poole, UK) or isotonicsaline. In experiment 2, rats were injected intraperitoneallywith either L-NAME HCl (50 mg/kg; Sigma) or isotonic saline. BothL-NNA and L-NAME compete with L-arginine for binding the arginine-bindingsite of NOS. After 4 hr, rats were injected intravenously withcholecystokinin (CCK) (20 µg/kg, cholecystokinin-(26-33)-sulfated;Bachem Ltd., Saffron Walden, Essex, UK), followed by 4 ml/kg 1.5M NaCl, intraperitoneally. Blood samples were collected beforeand after eachinjection.

In a further experiment, a guide cannula was inserted stereotaxically into a lateral cerebral ventricle, at least 2 hr beforeblood sampling before and after intraperitoneal hypertonic salineas above, for infusion of SNP (10 nmol/µl: 5 µl at 2 µl/min andthen 20 µl at 0.7 µl/min; Sigma) or vehicle, starting with theintraperitonealinjection.

The effect of L-NNA on Fos expression in rats treated with low doses of hypertonic saline. Virgin rats were pretreated witheither L-NNA (10 mg/kg, i.p.) or vehicle (isotonic saline). After4 hr, the rats were injected intraperitoneally with 2 ml/kg ofeither 1.5 M NaCl or isotonic saline and were decapitated 90 minlater. The brains were frozen and stored at $-$ 70°C. Frozen coronalsections (15 µm) were cut, fixed in 4% paraformaldehyde in 0.1M phosphate buffer (PB) pH 7.3-7.4 for 30 min, and washed in 0.1M PB. Endogenous peroxidase was blocked with hydrogen peroxidesolution 0.3%, with methyl alcohol 20% for 15 min. The slideswere then washed with PB-T (0.1 M PB containing 0.3% Triton X-100).Nonspecific binding was blocked by preincubation with 1% normalsheep serum for 1 hr. The sections were then incubated with apolyclonal antibody raised in rabbits against rat Fos (c-fos Ab-2;Oncogene Sciences, Uniondale, NY) at 1:1000 in preincubation buffercontaining 1% normal sheep serum. After 48 hr, the sections werewashed with PB-T and incubated for 24 hr with goat anti-rabbitIgG-peroxidase complex (Vector Laboratories, Orton Southgate,UK) at 1:1000 in buffer containing 1% normal sheep serum. Thesections were washed with PB-T, rinsed with 0.1 M acetate buffer,and incubated with glucose oxidase-Ni diaminobenzidine (DAB) (Sigma)solution. The reaction was terminated with stop solution (0.1M acetate buffer). The sections were then rinsed and dehydratedthrough serial concentrations of ethanol (70, 90, 95, and twicein 100%) and then into xylene before beingcoverslipped.

In a subsequent experiment, to test the effectiveness of L-NNA against a higher dose of hypertonic saline, virgin rats werepretreated with L-NNA (10 mg/kg, i.p.) or vehicle (isotonic saline).After 4 hr, rats were injected intraperitoneally with 4 ml/kg1.5 M NaCl. After 90 min, the rats were perfused transcardiallywith isotonic saline, followed by 4% paraformaldehyde in 0.1 MPB, pH 7.4. The brains were post-fixed for 2-5 hr, cryoprotectedin 30% sucrose in fixative overnight at 4°C, and then left in30% sucrose in PB at 4°C until they sank. Brains were then sectionedcoronally (50 µm) on a freezing microtome. Free-floating sectionswere washed in PB-T, endogenous peroxidase was deactivated, andnonspecific staining was blocked as above. The sections were incubatedfor 48 hr in Ab-2 Fos antibody and then in 1% biotinylated anti-rabbitimmunoglobulin (Vector Laboratories) and 3% normal goat serumin PB-T for 1 hr, and then washed in PB-T (three times for 10min each) and incubated in ABC complex solution (2% avidin DHand 2% biotinylated horseradish peroxidase in PB-T; Vector Laboratories)for 1 hr. The sections were then washed in PB-T, rinsed with 0.1M acetate buffer, and incubated with glucose oxidase-Ni DAB solutionfor 10 min. The reaction was terminated with stop solution, andsections were rinsed with PB, mounted serially, and left to dry.The sections were then dehydrated asabove.

The role of NO in the electrical activity of oxytocin and vasopressin cells. A femoral vein and the trachea were cannulated,and the pituitary stalk and right SON were exposed transpharyngeallyas described in detail previously (Leng and Dyball, 1991). Briefly,this surgery involves exposure of the sphenoid bone and the lateralwing of the palatine bone after cautery of the soft palate atthe roof of the mouth. A small burr hole is drilled in the sphenoidbone above the neural stalk. To expose the SON, a portion of thebone overlying the trigeminal nerve is removed, and the nervebundle, which lies between that and the dura overlying the SON,is dissected away. A U-shaped dialysis probe (membrane length,2.0 mm; Spectra/Por RC Hollow Fibers, Spectrum Medical Inc., GreatFalls, MT) was bent to position the loop of the membrane flatonto the exposed ventral glial lamina of the SON after removalof the meninges. A glass micropipette (filled with 0.15 M NaCl,20-40 M $Omega$ ) was introduced into the center of the loop to recordthe extracellular activity of single neurons in the SON (Ludwigand Leng, 1997). A bipolar stimulating electrode (SNEX-200X; ClarkeElectromedical Instruments, Reading, UK) was placed on the pituitarystalk and set to deliver single matched biphasic pulses (1 msec,< mA peak to peak) for antidromic identification of supraopticneurons. Neurons were identified as oxytocin cells by a transientexcitation and as vasopressin cells by no effect or short-terminhibition after intravenous injection of 20 µg/kg CCK (Renaudet al., 1987). The firing rates of cells were recorded using Spike2software (Cambridge Electronic Design, Cambridge, UK). ArtificialCSF (aCSF), pH 7.2 (in mM: NaCl 138, KCl 3.36, NaHCO₃ 9.52, Na₂HPO₄0.49, urea 2.16, and MgCl₂ 1.18) was dialyzed at 3 µl/min throughoutthe experiment. During recording, dialysis fluid was changed toaCSF containing SNP (10 mM, 100 mM), L-arginine (100 mM; Sigma),or L-NNA (10 mM). The concentrations of drugs in the dialysateare considerably in excess of those achieved in the extracellularfluid. From previous experiments that established the dialysisconcentration of tetrodotoxin needed to block spike activity inmagnocellular neurons, we can estimate that the concentrationsachieved within the main body of the SON by dialysis of the ventralzone are approximately three orders of magnitude lower (Ludwigand Leng, 1997).

The effect of NOS inhibitors and naloxone in late pregnancy. Age-matched virgin and day 22 pregnant rats were injected withL-NNA (10 mg/kg, i.p.) or isotonic saline. Four hours later, therats were injected intraperitoneally with hypertonic saline (virgin,4 ml/kg 1.5 M NaCl, i.p.; pregnant, 5 ml/kg 2 M NaCl). Becauseplasma [Na⁺] is reduced in pregnancy, the volume given to pregnant rats wasgreater than that given to virgin rats to produce a similar elevatedplasma [Na⁺]. Naloxone hydrochloride (5 mg/kg; Sigma) was injected intravenously40 min after the hypertonic saline. Plasma samples were collectedbefore and after eachinjection.

The effect of NOS inhibitors on oxytocin release after intravenous infusion of hypertonic saline in late pregnancy. Age-matchedvirgin and day 22 pregnant rats were injected intraperitoneallywith L-NNA (10 mg/kg) or isotonic saline. Four hours later, therats were infused intravenously with 2 ml of hypertonic salineover 1 hr (2 M NaCl in virgin rats and 2.6 M NaCl in pregnantrats). The different concentrations were chosen after pilot experimentshad indicated that these would produce a similar plasma [Na⁺] in virgin and pregnant rats at the end of the infusion. Bloodsamples were collected before, and every 10 min during, theinfusion.

NOS mRNA expression in the SON and PVN in pregnancy. Age-matched virgin, 16 d pregnant, and 22 d pregnant rats were decapitatedin the morning, and parturient rats were decapitated 2 hr afterthe birth of the first pup. The brains were frozen on dry iceand stored at $-$ 70°C. Coronal sections (15 µm) were cut on a cryostat,thaw-mounted onto gelatin-coated RNase-free slides, and storedat $-$ 70°C. Three 45-mer antisense oligonucleotide probes were used,complementary to bases 223-267 (5'-noncoding region), 4714-4758(3'-noncoding region) and 1662-1706 of the rat nNOS sequence (Bredtet al., 1991), and labeled at the 3' end with [ $alpha$ -³⁵S]deoxy-ATP (NEN, Boston, MA) using terminal deoxynucleotidyltransferase (Amersham Pharmacia Biotech, Little Chalfont, UK).The probe-specific activities were 482-1753 Ci/mmol.

Sections were fixed at room temperature with 4% paraformaldehyde in 0.1 M PB, pH 7.4, for 30 min, rinsed, and washed in 0.1M PBS, followed by acetylation in triethylamine solution (0.25%acetic anhydride in 0.1 M triethylamine-0.15 M NaCl) for 10 minto increase tissue permeability. The sections were then dehydratedthrough 70, 80, 95, and 100% ethanol, delipidated in chloroform,and partially rehydrated in 95% ethanol. After air-drying, theslides were placed in a humidified chamber. The sections werehybridized for 17 hr at 37°C in 40 µl of hybridization buffer[4× SSC, 50% formamide, 1× Denhardt's solution, 500 µg/ml shearedsalmon sperm DNA (Sigma), 10% dextran sulfate, and 0.3% mercaptoethanol]containing ³⁵S-labeled NOS oligonucleotide probes at 2500 dpm/µl. The slideswere stringently washed in SSC at 55°C, dipped in 300 mM ammoniumacetate, 70% ethanol, air-dried, placed in autoradiographic cassettes,and exposed to Hyperfilm- $beta$ max autoradiography film (Amersham PharmaciaBiotech) with ³⁵S brain paste standards. The films were exposed for 3 weeks at4°C, developed, and fixed. The sections were then dipped in IlfordG-5 emulsion and exposed for 4-5 weeks and then developed andfixed. The sections were then counterstained with cresyl violet,dehydrated in a graded ethanol series, andcoverslipped.

The nNOS mRNA was assessed by silver grain density of autoradiographic films, quantified (5× and 10× objective) using theNIH Image analysis system version 1.58. The density per unit areawas obtained by subtracting background measurements over adjacenttissue from each specific tissue measurement and dividing by thearea measurements. A logarithmic relationship was plotted forradioactivity against the grain density of the standards. Acceptablegrain density values lay on the straight portion of the curve.For each rat, the mean grain density per unit area was calculatedfor each brain region, and the group means werecalculated.

Statistical analysis. All data are reported as means ± SEM. Data were analyzed statistically by t test, one-way ANOVA, andtwo-way ANOVA for comparison differences between groups, a one-wayrepeated measures ANOVA for differences with time, and a two-wayrepeated measures ANOVA for differences between groups followedby Dunnett's method or Student-Newman-Keuls method. The pairedt test and the Wilcoxon signed rank test were used for comparingdifferences between, before, and after treatments withingroups.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effect of NOS inhibitors and an NO donor on oxytocin secretion in virgin rats

Urethane-anesthetized rats were injected intraperitoneally with the NOS inhibitors L-NNA or L-NAME, or isotonic saline, followedby CCK and hypertonic saline to stimulate the secretion of oxytocin(Fig. 1). Hypertonic saline injections lead to a sustained activationof both oxytocin and vasopressin cells, and this activation involvesboth intrinsic osmoreceptivity of the magnocellular neurons andinputs arising from anterior, periventricular structures. In contrast,intravenous injection of CCK activates oxytocin cells transientlyand selectively via a noradrenergic projection from the brainstem(Leng et al., 1999).

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Figure 1. Plasma oxytocin concentration in virgin rats injected with CCK (20 µg/kg, i.v.) and hypertonic saline (4 ml/kg 1.5 M NaCl, i.p.) after pretreatment with L-NAME (A) or L-NNA (B), or vehicle controls. Note that L-NAME and L-NNA significantly enhanced oxytocin secretion evoked in response to hypertonic saline but not secretion evoked by CCK. Data are means ± SEM; n = 6-8 rats per group; *p < 0.05 compared with basal; #p < 0.05 compared with controls.

The NOS inhibitors alone had no significant effect on the basal plasma [Na⁺] or the basal plasma oxytocin concentration. After intravenousinjection of CCK, the plasma concentration of oxytocin increasedin all rats, and this response was similar in rats pretreatedwith L-NNA or L-NAME and their respective control groups. Injectionof hypertonic saline produced a much larger increase in the concentrationof oxytocin in all rats, and strikingly, the oxytocin releasewas significantly greater in rats pretreated with either L-NNAor L-NAME than in their respective control groups (p < 0.05) (Fig.1). In a converse experiment, intracerebroventricular infusionof SNP (250 nmol in 25 µl) for 30 min after an intraperitonealinjection of 1.5 M NaCl (4 ml/kg) significantly reduced the hyperosmoticstimulation of oxytocin secretion compared with intracerebroventricularvehicle-infused controls. In the latter, plasma oxytocin concentrationat 60 min after hypertonic saline had increased to 228.9 ± 51.0pg/ml from a basal 56.4 ± 9.3 pg/ml (n = 8), but after intracerebroventricularSNP infusion, plasma oxytocin concentration increased to only105.1 ± 25.9 pg/ml (n = 6; p < 0.05 vs intracerebroventricularvehicle) from a basal value similar tocontrols.

Thus, L-NNA and L-NAME had no significant effect on the basal release of oxytocin or on CCK-evoked oxytocin release but potentiatedthe release evoked by intraperitoneally injected hypertonic saline,suggesting that endogenous NO exercises a restraining influenceon the secretion of oxytocin evoked by intense osmotic stimulation.The effects of the NO donor SNP, given by intracerebroventricularinfusion, demonstrated the further capacity of exogenous NO toinhibit osmotically stimulated oxytocinsecretion.

The effect of L-NNA on Fos expression in the SON and PVN in rats treated with hypertonic saline

In pentobarbitone-anesthetized rats injected intraperitoneally with 2 ml/kg 1.5 M NaCl, Fos immunoreactivity was seen in neuronalnuclei of magnocellular neurons of the SON and PVN in both L-NNA-pretreatedand vehicle-pretreated rats and was primarily absent from surroundingareas of the hypothalamus (Fig. 2). The expression was significantlygreater than in control rats injected with isotonic saline (p< 0.05) but did not differ significantly between L-NNA-pretreatedand vehicle-pretreated rats. In contrast, in rats injected intraperitoneallywith a higher dose of hypertonic saline (4 ml/kg 1.5 M NaCl),more SON cells expressed Fos in L-NNA-pretreated rats than invehicle-pretreated rats (Fig. 2) (24% increase; p < 0.05). A similarproportional increase in expression was observed in the magnocellularPVN, but this did not reach statistical significance.

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Figure 2. Expression of Fos in the SON and PVN of rats pretreated with L-NNA or vehicle, followed by intraperitoneal injection of either isotonic saline or 2 or 4 ml/kg 1.5 M NaCl (A). Note that a significant increase in the number of Fos-positive neurons was observed in the SON of L-NNA-pretreated rats compared with vehicle-pretreated rats after intraperitoneal administration of the higher dose of hypertonic saline. Data are means ± SEM; numbers of rats are above bars; *p < 0.05 compared with controls. B-E, Photomicrographs of Fos expression 90 min after intraperitoneal injection of 4 ml/kg 1.5 M NaCl in the PVN (B, C) and SON (D, E) in L-NNA-pretreated rats (C, E) and vehicle-pretreated controls (B, D). Mp, Medial parvocellular; Pm, posterior magnocellular; OC, optic chiasm; V3, third ventricle. Scale bars, 100 µm.

Thus, the Fos expression induced in the SON after intraperitoneal injection of a large dose of hypertonic saline was enhancedby L-NNA, whereas L-NNA had no effect on Fos induced by a lesserosmotic stimulus, indicating that the enhancement of stimulatedoxytocin release after L-NNA (Fig. 1) reflects, at least in part,increased responsiveness of oxytocin cells to strongstimulation.

The influence of NO on the electrical activity of oxytocin and vasopressin cells

Single neurons, antidromically identified as projecting to the posterior pituitary, were recorded from the SON of urethane-anesthetizedrats while drugs were administered to the nucleus by retrodialysis.In the above experiments with systemic NOS inhibitors or intracerebroventricularinfusion of an NO donor, the effects on osmotically stimulatedoxytocin secretion could result from NO actions at several keysites in the osmoreceptor complex regulating magnocellular neurons.The in vivo electrophysiology studies were designed to test NOactions in the immediate vicinity of the magnocellular neurons.The spontaneous firing rate of both oxytocin cells and vasopressincells was inhibited by retrodialysis of SNP in a dose-dependentmanner (Fig. 3A-C). During retrodialysis of 100 mM SNP, the spontaneousfiring rate of four oxytocin cells decreased by 3.01 ± 1.11 spikes/sec(98% decrease), and that of 12 continuously firing vasopressincells decreased by 7.01 ± 0.63 spikes/sec (97% decrease). In eachof four phasically firing vasopressin cells, retrodialysis of100 mM SNP onto the SON for 45 min caused a significant decreaseof firing rate, which involved a decrease in intraburst firingrate, but was principally a consequence of reduced burst lengthand longer silences evident as reduced activity quotient (timeactive/time silent; p < 0.05) (Fig. 3C). After 45 min of SNP administration,the mean firing rate was decreased by 4.38 ± 1.62 spikes/sec (73%decrease), the mean burst length was decreased by 115.01 ± 65.16spikes/sec (93% decrease), and the activity quotient of thesephasic vasopressin cells was decreased by 0.58 ± 0.20 (72% decrease).

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Figure 3. Effects of local application of SNP, L-arginine, and L-NNA on activity of vasopressin and oxytocin neurons. A-C, Retrodialysis of SNP onto the SON inhibited the electrical activity of oxytocin (A) and vasopressin (B) neurons, repeatedly and dose-dependently (SNP1, 10 mM; SNP2, 100 mM). C, A significant decrease in the activity quotient and the burst length of phasic vasopressin neurons was observed after retrodialysis of 100 mM SNP. *p < 0.05; n = 5 at 0 and 15 min and 4 at 45 min, respectively. D, Inhibition of a continuously firing putative vasopressin neuron during administration of L-arginine. E, L-NNA administered over 60 min induced an increase in the firing rate of this vasopressin neuron, identified by its inhibitory response to intravenous CCK.

The inhibition of neuronal activity by SNP was thus similar for oxytocin cells and vasopressin cells and was dose-dependent.Pooling data for oxytocin and vasopressin cells, the mean inhibitionof firing rate in response to dialysis of 10 mM SNP (approximatelythree orders of magnitude above predicted extracellular concentration;see Materials and Methods) was 50 ± 9.6% (n = 6); in responseto 50 mM SNP, cells were inhibited by 86 ± 5.5% (n = 10), andin response to 100 mM SNP by 91 ± 3.7% (n =16).

Six cells (two oxytocin cells and four vasopressin cells) were recorded during dialysis infusion of L-arginine, and all wereinhibited during the infusion by a mean of 2.44 ± 0.84 spikes/sec(34% decrease) (Fig. 3D). Conversely, the firing rates of bothoxytocin cells and vasopressin cells increased after local administrationof L-NNA (Fig. 3E). The mean firing rate of five oxytocin cellsincreased by 0.83 ± 0.20 spikes/sec (13% increase), and the meanfiring rate of 12 vasopressin cells increased by 1.78 ± 0.36 spikes/sec(18% increase) after retrodialysis of 10 mM L-NNA.

Thus, endogenous local NO restrains the electrical activity of both oxytocin cells and vasopressin cells in vivo.

The effect of NOS inhibition on hypertonic saline-stimulated oxytocin release in late-pregnant rats

The similarity of the enhancement of oxytocin release in response to hypertonic saline by blockade of NOS with L-NNA to thatafter blockade of opioid receptors with naloxone (Russell et al.,1995) prompted us to investigate the relationship between thesetwo mechanisms and to study the role of NO at the end of pregnancywhen the opioid system in the neural lobe is downregulated (Lenget al., 1997).

Anesthetized adult virgin rats and late-pregnant rats were pretreated with L-NNA or isotonic saline and then given an intraperitonealinjection of hypertonic saline. The virgin rats were given 4 ml/kg1.5 M NaCl and the pregnant rats were given 5 ml/kg 2 M NaCl toproduce similar changes in plasma [Na⁺] in the two groups. The basal plasma [Na⁺] and oxytocin concentrations were similar in the groups pretreatedwith L-NNA or isotonic saline. The plasma [Na⁺] was increased after intraperitoneal injection of hypertonicsaline in all rats, to a similar extent in rats pretreated withL-NNA or isotonic saline (data not shown). In all rats, oxytocinrelease was increased 30 min after injection of hypertonic saline.Again, in virgin rats, this response was significantly greaterin rats pretreated with L-NNA than in controls (p < 0.05). Incontrast, in late-pregnant rats, pretreatment with L-NNA had nosignificant effect. Thus, the effectiveness of the endogenousNO system is functionally downregulated in late-pregnant rats(Fig. 4).

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Figure 4. Plasma oxytocin concentration (shown on a log scale) in response to hyperosmotic stimulation and naloxone (5 mg/kg, i.v.) in virgin (A) (1.5 M NaCl; 4 ml/kg, i.p.) or pregnant (B) (2 M NaCl; 5 ml/kg, i.p.) rats pretreated with either L-NNA or isotonic saline. Oxytocin secretion was enhanced by pretreatment with L-NNA in virgin rats but not in pregnant rats. Means ± SEM; *p < 0.05 compared with basal; #p < 0.05 between groups.

Intravenous injection of naloxone significantly enhanced osmotically induced oxytocin release in all rats (Fig. 4). In virginrats, the plasma concentration of oxytocin increased by 734 ±80 pg/ml in rats pretreated with L-NNA (n = 15) and by 335 ± 37pg/ml in controls (n = 15) (difference significant at p < 0.001).In late-pregnant rats, the plasma concentration of oxytocin increasedby 401 ± 102 pg/ml in rats pretreated with L-NNA and by 337 ±80 pg/ml in controls (n = 15, NS). Naloxone increases oxytocinrelease by potentiating stimulus-secretion coupling (Russell etal., 1995); hence, its effect should be related to the oxytocinrelease rate prevailing before naloxone administration. The proportionateenhancement of oxytocin secretion was greater in virgin rats thanin pregnant rats (average of 6.5-fold enhancement of group meansin virgin rats vs 3.7-fold enhancement in pregnant rats, for ratspretreated with isotonic saline), consistent with the previouslydescribed downregulation of opioid restraint at the end of pregnancy.In pregnant rats pretreated with L-NNA, the proportionate enhancementof secretion by naloxone after L-NNA (4.4-fold enhancement) wassimilar to that in pregnant rats pretreated with vehicle. In contrast,in virgin rats pretreated with L-NNA, the average enhancementby naloxone was 10-fold, significantly higher than in virgin controls(p < 0.05, Dunnett's test, allowing for multiple comparisons,after one-way ANOVA on ranks showed significant differences amonggroups at p = 0.002).

Thus, in virgin rats, the restraining influence of endogenous NO on oxytocin release induced by intense electrical activationof oxytocin cells is independent of the known autoinhibitory opioidinfluence on oxytocin release, because the effectiveness of L-NNAis apparent after opioid receptorblockade.

The effect of NOS inhibitor on oxytocin secretion after intravenous infusion of hypertonic saline in late pregnancy

As well as elevating plasma osmolality, intraperitoneal injection of hypertonic saline produces peritoneal irritation, whichmay contribute to stimulation of oxytocin secretion by activationof afferent nociceptive pathways (Verbalis et al., 1986). To circumventthis, we administered hypertonic saline via intravenousinfusion.

Pretreatment with L-NNA had no significant effect on the basal plasma [Na⁺] or oxytocin concentration in either virgin or late-pregnantrats. In all rats, plasma [Na⁺] gradually increased throughout the course of the hypertonicsaline intravenous infusion, with no significant differences betweengroups. In all rats, the release of oxytocin increased in parallelwith the increase in [Na⁺]. The increase in L-NNA-treated virgin rats was significantlygreater than in control rats. In contrast, in late-pregnant rats,pretreatment with L-NNA had no significant effect (Fig. 5).

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Figure 5. Plasma oxytocin concentration during intravenous infusion at 2 ml/hr of hypertonic saline in virgin (A) (2 M NaCl) or pregnant (B) (2.6 M NaCl) rats pretreated with L-NNA or vehicle. Oxytocin secretion was enhanced by pretreatment with L-NNA in virgin rats but not in pregnant rats. Changes in plasma sodium concentrations (insets) were not different between the groups. Data are means ± SEM; *p < 0.05 compared with basal; #p < 0.05 compared with controls.

Thus, these experiments confirmed that, in virgin rats, endogenous NO restrains oxytocin release induced by hyperosmotic activationof oxytocin cells and confirmed that this restraint is functionallydownregulated in latepregnancy.

NOS gene expression in the SON and PVN in pregnancy

Age-matched virgin, 16 d pregnant, 22 d pregnant, and parturient rats were used to study nNOS mRNA expression. There werestrong hybridization signals for nNOS mRNA over the SON, the magnocellularregion of the PVN, the subfornical organ (SFO), and the medialamygdaloid nucleus (AMG). The silver grain density over the SONof 22 d pregnant rats was significantly less than in the othergroups (Fig. 6), with no significant differences for the PVN,SFO, or AMG (data not shown). No significant differences wereobserved in 16 d pregnant and parturient rats compared with virginrats. Inspection of emulsion-dipped sections revealed silver grainsdistributed over most, if not all, neuronal somata in the SON,consistent with expression in both vasopressin cells and oxytocincells as described previously (Luckman et al., 1997), with fewin the ventral glial zone or perinuclear zone of the SON.

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Figure 6. Neuronal NOS mRNA expression measured as film grain density over the SON (A). A significant decrease in nNOS mRNA expression was observed in late-pregnant rats (day 22), but not virgin, day 16, or parturient rats. Data are means ± SEM; *p < 0.05. Film autoradiographs of sections hybridized with a ³⁵S oligonucleotide probe against rat neuronal NOS mRNA in 16 d (B) and 22 d (C) pregnant rats. Scale bar, 1 mm.

Thus, the functional downregulation of the endogenous NO restraint of oxytocin release shown above is paralleled by a downregulationof NOS mRNA expression, specifically in neurons of the SON, atthe end ofpregnancy.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present results demonstrate that the NO donor SNP, applied locally to the SON, inhibits the electrical activity of bothoxytocin cells and vasopressin cells, and central administrationof SNP strongly inhibited the hyperosmotic stimulation of oxytocinsecretion. Conversely, systemic administration of the NOS inhibitorsL-NNA or L-NAME had little effect on the basal release of oxytocinbut, in virgin rats, enhanced the secretion of oxytocin in conditionsof strong stimulation. This enhancement derives, at least in part,from enhanced excitation of the magnocellular neurons, as revealedby Fos expression, and by electrophysiological studies, from anenhancement of the discharge rate of oxytocin cells. These findingssuggest that NO, produced by oxytocin cells in conditions of strongelectrical activity, is an inhibitory feedback regulator of electricalactivity. The evidence for an involvement of NO only during relativelyintense activation may suggest that either functionally significantrelease of NO only occurs above a threshold level of intracellularcalcium increase or the actions of NO are only significant abovea threshold concentration achieved during intenseactivity.

Importantly, however, inhibitors of NOS were not effective in late-pregnant rats, suggesting that, at the end of pregnancy,there is a functional downregulation of this feedback mechanism.This downregulation coincided with a downregulation of NOS mRNAexpression in the SON on day 22 of pregnancy and was not seenon day 16 of pregnancy. These findings are consistent with thedata reported by Okere and Higuchi (1996), who found fewer NADPH-diaphorase-positivecells in the SON and PVN and a decrease in NOS activity in theposterior pituitary in 19-21 d pregnant and parturient rats butnot in mid-pregnant rats. Luckman et al. (1997) also reportedno change in nNOS mRNA expression in either the SON or the PVNin mid-pregnancy. In contrast, other authors have reported thatthe number of NADPH-diaphorase-positive cells in the SON and PVNis increased in mid-pregnant rats (Popeski et al., 1999) and 22d pregnant rats (Woodside and Amir, 1996; Popeski et al., 1999),and one study (Popeski et al., 1999) has reported an upregulationof both nNOS protein and nNOS mRNA expression in the hypothalamusof 20 d pregnant rats assessed by Western blot and Northern blot,respectively (Xu et al., 1996). It may be that the timing of measurementsis critically important; the last 48 hr of pregnancy is a periodin which there are major fluctuations in the ovarian steroid milieuand in the activity of the oxytocinsystem.

After the decrease in expression in late pregnancy, we observed an acute increase in expression in the SON during parturition(significant increase from late pregnancy levels). This indicatesthat the activation of oxytocin cells during parturition may beassociated with stimulation of nNOS mRNA expression. Indeed, itis possible that the level of NOS expression in the SON may followthe level of electrical activity of the oxytocin cells; it isbelieved that the level of activity in oxytocin cells is low ~1d before parturition, when the oxytocin cells are inhibited bya centrally acting opioid system (Douglas et al., 1995). Theiractivity increases when oxytocin receptor expression increasesin the uterus, a few hours before the first delivery, when thesereceptors complete a positive feedback loop between oxytocin releaseand uterine contraction. Whereas nNOS mRNA expression appearsto be acutely upregulated during parturition itself, the lag beforeprotein translation is likely to mean that the functional consequencesof this upregulation are for lactation rather than parturitionitself.

In conclusion, in virgin rats, the endogenous NOS system has a potent restraining influence on oxytocin cell excitability.During late pregnancy, this influence is functionally downregulated.This is likely to cause the oxytocin system to become more excitableat term, resulting in the capacity for greater release of oxytocinduring parturition. Conversely, reimposition of NO inhibitionby central SNP infusion impedes parturition (Okere et al., 1996).

Two other phenomena have been described that would complement this downregulation. First, the secretion of oxytocin from thenerve terminals in the posterior pituitary is restrained by thecosecretion of dynorphin, acting via $kappa$ receptors on the oxytocinnerve terminals. This opioid auto-inhibition is upregulated inmid-pregnancy, contributing to an accumulation of oxytocin storesin the posterior pituitary at this time, but, like the NO systemdescribed here, is downregulated at term pregnancy (Leng et al.,1997). Second, the major extrinsic restraining influence on theelectrical activity of oxytocin cells is thought to be exertedby GABA. A high proportion of all terminals that synapse ontooxytocin cells contain GABA, and both the number of GABA-containingsynapses and the constitution of the postsynaptic GABA receptoritself change by the end of pregnancy (Fenelon and Herbison, 1996).The principal consequence of the observed change in GABA_A receptorsubunit composition appears to be that, as the concentration ofprogesterone in the circulation falls at the end of pregnancy,the duration of GABA-mediated IPSPs also falls, leading to anincrease in the excitability of oxytocin cells (Brussaard et al.,1997). In view of the proposed presynaptic excitatory action ofNO on GABA terminals in the SON (Horn et al., 1994; Ozaki et al.,2000), these changes in GABA receptors would be potentiated bythe downregulation ofNOS.

How a selective downregulation of nNOS mRNA expression occurs in the SON in late pregnancy deserves consideration. We cannotsafely conclude that there is no similar downregulation in thePVN; the data show a strong tendency in the same direction, andthis may be masked by nNOS expression in parvocellular neurons.However, it seems intrinsically unlikely that genomic regulationof nNOS in magnocellular neurons is substantially different fromthat in the amygdala or SFO, for example, in which no such trendwas evident. Possibly the simplest interpretation is that nNOSexpression is regulated in concert with electrical activity, aseither a consequence of electrical activity per se or a consequenceof intracellular mechanisms activated by the synaptic inputs thatdrive increased electrical activity. Thus, the downregulationof nNOS mRNA expression in late pregnancy described here mightreflect the electrical quiescence of oxytocin cells in the lastday of pregnancy described by Summerlee (1981).

Thus, several mechanisms act in concert on oxytocin cells at the end of pregnancy to contribute to both an increased excitabilityof oxytocin cells and an increased releasability of oxytocin fromthe nerveterminals.

  FOOTNOTES

Received March 29, 2000; revised June 12, 2000; accepted June 16, 2000.

This work was supported in part by grants from The Wellcome Trust and the Biotechnology and Biological Sciences Research Counciland by a Royal Thai Government scholarship to R.S.
Correspondence should be addressed to Prof. Gareth Leng, Department of Biomedical Sciences, University of Edinburgh MedicalSchool, George Square, Edinburgh EH8 9XD, UK. E-mail: gareth.leng{at}ed.ac.uk.

  REFERENCES

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RESULTS
DISCUSSION
REFERENCES

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