Neuron-to-Glia Signaling Mediated by Excitatory Amino Acid Receptors Regulates ErbB Receptor Function in Astroglial Cells of the Neuroendocrine Brain

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The Journal of Neuroscience, February 1, 2003, 23(3):915

Neuron-to-Glia Signaling Mediated by Excitatory Amino Acid Receptors Regulates ErbB Receptor Function in Astroglial Cells of the Neuroendocrine Brain
Barbara Dziedzic^*, Vincent Prevot^*, Alejandro Lomniczi, Heike Jung, Anda Cornea, and Sergio R. Ojeda
Division of Neuroscience, Oregon National Primate Research Center/Oregon Health & Science University, Beaverton, Oregon 97006

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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Hypothalamic astroglial erbB tyrosine kinase receptors are required for the timely initiation of mammalian puberty. Ligand-dependentactivation of these receptors sets in motion a glia-to-neuronsignaling pathway that prompts the secretion of luteinizing hormone-releasinghormone (LHRH), the neuropeptide controlling sexual development,from hypothalamic neuroendocrine neurons. The neuronal systemsthat may regulate this growth factor-mediated back signaling toneuroendocrine neurons have not been identified. Here we demonstratethat hypothalamic astrocytes contain metabotropic receptors ofthe metabotropic glutamate receptor 5 subtype and the AMPA receptorsubunits glutamate receptor 2 (GluR2) and GluR3. As in excitatorysynapses, these receptors are in physical association with theirrespective interacting/clustering proteins Homer and PICK1. Inaddition, they are associated with erbB-1 and erbB-4 receptors.Concomitant activation of astroglial metabotropic and AMPA receptorsresults in the recruitment of erbB tyrosine kinase receptors andtheir respective ligands to the glial cell membrane, transactivationof erbB receptors via a mechanism requiring metalloproteinaseactivity, and increased erbB receptor gene expression. By facilitatingerbB-dependent signaling and promoting erbB receptor gene expressionin astrocytes, a neuron-to-glia glutamatergic pathway may representa basic cell-cell communication mechanism used by the neuroendocrinebrain to coordinate the facilitatory transsynaptic and astroglialinput to LHRH neurons during sexualdevelopment.

Key words: glutamate receptors; astrocytes; growth factors; hypothalamus; neuron-glia signaling; erbB receptors; sexual development

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The initiation of mammalian puberty is determined by events that, taking place within the brain, result in an increased pulsatilesecretion of luteinizing hormone-releasing hormone (LHRH), theneurohormone controlling sexual development (Plant, 1994; Terasawa,1999). LHRH neurons, although intrinsically able to release LHRHepisodically (Martínez de la Escalera et al., 1992), do not initiatethe pubertal process themselves. Instead, their secretory activityincreases at puberty in response to changing inputs from functionallyconnected neuronal and astroglial networks (Ojeda and Terasawa,2002).

This dual neuronal-glial input provides the underpinnings for a set of regulatory processes collectively referred to as the"central drive" of puberty (Ojeda and Urbanski, 1994; Plant, 1994;Terasawa, 1999). The changes in central drive leading to the adventof sexual maturity appear to be determined by three major interrelatedevents, two of transsynaptic nature and one involving the activationof a glia-to-neuron communication pathway. A decrease in GABAergicinhibition (Terasawa, 1999 and an increase in glutamatergic stimulationof LHRH neurons (Ojeda and Urbanski, 1994; Bourguignon et al.,2000) currently are considered essential components of the transsynapticmechanism controlling LHRH neurosecretion at puberty (Ojeda andTerasawa, 2002). Perhaps not surprisingly, growth factors requiredfor early development of CNS neurons are emerging as sine quanon constituents of the back-signaling process used by astroglialcells to facilitate LHRH secretion during neuroendocrine sexualdevelopment (Ojeda et al., 2000).

Enhancement of glutamatergic neurotransmission, the primary mode of excitatory transsynaptic communication used by hypothalamicneurons (van den Pol and Trombley, 1993), increases LHRH secretion(Donoso et al., 1990; Claypool et al., 2000) and accelerates theinitiation of puberty in both rats and monkeys (Urbanski and Ojeda,1987; Plant et al., 1989; Urbanski and Ojeda, 1990). Glutamatergicneurons control LHRH secretion via at least two classes of ionotropicglutamate receptors: NMDA receptors, most of which are locatedon interneurons synaptically connected to LHRH neurons (Gore etal., 1996), and kainate receptors, which are expressed more abundantlyon LHRH neurons themselves (Eyigor and Jennes, 1997, 2000).

Astroglial cells regulate LHRH secretion both by inducing plastic rearrangements within the median eminence and by activatingspecific glia-to-glia and glia-to-neuron signaling pathways (forreview, see Ojeda et al., 2000). One of these pathways is setin motion by the epidermal growth factor-related peptides, transforminggrowth factor $alpha$ (TGF $alpha$ ) and neuregulins (NRGs). They elicit LHRHsecretion indirectly (Ojeda et al., 2000) via a juxtacrine/paracrinemode of communication consisting of three steps: ligand-dependentactivation of astroglial erbB-1 and erbB-4 receptors, releaseof bioactive substances (e.g., PGE₂), and stimulation of LHRHsecretion by a direct action of these substances on LHRH neurons(Ma et al., 1997, 1999; Rage et al., 1997). In hypothalamic astrocytesTGF $alpha$ signals via erbB-1 (Ma et al., 1992) and NRGs via erbB-4receptors (Ma et al., 1999). NRG binding to the latter resultsin the formation of heterodimeric erbB-4/erbB-2 complexes thatinitiate intracellular signaling (Ma et al., 1999). Pharmacologicaland genetic evidence now exists demonstrating that both erbB-1and erbB-4 receptors are required independently for normal sexualdevelopment. Thus either the blockade of median eminence erbB-1receptor tyrosine kinase activity (Ma et al., 1992) or an inactivatingpoint mutation of the erbB-1 gene (Apostolakis et al., 2000) delaysthe onset of female puberty in rodents. Similarly, female sexualdevelopment is delayed in mutant mice in which astroglial erbB-4function is disrupted specifically by the targeted expressionof a dominant-negative truncated form of the erbB-4 receptor (Prevotet al., 2003).

Although it follows that both glutamatergic neurotransmission and astroglial erbB-mediated back signaling are critical componentsof the neuroendocrine machinery controlling LHRH secretion duringsexual development, nothing is known about the potential mechanismsthat may be used by the neuroendocrine brain to relate these tworegulatory pathways functionally. The structural and biochemicalsubstrata required for such a relationship to operate are wellestablished, because astrocytes are endowed with glutamate receptors(Blankenfeld and Kettenmann, 1991; Gallo and Ghiani, 2000) andrespond to glutamate stimulation both with changes in immediategene expression (Arenander et al., 1989; McNaughton and Hunt,1992) and with the production of relevant bioactive molecules(Martin, 1992) such as PGE₂ (Bezzi et al., 1998) and glutamateitself (Parpura et al., 1994; Bezzi et al., 1998). The presentstudy demonstrates that the combined activation of ionotropicand metabotropic glutamate receptors (mGluRs) located on astroglialcells enhances the functional capability of astrocytic erbB signalingmodules by favoring, within a short time frame, the establishmentof productive ligand-erbB receptor interactions and inducing ona longer time basis an increase in erbB receptor geneexpression.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Cell culture
Hypothalamic and cerebrocortical astrocytes cultures were prepared from 1- to 2-d-old Sprague Dawley rats as recommended byMcCarthy and de Vellis (1980), with the modifications reportedpreviously (Ma et al., 1994, 1999). After initial purificationthe astrocytes were plated in either six-well plates (at 400,000cells per well) or in 15 cm dishes (at 1-1.5 million cells perdish). After reaching 90% confluence, the medium was replacedwith an astrocyte-defined medium (ADM) (Ma et al., 1999), andthe cells were used 48 hr later forexperiments.

Treatments
After 2 d in ADM the medium was replaced by fresh medium containing 100 µM 1S,3R-ACPD (Research Biochemicals, Natick, MA),100 µM AMPA (Research Biochemicals), or 100 µM 1S,3R-ACPD plus100µM AMPA, and the cultures were continued for 2, 4, or 8 hr. Atthe end of each interval the cells were collected for RNA extraction.When immunohistochemistry was performed, the cells were fixed(see below) 5, 15, and 120 min after initiation of the treatment.For phosphorylation studies (see below) cellular proteins werecollected from 15 cm dishes at 5 and 15 min after glutamate receptorstimulation.

RNA extraction and RNase protection assay
Total RNA was extracted using the procedure of Peppel and Baglioni (1990). The RNase protection assay that was used has beendescribed previously in detail (Ma et al., 1996, 1999). The onlydifference was that, after completion of the hybridization, nonhybridizingspecies were digested by using 20 U of RNase One (Promega, Madison,WI) instead of RNase A plusT1.

Probes
The antisense RNA probes used to detect metabotropic and AMPA receptor mRNAs in RNase protection assays were prepared withDNA templates corresponding to sequences contained in the codingregion of each mRNA. The original cDNAs encoding the entire codingregions of the metabotropic receptors mGluR1 to mGluR6 were generouslyprovided by Dr. S. Nakanishi (Institute for Immunology, KyotoUniversity, Kyoto, Japan). The cDNAs encoding the AMPA receptorsubunits GluR1, GluR2, GluR3, and GluR4 were the generous giftof Dr. J. Boulter (University of California, Los Angeles,CA).

Metabotropic receptors
Metabotropic glutamate receptor 1. A 499 base BglII/SphI fragment, corresponding to nucleotides (nt) 2433-2932 in the intracellular-encodingregion of mGluR1 cDNA (Masu et al., 1991), was subcloned intothe plasmid pSP72 (Promega). Antisense transcripts were preparedby transcription of the template with SP6 RNA polymerase afterlinearization with AccI.
Metabotropic glutamate receptor 2. The mGluR2 DNA template was obtained by cloning a 296 bp NcoI fragment, corresponding tont 1351-1647 in the extracellular domain-encoding portion of ratmGluR2 mRNA (Tanabe et al., 1992), into the NcoI site of pGEM-5zf.After linearization with StuI a cRNA probe was prepared by transcriptionwith SP6 RNApolymerase.
Metabotropic glutamate receptor 3. An mGluR3 cDNA template was prepared by cloning into pSP72 a SphI/SmaI 362 bp fragment,corresponding to nt 1348-1710 in the extracellular domain-encodingportion of rat mGluR3 mRNA (Tanabe et al., 1992). Antisense transcriptswere generated by transcription with T7 RNA polymerase after linearizationof the template with HindIII.
Metabotropic glutamate receptors 4, 5, and 6. The required cDNA templates were prepared by subcloning a HindIII/KpnI 285 bpfragment (nt 1428-1713 in the extracellular domain-encoding portionof rat mGluR4 mRNA) (Tanabe et al., 1992) into pGEM-3Z, a BalI403 bp fragment (nt 727-1129 in the extracellular domain-encodingportion of rat mGluR5 mRNA) (Abe et al., 1992) into the SmaI siteof pGEM-3Z, and a PvuII/PstI 305 bp fragment (nt 2269-2574 inthe transmembrane-intracellular domain-encoding portion of ratmGluR6 mRNA) (Nakajima et al., 1993) into pSP72. After linearizationwith HindIII, EcoRI, or XbaI the corresponding mGluR4, 5, and6 cRNAs were prepared by transcription with T7 (mGluR4) or SP6(mGluR5 and 6) RNApolymerases.

AMPA receptors
Glutamate receptors 1, 2, and 3. The cDNA templates were generated by cloning a PvuII 220 bp fragment (nt 956-1179 in ratGluR1 mRNA) (Hollmann et al., 1989), a KpnI/ApaI 342 bp fragment(nt 1014-1356 in rat GluR2 mRNA) (Boulter et al., 1990), and anEcoRI 279 bp fragment (nt 749-1028 in rat GluR3 mRNA) (Boulteret al., 1990) into the riboprobe vectors pSP72 (GluR1) and pBluescriptSK^+/ (GluR2 and 3). Antisense GluR1 transcripts were generated bytranscribing a XhoI-linearized plasmid with T7 RNA polymerase.The GluR2 and GluR3 cRNA probes were prepared by T3-mediated transcriptionof KpnI and HindIII-linearized plasmids,respectively.
Glutamate receptor 4. A cDNA template was prepared by first removing a XbaI 2548 bp fragment from the original pK46 plasmidcontaining a full-length GluR4 cDNA (Boulter et al., 1990), followedby religation of the remaining plasmid. A shorter antisense probe(206 bp) corresponding to nt 217-423 in rat GluR4 mRNA was generatedby linearizing the cDNA template with NcoI, followed by T3 RNApolymerase-mediatedtranscription.

ErbB receptors
ErbB-1. To generate a probe recognizing the 5' mRNA sequence common to the full-length and truncated forms of erbB-1 (Petchet al., 1990), we excised a 199 bp fragment from a cDNA templatedescribed previously (Junier et al., 1993), using an internalerbB-1 NsiI site and a SpeI site in the multiple cloning siteof pBluescript SK. After religation and linearization with XbaI,an erbB-1 antisense probe protecting 256 bp of erbB-1 mRNA wastranscribed with T7 RNApolymerase.
ErbB-2 and erbB-4. The cRNA probes used to detect erbB-2 and erbB-4 mRNAs were those described previously (Ma et al., 1999).

Reverse transcription-PCR
DNA fragments derived from the coding region of the mRNAs encoding the metabotropic receptor-clustering protein Homer 1a (Brakemanet al., 1997) and the AMPA receptor-interacting/clustering proteinsGRIP (glutamate receptor-interacting protein) (Dong et al., 1997),PICK1 (protein interacting with C-kinase) (Xia et al., 1999),and NSF (N-ethylmaleimide-sensitive fusion protein) (Nishimuneet al., 1998; Song et al., 1998) were generated by reverse transcription(RT)-PCR of total RNA extracted from rat hypothalamic astrocytes,hippocampus, and liver. Then 200 ng of RNA was transcribed intocDNA in a final volume of 20 µl containing 200 U of Maloney murineleukemia virus reverse transcriptase (Life Technologies, GrandIsland, NY), 20 U of RNase inhibitor (Promega), and 25 pmol ofoligo-dT primer. After a 2 hr incubation at 37°C the reactionwas stopped by heating at 95°C for 5min.
PCRs were performed by using 2 µl of each reverse transcription reaction and Taq DNA polymerase (Promega) in a volume of 25-60µl. The thermocycling conditions for Homer 1a, NSF, and PICK1were 95°C for 4 min, followed by 36 cycles of 94°C for 15 sec,55°C for 1 min, and 72°C for 2 min, followed by a final extensionperiod of 7 min at 72°C. The thermocycling conditions for GRIPwere those recommended for touch-down PCR (Hecker and Roux, 1996)
Homer 1a. A 270 bp DNA fragment was amplified with 20-mer oligodeoxynucleotide primers (sense, 5'-TCTTCAGCACTCGAGCTCAT-3',and antisense, 5'-GATGATGCTCAGAGGAGAAT-3') corresponding to nt583-602 and 833-851, respectively, in the open reading frame ofHomer 1a mRNA (Brakeman et al., 1997).
GRIP, glutamate receptor-interacting protein. A 267 bp DNA fragment complementary to nt 3189-3455 in rat GRIP mRNA (Dong etal., 1997) was amplified by using 20-mer primers (sense, 5'-TTCAGTGTGGC-AGATGGCCT-3',and antisense, 5'-TTCTGTTCGCTCCAGTCACT-3').
PICK1, protein interacting with C-kinase. A 246 bp PICK1 DNA fragment corresponding to nt 812-1058 in the murine PICK1 mRNAsequence (Staudinger et al., 1995) was amplified by using 21-merprimers (sense, 5'-ATGACGAGGAATACAGCTGCA-3', and antisense, 5'-GC-AGCACTGCATAGCAGTCA-3'.
NSF, N-ethylmaleimide-sensitive fusion protein. To amplify a 281 bp fragment of NSF mRNA, we used 21-mer primers (sense, 5'-TC-GACGCCATCTGCAAGCAGA-3',and antisense, 5'-ATCCGCAGAC-AGTAGCTGGTG-3') corresponding tont 993-1013 and 1253-1273, respectively, in the coding regionof NSF (GenBank accession number AF142097).
All cDNAs generated by RT-PCR were cloned into the riboprobe vector pGEM-T (Promega), and their identities were verified bysequencing.

Antibodies, growth factors, and inhibitors
The sheep polyclonal antibody used for the immunoprecipitation of erbB-1 was obtained from Fitzgerald Industries (Concord,MA). The rabbit polyclonal antibody used for the immunoprecipitationof erbB-4 (Ab-1) was obtained from NeoMarkers (Fremont, CA). Polyclonalantibodies used for the immunoprecipitation of Homer (sc-8921)and the Western blot detection of erbB-1 (sc-03-G) and erbB-4(sc-283) were purchased from Santa Cruz Biotechnology (Santa Cruz,CA). The rabbit polyclonal antibodies used for the Western blotdetection of GluR2/3 and mGluR5 were obtained from Upstate Biotechnology(Lake Placid, NY). The monoclonal antibody used for the detectionof phospho-Tyr (4G10) levels and the rabbit polyclonal antibodyagainst PICK1 were a generous gift from Drs. Brian Druker (OregonHealth & Science University, Portland, OR) and R. Huganir (JohnsHopkins University, Baltimore, MD), respectively. The secondaryantibodies, anti-mouse and anti-rabbit peroxidase conjugate (HRP),were from Pierce (Rockford, IL), and the anti-goat/sheep HRP (GT-34)was obtained from Sigma (St. Louis, MO). Betacellulin was fromR&D Systems (Minneapolis, MN), and the metalloproteinase inhibitorGM6001 (Ilomastat) was from Chemicon (Temecula,CA).

Immunoprecipitation
After treatment the cells were rinsed once with ice-cold PBS and snap-frozen on dry ice. Cell lysates were prepared in 25mM Tris, pH 7.4, containing (in mM) 50 $beta$ -glycerophosphate, 1.5EGTA, 0.5 EDTA, 1 sodium pyrophosphate, and 1 sodium orthovanadateplus (in µg/ml) 10 leupeptin and pepstatin, 10 aprotinin, 100PMSF, and 1% Triton X-100. Cell lysates were normalized accordingto protein concentration with the BSA kit (Bio-Rad; Hercules,CA). For immunoprecipitation of erbB receptors, Homer and PICK1,equal amounts of protein (0.8-1 mg) contained in a total volumeof 750 µl of lysis buffer were incubated with 2 µg of the respectiveantibody with gentle rocking for 1.5 hr at 4°C. Thereafter, 60µl of protein A-Sepharose (Sigma) was added, and the reactionwas allowed to proceed for 45 min. The Sepharose beads were washedtwice with ice-cold lysis buffer and boiled in 50 µl of samplebuffer containing 187 mM Tris-base, 9% SDS, 15% glycerol, and15% $beta$ -mercaptoethanol, pH 6.8. When it was necessary, the sampleswere stored at -85°C untiluse.

Western blotting
Samples were boiled again after thawing and electrophoresed for 2 hr at 130 V in 4-20% precast SDS-polyacrylamide gels (Gradipore,Frenchs Forest, Australia). After fractionation the proteins weretransferred onto polyvinylidene difluoride membranes (Pierce)for 3 hr at 4°C. Blots were blocked for 1 hr in 2.5% EIA gradegelatin (Bio-Rad, Hercules, CA) in Tris-buffered saline (TBS)at 37°C for phosphotyrosine detection, in SuperBlock blockingbuffer (Pierce) for erbB receptors detection, or in Tween/TBS(TBST) 3% nonfat milk at room temperature for the detection ofPICK1, Homer, GluR2/3, and mGluR5. Then the blots were reactedovernight with their respective primary antibody and washed inTBST before being exposed for 1 hr to HRP-conjugated secondaryantibodies. The immunoreactions were detected with Renaissancechemiluminescence reagents (NEN Life Sciences, Boston,MA).

Immunohistofluorescence-confocal microscopy
The cultures were washed twice with PBS, pH 7.4, and fixed in 4% paraformaldehyde for 30 min at room temperature. After extensivewashes in 0.02 M potassium phosphate buffer containing 0.9% NaCl(KPBS), the cells were incubated for 15 min in KPBS-A (0.02 MKPBS containing 0.4% Triton X-100), followed by 15 min in avidinblocking solution (avidin/biotin blocking kit, Vector Laboratories,Burlingame, CA) and 15 min in biotin blocking solution. Afterthree washes in LKPBS (KPBS containing 0.3% heat-inactivated goatserum and 0.1% Triton X-100) the cultures were incubated for 48hr at 4°C with the primary antibodies diluted in the samebuffer.
Depending on the antibodies used to visualize glutamate receptors or members of the erbB signaling module (see below), astrocyteswere labeled with either a monoclonal antibody to glial fibrillaryacidic protein (GFAP; 1:20,000; Sigma) or anti-GFAP polyclonalantibodies (1:100; Dako, Carpinteria, CA). The GFAP immunoreactionswere developed either with Texas Red-conjugated goat anti-mouseIgGs (1:250; Jackson ImmunoResearch Laboratories, West Grove,PA) when the GFAP antibody was monoclonal or with Texas Red-conjugatedgoat anti-rabbit IgGs (1:250, Jackson ImmunoResearch Laboratories)when the GFAP antibodies were polyclonal. The metabotropic receptormGluR5 and the AMPA receptors Glu2 and Glu3 were detected withrabbit polyclonal antibodies to mGluR5 (Upstate Biotechnology,Lake Placid, NY) or to GluR2/3 (Chemicon International, Temecula,CA), both at a 1:1000 dilution. ErbB-1 receptors were detectedwith sheep antiserum epidermal growth factor (EGF-R; FitzgeraldIndustries) diluted 1:200 and erbB-4 with monoclonal antibodyc-erbB-4, Ab-1 (NeoMarkers), at a 1:100 dilution. TGF $alpha$ was detectedwith rabbit polyclonal antibodies RGG-8040 (diluted 1:200; PeninsulaLaboratories, San Carlos, CA). The appropriate biotinylated goatanti-rabbit and goat anti-mouse IgGs (diluted 1:200) were usedto develop the immunohistochemical reactions of GluR2/3, mGluR5,or erbB-4 receptors with their respective primary antibodies.After several washes with KPBS the cultures were incubated withfluorescein (FITC)-conjugated streptavidin (1:400; Jackson ImmunoResearchLaboratories) for 1 hr at room temperature. The secondary antibodiesused to visualize TGF $alpha$ and erbB-1 were an FITC-conjugated donkeyanti-rabbit immunoglobulin (Vector Laboratories) diluted 1:600to detect TGF $alpha$ and a biotinylated donkey anti-sheep IgG (1:600;Vector Laboratories), followed by Texas Red-labeled streptavidin(1:600; Amersham Biosciences, Piscataway, NJ) to detect erbB-1.Control sections were incubated in the absence of primaryantibodies.
Confocal images were acquired and processed as described previously (Ma et al., 1999; Dissen et al., 2001), using a Leica(Nussloch, Germany) TCS SP confocal system with a 40× Plan Apochromatobjective and a 1.25 numericalaperture.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Hypothalamic astrocytes express the glutamate metabotropic receptor mGluR5 and the AMPA receptor GluR2 and GluR3 subunits

To determine whether metabotropic and AMPA receptor subunits are expressed in hypothalamic astrocytes, we subjected totalRNA from astrocyte cultures maintained in either ADM or serum-containingmedium (SCM) to an RNase protection assay. As observed previouslyin astrocytes of other brain regions (Martin et al., 1992; Condorelliet al., 1997), no mGluR1 mRNA was detected in hypothalamic astrocytescultured in ADM or SCM (Fig. 1). In contrast, and in agreementwith previous reports demonstrating the presence of mGluR5 mRNAin hypothalamic astrocytes in situ (van den Pol et al., 1995)and cortical astrocytes in culture (Miller et al., 1995; Balázset al., 1997; Nakahara et al., 1997), mGluR5 mRNA was expressedin astrocytes grown in either ADM or SCM (Fig. 1). No evidencefor the expression of mGluR2, mGluR3, mGluR4, or mGluR6 mRNAsin either hypothalamic or cerebrocortical astrocytes culturedin ADM or SCM was found, with the possible exception of low levelsof mGluR3 mRNA in astrocytes maintained in SCM (data not shown).Previous studies have reported the presence of mGluR3 in astrocytesin situ (Testa et al., 1994) and in vitro (Petralia et al., 1996;Bruno et al., 1997).

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Figure 1. Detection of Group I (mGluR1 and mGluR5) metabotropic glutamate receptor mRNAs in hypothalamic astrocytes (HA) cultured in astrocyte-defined medium (ADM) or serum-containing medium (SCM), as assessed by RNase protection assay. Note that only mGluR5 mRNA is expressed in these cells. M, RNA molecular markers; UP, undigested probe; DP, digested probe; cyclo, cyclophilin mRNA; L, liver; Hc, hippocampus; ID, incomplete digestion.

The most abundant AMPA receptor subunit mRNA expressed in hypothalamic astrocytes was GluR2 mRNA, which was present in culturesmaintained in either ADM or SCM (Fig. 2). GluR2 mRNA appearedto be equally abundant in hypothalamic and cerebrocortical astrocytes,with levels of expression decreasing when the cells were culturedin the absence of serum. The presence of serum appears to be necessaryfor the expression of GluR1 and GluR3 mRNAs, because they werenot detected in astrocytes cultured in ADM but were clearly presentin astrocytes grown in SCM (Fig. 2). In contrast, only tracesof GluR4 mRNA were detected in hypothalamic and cortical astrocytescultured in either ADM or SCM (Fig. 2). Thus mGluR5 and GluR2are the glutamate receptors most predominantly expressed in hypothalamicastrocytes.

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Figure 2. Detection of AMPA receptor subunits (GluR1-GluR4) in hypothalamic astrocytes (HA) and cerebrocortical astrocytes (CA) cultured in ADM or SCM. Note that only GluR2 mRNA is expressed in both ADM and SCM. Cx, Cerebral cortex. For other abbreviations, see legend to Figure 1.

Immunohistofluorescence-confocal microscopy studies that used antibodies against mGluR5 or GluR2/3 demonstrated that bothproteins are indeed present in these cells (Fig. 3). In both casesthe immunoreactivity was punctuated and appeared unevenly distributed,with dense areas adjacent to areas relatively free of immunoreactivematerial.

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Figure 3. Detection of the metabotropic mGluR5 receptor and the AMPA receptor subunits GluR2/3 in hypothalamic astrocytes cultured in ADM by immunohistofluorescence-confocal microscopy. Note the punctuated aspect and uneven distribution of the immunoreactive material. Scale bar, 20 µm.

Hypothalamic astrocytes express the genes encoding metabotropic and AMPA glutamate receptor anchoring/interacting proteins

To determine whether hypothalamic astrocytes express the mRNAs encoding Homer 1a, a metabotropic receptor-clustering/scaffoldprotein that binds mGluR1 and mGluR5 (Brakeman et al., 1997),and the AMPA receptor-interacting/clustering proteins GRIP (Donget al., 1997), NSF (Nishimune et al., 1998; Song et al., 1998),and PICK1 (Xia et al., 1999), we subjected total RNA from hypothalamicastrocytes to RT-PCR amplification with oligodeoxynucleotide primersintended to amplify DNA segments contained in the coding regionof Homer 1a, GRIP, NSF, and PICK1 mRNAs. After identificationof the PCR products by sequencing, the DNA fragments were usedas templates to prepare cRNA probes for RNase protection assay.Using this assay, we detected in hypothalamic astrocytes the mRNAsencoding Homer 1a, GRIP, NSF, and PICK1 (Figs. 4, 5). Overall,GRIP mRNA was the least abundant and PICK1 the most abundant.The astrocytic content of Homer 1a was similar to that of liverand lung, two peripheral tissues shown to express this protein(Brakeman et al., 1997), and lower than in the hippocampus (Fig.4, top), a region of the brain in which Homer 1a is expressedmore abundantly under resting conditions (Brakeman et al., 1997;Xiao et al., 1998). The content of GRIP mRNA, which encodes anonclustering protein (Xia et al., 1999) that associates withboth GluR2 and GluR3 AMPA receptor subunits (Dong et al., 1997),was much lower in astrocytes than in hippocampal tissue (Fig.4, bottom). Consistent with its preferential expression in theCNS (Püschel et al., 1994), NSF mRNA was more abundant in hypothalamicastrocytes than in liver, a peripheral tissue also expressingthe NSF gene (Püschel et al., 1994), but clearly less than inthe hippocampus (Fig. 5, top). In contrast, PICK1 mRNA encodinga synaptic protein that preferentially colocalizes with GluR2in excitatory synapses and induces clustering of AMPA receptors(Xia et al., 1999) was as abundant in hypothalamic astrocytesas in the hippocampus (Fig. 5, bottom).

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Figure 4. Detection of the mRNA encoding the mGluR1/R5 metabotropic receptor-interacting protein Homer 1a (top) and trace amounts of the AMPA receptor-clustering protein GRIP (bottom) in hypothalamic astrocytes cultured in ADM. Lg, Lung. For other abbreviations, see legend to Figure 1.

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Figure 5. Detection of the mRNAs encoding the AMPA receptor-clustering proteins NSF (top) and PICK1 (bottom) in hypothalamic astrocytes cultured in ADM. For abbreviations, see legend to Figure 1.

Homer/mGluR5 and PICK1/GluR2/3 are associated physically in hypothalamic astrocytes

To determine whether the Homer and PICK1 proteins actually are expressed in hypothalamic astrocytes and are able to interactwith mGluR5 and GluR2/3 as they do in neurons, we performed immunoblotsand coimmunoprecipitation assays. Both receptors and their interactingproteins were detected readily in Western blots (Fig. 6A/D andB/E, respectively). Consistent with the results of RNase protectionassays, hypothalamic astrocytes contain higher levels of PICK1(Fig. 6E) than Homer 1a protein (Fig. 6B). In turn, Homer 1a isexpressed at lower levels than other members of the Homer family(Homer 1b/c) detected by the antibody that was used, which recognizesthe common N terminus of all Homer 1 isoforms. This expressionprofile is in agreement with that observed in the normal brain,in which basal noninduced Homer 1a levels are considerably lowerthan those of the other, constitutively expressed, family members(Xiao et al., 1998). Immunoprecipitation with Homer antibodiesresulted in the coprecipitation of mGluR5 (Fig. 6C), and the immunoprecipitationof PICK1 coprecipitated GluR2/3 (Fig. 6F). Thus hypothalamic astrocytescontain the same metabotropic/AMPA glutamatergic receptor-interactingcellular protein complexes that neurons use for synaptic communication.

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Figure 6. Hypothalamic astrocytes contain mGluR5 receptors (A), the AMPA receptor subunits GluR2/3 (D), and their respective interacting proteins Homer (B) and PICK1 (E). Immunoprecipitation of astrocytic proteins with antibodies against Homer results in the coprecipitation of mGluR5 (C), and the immunoprecipitation of PICK1 coprecipitates GluR2/3 (F). Astr, Astrocytes; Hc, hippocampus.

Coactivation of metabotropic and AMPA/kainate receptors induces cellular redistribution of erbB receptors in hypothalamic astrocytes

Coactivation of AMPA and mGluRs results in astrocytic PGE₂ release via a mechanism that is not set in motion by the activationof each receptor class alone (Bezzi et al., 1998). To determinewhether AMPA and metabotropic receptors are able to affect erbBreceptor physiology individually or require a similar interaction,we exposed hypothalamic astrocytes cultured in ADM to either AMPAor tACPD alone or to a combination of both agonists. Immunohistofluorescence-confocalmicroscopy examination of the treated cells showed that underunstimulated conditions a significant fraction of the erbB-4 receptorshad a perinuclear localization (Fig. 7A,A1; examples denoted byarrowheads) suggestive of an association of the protein with theGolgi apparatus. Although activation of metabotropic receptorsalone with tACPD somewhat changed this localization (Fig. 7B,B1;examples denoted by arrows), treatment with AMPA (Fig. 7C,C1)and, particularly, coactivation of metabotropic and AMPA/kainatereceptors (Fig. 7D,D1) resulted in redistribution of erbB-4 receptorimmunoreactive material to the cell membrane (examples denotedby arrows). Similar changes were observed in the case of erbB-1receptors (data not shown).

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Figure 7. Coactivation of metabotropic and AMPA receptors induces cellular redistribution of erbB-4 receptors in hypothalamic astrocytes as assessed by immunohistofluorescence-confocal microscopy. Under basal unstimulated conditions a substantial fraction of the erbB-4 immunoreactive material has a perinuclear localization (A, A1; examples denoted by arrowheads). Treatment with tACPD to activate metabotropic receptors partially changes this localization (B, B1; examples of redistribution denoted by arrows), but AMPA (C, C1) and especially tACPD plus AMPA (D, D1) induce redistribution of the immunoreactivity to the cell membrane (denoted by arrows). Scale bar, 40 µm.

Coactivation of metabotropic and AMPA/kainate receptors induces physical approximation of erbB receptors and their respective ligands on the cell membrane of astrocytes

Under basal unstimulated conditions a substantial fraction of TGF $alpha$ and its erbB-1 receptor appeared to have a perinuclearand cytoplasmic localization (Fig. 8, top panels). Little, ifany, immunoreactivity was associated with the cell membrane (Fig.8, arrowheads) visualized by differential interference contrast(DIC) (Fig. 8, bottom panels, arrowheads). Within 15 min of simultaneouslyexposing the astrocytes to tACPD and AMPA, we could visualizeboth TGF $alpha$ and erbB-1 immunoreactive material in apparent associationwith cell membranes (Fig. 8, middle panels, examples denoted byarrows; DIC image shown in bottom panels). Overlapping of bothimmunoreactivities was also evident (Fig. 8, right middle panel),suggesting a close proximity of the TGF $alpha$ ligand to its erbB receptor.Similar changes were observed in the case of NRG- $beta$ and its erbB-4receptor (data not shown).

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Figure 8. Coactivation of metabotropic and AMPA receptors enhances the physical proximity of TGF $alpha$ and its erbB-1 receptor on the cell membrane of cultured astrocytes as assessed by immunohistofluorescence-confocal microscopy. Under basal unstimulated conditions both TGF $alpha$ and erbB-1 immunoreactivities have a predominant perinuclear and cytoplasmic localization (top panels), with almost no detectable material associated to cell membranes (examples of this absence are denoted by arrowheads). Within 15 min of concomitant treatment with tACPD (to activate metabotropic receptors) and AMPA (to activate AMPA/kainate receptors) a fraction of both TGF $alpha$ and erbB-1 immunoreactivities becomes associated to the cell membrane and in close proximity with each other (middle panels; examples of regions exhibiting overlapping immunoreactivity in association with the cell membrane are denoted by arrows). The two bottom panels depict DIC images of the cells shown in the top panels, identifying the cell boundaries (arrowheads point to cell membranes lacking TGF $alpha$ or erbB-1 immunoreactivity in unstimulated cells; arrows point to cell membranes showing overlapping TGF $alpha$ and erbB-1 immunoreactive material). Scale bar, 20 µm.

Both TGF $alpha$ and its receptor erbB-1 also were seen in the cell nucleus of both unstimulated and treated cells, in agreementwith recent observations showing the nuclear localization of bothproteins (Lin et al., 2001; Grasl-Kraupp et al., 2002), wherethey may function as transcription factors (Lin et al., 2001).

Coactivation of metabotropic and AMPA/kainate receptors leads to a metalloproteinase-dependent activation of astrocytic erbB receptors

To determine whether the apparent ligand/erbB receptor approximation induced by AMPA/tACPD treatment leads to a productiveinteraction, we examined treated and untreated astrocytes forerbB receptor phosphorylation. Within 5-15 min of exposure totACPD/AMPA there was tyrosine phosphorylation of both erbB-1 anderbB-4 receptors (Fig. 9A), indicating that the physical approximationbetween TGF $alpha$ and NRG and their respective receptors suggestedby confocal microscopy indeed results in receptor activation.As expected, exposure of the cultures to betacellulin, an EGFfamily member that binds and activates both erbB-1 and erbB-4homodimers and all possible heterodimeric erbB receptor complexes(Dunbar and Goddard, 2000), resulted in strong phosphorylationof both erbB-1 and erbB-4 receptors (Fig. 9A).

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Figure 9. A, Concomitant activation of metabotropic and AMPA receptors results in the metalloproteinase-dependent transphosphorylation of both erbB-1 and erbB-4 receptors in hypothalamic astrocytes. Left, ErbB-1 receptors. Astrocytes were cultured in serum-defined medium and were exposed to tACPD/AMPA (at 100 µM each) for 15 min. To block metalloproteinase activity, we pretreated some cultures for 30 min with GM 6001 (50 µM). Proteins were collected after the AMPA/tACPD treatment and immunoprecipitated (IP) with a specific erbB-1 antibody, electrophoresed to size-fractionate the immunoprecipitated species, and immunoblotted (IB) with antibodies to phosphotyrosine (4G10). Then the immunoblot was stripped and reprobed with antibodies to erbB-1 to ensure that equal amounts of erbB-1 protein had been immunoprecipitated and loaded on the gel. Right, ErbB-4 receptors. Astrocytes were treated with tACPD/AMPA (at 100 µM each) for 5 min and exposed to GM 6001 for 30 min before this treatment. After the treatment with AMPA/tACPD the erbB-4 was immunoprecipitated, and the phosphorylated species were detected by immunoblotting with antibody 4G10. Then the immunoblot was stripped and reprobed with antibodies to erbB-4. B, Hypothalamic astrocytes were cultured as indicated above; the cellular proteins were collected and immunoprecipitated with specific antibodies to either erbB-1 or erbB-4. After electrophoresis of the immunoprecipitated species the proteins were transferred to nylon membranes and immunoblotted with antibodies to either Glu2/3 or mGluR5.

Transactivation of erbB-1 receptors induced by activation of G-protein-coupled receptors has been shown to involve cleavageof membrane-bound erbB ligands by metalloproteinases (Prenzelet al., 1999). Moreover, TACE [tumor necrosis factor- $alpha$ -convertingenzyme; ADAM-17 (a disintegrin and metalloproteinase)], a memberof the ADAM family of metalloproteinases, has been shown to beessential for the release of the mature TGF $alpha$ peptide from itsmembrane-anchored precursor (Peschon et al., 1998). It then followsthat that regulation of ligand availability by metalloproteinase-dependentmechanisms may be an integral component of the process by whicherbB receptors are activated by their ligands. To determine whetherthis mechanism contributes to the process by which glutamate receptorsinduce astrocytic erbB receptor phosphorylation, we treated hypothalamicastrocytes with GM6001, a broad spectrum inhibitor of metalloproteinaseactivity, for 30 min before exposing them to tACPD/AMPA. As shownin Figure 9, inhibition of metalloproteinase activity obliteratedthe ability of these glutamate receptor agonists to induce botherbB-1 and erbB-4 receptor phosphorylation. Thus cleavage of erbBreceptor ligands followed by binding to their respective receptorsis likely to underlie the activation of erbB receptor signalinginduced by glutamate on hypothalamicastrocytes.

The functional relationship between AMPA/metabotropic receptors and astrocytic erbB receptors shown by the aforementionedstudies may reflect the existence of a physical association betweenthese receptors. To examine this possibility, we performed coimmunoprecipitationassays and found that immunoprecipitation of either erbB-1 orerbB-4 results in the coprecipitation of GluR2/3 and mGluR5 (Fig.9B). Similar assays performed to determine whether erbB-1 and/orerbB-4 is/are in complex with either Homer or PICK1 resulted ina low level of coprecipitation (data not shown), suggesting theabsence of a direct interaction between theseproteins.

Coactivation of metabotropic and AMPA/kainate receptors induces erbB receptor expression in hypothalamic astrocytes

Treatment of hypothalamic astrocytes for 2-8 hr with either tACPD or AMPA (at 100 µM each) to activate selectively the metabotropicor AMPA/kainate receptors did not affect the steady-state levelsof the mRNAs encoding erbB-1, erbB-2, or erbB-4, the three membersof the erbB family of tyrosine kinase receptors expressed in thesecells (Ma et al., 1999) (Fig. 10). In contrast, coactivation ofAMPA/kainate metabotropic receptors significantly (p < 0.05) increasederbB-1 and erbB-2 mRNA levels within 4 hr of treatment (Fig. 10),with the effect persisting after 8 hr (p < 0.01). Unexpectedly,the erbB-4 gene did not respond like its congeners, because erbB-4mRNA content remained unchanged throughout the duration of thetreatment (Fig. 10).

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Figure 10. Coactivation of metabotropic and AMPA receptors increases steady-state levels of the mRNA encoding the tyrosine kinase receptors erbB-1 (top panels) and erbB-2 (middle panels), but not erbB-4 (bottom panels), in astrocytes cultured in ADM as assessed by RNase protection assay. The mRNA levels are expressed in arbitrary densitometric units as the ratio between the erbB mRNA signal and the signal obtained with the constitutively expressed gene cyclophilin in each sample. The numbers above each column are the number of independent observations per group. Error bars indicate SEM; *p < 0.05 and **p < 0.01 versus untreated control group.

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The present results indicate that costimulation of metabotropic and AMPA receptors on hypothalamic astrocytes leads to transactivationof erbB-1 and erbB-4 receptor signaling in these cells. The cellularunderpinnings of this activation include recruitment of the erbBreceptors to the cell membrane, physical approximation of thereceptors to their respective membrane-bound TGF $alpha$ and NRG ligands(also located on astrocytes), and the phosphorylation of eacherbB receptor by a mechanism that appears to require processingof erbB ligand precursors by extracellular proteases of the matrixmetalloproteinase family. By revealing the involvement of glutamatereceptors in a neuron-to-glia communication pathway able to activateerbB receptor signaling in hypothalamic astrocytes, these resultsimplicate this pathway as a mechanism that the neuroendocrinebrain may use to coordinate the activation of glutamatergic neuronsand astroglial cells during sexualdevelopment.

The increase in LHRH secretion required for the initiation of the pubertal process appears to be determined by a coordinateddecrease in transsynaptic GABA inhibition of LHRH neuronal function(Terasawa, 1999), an increase in glutamatergic inputs to theseand other synaptically connected neuronal networks (Bourguignonet al., 2000; Ojeda et al., 2001), and the activation of a glia-to-neuronsignaling pathway mediated by erbB receptors and their ligandsoperating in astrocytes of the neuroendocrine brain (Ojeda etal., 2000) (for review, see Ojeda and Terasawa, 2002). Althougheach of these regulatory mechanisms has been characterized individually,the cell-cell mechanisms responsible for the coordination of neuron-to-neuronand neuron-to-glia inputs to the LHRH neuronal network have notbeen identified. Emerging evidence suggests that in other regionsof the brain GABAergic neurons are controlled by glutamatergicneurons, which use AMPA and kainate receptors to inhibit GABAneurotransmisssion (Rodriguez-Moreno and Lerma, 1998; Min et al.,1999; Satake et al., 2000). The existence of such a glutamate-to-GABAhierarchy in hypothalamic neuronal circuitries, predicted by thepredominance of glutamatergic over GABA synapses in this brainregion (Thind and Goldsmith, 1995), has led to the suggestionthat an increase in glutamatergic activity is one of the primarychanges underlying the activation of LHRH release at puberty (Ojedaand Urbanski, 1994; Bourguignon et al., 1995). In contrast toits kainate receptor-mediated inhibition of GABAergic neurotransmission,glutamate uses both NMDA and kainate receptors to stimulate LHRHrelease (Urbanski and Ojeda, 1987; Plant et al., 1989; Urbanskiand Ojeda, 1990). Although a significant fraction of the kainatereceptor-mediated stimulation appears to be exerted directly onLHRH neurons (Eyigor and Jennes, 1997; Eyigor and Jennes, 2000),the NMDA-mediated stimulation may require the intermediacy ofother excitatory neurotransmitter systems (Gore et al., 1996)that, endowed with NMDA receptors, are connected synapticallyto LHRH neurons. The present results, considered in conjunctionwith these observations, suggest that, in addition to NMDA andkainate receptors required for the coordination of neuron-to-neuroncommunication, glutamate uses metabotropic and AMPA receptorsto coordinate neuron-to-astrocyte signaling in the developinghypothalamus.

It was demonstrated previously that the coactivation of AMPA/kainate and metabotropic receptors on astrocytes results in astrocyticglutamate release and that this release requires the productionof prostaglandin E₂ (Bezzi et al., 1998). In contrast, the independentactivation of each of these two receptor subtypes was ineffective.By now showing that coactivation of AMPA and metabotropic receptorsresults in initiation of erbB-mediated signaling, our resultsexpand these observations and raise the possibility of an involvementof erbB receptors in the process by which neuronal glutamate inducesastrocytic PGE₂ formation. Astroglial erbB-1 and erbB-4 receptorsmay contribute to this process because their ligand-mediated activationresults in release of PGE₂ (Ma et al., 1997, 1999), which thenact on LHRH neurons to elicit LHRH secretion. In addition to demonstratingthe interdependent involvement of metabotropic and AMPA receptorsin glutamate-induced activation of astrocytic erbB signaling,our RNase protection assays and immunoblot analyses identify mGluR5and GluR2 as the receptor subtypes that are involved. Furthermore,they demonstrate that Homer and PICK1, i.e., the same proteinsinteracting with these receptors in synapses, are present in hypothalamicastrocytes and that, like in neurons, mGluR5/Homer and Glu2/3/PICK1are associated physically. The role that these proteins have inastrocytes is unknown, but one of their functions may be to targetmGluR5 and GluR2 receptors to sites on the cell membrane nearerbB receptors. This possibility is supported by the finding thatimmunoprecipitation of either erbB-1 or erbB-4 receptors resultsin the coprecipitation of both GluR2/3 and mGluR5. Consistentwith this view, Homer proteins have been shown to target mGluR5to either dendrites or axons, depending on the type of Homer proteinthat is involved (Ango et al., 2000), and a very recent reportdemonstrated that mGluR 5 is associated physically with erbB-1receptors in cerebrocortical astrocytes (Peavy et al., 2001).Our results show that GluR2/3 and mGluR5 receptors share witherbB-1/erbB-4 a functional relationship that allows astrocytesto transduce glutamatergic inputs into growth factor receptortyrosine kinase-mediated signaling. The existence of such a relationshipis demonstrated further by the recent finding that mGluR5-mediatedactivation of extracellular signal-regulated kinase (ERK) phosphorylationin astrocytes requires the intermediacy of erbB-1 (Peavy et al.,2001).

We do not know the mechanism used by mGluR5/GluR2 receptors to promote the recruitment of erbB receptors and their ligandsto the cell membrane. One possibility is that Homer, and perhapsPICK1, is involved in this process. There is substantial evidencethat Homer acts in neurons to regulate membrane targeting (Angoet al., 2000) and clustering of metabotropic receptors (Xiao etal., 1998), in addition to coupling these receptors to membraneion channels (Kammermeier et al., 2000) and membrane proteinsinvolved in calcium signaling (Tu et al., 1998). Homer also maymediate interactions of membrane receptors with the actin cytoskeleton(Foa et al., 2001). Similar homologous and heterologous receptor-clusteringfunctions have been ascribed to PICK1 (Xia et al., 1999; Boudinet al., 2000). Our results show the existence of distinct physicalassociations between mGluR5 and Homer, Glu2/3 and PICK1, and eachof these two receptors with erbB-1 and erbB-4, but a much weakerassociation between Homer or PICK1 with the erbB receptors. ThusHomer and PICK1 may not be involved directly in recruiting astrocyticerbB receptors and their ligands to the cell membrane and bringingthem together with the activation of mGluR5/GluR2 receptors. However,their association with Glu2/3 and mGluR5 (which in turn are associatedwith the erbB receptors) indicates that both are part of the glutamate/erbBreceptor complex that functions in astrocytes to transduce glutamatergicinputs into erbB-mediatedsignaling.

In addition to linking glutamate receptors to the erbB signaling system in astrocytes, our results show that the mGluR5/GluR2-dependenttransphosphorylation of astrocytic erbB-1 and erbB-4 receptorsinvolves stimulation of a metalloproteinase activity. Metalloproteinase-mediatedprocessing of membrane-bound erbB ligands has been shown to bea likely mechanism underlying the activation of erbB receptorsby their respective ligands between cells in contact (Dong etal., 1999; Prenzel et al., 1999). Thus our results suggest thatglutamate receptor-induced erbB transphosphorylation requiresthis proteolytic processing step, which by releasing erbB ligandsfrom their transmembrane precursors would enable them to bindto their cognate receptors. Although the specific metalloproteinaseinvolved in this transactivational process in astrocytes remainsto be identified, TACE (ADAM-17) and meltrin $beta$ (ADAM-19), twomembers of the ADAM family of metalloproteinases, appear as alikely candidates to mediate the release of mature TGF $alpha$ and NRG $beta$ from their respective membrane precursors. Although TACE/ADAM-17is thought to be involved physiologically in the cleavage of theTGF $alpha$ precursor in different cell types (Peschon et al., 1998),meltrin $beta$ has been shown recently to enhance the processing ofNRG- $beta$ s preferentially (Shirakabe et al., 2001). NRG- $beta$ s stimulatePGE₂ release from hypothalamic astrocytes (Ma et al., 1999; Prevotet al., 2003). We now know that TACE is expressed in hypothalamicastrocytes, and its biological activity is enhanced by coactivationof metabotropic and AMPA receptors (A. Lomniczi, V. Prevot, A.Costa, A. Cornea, and S. R. Ojeda, unpublished observations).An interesting aspect of this process of regulated ectodomainshedding is the finding that TACE is involved not only in theextracellular processing of erbB receptor ligands but also inthe juxtamembrane cleavage of erbB-4 (Rio et al., 2002). In thiscase the activation of TACE, recently shown to be induced by NRGsthemselves (Zhou and Carpenter, 2000), results in both the releaseof the extracellular domain of erbB-4 and the transient translocationof the native receptor to a detergent-insoluble fraction, whereit appears in a hyperphosphorylated state (Zhou and Carpenter,2000).

Although the physiological importance of ligand-induced shedding of the erbB-4 ectodomain remains to be established, a recentreport has shown that the resulting membrane-associated C-terminalfragment of the receptor is cleaved subsequently by a presenilin-dependent $gamma$ -secretase, resulting in the release of the intracellular domainof erbB-4 (Lee et al., 2002). Then this domain is transferredto the cell nucleus, where it may function as a transcriptionfactor (Lee et al., 2002). It thus appears that activation ofastrocytic metalloproteinase activity, via stimulation of metabotropicand AMPA receptors, may result in the spectrum of signaling eventsknown to be associated with the stimulation of erbB receptorsby their ligands. The use of astrocytes derived from TACE-deficientmice would help to verify the validity of thisnotion.

In summary, the present results suggest that the glutamatergic neuronal system is linked functionally to astrocytic erbB signalingin the neuroendocrine brain and indicate that this might be animportant communication pathway used by glutamatergic neuronsto coordinate the activation of stimulatory neuronal and glialinputs to LHRH neurons that are required for the initiation ofmammalianpuberty.

  FOOTNOTES

Received July 1, 2002; revised Oct. 29, 2002; accepted Nov. 11, 2002.

^* B.D. and V.P. contributed equally to thisstudy.

This work was supported by National Institutes of Health (NIH) Grant HD-25123 and National Institute of Child Health and HumanDevelopment/NIH through cooperative Grant U54 HD18185-16 as partof the Specialized Cooperative Centers Program in ReproductionResearch and by Grant RR00163 for the operation of the OregonNational Primate Center. B.D. was a visiting scientist supportedby Grant TW05408 from the Fogarty International Center, NIH. H.J.was a visiting scientist supported by a grant from the EuropeanSociety for Pediatric Endocrinology. V.P. was a postdoctoral ResearchFellow supported by a grant from Institut National de la Santéet de la Recherché Médicale (Paris,France).

Correspondence should be addressed to Sergio R. Ojeda, Division of Neuroscience, Oregon National Primate Research Center/OregonHealth & Science University, 505 North West 185th Avenue, Beaverton,OR 97006. E-mail: ojedas{at}ohsu.edu.

B. Dziedzic's present address: Department of Physiology, Medical University of Lodz, 91-130 Lodz,Poland.

H. Jung's present address: Eli Lilly and Company, D-61350 Bad Homburg,Germany.

V. Prevot's present address: Institut National de la Santé et de la Recherché Médicale U422, Place de Verdum, 59045 LilleCedex,France.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Abe T, Sugihara H, Nawa H, Shigemoto R, Mizuno N, Nakanishi S (1992) Molecular characterization of a novel metabotropic glutamate receptor mGluR5 coupled to inositol phosphate/Ca²⁺ signal transduction. J Biol Chem 267:13361-13368[Abstract/Free Full Text].
Ango F, Pin JP, Tu JC, Xiao B, Worley PF, Bockaert J, Fagni L (2000) Dendritic and axonal targeting of type 5 metabotropic glutamate receptor is regulated by Homer1 proteins and neuronal excitation. J Neurosci 20:8710-8716[Abstract/Free Full Text].
Apostolakis EM, Garai J, Lohmann JE, Clark JH, O'Malley BW (2000) Epidermal growth factor activates reproductive behavior independent of ovarian steroids in female rodents. Mol Endocrinol 14:1086-1098[Abstract/Free Full Text].
Arenander AT, de Vellis J, Herschman HR (1989) Induction of c-fos and TIS genes in cultured rat astrocytes by neurotransmitters. J Neurosci Res 24:107-114[ISI][Medline].
Balázs R, Miller S, Romano C, deVries A, Chun Y, Cotman CW (1997) Metabotropic glutamate receptor mGluR5 in astrocytes: pharmacological properties and agonist regulation. J Neurochem 69:151-163[ISI][Medline].
Bezzi P, Carmignoto G, Pasti L, Vesce S, Rossi D, Rizzini BL, Pozzan T, Volterra A (1998) Prostaglandins stimulate calcium-dependent glutamate release in astrocytes. Nature 391:281-285[Medline].
Blankenfeld GV, Kettenmann H (1991) Glutamate and GABA receptors in vertebrate glial cells. Mol Neurobiol 5:31-43[ISI][Medline].
Boudin H, Doan A, Xia J, Shigemoto R, Huganir RL, Worley P, Craig AM (2000) Presynaptic clustering of mGluR7a requires the PICK1 PDZ domain binding site. Neuron 28:485-497[ISI][Medline].
Boulter J, Hollmann M, O'Shea-Greenfield A, Hartley M, Deneris E, Maron C, Heinemann S (1990) Molecular cloning and functional expression of glutamate receptor subunit genes. Science 249:1033-1037[Abstract/Free Full Text].
Bourguignon J-P, Gérard A, Alvarez Gonzalez ML, Purnelle G, Franchimont P (1995) The role of excitatory amino acids in triggering the onset of puberty. In: The neurobiology of puberty (Plant TM, Lee PA, eds), pp 129-138. Bristol, UK: Journal of Endocrinology.
Bourguignon J-P, Lebrethon MC, Gérard A, Purnelle G, Vandersmissen E, Parent AS, Yamanaka C (2000) Amino acid neurotransmission and early ontogeny of pulsatile GnRH secretion from the rat hypothalamus. In: The onset of puberty in perspective (Bourguignon J-P, Plant TM, eds), pp 119-129. Amsterdam: Elsevier.
Brakeman PR, Lanahan AA, O'Brien R, Roche K, Barnes CA, Huganir RL, Worley PF (1997) Homer: a protein that selectively binds metabotropic glutamate receptors. Nature 386:284-287[Medline].
Bruno V, Sureda FX, Storto M, Casabona G, Caruso A, Knopfel T, Kuhn R, Nicoletti F (1997) The neuroprotective activity of group II metabotropic glutamate receptors requires new protein synthesis and involves a glial-neuronal signaling. J Neurosci 17:1891-1897[Abstract/Free Full Text].
Claypool LE, Kasuya E, Saitoh Y, Marzban F, Terasawa E (2000) N-methyl D,L-aspartate induces the release of luteinizing hormone-releasing hormone in the prepubertal and pubertal female rhesus monkey as measured by in vivo push-pull perfusion in the stalk-median eminence. Endocrinology 141:219-228[Abstract/Free Full Text].
Condorelli DF, Dell'Albani P, Corsaro M, Giuffrida R, Caruso A, Trovato Salinaro A, Spinella F, Nicoletti F, Albanese V, Giuffrida Stella AM (1997) Metabotropic glutamate receptor expression in cultured rat astrocytes and human gliomas. Neurochem Res 22:1127-1133[ISI][Medline].
Dissen GA, Romero C, Hirshfield AN, Ojeda SR (2001) Nerve growth factor is required for early follicular development in the mammalian ovary. Endocrinology 142:2078-2086[Abstract/Free Full Text].
Dong H, O'Brien RJ, Fung ET, Lanahan AA, Worley PF, Huganir RL (1997) GRIP: a synaptic PDZ domain-containing protein that interacts with AMPA receptors. Nature 386:279-284[Medline].
Dong J, Opresko LK, Dempsey PJ, Lauffenburger DA, Coffey RJ, Wiley HS (1999) Metalloprotease-mediated ligand release regulates autocrine signaling through the epidermal growth factor receptor. Proc Natl Acad Sci USA 96:6235-6240[Abstract/Free Full Text].
Donoso AO, López FJ, Negro-Vilar A (1990) Glutamate receptors of the non-N-methyl-D-aspartic acid type mediate the increase in luteinizing hormone-releasing hormone release by excitatory amino acid in vitro. Endocrinology 126:414-420[Abstract].
Dunbar AJ, Goddard C (2000) Structure-function and biological role of betacellulin. Int J Biochem Cell Biol 32:805-815[ISI][Medline].
Eyigor O, Jennes L (1997) Expression of glutamate receptor subunit mRNAs in gonadotropin-releasing hormone neurons during the sexual maturation of the female rat. Neuroendocrinology 66:122-129[ISI][Medline].
Eyigor O, Jennes L (2000) Kainate receptor subunit-positive gonadotropin-releasing hormone neurons express c-Fos during the steroid-induced luteinizing hormone surge in the female rat. Endocrinology 141:779-786[Abstract/Free Full Text].
Foa L, Rajan I, Haas K, Wu GY, Brakeman P, Worley P, Cline H (2001) The scaffold protein, Homer 1b/c, regulates axon pathfinding in the central nervous system in vivo. Nat Neurosci 4:499-506[Medline].
Gallo V, Ghiani CA (2000) Glutamate receptors in glia: new cells, new inputs, and new functions. Trends Pharmacol Sci 21:252-258[Medline].
Gore AC, Wu TJ, Rosenberg JJ, Roberts JL (1996) Gonadotropin-releasing hormone and NMDA receptor gene expression and colocalization change during puberty in female rats. J Neurosci 16:5281-5289[Abstract/Free Full Text].
Grasl-Kraupp B, Schausberger E, Hufnagl K, Gerner C, Low-Baselli A, Ro