Glutamate Transporter GLT-1 Is Transiently Localized on Growing Axons of the Mouse Spinal Cord before Establishing Astrocytic Expression

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The Journal of Neuroscience, August 1, 1998, 18(15):5706-5713

Glutamate Transporter GLT-1 Is Transiently Localized on Growing Axons of the Mouse Spinal Cord before Establishing Astrocytic Expression
Keiko Yamada¹, Masahiko Watanabe¹, Takashi Shibata², Masabumi Nagashima¹, Kohichi Tanaka³, and Yoshiro Inoue¹
Departments of ¹ Anatomy and ² Urology, Hokkaido University School of Medicine, Sapporo 060-8638, Japan, and ³ Department of Degenerative Neurological Diseases, National Institute of Neuroscience, National Center of Neurology and Psychiatry, Kodaira 187-8502, Japan

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The glutamate transporter GLT-1 is expressed in astrocytes of the mature brain and spinal cord. In the present study, we examinedits expression in the developing mouse spinal cord. By in situhybridization, ³⁵S-labeled antisense oligonucleotide probes for GLT-1 mRNA consistentlylabeled the mantle zone/gray matter from embryonic day 11 throughthe adult stage. However, immunohistochemistry with a specificantibody visualized distinct regional and cellular localizationsduring the time between the fetal and postnatal stages. At fetalstages, GLT-1 immunoreactivity predominated in the marginal zone/whitematter, observed as tiny puncta in cross-sections and as thinfibers in longitudinal sections. The GLT-1-immunopositive structureswere also labeled for neuron-specific enolase, a glycolytic enzymespecific to postmitotic neurons and endocrine cells. By electronmicroscopy, GLT-1 immunoreactivity was detected in axons formingfrequent enlargements and was focally localized on a small portionof the axolemma, particularly that facing adjacent axons. At earlypostnatal stages, GLT-1 disappeared from axons in white mattertracts and, instead, appeared in astrocytic processes surroundingvarious neuronal elements in the gray matter. Therefore, beforeswitching to astrocytic expression, GLT-1 is transiently expressedin neurons and localized in differentiating axons. Together withour previous finding on the localization of glutamate transporterGLAST in radial glial fibers, GLT-1 and GLAST are thus localizedduring development on distinct directional cellular elements alongwhich young neurons elongate their axons or move their cell bodies,respectively.

Key words: glutamate transporter; GLT-1; mouse; spinal cord; growth cone; astrocyte; immunoblot; immunohistochemistry; in situ hybridization; electron microscopy; development

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Glutamate is a major neurotransmitter mediating the fast excitatory transmission at central synapses and plays critical rolesin synaptic plasticity and development (Mayer and Westbrook, 1987;Monaghan et al., 1989). The extracellular glutamate concentrationhas to be kept low enough to terminate glutamate receptor activationand to protect neurons from glutamate excitotoxicity (Herz, 1979;Choi, 1992). The low extracellular concentration is attributableto the action of high-affinity sodium-dependent glutamate transporters.Molecular cloning studies have identified several subtypes ofthe glutamate transporter with distinct structures, functions,and expressions (Kanai et al., 1997). Of these, GLT-1 and GLASTare astrocytic glutamate transporters in the adult CNS; the formeris highly expressed in the telencephalon, and the latter predominatesin the cerebellum (Kanai and Hediger, 1992; Storck et al., 1992;Tanaka, 1993; Rothstein et al., 1994; Torp et al., 1994; Lehreet al., 1995; Shibata et al., 1996). These brain regions are knownto receive massive glutamatergic inputs. Both transporters areabundantly localized on the astrocytic cell membrane, particularlythat surrounding synapses (Chaudhry et al., 1995). Inactivationof the GLT-1 gene results in a prolonged presence of glutamatein the synaptic cleft and causes neuronal degeneration in thehippocampus, whereas that of the GLAST gene increases the vulnerabilityto acute cerebellar injury (Watase et al., 1998; Tanaka et al.,1997). All of the evidence indicates important roles of astrocyticglutamate transporters in the clearance of synaptically releasedglutamate and the protection of neurons from glutamate excitotoxicity.

From early stages before synaptogenesis, GLAST and GLT-1 mRNAs are also expressed, showing different spatial distributionsfrom each other (Shibata et al., 1996; Sutherland et al., 1996).In mice, cells expressing GLAST mRNA are restricted to the ventricularzone at embryonic day 13 (E13) and then appear and spread overthe mantle zone/gray matter. Recently, we have demonstrated inthe mouse spinal cord that GLAST is expressed in the radial glia-astrocytelineage (Shibata et al., 1997); radial glia comprises a distinctcell class of neuroglia, which guides neuronal migration and transformslater into astrocytes and oligodendrocytes (Rakic, 1971; Choi,1981; Raff et al., 1983). On the other hand, GLT-1 mRNA is primarilyexpressed in the mantle zone/gray matter from early brain development.To understand the cellular and molecular system for glutamatetransporters in the developing CNS, we examined the mouse spinalcord by in situ hybridization using ³⁵S-labeled antisense oligonucleotide probes and by immunohistochemistrywith affinity-purified specific antibodies. We report here thatGLT-1 exhibits transient neuronal expression and axonal localizationbefore its astrocytic expression is established.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Antibody. To raise polyclonal antibodies in rabbits and guinea pigs, several N- and C-terminal sequences of the mouse GLT-1were chosen for the antigen. The amino acid sequences of threesynthetic peptides, which are predicted to be intracellular, wereMASTEGANNMPKQVEVRMHDSHLSSDEP, LDTIDSQHRMQEDIEMTKTQSIYDDK, andKSADCSVEEEPWKREK, which correspond to amino acid residues 1-28(termed GLT/3), 500-525 (GLT/1), and 557-572 (GLT/5) of the mouseGLT-1, respectively (Mukainaka et al., 1995). A cysteine residuewas introduced at the C or N terminus of the first two peptidesto facilitate the conjugation to keyhole limpet hemocyanin withthe 3-maleidobenzoic acid N-hydroxysuccinimide ester method, whereasthe latter was coupled to thyroglobulin with glutaraldehyde. Inaddition, amino acid residues 1-73 (GLT/9) were expressed as aglutathione S-transferase fusion protein, using the pGEX-4T-2plasmid vector (Pharmacia, Uppsala, Sweden). The fusion proteinwas purified with glutathione-Sepharose 4B, cleaved by thrombin,and purified by reverse-phase HPLC, as described previously (Watanabeet al., 1998). Antigen peptides were emulsified with Freund'scomplete adjuvant (Difco, Detroit, MI) and injected subcutaneouslyinto New Zealand white rabbits and Hartley guinea pigs at intervalsof 2-4 weeks. From antiserum sampled 2 weeks after the sixth injection,the IgG fraction was purified using protein G-Sepharose (Pharmacia).GLT-1-specific IgG was then affinity-purified using syntheticpeptides or fusion protein coupled to cyanogen bromide-activatedSepharose 4B (Pharmacia).

In the present study, we also used a guinea pig anti-GLAST polyclonal antibody, whose specificity has been reported previously(Shibata et al., 1997). Rabbit polyclonal antibody against humanneuron-specific enolase (NSE) was purchased from Dako (Carpinteria,CA), and the specificity was reported previously (Watanabe etal., 1990).

Immunoblot. Membrane extracts from the adult C57BL mouse brain were prepared as described previously (Yamada et al., 1996).Seven micrograms of protein were analyzed by 11% SDS-PAGE underreducing conditions. Proteins in the gel were electroblotted ontoa nitrocellulose membrane, incubated with 1 µg/ml affinity-purifiedantibodies in PBS containing 0.1% Tween 20, and visualized withthe ECL detection system (Amersham, Arlington Heights, IL).

In situ hybridization. Under deep pentobarbital anesthesia, the lumbar cord was freshly sampled from C57BL mice at E11, E13,E15, E18, postnatal day 1 (P1), P7, P14, P21, and 4 months (adult)and frozen in powdered dry ice. The next day of overnight matingwas counted as E0. Fresh frozen sections were prepared by cryostat(20 µm thick) and processed for in situ hybridization. The sequenceof two nonoverlapping antisense oligonucleotide probes and theprocedures for in situ hybridization were the same as reportedpreviously (Shibata et al., 1996). Briefly, hybridization wasperformed overnight with 10,000 dpm/µl ³⁵S-labeled probes at 42°C in the presence of 50% formamide, followedby washing in 0.1× SSC containing 0.1% sarcosyl at 55°C. Sectionswere exposed to nuclear track emulsion (NTB-2; Kodak, Rochester,NY) for 2 months.

Immunohistochemistry. For immunohistochemistry, fetuses at E11, E13, E15, and E18 were fixed at 4°C by overnight immersionin Bouin's fixative for paraffin sections or in 4% paraformaldehydein 0.1 M sodium phosphate buffer (PB), pH 7.2, for cryostat sections,whereas mice at P1, P7, P14, P21, and adult (4 months old) wereall perfused transcardially with the latter fixative under deeppentobarbital anesthesia. As a specificity control, GLT-1( $-$ / $-$ )mice at E13 and the adult stage (Tanaka et al., 1997) were similarlyfixed as above. Paraffin (5 µm) and cryostat sections (20 µm)were prepared and incubated overnight with GLT-1 antibodies (0.1-0.3µg/ml) at room temperature. Sections were then incubated withbiotinylated goat anti-rabbit IgG for 1 hr and streptavidin for30 min, using a Histofine SAB-PO(R) kit (Nichirei Corp., Tokyo,Japan). Immunoreaction was visualized with 3,3'-diaminobenzidine.For immunoelectron microscopy, immunostained sections were furthertreated with osmium tetroxide and uranyl acetate, dehydrated,and embedded in Epon 812.

For double labeling for GLT-1 and GLAST, paraffin sections were first processed for rabbit anti-GLT-1 antibody (0.3 µg/ml)and Histofine SAB-PO(R) kit, followed by visualization with theTyramide signal amplification kit [TSA-DIRECT (Green); NEN LifeScience, Boston, MA]. The second immunoreaction was done withguinea pig anti-GLAST antibody (2.5 µg/ml) and phosphatase-linkedanti-guinea pig IgG (Kirkegaard & Perry, Gaithersburg, MD) andvisualized with the HNPP fluorescent detection set (BoehringerMannheim, Mannheim, Germany). For double labeling for GLT-1 andNSE, cryostat sections were first incubated with guinea pig anti-GLT-1antibody (1.0 µg/ml), biotinylated goat anti-guinea pig IgG (1:200)(Vector Laboratories, Burlingame, CA), and streptavidin-peroxidase,followed by visualization with TSA-DIRECT (Red). The second immunoreactionwas done with rabbit anti-NSE antibody (1:3000) and FITC-labeleddonkey anti-rabbit IgG (1:100) (Jackson ImmunoResearch, West Grove,PA). Sections were photographed by a confocal laser scanning microscope(MRC 1024; Bio-Rad, Hercules, CA).

Electron microscopy. Mice at E13 were immersed overnight in 4% paraformaldehyde in 0.1 M PB, pH 7.2, and post-fixed for 2hr with 1% osmium tetroxide in 0.1 M PB. After block stainingin 1% aqueous uranyl acetate solution and dehydration, tissuespecimens were embedded in Epon 812. Silver-gold ultrathin sectionswere prepared on an Ultracut ultramicrotome (Leica, Nussloch,Germany) and stained with 1% uranyl acetate for 5 min and a mixedlead solution for 2 min. Electron micrographs were taken on anH7100 electron microscope (Hitachi, Tokyo, Japan).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In situ hybridization

By in situ hybridization with ³⁵S-labeled antisense oligonucleotide probes, developmental changes of GLT-1 mRNA expression wereexamined in cross-sections of the mouse lumbar cord from E11 tothe adult stage (Fig. 1). At E11, low levels of GLT-1 mRNA weredetected in a thin outer layer (the mantle zone), whereas no significantsignals were found in the large central region (the ventricularzone) (Fig. 1A). In good accordance with the marked expansionof the mantle zone with concomitant reduction of the ventricularzone and central canal, GLT-1 mRNA became detectable in most regionsof the spinal cord by E15 (Fig. 1B,C). In postnatal development,levels of GLT-1 mRNA exhibited a prominent increase in the graymatter, peaking at P14 (Fig. 1D-F). Weaker signals were also detectedin the white matter at P14 and thereafter. Almost identical resultswere obtained with another nonoverlapping antisense probe (datanot shown).

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Figure 1. Developmental changes of GLT-1 mRNA expression in the mouse spinal cord. A, E11; B, E13; C, E15; D, P1; E, P14; F, P120. Dark-field micrographs were taken and printed at the same magnification. DH, Dorsal horn; VH, ventral horn; VZ, ventricular zone. Scale bar, 100 µm.

Antibody preparation

Using N- and C-terminal peptides as antigens, four polyclonal antibodies against the mouse GLT-1 were obtained in rabbitsand guinea pigs. By immunoblot analysis, all of these antibodiesrecognized a 60-70 kDa band in the brain of the adult wild-typemouse (Fig. 2A). With C-terminal antibodies, the band was diminishedin intensity in the GLT-1(+/ $-$ ) mouse brain and disappeared inthe GLT-1( $-$ / $-$ ) mouse brain. Immunohistochemistry with microslicersections showed that each antibody widely stained the adult brainand showed the highest levels in the telencephalon, includingthe cerebral cortex, hippocampus, caudate-putamen, and olfactorytubercle (Fig. 2B). The distribution of GLT-1 protein was similarto that of GLT-1 mRNA (Fig. 2C). In the adult spinal cord, eachantibody stained neuropil regions of the gray matter, higher inthe dorsal horn than in the ventral horn (Fig. 2D). The resultsfrom immunoblotting and immunohistochemistry are consistent withprevious reports (Rothstein et al., 1994; Lehre et al., 1995).Of the four antibodies, the strongest immunohistochemical signalwas given by C-terminal antibodies: rabbit antibody against aminoacid residues 557-572 and guinea pig antibody against amino acidresidues 500-525. All immunohistochemical data presented herewere obtained with the two antibodies.

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Figure 2. Characterization of GLT-1 antibody. A, Immunoblot analysis using brain extracts from the adult wild-type (a), GLT-1(+/ $-$ ) (b), and GLT-1( $-$ / $-$ ) (c) mice. The size of protein markers is 205, 116, 80, and 49.5 kDa from the above. B, Immunohistochemistry for GLT-1 in the adult mouse brain. C, In situ hybridization for GLT-1 mRNA in the adult mouse brain. D, Immunohistochemistry for GLT-1 in the adult mouse spinal cord. Cb, Cerebellum; CP, caudate-putamen; Cx, cerebral cortex; DH, dorsal horn; Di, diencephalon; Hi, hippocampus; Mb, midbrain; MO, medulla oblongata; Po, pons; Tu, olfactory tubercle; VH, ventral horn. Scale bars: B, C, 2 mm; D, 100 µm.

Preabsorption of antibodies (for example, addition of 7.5 µg/ml antigen peptide at adult and 0.075 µg/ml at E13 to rabbitantibody against amino acid residues 557-572) completely abolishedthe characteristic staining in the spinal cord (data not shown).Under the same conditions, C-terminal antibodies yielded no significantimmunohistochemical signals in the adult spinal cord of the GLT-1( $-$ / $-$ )mouse (data not shown). Therefore, immunohistochemical signalsby the present antibodies were judged to be specific to GLT-1.

Immunohistochemistry

Developmental changes at the protein level were followed by light-microscopic immunoperoxidase (Fig. 3, see Fig. 6A-E,G),immunofluorescence (Fig. 4), and immunoelectron microscopy (Figs.5B, 6F). At E11 when the mouse spinal cord consists of a largeventricular zone, a small oval bulging of the ventral horn, anda thin peripheral layer of the marginal zone (Shibata et al.,1997), very weak immunoreactivity was found in the marginal zone/whitematter layer (data not shown).

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Figure 3. Histology and immunohistochemistry for GLT-1 in the mouse spinal cord at E13. A-C, Low-power micrographs of paraffin cross-sections stained with hematoxylin (A) and by rabbit anti-GLT-1 antibody (B and C). Immunostainings in the marginal zone/white matter (arrowheads) and in the dorsal horn (DH) are seen in the wild-type mouse (B), but not in the GLT-1( $-$ / $-$ ) mouse (C). D, High-power view of the ventral cord. GLT-1 is detected as tiny puncta in the marginal zone/white matter (WM). E, F, Longitudinal cryostat sections stained by rabbit anti-GLT-1 antibody. GLT-1 is detected as longitudinal fibers running in the marginal zone/white matter (WM or arrowheads), from which transverse fibers with lower immunoreactivity enter the ventral horn (VH). FP, Floor plate; P, pia mater; RP, roof plate. Asterisks indicate ventricular zone. Scale bars: A-C, 100 µm; D, 10 µm; E, F, 100 µm.

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Figure 4. Images by confocal laser scanning microscopy. A, B, Double immunofluorescence for GLT-1 (green, rabbit antibody) and GLAST (red, guinea pig) in a paraffin cross-section at E13. GLT-1 immunoreactivity is seen in the marginal zone/white matter (WM) of the ventral cord and in the dorsal horn (DH), showing no overlaps with GLAST. A few transverse fibers (arrows) with GLT-1 immunoreactivity enter the ventral horn (VH). C, D, Double immunofluorescence for GLT-1 (red, guinea pig) and NSE (green, rabbit) in a cryostat cross-section at E13. Note their colocalization in the marginal zone/white matter (WM), but not in the ventral horn (VH). E, Double immunofluorescence for GLT-1 (green, rabbit) and GLAST (red, guinea pig) in a cross paraffin section at P14. c, Cell bodies; FP, floor plate; P, pia matter; RP, roof plate. Asterisks indicate the ventricular zone. Scale bars: A, C, 50 µm; B, D, E, 10 µm.

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Figure 5. Electron micrographs of the spinal marginal zone at E13. A, Ultrastructure. Enlarged axonal portions are marked by asterisks. Arrowheads indicate growth cone parcels, which have been originally described for structures contained in growing pyramidal tract axons of neonatal rats (Gorgels, 1991a). B, Immunoelectron micrograph showing GLT-1. GLT-1 is detected in a small part of the axolemma apposing adjacent axons and sometimes to radial glial fibers (arrowheads). EF, End foot; RG, radial glial fiber. Scale bars, 1 µm.

At E13, GLT-1 immunoreactivity in the marginal zone was increased and distributed in the ventral and lateral funiculi (Fig.3A,B). The mantle zone, on the other hand, was associated withlittle immunoreactivity, except for labelings scattered in thedorsal horn. No immunoreactivity was detected in the spinal cordof the GLT-1( $-$ / $-$ ) mouse (Fig. 3C). At higher magnification, GLT-1immunoreactivity in the marginal zone was observed as numeroustiny puncta in cross-sections (Fig. 3D) and as fibrous structuresrunning rostrocaudally in longitudinal sections (Fig. 3E,F). Byconfocal laser scanning microcopy with a high-sensitive fluorescencesignal amplification system, the distribution of GLT-1 immunoreactivitywas visualized more clearly (Fig. 4A,B, green). Within the marginalzone, labeled structures were more numerous and intense in deeperregions than in superficial regions just beneath the pial surface(Fig. 4B). In the mantle zone, there were some transverse fibersthat ran toward the marginal zone and showed low GLT-1 immunoreactivity(Fig. 4B, arrows). When compared with glutamate transporter GLASTexpressed in radial glial cells (Fig. 4A,B, red), both showedno overlaps; GLT-1-immunopositive puncta were all immunonegativefor GLAST, and GLAST-immunopositive radial fibers running in themantle and marginal zones were all immunonegative for GLT-1. Bydouble immunofluorescence for NSE, a soluble glycolytic enzymespecific to postmitotic neurons and endocrine cells (Calker etal., 1978; Watanabe et al., 1993), immunoreactivities for GLT-1(Fig. 4C, red) and NSE (Fig. 4C, green) were both detected inthe marginal zone and dorsal horn, yielding a fused yellow toorange color. At higher magnification, GLT-1 was overlapped withNSE but was more concentrated as tiny spots within larger NSE-immunoreactivestructures (Fig. 4D). In the mantle zone, NSE was detected diffuselyin neuronal perikarya as well, in which GLT-1 was sparsely distributed(Fig. 4C).

To clarify structural components in the marginal zone at E13, the lateral funiculus was examined by electron microscopy (Fig.5A). In cross-sections, the marginal zone was occupied exclusivelyby round to irregular profiles variable in size, ranging from0.04 to 2 µm. They contained various organelles, including smoothendoplasmic reticulum, clusters of vacuoles and vesicles, microtubules,intermediate filaments, and mitochondria. In general, larger profileswere irregular in shape and characterized by the cytoplasm witha fine filamentous meshwork and often had round structures limitedby two concentric membranes (Fig. 5A, arrowheads), which havebeen referred to as "growth cone parcels" by Gorgels (1991a).On the other hand, smaller profiles were round to oval in shapeand were relatively abundant in microtubules and intermediatefilaments. In longitudinal sections, most, if not all, of theprofiles in cross-sections turned out to be segments through axonsforming frequent enlargements (data not shown). Axons were closelyapposed to each other, having no junction-like specializationsbetween them. Moreover, the cell membrane of axon profiles camein close contact with that of radial glial fibers (data not shown).By preembedding immunoelectron microscopy, GLT-1 was detectedin some of the axon profiles (Fig. 5B). Within the labeled axons,immunoreaction products were not distributed evenly but were preferentiallyconcentrated in only a small part of the axolemma. These immunoreactivepatches were observed in axolemmal portions apposing adjacentaxons and sometimes to shafts of radial glial fibers, but notto their end feet. No particular accumulations of organelles,such as vesicles, were observed beneath the labeled axolemma.

In cross-sections from E15 to P1, punctate labelings in the marginal zone/white matter were found in the ventral, lateral,and dorsal funiculi, particularly intensely in the lateral funiculusadjacent to the dorsal horn (Fig. 6A,B), but they disappearedfrom any regions of the white matter at P7 and thereafter (Fig.6C,E,G). Instead, weak immunoreactivity emerged in the mantlezone/gray matter at P1 (Fig. 6B), and the immunoreactivity showeda remarkable increase during the early postnatal period, peakingat P21 (Fig. 6C,G). In the spinal cord at P14, GLT-1 showed denselocalization in neuropil regions, which surrounded immunonegativeneuronal cell bodies and stem dendrites, and were also detectedin fibrous structures traversing the white matter toward the pialsurface (Fig. 6C,E). This pattern of immunostaining was very similarto that for GLAST (Fig. 6D). By double immunofluorescence, GLT-1(Fig. 4E, green) was colocalized almost completely with GLAST(Fig. 4E, red) in reticular structures in the neuropil, yieldinga fused yellow color. Furthermore, immunoelectron microscopy showedthe presence of GLT-1 immunoreactivity in astrocytic processes,which entered elaborately between various neuronal elements tosurround them (Fig. 6F).

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Figure 6. Spinal cords from E15 to P21. Cross paraffin sections were immunostained for GLT-1 (rabbit antibody) at E15 (A), P1 (B), P14 (C), and P21 (G), and for GLAST at P14 (rabbit antibody) (D). Arrowheads indicate GLT-1 immunoreactivity in the marginal zone/white matter. E, High-power view of the ventral cord in C. F, Immunoelectron micrograph at P14 showing the localization of GLT-1 in astrocytic processes (As) surrounding immunonegative nerve terminals (NT), dendritic spines (DS), and dendrites (Dn). DH, Dorsal horn; n, neuronal cell bodies; VH, ventral horn; WM, white matter. Scale bars: A-D, G, 100 µm; E, 10 µm; F, 1 µm.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In the present study, we have examined the expression of GLT-1 in the developing mouse spinal cord and disclosed distinctcellular and subcellular localizations in the period between fetaland postnatal stages.

During the fetal stages, we found contrasting distributions of GLT-1 mRNA and protein. The former was detected in the mantlezone/gray matter, whereas the latter was mainly in the marginalzone/white matter. From the unexpected distributions, we carefullyevaluated the authenticity of histochemical signals by confirmingidentical hybridization patterns with two antisense oligonucleotideprobes and identical immunohistochemical patterns with four polyclonalantibodies. Recently, GLT-1 has also been reported to be presentin white matter tracts of the developing rat CNS (Furuta et al.,1997).

Transient neuronal expression of GLT-1

In mice, motoneurons in the spinal ventral horn are generated at E9-E10.5, and dorsal horn neurons are generated at approximatelyE12 (Sims and Vaughn, 1979). Reflecting the active neurogenesisand successive migration, cell number in the mantle zone displaysa remarkable increase between E11 and E13 (Shibata et al., 1997).At this period, GLT-1 and GLAST mRNAs show distinct distributions:the former in the mantle zone and the latter in the ventricularzone (compare Fig. 1A,B in the present study with Fig. 2A,B byShibata et al., 1997). Using a specific antibody, we have shownpreviously that cells expressing GLAST at E11-E13 display morphologicalfeatures characteristic of the radial glia, i.e., localizationof cell bodies in the ventricular zone and radial fibers spanningthe neural wall (Shibata et al., 1997). At E15, the cells beginto migrate to the mantle zone and to transform into astrocytes.Precursors of oligodendrocytes, which also exhibit the morphologyof radial glia cells (Ono et al., 1997), are localized in theventrobasal region of the rat spinal ventricular zone at E13 andE14 (Pringle and Richardson, 1993; Timsit et al., 1995). Therefore,the distribution of GLT-1 mRNA in the mantle zone at E11-E13 suggestsits expression in a distinct cell population other than radialglial cells, most likely young neurons. Such a wide distributionof GLT-1 mRNA over the mantle zone has also been shown in thefetal mouse brain (Shibata et al., 1996; Sutherland et al., 1996).

GLT-1 is localized at nonsynaptic sites of growing axons

The marginal zone of the ventral cord at E13 was occupied exclusively by axons descending or ascending the cord. Comparedwith mature stages, these axons are characterized by extensiveformation of enlargements, richness of organelles, and absenceof glial ensheathment (except small contacts with radial glialfibers). These morphological features are common in many respectsto axons in the rat corticospinal tract at approximately birth(De Kort et al., 1985; Gorgels, 1991a). GLT-1 was detected mainlyin longitudinal fibers in the marginal zone at E13, when theywere also immunopositive for NSE, a neuronal marker protein (Calkeret al., 1978; Watanabe et al., 1993). In the mantle zone, on theother hand, GLT-1 was scarcely found except for a few transversefibers running toward the marginal zone, whereas NSE was detectedin neuronal cell bodies as well. These immunohistochemical results,together with the distribution of GLT-1 mRNA in the mantle zone,suggest that the GLT-1 protein synthesized in neuronal cell bodiesis transported preferentially to growing axons. The axonal localizationof GLT-1 was confirmed by immunoelectron microscopy. In cross-sectionsthrough the white matter at P7, punctate labelings representingaxonal localization disappeared. Therefore, GLT-1 is transientlyexpressed on immature axons growing out in white matter tracts.

GLT-1 exhibits a patch-like localization on the axolemma apposing other cellular elements. They are mostly neighboring axonsand sometimes shafts of radial glial fibers. With such neuronaland glial elements, growing axons are known to form transientcontacts having synapse-like junctional specializations (Henriksonand Vaughn, 1974; Vaughn et al., 1974, 1976; De Kort et al., 1985;Gorgels, 1991a,b). The specializations include a few clear vesiclesin presynaptic axons, dense materials associated with presynapticand postsynaptic membranes, and intercellular matrix in the synapticcleft. In the spinal marginal zone of mice, the axoglial synapsesare found at E13 and E14, but disappear thereafter (Henriksonand Vaughn, 1974). We also observed by electron microscopy someaxoglial contacts with junction-like specialization at E13 (ourunpublished observations), but they were much less frequent thanGLT-1-immunopositive patches on the axolemma. Moreover, clearvesicles were not found in the vicinity of immunopositive patches.Therefore, it is safe to conclude that GLT-1 is localized primarilyin nonspecialized axolemma apposing neighboring structures. However,the present immunoelectron microscopy with use of diffusible peroxidasesubstrate cannot exclude the possibility that some immunoreactionproducts, if not all, result from the diffusion from the originalimmunoreaction sites. In future studies, precise localizationon growing axons needs to be determined by immunogold cytochemistry.

Speculated role in glutamatergic signaling between growing axons

Neuronal growth cones are highly motile enlargements and are thought to navigate a precise route through the developing nervoussystem and to recognize an appropriate synaptic partner. It isknown that various neurotransmitters, including glutamate, haveeffects on growth cone movement (Mattson, 1988). Although theprecise localization of glutamate receptors remains unknown atstages much earlier than synaptogenesis, transcripts of the receptorchannel subunits are expressed (Monyer et al., 1991; Watanabeet al., 1992), and glutamate receptors are functionally activefrom early fetal stages (LoTurco et al., 1991). Recently, Owenand Bird (1997) have reported that the application of glutamateinhibits growth and motility of axons in cultured mouse spinalcord neurons, and the inhibitory actions are blocked by antagonistto the non-NMDA receptor, but not to the NMDA receptor. Zhenget al. (1996) have shown that growth cones of cultured Xenopusspinal cord neurons exhibit chemotropic turning responses forglutamate, and the response depends on the activation of the NMDAreceptor. Glutamate transporters can either take in extracellularglutamate or release intracellular glutamate to the extracellularspace, according to the electrochemical gradient across the cellmembrane (Nicolls and Attwell, 1990). From the transient axonallocalization at stages when growth cone-like axonal enlargementsare actively formed, it is speculated that GLT-1 on growing axonssubserves as a source of glutamate or its gradient to regulatethe activation of glutamate receptors. Such a role of a transporteras the source of transmitters has been reported for GABA transporterson growth cones (Taylor and Gordon-Weeks, 1991) and has also beenproposed for glutamate transporters on developing optic nerveaxons (Chiu and Kriegler, 1994).

Homozygous mice defective in the GLT-1 gene are born at the frequency predicted by Mendelian ratios but suffer from spontaneousseizures leading to sudden death (Tanaka et al., 1997). In addition,these mice exhibit an abnormal posture, characterized by claspingthe hindlimbs tightly, when the animals were lifted by the tail(our unpublished observations). Detailed neuroanatomical analysesshould be challenged in future studies regarding development ofwhite matter tracts, such as the corticospinal (pyramidal) tract.

Switch to astrocytic expression at synaptogenic phase

GLT-1 appeared in the gray matter at birth, and the intensity displayed a remarkable elevation during the early postnatalperiod. At P14, GLT-1 was densely distributed in the neuropil,observed as reticular stainings surrounding neuronal cell bodiesand stem dendrites. Immunoelectron microscopy has demonstratedits localization in astrocytic processes surrounding synapses.Thus, it is evident that, although GLT-1 mRNA is continuouslyexpressed in the mantle zone/gray matter, cells expressing thetranscripts switch from neurons to astrocytes. As a result, GLT-1becomes colocalized well with GLAST in astrocytic processes atP14. Compared with GLAST (Shibata et al., 1997), the appearanceof reticular neuropilar staining is considerably late for GLT-1.Simultaneous with the onset of radial glial migration, the transformationinto astrocytes begins at E15, when tiny membranous protrusionshaving GLAST immunoreactivity appear around radial fibers (Shibataet al., 1997). During the late fetal and early postnatal periods,the tiny protrusions progressively increase with concomitant reductionand disappearance of radial fiber staining. Therefore, GLT-1 becomesrecruited on preexisting astrocytic processes during the earlypostnatal period. The relatively late appearance of GLT-1 in astrocyteshas also been reported in the rat brain (Ullensvang et al., 1997).In the adult, levels of GLT-1 and GLAST are differentially downregulatedin astrocytes of different neural regions, thus establishing theirdistinct spatial distributions in the mature CNS (Rothstein etal., 1994; Torp et al., 1994; Lehre et al., 1995; Shibata et al.,1996). From these results, dense colocalization of GLT-1 and GLASTat early postnatal stages may suggest increasing demands for astrocyticglutamate transporters at synaptogenic stages.

In conclusion, it is now clear that GLT-1 and GLAST are localized first on growing axons and radial glial fibers, respectively,and later on astrocytic processes. Considering that the activationof glutamate receptors affects radial glia-guided neuronal migration(Rakic, 1971; Komuro and Rakic, 1993) and growth cone movement,it is interesting to think that the two glutamate transportersmight play cooperative and complementary roles in neural development,as they do in rapid clearance of synaptically released glutamateto protect mature neurons from excitotoxicity.

  FOOTNOTES

Received March 13, 1998; revised May 11, 1998; accepted May 13, 1998.

This investigation was supported by research grants to M.W. from the Ministry of Education, Science, Sports, and Culture,the Ministry of Health and Welfare, the Science and TechnologyAgency (Strategic Promotion System for Brain Science), Naito Foundation,Suhara Foundation, and Kanahara Foundation and to K.Y. from theResearch Fellowships of the Japan Society for the Promotion ofScience for Young Scientists.
Correspondence should be addressed to Masahiko Watanabe, Department of Anatomy, Hokkaido University School of Medicine, Sapporo060, Japan.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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