Expression of Neural RNA-Binding Proteins in the Postnatal CNS: Implications of Their Roles in Neuronal and Glial Cell Development

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Volume 17, Number 21, Issue of November 1, 1997 pp. 8300-8312
Copyright ©1997 Society for Neuroscience

Expression of Neural RNA-Binding Proteins in the Postnatal CNS: Implications of Their Roles in Neuronal and Glial Cell Development

Shin-ichi Sakakibara¹ and Hideyuki Okano¹^,²
¹ Department of Neuroanatomy, Biomedical Research Center, Osaka University Medical School, Suita, Osaka 565, Japan, and ² Core Research for Evolutional Science and Technology (CREST), Japan Science and Technology Corporation, Shinagawa, Tokyo 140, Japan

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

There is an increasing interest in the role of RNA-binding proteins during neural development. Mouse-Musashi-1 (m-Msi-1) isa mouse neural RNA-binding protein with sequence similarity toDrosophila musashi (d-msi), which is essential for neural development.m-Msi-1 is highly enriched in neural precursor cells that arecapable of generating both neurons and glia during embryonic CNSdevelopment. The present study characterized m-Msi-1-expressingcells in the postnatal and adult CNS. Postnatally, m-Msi-1 wasexpressed in proliferative neuronal precursors in the externalgranule cell layer of the cerebellum and in the anterior cornerof the subventricular zone of the lateral ventricles. In gliogenesis,the persistent expression of m-Msi-1 was observed in cells ofthe astrocyte lineage ranging from proliferative glial precursorsin the subventricular zone (SVZ) to differentiated astrocytesin the parenchyma. In addition, we showed that m-Msi-1 was stillexpressed in proliferating cells in the adult SVZ, which may containneural precursor or stem cells. Another neural RNA-binding proteinHu (the mammalian homolog of a Drosophila neuronal RNA-bindingprotein Elav) was present in postmitotic neurons throughout thedevelopment of the CNS, and its pattern of expression was comparedwith that of m-Msi-1. These observations imply that these twoRNA-binding proteins may be involved in the development of neuronsand glia by regulating gene expression at the post-transcriptionallevel.
Key words: RNA-binding proteins; postnatal CNS; mouse-Musashi-1 (m-Msi-1); Hu; Drosophila musashi; neuronal and glial precursor cells; astrocyte lineage

INTRODUCTION

A number of transcription factors that function in the proliferation and differentiation of neural precursor cells have beenidentified. However, the recent discovery of neural-specific RNA-bindingproteins raises the possibility that the development of neuralcells from the precursors may also be regulated at the post-transcriptionallevel. We believe that at least two gene families are representedby the neural RNA-binding proteins found in both invertebratesand vertebrates (Okano, 1995; Sakakibara et al., 1996). One, theElav family, includes Drosophila elav genes (Yao et al., 1993)and their mammalian homologs, the Hu genes (Szabo et al., 1991).Members of this family share extensive sequence similarity withone another, and they seem to be expressed mainly in postmitoticneurons (Okano and Darnell, 1997). The other Msi family is composedof Drosophila musashi (Nakamura et al., 1994), Xenopus laevisnrp-1 (Richter et al., 1990), and their mouse homolog mouse-musashi-1(m-msi-1) (Sakakibara et al., 1996). d-Msi is required for thetwo successive asymmetric cell divisions of sensory organ precursors(Nakamura et al., 1994). In contrast to the Elav family, the membersof the Msi family are expressed in the neural precursor cellsat least during embryonic CNS development (Sakakibara et al.,1996). Although the molecular functions and the in vivo RNA targetsof Msi and Elav families remain largely unknown, these differentexpression patterns suggest that the Msi and Elav families mayplay distinct roles in the development and maintenance of neuralcells.

During CNS development, neurons and glial cells are thought to be generated from common neural precursor cells (multipotentCNS stem cells) (Davis and Temple, 1994). Our previous study hassuggested that m-Msi-1 is expressed predominantly in proliferatingmultipotent neural precursor cells that may give rise to neuronsand/or glia, but is not expressed in newly generated postmitoticneurons (Sakakibara et al., 1996). The expression of m-Msi-1 islargely downregulated with the successive progression of neurogenesis.However, a considerable amount of m-Msi-1 transcripts is presentin the brain during postnatal development, and low level expressionpersists into adulthood (Sakakibara et al., 1996). Recent studieshave indicated the presence of neural precursor cells in postnatalneural development. To further study the role of m-Msi-1 in neuralprecursor cells in the postnatal and adult CNS, the spatiotemporaldistribution of m-Msi-1-expressing cells was examined. The m-Msi-1protein can be detected in proliferating neuronal and/or glialprecursor cells in the SVZ and in cells of the astrocyte lineagein the postnatal and adult CNS. These observations suggest alsothat m-Msi-1 may be an excellent marker for protoplasmic astrocytes.

MATERIALS AND METHODS
Animals and tissue preparation. ICR mice and Wistar rats used throughout the experiments were purchased from Charles RiverJapan Inc. The day of birth was designated as postnatal day (P)0. Pups and adults (anesthetized by ether inhalation) were perfusedthrough the left ventricle with 4% paraformaldehyde in 0.1 M PBS,pH 7.4, and then the brains were dissected and post-fixed overnightat 4°C in the same fixative. For paraffin sectioning, tissue blockswere rinsed twice with PBS for 30 min each time and dehydratedthrough a series of increasing concentrations of ethanol. Afterdehydration, they were cleared with chloroform and xylene andthen embedded in paraffin (Tissue Prep, Fisher, Pittsburgh, PA)at 62°C. Sections (4 µm) were cut on a microtome and mounted ongelatin/chrome-coated slides. Paraffin sections were used forhematoxylin-eosin and immunohistochemical staining with a singleprimary antibody. For cryosectioning, sample blocks rinsed withPBS were cryoprotected in 30% sucrose in PBS overnight at 4°C,embedded in O.C.T. compound (Tissue Tek, Miles, Elkhart, IN),and frozen on dry ice. Cryostat sections (12 µm) were cut andaffixed to glass slides precoated with gelatin/chrome. These sectionswere used for double-immunostaining.

Immunohistochemical analysis. The following primary antibodies were used: m-Msi-1 (affinity-purified rabbit polyclonal antibody,used at 1:500 dilution) (Sakakibara et al., 1996); Hu proteins(mouse monoclonal IgG2B, clone 16A11, which binds to Hu proteinsincluding HuD, HuC, and HelN-1, supplied by Dr. M. F. Marusich,University of Oregon; used at 1:500 dilution) (Marusich et al.,1994); nestin (mouse monoclonal IgG, clone RE6-96 supplied byDr. M. Ogawa, Kochi Medical School, Japan); ascitic fluid usedat 1:1000 dilution (Miyata and Ogawa, 1994); proliferating cellnuclear antigen (PCNA) (mouse monoclonal IgG1, used at 1:200 dilution;Novocastra Laboratories); glial fibrillary acidic protein (GFAP)(mouse monoclonal IgG1, clone G-A-5, used at 1:400 dilution) (Sigma,St. Louis, MO); 2 $'$ , 3 $'$ -cyclic nucleotide-3 $'$ -phosphohydrolase (CNPase)(mouse monoclonal IgG1, clone 11-5B, used at 1:100 dilution) (Sigma);bromodeoxyuridine (BrdU) (mouse monoclonal IgG1, clone BU-33,used at 1:5000 dilution) (Sigma); MacI (mouse monoclonal IgG1,used at 1:100 dilution) (Boehringer Mannheim, Indianapolis, IN),platelet-derived growth factor $alpha$ -receptor (PDGF $alpha$ -R) (rat monoclonalIgG, a kind gift from Dr. S.-I. Nishikawa, Kyoto University, Japan;used at 1:5000 dilution) (Takakura et al., 1996), and NG2 (mousemonoclonal IgG1, a kind gift from Dr. W. D. Richardson, UniversityCollege London, UK; used at 1:100 dilution) (Stallcup and Beasley,1987). Secondary and tertiary reagents were obtained commerciallyfrom Vector Laboratories (Burlingame, CA) or Jackson ImmunoResearch(West Grove, PA). The specificity of the polyclonal antibody tom-Msi-1 was confirmed by the immunoblot analysis of the m-msi-1knock-out mice (our unpublished results). Immunolabeling witha single primary antibody was performed with an avidin-biotin-peroxidasetechnique. Briefly, dewaxed and rehydrated serial paraffin sectionswere quenched for endogenous peroxidase activity by treating with0.3% hydrogen peroxide in methanol for 30 min at room temperature,blocked for 1 hr in 10% normal goat serum and 0.1% Triton X-100in PBS, and then incubated with a primary antibody diluted inthe same blocking solution overnight at 4°C. Sections were placedin an appropriate biotinylated secondary antibody diluted withthe blocking solution (biotinylated goat anti-mouse, rat, or rabbitIgG; Jackson) at 1:750 for 1 hr, followed by incubation with avidin-conjugatedhorseradish peroxidase (HRP at 1:1000) (Vector), and HRP was visualizedusing 0.5 mg/ml of diaminobenzidine (DAB) and 0.03% H₂O₂. Eachstep was followed by four washes in PBS. Double indirect immunostainingwas performed on the frozen sections; the cells were permeabilizedin 0.1% Triton X-100 in PBS for 30 min and blocked as above. Polyclonalantibody to m-Msi-1 was used in combination with antibodies againstHu, GFAP, CNPase, BrdU, MacI, PDGF $alpha$ -R, NG2, or nestin. After fourwashes with PBS, bound antibodies were visualized by incubationwith fluorochrome-conjugated secondary antibodies: Cy-3-, or fluorescein-isothiocyanate(FITC)-labeled goat anti-mouse IgG, FITC-labeled goat anti-rabbitIgG, and Texas Red-labeled goat anti-rat IgG (used at 1:200 dilutionwith 0.1% Triton X-100 in PBS; Jackson). After another four washes,the sections were mounted and examined with a Leitz DMRD microscopeequipped with L4, ND, N2.1, and TX (Leica Inc., Buffalo, NY) epifluorescentfilters. Laser scanning confocal microscopy was performed witha Zeiss LSM410 cofocal imaging system.

BrdU incorporation in vivo. To label the dividing cells in the postnatal SVZ, P7 mice were given two intraperitoneal injections,1.5 hr apart, of 100 mg/kg of body weight of BrdU (Sigma) dissolvedin PBS, and then were killed by perfusion 1.5 hr after the secondinjection. In adult animals (3 months old), to label the entirepopulation of proliferating subependymal cells, which have a cellcycle time of ~12.7 hr in mouse (Morshead and van der Kooy, 1992),BrdU (75 mg/kg of body weight) was injected intraperitoneallyevery 2 hr for 12 hr, and the animals were killed by perfusion0.5 hr after the last injection. The BrdU-injected brains wereremoved and post-fixed overnight at 4°C, and serial frozen sectionswere prepared in the coronal plane as described above. For immunostainingwith anti-BrdU antibody, sections were incubated in 1 N HCl for30 min at 60°C to denature the DNA, followed by 0.1 M sodium borate,pH 8.5, for 10 min. After three washes with PBS, indirect double-immunolabelingfor BrdU and m-Msi-1 was performed as described above.

Surgical procedures for brain lesions. Adult ICR mice, 3 months old, were anesthetized with Nembutal injections (10 mg/kg)(Abbott Laboratories, North Chicago, IL), and a midline skin incisionwas made. A unilateral linear craniectomy was performed on theskull by using a drill 3 mm left of the midline. The wound wasmade in the left cerebral hemisphere; a 27 gauge stainless steelneedle was placed 3 mm lateral to the sagittal fissure and 2 mmanterior to the lambda line, and inserted through the pia to adepth of 1.5 mm. The brain was cut sagittally 4 mm anterior tothe lambda line. The creviced skull was filled with Bonewax, andthe wound was closed with sutures. These lesioned animals showedno obvious behavioral or motor deficits. At 24 hr and 4 d aftersurgery, the lesioned animals were given two intraperitoneal injectionsof BrdU (100 mg/kg of body weight) (Sigma) over a 2 hr periodand were again anesthetized and then killed by perfusion 2 hrafter the second injection. The brains were removed, and serialfrozen sections were cut in the coronal plane at the level ofthe wound and processed for double-immunofluorescent stainingas described above.

RESULTS

m-Msi-1 expression in the SVZ of the forebrain
In the present study we characterized postnatal expression of m-Msi-1 in the CNS (Table 1). Consistent with the previousNorthern blot analysis (Sakakibara et al., 1996), the immunoblotanalysis indicated that the expression of m-Msi-1 remained inCNS during the postnatal development, albeit at a lower levelthan that observed in the embryonic CNS (data not shown). An immunohistochemicalanalysis was performed to examine the spatiotemporal pattern ofm-Msi-1 expression in the postnatal brain. We first examined m-Msi-1expression in the early postnatal forebrain, which contains theSVZ. In the P3 forebrain, a significant level of m-Msi-1 expressionwas observed in the tightly packed round cells in the SVZ, whichwas composed of PCNA-positive proliferating cells (Fig. 1D,E)(Galand and Degraef, 1989), near the anterior part of the lateralventricle (SVZa), and was also detected in the migratory pathwaytoward the olfactory bulb (Fig. 1B). This pattern of expressioncorresponded to the well described pathway of neuronal precursorcells, which lack radial glial fibers, to the olfactory bulb,where they differentiate into the interneurons of the granulecell layer and the glomerular layer (Luskin, 1993). Therefore,m-Msi-1 is probably expressed in neuronal precursor cells andimmature interneurons migrating into the olfactory bulb. In additionto the SVZa, m-Msi-1 was also expressed uniformly in the posteriorregions of the SVZ, which also contain PCNA-positive proliferatingcells (Figs. 1B, 6A,B), corresponding to the region that exclusivelycontains glial precursors (Privat, 1975). Taken together, theseresults suggest that m-Msi-1 expression is associated with gliogenesisas well as neurogenesis in the early postnatal forebrain.

Table 1. Postnatal distribution of m-Msi-1 in the CNS

Region P3-P7 Adult

SVZ and ventricular zone (lateral, third and fourth ventricles) +++ +++ SVZ cells (subependymal cells) Ependymal cells

White matter tracts

  Corpus callosum ++ ++ Astrocytes

  Cerebellar folia white matter ++ + Astrocytes

Cerebral cortex

  Layer I + ++ Astrocytes (fibrous?)

  Layers II-VI + ++ Astrocytes (protoplasmic?)

Hippocampus

  CA1 $-$ $-$

  CA2 $-$ $-$

  CA3 $-$ $-$

  Dentate gyrus + + Astrocytes (subgranular layer)

  Hilus + + Astrocytes

  Stratum radiatum + + Astrocytes

Basal nuclei

  Caudate-putamen ++ + Astrocytes

  Globus pallidus ++ + Astrocytes

Colliculi

  Inferior + + Astrocytes

  Superior + + Astrocytes

Cerebellum

  External granular cell layer ++ $-$

  Molecular layer ++ + Stellate cells

  Purkinje cell layer ++ + Bergmann glia

  Internal granular cell layer + + Astrocytes

The immunoreactivities are assessed as intense, +++; moderate, ++; weak, +; or not detectable, $-$ .

Fig. 1. m-Msi-1 expression in P3 forebrain. Serial sagittal sections of the forebrain at P3 with hematoxylin-eosin staining (A, C),immunolocalizations of m-Msi-1 (B, D), and PCNA (E). Anterioris to the right and dorsal is up. C-E, Higher magnifications ofthe anterior corner of the lateral ventricle (SVZa) shown in thebracketed portion of A. m-Msi-1 immunostaining was observed inPCNA-positive proliferating cells in SVZa. Note that m-Msi-1 expressionwas also detected in the posterior SVZ in addition to the migratoryroute of neuronal precursor cells from SVZa into the olfactorybulb described previously (Luskin, 1993). Scale bars: A, B, 500µm; C-E, 50 µm. SVZa, Anterior region of the SVZ; lv, lateralventricle.
[View Larger Version of this Image (165K GIF file)]

Fig. 6. Immunolocalization of m-Msi-1 and Hu in the developing and adult cerebrum. A, B, Serial sagittal sections showing the expressionof m-Msi-1 (A) and PCNA (B) in the SVZ and the adjacent intermediatezone at P3. Dorsal is to the right. The lateral ventricle is markedwith asterisks. At P3, m-Msi-1 is strongly expressed in tightlypacked, small round cells in the SVZ, which seem to correspondto PCNA-positive proliferating cells. It is also noted that thereare some m-Msi-1-positive cells with a few processes extendinginto the dorsal parenchyma as if they were migrating out of theSVZ. C-F, Serial sagittal sections of the P7 (C, D) and adult(E, F) cerebral cortex showing the distribution of m-Msi-1 (C,E) and Hu antigens (D, F). The pial surface is at the top. G-J,High-power photomicrographs of individual cells expressing m-Msi-1in the gray matter (layers III-IV, H and I) and white matter (layerI, G; subcortical white matter, J) in the adult cerebral cortex.By P7, in addition to the high level of expression of Msi-1 inthe SVZ, small scattered m-Msi-1-positive cells become localizedthroughout the cortex. At the same time, Hu expression is almostconfined to neurons residing in the cortical gray matter. In theadult cerebral cortex, a larger number of m-Msi-1-positive cellsare distributed uniformly in both gray and white matter, and thesehave small oval cell bodies with multiple short processes (G,I) or bipolar processes (H, J). Hu antigens continue to be expressedin large round neurons in the gray matter. MZ, Marginal zone;CP, cortical plate; CC, corpus callosum; SVZ, subventricular zone.I, II, III, V, and VI represent the cortical layers with the samedesignation. K-N, Double-immunofluorescent labeling of sectionsthrough the adult cerebral cortex: m-Msi-1 (K), GFAP (L), m-Msi-1(M), and CNPase (N). m-Msi-1-positive cells, which have multiplebranched processes, are seen throughout the cortex. Astrocytesin the superficial molecular layer and near the pial surface showcolocalization of m-Msi-1 and GFAP (arrowheads in K and L), whereasCNPase-positive oligodendroglial cell bodies predominantly presentin the molecular layer are m-Msi-1-negative (arrows in M and N).Scale bars: A, B, 18 µm; C, D, 71 µm; E, F, 36 µm; G-J, 8 µm;J-N, 10 µm.
[View Larger Version of this Image (70K GIF file)]

To determine whether m-Msi-1 is expressed in proliferating glial precursor cells within the developing SVZ, we pulse-labeledthe SVZ of P7 mice with BrdU for 3 hr before the mice were killed,and prepared coronal sections. With combined m-Msi-1 and BrdUimmunostaining, it was possible to distinguish the expressionof m-Msi-1 in dividing cells from that in postmitotic cells throughoutthe labeling period. Consequently, the majority of cells expressingm-Msi-1 were confined to SVZ regions and ependymal cells surroundingthe lateral ventricle in a pattern similar to that of BrdU incorporation(Fig. 2A,B). In particular, a large number of m-Msi-1 and BrdUdouble-positive dividing cells were detected in the dorsolateralarea (Fig. 2A,B, insets), where precursors for astrocytes andoligodendrocytes are more enriched than in other areas such asthe medial and dorsal areas of the SVZ (Levison and Goldman, 1993;Levison et al., 1993; Zerlin et al., 1995). These observationsstrongly suggested that m-Msi-1 expression occurs in the proliferatingglial precursors located within the developing SVZ. Cells immunoreactivefor m-Msi-1 within the SVZ seemed to be tightly packed and tohave small round cell bodies (Figs. 2A, 6A), with a morphologysimilar to those described previously for glial precursor cells(Levison and Goldman, 1993; Levison et al., 1993; Zerlin et al.,1995).
Fig. 2. m-Msi-1 expression in proliferating cells residing in the postnatal and adult SVZ. To label the entire constitutively proliferatingpopulation surrounding the lateral ventricles, P7 and adult micereceived 3 and 12.5 hr of BrdU injections, respectively. Double-immunofluorescentlabeling of coronal sections through the SVZ surrounding the lateralventricle in P7 forebrain (A, B) and adult forebrain (C, D) withantibodies to m-Msi-1 (A, C; FITC) and BrdU (B, D; Cy3). Lateralis to the right and dorsal is up. Insets in A and B, Higher magnificationsof the dorsolateral corner of the P7 SVZ. Many dividing, small,densely packed cells that are brightly immunostained with bothm-Msi-1 and BrdU are observed in the postnatal developing SVZ(arrowheads in insets in A and B). Similarly, a considerable numberof m-Msi-1- and BrdU-positive dividing cells are also presentin the adult subependyma (arrowheads in C and D), although itis obvious that there is a subpopulation of m-Msi-1-positive butBrdU-negative cells (arrows in C and D). Scale bars: A, B, 36µm; insets, C and D, 18 µm. Asterisks, Lateral ventricle; cc,corpus callosum; str, striatum.
[View Larger Version of this Image (106K GIF file)]

To characterize the m-Msi-1-expressing cells in this region, double-label indirect immunostaining was performed with antibodiesto m-Msi-1 and to a cell-type specific marker protein, includingthe Hu proteins HuD (Szabo et al., 1991), HuC (Liu et al., 1995),and HelN-1 (Levine et al., 1993), which label immature and differentiatedneurons, CNPase for myelinating and nonmyelinating differentiatedoligodendrocytes (Sprinkle, 1989), and GFAP for astrocytes. GFAPis an intermediate filament that is specifically expressed inmature astrocytes (Bignami and Dahl, 1974). Hu-positive immatureneurons and CNPase-positive oligodendrocytes were visible withinthe dorsolateral region of the SVZ at P7, but we observed no m-Msi-1immunoreactivity in these cells (Fig. 3A-D, arrows). GFAP immunoreactivitywas not detected in the dorsolateral corner of the SVZ (Fig. 3F).These observations suggested that m-Msi-1 is not expressed inthese differentiated cells but is confined to immature and proliferatingneuronal and glial precursors in the developing SVZ.
Fig. 3. Cell type of m-Msi-1-positive cells in the developing SVZ and the corpus callosum. Double-labeling of coronal sections justdorsolateral to the region of the P7 SVZ (A-F) and the P7 corpuscallosum (G-L) with anti-m-Msi-1 antibody (A, C, E, G, I, andK; FITC), anti-Hu (B, H; Cy3), anti-CNPase (D, J; Cy3), and anti-GFAP(F, L; Cy3). The bar in E represents 18 µm. Antibodies to CNPaseand Hu label populations that are distinct from m-Msi-1-positivecells in both the SVZ and the corpus callosum. The arrows pointto the Hu-positive but m-Msi-1-negative cells (A, B, G, H), andCNPase-positive but m-Msi-1-negative cells (C, D, I, J). AlthoughGFAP immunoreactivity is not detected in the SVZ, a few m-Msi-1-and GFAP-positive cells that have multiple processes or shortbranched processes are now present in the developing corpus callosum(arrowheads in K and L) among the more numerous m-Msi-1-positivecells.
[View Larger Version of this Image (106K GIF file)]

As gliogenesis proceeds in postnatal development, the SVZ becomes thinner. However, it persists throughout adulthood as amitotically active layer known as the subependyma (Smart, 1961;Lewis, 1968; Privat and Leblond, 1972). Recent in vivo and invitro studies have suggested that the subependyma of the adultmammalian forebrain may be a source of neural stem cells, whichmay proliferate and differentiate into both neurons and glia (Loisand Alvarez-Buylla, 1993, 1994; Morshead et al., 1994; Craig etal., 1996; Gritti et al., 1996; Johe et al., 1996). To test whetherm-Msi-1 is expressed in neural stem cells including the constitutivelyproliferating population in the adult subependyma, we pulse-labeledadult mice with BrdU for 12.5 hr before they were killed, resultingin the labeling of the entire proliferating population of subependymalcells, the constitutively proliferating cells known to have acell-cycle time of ~12.7 hr in mouse (Morshead and van der Kooy,1992). The BrdU-incorporated cells were mostly confined to thesubependymal region surrounding the SVZ but were not detectedin the parenchyma surrounding the subependyma (Fig. 2D). In particular,the dorsolateral corner of the subependyma bordered by the striatumand overlying corpus callosum contained many proliferating cellsthat incorporated BrdU (Fig. 2D). These distributions of constitutivelyproliferating cells were consistent with the results from previousstudies (Morshead et al., 1994; Gates et al., 1995). Similarly,many m-Msi-1-positive cells were distributed within most regionsof the subependyma and ependyma (Fig. 2C). Double-immunofluorescencerevealed that the majority of the BrdU-positive cells in the subependymawere also immunoreactive for m-Msi-1 (Fig. 2C,D, arrowheads).The double-positive cells predominantly observed in the dorsolateralregion of the subependyma were tightly packed, small round cells,similar to the dividing cells found in the developing SVZ describedabove. In addition, some populations of cells were only labeledwith m-Msi-1 within the ependyma and subependyma (Fig. 2C,D, arrows).These m-Msi-1-positive and BrdU-negative cells may represent theslowly dividing stem cells, which are shown to have a cell-cycletime of >12.7 hr and replenish the constitutively proliferatingneural precursors in the subependyma (Morshead and van der Kooy,1992; Morshead et al., 1994). The distribution of m-Msi-1-positivecells in the adult subependyma also supported the idea that m-Msi-1is expressed in proliferative neuronal and/or glial precursorcells.

m-Msi-1 expression in the cerebrum
In the postnatal cerebrum, immature neurons and glial cells, which had originated from the embryonic ventricular zone or thepostnatal SVZ, respectively, migrate into appropriate layers throughformative white matter, including the corpus callosum that liesadjacent to the SVZ. The completion of cerebral cortex stratificationoccurs at around P6 in mouse. As described above, it was obviousthat there were a large number of m-Msi-1-positive and denselypacked cells localized within the SVZ from early postnatal stagesinto adulthood. However, some populations of m-Msi-1-expressingcells were also found in other parenchymal regions of the cerebruminto adulthood, including the cerebral cortex, corpus callosum,and striatum, whereas they showed a lower immunoreactivity anda sparser distribution than those found in the SVZ.
The white matter In formative white matter, including the corpus callosum in the early postnatal period, cells immunoreactive for m-Msi-1 seemedto be distributed sparsely and to contain populations that haduni- or multipolar processes (Figs. 3G,I,K, 6A) rather than theimmature round cells observed in the developing SVZ (Figs. 2A,6A). These m-Msi-1-positive cells were similar to those of earlydifferentiating astrocytes derived from the SVZ that migrate tothe cortex, subcortical white matter, and striatum, as describedpreviously (Zerlin et al., 1995). As early as P7, GFAP was evidentin the corpus callosum, where some cells bearing multiple processesor short branches were stained with both m-Msi-1 and GFAP (Fig.3K,L, arrowheads). m-Msi-1 is therefore also expressed in astrocytes,including GFAP-negative immature astrocytes, in the developingwhite matter.

At this early stage, although the number of cells positive for CNPase or Hu was low in this region, neither of the antigenswere colocalized with m-Msi-1 protein (Fig. 3G-J, arrows), indicatingthat astrocytes retain expression of m-Msi-1, whereas it is notexpressed in differentiated or immature neurons and oligodendrocytes.Some antigenic markers have been used for analysis of the sequentialdifferentiation of oligodendrocytes from dividing precursors,including O-2A progenitor cells, into quiescent oligodendrocytesin vitro and in vivo (Hardy and Reynolds, 1991; Nishiyama et al.,1996). PDGF $alpha$ -R is expressed in the developing and adult rodentCNS by the O-2A oligodendrocyte progenitors and preoligodendrocytes(Pringle et al., 1992; Ellison and de Vellis, 1994; Nishiyamaet al., 1996). Similarly, NG2, a core membrane protein associatedwith chondroitin sulfate proteoglycan, is also expressed in mitoticO-2A progenitor cells localized in the gray and white matter ofperinatal to adult rat brain and disappears as these cells differentiateinto oligodendrocytes (Stallcup and Beasley, 1987; Nishiyama etal., 1996). Although the majority of NG2-positive cells also expressPDGF $alpha$ -R, a recent detailed immunohistochemical comparison of theexpression of PDGF $alpha$ -R and NG2 throughout CNS development demonstratedthat the small population of the PDGF $alpha$ -R-positive NG2-negativecells lies in the SVZ through the first postnatal week (Nishiyamaet al., 1996). These NG2-negative, PDGF $alpha$ -R-positive cells residingin the SVZ were proposed to be the earliest form of O-2A progenitorcells, which divide in the SVZ to give rise to slightly more differentiatedcells of the oligodendrocyte lineage expressing both NG2 and PDGF $alpha$ -Rin the nascent parenchyma, such as the corpus callosum and thecortex. To determine whether m-Msi-1 is expressed in the precursorcells committed to become oligodendrocytes (O-2A progenitor cells),double-immunofluorescent labeling with antibody to PDGF $alpha$ -R orNG2 was performed with sections prepared from the P2 mouse orthe P7 rat forebrain, respectively. Double-labeling for m-Msi-1and PDGF $alpha$ -R, however, demonstrated that these PDGF $alpha$ -R-positivecells did not overlap with the population of cells reactive form-Msi-1 within both the SVZ and the adjacent parenchyma (Fig.4). In addition, in the developing rat corpus callosum (P7), therewere a considerable number of sparsely distributed NG2-positivecells (Fig. 5), whereas we could not detect any cells reactivefor NG2 within the SVZ (data not shown), where m-Msi-1-positivecells were condensed. Double-labeling for m-Msi-1 and NG2 failedto reveal any double-positive cells in the corpus callosum. Cellsimmunoreactive for m-Msi-1 in the corpus callosum (Fig. 5, arrows)seemed to possess more rounded cell bodies and slightly shorterprocesses than those of NG2-positive cells (Fig. 5, arrowheads).The optic nerve of the early postnatal rat brain is also knownto contain a large number of proliferating and migrating O-2Aprogenitor cells (Miller et al., 1985; Small et al., 1987; Fultonet al., 1992). Double-labeled sections of the P7 rat optic nerveshowed that neither the PDGF $alpha$ -R/NG2-positive O-2A cells nor theCNPase-positive oligodendrocytes expressed m-Msi-1, but therewere a few astrocytes that expressed both m-Msi-1 and GFAP (datanot shown).
Fig. 4. Top. Absence of m-Msi-1 expression in PDGF $alpha$ -R-positive, early O-2A cells lying in the SVZ. Scanning confocal imagesrepresenting the expression of PDGF $alpha$ -R (red) and m-Msi-1 (green).A, Coronal section through the SVZ surrounding the dorsolateralcorner of the lateral ventricle and the adjacent corpus callosumof the P2 mouse forebrain. B, Higher magnification of the SVZsurrounding the lateral ventricle. Many PDGF $alpha$ -R-positive cells,which seem to have small cell bodies with a few processes, areobserved not only in the corpus callosum and the striatum butalso in the SVZ, where m-Msi-1-positive small cells are condensed.Note that these two populations of cells distribute intermingledbut never overlap with each other. Scale bars: A, 20 µm; B, 10µm. lv, Lateral ventricle.
Fig. 5. Bottom. Absence of m-Msi-1 expression in NG2-positive O-2A cells. Double-labeling of a section through the P7 rat corpuscallosum with anti-m-Msi-1 (A) and anti-NG2 (B) antibodies failsto reveal double-positive cells. Arrows indicate m-Msi-1-positiveand NG2-negative cells. Arrowheads point to cells that are m-Msi-1-negativebut NG2-positive. Scale bar, 30 µm.

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The gray matter In the developing cerebral cortex at P3, there were only a few cells immunoreactive for m-Msi-1 (data not shown). At P7, asthe stratification of the cortex proceeded, we observed the accumulationof m-Msi-1-positive cells throughout the cerebral cortex (Fig.6C), where most of them had small, round to oval cell bodies anda few short processes, resembling astrocytes in the process ofdifferentiation. In contrast, Hu proteins were expressed exclusivelyin a population of large round neurons in the P7 cortical graymatter, distinct from the m-Msi-1-positive small cells (Fig. 6D).At subsequent developmental stages into the adult, there was acontinuously increasing number of m-Msi-1-positive cells. Thesecells were distributed uniformly within the cortex and had smallcell bodies with a few or multiple long processes extending inall directions (Fig. 6E, G-J), giving them an appearance of differentiatedastrocytes. Hu was still expressed in large round cells, whichseemed to be neurons, throughout the forebrain, including thepyramidal neurons in the cerebral cortex (Fig. 6F). Double-labelingwith Hu and m-Msi-1 antibodies clearly revealed that cells thatwere intensely positive for m-Msi-1 were Hu-negative, and conversely,cells with larger, round cell bodies that expressed high levelsof Hu proteins were m-Msi-1-negative, indicating that m-Msi-1was expressed in non-neuronal cells (data not shown). Moreover,many astrocytes closely associated with vascular blood vessels,often appearing to make contact with the endothelial cells (datanot shown) and cells lying under the pial surface (Fig. 6K), werealso immunoreactive for m-Msi-1. Most of the m-Msi-1-positivecells in the adult cortex seemed to express the antigen throughoutthe entire cell body and processes (Fig. 6G-J).

To confirm the glial cell types expressing m-Msi-1 in the adult cerebral cortex, double-label immunofluorescence experimentswere performed. The distribution of m-Msi-1-positive cells wascompared with that of cells stained by the glial markers CNPaseand GFAP. Sections double-labeled with antibodies to m-Msi-1 andGFAP revealed that there were many cells immunoreactive for bothantigens in the adult cerebral cortex, as expected (Fig. 6), althougha proportion of cells expressing m-Msi-1 were not reactive forGFAP. Cells that were positive for both m-Msi-1 and GFAP, whichwere predominantly distributed in the molecular layer (layer I)and near the pial surface in the cerebral cortex, possessed relativelythick and branched processes, typical of differentiated astrocytes(Fig. 6). In addition, a considerable number of m-Msi-1-positivebut GFAP-negative cells were observed in the deeper layers (layersII-VI) of the cortex (Fig. 6E,K,L). These cells may representprotoplasmic astrocytes, which are numerous in cortical layersII-VI but are sparse in layer I. Many of them were not stainedby GFAP immunohistochemistry (Miller and Raff, 1984).

In oligodendrocytes, nonoverlapping populations of cells were positive for CNPase or m-Msi-1 in the adult cerebral cortex.Many CNPase-positive oligodendrocytes could be found in the molecularlayer of the gray matter and the subcortical white matter of thecerebral cortex. These cells had elongated cell bodies and processesbranching parallel to the axons (Fig. 6N). Although m-Msi-1-positivecells and CNPase-positive cells were found to be comingled throughoutthe gray and white matter, CNPase-positive cells were exclusivelynegative for m-Msi-1, and m-Msi-1-positive cells expressed noCNPase (Fig. 6M, N). Oligodendrocytes labeled with CNPase seemedto have oval cell bodies and processes that were finer than thoseof m-Msi-1-positive cells.

These data indicated that m-Msi-1 expression was largely restricted to the mitotic glial precursor cells in the SVZ and astrocytes,which included GFAP-negative protoplasmic astrocytes and GFAP-positivedifferentiated astrocytes.

m-Msi-1 expression in the cerebellum
A dynamic pattern of m-Msi-1 expression was also observed in the developing cerebellum. In the cerebellar primordium at embryonicday 16.5, m-Msi-1 was largely expressed in the tightly packedsmall cells of the external granule cell layer (EGL) migratingout of the rhombic lip of the lateral recess, and also in theventricular zone of the fourth ventricle (data not shown). ByP3, significant m-Msi-1 expression could be detected in the EGL(Fig. 7D), which covers the surface of the developing cerebellumand is known to be composed exclusively of proliferating neuronalprecursors. As neurogenesis progresses, two populations of cellsappear in the EGL: cells proliferating in the superficial aspectof the EGL (EGLa) and cells undergoing the initial step of neuronaldifferentiation in the deeper aspect of the EGL (EGLb) (Altman,1972; Kuhar et al., 1993). At P7, m-Msi-1 expression was mainlyobserved within the PCNA-positive proliferating cells in the superficialEGLa, although very low expression was also detected in the deeperlayer EGLb (Fig. 7A,C). Conversely, Hu expression was restrictedto the PCNA-negative postmitotic granule neurons within the EGLb(Fig. 7B,C). The numerous neurons in the internal granule celllayer (IGL), including the Purkinje cells forming a single row,were reactive for Hu but not for m-Msi-1 (Fig. 7A,B, arrowheads).
Fig. 7. Distribution of m-Msi-1 and Hu in the developing (A-D) and adult (E-K) cerebellum. D, m-Msi-1 expression in the P3 cerebellum.m-Msi-1 is expressed in neuronal precursor cells in the externalgranule cell layer (EGL) and in the vast number of small cellsthat have a few processes in the deep cerebellar regions. Intensem-Msi-1 staining is also noted in densely packed small cells inthe SVZ lining the fourth ventricle (IV) and in the superior medullaryvelum (SMV) located at the base of the cerebellum. A-C, Serialsagittal sections showing the immunolocalization of m-Msi-1 (A),Hu (B), and PCNA (C) in the EGL, the deep cerebellar regions,and folia white matter (WM) at P7. The EGL is toward the top ofthe panels. At P7, weak expression of m-Msi-1 is seen mainly inthe EGLa, which contains the PCNA-positive outer proliferatingzone of the EGL, whereas Hu expression is observed in the EGLb,which contains the PCNA-negative inner early differentiating neurons.Granule neurons within the internal granule layer (IGL) and Purkinjecells (arrowheads) forming a single row show immunoreactivityfor Hu but not for m-Msi-1. m-Msi-1 expression is retained bysmall oval cells that have a few processes and reside in the deepcerebellar regions and WM. G, H, Sagittal sections showing theexpression of m-Msi-1 (G) and Hu (H) in the adult cerebellum.E, F, Higher magnifications of the molecular layer (ML), Purkinjecell layer (PL), and IGL shown in G and H, respectively. I-K,High-power photomicrographs of individual cells expressing m-Msi-1in the PL (I), IGL (J), and WM (K) of the adult cerebellum. Inthe PL, m-Msi-1 is expressed in Bergmann glia, the cell bodiesof which are located adjacent to the large cell bodies of Purkinjecells (Pr) and extend their tangential processes into the ML.In addition, sparsely distributed putative astrocytes in the IGLand WM, which exhibit oval or elongated cell bodies with multipleshort processes (J) or bipolar processes (K), are labeled withthe m-Msi-1 antibody. IC, Inferior colliculus. Scale bars: A-C,36 µm; D, G, H, 71 µm; E, F, 25 µm; I-K, 8 µm.
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In addition, there were a large number of m-Msi-1-positive cells within the developing IGL, the deep cerebellar regions, andthe putative white matter tracts (Fig. 7A,D). Most of these cellsshowed small oval cell bodies with unipolar or bipolar processes,which seemed to be migrating or differentiating glial cells. m-Msi-1was also strongly expressed in small round cells without processesin the SVZ lining the fourth ventricle, including the cerebralaqueduct, and in the superior medullary velum located at the baseof the cerebellum (Fig. 7D), whereas Hu was completely absentfrom these cells (data not shown). Small numbers of scatteredm-Msi-1-positive cells were observed over the developing inferiorcolliculus, which was continuous with the base of the cerebellumvia the superior medullary velum, but the number was small comparedwith those seen in the cerebellum (Fig. 7D). Although we havenot demonstrated the route of migration of m-Msi-1-positive cellsper se, the expression pattern of m-Msi-1 in the developing cerebellumseemed to be consistent with patterns of glial precursor cellsand migrating immature glial cells that originate from the SVZcells of the fourth ventricle (Goldman et al., 1984; Curtis etal., 1988; Reynolds and Wilkin 1988).

In the adult there was a decrease in the number of m-Msi-1-positive cells, although expression was still found in scatteredcells in most regions of the cerebellum (Fig. 7G). In the Purkinjecell layer, which contains the Purkinje neurons and cell bodiesof the Bergmann glia, m-Msi-1 expression seemed to be restrictedto the radially aligned Bergmann glial cells and their fibersthat course from the Purkinje cell layer through the molecularlayer to the pial surface and was not detected in the adjacentPurkinje neurons (Fig. 7E,G,I). In the IGL, most of the m-Msi-1-positivecells were sparsely distributed, with small oval cell bodies andmany short processes (Fig. 7E,J). The distribution and morphologywere clearly distinct from those of Hu-positive granule neurons(Fig. 7B,F,H). In the central white matter tracts of the cerebellum,m-Msi-1 was expressed in scattered oval cells bearing unipolaror bipolar processes (Fig. 7A,K). To assess the type of cellsthat were immunoreactive for m-Msi-1, we performed indirect double-labelingon tissue sections of adult cerebellum with antibodies to GFAP,CNPase, and Hu. Colocalization of m-Msi-1 and GFAP was observedin various regions, including the Purkinje cell layer (Bergmannglia), IGL, and foliar white matter tracts. Neither CNPase norHu, however, was coexpressed with m-Msi-1 in these regions (datanot shown), confirming that m-Msi-1 was expressed in differentiatedastrocytes, including Bergmann glial cells. However, we noticedthat small populations of differentiated neurons in the cerebellarnuclei or interneurons, such as the stellate cells residing inthe molecular layer, expressed m-Msi-1 (Fig. 7E-H). Similarly,we observed a weak expression of m-Msi-1 in some populations ofdifferentiated neurons in the suprageniculate nucleus and paraventricularnucleus of the adult thalamus and hypothalamus (data not shown).

Taken together, the spatiotemporal distribution of m-Msi-1 strongly supports the idea that during the development of the cerebellum,the expression of m-Msi-1 is mainly restricted to the glial precursorcells and postmitotic and differentiated astrocytes, in additionto proliferating neuronal precursors found in the EGL. This expressionpattern seemed to be comparable with that in the developing cerebrum.However, the expression of m-Msi-1 in some populations of differentiatedneurons cannot be explained in this context.

Changes in m-Msi-1 immunoreactivity after injury
The present results indicating that m-Msi-1 was expressed in the cells of astrocyte lineage in postnatal brain led us to examinethe changes in m-Msi-1 expression during the formation of glialscars after CNS injury. Small puncture lesions were made in thecerebral cortices of anesthetized adult mice. The appearance ofnormal adult cerebral tissue stained with the m-Msi-1 antibodyis shown in Figure 6E as a control. Experimentally induced damageto the CNS leads to multiple changes in the glial cells surroundingthe damaged tissue and to formation of a glial scar at the siteof injury. Immunohistochemical and autoradiographic studies haveindicated that hypertrophic and hyperplastic reactive astrocytesin the regions immediately adjacent to the injury site displayincreased levels of GFAP and become mitotically active (Miyakeet al., 1988, 1992; Takamiya et al., 1988).

At 1 d postlesion, most of the m-Msi-1-positive cells around the lesion site exhibited no significant differences from m-Msi-1-positivecells in undamaged areas of the same tissue section (data notshown). At 4 d postlesion, there was a dramatic increase in thenumber of m-Msi-1-positive cells in the vicinity of the injurysite of the cerebral cortex (the region within 100-200 µm of theinjury site) (Fig. 8). Compared with cells lying within the undamagedcerebral hemisphere, these cells exhibited an enhanced reactivityto m-Msi-1 antibody and had enlarged or elongated cell bodieswith thick processes, occasionally with unipolar or bipolar processesoriented parallel to the needle track (Fig. 8). In addition tothe effects in the immediate vicinity of the injury, there werealso significant changes farther away from the injury site (regions>200 µm from the lesion; data not shown). The fact that thesemorphologically altered cells were not confined to the bordersof the lesion suggests that the changes in m-Msi-1 expressionare not attributable to direct physical damage of the cells.
Fig. 8. m-Msi-1 expression in reactive astrocytes in the injured region of adult cerebral cortex. Double-label fluorescent localizationof m-Msi-1 and BrdU, GFAP, nestin, or MacI at 4 d postlesion.I, Schematic illustration of a coronal section through the injuredforebrain. All photomicrographs correspond to the boxed regionin I. The lesioned sites are toward the top in all panels. A,m-Msi-1 (Cy3). B, Same field, BrdU (FITC). To label a proliferatingpopulation after brain injury, mice received BrdU injections for3 hr before they were killed. m-Msi-1 is expressed in a populationof BrdU-positive proliferating cells (arrowheads) that lie closeto the injury site and have enlarged cell bodies with multipleprocesses. C, m-Msi-1 (Cy3). D, Same field, GFAP (FITC). Intensem-Msi-1 staining is observed in an increased number of GFAP-positivereactive astrocytes surrounding the lesioned site; these cellsexhibit enlarged, elongated cell bodies with multiple processes.E, m-Msi-1 (Cy3). F, Same field, nestin (FITC). The simultaneousexpression of nestin is induced in a subpopulation of m-Msi-1-positivereactive cells near the lesioned site. G, m-Msi-1 (FITC). H, Samefield, MacI (Cy3). Large numbers of macrophages or ameboid microglia,which are MacI-positive but m-Msi-1-negative, form a dense plaquesurrounding the lesion site. Arrows indicate the MacI-positiveramified microglia that are immunonegative for m-Msi-1. Scalebar (shown in A): 18 µm. lv, Lateral ventricle; cc, corpus callosum;str, striatum.
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To determine whether this increased population of m-Msi-1-positive cells represents a so-called reactive astrocyte that proliferatesin an injured area and participates in a glial scar formationat the site of injury (Miyake et al., 1988, 1992), we performeddouble-label immunostaining for m-Msi-1 and GFAP. As shown inFigure 8, in areas immediately adjacent to the injury site, numerousGFAP-positive astrocytes were present that had long and wavy processesextending in all directions or parallel to the needle track andseemed to form a thick bundle of glial array in the scar tissue,characteristics typical of reactive astrocytes. Double-labeledsections revealed that most of the m-Msi-1-positive cells in theseareas also expressed GFAP (Fig. 8C,D). This colocalization ofm-Msi-1 and GFAP and the morphological characteristics of thecells strongly suggested that at least in the regions adjacentto the injury site, m-Msi-1 was expressed at high levels in reactiveastrocytes that have been generated in response to injury andhave a hyperplastic appearance.

The increases in the level of m-Msi-1 staining and in the number of cells expressing m-Msi-1 within the 4 d after injury suggestthat this population of m-Msi-1-positive glial cells may be stimulatedto proliferate by the injury. To assess this possibility directly,animals were given two injections of BrdU, and cerebral coronalsections were prepared for double-immunolabeling with antibodiesto m-Msi-1 and BrdU. At 1 d postlesion, there were no m-Msi-1-positivecells that incorporated BrdU throughout the injured cerebrum (datanot shown). At 4 d postlesion, a number of cells that had incorporatedBrdU appeared in regions adjacent to the site of the lesion. Approximately20% of these BrdU-labeled cells also expressed m-Msi-1 (Fig. 8A,B).These BrdU- and m-Msi-1-positive cells exhibited enlarged or elongatedcell bodies (Fig. 8A,B, arrowheads), similar to GFAP-positivereactive astrocytes. This was consistent with previous studiesshowing the occurrence of cell division among GFAP-expressingastrocytes induced by brain injury (Miyake et al., 1988, 1992).In addition, the colocalization of BrdU and m-Msi-1 was observedin a few cells that were >100 µm away from the injury site. Thesecells frequently appeared in the subependymal region and the corpuscallosum in the injured hemisphere, although by our method ofBrdU administration, we found no BrdU-positive cells within theuninjured brain hemisphere (data not shown). Interestingly, bothof these sources of dividing m-Msi-1-positive cells also expressedanother intermediate filament protein, nestin (Fig. 8E,F), whichis a well defined marker for neural precursors or stem cells duringnormal development of the CNS (Hockfield and McKay, 1985; Frederiksenand McKay, 1988; Lendahl et al., 1990; Zimmerman et al., 1994).Although the uninjured adult forebrain had weak nestin immunoreactivity,marked induction of nestin was observed 4 d after injury in bothregions adjacent to the injury site (Fig. 8F) as well as in regionsdistant from the injury site, such as the subependyma and theoverlying corpus callosum (data not shown). The colocalized expressionof nestin and m-Msi-1 after injury may further imply that theexpression of m-Msi-1 is maintained by cells that are in a precursorstate and able to proliferate in response to injury.

On the other hand, the area adjacent to the injury site contained many BrdU-positive proliferating cells that were immunonegativefor m-Msi-1 at 4 d postlesion (Fig. 8). Most of these cells seemedto be activated microglia, which proliferated in response to theinjury, or proliferating macrophages and monocytes, which rapidlyinfiltrated into the injured parenchyma from the circulation whenthe injury also disrupted the blood-brain barrier. To examinewhether m-Msi-1 expression was induced in the microglia and macrophagesafter injury, sections through the damaged area were double-stainedwith antibodies to m-Msi-1 and the monoclonal antibody MacI (Thomas,1992), which identifies microglia, macrophages, and monocytes.As shown in Figure 8, MacI-positive cells rapidly became activatedby injury and increased in number in the damaged tissue. At 4d postlesion, numerous MacI-positive cells appeared at the bordersof the injury and formed a dense network, surrounding and partiallyfilling the injury site (Fig. 8H). These cells seemed to be composedlargely of activated ameboid microglia having large round cellbodies, and partially composed of macrophages and monocytes, whichinfiltrated from the circulation. There were also many MacI-positiveramified cells, located 50 µm or more from the injury site, whichwere microglia and were unaffected by the injury (Fig. 8H, arrows).Indirect fluorescent double-labeling revealed that m-Msi-1 stainingdid not overlap with either the ameboid MacI-positive cells atthe borders of the injury or the ramified ones in locations distantfrom the site of injury (Fig. 8G,H). This observation showed thatboth activated and ramified microglia did not express m-Msi-1.

DISCUSSION

m-Msi-1 may function in the generation of astrocytes in addition to neuronal precursor cells
The present results indicated that m-Msi-1 is expressed in proliferative neuronal precursor cells, such as cells in the cerebellarEGLa and cells migrating from the SVZa into the olfactory bulbin the early postnatal CNS. Consistent with this, m-Msi-1-positivecells are present in the proliferative ventricular zone of theembryonic forebrain and spinal cord (Sakakibara et al., 1996).In addition, we showed that m-Msi-1 is expressed in proliferativeglial precursor cells present in the postnatal SVZ and in constitutivelyproliferating cells (neural stem cells) in the adult subependyma,which may differentiate into neurons and glia in vitro (Lois andAlvarez-Buylla, 1993; Gritti et al., 1996; Johe et al., 1996).

m-Msi-1 is likely to be preferentially expressed in the astrocyte lineage during the development of glial cells. This doesnot necessarily suggest, however, that m-Msi-1-positive precursorcells in the SVZ have fates that are more restricted toward astrocytelineage in glial cell development. Because a recent study usingretroviral labeling of a single SVZ precursor cell in vivo inpostnatal rats demonstrated the presence of bipotential glialprecursor cells that give rise to both oligodendrocytes and astrocytes(Levison and Goldman, 1993), m-Msi-1-positive precursor cellsin the SVZ may also potentially give rise to oligodendrocytes.However, m-Msi-1 was not expressed in the PDGF $alpha$ -R/NG2-positiveO-2A cells, the probable intermediate precursors of the oligodendrocytelineage (Ellison and de Vellis, 1994; Nishiyama et al., 1996).Thus, if m-Msi-1 is expressed in the bipotential glial precursorcells in the SVZ, m-Msi-1 expression must be largely downregulatedat the very early stage of differentiation of oligodendrocytelineage when PDGF $alpha$ -R/NG2 expression begins in O-2A cells (Fig.9).
Fig. 9. Schematic representation of cells expressing m-Msi-1 during embryonic and postnatal CNS development. Solid patterns representm-Msi-1-positive cells. In the embryonic CNS, m-Msi-1 is expressedin proliferating neural precursors in the ventricular zone (VZ);these cells are capable of self-renewal and generate postmitoticneurons, as described previously (Sakakibara et al., 1996). Inthe perinatal stage, the VZ shrinks and a second proliferativeSVZ appears. Postnatally, m-Msi-1 expression is seen in proliferatingglial precursors in the SVZ and cells of astrocyte lineage, includingependymal cells and Bergmann glia. At present, it is not knownwhether neural precursors in the embryonic VZ generate glial precursorsin the postnatal SVZ, or whether bipotent glial precursors inthe postnatal SVZ generate the astrocyte and O-2A-oligodendrocytelineages through an "asymmetric cell division." However, thisasymmetric division at least may occur when neuronal precursorsgive rise to neurons in the embryonic VZ (Chenn and McConnell,1995). The expression of m-Msi-1 in some populations of neuronsis not represented for reasons of simplicity.
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The role of m-Msi-1 in the generation of astrocytes from precursor cells in the SVZ during the early postnatal developmentof the forebrain may be explained by the following sequentialevents. First, proliferating m-Msi-1-positive glial precursorsin the SVZ give rise to numerous m-Msi-1-positive and GFAP-negativeimmature astrocytes exhibiting single or bipolar processes andpredominantly residing in the regions adjacent to the SVZ. Subsequently,these immature astrocytes migrate into the overlying parenchymadorsal and lateral to the corpus callosum, and finally a populationof these cells become dispersed in almost all regions of the forebrainwhere they have terminally differentiated and undergone morphologicalchanges or acquired GFAP immunoreactivity. This developmentalprofile of astrocytes from SVZ precursor cells is also supportedby previous ³H-thymidine labeling studies (Paterson et al., 1973; Imamoto etal., 1978) and lineage tracing of retroviral-labeled SVZ precursorcells (Levison and Goldman, 1993; Levison et al., 1993; Zerlinet al., 1995).

What type of astrocytes are m-Msi-1-positive cells? Astrocytes in the adult cerebrum are classified into two major types basedon morphology and anatomical distribution. GFAP-positive fibrousastrocytes are located mainly in the white matter and the molecularlayer of the cortex, and protoplasmic astrocytes are found mainlyin the gray matter and frequently exhibit undetectable levelsof GFAP-immunoreactivity (Miller and Raff, 1984). In the adultcerebrum, coexpression of m-Msi-1 and GFAP was observed predominantlyin the superficial molecular layer, whereas there were a largenumber of m-Msi-1-positive but GFAP-negative cells in the deepergray and white matter. Thus, the majority of m-Msi-1-positiveastrocytes in the molecular layer and in deeper layers of cortexmay correspond to the anatomically defined fibrous and protoplasmicastrocytes, respectively. In this context, m-Msi-1 may providean excellent marker for astrocytes, including GFAP-negative protoplasmicastrocytes.

After brain injury, upregulation of m-Msi-1 expression was observed in a vast number of cells in broad regions of the injuredcerebral hemisphere, including the subependyma distant from theinjury site, as well as in the GFAP-positive proliferating reactiveastrocytes in the immediate vicinity of the lesioned site. Previousstudies suggested that protoplasmic astrocytes can transform intothe fibrous type in response to injury and that the marked increasein the number of GFAP-positive reactive astrocytes in the injuredcortex is principally attributable to upregulation of GFAP expressionin already existing protoplasmic astrocytes surrounding the injurysite, rather than to the induction of proliferation of GFAP-positivereactive astrocytes themselves (Bignami and Dahl, 1976; Graeberand Kreutzberg, 1986; Miyake et al., 1988, 1992). Consistent withthe presumptive m-Msi-1 expression in the protoplasmic astrocytesin the normal cerebral cortex, the majority of m-Msi-1-positivecells observed at least in the vicinity of the lesioned site mayrepresent overproduced protoplasmic astrocytes that are destinedto become reactive astrocytes in the injured area. To confirmthis possibility, however, lineage-tracing experiments of m-Msi-1-expressingcells are required (discussed below).

These results, taken together with the previous lineage study of SVZ cells using retroviral gene transfer (Levison and Goldman,1993), suggest that m-Msi-1-positive cells in both the deepercortical layer (GFAP-negative) and the molecular layer (GFAP-positive)may belong to the same astrocyte lineage derived from a commonprecursor cell proliferating in the SVZ. Then cells expressingm-Msi-1 but not GFAP may represent astrocytes that are in theprocess of development, before terminal differentiation. To addressthese issues as well as the possible expression of m-Msi-1 inthe bipotential glial precursor cells, it will be necessary toperform lineage-tracing experiments, for example using the GFPreporter driven by the m-msi-1 promoter in a recombinant retrovirus,or knock-in mice combined with explant culture techniques. Moresophisticated lineage experiments using the Cre/loxP system arealso going to be examined.

Possible functions of m-Msi-1 in neural development
On the basis of an analogy with Drosophila d-Msi, and the in vivo and in vitro expression pattern of m-Msi-1 in the embryonicCNS, we proposed previously that m-Msi-1 may be required for neuronallineage formation from undifferentiated neural precursor cellsthat can give rise to both neurons and glia, or in the maintenanceof these precursor cells (Sakakibara et al., 1996). In the presentstudy, we observed m-Msi-1 expression not only in neuronal precursorsbut also in glial precursor cells and astrocytes during postnatalCNS development. m-Msi-1 protein may regulate the expression ofRNA molecules, which are required for the maintenance of bothneuronal and glial precursor cells and differentiated astrocytes.If m-Msi-1 was shown to be expressed in bipotent glial precursorcells that give rise to both O-2A/oligodendrocytes and astrocytesby the lineage studies, it would be tempting to speculate thatm-Msi-1 might be involved in the determination and maintenanceof an astrocyte lineage from a bipotent glial precursor cell inSVZ (summarized in Fig. 9). This may be achieved by controllingthe expression of target genes to repress the generation of O-2A/oligodendrocytelineage from a bipotent glial precursor cell, consistent withthe observations showing the absence of m-Msi-1 expression fromthe early stage of oligodendrocyte (O-2A) development and persistentexpression in the SVZ glial precursor cells. This idea is alsocomparable with the loss of m-Msi-1 expression in differentiatingneurons during embryonic (Sakakibara et al., 1996) and postnatalneurogenesis (Fig. 9). Thus, m-Msi-1 may regulate common key RNAmolecules, which are required for the determination of these cell-fatesfrom both glial and neuronal precursors.

The elucidation of the target RNA molecules of m-Msi-1, which is currently in progress in our laboratory, will unequivocallyreveal the function of this protein. Phenotypic analysis of m-msi-1knock-out mice will also help us to understand the role of thisgene product in the embryonic and postnatal CNS development.

FOOTNOTES

Received May 14, 1997; revised Aug. 18, 1997; accepted Aug. 19, 1997.

This work was supported by grants from the Japanese Ministry of Education, Science and Culture (S.S., H.O.), and by Core Researchfor Evolutional Science and Technology (CREST), Japan Scienceand Technology Corporation. S.S. is a research fellow of the JapanSociety for the Promotion of Science. We thank Drs. Miyuki Yamamotoand Masato Nakafuku for their critical reading of this manuscript.

Correspondence should be addressed to Dr. Hideyuki Okano, Department of Neuroanatomy, Biomedical Research Center, Osaka University,Suita, Osaka 565, Japan.

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