Local Morphine Withdrawal Increases c-fos Gene, Fos Protein, and Oxytocin Gene Expression in Hypothalamic Magnocellular Neurosecretory Cells

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MORPHINE
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The Journal of Neuroscience, February 1, 2000, 20(3):1272-1280

Local Morphine Withdrawal Increases c-fos Gene, Fos Protein, and Oxytocin Gene Expression in Hypothalamic Magnocellular Neurosecretory Cells
Louise E. Johnstone¹, Colin H. Brown¹, Hanneke K. M. Meeren¹, Chrétienne L. Vuijst¹, Philip J. Brooks², Gareth Leng¹, and John A. Russell¹
¹ Department of Biomedical Sciences, University Medical School, Edinburgh, EH8 9XD, Scotland, United Kingdom, and ² National Institute on Alcohol Abuse and Alcoholism, National Institutes of Health, Rockville, Maryland 20852

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We measured stimulation of c-fos and oxytocin gene expression during excitation of oxytocin cells induced by systemic or localmorphine withdrawal. Female rats were made morphine-dependentby intracerebroventricular morphine infusion over 5 d. Morphinewithdrawal, induced by systemic injection of the opioid antagonistnaloxone (5 mg/kg) in conscious or anesthetized rats, increasedthe density of c-fos messenger RNA and of oxytocin heterogeneousnuclear RNA in supraoptic nucleus cells compared with those ofnonwithdrawn rats; c-fos messenger RNA was also increased in themagnocellular and parvocellular paraventricular nuclei of withdrawnrats. Morphine withdrawal increased the number of Fos-immunoreactivecells in the supraoptic and magnocellular paraventricular nucleiof conscious or pentobarbitone-anesthetized rats. Morphine withdrawalalso increased Fos-immunoreactive cell numbers in the parvocellularparaventricular nucleus of conscious but not anesthetized rats.Central administration of the $alpha$ ₁-adrenoreceptor antagonist benoxathian(5 µg/min) did not prevent morphine withdrawal-induced increasesin the numbers of Fos-immunoreactive neurons in the supraopticor magnocellular paraventricular nucleus. Unilateral microdialysisadministration of naloxone (10⁵ M) into the supraoptic nucleus of anesthetized morphine-dependentrats increased Fos-immunoreactive cell numbers compared with thecontralateral nucleus. Finally, we investigated whether dependencecould be induced by chronic unilateral infusion of morphine intoa supraoptic nucleus; systemic naloxone (5 mg/kg) increased Fos-immunoreactivecell numbers in the morphine-infused nucleus compared with thecontralateral nucleus. Thus, morphine withdrawal excitation increasesc-fos and oxytocin gene expression in supraoptic nucleus neurons.This occurs independently from excitation of their ascending noradrenergicinputs, and both dependence and withdrawal can be induced withinthe supraopticnucleus.

Key words: adrenoreceptors; benoxathian; dependence; hypothalamic paraventricular nucleus; microdialysis; naloxone; opioid; supraoptic nucleus

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Magnocellular neurosecretory cells of the hypothalamic supraoptic nucleus (SON) and paraventricular nucleus (PVN) projectto the neurohypophysis (posterior pituitary gland) in which theysecrete oxytocin or vasopressin into the systemic circulation(Hatton, 1990). The µ-opioid agonist morphine inhibits oxytocincells in vivo, an effect that is reversed by the opioid antagonistnaloxone (Ludwig et al., 1997a). Oxytocin cells develop toleranceto, and dependence on, morphine during prolonged central administrationof this opioid (Pumford et al., 1991). Tolerance involves downregulationof µ-receptors within the supraoptic nucleus (Sumner et al., 1990),but the mechanisms underlying morphine dependence in oxytocin(or any other) neurons have yet to be fullyelucidated.

Naloxone-precipitated morphine withdrawal causes a robust hyperexcitation of oxytocin cells, evident as a marked (approximatethreefold) increase in firing rate (Leng et al., 1989). In combinationwith naloxone antagonism of endogenous opioid actions at $kappa$ -opioidreceptors on the neurohypophysial neurosecretory terminals (Russellet al., 1993) and frequency facilitation of hormone release (Bicknell,1988), this excitation causes a 100-fold increase in systemicoxytocin release (Bicknell et al., 1988). Vasopressin cells arelittle affected by morphine and do not show morphine withdrawalexcitation (Bicknell et al., 1988). Direct application of naloxoneinto the supraoptic nucleus of morphine-dependent rats elicitselectrical excitation of oxytocin cells typical of morphine withdrawal(Ludwig et al., 1997a). Thus, the mechanisms that underlie morphinedependence-withdrawal of oxytocin neurons may reside within thesecells or at localsynapses.

Fos protein (the product of the immediate early gene c-fos) expression is a reliable marker of activation in magnocellularneurosecretory neurons (Hoffman et al., 1993). Electrical excitationof oxytocin cells during withdrawal is accompanied by increasedFos expression in the supraoptic and paraventricular nuclei (Stornettaet al., 1993; Jhamandas et al., 1996; Murphy et al., 1997). Currently,the consequences of increased Fos expression in magnocellularneurosecretory cells are uncertain. Fos has been proposed to beinvolved in oxytocin gene regulation (Ivell and Richter, 1984;Walther et al., 1991), but it is not known whether increased Fosexpression is followed by oxytocin genestimulation.

Morphine withdrawal also induces Fos expression in brainstem sites that project to the supraoptic nucleus (Aghajanian, 1978;Stornetta et al., 1993; Murphy et al., 1997), including the A2noradrenergic cell group in the nucleus tractus solitarii (NTS).Such evidence, and that from other studies, has led to the proposalthat other non-noradrenergic neurons are activated by their excitednoradrenergic input during withdrawal (Redmond and Krystal, 1984).Although oxytocin cell withdrawal excitation is temporarily interruptedby acute $alpha$ ₁-adrenoreceptor blockade, it is unaffected by chronicneurotoxin-induced hypothalamic noradrenaline depletion (Brownet al., 1998).

Here, we measured the expression of c-fos messenger RNA (mRNA), Fos protein, and oxytocin heterogeneous nuclear RNA (hnRNA)in magnocellular neurosecretory cells during naloxone-precipitatedmorphine withdrawal to determine whether changes in activity ofthe c-fos gene are accompanied by altered expression of the oxytocingene. Subsequently, we used Fos protein expression to test whetherdependence and withdrawal excitation could be induced by localactions of morphine and naloxone within the supraopticnucleus.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Induction of tolerance-dependence by intracerebroventricular morphine. Morphine tolerance-dependence was induced as describedpreviously (Rayner et al., 1988). Briefly, virgin female rats(250-350 gm) were implanted, under ether (in some experiments)or halothane anesthesia, with a cannula in a lateral cerebralventricle connected via polyethylene tubing to a subcutaneousosmotic minipump (1 µl/hr; Alzet 2001; Alza Corporation, PaloAlta, CA), filled with morphine sulfate (50 µg/µl). The tubingcontained 40 µl of 10 µg/µl morphine solution, followed by 40µl of 20 µg/µl morphine solution. After surgery, the rats werehoused singly for 5d.

In situ hybridization for c-fos mRNA. Morphine-dependent rats were anesthetized with urethane (ethyl carbamate, 1.25 gm/kg,i.p.), and a cannula was inserted into a femoral vein for removalof blood samples. These are conditions identical to those in whichwe have studied previously oxytocin neuron tolerance and dependenceand withdrawal excitation with electrophysiological techniques(Russell et al., 1995; Ludwig et al., 1997a; Brown et al., 1998).The rats were injected with naloxone (5 mg/kg, 10 mg/ml, s.c.;n = 4) or 0.15 M saline (subcutaneously; n = 4) at least 2 hrafter the completion of the surgery and decapitated an additional45 min later. The brains were rapidly removed, frozen on crusheddry ice, and stored at $-$ 70°C until processed for c-fos mRNA insitu hybridization. Blood samples (0.3 ml) were removed 5 minbefore and 5 and 30 min after naloxone-vehicle administration,and the separated plasma was stored at $-$ 20°C until assayed foroxytocincontent.

The in situ hybridization for c-fos mRNA was performed as described previously (Hamamura et al., 1991). Briefly, 10 µm coronalcryostat sections were cut through the hypothalamus and througha series of brain paste ³⁵S standards and mounted onto RNase-free, gelatin-chrome alum-coatedslides, air-dried, and fixed in 3% paraformaldehyde and 0.03%diethyl pyrocarbonate in 0.1 M phosphate buffer. After dehydration,the sections were stored desiccated at $-$ 70°C. Representative brainpaste standard sections were counted in a scintillation counter.The sections were prehybridized and hybridized overnight at 37°Cusing a ³⁵S-dATP-labeled oligonucleotide probe corresponding to base pairs138-185 of the rat c-fos gene (Curran et al., 1987). After washing,the sections were exposed to autoradiographic film for 2 weeks,dipped in K5 emulsion (Ilford Imaging, Mobberley, UK), and exposedfor an additional 9 weeks before development and counterstainingwith methyleneblue.

Autoradiographs of the supraoptic nucleus were quantified with a computer-based analysis system (µMagiscan; Joyce-Loebl Ltd.,Gateshead, UK) with images magnified in a microscope (10× objective)and collected by a CCD video camera (Cohu Inc., San Diego, CA).The analyzer was set to measure silver grain area per supraopticnucleus profile, and hence grain density per unit area of supraopticnucleus. Background density was measured over an adjacent tissue-freearea of film and subtracted. From the standards, the tissue measurementswere on the linear part of the relationship between natural log[radioactivity]and silver grain density. Animal means were calculated from theindividual supraoptic nucleus measurements in each animal. Theemulsion-dipped autoradiographs showed that the hybridizationsignal was over neurons and not glia (Ludwig et al., 1997b).

Fos protein immunocytochemistry. Conscious morphine-dependent rats and morphine-naïve rats (implanted with a vehicle-containingminipump attached via polyethylene tubing to the intracerebroventricularcannula) were injected on day 6 with naloxone (5 mg/kg, s.c.)or 0.15 M saline (all four groups n = 7) and decapitated 90 minlater. The brains were rapidly removed, frozen on crushed dryice, and stored at $-$ 70°C until processed to detect Fos-immunoreactive(IR)cells.

Coronal 15 µm cryostat sections were cut through the supraoptic and paraventricular nuclei, mounted on gelatin-coated slides,and fixed in 4% paraformaldehyde in phosphate buffer. The sectionswere then processed immunocytochemically using a rabbit polyclonalantibody raised against the N terminal of rat Fos protein (1:1000dilution; Oncogene Science, Uniondale, NY), with incubation for24 hr in a humidified chamber at 4°C. Sections were incubatedfor an additional 24 hr at 4°C with peroxidase-labeled goat anti-rabbitIgG (1:500 dilution; Vector Laboratories, Burlingame, CA). Then,Fos protein immunoreactivity was visualized as a black precipitateusing a glucose oxidase-based, Ni-intensified, 3,3'-diaminobenzidine(DAB) procedure (Shu et al., 1988). The slides were then dehydratedthrough an alcohol series, dewaxed in xylene, and coverslippedin DePeX mountant. Immunocytochemically processed sections fromeach rat containing the supraoptic nucleus [1.3-1.4 mm posteriorto bregma (Paxinos and Watson, 1996)] and the magnocellular (1.8mm) and parvocellular paraventricular nucleus (1.8-2.12 mm) wereselected for analysis. The number of Fos-IR cells within the supraopticand paraventricular nuclei were counted on coded sections (n =6-8 per region per rat) under a light microscope (10× objective).The animal mean number of Fos-IR cells per section for each regionand finally the group mean ± SEM was then calculated. Becauseactivation may enlarge magnocellular neurons and the section thicknesswas constant, any activation-induced enlargement of the neuronswould decrease the number of neurons in each section; no correctionwas made for this possibility. The results show large increasesin number of Fos-positive neurons per SON-PVN section with morphinewithdrawal so any contribution from this counting error is notimportant for interpretation in thisstudy.

Some supraoptic nucleus sections were processed further after the Fos immunocytochemical procedure to identify oxytocin neuronsimmunocytochemically. Rabbit anti-oxytocin antibody (Higuchi etal., 1985) (1:50,000 dilution) was applied and visualized afterincubation for 24 hr at 4°C with goat anti-rabbit IgG-peroxidasecomplex (24 hr, 4°C) andDAB.

In situ hybridization for oxytocin hnRNA. In this experiment, conscious rats were given an injection of either naloxone (5mg/kg, 10 mg/ml, s.c.; n = 6) or vehicle (0.15 M NaCl; n = 5)on the sixth day of intracerebroventricular morphine infusion.The rats were decapitated 2 hr later, and the brains were removedand frozen on crushed dry ice before storage at $-$ 70°C until processedfor oxytocin hnRNA in situ hybridization, as described previously(Douglas et al., 1998). Briefly, 10 µm coronal sections were cutthrough the supraoptic nucleus at $-$ 14°C and mounted onto RNase-free,gelatin-subbed slides. Oxytocin hnRNA was detected using a single-stranded³H-cDNA probe directed against intron 1 of the primary transcriptof the rat preprooxytocin gene (Brooks et al., 1993). Slides containingsupraoptic nucleus sections (between 0.92 and 1.30 mm posteriorto bregma) were incubated in prehybridization buffer at 42°C for2 hr, rinsed, air dried, and then incubated overnight at 42°Cin hybridization buffer containing 100,000 counts per minute persection. Sections were washed, incubated overnight with gentleagitation, and finally washed for 30 min at 50°C. Slides weredipped in G5 photographic emulsion and exposed for 50 d at 4°C.The sections were then counterstained with hematoxylin and eosinand mounted in DePeX. Sections (10 µm) of autoradiographic [³H] microscales cut from polymer blocks (Amersham, Arlington Heights,IL) were mounted onto subbed slides, dipped in photographic emulsion,exposed, and developed simultaneously with the brain sections.Control sections (RNase A pretreated before hybridization or incubatedin hybridization buffer without labeled probe) showed no specifichybridization over the hypothalamic magnocellularnuclei.

Four sections per animal were viewed on a computer monitor using a CCD video camera (Cohu) connected to a Vickers M17 microscope.Measurements were made on coded sections containing the SON ata level of 1.30 mm posterior to bregma (Paxinos and Watson, 1996)using an image analyzer. Cells were considered positive when anaccumulation of silver grains (at least three times greater thanbackground) could be discerned over the nucleus (Brooks et al.,1993; Xing et al., 1993). The area of the supraoptic nucleus profilewas measured using a calibrated image analyzing system, and thenumber of positive cells was calculated per supraoptic nucleusarea (in square micrometers) for eachsection.

Silver grain area, representing hybridization of oxytocin hnRNA, over the cell nucleus was measured (50× oil immersion objective).All positive cells in four supraoptic nucleus profiles were measuredfor each animal, at least five background measurements were obtainedfrom adjacent tissue dorsolateral to the supraoptic nucleus, andthe mean background was subtracted from each supraoptic nucleuscell silver grain measurement. The mean silver grain area permagnocellular cell nucleus was then calculated for eachprofile.

Grain area was measured for each level of the calibrated radioactive microscale, and corresponding backgrounds were subtracted.For each experiment, a semilog curve was plotted for the averagegrain area per ³H standard (corresponding to an area equivalent to a neuronalnucleus or cytoplasm or supraoptic nucleus) against the tissueequivalent radioactivity. All detected grain areas in tissue layon the linear part of the relationship between radioactivity andgrainarea.

Oxytocin radioimmunoassay. Plasma oxytocin concentrations were measured in duplicate aliquots by specific radioimmunoassayas described previously (Leng et al., 1988) using antiserum kindlyprovided by Dr. T. Higuchi (Fukui Medical University, Fukui, Japan)(Higuchi et al., 1985). The oxytocin concentrations in all sampleswere determined in a single assay. The assay sensitivity was <2.4pg/ml, and the intra-assay coefficient of variation was <12%.

Central $alpha$ ₁-antagonist administration to morphine-dependent rats. Rats were prepared for chronic intracerebroventricular morphine(n = 12) or vehicle (n = 12) infusion as described above, withthe addition that a 28 gauge stainless steel cannula (PlasticsOne, Roanoke, VA) was placed into the left lateral cerebral ventricle(0.6 mm caudal, 1.6 mm lateral to bregma, and 4.5 mm below thesurface of the skull) at the time of implantation of the morphine-containingminipump for subsequent intracerebroventricular infusion of thepotent and selective $alpha$ ₁-adrenoreceptor antagonist benoxathian(Melchiorre et al., 1984). On the sixth day after surgery, therats were anesthetized with pentobarbitone (60 mg/kg, i.p.), andan intracerebroventricular infusion of benoxathian (5 µg/min;0.5 µl/min in 0.9% saline) or vehicle from a slow infusion pumpwas started at least 2 hr later. Naloxone was administered (5mg/kg, s.c.) 30 min into the benoxathian-vehicle infusion, andthe infusion was continued until the rats were decapitated 90min later. Again, the brains were removed, frozen on crushed dryice, and stored at $-$ 70°C until processed for Fos-IR asabove.

We used barbiturate anesthesia in this and the next experiments to avoid the stimulation of Fos expression that can be seenwith urethane anesthesia (Takayama et al., 1994). A time coursestudy in barbiturate-anesthetized morphine-dependent rats showedno Fos expression in the supraoptic nucleus or magnocellular paraventricularnucleus after subcutaneous vehicle injection (at 30, 45, 60, 90,and 120 min after injection; four rats per time point), but therewas a significant increase in Fos expression in both nuclei afternaloxone injection at all time points except 30 min (four ratsper time point). There was no significant difference in the numberof Fos-positive neurons between 45 and 120 min after naloxone,but the variance was least at 90 min, and so this was selectedas the sampling point in the mainexperiments.

Fos immunocytochemistry was performed on coronal brainstem sections through the A1 and A2 groups of noradrenergic neuronsfrom benoxathian-infused rats and theircontrols.

Microdialysis administration of naloxone into the supraoptic nucleus of morphine-dependent rats. A U-shaped microdialysisprobe [molecular weight cutoff, 5 kDa; 3.0 mm long × 1.0 mm outerdiameter; 0.2 mm inner diameter (i.d.)] was placed adjacent tothe left supraoptic nucleus (0.9 mm caudal, 1.7 mm lateral, and9.1 mm below bregma) at the time of implantation of the intracerebroventricularchronic infusion cannula and morphine-containing minipump. Fivedays later, the probe was used for microdialysis administration(retrodialysis) of naloxone under sodium pentobarbitone anesthesia(60 mg/kg, i.p.). Identical probes, when inserted into the brainparenchyma, have been shown to effectively dialyze a brain volumewith a radius of ~1 mm after infusion through the probe for 30min (Ludwig and Leng, 1997). A 1 ml Hamilton syringe was mountedon a slow infusion pump (flow rate set at 2.84 µl/min) and connectedto the microdialysis probe via polyethylene tubing (0.4 mm i.d.).This was filled with artificial CSF (aCSF) (in mM: NaCl 138, KCl3.36, NaHCO₃ 9.52, Na₂HPO₄ 0.49, urea 2.16, CaCl₂ 1.26, and MgCl₂1.18, pH 7.2). The rats were left for ~120 min before the dialysatewas switched to aCSF containing 10⁵ M naloxone (n = 10) or aCSF alone (n = 9). The rats were killedby decapitation 90 min later, and their brains were processedfor Fos-IR as describedabove.

Chronic intrasupraoptic nucleus morphine infusion. Rats were anesthetized with 5% halothane. A 28 gauge stainless steel cannulafilled with morphine or Ringer's solution (in mM: 147 NaCl, 4KCl, and 2.5 CaCl₂) was inserted immediately dorsal to the rightsupraoptic nucleus (0.9 mm caudal and 1.7 mm lateral to bregmaand 9.1 mm below the surface of the skull). The cannula was attachedvia silicone tubing (0.25 mm i.d.; 0.91 mm wall thickness) toa subcutaneous Alzet 2002 miniosmotic pump set to deliver morphineat 0.25 µg/hr or Ringer's solution at 0.5 µl/hr. The cannula wassecured using dental acrylic bonded to stainless steel screwsinserted in the skull. After surgery, the rats were housed individuallywith access to food and water ad libitum.

On the sixth day after implantation of the minipump, the rats were anesthetized with pentobarbitone (60 mg/kg, i.p.) and injected(intraperitoneally) with naloxone (5 mg/kg; n = 7) or 0.15 M saline(n = 5) at least 2 hr later. The rats were decapitated an additional90 min later, and the brains were rapidly removed, frozen on crusheddry ice, and stored at $-$ 70°C until processed for Fos-IR.

Statistics. Statistical tests were completed using the SigmaStat software package (Jandel Scientific GmbH, Erkrath, Germany).Data from each experiment were analyzed by using Student's t testor, where appropriate, two-way repeated measures ANOVA or one-wayANOVA on ranks. Where the F ratio was significant, post hoc analyseswere performed between groups using Student-Newman-Keuls testor Dunn's method depending on groupnumbers.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

c-fos mRNA expression in the supraoptic and paraventricular nuclei after morphine withdrawal

Plasma oxytocin concentrations were determined to confirm the expression of morphine withdrawal excitation by oxytocin neuronsin each rat under urethane anesthesia. The mean initial plasmaoxytocin concentrations in the two groups of morphine-dependentrats subsequently administered vehicle or systemic naloxone were58.4 ± 25.6 and 29.0 ± 12.8 pg/ml, respectively (both n = 4).Five and 30 min after vehicle administration (0.15 M saline, s.c.),the plasma oxytocin concentrations were 36.6 ± 15.0 and 32.0 ±15.8 pg/ml, respectively. In the rats administered naloxone (5mg/kg, s.c.), the plasma oxytocin concentrations were 1315.6 ±260.7 and 365.6 ± 53.2 pg/ml at 5 and 30 min after the naloxoneinjection (both p < 0.05; two-way repeated measures ANOVA, followedby Student-Newman-Keuls test), indicative of morphine withdrawalexcitation.

Forty-five minutes after naloxone administration (5 mg/kg, s.c.), c-fos gene expression was increased with respect to vehicle-injected(0.15 M saline, s.c.) controls in both the supraoptic nucleus(p < 0.01; Student's t test) and in the magnocellular (p < 0.01)and parvocellular (p < 0.05) portions of the paraventricular nucleus(Fig. 1).

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Figure 1. Changes in expression of c-fos mRNA in the supraoptic and paraventricular nuclei during morphine withdrawal. Mean silver grain density [arbitrary units (a.u.) + SEM] in c-fos-labeled sections through the SON and PVN (magnocellular and parvocellular divisions, MPVN and PPVN, respectively) of morphine-dependent rats 45 min after vehicle (VEH; 0.15 M saline, s.c.; n = 4, magnocellular and parvocellular paraventricular nuclei combined) or naloxone (NLX; 5 mg/kg, s.c.; n = 4) administration. *p < 0.05, **p < 0.01 versus vehicle; Student's t test.

Hypothalamic Fos protein expression after morphine withdrawal excitation

We used immunocytochemistry to investigate whether the increased expression of the c-fos gene induced by morphine withdrawalresults in increased translation into Fos protein. In consciousmorphine-dependent rats, systemic naloxone induced the behavioralsigns of withdrawal (e.g., wet dog shakes, teeth-chattering, defecation),and Fos-IR nuclei were prominent in magnocellular neurosecretorycells of the supraoptic (Fig. 2) and paraventricular nuclei, aswell as in parvocellular cells of the paraventricular nucleus.The expression of Fos-IR cells in the forebrain was discrete,with substantial numbers consistently found in the anterior hypothalamus,primary olfactory cortex, medial amygdaloid nucleus, anteriorparaventricular thalamic nucleus, endopiriform nucleus, and thecerebral cortex surrounding the cingulate gyrus. There were onlya few Fos-IR cells in the perinuclear zone adjacent to the supraopticnucleus in all groups.

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Figure 2. Fos protein in the supraoptic nuclei of morphine-naïve and -dependent rats. Photomicrographs of coronal sections through the SON processed for Fos immunohistochemistry from a morphine-naïve rat given vehicle (0.9% saline, 0.5 ml/kg, s.c.) (A), a morphine-naïve rat given naloxone (5 mg/kg, s.c.) (B), a morphine-dependent rat given vehicle (C), and a morphine-dependent rat given naloxone (D). Nuclei immunoreactive for Fos protein appear as intense black staining (arrow). OC, Optic chiasma. Scale bars, 50 µm.

The number of Fos-IR cells in the supraoptic nucleus of the morphine-dependent rats given naloxone (5 mg/kg, s.c.) was significantlygreater (p < 0.05) than that of all other groups (Fig. 3). Thenumber of Fos-IR cells in the supraoptic nucleus of morphine-naïverats given 0.15 M saline (subcutaneously; n = 6) was not differentfrom that found in the supraoptic nuclei of morphine-naïve ratsgiven naloxone (n = 6) or that of morphine-dependent rats givensaline (subcutaneously; n = 6) (Fig. 3).

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Figure 3. Fos protein in the supraoptic and paraventricular nuclei of morphine-naïve and -dependent rats. The mean + SEM number of Fos-IR cells in the SON, the magnocellular paraventricular nucleus (MPVN), the parvocellular paraventricular nucleus (PPVN), morphine-naïve rats (NAIVE) given 0.15 M saline (VEH; subcutaneously; n = 6 or 7) or naloxone (NLX; 5 mg/kg, s.c.; n = 6) and morphine-dependent rats (DEPENDENT) given saline (VEH; subcutaneously; n = 6 or 7) or naloxone (NLX). *p < 0.05 versus morphine-naïve vehicle or naloxone-injected rats, and morphine-dependent vehicle-injected rats; one-way ANOVA on ranks, followed by Student-Newman-Keuls test.

Similarly to its effects in the supraoptic nucleus, naloxone (5 mg/kg, s.c.) significantly increased the number of Fos-IRcells in the magnocellular and parvocellular paraventricular nucleiof morphine-dependent rats (both p < 0.05; n = 7) (Fig. 3). Thenumber of Fos-IR cells in the magnocellular and parvocellularparaventricular nuclei of morphine-naïve rats given 0.15 M saline(subcutaneously) were similar to those in these nuclei after administrationof naloxone (5 mg/kg, s.c.) to morphine-naïve rats or of vehicleto morphine-dependent rats (all n = 5) (Fig. 3).

In supraoptic nucleus sections processed for both Fos and oxytocin immunocytochemistry, the great majority of oxytocin neuronscontained Fos-positive nuclei. Some supraoptic nucleus neuronsthat did not show oxytocin immunoreactivity and were presumptivevasopressin neurons also contained Fos-positivenuclei.

Effects of morphine withdrawal excitation on supraoptic nucleus oxytocin hnRNA expression

After morphine withdrawal excitation in conscious rats, labeling with the intronic oxytocin hnRNA probe was restricted predominantlyto the dorsal oxytocin cell-rich region of the supraoptic nucleus.For oxytocin hnRNA, hybridization was confined to the nuclei ofmagnocellular cells and was evident as discrete accumulationsof silver grains, as described previously (Brooks et al., 1993)(Fig. 4). The number of oxytocin hnRNA-labeled neurons in thesupraoptic nucleus (Fig. 5A) and the area of silver grain perlabeled supraoptic neuronal nucleus (Fig. 5B) were significantlygreater (p < 0.05; Student's t test) in the morphine-dependentgroup given naloxone (n = 6) compared with the vehicle-treatedmorphine-dependent group (n = 5). In untreated virgin rat brains(n = 6) processed with the morphine-treated rat brains, the numberof oxytocin hnRNA-labeled cells (12.2 ± 2.0) and the area of silvergrain per labeled neuronal nucleus (6.9 ± 0.6 µm²) in the supraoptic nucleus were similar to those in morphine-dependentvehicle-treated rats.

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Figure 4. Oxytocin hnRNA expression in the supraoptic nucleus of morphine-dependent and morphine-withdrawn rats. Hypothalamic sections containing the SON were pretreated and hybridized for oxytocin hnRNA (with a ³H-labeled cDNA probe complementary to 210 bases of intron 1). The sections were exposed to gel emulsion for 50 d. Autoradiographs are of oxytocin hnRNA labeling in supraoptic nucleus neurons in morphine-dependent (A) and morphine-withdrawn (B) rats. Note foci of labeling over the neuronal nuclei (arrows). Scale bars, 20 µm.

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Figure 5. Changes in expression of oxytocin hnRNA in supraoptic nucleus cells during morphine withdrawal. Coronal sections containing the supraoptic nucleus from rats treated with either chronic morphine and acute subcutaneous 0.15 M saline (VEH; n = 5) or chronic morphine and acute naloxone (NLX; 5 mg/kg, s.c; withdrawn, n = 6) were hybridized with a ³H-labeled cDNA probe complementary to 210 bases of intron 1 of rat oxytocin hnRNA. A, Mean + SEM number of oxytocin hnRNA-positive cells per supraoptic nucleus section. B, Mean + SEM silver grain area per supraoptic nucleus neuronal nucleus. *p < 0.05; Student's t test.

Effects of central $alpha$ ₁-adrenoreceptor antagonism on Fos protein expression in magnocellular neurosecretory cells during morphine withdrawal

Because noradrenergic systems also undergo morphine withdrawal excitation and project to magnocellular neurosecretory cells,we induced withdrawal during intracerebroventricular infusionof the $alpha$ ₁-adrenoreceptor antagonist benoxathian. First, Fos expressionwas increased in supraoptic and magnocellular paraventricularnucleus neurons after morphine withdrawal under barbiturate anesthesia(Fig. 6), and this was quantitatively similar to the expressionin conscious withdrawn rats (Fig. 3). Fos expression in parvocellularparaventricular nucleus neurons was barely, although significantly,increased by morphine withdrawal in barbiturate-anesthetized ratscompared with controls (Fig. 6). However, this expression wassignificantly less than that seen in conscious withdrawn rats(Fig. 3). Second, benoxathian infusion (5 µg/min over 2 hr) didnot affect the number of Fos-IR cells in the supraoptic nucleus,magnocellular paraventricular nucleus, or the parvocellular paraventricularnucleus in morphine-naïve or morphine-dependent rats administerednaloxone (5 mg/kg, i.p.) 30 min into the benoxathian-vehicle infusion(Fig. 6). In addition, the number of Fos-IR cells in the A2 cellgroup of the NTS and the A6 cell group of the locus ceruleus ofbenoxathian-infused morphine-withdrawn rats (at 6.94 ± 2.37 and3.30 ± 1.97 Fos-IR cells per section, respectively) were similarto those of vehicle-infused morphine-withdrawn rats (at 8.43 ±2.43 and 2.26 ± 0.42 Fos-IR cells per section, respectively).

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Figure 6. Effects of $alpha$ ₁-adrenoreceptor antagonism on Fos protein expression in magnocellular and parvocellular cells in morphine-dependent and morphine-withdrawn rats. Mean + SEM number of Fos-IR cells in the SON, the magnocellular paraventricular nucleus (MPVN), and the parvocellular paraventricular nucleus (PPVN). Morphine-naïve (NAIVE) and morphine-dependent (DEPENDENT) rats were pentobarbitone-anesthetized, infused for 2 hr with 0.15 M saline (intracerebroventricularly; VEH) or benoxathian (5 µg/min, i.c.v.; BEN), and decapitated 90 min after administration of naloxone (5 mg/kg, i.p., 30 min into the intracerebroventricular infusion; n = 5-7). *p < 0.05 versus morphine-naïve vehicle-infused rats; $dagger$ p < 0.05 versus morphine-naïve benoxathian-infused rats; one-way ANOVA on ranks, followed by Dunn's method.

Fos protein expression after unilateral administration of naloxone into a supraoptic nucleus of morphine-dependent rats

To determine whether the mechanisms that generate excitation of oxytocin cells upon morphine withdrawal reside within thesupraoptic nucleus, we applied naloxone (10⁵ M) directly into a supraoptic nucleus unilaterally using microdialysisin barbiturate-anesthetized morphine-dependent rats. The resultantincrease in cells that expressed Fos-IR in the naloxone-dialyzedsupraoptic nucleus was significantly greater than that found inthe contralateral nucleus in the same rats or the ipsilateralsupraoptic nucleus in vehicle-dialyzed morphine-dependent rats(both p < 0.05) (Fig. 7A).

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Figure 7. Fos protein expression in the supraoptic nucleus after unilateral naloxone or morphine infusion. A, Intracerebroventricular infusion of morphine for 5 d. Mean + SEM number of Fos-IR cells in the SON of morphine-dependent rats dialyzed with aCSF (VEH) or naloxone (NLX; 10 ⁵ M) and in the respective contralateral (CON) supraoptic nucleus. *p < 0.05 versus aCSF-dialyzed SON, the SON contralateral (CON) to naloxone SON, and the SON contralateral (CON) to aCSF SON (one-way ANOVA on ranks, followed by Dunn's method). B, Unilateral infusion of morphine (0.25 µg/hr, for 5 d) into a supraoptic nucleus. Mean + SEM number of Fos-IR cells in the morphine-infused (filled bars) and contralateral (CON; open bars) supraoptic nuclei of rats given 0.15 M saline (VEH; intraperitoneally) or naloxone (NLX; 5 mg/kg, i.p.). *p < 0.05 versus the SON contralateral to morphine infusion, the morphine-treated nucleus in vehicle-injected rats (VEH; intraperitoneally), and the contralateral (CON) nucleus in vehicle-injected rats (one-way ANOVA on ranks, followed by Dunn's method).

Systemic naloxone-induced Fos protein expression after chronic unilateral morphine infusion into a supraoptic nucleus

Similarly, to investigate whether the mechanisms that induce morphine dependence in oxytocin cells also reside within thesupraoptic nucleus, we unilaterally infused morphine into thesupraoptic nucleus for 5 d. We then injected naloxone (5 mg/kg,i.p.) under barbiturate anesthesia to induce morphine withdrawal.The naloxone-induced increase in number of neurons expressingFos-IR in the morphine-infused supraoptic nucleus was significantlygreater than that found in the contralateral nucleus in the samerats or in the ipsilateral vehicle-infused supraoptic nucleus(both p < 0.05) (Fig. 7B).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Here, we have shown that morphine withdrawal elicits a rapid increase in oxytocin gene transcription in magnocellular supraopticneurons. This increase in the activity of the oxytocin gene ispreceded by an increase in c-fos gene transcription in magnocellularneurosecretory cells and by increased Fos protein expression inoxytocin neurons in the supraoptic nucleus. We have shown thatmorphine withdrawal-induced increases in supraoptic nucleus Fosprotein expression result from actions of morphine and naloxoneexerted within the supraoptic nucleus itself that do not requirethe ascending noradrenergic input to oxytocincells.

Activation of the c-fos and oxytocin genes by morphine withdrawal

In the rat, naloxone-precipitated morphine withdrawal excitation of oxytocin cells is a highly robust phenomenon, causinga threefold increase in the firing rate of the cells (Leng etal., 1989) and consequently a 100-fold rise in plasma oxytocinconcentrations (Bicknell et al., 1988). The augmentation of thesecretory response is partly a consequence of frequency facilitationof hormone release (Bicknell, 1988) and of antagonism of $kappa$ -opioidactivity at the posterior pituitary (Russell et al., 1993). Thiswithdrawal excitation of oxytocin secretion is seen in conscious,as well as urethane- and barbiturate-anesthetized, rats (Bicknellet al., 1988; Rayner et al., 1988; Brown et al., 1998). Here,we have shown that these alterations in the activity of oxytocincells are accompanied by increases in the activity of the c-fosand oxytocin genes in these neurons, after only 45 min and by2 hr after morphine withdrawal, respectively. The rat oxytocingene promoter contains an activator protein-1-like site (Ivelland Richter, 1984), and Fos protein expression is elevated inthe supraoptic nucleus between 30 and 45 min after morphine withdrawal(data not shown). Thus, Fos protein expression in oxytocin cellsmay be involved in the increased oxytocin gene transcription observed2 hr after withdrawal. The rapid stimulation of oxytocin geneexpression in supraoptic neurons by morphine withdrawal is comparablewith the stimulation by parturition (Douglas et al., 1998), whichis also accompanied by Fos expression (Luckman et al., 1993).However, other transcription factors are also likely to be involvedin the regulation of oxytocin gene expression (Burbach et al.,1994; Luckman et al., 1996), but their expression during withdrawalhas not beencharacterized.

The withdrawal-induced increase in c-fos gene activity in the supraoptic and paraventricular nuclei is more rapid than hasbeen reported for locus ceruleus neurons that also undergo withdrawalexcitation (Nye and Nestler, 1996). The increased electrical activityin oxytocin cells occurs within the first few minutes after morphinewithdrawal (Leng et al., 1989), as it does in locus ceruleus neurons(Rasmussen et al., 1990). It appears that increased activity ofthe c-fos gene (and consequently of the oxytocin gene) occursin parallel with the other manifestations of withdrawal excitationrather than driving these events. The induction of Fos proteinexpression in magnocellular neurosecretory cells does not simplyreflect increased electrical activity and is not a direct consequenceof increased secretory activity (Luckman et al., 1994; Ludwiget al., 1997b). It follows that the increased c-fos gene activityinduced by morphine withdrawal excitation involves receptor-mediatedevents or mechanisms that converge on the second messenger systemsthat normally activate the c-fos gene (Sheng and Greenberg, 1990).

Fos protein expression and the mechanism of excitation of oxytocin neurons by morphine withdrawal

It follows from the above that Fos protein expression in oxytocin neurons is a marker of the activation of intracellular regulatorymechanisms during withdrawal that is independent of excitationof electrical or secretory activity of the neurons. We used thisprinciple to explore the role of the noradrenergic input to theoxytocin neurons in morphine withdrawal excitation and whetherthe mechanisms leading to dependence are likely to reside in theoxytocin neuronsthemselves.

Noradrenergic inputs to the supraoptic nucleus are activated during morphine withdrawal (Murphy et al., 1997) and may contributeto the excitation of oxytocin cells at this time (Brown et al.,1998). However, lesioning of the noradrenergic inputs with 6-hydroxydopaminedoes not prevent morphine withdrawal-induced oxytocin secretion,thus it is clear that the noradrenergic input is not essentialfor withdrawal to occur (Brown et al., 1998). The $alpha$ ₂-adrenoreceptoragonist clonidine reduces withdrawal-induced Fos protein expressionin the C1 adrenergic cell group in the rostral ventrolateral medulla,as well as in neurons in the locus ceruleus (Baraban et al., 1995).Clonidine also reduces the withdrawal excitation of oxytocin secretionin dependent rats (Brown et al., 1998). We used the specific $alpha$ ₁-antagonistbenoxathian to eliminate synaptic activation of oxytocin cellsby noradrenergic inputs during morphine withdrawal because benoxathianhas been shown previously to block excitation of oxytocin cellsin response to intravenous cholecystokinin, a response establishedto arise from activation of A2 cells of the NTS (Brown et al.,1998). The dose of benoxathian used reverses morphine withdrawal-inducedincreases in electrical and secretory activity of oxytocin cells(Brown et al., 1998), but Fos protein expression in the supraopticand magnocellular paraventricular nuclei was unaffected. Thisindicates that the induction of Fos protein in these neurons bywithdrawal does not require activation through noradrenergic synapses.It can be inferred also that it does not require excitation ofthe firing rate or secretory activity of theneurons.

This argument is further supported by considering the observation that both the A2 noradrenergic cell group in the NTS andthe A1 noradrenergic cell group in the ventrolateral medulla areactivated by morphine withdrawal (Murphy et al., 1997). The A2cell group projects preferentially to oxytocin cells and the A1cell group preferentially to vasopressin cells (Cunningham andSawchenko, 1988). Nevertheless, only oxytocin cells are electricallyactivated upon morphine withdrawal (Bicknell et al., 1988). Furthermore,there is little increase in noradrenaline release in the supraopticnucleus during withdrawal (Murphy et al., 1997), and systemiccholecystokinin, which activates A2 neurons and thus oxytocinneurons, neither triggers withdrawal nor has an attenuated effectduring withdrawal (Brown et al., 1996). Thus, morphine withdrawalphenomena, including Fos expression, in oxytocin cells are unlikelyto result solely from an increase in the activity of noradrenergicinputs to these cells. Similarly, other well characterized inputsto the supraoptic nucleus are not extensively activated duringor essential for morphine withdrawal (Russell et al., 1992; Murphyet al., 1997). Rather, the withdrawal phenomena in oxytocin neuronsmay follow the triggering of intracellular mechanisms when naloxonedisplaces morphine from chronic occupancy of µ-opioid receptorson theseneurons.

Direct application of naloxone into the supraoptic nucleus of morphine-dependent rats increases intranuclear oxytocin releaseand the firing rate of oxytocin cells (Brown et al., 1997; Ludwiget al., 1997a), indicating that the mechanisms underlying withdrawalexcitation reside in the nucleus itself. The present study furthershows that, in morphine-dependent rats, activation of the c-fosgene (increased Fos protein expression) in supraoptic neuronscan be induced by local application of naloxone within the nucleus.Furthermore, direct chronic application of morphine into the nucleusalso induced morphine dependence in oxytocin cells. Given theabove conclusion that neither the A2 noradrenergic input nor otherinputs drive withdrawal excitation in oxytocin cells (Brown etal., 1998), it appears likely that these mechanisms are locatedwithin the oxytocin neuronsthemselves.

Excitation of parvocellular paraventricular nucleus cells by morphine withdrawal

In conscious rats, the stimulation of c-fos and Fos expression in parvocellular paraventricular nucleus neurons by morphinewithdrawal was evident in conscious and urethane-anesthetizedrats but was essentially suppressed by barbiturate anesthesia.These neurons express corticotrophin-releasing factor and met-enkephalin,and some also express vasopressin. These genes are activated bystressors, including naloxone-precipitated morphine withdrawalin conscious or urethane-anesthetized rats (Lightman and Young,1987; Harbuz et al., 1991). Fos may have a role in regulatingthe vasopressin gene in these neurons (Kovacs and Sawchenko, 1996).The persistence of withdrawal excitation of oxytocin neurons underbarbiturate anesthesia and the suppression of Fos induction inparvocellular paraventricular nucleus neurons points to activationof the latter by the stressful nature of withdrawal in the consciousstate. In particular, this also indicates that, unlike oxytocinneurons, the parvocellular paraventricular nucleus neurons donot themselves develop morphinedependence.

Conclusions

Morphine withdrawal elicits a rapid increase in oxytocin gene transcription that is preceded by, and perhaps results from,an increase in the activity of the c-fos gene in magnocellularneurosecretory cells. The induction of Fos protein expressionin oxytocin neurons by naloxone-precipitated morphine withdrawalresults from actions of morphine and naloxone exerted within thesupraoptic nucleus that do not require ascending noradrenergicinputs to oxytocin cells. Thus, it appears that oxytocin neuronsdevelop morphine dependence and express morphine withdrawal excitationseparately from the afferent inputs. Therefore, the mechanismsthat generate morphine dependence, as well as those that generatewithdrawal excitation, in oxytocin cells reside within the oxytocincells themselves. However, exactly what these mechanisms are hasstill to bedefined.

  FOOTNOTES

Received May 8, 1999; revised Nov. 15, 1999; accepted Nov. 15, 1999.

This work was supported by the Biotechnology and Biological Sciences Research Council (L.E.J. and C.H.B.). H.K.M.M. and C.L.V.were Erasmus Exchange students, partially funded by the EuropeanCommission. We thank Dr. M. Hamamura, Dr. B. E. H. Sumner, andI. Murray for expert assistance with hybridization, K. Opstadfor technical assistance, and Dr. G. Blackburn-Munro for expertassistance in the preparation of thefigures.
Correspondence should be addressed to Dr. J. A. Russell, Department of Biomedical Sciences, University Medical School, Edinburgh,EH8 9XD, UK. E-mail: j.a.russell{at}ed.ac.uk.

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