Normal Female Sexual Development Requires Neuregulin-erbB Receptor Signaling in Hypothalamic Astrocytes

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The Journal of Neuroscience, January 1, 2003, 23(1):230-239

Normal Female Sexual Development Requires Neuregulin-erbB Receptor Signaling in Hypothalamic Astrocytes
Vincent Prevot²^,^*, Carlos Rio¹^,^*, Gyeong J. Cho², Alejandro Lomniczi², Sabine Heger², Craig M. Neville³, Nadia A. Rosenthal³, Sergio R. Ojeda², and Gabriel Corfas¹
¹ Division of Neuroscience, Children's Hospital, Harvard Medical School, Boston, Massachusetts 02115, ² Division of Neuroscience, Oregon Regional Primate Research Center/Oregon Health Sciences University, Beaverton, Oregon 97006, and ³ Cardiovascular Research Center, Massachusetts General Hospital, Charlestown, Massachusetts 02129

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The initiation of mammalian puberty requires the activation of hypothalamic neurons secreting the neuropeptide luteinizinghormone-releasing hormone (LHRH). It is thought that this activationis caused by changes in trans-synaptic input to LHRH neurons.More recently, it has been postulated that the pubertal increasein LHRH secretion in female animals also requires neuron-gliasignaling mediated by growth factors of the epidermal growth factor(EGF) family and their astrocytic erbB receptors. Although itappears clear that functional astrocytic erbB1 receptors are necessaryfor the timely advent of puberty, the physiological contributionthat erbB4 receptors may make to this process has not been established.To address this issue, we generated transgenic mice expressinga dominant-negative erbB4 receptor (DN-erbB4) under the controlof the GFAP promoter, which targets transgene expression to astrocytes.DN-erbB4 expression is most abundant in hypothalamic astrocytes,where it blocks the ligand-dependent activation of glial erbB4and erbB2 receptors, without affecting erbB1 (EGF) receptor signaling.Mice carrying the transgene exhibit delayed sexual maturationand a diminished reproductive capacity in early adulthood. Theseabnormalities are related to a deficiency in pituitary gonadotropinhormone secretion, caused by impaired release of LHRH, the hypothalamicneuropeptide that controls sexual development. In turn, the reductionin LHRH release is caused by the inability of hypothalamic astrocytesto respond to neuregulin (NRG) with production of prostaglandinE₂, which in wild-type animals mediates the stimulatory effectof astroglial erbB receptor activation on neuronal LHRH release.Thus, neuron-astroglia communication via NRG-erbB4/2 receptorsignaling appears to be essential for the timely unfolding ofthe developmental program by which the brain controls mammaliansexualmaturation.

Key words: neuregulin; neuroendocrine; mammalian puberty; hypothalamus; astrocytes; neuron-glia interactions

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The onset of puberty, one of the most critical developmental events in postnatal mammalian life, is determined by changesthat occur within the CNS and, in particular, the hypothalamus.The pubertal activation of the hypothalamic-pituitary-gonadalaxis requires an increased secretion of luteinizing hormone-releasinghormone (LHRH) by neuroendocrine neurons, which in rodents arelocated in the preoptic region of the hypothalamus. These neuronsextend their neurosecretory axons to the median eminence, whereLHRH is released into the portal vasculature for delivery to theadenohypophysis. There, LHRH induces the secretion of pituitarygonadotropin hormones that promote gonadal development and supportreproductive physiology. In this way, LHRH is essential for bothsexual development and mature reproductivefunction.

The mechanisms responsible for the timely release of LHRH during puberty are incompletely understood. Early studies showedthat the increase in LHRH release is not caused by events intrinsicto the LHRH neurons themselves but occurs in response to changinginputs from synaptically connected neuronal networks (Terasawa,1999; Ojeda et al., 2001). However, other experiments suggestedthat, in addition to trans-synaptic communication, neuron-gliasignaling in the hypothalamus might be of critical importancefor the activation of LHRH secretion during female sexual development(for review, see Ojeda et al., 2000).

These studies indicated that receptors of the epidermal growth factor receptor (EGFR) family, also known as erbB receptors,may play important roles in the hypothalamic control of puberty.There are four known members of the erbB receptor family. Threeof them, erbB1, erbB3, and erbB4, bind and are activated by cognateligands. In contrast, erbB2 acts as a coreceptor or auxiliarysubunit recruited by ligand binding to the other receptors (forreview, see Yarden and Sliwkowski, 2001). Hypothalamic astrocytesexpress the erbB1, erbB2, and erbB4 receptors but not erbB3. Inaddition, cells in the hypothalamus express the erbB1 ligand transforminggrowth factor $alpha$ (TGF $alpha$ ) and several forms of the erbB4 ligand neuregulin(NRG) (Ma et al., 1992, 1994, 1999; Chen et al., 1994; Corfaset al., 1995).

Pharmacological inhibition of EGFRs (erbB1) targeted to the median eminence of the hypothalamus (Ma et al., 1992) or inhibitionof erbB2 synthesis via the intracerebral administration of antisenseoligodeoxynucleotides (Ma et al., 1999) delayed the onset of femalepuberty in rats. Moreover, in vitro studies using astrocytes andan LHRH-producing neuronal cell line showed that erbB receptorligands can stimulate LHRH release from the neuronal cells, butdo so indirectly, by inducing astrocytes to secrete prostaglandinE₂ (PGE₂) (Ma et al., 1997, 1999), which can then elicit releaseof the neuropeptide from the neuronal cell line (Voigt et al.,1996). These observations led to the hypothesis that erbB receptorsare components of the cell-to-cell communication system used byastrocytes to regulate LHRH secretion during development and hencethe initiation of puberty. However, despite of the insights offeredby these studies, the physiological contribution of astrocyticerbB4 receptor signaling to normal sexual development has notbeen demonstrated, primarily because of the unavailability ofan animal model in which the function of these receptors is disruptedin a cell-specific manner. Mice lacking the genes encoding NRGor any of its erbB receptors (erbB2, erbB3, or erbB4) die duringembryonic life or at birth (Gassmann et al., 1995; Lee et al.,1995; Erickson et al., 1997; Riethmacher et al., 1997; Wolpowitzet al., 2000), precluding their use to study the involvement oferbB receptors in postnatal events. Furthermore, although theimportance of erbB2 receptors in the control of puberty has beendefined by the ability of intracerebral administration of erbB2antisense oligodeoxynucleotides to delay puberty (Ma et al., 1999),these results identified neither the receptor subtype involved(erbB1 or erbB4) nor the cell type in which an intact receptorcomplement must be present to ensure normal function. To definethe role of the NRG receptors erbB2, erbB3, and erbB4 in astrocytes,we generated transgenic mice in which the function of these receptorsis specifically disrupted in these cells by overexpression ofa dominant-negative erbB4 receptor (DN-erbB4) using the promoterfor theGFAP.

Here we report that DN-erbB4 expression abolishes astrocytic erbB4-erbB2 receptor signaling without affecting that mediatedby erbB1. In keeping with the pattern of GFAP expression in thenormal brain, the mutant receptor is expressed most abundantlyin hypothalamic astrocytes. Mutant female mice have delayed sexualdevelopment and delayed initiation of reproductive capacity. Transgenicfemale mice also show a selective reduction in NRG-induced LHRHrelease from the median eminence and in NRG-induced astrocyticPGE₂ production, whereas responses to TGF $alpha$ are normal. Thus, theresults define the physiological relevance of the NRG-astrocyticerbB4-erbB2 receptor system in the hypothalamic control of femalesexual development. They also establish the concept that thisneuron-glia communication system is a core component of the cell-to-cellsignaling mechanism used by the hypothalamus to control the initiationof mammalianpuberty.

  Materials and Methods

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Introduction
Materials and Methods
Results
Discussion
REFERENCES

Generation of transgenic mice. The LacZ gene was removed from the pGfa2-Lac-1 plasmid (Brenner et al., 1994) by BamHI restriction.The 5.4 kb plasmid backbone containing the Gfa2 promoter was blunt-endedand dephosphorylated. The blunt-ended 2.2 kb DN-erbB4-FLAG DNAwas ligated to the Gfa2-containing plasmid with T4 DNA ligase.Several clones were obtained and characterized by restrictionmapping and sequencing of the junction region. The resulting pGfa2-DN-erbB4plasmid was excised with BglII, and the 5 kb Gfa2-DN-erbB4 DNAwas gel purified (JETsorb; Genomed, Bad Oeymhausen, Germany) andused for the generation of transgenicmice.

Transgenic mice were generated in an FVB background using standard procedures (Hogan et al., 1994). Animals carrying the transgenewere identified by PCR. Tail clips were incubated in 500 µl oflysis buffer (100 mM Tris HCl, pH 8.5, 5 mM EDTA, 0.2% SDS, 200mM NaCl) with 5 µg/ml Proteinase K at 58°C overnight. The supernatantwas subjected to isopropanol precipitation, and the genomic DNAwas resuspended in 100 µl of TE buffer. One microliter aliquotsof DNA were amplified in a 25 µl PCR with the 5' primer TGCTGAAGGAATGGTGTGCand the 3' primer CTTGTCGTCATCGTCTTTG, and the PCR products wereanalyzed by agarose gel electrophoresis. Hemizygous mice of eachline were intercrossed, and putative homozygous mice were identifiedby Southern blot using a DN-erbB4 probe. The genotypes of homozygousmice were confirmed by analyzing the progeny of presumptive homozygotemice backcrossed to wild-typemice.

Growth factors and prostaglandins. Human recombinant NRG $beta$ 1 was initially obtained from Genentech (San Francisco, CA) and thenpurchased from Neomarkers (Union City, CA). TGF $alpha$ was suppliedby Becton Dickinson Biosciences (Bedford, MA), and PGE₂ was obtainedfrom Sigma (St. Louis,MO).

Cell culture. Astrocytes were isolated from the hypothalamus or the whole brain of 1- to 2-d-old wild-type and transgenicmice and cultured as described previously (Ma et al., 1994, 1999).After a growth period of 8-10 d in 75 cm culture flasks containingDMEM-F12 medium supplemented with 10% calf serum, the astrocyteswere isolated from contaminant cells by overnight shaking at 250rpm and were replated in either 15 cm dishes for immunoblot analysisor six well plates for prostaglandin release experiments. Afterreaching 80-90% confluence, the medium was replaced with a serum-free,astrocyte-defined medium consisting of DMEM devoid of phenol red,supplemented with 2 mM L-glutamine, 15 mM HEPES, 5 µg/ml insulin,and 100 µM putrescine (Ma et al., 1999). The cells were used 2d later for the experiments. To examine the effect of NRG $beta$ 1 andTGF $alpha$ on PGE₂ release, the astrocytes were incubated in the presenceof either peptide (at 100 ng/ml each) for 16 hr at 37°C.

Immunoprecipitation and Western blots. Cell cultures were lysed in radioimmunoprecipitation assay buffer, and the resultingprotein extracts were size-fractionated by SDS-PAGE, as describedpreviously (Rio et al., 1997; Ma et al., 1999). The separatedproteins were then transferred to polyvinylidene difluoride (PVDF)membranes and immunoblotted with different antibodies (see below)to identify the DN-erbB4 transgene, GFAP, and the different erbBreceptors. Immunoprecipitations were performed using polyclonalanti-erbB1 and anti-erbB2 antibodies directed against epitopescontained within the intracellular domain of the receptors (sc-03-Gand sc-284, respectively; Santa Cruz Biotechnology, Santa Cruz,CA), and a monoclonal anti-erbB4 antibody (Ab-1, Neomarkers) thatrecognizes an epitope present in the extracellular domain of erbB4.Cell lysates (750-1000 µg of protein) were incubated for 90 minat 4°C with 1.5 µg of each antibody. Thereafter, the receptor-antibodycomplexes were incubated with slurry of protein A-Sepharose (30µl of Sepharose beads per 750 µl immunoreaction for 45 min at4°C). The Sepharose beads were collected by centrifugation, washedtwo times with lysis buffer, resuspended in 2× sample buffer,and boiled for 5 min before loading onto 8% polyacrylamide-SDSgels. After electrophoresis, the size-fractionated proteins weretransferred to PVDF membranes and subjected to immunoblottingusing the monoclonal phosphotyrosine antibody 4G10 (1.5 µg/ml;Upstate Biotechnology, Lake Placid, NY). To develop the immunoreaction,the blots were incubated with horseradish peroxidase-conjugatedsecondary antibodies (Jackson ImmunoResearch, West Grove, PA),developed using enhanced chemiluminescence (Renaissance; NEN,Boston, MA), and exposed to film. After stripping (62.5 mM TrisHCl, pH 6.7, 2% SDS, 100 mM $beta$ -mercaptoethanol, 30 min at 60°C),the membranes were reprobed with the same erbB1 or erbB2 antibodiesused for immunoprecipitation or with a polyclonal anti-erbB4 antibody(sc283; Santa Cruz Biotechnology) that recognizes an amino acidsequence contained within the C terminus of erbB4. The DN-erbB4protein was detected in tissues or cultured cell lysates usingan antibody against the FLAG epitope (10 µg/ml, sc-807; SantaCruz Biotechnology); GFAP was detected with a mouse monoclonalantibody (MAB360; Chemicon, Temecula, CA), and $beta$ -actin was detectedwith a mouse monoclonal antibody(Sigma).

RNase protection assays. Detection of mutant mRNA transcripts was performed using RNase protection assays as reported previously(Ma et al., 1996). Total RNA (15 µg) from brain tissues of 12-d-oldmice was hybridized to a [³²P]UTP-labeled erbB4-FLAG cRNA complementary to nucleotides 1684-2217in the extracellular domain of human erbB4 mRNA (HER4 JM-b) (Plowmanet al., 1993; Elenius et al., 1997) and to the FLAG encoding sequence(CAAAGACGATGACGACAAG). For normalization purposes, the hybridizationmixture also included a [³²P]UTP-labeled mouse cyclophilin probe. After completion of thehybridization, the samples were treated with RNase A and T1 todigest unhybridized RNA species and were size-fractionated byPAGE. The hybridization signals were visualized by exposing thedried gels to Reflection x-ray film(NEN).

Immunostaining. The brains of 12-d-old female mice were fixed by transcardiac perfusion with Zamboni's fixative and subjectedto double immunohistofluorescence confocal microscopy as describedpreviously (Ma et al., 1999), but using 16 µm cryostat sections.DN-erbB4 was detected with a monoclonal antibody raised againstthe extracellular domain of human erbB4 (1:200, Ab-1; Neomarkers).Astrocytes were identified with a rabbit polyclonal antibody toGFAP (1:500, Dako, Carpinteria, CA), and LHRH neurons were identifiedwith the antiserum HU60 (1:3000) (Urbanski et al., 1990). Confocalimages were acquired using a Leica (Nussloch, Germany) TCS NTconfocal system, as described previously (Jung et al., 1999),using the 488 and 568 nm lines of argon and krypton gas lasersto detect the FITC and Texas Red fluorochromes used to visualizeeach immunoreaction. Single-plane images were processed and mergedusing Photoshop 5.0 (Adobe Systems, San Jose,CA).

Incubation of median eminence tissue. The median eminence of 12-d-old mice was dissected as described previously (Negro-Vilaret al., 1979) and incubated at 37°C in 250 µl of Krebs-Ringerbicarbonate buffer, pH 7.4, containing 4.5 mg/ml D-dextrose, underan atmosphere of 95% O₂ and 5% CO₂ with shaking (60 cycles perminute). In all experiments, the tissues were preincubated for30 min, followed by a 2 hr incubation period to determine thebasal release of LHRH. At this time, the medium was replaced byfresh medium containing either NRG $beta$ 1 or TGF $alpha$ (at 100 ng/ml each),or PGE₂ (at 1 µM), and the incubation was extended for an additional2 hr in the presence of eachsecretagogue.

Evaluation of sexual maturation and adult reproductive function. To determine whether the astrocytic expression of DN-erbB4mutant receptors affects the release of pituitary gonadotropins,groups of wild-type and transgenic animals were killed every 4d starting on postnatal day 4, and trunk blood was collected forluteinizing hormone (LH) and follicle-stimulating hormone (FSH)measurement. The uterine weights were also recorded to determinewhether uterine growth (a physiological index of estrogen secretion)is affected in mutant animals. Starting on postnatal day 26, themice were inspected daily for inperforation of the vaginal membrane("vaginal opening"). Thereafter, vaginal lavages were performeddaily to detect the appearance of cornified cells, which identifythe estrous phase of the rodent estrous cycle. Both vaginal openingand cornification of the vaginal epithelium (estrus) result fromthe rise in estrogen secretion that accompanies the onset of pubertyin rodents (Ojeda and Urbanski, 1994). Ovulation normally occurson the day of estrus, but in mice it cannot be assumed to occurunless vaginal cornification is followed by the appearance ofa predominance of leukocytes in the vaginal lavage (Nelson etal., 1990). This abundance of leukocytes defines the diestrousphase of the estrous cycle and indicates that a functional corpusluteum was formed after ovulation. Therefore, both the age atvaginal opening and the age at first estrus were recorded, thelatter being considered as a true first estrus (and thus the ageat first ovulation) only when the cornified cells in the vaginallavages were replaced by at least 2 d of lavages containing primarilyleukocytes.

To determine whether the astrocytic blockade of NGR signaling affects early postpubertal reproductive capacity, young adult(50-d-old) wild-type and mutant mice were exposed to a fertilemale (one male per female), and the interval between the initialexposure and the birth of the first litter wasrecorded.

Ovariectomy. Ovariectomy was performed on postnatal day 12. The ovaries were aseptically removed from animals anesthetizedwith isofluorane via a single dorsal skin incision followed byblunt separation of the underlying muscle-aponeurosis interfase,and different groups of mice were killed 2 and 4 dlater.

Measurements of LHRH, PGE₂, and serum gonadotropin hormones. LHRH released from the median eminence or present in hypothalamictissue and PGE₂ released from astrocytes were detected by radioimmunoassay,as described previously (Ojeda et al., 1986). In the case of LHRH,we used ¹²⁵I-labeled LHRH and the rabbit polyclonal antibody HU60, whichrecognizes the fully processed, mature decapeptide (Urbanski etal., 1990), at a 1:25,000 dilution. The sensitivity of this assayis 0.4 pg per tube. PGE₂ was measured using antibody SC10-11/23(Campbell and Ojeda, 1987) at a 1:8000 dilution and using tritiatedPGE₂ ([5,6,8,11,14,15-N-³H] PGE₂; NEN) as the trace. The sensitivity of this assay was3.6 pg pertube.

Serum levels of LH and FSH were measured by radioimmunoassay using reagents for rat hormones provided by the National Hormoneand Pituitary program of the National Institute of Diabetes andDigestive and Kidney Diseases. FSH was measured in duplicate (15µl) samples from individual mice; LH was measured in single samples(25 µl). All samples from a given experiment were measured inthe sameassay.

Statistics. The differences between several groups were analyzed by ANOVA followed by the Student-Newman-Keuls' multiple comparisontest for unequal replications. The Student's t test was used tocompare two groups. When comparing percentages, groups were subjectedto arc-sine transformation before statistical analysis to convertthem from a binomial to a normal distribution (Zar, 1984).

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The GFAP promoter drives expression of DN-erbB4 to hypothalamic astrocytes

To specifically disrupt the function of all NRG receptors (erbB2, erbB3, and erbB4) in astrocytes, we engineered transgenicmice carrying DN-erbB4 under the control of the human GFAP promoter(gfa2) (Besnard et al., 1991). This mutant receptor contains theextracellular and transmembrane domains of human erbB4 but lacksmost of the intracellular domain, including the entire tyrosinekinase domain and all tyrosine phosphorylation sites (Rio et al.,1997). We have shown previously that high expression of DN-erbB4blocks NRG-induced activation of erbB receptors in muscle andastroglial cells in culture (Rio et al., 1997). The gfa2 promoter,consisting of 2.2 kb of the 5'-flanking region from the humanGFAP gene, directs astrocyte-specific transcription in both cellcultures (Besnard et al., 1991) and transgenic mice (Brenner etal., 1994; Delaney et al., 1996). Although in vivo transgene expressiondriven by this promoter starts at late embryonic stages, highlevels of expression are achieved only after birth (Brenner etal., 1994; Delaney et al., 1996). Several founder mice were obtained,and two independent lines (lines 18 and 34), shown by Westernblot analysis to express DN-erbB4 with the proper cell specificity(see below), were bred to homozygosity to achieve the highestpossible level of DN-erbB4 expression. The mice appeared normal,and no overt disruptions in CNS histology wereobserved.

Western blot and RNase protection assays showed that the transgenic animals express DN-erbB4 in the brain, with the highestlevel of expression in the hypothalamus (Fig. 1A,B). This wasconsistent with the detection of higher levels of GFAP proteinin the hypothalamus than in the cerebral cortex (Fig. 1A), andindicated that the pattern and level of transgene expression wasappropriate. Importantly, the DN-erbB4 protein was undetectablein non-neural tissues involved in reproductive control, such asthe ovaries and uterus (Fig. 1A), or in other organs such as theliver (data not shown). Trace amounts of DN-erbB4 immunoreactivitywere detected in a pituitary gland sample, which included boththe endocrine and neural components of the gland.

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Figure 1. Analysis of transgene expression by Western blot and RNase protection assays. A, DN-erbB4 protein is expressed in both hypothalamic and cortical tissues but not in peripheral organs involved in reproductive function. Notice that the relative abundance of both DN-erbB4 and GFAP proteins is much greater in the hypothalamus than in the cerebral cortex. $beta$ -Actin was used as a loading control. Hyp, Hypothalamus; Ctx, cerebral cortex. B, The content of DN-erbB4 mRNA detected by RNase protection assay is greater in the hypothalamus than in other brain regions. RL, RNA ladder; UP, undigested probe; DP, digested probe; Cyclo, cyclophilin; Hc, hippocampus; Cereb, cerebellum; Wt, wild type.

To determine the pattern of expression of DN-erbB4 at the cellular level, tissue sections were stained with anti-GFAP antibodiesand with antibodies that recognize the extracellular domain oferbB4. These anti-erbB4 antibodies are directed against the humanerbB4 but can also recognize the murine receptor. Confocal microscopydemonstrated that the DN-erbB4 transgene is specifically expressedin astrocytes and verified that the highest level of expressionoccurs in hypothalamic astrocytes (Fig. 2). erbB4 immunoreactivityin astrocytes of the median eminence, the main terminal fieldof neuroendocrine LHRH neurons, was conspicuously higher in micecarrying the transgene (Fig. 2D-F) than wild-type animals (Fig.2A-C). erbB4 immunostaining was also much more abundant in astroglial-likecells surrounding LHRH cell bodies in the preoptic region of transgenicanimals than in wild-type mice, but no expression was detectedin LHRH neurons (Fig. 2G,H). As predicted by the results of theWestern blot analysis (Fig. 1), hypothalamic astrocytes had amuch higher content of immunoreactive DN-erbB4 than astrocytesof the cerebral cortex (Fig. 2I-N). No overt differences in thedensity of astrocytes or neurons of either region were noted betweenwild-type and transgenic mice.

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Figure 2. Analysis of DN-erbB4 expression in the hypothalamus of 12-d-old mice by confocal microscopy. A-F, erbB4 immunoreactivity in astrocytes of the median eminence-medial basal hypothalamus of wild-type mice (A-C) and DN-erbB4 transgenic mice (D-F). A, D, erbB4 staining (green). B, E, GFAP staining (red). C, F, Merged images of erbB4-GFAP immunoreactive cells. G, H, Astrocytes of the preoptic area, which contains the cell bodies of LHRH neurons (red), show a much greater abundance of immunoreactive erbB4 (green) in DN-erbB4 mutant mice (H) than in wild-type animals (G). I-N, In DN-erbB4 mice, erbB4 immunoreactivity (green) is more abundant in hypothalamic astrocytes (L-N) than in astrocytes of the cerebral cortex (I-K). Astrocytes are identified by their GFAP immunoreactivity (red; J, M). Merged images for each brain area are shown in K (cerebral cortex) and N (hypothalamus). Scale bars: A-F, 100 µm; G, H, 10 µm; I-N, 5 µm.

DN-erbB4 expression disrupts astrocytic erbB4 and erbB2 but not EGF receptor signaling

Previous observations have shown that in situ differences in GFAP expression among astrocytes from different brain regionsare no longer apparent in vitro. In keeping with these findings,the mutant receptor was abundantly expressed in cultured astrocytesfrom either the whole brain or the hypothalamus (Fig. 3A). Therefore,astrocytes from the whole brain were used to assess the abilityof the mutant receptor to disrupt erbB-mediated signaling. Westernblot analysis combined with immunoprecipitation showed that NRG-inducedphosphorylation of astrocytic wild-type erbB4 receptors is abolishedin astrocytes obtained from mutant mice (Fig. 3B).

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Figure 3. DN-erbB4 expression in astrocytes blocks ligand-induced erbB4 and erbB2 receptor phosphorylation without affecting erbB1-mediated signaling. A, DN-erbB4 is expressed in cultured astrocytes isolated from either the whole brain (top panel) or the hypothalamus (bottom panel). Cell homogenates prepared from primary astrocyte cultures or COS-7 cells transfected with DN-erbB4 FLAG were subjected to SDS-PAGE and then immunoblotted (IB) with FLAG, erbB4, or GFAP antibodies. B, Inhibition of erbB4 receptor phosphorylation by the transgenic expression of DN-erbB4 in whole brain astrocyte cultures. Cells were treated with NRG $beta$ ₁ (50 ng/ml for 5 min), lysed, immunoprecipitated (IPP) with erbB4 antibodies, subjected to SDS-PAGE separation, and blotted with 4G10 anti-phosphotyrosine antibodies (top panel). The membrane was stripped and incubated with an antibody that recognizes the intracellular domain of erbB4, showing the relative amount of receptor immunoprecipitated in each sample (middle panel). After stripping again, the membrane was incubated with an anti-FLAG antibody, showing that DN-erbB4 was only expressed in mutant cells, and that the level of expression was similar in all conditions. C, DN-erbB4 expression does not affect ligand-induced erbB1 receptor phosphorylation but abolishes erbB2 phosphorylation. Brain astrocyte cultures were treated with betacellulin (50 ng/ml for 5 min), lysed, and immunoprecipitated with either erbB1 (left panel) or erbB2 (right panel) antibodies, before SDS-PAGE and immunoblotting with 4G10 antiphosphotyrosine antibodies, followed by stripping and immunoblotting with either erbB1 or erbB2 antibodies to ensure that each receptor had been immunoprecipitated. Wt, Wild type.

In addition to erbB4, hypothalamic astrocytes express erbB2 and EGF receptors (erbB1) but do not contain erbB3 receptors (Maet al., 1999). Because it is clear that erbB4 can heterodimerizewith erbB2, and because experiments suggest that it may also dimerizewith erbB1 (Tzahar et al., 1997; Pinkas-Kramarski et al., 1998),we tested the possibility that expression of DN-erbB4 would affectastrocytic erbB2 and/or erbB1 signaling. Mutant and wild-typeastrocytes were exposed to betacellulin, an EGF family memberthat binds and activates both erbB1 and erbB4 homodimers and allpossible heterodimeric erbB receptor complexes (Dunbar and Goddard,2000). Then the extent of erbB1 and erbB2 tyrosine phosphorylationwas determined by immunoprecipitation with antireceptor antibodiesfollowed by immunoblotting with anti-phosphotyrosine antibodies.Although betacellulin-induced erbB1 phosphorylation was not affectedin DN-erbB4 expressing astrocytes (Fig. 3C, left panels), tyrosinephosphorylation of erbB2 receptors was abolished (Fig. 3C, rightpanels). These results show that erbB2 receptors, presumably formingunproductive heterodimers with DN-erbB4, cannot be activated byerbB4 ligands. They also demonstrate that DN-erbB4 specificallyblocks astrocytic erbB4-erbB2 signaling but not that oferbB1.

Expression of DN-erbB4 in astrocytes blocks the NRG-induced release of PGE₂ and LHRH from hypothalamic cells

We have shown previously that NRG-induced erbB4-erbB2 activation in cultured astrocytes results in the production of PGE₂,and that PGE₂ induces LHRH secretion from an immortalized LHRH-producingcell line (Ma et al., 1999) and from the median eminence of thehypothalamus (Ojeda et al., 1990). These results suggested thatNRG regulates LHRH production and/or secretion through its effectson astrocytic PGE₂ production. Therefore, we tested whether astrocyticexpression of DN-erbB4 alters the production and/or secretionof PGE₂ and LHRH production by hypothalamic cells. Although bothNRG $beta$ and TGF $alpha$ , a member of the EGF family that signals via erbB1receptors, induced PGE₂ release from wild-type hypothalamic astrocytes,NRG $beta$ ₁ was completely ineffective in cells from DN-erbB4 mutantanimals (Fig. 4A). In contrast, TGF $alpha$ induced PGE₂ release fromDN-erbB4-expressing astrocytes as efficiently as in wild-typecells, also demonstrating that erbB1 signaling is not affectedby DN-erbB4 expression. The presence of DN-erbB4 in astrocytesalso disrupted NRG $beta$ ₁-induced release of LHRH from median eminencefragments containing the neurosecretory terminals of LHRH neurons,without affecting the stimulatory effect of TGF $alpha$ (Fig. 4B). Theseresults suggested that the inability of NRG to induce LHRH releasecould be attributable to a lack of PGE₂ production in DN-erbB4-expressingastrocytes. To test this possibility we determined whether LHRHrelease from median eminence nerve terminals could be inducedby PGE₂. Treatment with the prostaglandin (1 µM) stimulated LHRHrelease equally well in both normal and mutant tissues (Fig. 4C).Thus, the reduced secretory response of LHRH neurons to NRG $beta$ ₁observed in DN-erbB4 mutant mice is the direct result of impairedastrocytic erbB4-erbB2 signaling and not the consequence of aneuronal defect resulting from the astrocytic expression of mutanterbB4 receptors.

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Figure 4. DN-erbB4 expression suppresses NRG-induced release of LHRH from median eminence nerve terminals and PGE₂ from hypothalamic astrocytes. A, NRG $beta$ ₁-induced PGE₂ release from primary cultures of hypothalamic astrocytes is abolished in DN-erbB4 mutants, whereas TGF $alpha$ -stimulated PGE₂ release is not altered [basal PGE₂ release was similar in wild-type and DN-erbB4 cultures (238 ± 13 vs 223 ± 16 pg/ml, respectively)]. B, DN-erbB4 expression suppresses NRG $beta$ ₁-induced but not TGF $alpha$ -induced LHRH release from the median eminence. C, PGE₂ treatment (1 µM for 30 min) stimulates LHRH release from the median eminence of both wild-type and transgenic mice incubated in Krebs-Ringer bicarbonate buffer. In all panels, *p < 0.05, **p < 0.01, ***p < 0.001 versus basal release. Bars are means, vertical lines are the SEM, and the numbers inside the bars are the number of independent observations per group. Wt, Wild type.

Expression of DN-erbB4 in hypothalamic astrocytes results in hormonal defects in vivo

The in vitro experiments described above indicated that the GFAP-DN-erbB4 transgenic mice could have defects in LHRH productionor secretion. Measurements of total hypothalamic LHRH contentduring prepubertal development showed no differences between transgenicand wild-type mice (Fig. 5A), suggesting that LHRH productionis normal. During early mammalian sexual development, a transientactivation of LHRH secretion (Hompes et al., 1982) induces anelevation in serum levels of pituitary gonadotropin hormones,in particular those of FSH (Ojeda and Urbanski, 1994; Grumbachand Styne, 1998). In rodents, this increase occurs during thesecond week of postnatal life (Ojeda and Urbanski, 1994). In wild-typemice, plasma FSH levels rose markedly during the first 2 weeksof life, reaching maximum values by day 12, and decreased abruptlythereafter (Fig. 5B). In contrast, in mutant mice, the FSH peakwas blunted by 50% (Fig. 5B, top panel). Interestingly, the lowmean LH levels observed normally at this stage of developmentwere not different between wild-type and mutant mice (Fig. 5B,bottom panel). It thus appears that the physiological requirementfor erbB4-erbB2 signaling in NRG-induced LHRH release from medianeminence explants in vitro has the appropriate in vivo correlate(i.e., an attenuated infantile surge of FSH that likely reflectsa reduced LHRH release in the face of a normal hypothalamic LHRHcontent).

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Figure 5. Transgenic mice exhibit a normal content of LHRH in the hypothalamus but have reduced serum FSH levels and a reduced FSH secretory response to removal of ovarian steroid inhibitory control during the infantile period of development. A, Hypothalamic LHRH content measured by radioimmunoassay is similar in wild-type and mutant mice throughout neonatal-infantile development. B, The infantile increase in serum FSH levels that characterizes early postnatal development of the hypothalamic-pituitary unit in rodents is blunted in transgenic mice (top panel), whereas the low serum LH levels observed at this time remain unchanged (bottom panel) (10-20 mice per point). C, Ovariectomy (OVX) on postnatal day 12 results in a significant increase in serum FSH levels 2 and 4 d later in wild-type mice but not in mutant mice. Numbers inside the bars are the number of mice per group. Vertical lines are the SEM. In B, **p < 0.01 versus the wild-type group. In C, *p < 0.05 and **p < 0.01 between ovariectomized and nonovariectomized wild-type groups. Wt, Wild type.

To further test the function of the hypothalamic-pituitary-gonadal axis, we examined the effects of ovariectomy, which innormal animals relieves the hypothalamic-pituitary unit of steroid-dependentinhibitory feedback control, resulting in increased circulatinglevels of pituitary gonadotropins (Ojeda and Urbanski, 1994; Grumbachand Styne, 1998). As expected, the ovariectomy of 12-d-old wild-typemice led to a significant increase in serum FSH levels 2 and 4d later (Fig. 5C). In contrast, mutant mice failed to respond(Fig. 5C) within the time frame examined, indicating that theability of the LHRH neuronal network to increase its secretoryoutput in response to the loss of ovary-dependent inhibitory controlis disrupted in theseanimals.

GFAP-DN-erbB4 female mice show delayed sexual maturation and a diminished reproductive capacity in early adulthood

The deficits in LHRH-FSH secretion seen in ovary-intact mutant mice were accompanied by a reduction in uterine growth in bothtransgenic lines (Fig. 6A), indicating that ovarian estrogen outputwas compromised in DN-erbB4 mice. This deficiency is likely toresult from the reduction in FSH levels, because this hormoneis required for both antral follicular growth and ovarian estrogensecretion (Schwartz, 1974; Kumar et al., 1997). Consistent withthe hindering of uterine growth, the time of puberty (definedby the age at first ovulation) was significantly delayed in DN-erbB4animals compared with wild-type mice (Fig. 6B). Once the mutantmice achieved puberty, their reproductive performance was alsoaffected; when a wild-type male was introduced in the cage ofa sexually mature female, the birth of the first litter was delayedby >10 d in DN-erbB4 mice compared with wild-type females (Fig.6C). Young-adult gestational capacity did not appear to be affected,because the mutant animals, once they were able to reproduce,delivered a normal number of pups per litter for at least fiveconsecutive pregnancies.

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Figure 6. Transgenic mice have retarded uterine growth, delayed sexual development, and reduced reproductive capacity in early adulthood. A, Uterine growth is reduced in mutant mice (8-12 animals per point, except day 12, in which each point has 30-44 mice). B, The age at first ovulation is delayed in transgenic mice. C, The age at first pregnancy is delayed in transgenic mice. In all panels, *p < 0.05, **p < 0.01, and ***p < 0.001 versus wild-type values. Circles, triangles, or bars are means; vertical lines represent the SEM. L18 and L34 are transgenic lines. Wt, Wild-type mice. Numbers inside the bars are the number of animals per group.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The present results indicate that erbB4 receptor signaling in hypothalamic astroglial cells is an essential component of themechanisms by which the brain controls female sexual developmentand the acquisition of reproductive competence in mammals. Byshowing that the astrocyte-specific blockade of erbB4-erbB2 receptorfunction disrupts these landmark events, these results providefor the first time evidence that NRG-erbB signaling is necessaryfor specific neuron-astrocyte interactions in the normal postnatalbrain. Although in addition to hypothalamic astrocytes, DN-erbB4is expressed in cerebrocortical and cerebellar astrocytes, thehigh levels of expression required for effective blockade of wild-typereceptors appear to be achieved only in the hypothalamus, suggestingthat this is the site where fully functional erbB4 receptors arerequired for normal sexual development. Because DN-erbB4 was abundantin astrocytes of both the preoptic area (where the LHRH cell bodiesare located) and the median eminence (which contains the LHRHsecretory nerve terminals), it is likely that the astrocytic defectin erbB4 signaling affects LHRH neuronal function at these twoneuroanatomical levels. Previous studies have, in fact, shownthat both sites are subjected to erbB receptor-mediated regulation(Rage et al., 1997). Although we cannot rule out defects in astrocytesoutside the hypothalamus, extensive testing of these mice indicatesthat other brain functions are not affected by astrocytic DN-erbB4expression, thus supporting this conclusion. For example, themutant mice show no overt defects in motor function, coordination,or locomotor activity (data not shown), implying the absence ofdefects in extrapyramidal circuitries and/or cerebellar function.Moreover, recordings from hippocampal slices showed no differencesin basic physiological parameters and in physiological plasticity(long-term potentiation and kindling) (data not shown). Finally,histological analysis of hippocampal and cortical tissues (hematoxylin-eosinstaining, silver staining, immunostaining with neuronal and gliamarkers, electron microscopy) failed to reveal overt abnormalities(data notshown).

Because the mutant erbB4 receptor is highly expressed throughout the hypothalamus, it is possible that the reproductive defectsobserved in DN-erbB4 animals are the consequences of a generalizedalteration in hypothalamic function instead of a specific defectaffecting the neuronal-glial system controlling reproductive maturation.However, this is unlikely, because key indicators of various otherhypothalamic functions show no alterations in DN-erbB4 mice. Themutant mice have normal body weights, implicating a normal rateof growth hormone secretion; they nurse their litters normally,implying no defects in maternal behavior, milk production (prolactinsecretion), or milk ejection (oxytocin secretion); and, finally,routine daily inspection of water bottles showed that water intakewas not different from that of wild-type controls, implying nodefects in the control of water balance (vasopressin secretion).Although it could also be argued that the reproductive defectsmay be secondary to defects in sexual behavior, the clear-cutdefects in LHRH and gonadotropin secretion observed in prepubertalmutant mice speak against such a possibility. Thus, the presentresults support the conclusion that the reproductive phenotypeobserved in DN-erbB4 animals is related to a functional lesionaffecting a specific astrocyte-neuronal communication pathwayrequired for normal LHRHrelease.

A previous study showed that intraventricular infusion of an antisense oligodeoxynucleotide that disrupts erbB2 synthesisdelays the initiation of female puberty in rats (Ma et al., 1999).Although those experiments demonstrated that erbB2 signaling isimportant for this process, they did not define the cell type(neuron or glia) where erbB2 receptors are acting, the regionof the brain where erbB2 signaling contributes to the controlof sexual development, and the erbB receptor subtype (erbB1, erbB3,or erbB4) with which erbB2 heterodimerizes for signaling. Thepresent results provide an answer to these questions. Althoughthe preferential expression of the mutant erbB4 receptors in thehypothalamus establishes this region as the relevant site of erbBreceptor action in the control of female puberty, the use of theGFAP promoter to drive expression of DN-erbB4 only to astrocytesdemonstrates that this cell type is the site where erbB4 signalingmust occur for sexual development to proceed normally. Finally,the finding that DN-erbB4 disrupts both erbB4 and erbB2 function,without compromising erbB1-mediated signaling, identifies erbB4as the necessary partner used by erbB2 in hypothalamic astrocytesto fulfill its function in the central control of sexualdevelopment.

The observation that serum FSH levels were lower in transgenic mice than in wild-type mice at day 12 indicates that regulationof LHRH release by erbB4/2 signaling is important for the regulationof FSH production. Nevertheless, FSH levels still increased duringdevelopment (day 8 vs day 12) in DN-erbB4 transgenic mice, suggestingthat other mechanisms contribute to facilitating the release ofLHRH. Based on our previous studies and on the present results,we propose that astrocytes control LHRH release via a dual mechanisminvolving erbB1 receptor activation by TGF $alpha$ (which is not affectedby overexpression of truncated erbB4 receptors) and erbB4 receptoractivation by NRGs (which are inhibited by DN-erbB4). Thus, assuggested by the in vivo results depicted in Figure 4, the changesin serum FSH observed in the mutant animals are likely to reflect,at least in part, the presence of an intact erbB1-mediated signalingsystem. This could be tested by studying FSH release in animalsin which both erbB1 and erbB4/2 signaling are abolished in hypothalamicastrocytes. However, it must also be recognized that LHRH neuronsare strongly regulated by trans-synaptic inputs, which are likelyto be functional even if both erbB1 and erbB4 astrocytic signalingsystems are inhibited, thus contributing to the developmentalchanges in FSH release observed in the transgenicmice.

In contrast to the receptors, the source and type of the NRG that may be physiologically involved in activating erbB receptorsin hypothalamic astrocytes remains undetermined. Ma et al. (1999)originally reported that NRG $beta$ 2, but not NRG $beta$ 1, was effective ininducing PGE2 release from astrocytes, but the present experimentsshow that NRG $beta$ 1 is active in this system. We believe that thedisparity between these results is most likely attributable toa less-than-optimal biological activity of the reagent used inthe previous study, and that both of these forms can elicit PGE₂release from hypothalamic astrocytes. Although in situ hybridizationstudies suggest that NRGs are primarily expressed by neurons (Chenet al., 1994; Corfas et al., 1995), cultured hypothalamic astrocytesalso contain the mRNAs encoding NRGs (Ma et al., 1999). Thus,it is possible that the astrocytic erbB receptors that contributeto the control of sexual development are activated in a paracrineor an autocrine manner. We do not know whether adult estrus cyclicity,cycle-related changes in hormone levels, and/or reproductive lifespan are affected in the transgenic mice. Future experiments areneeded to address theseissues.

Together, the present results demonstrate that functional integrity of a single astrocytic component involved in neuron-gliasignaling is required for normalcy of the centrally driven developmentalprogram that controls sexual maturation in mammals. As such, theresults provide important insights into the cell-to-cell communicationmechanisms used by the neuroendocrine brain to control the adventof puberty. They also furnish an experimental framework for theconcept that a derangement of specific neuron-glia signaling pathwaysmay underlie some of the poorly understood, centrally originatedalteration in the onset of human puberty. The delayed sexual development,followed by a transient deficiency in adult reproductive capacity,observed in animals with impaired astrocytic NRG-erbB4/2 receptorsignaling is highly reminiscent of the syndrome of idiopathicdelayed puberty of central origin related to gonadotropin deficiencyin humans (Grumbach and Styne, 1998). A hallmark of this syndromeis that affected individuals have delayed puberty but can reproducenormally after reaching sexualmaturity.

  FOOTNOTES

Received May 15, 2002; revised Oct. 8, 2002; accepted Oct. 17, 2002.

^* V.P. and C.R. contributed equally to thiswork.

This research was supported in part by National Institute of Neurological Disorders and Stroke Grant R01 NS35884 (G.C.), bythe EJLB Foundation (G.C.), by Mental Retardation Research CenterGrant NIH P30-HD 18655 (G.C.), and by National Institutes of HealthGrants HD25123 (S.R.O.), HD U54 HD18185 (S.R.O.), and RR00163for the operation of the Oregon Regional Primate Research Center(S.R.O.). We thank Michael Brenner for kindly providing us withthe GFAP promoter, Genentech for its generous gift of NRG- $beta$ ₁,Les Dees for doing the radioimmunoassays for LH and FSH, and HenrykF. Urbanski for his generous supply of antibodies to LHRH. Wealso thank Maria E. Costa for her expert technical assistance,Pieter Dikkes for his help with the histological analysis, andRussell Sanchez, Carl Wang, and Frances Jensen for their helpwith the electrophysiological tests. We are grateful to MichelGreenberg, Thomas Schwarz, and Zhigang He for their valuable commentson thismanuscript.

Correspondence should be addressed to either of the following: Gabriel Corfas, Division of Neuroscience, Children's Hospital,300 Longwood Avenue, Boston, MA 02115, E-mail, gabriel.corfas{at}tch.harvard.edu;or Sergio R. Ojeda, Division of Neuroscience, Oregon NationalPrimate Research Center, 505 Northwest 185th Avenue, Beaverton,OR 97006, E-mail: ojedas{at}ohsu.edu.

G. Cho's present address: Department of Anatomy, College of Medicine, Gyeongsang National University, 92 Chilam-dong, Chinju,Kyungham, 660-751 SouthKorea.

C. Neville's present address: Department of Surgery, Massachusetts General Hospital, 55 Fruit Street, Warren 1157, Boston,MA02114.

C. Río's present address: DIATER, C/Soledad 37, 28330 San Martín de la Vega, Madrid,Spain.

N. Rosenthal's present address: European Molecular Biology Laboratory Programme in Mouse Biology, via Ramarini 32 00016, Monterotondo,Rome,Italy.

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