Reduced Activity of Hypothalamic Corticotropin-Releasing Hormone Neurons in Transgenic Mice with Impaired Glucocorticoid Receptor Function

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The Journal of Neuroscience, May 15, 1998, 18(10):3909-3918

Reduced Activity of Hypothalamic Corticotropin-Releasing Hormone Neurons in Transgenic Mice with Impaired Glucocorticoid Receptor Function
Ivar Dijkstra¹, Fred J. H. Tilders¹, Greti Aguilera², Alexander Kiss², Cristina Rabadan-Diehl², Nicholas Barden³, Sharada Karanth⁴, Florian Holsboer⁴, and Johannes M. H. M. Reul⁴
¹ Graduate School Neurosciences Amsterdam, Department of Pharmacology, Research Institute Neurosciences Vrije Universiteit, 1081 BT Amsterdam, The Netherlands, ² Section on Endocrine Physiology, Developmental Endocrinology Branch, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892, ³ Neuroscience, Centre Hospitalier de l'Université Research Centre and Department of Physiology, Laval University, Québec, Canada G1V 4G2, and ⁴ Max Planck Institute of Psychiatry, Department of Neuroendocrinology, Section Neuroimmunoendocrinology, D-80804 Munich, Germany

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Loss of central glucocorticoid receptor (GR) function is thought to be involved in the development of neuroendocrine and psychiatricdisorders associated with corticotropin-releasing hormone (CRH)hyperactivity. The possible causal relationship between defectiveGR function and altered activity of CRH neurons was studied intransgenic mice (TG) expressing antisense RNA against GR. Immunocytochemicalstudies showed significant reductions in CRH immunoreactive neuronsin the paraventricular nucleus (PVN) and in CRH and vasopressin(AVP) stores in the external zone of the median eminence. Concomitantly,stimulus-evoked CRH secretion from mediobasal hypothalami of TGmice in vitro was reduced significantly. However, CRH mRNA levelsin the PVN of TG mice were marginally lower than those in wild-type(WT) mice. ¹²⁵I-CRH binding autoradiography revealed no differences betweenWT and TG animals in any of the brain regions that were studied.Basal plasma corticosterone (cort) levels and ¹²⁵I-CRH binding, CRH-R₁ mRNA, POMC mRNA, and POMC hnRNA levels inthe anterior pituitary gland were similar in WT and TG mice. Intraperitonealinjection of interleukin-1 $beta$ (IL-1 $beta$ ) increased plasma cort levels,CRH mRNA in the PVN, and anterior pituitary POMC hnRNA similarlyin WT and TG mice. The injection of saline significantly reducedanterior pituitary CRH-R₁ mRNA levels in WT mice, but not in TGmice, whereas IL-1 $beta$ produced a decrease in these mRNA levels inboth strains.
The data show that long-term GR dysfunction can be associated with reduced activity of CRH neurons in the PVN and decreasedsensitivity of pituitary CRH-R₁ mRNA to stimulus-induced downregulation.Moreover, the hypothalamic changes observed in this model suggestthat impaired GR function, at least if present since early embryoniclife, does not necessarily result in CRH hyperexpression characteristicsof disorders such as major depression.

Key words: corticotropin-releasing hormone (CRH); glucocorticoid receptor (GR); transgenic (TG) mice; IL-1 $beta$ ; paraventricular nucleus; HPA axis; CRH receptor

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Impaired glucocorticoid receptor (GR) function has been considered to be an important factor in the development and/or maintenanceof various pathological conditions in man, including (familial)glucocorticoid resistance (Lamberts et al., 1992) and major depression(Barden et al., 1995). Patients suffering from major depressiontypically show increased circulating cortisol levels (Linkowskiet al., 1985; Rubin et al., 1987; Deuschle et al., 1997), inadequatesuppression of cortisol by dexamethasone (Carroll et al., 1968;Rubin et al., 1987), blunted adrenocorticotropic hormone (ACTH)responses to a corticotropin-releasing hormone (CRH) challenge(Holsboer et al., 1984; Gold et al., 1986), and exaggerated ACTHand cortisol responses to CRH after low-dose dexamethasone pretreatment(Heuser et al., 1994). These changes in hormonal responses maybe the result of CRH-producing neurons in the hypothalamic paraventricularnucleus (PVN) (Owens and Nemeroff, 1991; Chrousos and Gold, 1992;Holsboer et al., 1994). In line with this notion is the observationthat patients with major depression show increased CRH levelsin the cerebrospinal fluid (Nemeroff et al., 1984; Banki et al.,1992), increased numbers of CRH and CRH/vasopressin (AVP)-expressingneurons in the PVN, (Raadsheer et al., 1994), and increased CRHmRNA levels in the PVN (Raadsheer et al., 1995). Decreased levelsof central CRH receptors have been found in the frontal cortexof suicide victims, possibly as a result of chronic hyperactivityof brain CRH systems (Nemeroff et al., 1988). Recently, it wasshown that chronically elevated brain CRH levels produce markedchanges in baseline and stimulus-evoked physiological, neurochemical,and behavioral responses, suggesting that chronic CRH hypersecretionis an important factor in the etiology of stress-related disorders(Linthorst et al., 1997). However, until now, studies in humanscould not resolve whether hypersecretion of CRH or GR dysfunctionplays a primary role or any role in the physiological and behavioralanomalies associated with stress-related disorders.

To test whether long-term GR dysfunction is a determining factor for hyperactivity of brain CRH neurons, we studied the numbersof hypothalamic CRH neurons, CRH mRNA levels, CRH and AVP peptidestores, and CRH release from mediobasal hypothalami (MBH) in vitroin transgenic (TG) mice with impaired GR function. In addition,we studied putative changes in CRH receptor expression and regulationin several brain regions.

The TG mouse used as a model for impaired GR function was constructed by the insertion of a transgene expressing constitutivelyantisense RNA against GR (Pepin et al., 1992a). These TG miceshow reduced GR mRNA levels in brain (Pepin et al., 1992a; Marchettiet al., 1994), pituitary (Morale et al., 1995), and some peripheraltissues (Pepin et al., 1992a), reduced brain glucocorticoid receptorbinding (Pepin et al., 1992a), and reduced hypothalamus-pituitary-adrenal(HPA axis) sensitivity to glucocorticoids (Stec et al., 1994;Barden et al., 1997; Karanth et al., 1997). As a consequence ofthe impaired GR function, the regulation of the HPA axis in theseanimals is disturbed. Transgenic animals display exaggerated ACTHresponses to stress and to exogenously administered CRH, whereasthe responses in corticosterone (cort) are normal (Montkowskiet al., 1995; Barden et al., 1997; Karanth et al., 1997) becauseof the hyposensitivity of the adrenal gland to ACTH (Barden etal., 1997). Hence, these TG mice show reduced GR capacity, whichis not compensated for by elevations in circulating glucocorticoidlevels.

In marked contrast to the predicted results, we found a substantial reduction in the number of CRH neurons, CRH mRNA levels,CRH and AVP stores, and in vitro CRH release despite augmentedCRH- and stressor-induced ACTH responses, as previously reportedin these TG mice (Montkowski et al., 1995; Barden et al., 1997;Karanth et al., 1997). To determine whether these responses inTG mice were attributable to adaptation at the level of the anteriorpituitary gland, we studied ¹²⁵I-CRH binding and POMC mRNA, POMC heteronuclear RNA (hnRNA), andCRH receptor mRNA levels under resting conditions and after intraperitonealinjection of interleukin-1 $beta$ (IL-1 $beta$ ), a known activator of centralCRH neurons (Berkenbosch et al., 1987; Sapolsky et al., 1987).

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals. Adult male mice of the B₆C₃F₁ strain (wild-type, WT) were purchased from Charles River Wiga (Sulzfeld, Germany).Male B₆C₃F₁ transgenic mice (TG; line 1.3) were used, in whicha transgene was inserted in the genome constitutively expressingantisense RNA against the GR (Pepin et al., 1992a). The transgenewas driven by a neurofilament promotor. In the cohort of animalsused, GR mRNA levels in the brain and pituitary of TG mice weredecreased by ~50% as compared with the levels in WT mice. Micewere bred in the animal unit of the Clinical Institute of theMax Planck Institute of Psychiatry, Munich, Germany. The animalswere housed five per cage in a temperature (23°C), humidity (60%),and light (lights on from 6:00 A.M. until 6:00 P.M.) controlledroom. Mice used for quantitative immunofluorescence microscopywere housed two per cage. Food and tap water were available adlibitum. The animals were kept in the animal room for at least2 weeks before the experiments.

Experimental procedures. In a first experiment, groups (n = 6) of WT and TG mice (60 d old) were anesthetized quickly withhalothane (Hoechst, Frankfurt am Main, Germany) and decapitated.Their brains were removed from the skull and subsequently wereprocessed for quantitative immunocytochemistry of CRH and AVP,as described elsewhere (De Goeij et al., 1991; Schmidt et al.,1995). In addition, we quantified the relative numbers of CRHimmunoreactive neurons in the PVN of WT and TG mice.

In a second experiment, we studied the release of CRH from MBH in vitro. Groups of mice (n = 10-11) were anesthetized quicklywith halothane and decapitated. The MBHs were dissected by sagittalcuts along the lateral hypothalamic sulci, and frontal cuts weremade through the optic chiasma and anterior margin of the mamillarybodies. A horizontal cut 1 mm from the base of the brain was conductedto separate the island of MBH tissue from the rest of the brain.Subsequently, the dissected tissue was used for in vitro stimulationof CRH release (see below).

In a third series of experiments, groups (n = 10) of WT and TG animals were injected intraperitoneally with 0.9% saline (SAL)or human recombinant IL-1 $beta$ (1 µg/mouse) (provided by Dr. E. B.De Souza and the DuPont-Merck Pharmaceutical Company, Wilmington,DE) or were left undisturbed (UNT). The animals were decapitated4 hr later between 1:00 P.M. and 3:00 P.M. Trunk blood was collectedwithin 45 sec after disturbance of the animals in ice-chilledEDTA-coated (1.5 ml) tubes containing 25 µg of aprotinin. Thisallowed for the measurement of undisturbed cort, but not of restingACTH concentrations in plasma. Plasma was stored at $-$ 20°C untilit was assayed for cort. Brains and pituitaries were dissectedand rapidly frozen in isopentane at $-$ 40°C or in liquid nitrogen,respectively, and thereafter stored at $-$ 70°C until further processingfor in situ hybridization histochemistry (for CRH mRNA and CRH-R₁mRNA in brain and POMC mRNA, POMC hnRNA, and CRH-R₁ mRNA in theanterior pituitary) and ¹²⁵I-CRH binding in brain and anterior pituitary.

Tissue processing for immunocytochemistry of CRH and AVP. After decapitation, brains were removed from the skull and immersion-fixedin 4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.6, for4 hr at 4°C. Subsequently, the brains were incubated in 5% sucrosein 0.1 M phosphate buffer for 48 hr at 4°C. Thereafter, the hypothalamiwere dissected and embedded together (up to 30 specimens) in acryomold containing OCT compound (Sakura Finetechnical, Tokyo,Japan). The cryomold was frozen in isopentane cooled with liquidnitrogen, and frontal serial sections (10 µm) were cut with amotor-driven cryostat (Micron HM 500 M, Walldorf, Germany).

Quantitative immunocytochemistry of CRH and AVP. Serial sections (50 µm interval) were incubated with rabbit antiserum torat/human CRH (5Bo, 1:500) for 48 hr at 4°C. Adjacent serial sectionswere incubated with rabbit antiserum to AVP (Truus, 1:1000). Subsequently,sections were incubated with goat anti-rabbit antiserum conjugatedto FITC (Tago, Burlingame, CA) for 2 hr at room temperature (21°C).Sections were enclosed in Vectashield anti-fading medium (VectorLaboratories, Burlingame, CA). All incubations were performedin 0.1 M Tris-buffered saline (TBS), pH 7.6, containing 0.5% TritonX-100, 0.2% BSA, 1% normal goat serum (Dakopatts, Glostrup, Denmark),and 0.01% sodium azide.

The immunofluorescence staining intensity was quantified by using a computer-controlled microfluorometer (Leitz-Combi, Leitz,Wetzlar, Germany) as described previously (De Goeij et al., 1991;Schmidt et al., 1995). Three sections of each median eminence(50 µm interval) were analyzed. Earlier studies in rats demonstrateda linear relationship between quantitative immunocytochemicaldata and those of radioimmunoassayable CRH in median eminencetissue extracts (r = 0.86-0.99) (Berkenbosch and Tilders, 1988).For specificity of the AVP antiserum, see De Goeij and colleagues(1991). Quantification of AVP stores in the internal zone of themedian eminence (ZIME) served as control for the specificity ofthe AVP signal in the external zone of the median eminence (ZEME).The CRH antiserum 5Bo displays characteristics identical to thoseof 3B3 described earlier (Berkenbosch et al., 1986; De Goeij etal., 1991). Preincubation of 5Bo with 10 µM r/hCRH41 (PeninsulaLaboratories, Belmont, CA) for 2 hr at 37°C prevented CRH immunostainingof murine hypothalami. Preincubation of 5Bo with up to 100 µMAVP (Sigma, St Louis, MO), oxytocin (Bachem Feinchemicalien, Torrance,CA), or $alpha$ MSH (Ciba Geigy, Basel, Switzerland) did not inhibitCRH immunostaining.

CRH immunoreactive neurons in the PVN. To estimate the relative numbers of CRH-producing neurons in the PVN, we embedded hypothalamiof WT and TG mice together and incubated serial 10 µm sections(50 µm apart) throughout the full rostrocaudal extension of thePVN with rabbit antiserum to CRH (5Bo, 1:500) for 2 d at 4°C,followed by incubation with goat anti-rabbit antiserum conjugatedto CY3 (Jackson ImmunoResearch, West Grove, PA) for 2 hr at roomtemperature (21°C). Sections were enclosed as described above.The numbers of nucleated CRH immunoreactive neural profiles inthe PVN of WT and TG mice were counted bilaterally by two independentinvestigators on photographs of coded preparations following ablinded protocol. Only those animals with a complete series ofsections throughout the PVN were used. The data represent cumulativenumbers of nucleated CRH profiles in three sections, 50 µm apart,in the medial part of the PVN.

In vitro CRH release from mediobasal hypothalami. After dissection, each MBH was incubated in 250 µl of Krebs' Ringer's bicarbonate(KRB) buffer supplemented with 20 µM bacitracin to inhibit peptidases.The tissues were incubated at 37°C in an atmosphere of 95% O₂/5%CO₂ in a metabolic shaker (50 cycles/sec) for 45 min. Next, themedium was discarded, and the tissues were incubated with 250µl of KRB or KRB containing 56 mM K⁺ for 30 min to determine basal and depolarization-induced CRHrelease, respectively. Medium was collected and stored at $-$ 80°Cuntil it was assayed for CRH.

Tissue processing for in situ hybridization histochemistry and ¹²⁵I-CRH binding by autoradiography. After decapitation, brains werefrozen in isopentane at $-$ 40°C and stored at $-$ 70°C. For in situhybridization, serial sections (12 µm) were cut in a cryostat(Jung Frigocut, Leica, Germany) at $-$ 22°C. Selected regions werethaw-mounted on poly-L-lysine-coated slides and stored at $-$ 70°Cuntil they were processed for CRH binding or in situ hybridization.Serial sections (60 µm apart) of the PVN were collected on separateslides. Pituitary glands were mounted in OCT compound, and serialsections (12 µm) were cut by using a cryostat at $-$ 22°C. Five consecutivesections (12 µm) were collected per slide.

¹²⁵I-CRH binding by autoradiography in brain and anterior pituitary. Brain and pituitary sections were placed in a dessicatorfor 8 hr at 4°C before the binding assay. Sections were preincubatedfor 15 min at room temperature in 50 mM Tris-HCl, pH 7.4, containing(in mM) 2 EGTA, 5 MgCl₂, 0.1 PMSF, and 140 NaCl plus 0.1% BSAand 100 KIU/ml aprotinin, were rinsed twice in 50 mM Tris-HCl,and were incubated with 3.0 × 10⁵ cpm/8 ml ¹²⁵I-Tyr-oCRH (DuPont-New England Nuclear, Boston, MA) in 50 mM Tris-HCl,pH 7.4, containing (in mM) 2 EGTA, 5 MgCl₂, 0.1 PMSF, and 1 DTTplus 0.1% BSA and 100 KIU/ml aprotinin at room temperature for1 hr. For nonspecific binding, sections were incubated in thepresence of 1 µM unlabeled CRH. Next, the sections were washedthree times in ice-cold 50 mM Tris-HCl, rinsed in distilled water,and dried immediately. Sections were exposed to Hyperfilm $beta$ -Max(Amersham, Arlington Heights, IL).

Sections of control groups and experimental groups were processed and exposed to film simultaneously. Light transmittanceof the autoradiographs was quantitated via a computerized imageanalysis system (Imaging Research, Ontario, Canada). Values obtainedfrom three to four sections of each mouse were averaged beforethe nonspecific binding was subtracted. The data are presentedas the mean transmittance of the number of mice indicated in Resultsor in the figures.

In situ hybridization histochemistry. Before hybridization, brain and pituitary sections were allowed to thaw at room temperaturefor 10 min and then fixed in 4% formaldehyde solution, acetylated,dehydrated, and air-dried.

CRH mRNA levels in the PVN were measured with [³⁵S]deoxy-ATP-labeled 48-mer synthetic oligonucleotide probes directed to exonicsequences from bp 1254 to 1302 of murine CRH cDNA. CRH receptormRNA levels in the anterior pituitary were measured by using a³⁵S-labeled cRNA probe prepared by transcription of a full cDNAclone of the murine type 1 CRH receptor (provided by Dr. A. AbouSamra, Massachusetts Institute of Technology, Boston, MA). POMCmRNA in the anterior pituitary was measured with [³⁵S]deoxy-ATP-labeled 48-mer synthetic oligonucleotide probes directedto exonic sequences of rat POMC, as described previously (Harbuzand Lightman, 1989). This probe shows 98% homology to the equivalentfragment of murine POMC. POMC hnRNA in the pituitaries was measuredwith a ³⁵S-labeled cRNA intronic probe corresponding to 1.2 kb of intronB of the murine POMC gene. The 1.2 kb DNA was generated by PstIdigestion of the genomic clone JA3 (kindly provided by Dr. J.Drouin, Montreal, Canada) and subcloned into PGEM-4Z plasmid.For synthetic oligonucleotide probes, sections were covered with90-100 µl of hybridization solution containing [³⁵S]deoxy-ATP-labeled probe (3 × 10⁶ cpm/ml), 50% formamide, 4× SSC, 500 µg/ml sheared single-strandedDNA, 250 µg/ml yeast tRNA, 1× Denhardt's solution, 10% dextransulfate, and 100 mM DTT. Slides were covered with coverslips andincubated for 18 hr at 42°C in a humidified chamber. After removalof coverslips and three rinses in 1× SSC, slides were washed consecutivelyfour times for 15 min in 1× SSC at 55°C, twice for 30 min in 1×SSC at room temperature, rinsed in water followed by ethanol,and blow-dried. For cRNA probes, the sections were covered with90-100 µl of hybridization solution containing [³⁵S]-labeled cRNA probe (1.3 × 10⁶ cpm/ml), 50% formamide, 50 mM Tris-HCl buffer, 2.5 mM EDTA, 250µg/ml yeast tRNA, 1× Denhardt's solution, 10% dextran sulfate,200 mM NaCl, and 100 mM DTT. Slides were covered with coverslipsand incubated for 18 hr at 55°C in a humidified chamber. Afterthe removal of the coverslips, the slides were washed three timesin 4× SSC for 5 min at room temperature, dehydrated, washed in50% formamide/250 mM NaCl at 60°C for 10 min, RNase-A-treated(20 µg/ml) at 37°C for 30 min, washed in 2× to 0.1× SSC, dehydrated,and blow-dried.

Sections of control groups and experimental groups were processed and exposed to film simultaneously. For determination ofmRNA levels, the sections were exposed to Hyperfilm $beta$ -Max (Amersham).Light transmittance of the autoradiographs was quantitated viaa computerized image analysis system (Imaging Research). Valuesrepresent the mean of the number of mice indicated in Resultsor in the figures.

Hormone assays. Plasma corticosterone concentrations were measured by radioimmunoassay (RIA; ICN Biomedicals, Costa Mesa,CA). The detection limit was 1.5 ng/ml plasma. Intra- and interassayvariations were 4% and 7%, respectively.

The CRH concentrations in the in vitro incubation medium were determined by RIA (Phoenix Pharmaceuticals, Mountain View, CA).The detection limit was 1 pg/tube (10 pg/ml). The intra- and interassayvariations were 4% and 8%, respectively.

Statistical analysis. Statistical significance of differences between groups was determined by ANOVA (one- or two-way ANOVAwhere appropriate), followed by post hoc multiple comparisonswith Bonferroni correction for treatment effects or independentsamples t test for group comparisons. Statistical evaluation wasperformed with the SPSS for Windows statistical program (SPSS,Chicago, IL). Significance was defined at the p < 0.05 level.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

CRH and AVP stores in the median eminence (ZEME) and numbers of CRH neurons in the PVN

Parvocellular CRH-producing neurons in the PVN project their secretory terminals to the ZEME (Fig. 1A). CRH neurons are knownto produce AVP as well, which is stored together with CRH in theZEME (Whitnall et al., 1985; De Goeij et al., 1991; Bertini andKiss, 1991). AVP in the ZIME is located in fibers en passant thatoriginate from magnocellular AVP-producing neurons in the PVNand supraoptic nucleus (SON) and project to the posterior lobeof the pituitary gland.

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Figure 1. A-D, Photomicrographs showing immunocytochemical staining of AVP (A, B) and CRH (C, D) in representative frontal sections of the external zone of the median eminence (ZEME) of wild-type (A, C) and GR antisense transgenic (B, D) mice. ZIME, Internal zone of the median eminence; III, third ventricle. E, CRH and AVP stores in the external zone of the median eminence (ZEME) in TG (hatched bars) and WT mice (black bars). CRH and AVP immunoreactivity in the ZEME and ZIME was evaluated by quantitative immunocytochemistry. CRH and AVP are expressed as a percentage of the mean values found in WT mice (% CTRL). Data are expressed as mean and SEM (n = 6); *p < 0.05, TG versus WT.

As shown in Figure 1B, CRH and AVP stores in the ZEME of untreated TG mice were decreased (t test, p < 0.05) by 45% and 42%,respectively. Quantification of AVP in the ZIME revealed no differencesbetween WT and TG animals, indicating a selective reduction ofpeptide stores in parvocellular CRH neurons in TG mice.

Parvocellular CRH neurons and magnocellular AVP neurons in TG and WT mice do not show a clear differential distribution withinthe PVN, as is the case in rats. Rostrocaudal extensions of theseCRH and AVP neurons are similar in WT and TG mice (Fig. 2A). Asillustrated in Figure 2B, the numbers of nucleated CRH immunoreactiveneural profiles in the PVN of TG mice were decreased by 54% (p< 0.001). The drop in the numbers of CRH neurons was found throughoutthe PVN.

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Figure 2. Distribution of CRH and AVP neurons (A) and relative numbers of CRH immunoreactive neurons (B) in the PVN of transgenic (TG) and wild-type (WT) mice. A, Area containing vasopressin neurons (hatched fields) in frontal sections (50 µm apart) throughout the PVN of a TG (left panels) and a WT mouse (right panels). Note the absence of a clear separation of parvocellular CRH neurons and magnocellular AVP neurons. Dots indicate the positions of nucleated CRH immunoreactive neural profiles. B, Cumulative numbers of nucleated CRH immunoreactive neurons in the PVN of WT and TG mice. Data represent mean and SEM (n = 4-5); *p < 0.05, TG versus WT.

Stimulated CRH release from mediobasal hypothalami in vitro

To study the capacity of hypothalamic CRH neurons to release CRH, we selected an in vitro approach. Unstimulated CRH releasefrom MBH in vitro of both WT and TG animals was below the detectionlimit. Figure 3 shows that the K⁺-stimulated CRH release from MBH of TG mice in vitro was 44% lower(p < 0.05) than that of WT animals.

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Figure 3. Stimulated release of CRH from mediobasal hypothalami (MBH) in vitro of transgenic mice (TG) and wild-type mice (WT). After preincubation for 45 min, depolarization-induced CRH release was evoked by incubation of the MBHs in the presence of KRB containing 56 mM K⁺ for 30 min. Data are expressed as mean and SEM (n = 10-11); *p < 0.05 versus WT.

Unstimulated levels of plasma cort, CRH mRNA, and ¹²⁵I-CRH binding in the brain and POMC mRNA, POMC hnRNA, ¹²⁵I-CRH binding, and CRH-R₁ mRNA in the anterior pituitary gland

As illustrated in Figure 4, baseline plasma cort concentrations were not significantly different in TG as compared with thoseof WT mice. Under basal conditions (UNT) the mean CRH mRNA levelsin the PVN of TG animals were reduced somewhat but were not statisticallydifferent from those in WT mice (Fig. 5).

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Figure 4. Effect of interleukin-1 $beta$ on plasma concentrations of corticosterone (Cort) in wild-type mice (black bars) and GR antisense transgenic mice (hatched bars). Groups of mice were injected intraperitoneally with hrIL-1 $beta$ (1 µg/mouse; IL-1 $beta$ ) or vehicle (SAL) or were left untreated (UNT) and then were decapitated 4 hr later. Data are expressed as mean and SEM (n = 9-10); *p < 0.05 versus SAL and UNT.

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Figure 5. Effect of interleukin-1 $beta$ on CRH mRNA levels in PVN of wild-type mice (black bars) and GR antisense transgenic mice (hatched bars). Groups of mice were injected intraperitoneally with hrIL-1 $beta$ (1 µg/mouse; IL-1 $beta$ ) or vehicle (SAL) or were left untreated (UNT) and then were decapitated 4 hr later. CRH mRNA levels are given as transmittance, and data are expressed as mean and SEM (n = 5); *p < 0.05 versus SAL and UNT.

Autoradiographic analysis of ¹²⁵I-Tyr-oCRH binding revealed a similar pattern in the brains of WT and TG mice (Table 1). Two-wayANOVA revealed no strain differences in ¹²⁵I-CRH binding in any of the brain regions studied, with the exceptionof the inner layers of the olfactory bulb (OB/layer 2-5).


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Table 1. ¹²⁵I-CRH binding in different brain areas of wild-type (WT) and glucocorticoid receptor antisense transgenic (TG) mice

As illustrated in Figures 6 and 7, also anterior pituitary ¹²⁵I-CRH binding and anterior pituitary CRH-R₁ mRNA, POMC mRNA, andPOMC hnRNA levels were similar in untreated WT and TG mice.

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Figure 6. Effect of interleukin-1 $beta$ on ¹²⁵I-CRH binding (top panel) and CRH receptor mRNA levels (bottom panel) in anterior pituitary glands of wild-type mice (black bars) and GR antisense transgenic mice (hatched bars). Groups of mice were injected intraperitoneally with hrIL-1 $beta$ (1 µg/mouse; IL-1 $beta$ ) or vehicle (SAL) or were left untreated (UNT) and then were decapitated 4 hr later.¹²⁵I-CRH binding and CRH-R₁ mRNA are given as transmittance, and data are expressed as mean and SEM (n = 9-10). *p < 0.05 versus UNT; **p < 0.05 versus SAL and UNT; ⁺p < 0.05 versus wild type.

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Figure 7. Effect of interleukin-1 $beta$ on POMC mRNA levels (top panel) and POMC heteronuclear RNA (POMC hnRNA) levels (bottom panel) in anterior pituitary glands of wild-type mice (black bars) and GR antisense transgenic mice (hatched bars). Groups of mice were injected intraperitoneally with hrIL-1 $beta$ (1 µg/mouse; IL-1 $beta$ ) or vehicle (SAL) or were left untreated (UNT) and then were decapitated 4 hr later. POMC mRNA and POMC hnRNA levels are given as transmittance, and data are expressed as mean and SEM (n = 5 and n = 9-10 for POMC mRNA and POMC hnRNA, respectively); #p < 0.05 versus UNT (one-way ANOVA on pooled data of wild-type and transgenic mice).

Interleukin-1 $beta$ -induced responses

As shown in Figure 4, plasma cort concentrations were not statistically different in TG animals as compared with those ofWT animals 4 hr after intraperitoneal administration of saline.At this time, intraperitoneal administration of IL-1 $beta$ had increased(p < 0.05) plasma cort concentrations to the same extent in WTand TG mice.

Like in the untreated animal groups, the mean CRH mRNA levels in the PVN of saline-treated TG animals were somewhat lowerbut were not statistically different from those in saline-treatedWT mice (see Fig. 5). Administration of IL-1 $beta$ tended to increaseCRH mRNA levels in the PVN but reached statistical significanceonly in TG mice (p < 0.05).

Two-way ANOVA of ¹²⁵I-Tyr-oCRH binding to brain sections (see Table 1) showed an overall effect of treatment with saline orIL-1 $beta$ on CRH receptor binding in the striatum and hippocampus(p < 0.05) 4 hr postinjection without any strain differences.Further analyses on pooled data of WT and TG animals revealedthat saline injection increased ¹²⁵I-CRH binding in the ventrolateral and dorsomedial regions ofthe striatum (p < 0.05), as compared with binding in untreatedand IL-1 $beta$ -injected mice, whereas injection of either saline orIL-1 $beta$ decreased ¹²⁵I-CRH binding in the Ammon's horn of the hippocampus (p < 0.05).

Autoradiographic analysis of ¹²⁵I-Tyr-oCRH binding in the anterior pituitary revealed an effect of treatment (two-way ANOVA;p < 0.05), but no strain differences (see Fig. 6, top panel).Post hoc analysis revealed no group differences.

Saline and IL-1 $beta$ treatment had differential effects on CRH-R₁ mRNA levels (see Fig. 6, bottom panel) in WT and TG animals(two-way ANOVA; treatment effect, p < 0.001; strain effect, p< 0.001; interaction treatment and strain, p < 0.001). The injectionof saline markedly reduced CRH-R₁ mRNA levels in pituitaries ofWT mice (p < 0.05), but not of TG mice. Thus, after saline treatmentCRH-R₁ mRNA expression was lower in WT than in TG mice (t test,p < 0.05). After IL-1 $beta$ , both WT and TG mice showed reduced CRH-R₁mRNA levels (p < 0.05), as compared with those of untreated controls.Accordingly, the CRH-R₁ mRNA attained similar levels in WT andTG animals after treatment with IL-1 $beta$ .

POMC mRNA levels were not affected by saline injection or IL-1 $beta$ injection in WT or in TG mice (see Fig. 7, top panel). However,two-way ANOVA revealed a treatment effect (p < 0.05) on primaryPOMC transcript RNA (POMC hnRNA) levels in the anterior pituitary(see Fig. 7, bottom panel) that was similar in WT and TG mice.Further analysis on pooled data of WT and TG animals revealedthat IL-1 $beta$ increased POMC hnRNA levels, as compared with thoseof untreated mice (p < 0.05).

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

In the present study we have demonstrated that the numbers of CRH immunoreactive neurons in the PVN of TG mice are reducedsubstantially, as compared with those of their WT control. Moreover,CRH and AVP stores in the ZEME are decreased in adult TG mice,as is the stimulated CRH release from their MBH in vitro. Thereduction in CRH neurons in TG mice is not reflected in a decreasein basal morning plasma ACTH and cort levels (Barden et al., 1997;Karanth et al., 1997). Earlier reports of elevated hormone levelsin TG mice may have been attributable to nonspecific stress effectsat the time of death (Pepin et al., 1992a,b; Beaulieu et al.,1994; Morale et al., 1995). As reported previously (Beaulieu etal., 1994; Barden et al., 1997; Karanth et al., 1997), we foundsimilar plasma cort concentrations in WT and TG animals in theearly afternoon (this study). Evening plasma ACTH and cort levelsin TG animals have been reported to be either normal (Barden etal., 1997) or decreased (Beaulieu et al., 1994), which is surprisingin view of the presumed role of GR in the regulation of diurnalpeak HPA activity (De Kloet et al., 1993; Bradbury et al., 1994).Because at least in rats HPA axis activity in the evening, butnot in the morning, is driven by CRH (Van Oers and Tilders, 1991;Schmidt et al., 1997), the "normal" or decreased evening levelsof cort in TG animals may be attributable to the decreased activityof hypothalamic CRH neurons rather than to the impaired GR functionper se.

Despite GR impairment and decreased numbers of CRH-expressing neurons in the PVN of TG mice, HPA hormone levels are not alteredseverely either under baseline conditions or after stress, althoughpoststress ACTH responses overshoot in these animals. These observationsindicate that secondary changes may have occurred at the levelof the adrenal and/or pituitary glands. However, TG animals displayno evident adrenal hyperplasia and, rather, show reduced adrenocorticaloutput to ACTH stimulation (Barden et al., 1997). In rats, anintra-adrenal CRH system has been demonstrated that, in conjunctionwith the sympathetic input, plays an important role in the regulationof adrenal sensitivity to ACTH (Van Oers et al., 1992; Jasperand Engeland, 1994). Therefore, hyposensitivity of the adrenalglands to ACTH in TG mice may relate to a generalized hypoactivityof CRH systems in these animals and/or reduced sympathetic activity.Indeed, sympathetic function was found to be reduced in TG mice(see below) (Richard et al., 1993; A. C. E. Linthorst, unpublisheddata). Thus, it is clear that the GR impairment in TG mice isnot compensated for by increased adrenal cort secretion, whichmay result in a functional glucocorticoid insufficiency predominantlyat the CNS and pituitary level (Karanth et al., 1997). In contrastto these TG animals, mice with a complete GR knock-out exhibitadrenocortical hypertrophy and hypersecretion of HPA hormones(Cole et al., 1995), suggesting that a complete ablation of GRfunction entails distinct (counter-) regulatory mechanisms fromthose in TG mice.

In the pituitary gland of TG mice, ACTH responses to various stimuli in vivo and in vitro are enhanced (Montkowski et al.,1995; Barden et al., 1997; Karanth et al., 1997). Accordingly,CRH-stimulated ACTH release from pituitary glands in vitro andin vivo was found to be larger in TG than in WT animals, whichis in line with an overall reduced drive of endogenous CRH. Onthe other hand, pituitary glands of WT and TG animals containcomparable amounts of ACTH (Barden et al., 1997; Karanth et al.,1997), which is consistent with similar levels of both POMC mRNAand POMC hnRNA found in the present study. Because ¹²⁵I-CRH binding and CRH-R1 mRNA expression levels are not differentin TG and WT mice, we considered the possibility that postreceptormechanisms may be enhanced, which may relate to reduced pituitaryGR function. Because of the finding that K⁺-induced ACTH secretion from the pituitary gland in vitro alsois enhanced in TG animals, as compared with that of WT animals,we believe that reduced GR function possibly interfere with mechanismsinvolved in ACTH secretion rather than with receptor activation-dependentmechanisms.

We observed markedly different changes in anterior pituitary CRH-R₁ mRNA levels between WT and TG mice after stressful stimuli.An intraperitoneal saline injection, which may be considered asa weak stimulus, substantially reduced CRH-R₁ mRNA levels in WTmice, but not in TG mice. Peripheral administration of IL-1 $beta$ ,which is a strong stimulus for CRH neurons in the PVN, substantiallyreduced CRH-R₁ mRNA levels in the anterior pituitary of both WTand TG untreated mice. These data indicate that only strong stimuliwere able to decrease anterior pituitary CRH-R₁ mRNA levels inTG mice, suggesting that stimulus-induced reduction of these mRNAlevels appears less sensitive in TG mice than in WT mice. It hasbeen shown that CRH induces acute downregulation of CRH-R1 mRNAin the pituitary gland (Pozzoli et al., 1996; Rabadan-Diehl etal., 1996; Sakai et al., 1996). CRH appears to play an importantrole in the IL-1 $beta$ -induced decrease in CRH-R₁ mRNA levels in therat pituitary, because this response can be prevented by immunoneutralizationof CRH (F. Tilders, G. Aguilera, E. Schmidt, A. Kiss, S. Lolait,unpublished data). Thus, the relative resistance of TG mice tostimulus-induced reduction in CRH-R₁ mRNA levels in the anteriorpituitary may be attributable to the decreased CRH secretion inthese animals. In addition to CRH, GRs have been shown to mediatethe glucocorticoid-induced decline in pituitary CRH-R₁ mRNA levels(Luo et al., 1995; Makino et al., 1995; Pozzoli et al., 1996).Thus, both impaired GR function and reduced hypothalamic CRH expressionare likely to contribute to the mechanisms underlying the relativeresistance of CRH-R₁ mRNA to stressor-induced downregulation inTG mice.

In keeping with observations during acute stress (Rabadan-Diehl et al., 1996), the decreases in pituitary CRH-R1 mRNA afterIL-1 injection were not associated with downregulation of CRHbinding. This is probably attributable to rapid increases in receptorsynthesis or recruitment of cryptic receptors to the plasma membranein response to acute stimulation. In contrast to the effects ofchronic glucocorticoid deficiency induced by adrenalectomy (Wynnet al., 1985; Holmes et al., 1987; Anderson et al., 1993), therewas no downregulation of resting CRH binding levels in the pituitarygland of TG mice. Because pituitary CRH receptor downregulationafter adrenalectomy is attributable mainly to increased CRH andAVP exposure (Holmes et al., 1987; Wynn et al., 1988; Hauger andAguilera, 1993), normal levels of CRH binding in TG mice are consistentwith the hypoactivity of hypothalamic CRH neurons, as shown inthe present study.

Several studies have indicated that alterations in central CRH systems may lead to reciprocal changes in CRH receptors inthe brain. For example, the density of CRH binding sites in thefrontal cortex of suicide victims was found to be decreased, possiblyas a consequence of CRH hyperactivity (Nemeroff et al., 1988),whereas in Alzheimer's disease CRH receptor densities were increasedin frontal, temporal, occipital, and cingulate cortex, possiblybecause of decreased central CRH activity (De Souza et al., 1993).In rats, prolonged central administration of CRH decreased CRHreceptor levels in the amygdala (Hauger et al., 1993). In viewof these observations, we were interested to see whether reducedhypothalamic CRH activity in TG mice would affect CRH receptorsin the brain. Our findings show that, with the exception of theolfactory bulb, no differences in ¹²⁵I-CRH binding exist between WT and TG animals in any of the brainregions that were studied. Although we cannot exclude the possibilitythat compensatory changes in the expression of CRH-BP in thesebrain areas may have occurred during development, this may indicatethat in TG animals extrahypothalamic CRH neuronal systems areless affected than that in the PVN.

Brain CRH neurons are involved not only in the control of HPA responses to stress, but they also play a major role in a widevariety of other stress-induced neuroendocrine, metabolic, autonomic,and behavioral responses (Owens and Nemeroff, 1991). Central administrationof CRH induces behavioral activation in a familiar environment(Sutton et al., 1982; Dunn and Berridge, 1990; Linthorst et al.,1997), induces anxiety-related behavior in unfamiliar conditions(Menzaghi et al., 1994; Heinrichs et al., 1995), increases sympatheticactivity (Brown et al., 1982, 1985; Brown and Fisher, 1983; Diamantet al., 1992b), increases metabolic activity (Rothwell, 1990),induces hyperthermia (Rothwell, 1990; Diamant et al., 1992a; Linthorstet al., 1997), and leads to immune suppression (Labeur et al.,1995). Some of these observations correspond with changes seenin transgenic mice constitutively overexpressing CRH (Stenzel-Pooreet al., 1992, 1994, 1996). In contrast to CRH-overexpressing miceand CRH-treated rats, GR-impaired TG mice show a number of physiologicaland behavioral characteristics that accord with a generally reducedactivity of hypothalamic CRH systems rather than with CRH hyperactivity.Accordingly, TG animals show an overall decreased locomotor activityin their home cage (A. C. E. Linthorst, unpublished data), decreasedoxygen consumption (Richard et al., 1993), cognitive deficits(Montkowski et al., 1995), and decreased indices of sympatheticactivity in peripheral fat tissue and heart (Richard et al., 1993).Accordingly, the greatly increased fat deposition in TG animals(after the age of 4 months), especially accumulated in adiposetissue (Pepin et al., 1992a), may be attributable to the decreasedsympathetic nervous activity rather than to GR dysfunction. Becausesympathetic activity enhances ACTH-dependent cort secretion fromthe adrenal gland (Edwards and Jones, 1987; Engeland and Gann,1989; Bornstein et al., 1990; Jasper and Engeland, 1994; Dijkstraet al., 1996), the decreased sensitivity of the adrenal glandfor ACTH (Barden et al., 1997) may be a consequence of the reducedsympathetic outflow in TG mice. Thus, it is important to notethat the phenotype of the GR defunct mice appears for a largepart to be determined by the reduced hypothalamic CRH activity.

Originally, the TG mice had been developed to serve as a model for the HPA axis aberrations seen in major depression. However,as discussed previously in detail (Barden et al., 1997; Karanthet al., 1997), these TG mice show similarities as well as majordifferences with the neuroendocrine features during this psychiatricillness (and familial glucocorticoid resistance, as well). Theprimary goal of the present study was to gain insight in the cause-and-effectrelationship between CRH hypersecretion and GR dysfunction. Itis clear from our data that long-term GR dysfunction does notnecessarily generate CRH hyperexpression, thus challenging theconcept of CRH hypersecretion in major depression as the consequenceof impaired GR function. Rather, it may be postulated that chronicCRH hypersecretion caused by chronic stress in conjunction withgenetically determined vulnerabilities is the primary determinantproducing GR dysfunction in addition to the observed neurochemical,physiological, and behavioral disturbances (Linthorst et al.,1997).

The hypoactivity of hypothalamic CRH neurons in TG mice clearly differs from the enhancement observed in rats with completedeletion of GR function that is caused by adrenalectomy (Swansonet al., 1983; Whitnall et al., 1985; Whitnall, 1988). The differencecould be the result of the timing of the glucocorticoid deficiency(from early fetal life vs adult). However, this is unlikely becausecomplete GR knock-out mice show increases in CRH mRNA in the PVN(Reichardt and Schutz, 1996). Because the control of CRH expressioninvolves interaction of glucocorticoids with other regulators,it is possible that the degree of glucocorticoid dysfunction (totalin adrenalectomy and GR knock-out animals vs partial in this TGmodel) may determine the outcome. Furthermore, reduced GR function,in addition to direct effects in hypothalamic CRH neurons, islikely to affect stimulatory as well as inhibitory brain circuits,neurotransmitters, and receptors that affect CRH neurons (De Kloetet al., 1997; Herman and Cullinan, 1997). Therefore, the suppressionof hypothalamic CRH may result from a GR dysfunction-induced shiftin the balance between excitatory and inhibitory input.

In addition, changes in mineralocorticoid receptors (MR) may have to be taken into consideration. Although MRs are virtuallyabsent in the PVN (Reul and De Kloet, 1985), they are abundantlypresent in the hippocampus and mediate transsynaptic tonic inhibitionon PVN CRH neurons (Reul and De Kloet, 1985; De Kloet and Reul,1987). However, preliminary observations indicate that hippocampalMR levels are decreased in TG mice (J. Reul, unpublished observations),which is in line with the role of GR in the regulation of MR expression(Reul et al., 1987, 1989). Accordingly, reduced MR levels in thehippocampus would result in enhanced PVN CRH expression, whichis clearly not the case in TG animals. Changes in MR do not, therefore,provide an explanation for the reduced CRH expression in theseanimals.

In conclusion, we demonstrate that transgenic mice expressing antisense RNA directed against GR develop reduced activity ofhypothalamic CRH neurons, indicating that defunct GR, at leastif present since an early embryonic stage, is not necessarilyassociated with CRH hyperactivity. Counter-regulatory mechanismsat the level of CRH-R₁ mRNA regulation may be involved in maintainingthe responsiveness of pituitary corticotrophs during stress. Finally,it seems that a number of phenotypic changes in the physiologyand behavior of the TG animals are a consequence of hypothalamicCRH hypoactivity rather than of GR dysfunction per se.

  FOOTNOTES

Received Dec. 31, 1997; revised Feb. 27, 1998; accepted March 3, 1998.

This work was supported by the Dutch Foundation for Scientific Research (Nederlands Wetenschappelijk Onderzoek, Grant 900-564-034)and the Volkswagen Foundation (Germany; Grant I/70 543). We thankDrs. R. M. Buijs and F. W. van Leeuwen (Amsterdam, The Netherlands)for providing the anti-AVP antiserum "Truus," Dr. E. B. De Souzaand the DuPont-Merck Pharmaceutical Company for providing hrIL-1 $beta$ ,Drs. J. Drouin and A. Abou Samra for providing the murine POMCgenomic clone and the murine CRH receptor clone, respectively,and Mr. A. W. J. W. Janszen for his expert technical assistance.
Correspondence should be addressed to Dr. F. J. H. Tilders, Research Institute Neurosciences Vrije Universiteit, Faculty ofMedicine, Department of Pharmacology, van der Boechorststraat7, 1081 BT Amsterdam, The Netherlands.

Dr. Kiss's present address: Institute of Experimental Endocrinology, Slovak Academy of Sciences, Bratislava, Slovak Republic.

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Materials & Methods
Results
Discussion
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