Subpallial Dlx2-Expressing Cells Give Rise to Astrocytes and Oligodendrocytes in the Cerebral Cortex and White Matter

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The Journal of Neuroscience, November 15, 2002, 22(22):9821-9830

Subpallial Dlx2-Expressing Cells Give Rise to Astrocytes and Oligodendrocytes in the Cerebral Cortex and White Matter
Christine A. G. Marshall¹ and James E. Goldman¹^,²
¹ Center for Neurobiology and Behavior, and ² Division of Neuropathology, Department of Pathology, Columbia University, College of Physicians and Surgeons, New York, New York 10032

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The precise origins of postnatal subventricular zone (SVZ) cells are not known. Furthermore, the gliogenic potential of progenitorsexpressing Dlx genes that migrate ventrodorsally from the ganglioniceminences has not been explored in vivo. Here, we identify theembryonic origins of two distinct populations of postnatal SVZcells: SVZ border cells, which express Zebrin II, and migratorycells in the central SVZ, which are generally devoid of ZebrinII expression (Staugaitis et al., 2001). Zebrin II is expressedby all cells of the telencephalic primordium, with its expressionbecoming restricted to astrocytes in the mature telencephalon.As the neuroepithelium folds during corticostriatal sulcus formation(embryonic day 13-15), a wedge of Zebrin II+ cells is createdat the presumptive site of the dorsolateral SVZ. At this time,Dlx2-expressing cells and their progeny begin to migrate ventrodorsallyalong a medial path from the ganglionic eminences. These migratorysubpallial cells invade the wedge of Zebrin II+ cells to formthe central region of the SVZ. We used a Dlx2/tauLacZ knock-into perform a short-term lineage analysis of Dlx2-expressing cellsthroughout SVZ formation and the postnatal peak of gliogenesis.Dlx2/tauLacZ [ $beta$ -galactosidase ( $beta$ -gal)]-expressing cells populatethe central SVZ, whereas Zebrin II-expressing cells form its borders.Furthermore, $beta$ -gal expression demonstrates a lineage relationshipbetween Dlx2-expressing cells and glia residing in the dorsaltelencephalon. We propose a model for the formation of the postnatalSVZ and demonstrate that subpallium-derived Dlx2-expressing cellsgive rise to astrocytes and oligodendrocytes in the white matterand cerebralcortex.

Key words: mouse; glia; subventricular zone; Zebrin II; Dlx2; ganglionic eminence; lateral ganglionic eminence; medial ganglionic eminence

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Astrocytes and oligodendrocytes are generated throughout embryonic and postnatal development in the murine telencephalon.Astrocytes originate from two sources: from the neuroepithelium,via a radial glial phenotype (Luskin et al., 1988; Price and Thurlow,1988; Voigt, 1989), and from migratory progenitors that emergefrom the dorsolateral subventricular zone (SVZ) to colonize adjacentgray and white matter (Levison and Goldman, 1993; Luskin and McDermott,1994). Oligodendrocytes are thought to originate from the ventralneuroepithelium and to become specified by exposure to Sonic hedgehog(Shh) during embryogenesis (Woodruff et al., 2001). However, itis not clear whether all oligodendrocytes are specified ventrally.Postnatally, progenitors emigrate from the SVZ into the striatum,white matter, and cortex, where some develop into oligodendrocytes(Levison and Goldman, 1993; Luskin and McDermott, 1994). Manyof these cells are not committed irrevocably to an oligodendrocytefate, as SVZ progenitors generate clones containing both astrocytesand oligodendrocytes in vivo and mixed neuronal-glial clones invitro (Levison and Goldman, 1993; Levison and Goldman, 1997; Parnavelas,1999). How can one reconcile the ventral specification of oligodendrocyteswith the emergence of both astrocytes and oligodendrocytes fromthe postnatal SVZ? In one possible model, progenitors originatein the ventral telencephalon and migrate dorsally into the SVZ.Some are specified as oligodendrocyte precursors, whereas othersrepresent astrocyte or neuronal precursors or perhaps remain uncommitted.A ventrodorsal migration of oligodendrocyte or astrocyte precursorsinto the dorsal telencephalon has not been demonstrated previously.Our hypothesis requires that telencephalic astrocytes and oligodendrocytesbe traced back to progenitors in the embryonic ventraltelencephalon.

Recent studies demonstrate tangential cell migration from the ventral basal ganglia into the dorsal cortex and hippocampus(Marin and Rubenstein, 2001). Some of these migratory progenitorsexpress the ventral forebrain markers Dlx1/2 (Anderson et al.,1997) and give rise to interneurons, but the fate of the entiredorsally migrating population is not known. Progenitors from theganglionic eminences have the potential to give rise to neuronsand glia in vitro (He et al., 2001), but their ability to contributeastrocytes and oligodendrocytes to the dorsal telencephalon hasnot been demonstrateddirectly.

To begin examining SVZ origins, we divided the postnatal SVZ into two subpopulations of cells on the basis of the expressionof Zebrin II (Aldolase C). Large, polygonal cells situated atthe borders of the SVZ express Zebrin II, whereas smaller, roundmigratory progenitors residing in the central SVZ generally donot (Staugaitis et al., 2001). Subsequently, we characterizedthe expression of Zebrin II throughout embryonic and early postnataldevelopment, observing that it is a general marker for ventricularzone (VZ) cells. We used a Dlx2/tauLacZ knock-in mouse (Corbinet al., 2000) to perform a short-term lineage analysis of subpallium-derivedDlx2-expressing cells, following the fates of these cells andtheir progeny well into postnatal development. We found that cellsderived from subpallial, Dlx2-expressing progenitors migrate dorsallyand intermix with Zebrin II-expressing VZ cells at the corticostriatalsulcus to form the dorsolateral SVZ. Furthermore, these progenitorsdevelop into astrocytes and oligodendrocytes of the postnatalcerebral cortex and whitematter.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. C57BL/J6 mice were used in all experiments requiring wild-type animals. The morning of vaginal plug formation wasconsidered embryonic day 0 (E0) for gestational staging purposes.Mouse colonies are maintained at the Columbia University HealthSciences Campus in accordance with National Institutes of Healthand United States Department of Agricultureguidelines.

Slice cultures. Organotypic slice cultures of embryonic mouse telencephalon were prepared as follows. E16 brains were dissected,embedded in a 4% low-melting-point agarose (Bio-Rad, Hercules,CA) solution with HBSS (Invitrogen, San Diego, CA), placed directlyon ice, and cut into 300 µm coronal slices with a vibratome. Slicesat the level of the septal nuclei were collected into ice-coldHBSS and transferred gradually into a culture medium containingBME; penicillin-streptomycin (20 U/ml; Invitrogen); L-glutamine(2 mM; Invitrogen); 5 µg/ml insulin, 5 µg/ml transferrin, and5 ng/ml sodium selenite (Sigma, St. Louis, MO),;bovine serum albumin(1 gm fraction V; Sigma); and glucose (0.5%, Sigma). Slices werethen placed onto Millicell CM tissue culture inserts (30 mm diameter,0.4 µm pore; Millipore, Bedford, MA) in six-well plates (Falcon,Franklin Lakes, NJ) containing 1.2 ml medium and cultured in asterile incubator (5% CO₂, 37°C). During the first hour afterplating, slices were cultured in the defined medium listed abovewith 10% fetal calf serum (Invitrogen). After 1 hr, the mediumwas exchanged with the defined serum-free culture medium listedabove with N2 and B27 supplements (1X;Invitrogen).

Retroviral infections. Retrovirus encoding cDNA for green fluorescent protein (GFP) was produced by a packaging cell line(generous gift from Drs. Suhr and Palmer, Laboratory of Genetics,The Salk Institute for Biological Studies, La Jolla, CA) thathad been transfected with a retrovirus plasmid (pNIT) containinga cDNA fragment of GFP (enhanced GFP c2) (Clontech, Palo Alto,CA) and harvested as described previously (Kakita and Goldman,1999). Virus titer was ~5 × 10⁵ cfu/ml. Retrovirus was drawn by capillary action into a pulledglass micropipette (Drummond, Broomall, PA), and a minimal volume(<1 µl) was directed into the merged lateral ganglionic eminence(LGE) and medial ganglionic eminence (MGE) of E16 organotypicslices by hand using a dissecting microscope. Images of slices(10×) were captured after 24 hr in culture to detect GFP-expressing,retrovirally infected cells within the LGE/MGE using an Axioplanepifluorescence microscope with an Axiocam digital camera (CarlZeiss, Thornwood, NY) and Openlab 3.0 imaging software (Improvision,Ltd, Lexington,MA).

Immunohistochemistry. Pregnant dams were anesthetized with the inhalent Halothane, United States Pharmacopeia (HalocarbonLabs, River Edge, NJ), and embryos were removed through a laparoscopicincision. Embryos younger than E16 were decapitated, and headswere immersion-fixed in 4% paraformaldehyde in PBS overnight at4°C. Embryos (E16 and older) and neonates were anesthetized witha mixture of xylazine (75 mg/kg) and ketamine (5 mg/kg) (HenrySchein, Melville, NY) and perfused transcardially with 4% paraformaldehydein PBS. Brains were postfixed for 4 hr at 4°C. All tissue wascryoprotected in 30% sucrose in PBS at 4°C, frozen at $-$ 80°C, cutinto 16-20 µm coronal sections with a cryostat, and mounted onSuperfrost Plus slides (Fisher, Pittsburgh, PA). Frozen braintissue from Dlx2/tauLacZ mice (received from Drs. J. Corbin andG. Fishell, New York University Medical Center, New York, NY)was sectioned and mounted similarly. Organotypic slices were fixedin 4% paraformaldehyde in PBS for 2 hr at room temperature, rinsedin PBS, cryoprotected, and resliced into 25 µm coronal sectionsforimmunohistochemistry.

Immunohistochemistry with monoclonal antibodies against Zebrin II (1:100; gift from R. Hawkes, University of Calgary, Alberta,Canada), the polysialylated form of neural cell adhesion molecule(PSA-NCAM)/5A5 (1:5; gift from J. Dodd, Columbia University, NewYork, NY), RC2 (1:1; Developmental Studies Hybridoma Bank, IowaCity, IA), TUJ-1 (1:500; Babco, Richmond, CA), CNPase (1:200;Sigma), and polyclonal antibodies against Dlx2 (1:200; gift fromJ. Rubenstein, University of California, San Francisco, CA), astrocyte-specificglutamate transporter (GLAST) (1:1000; Chemicon, Temecula, CA),and $beta$ -galactosidase ( $beta$ -gal) (1:1000; Cortex Biochemical, San Leandro,CA) was performed as follows. Cryosections were air-dried at roomtemperature, rinsed with PBS, and blocked in 5% normal goat serum,0.2% Triton X-100 in PBS for 1 hr before incubation in primaryantibodies diluted in blocking solution overnight at 4°C. Sectionswere washed the following day for 1 hr in PBS and incubated insecondary antibodies conjugated to FITC or tetramethylrhodamineisothiocyanate (TRITC) fluorochromes (Southern Biotechnology,Birmingham, AL) for 1-2 hr at room temperature. Selected sectionswere also rinsed in Syto-11 (1:10,000; Molecular Probes, Eugene,OR) to reveal nuclei before coverslipping in Gelmount (Biomeda,Foster City, CA). An antigen retrieval step was included for sectionsstained with the monoclonal antibodies to Zebrin II and CNPase:sections were incubated in 1 mM EDTA for 20 min at 65°C beforeblocking and the addition of primary antibody. A Zeiss laser scanningmicroscope (LSM) 510 confocal microscope and Zeiss LSM 510 imagingsoftware were used to capture fluorescent immunoreactivity andGFP expression data from cryosections and organotypicslices.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Zebrin II expression in the embryonic forebrain

The Zebrin II antibody recognizes Aldolase C, a CNS-specific isoform of fructose-1,6-diphosphate aldolase expressed in astrocytes,pia mater, Bergmann glia, and Purkinje cells of adult mammals,including humans (Thompson et al., 1982; Kumanishi et al., 1985;Ahn et al., 1994; Walther et al., 1998). Zebrin II expressionpatterns in the developing telencephalon had not been investigatedthoroughly until recently, when a partial sequence for ZebrinII was identified during a screen for genes highly expressed inthe perinatal SVZ (Staugaitis et al., 2001). Zebrin II expressionwas detected in the border regions of the dorsolateral SVZ atpostnatal day 5 (P5)-P7.

To begin characterizing the source of Zebrin II/Aldolase C-expressing SVZ border cells, we examined the patterns of embryonicZebrin II expression. Zebrin II is expressed by all cells of thepseudostratified telencephalic primordium (Fig. 1A,B). As neuroblastsmigrate from the VZ during midgestation (Angevine and Sidman,1961; Berry and Rogers, 1965; Rakic, 1974), they begin to express $beta$ -3-tubulin (TUJ-1) (Fig. 1C,D), a tubulin isoform specific toearly differentiating neurons (Lee et al., 1990). The expressionof neuronal markers is coincident with a downregulation of ZebrinII expression in the intermediate and marginal zones, as demonstratedby a temporal loss of immunoreactivity with the Zebrin II monoclonalantibody (Fig. 1E,F).

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Figure 1. Zebrin II is expressed by cells of the telencephalic primordium. A, B, Coronal sections (20 µm) of E10 cortical ventricular zone at the level of the septal nuclei show Zebrin II immunoreactivity (TRITC); Syto-11 (FITC) reveals nuclei and mitotic activity of Zebrin II+ cells at the surface of the lateral ventricle. C, D, Neuronal precursors coexpress Zebrin II (FITC) and TUJ-1 (TRITC) within the neuroepithelium at E10 and E12. E, F, TUJ-1+ neurons lose Zebrin II immunoreactivity after translocating or migrating from the ventricular zone at E14. Scale bars: B, 10 µm; D, 20 µm; F, 200 µm.

Progenitors originating in the embryonic VZ that are positive for the radial glial marker RC2 (Misson et al., 1988; Edwardset al., 1990) and the glutamate transporter GLAST (Rothstein etal., 1994; Furuta et al., 1997; Shibata et al., 1997) and possesslong radial glia-like processes are immunoreactive for ZebrinII regardless of nuclear position within the developing cerebrum(Fig. 2A,B). Brightly labeled Zebrin II+ radial glial end feetarborize at the pial surface of the developing cortex (Fig. 2C,D).Furthermore, process-bearing cells in the developing cortex andstriatum coexpress Zebrin II along with RC2, probably representingradial glia transforming into mature, stellate astrocytes (Missonet al., 1988; Voigt, 1989) (Fig. 2E,F). Zebrin II/Aldolase C expressionis specific to mature astrocytes in the forebrain (Thompson etal., 1982; Kumanishi et al., 1985; Ahn et al., 1994; Walther etal., 1998; Staugaitis et al., 2001). Hence, we infer that astrocytesoriginating directly from the neuroepithelium and indirectly viaa radial-glial phenotype maintain the expression of Zebrin IIduring differentiation.

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Figure 2. Zebrin II is expressed by glial progenitors regardless of nuclear position. A, B, Zebrin II+ cells (FITC) coexpress GLAST and RC2 (both TRITC) within the neuroepithelium at E12. C, D, Radial glial end feet coexpress Zebrin II (FITC) and GLAST (TRITC) at E14. E, F, Process-bearing cells within the developing cerebral cortex coexpress Zebrin II (FITC) and RC2 (TRITC) and demonstrate the morphology of differentiating astrocytes at P0. Scale bars: B, 20 µm; D, 10 µm; F, 40 µm.

Zebrin II-expressing VZ cells intermix with Dlx2-expressing cells at the corticostriatal boundary

As the LGE enlarges during midgestation (E12-E14), the pallial VZ "zippers up" (folds at an acute angle) during corticostriatalsulcus formation, generating a wedge-shaped zone of Zebrin II+VZ cells (Fig. 3A,D). During the subsequent perinatal week, thisarea undergoes a transformation such that Zebrin II-expressingcells become distributed at the medial, dorsal, and lateral peripheryof the SVZ, with a large number of Zebrin II-negative cells populatingthe central region (Staugaitis et al., 2001). We hypothesizedthat these Zebrin II-negative cells originate in more ventrallocations and migrate dorsally into the SVZ.

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Figure 3. The VZ zippers up at the corticostriatal boundary by E14. A, Fasciculating fibers emanate from Zebrin II+ (FITC) cells at the E14 lateral VZ. B, Dlx2 immunoreactive cells (FITC) are dispersed throughout the LGE and collect at the Zebrin II+ (TRITC) wedge of VZ at E16. C, By E19/P0, Dlx2+ cells (FITC) reside in the LGE, dorsolateral SVZ, and overlying white matter. D, The VZ zippers up, by folding at an acute angle during corticostriatal sulcus formation. Scale bars: A, B, 100 µm; C, 50 µm.

As one test of our hypothesis, we studied the position of Dlx2-expressing progenitors relative to the Zebrin II+ VZ cellsfrom midembryogenesis through postnatal stages. Dlx2-immunoreactivecells collected at the ventral aspect of the Zebrin II wedge byE14-E16 but did not themselves express Zebrin II (Fig. 3B). Arelative minority of Dlx2-expressing cells appeared to be scatteredwithin and just dorsal to the Zebrin II+ wedge by this time; however,a large majority of cells remained ventral to the wedge at E16.By E19/P0, Dlx2 expression was still found in the LGE but wasalso in central portions of the dorsolateral SVZ and in the overlyingwhite matter (Fig. 3C). Hence, Dlx2+ cells populated at leasta portion of the forming dorsolateral SVZ during perinatal development,corresponding precisely to the late, medial migration pathwaydescribed previously (Anderson et al., 2001).

Cells derived from Dlx2-expressing progenitors are positive for PSA-NCAM

Dlx2-expressing cells did not account for all of the Zebrin II-negative cells within the dorsolateral SVZ. Hence, we studiedthe expression pattern of molecular markers present within thedeveloping SVZ and examined the PSA-NCAM, for two reasons. First,PSA-NCAM is expressed by the majority of perinatal SVZ cells thatultimately differentiate into astrocytes and oligodendrocytesin vivo (Levison et al., 1993) and on transplantation from theadult SVZ into demyelinating lesion sites within the CNS (Keirsteadet al., 1999; Nait-Oumesmar et al., 1999). Second, PSA-NCAM expressionhas also been associated with migratory SVZ neuroblasts (Doetschand Alvarez-Buylla, 1996; Bruses and Rutishauser, 2001). We foundthat many PSA-NCAM-expressing cells also collected at the ventrallimit of the Zebrin II+ wedge by E14-E16 and, like the Dlx2+ cellsthat collected here, did not themselves express Zebrin II (Fig.4A-C). Many PSA-NCAM+ cells extended leading processes directeddorsally toward the cortex and possessed the simple unipolar orbipolar morphology common to migratory progenitors in this regionstudied previously with time-lapse microscopy (Fig. 4B,C) (Kakitaand Goldman, 1999). By P0, the central Zebrin II-negative regionof the SVZ was populated primarily by PSA-NCAM-positive cells(see below).

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Figure 4. PSA-NCAM+ cells are the progeny of Dlx2-expressing cells. By E16, PSA-NCAM-expressing cells also collect at the ventral aspect of the Zebrin II+ VZ wedge, the site of the nascent dorsolateral SVZ. A-C, Immunoreactivity for PSA-NCAM (TRITC) and Zebrin II (FITC) at the acute dorsolateral angle of the lateral ventricle. B, C, asterisk, The PSA-NCAM+ cell extends leading processes ventrodorsally. Dlx2/tauLacZ ( $beta$ -gal) labels PSA-NCAM+ progeny of Dlx2-expressing cells at the ventral aspect of the VZ. D-H, Immunoreactivity for $beta$ -galactosidase (TRITC) and PSA-NCAM (FITC) within the LGE at E16 (D-F) and forming dorsolateral SVZ at P0 (G-H). H, Enlargement of boxed area in G. Scale bars: B, 50 µm; E, G, 100 µm.

None of the PSA-NCAM-positive cells within the LGE and perinatal SVZ also expressed Dlx2. Hence, it was unclear whether thesetwo distinct populations shared common origins. Using a Dlx2/tauLacZknock-in mouse (Corbin et al., 2000), we performed a short-termin vivo lineage analysis of the Dlx2-expressing cell populationwithin the perinatal LGE and SVZ. Using antibodies to $beta$ -gal andPSA-NCAM, we found a large overlap in expression of the two markerswithin the LGE at E16 (Fig. 4D-F) and presumptive dorsolateralSVZ at P0 (Fig. 4G,H). Thus, cells that downregulated the Dlx2protein but retained the relatively stable tauLacZ ( $beta$ -gal) reporteralso expressed PSA-NCAM, demonstrating a direct lineage relationshipbetween the two cellpopulations.

Cells defined by Zebrin II or Dlx2/tauLacZ expression form the postnatal SVZ

Extensive cell proliferation and mixing during the perinatal week results in a heterogeneous assortment of postnatal SVZ cells;however, the complex mixture could be delineated by Zebrin IIand $beta$ -gal expression. The VZ wedge becomes fenestrated as cellsfrom ventral areas invade it, with the most dorsolateral ZebrinII+ cells becoming "displaced" from more medial VZ wedge cells.Analysis of the Zebrin II expression pattern at each day throughoutthe perinatal and early postnatal weeks reveals that the accumulationof these migrating cells progressively displaces the Zebrin II-positiveresidual neuroepithelium laterally (data not shown). This embryologicaldisplacement should not be confused with migration. We find noevidence suggesting that these wedge cells are migratory. Rather,the lateral wedge cells, which form the dorsolateral tip of theSVZ, appear to be relatively stationary. Stationary Zebrin II+SVZ border cells are characterized by "large polygonal cell bodieswith several fine processes," resembling the light border cellsdescribed previously by Smart (1961) (Staugaitis et al., 2001).These cells are morphologically and molecularly distinct fromthose displaying small, round cell bodies with dark nuclei andone or two fine processes that populate the central SVZ (Smart,1961). The central SVZ population was shown to be relatively moreproliferative and migratory than border cells and to be generallydevoid of Zebrin II mRNA and protein expression (Staugaitis etal., 2001).

The collection of Dlx2-expressing cells with their descendants, as defined by Dlx2/tauLacZ expression, constituted the vastmajority of Zebrin II-negative cells in the forming perinatalSVZ (Fig. 5A-C). By P6-P10, a $beta$ -gal+ subpopulation was positionedcentrally within the dorsolateral SVZ, whereas Zebrin II+ residualVZ cells formed its outer boundaries (Fig. 5D-I). $beta$ -gal+ cellsappear in the overlying white matter and cortex (Fig. 5D,F) (seebelow).

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Figure 5. Dlx2-expressing cells and their progeny, defined by Dlx2/tauLacZ ( $beta$ -gal) expression, intermix with Zebrin II+ VZ cells to form the dorsolateral SVZ. A-C, $beta$ -gal (TRITC)- and Zebrin II (FITC)-immunoreactive cells begin to mix perinatally. D-I, Postnatally, Zebrin II+ cells are displaced to form the outer limits of the SVZ, whereas $beta$ -gal+ cells constitute the Zebrin II $-$ central region at P6 (D-F) and P10 (G-I). Note that in A and D, $beta$ -gal+ cells also stream into the overlying white matter. Scale bars: B, 100 µm; E, 50 µm; H, 20 µm.

PSA-NCAM-expressing progenitors migrate ventrodorsally from the ganglionic eminences into the dorsolateral SVZ

The migratory behavior of Dlx2-expressing cells has been demonstrated previously (Anderson et al., 1997, 2001). The patternof PSA-NCAM expression within the ganglionic eminences and perinatalSVZ suggested that the PSA-NCAM+ population also invades the VZwedge during the formation of the perinatal SVZ. However, an assayof cell migration was necessary to demonstrate the dynamic invasionas opposed to a gradual expansion or ventrodorsal wave of PSA-NCAMexpression by cells within the developing SVZ. A retrovirus encodingthe cDNA for GFP was injected into the lateral and medial ganglioniceminences (merged LGE/MGE) of organotypic slices harvested fromembryos at E16. At E16, the LGE and MGE at the level of the septalnuclei are fused and cannot be targeted individually by retrovirallabeling strategies. Hence, we predict that our migration assaysincluded labeled cells from both the MGE and LGE. After 24 hr,slices were imaged to detect the location of GFP-expressing cellswithin the merged LGE/MGE structure (n = 16) (Fig. 6A,B). Sliceswere cultured up to 72 hr to allow migration to occur before beingfixed, cryoprotected, and resliced into thin sections for immunolabelingwith a monoclonal antibody to PSA-NCAM (n = 14). PSA-NCAM+, GFP-expressingcells were identified within the perinatal SVZ of each slice (Fig.6C-E), demonstrating the dorsal migratory nature of this populationof cells and their ability to invade the VZ wedge during the perinatalperiod. Therefore, two populations of cells, identified eitherby Dlx2 or PSA-NCAM protein expression, invade the Zebrin II+VZ wedge to form collectively the central dorsolateral SVZ.

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Figure 6. Migration assays in organotypic slice cultures confirm ventrodorsal migration of PSA-NCAM-expressing cells into the SVZ. A, Retrovirus was injected into the merged LGE/MGE of organotypic slices harvested from E16 telencephalon at the level of the septal nuclei. Asterisk, Site of injection. B, GFP expression by infected LGE/MGE cells after 24 hr in culture. B, inset, Cells migrate radially into the developing striatum and tangentially or ventrodorsally toward the VZ wedge. C-E, GFP-expressing cells that migrate into the dorsolateral SVZ show immunoreactivity for PSA-NCAM (TRITC) after 72 hr in culture. C, asterisk, Dorsolateral tip of the lateral ventricle. WM, White matter. Scale bars: A, 500 µm; B (inset), 300 µm; C-E, 50 µm.

Dlx2/tauLacZ defined cells give rise to astrocytes and oligodendrocytes in the dorsal telencephalon

To determine whether any of the $beta$ -gal+ cells migrated into the dorsal telencephalon to become glia, we looked for coexpressionof $beta$ -gal and glial markers. Indeed, $beta$ -gal+ cells within the striatum,white matter, and cortex developed into astrocytes and oligodendrocytes(Fig. 7). Some cells in white matter that possessed an immaturephenotype characteristic of migratory SVZ progenitors (Kakitaand Goldman, 1999) coexpressed $beta$ -gal and Zebrin II (Fig. 7A-C).We infer that these cells are early astrocytes, as Zebrin II-negativecells migrate from the central SVZ and initiate Zebrin II expressionalong with vimentin and glial fibrillary acidic protein (GFAP)as they differentiate into astrocytes (Staugaitis et al., 2001).Other $beta$ -gal+ cells exhibited a more differentiated astrocyticphenotype, coexpressing GFAP and associating with blood vessels(Fig. 7D-F). In addition, other $beta$ -gal+ cells developed the morphologicaland molecular phenotype of mature oligodendrocytes in the whitematter (Fig. 7G-I) and cortex (Fig. 7J-L). They possessed largesomas, long processes of uniform width that were oriented alongfiber tracts, and coexpressed the oligodendrocyte-specific enzymeCNPase.

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Figure 7. Subpallium-derived cells defined by Dlx2/tauLacZ reporter expression adopt mature glial phenotypes in the postnatal dorsal forebrain (P6-P10). A-C, Immature $beta$ -gal+ cells (TRITC) positioned within the corpus callosum coexpress Zebrin II (FITC). D-F, $beta$ -gal+ cells (FITC) exhibiting a more differentiated astrocytic phenotype coexpress GFAP (TRITC) and associate with blood vessels (note asterisk in F). $beta$ -gal+ cells coexpress CNPase and possess the morphology of mature oligodendroglia in the white matter (G-I) and cerebral cortex (J-L).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we identified the embryonic origins of two distinct populations of SVZ cells. Zebrin II+ residual ventricularzone cells form the borders of the SVZ. Cells sharing a Dlx2-expressing,subpallial origin migrate along a medial ventrodorsal pathwayto populate the central SVZ and give rise to astrocytes and oligodendrocytesin the developing cerebral cortex and white matter (Fig. 8, model).

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Figure 8. Formation of the postnatal SVZ. E10, Zebrin II is expressed by all cells of the telencephalic primordium. E14, A Zebrin II+ wedge emerges during corticostriatal sulcus formation. E16, E16 Box, The Zebrin II+ wedge is fenestrated by Dlx2+ or PSA-NCAM+ migratory, subpallium-derived cells. PSA-NCAM+ cells are the progeny of Dlx2+ cells. At P0, the total population of Dlx2-expressing cells and their PSA-NCAM+ progeny can be defined by Dlx2/tauLacZ ( $beta$ -gal) expression. Subpallium-derived cells defined by Dlx2/tauLacZ ( $beta$ -gal) expression form the central region of the perinatal SVZ. At P10 (and for the P10 box), the postnatal SVZ can be delineated into two subpopulations of cells based on the expression of Zebrin II or the Dlx2/tauLacZ reporter. Zebrin II+ residual VZ cells form the outer borders of the SVZ. Cells sharing a Dlx2-expressing subpallial origin, as defined by Dlx2/tauLacZ ( $beta$ -gal) expression, populate the central SVZ and give rise to astrocytes (astros) and oligodendrocytes (oligos) in the striatum, white matter, and cortex. Note: model is not drawn to scale.

Zebrin II: a novel marker for cells of the ventricular zone

Zebrin II is expressed uniformly throughout the dorsoventral axis of the telencephalon until E10, when differentiation ofthe basal forebrain and cerebral cortex begins (Fig. 8, E10) (Angevineand Sidman, 1961; Berry and Rogers, 1965; Rakic, 1974; Eisenstatet al., 1999; Wilson and Rubenstein, 2000). Zebrin II expressionappears to be a quality common to all telencephalic VZ cells,including neuroblasts and glioblasts, and does not appear to beregulated by the dorsoventral patterning genes Nkx2.1, Dlx1/2,or Pax6. For example, the pattern of Zebrin II expression is notdisrupted in Nkx2.1 or Dlx1/2 mutants (our unpublished observations);hence, it does not appear to be regulated by these transcriptionfactors. In small-eye (Sey) mice in which the Pax6 gene is disrupted,radial glia are not generated; hence, the overall number of dorsalVZ cells is diminished (Hill et al., 1991; Stoykova et al., 1996).However, Zebrin II is still expressed by remaining VZ cells (ourunpublishedobservations).

Origins of astrocytes

Two temporospatially distinct sources of astrocytes exist within the developing forebrain. Embryonically, astrocytes are generatedfrom the ventricular zone (Luskin et al., 1988; Price and Thurlow,1988) via a radial glial intermediate phenotype (Voigt, 1989).We argue that these astrocytes retain Zebrin II expression throughouttheir differentiation. The postnatal SVZ serves as another sourceof forebrain astrocytes (Smart, 1961; Lewis, 1968; Privat andLeblond, 1972; Paterson et al., 1973; Levison and Goldman, 1993;Luskin and McDermott, 1994), giving rise to a second class ofastrocyte precursor cell. These precursors emerge from ZebrinII-negative cells within the postnatal SVZ, initiate Zebrin IIexpression, and differentiate into mature astrocytes within thestriatum, white matter, and cortex (Staugaitis et al., 2001).Although astrocytes derived from both sources express GFAP andassociate with blood vessels, it is possible that they possessqualities making them distinct from one another. The comparisonof diverse classes among Zebrin II-expressing astrocytes may enableus to understand better the roles astrocytes serve in the normaland diseasedCNS.

Origins of oligodendrocytes

Recent work has described a ventral origin and specification of telencephalic oligodendrocytes during embryonic development(Woodruff et al., 2001). Before birth, progenitors isolated fromthe rat striatum have a much greater competence to generate oligodendrocytesin vitro than those harvested from cerebral cortex. However, progenitorsfrom the postnatal cerebral cortex have the potential to giverise to significant numbers of oligodendrocytes (Birling and Price,1998). One popular interpretation of this phenomenon is that alloligodendrocyte precursors are specified by Shh and migrate intothe dorsal telencephalon during the course of embryogenesis (Woodruffet al., 2001). This interpretation is based on studies in whicha gradient of DM-20, an alternatively spliced isoform of myelinproteolipid protein, and platelet-derived growth factor receptor- $alpha$ (PDGFR- $alpha$ ) expression emanates from the boundary separating theanterior hypothalamus and MGE and extends into the dorsal telencephalon(Pringle and Richardson, 1993; Spassky et al., 1998; Tekki-Kessariset al., 2001). The migratory nature of these DM-20+/PDGFR- $alpha$ + cellshas been inferred from the ability of oligodendrocyte precursorsin the optic nerve to migrate long distances (Ono et al., 1997)but has not been demonstrated directly. The ventrodorsal gradientof DM-20 and PDGFR- $alpha$ expression could represent the migrationof such cells or the acquisition of these markers by some precursorsduring the course of their migration. Alternatively, some cellsmight remain DM-20/PDGFR- $alpha$ -negative during migration and expressthese markers only once they have settled in the dorsal whitematter or cortex. Hence, some ventrally originating progenitors,which are competent to form oligodendrocytes but do not yet expresscommon oligodendrocyte-specific markers, may migrate dorsallyinto the forming dorsolateral SVZ. Regardless of the precise stageat which ventrally derived cells begin to express oligodendrocyte-specificmarkers, it is clear that gliogenesis is well under way throughoutthe developing cerebrum by the day of birth, with the peak ofoligodendrocyte and astrocyte generation occurring during thefirst 2 postnatalweeks.

We observed very little PDGFR- $alpha$ expression by cells migrating along a medial tangential pathway from the ganglionic eminenceor by cells within the dorsolateral SVZ itself (data not shown).However, a subset of cells that were retrovirally labeled withinthe SVZ and have migrated into the overlying white matter do beginto express PDGFR- $alpha$ , along with other markers thought to be specificto developing oligodendrocytes (J. Power, unpublished observations).This observation is consistent with previous work (Pringle etal., 1992) demonstrating a lack of PDGFR- $alpha$ expression by SVZ cellsand an upregulation of the receptor by cells within the surroundingparenchyma. Although PDGFR- $alpha$ expression may identify oligodendrocyteprecursors in the beginning stages of differentiation, the identificationof many migratory oligodendrocyte precursors could be more elusive.It is possible that ventrally originating cells become competentto give rise to oligodendrocytes by exposure to extrinsic patterningfactors such as Shh without committing to an oligodendrocyte lineageor necessarily expressing early oligodendrocyte markers such asDM-20 or PDGFR- $alpha$ . These "oligocompetent" cells may remain as multipotentprogenitors or glioblasts until they have migrated dorsally andestablished residence within the SVZ. Alternatively, extrinsicfactors within the postnatal SVZ, or even within the white matteror cortex, might serve to specify oligodendrocyteslocally.

We demonstrate that a population of cells derived from Dlx2-expressing cells within the ganglionic eminences migrates withinthe medial tangential pathway (Anderson et al., 2001) into thedorsolateral SVZ. Extensive study of the expression of patterninggenes in the developing forebrain led us to believe that cellsexpressing Dlx genes originate within the subpallium (Eisenstatet al., 1999; Puelles et al., 2000). The proportion of cells fromthis population that differentiate into glial cells rather thaninterneurons is unclear. We did not observe any cells that coexpressedDlx2 protein and oligodendrocyte-specific markers. We infer thatoligodendrocyte differentiation begins after Dlx2 protein expressionis downregulated by subpallium-derived precursors. Stable Dlx2-tauLacZreporter expression enabled us to trace the lineage of Dlx2-expressingcells into later stages that overlapped with oligodendrocyte differentiation.We observed Dlx2-tauLacZ ( $beta$ -gal) expression in a minority of glialcells in the white matter and cortex. As glioblasts proliferateduring migration, the $beta$ -gal reporter may become titrated in glialsublineages below levels detectable by immunohistochemistry. Thereporter might also become degraded before the expression of glia-specificmarkers by a large number of cells. Additional lineage analysesperformed in vivo are necessary to determine the lineal relationshipamong interneurons and glia within the Dlx2-expressing progenitorpopulation.

Cells within the white matter of the perinatal telencephalon were found to be coimmunoreactive for a pan-Dlx antibody andan antibody to the NG2 proteoglycan expressed by oligodendrocyteprecursors (He et al., 2001). These data suggest that these oligodendrocytescoexpress Dlx1/2 or Dlx5/6 and imply that they were derived fromDlx1/2-expressing LGE cells. However, a direct lineage relationshipwas not demonstrated in vivo. Our results show that subpallium-derivedDlx2-expressing cells and their progeny, as defined by Dlx2-tauLacZ( $beta$ -gal) expression, populate the central zone of the dorsolateralSVZ during the first postnatal week. Furthermore, we show thatthese cells give rise to oligodendrocytes and astrocytes in thedevelopingcerebrum.

Sublineages within the postnatal SVZ

The SVZ is composed of a heterogeneous mixture of cells from a variety of different lineages. Some SVZ cells become specifiedas astroblasts or oligodendroblasts (Levison and Goldman, 1993;Luskin and McDermott, 1994; Parnavelas, 1999). Others remain uncommittedas glioblasts until they migrate into the overlying parenchyma,where they diverge into lineages of astrocytes or oligodendrocytes(Levison et al., 1993) (M. Zerlin, unpublished observations).Many SVZ cells appear to commit to a neuronal lineage and takea rostral migratory route toward the olfactory bulb, where theygive rise to interneurons (Luskin, 1993; Lois and Alvarez-Buylla,1994). A subset of SVZ cells may remain multipotent. Clonal analysesof progenitors isolated from the LGE (He et al., 2001) and thepostnatal dorsolateral SVZ (Levison and Goldman, 1997) demonstratethe potential of many of these immature cells to give rise toboth neurons and glia in vitro. Hence, fate specification mayoccur within the SVZ or even after emigration from the SVZ. Invivo, instructive or permissive factors enable some precursorcells to migrate into the developing cerebrum, whereas othersremain within the SVZ. The extent to which a relationship existsbetween migration pathways and fate specification remains unknown.An understanding of the mechanisms behind telencephalic neuronal-glialspecification and the release of progenitors from the SVZ is essentialto better understand gliogenesis within the embryonic and postnatalforebrain.

  FOOTNOTES

Received June 11, 2002; revised Aug. 29, 2002; accepted Aug. 29, 2002.

This work was supported by National Institutes of Health Grant NS-17125 (J.E.G.). We thank Gord Fishell and Stewart Andersonfor offering insightful comments regarding this work. We alsothank Gord Fishell and Joshua Corbin for the generous gift ofDlx2/tauLacZ and Pax6 (Sey) mutant tissue, John Rubenstein andStewart Anderson for the generous gift of Dlx1/2 and Nkx2.1 mutanttissue, Carol Mason for graciously sharing imaging equipment,and Peter Canoll and Ana Milosevic for critically reading thismanuscript. Dritan Agalliu and Satoshi Suzuki extended adviceregarding slice cultures, and Theresa Swayne offered expert assistancewith confocalimaging.

Correspondence should be addressed to James E. Goldman, 630 West 168th Street, P&S Building, #15-420, New York, NY 10032.E-mail: jeg5{at}columbia.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ahn AH, Dziennis S, Hawkes R, Herrup K (1994) The cloning of zebrin II reveals its identity with aldolase C. Development 120:2081-2090[Abstract].
Anderson SA, Eisenstat DD, Shi L, Rubenstein JLR (1997) Interneuron migration from basal forebrain to neocortex: dependence on Dlx genes. Science 278:474-476[Abstract/Free Full Text].
Anderson SA, Marin O, Horn C, Jennings K, Rubenstein JLR (2001) Distinct cortical migrations from the medial and lateral ganglionic eminences. Development 128:353-363[Abstract].
Angevine Jr JB, Sidman RL (1961) Autoradiographic study of cell migration during histogenesis of cerebral cortex in the mouse. Nature 192:766-768[Medline].
Berry M, Rogers AW (1965) The migration of neuroblasts in the developing cerebral cortex. J Anat 99:691-709[ISI][Medline].
Birling MC, Price J (1998) A study of the potential of the embryonic rat telencephalon to generate oligodendrocytes. Dev Biol 193:100-113[ISI][Medline].
Bruses JL, Rutishauser U (2001) Roles, regulation, and mechanism of polysialic acid function during neural development. Biochimie 83:635-643[Medline].
Corbin JG, Gaiano N, Machold RP, Langston A, Fishell G (2000) The GSH2 homeodomain gene controls multiple aspects of telencephalic development. Development 127:5007-5020[Abstract].
Doetsch F, Alvarez-Buylla A (1996) Network of tangential pathways for neuronal migration in adult mammalian brain. Proc Natl Acad Sci USA 93:14895-14900[Abstract/Free Full Text].
Edwards MA, Yamamoto M, Caviness Jr VS (1990) Organization of radial glial and related cells in the developing murine CNS: an analysis based upon a new monoclonal antibody marker. Neuroscience 36:121-144[ISI][Medline].
Eisenstat DD, Liu JK, Mione M, Zhong W, Yu G, Anderson SA, Ghattas I, Puelles L, Rubenstein JLR (1999) Dlx-1, Dlx-2, and Dlx-5 expression define distinct stages of basal forebrain differentiation. J Comp Neurol 414:217-237[ISI][Medline].
Furuta A, Rothstein JD, Martin LJ (1997) Glutamate transporter protein subtypes are expressed differentially during rat CNS development. J Neurosci 17:8363-8375[Abstract/Free Full Text].
He W, Ingraham C, Rising L, Goderie S, Temple S (2001) Multipotent stem cells from the mouse basal forebrain contribute GABAergic neurons and oligodendrocytes to the cerebral cortex during embryogenesis. J Neurosci 21:8854-8862[Abstract/Free Full Text].
Hill RE, Favor J, Hogan BL, Ton CC, Saunders GF, Hanson IM, Prosser J, Jordan T, Hastie ND, van Heyningen V (1991) Mouse small eye results from mutations in a paired-like homeobox-containing gene. Nature 354:522-525[Medline].
Kakita A, Goldman JE (1999) Patterns and dynamics of SVZ cell migration in the postnatal forebrain: monitoring living progenitors in slice preparations. Neuron 23:461-472[ISI][Medline].
Keirstead HS, Ben-Hur T, Rogister B, O'Leary MT, Dubois-Dalcq M, Blakemore WF (1999) Polysialylated neural cell adhesion molecule-positive CNS precursors generate both oligodendrocytes and Schwann cells to remyelinate the CNS after transplantation. J Neurosci 19:7529-7536[Abstract/Free Full Text].
Kumanishi T, Watabe K, Washiyama K (1985) An immunohistochemical study of aldolase C in normal and neoplastic nervous tissues. Acta Neuropathol (Berl) 67:309-314[Medline].
Lee MK, Tuttle JB, Rebhun LI, Cleveland DW, Frankfurter A (1990) The expression and posttranslational modification of a neuron-specific beta-tubulin isotype during chick embryogenesis. Cell Motil Cytoskel 17:118-132[ISI][Medline].
Levison SW, Goldman JE (1993) Both oligodendrocytes and astrocytes develop from progenitors in the subventricular zone of postnatal rat forebrain. Neuron 10:201-212[ISI][Medline].
Levison SW, Goldman JE (1997) Multipotential and lineage restricted precursors coexist in the mammalian perinatal subventricular zone. J Neurosci Res 48:83-94[ISI][Medline].
Levison SW, Chuang C, Abramson BJ, Goldman JE (1993) The migrational patterns and developmental fates of glial precursors in the rat subventricular zone are temporally regulated. Development 119:611-622[Abstract].
Lewis PD (1968) The fate of the subependymal cell in the adult rat brain, with a note on the origin of microglia. Brain 91:721-738[Free Full Text].
Lois C, Alvarez-Buylla A (1994) Long-distance neuronal migration in the adult mammalian brain. Science 264:1145-1148[Abstract/Free Full Text].
Luskin MB (1993) Restricted proliferation and migration of postnatally generated neurons derived from the forebrain subventricular zone. Neuron 11:173-189[ISI][Medline].
Luskin MB, McDermott K (1994) Divergent lineages for oligodendrocytes and astrocytes originating in the neonatal forebrain subventricular zone. Glia 11:211-226[ISI][Medline].
Luskin MB, Pearlman AL, Sanes JR (1988) Cell lineage in the cerebral cortex of the mouse studied in vivo and in vitro with a recombinant retrovirus. Neuron 1:635-647[ISI][Medline].
Marin O, Rubenstein JLR (2001) A long, remarkable journey: tangential migration in the telencephalon. Nat Rev Neurosci 2:780-791[ISI][Medline].
Misson J-P, Edwards MA, Yamamoto M, Caviness Jr VS (1988) Identification of radial glial cells within the developing murine central nervous system: studies based upon a new immunohistochemical marker. Brain Res Dev Brain Res 44:95-108[Medline].
Nait-Oumesmar B, Decker L, Lachapelle F, Avellana-Adalid V, Bachelin C, Van Evercooren AB (1999) Progenitor cells of the adult mouse subventricular zone proliferate, migrate and differentiate into oligodendrocytes after demyelination. Eur J Neurosci 12:4357-4366.
Ono K, Yasui Y, Rutishauser U, Miller RH (1997) Focal ventricular origin and migration of oligodendrocyte precursors into the chick optic nerve. Neuron 19:283-292[ISI][Medline].
Parnavelas JG (1999) Glial cell lineages in the rat cerebral cortex. Exp Neurol 156:418-429[ISI][Medline].
Paterson JA, Privat A, Ling EA, Leblond CP (1973) Investigation of glial cells in semithin sections. III. Transformation of subependymal cells into glial cells as shown by radioautography after ³H-thymidine injection into the lateral ventricle of the brain of young rats. J Comp Neurol 149:83-102[ISI][Medline].
Price J, Thurlow L (1988) Cell lineage in the rat cerebral cortex: a study using retroviral-mediated gene transfer. Development 104:473-482[Abstract/Free Full Text].
Pringle NP, Richardson WD (1993) A singularity of PDGF alpha-receptor expression in the dorsoventral axis of the neural tube may define the origin of the oligodendrocyte lineage. Development 117:525-533[Abstract].
Pringle NP, Mudhar HS, Collarini EJ, Richardson WD (1992) PDGF receptors in the rat CNS: during late neurogenesis, PDGF alpha-receptor expression appears to be restricted to glial cells of the oligodendrocyte lineage. Development 115:535-551[Abstract].
Privat A, Leblond CP (1972) The subependymal layer and neighboring region in the brain of the young rat. J Comp Neurol 146:277-302[ISI][Medline].
Puelles L, Kuwana E, Puelles E, Bulfone A, Shimamura K, Keleher J, Smiga S, Rubenstein JLR (2000) Pallial and subpallial derivatives in the embryonic chick and mouse telencephalon, traced by the expression of the genes Dlx-2, Emx-1, Nkx-2.1, Pax-6, Tbr-1. J Comp Neurol 424:409-438[ISI][Medline].
Rakic P (1974) Neurons in rhesus monkey visual cortex: systemic relation between time of origin and eventual disposition. Science 183:425-427[Abstract/Free Full Text].
Rothstein JD, Martin LJ, Levey AI, Dykes-Hoberg M, Jin L, Wu D, Nash N, Kuncl RW (1994) Localization of neuronal and glial glutamate transporters. Neuron 13:713-725[ISI][Medline].
Shibata T, Yamada K, Watanabe M, Ikenaka K, Wada K, Tanaka K, Inoue Y (1997) Glutamate transporter GLAST is expressed in the radial glia-astrocyte lineage of developing mouse spinal cord. J Neurosci 17:9212-9219[Abstract/Free Full Text].
Smart I (1961) The subependymal layer of the mouse brain and its cell production as shown by radioautography after thymidine-³H injection. J Comp Neurol 116:325-347[ISI].
Spassky N, Goujet-Zalc C, Parmantier E, Olivier C, Martinez S, Ivanova A, Ikenaka K, Macklin W, Cerruti I, Zalc B, Thomas JL (1998) Multiple restricted origin of oligodendrocytes. J Neurosci 18:8331-8343[Abstract/Free Full Text].
Staugaitis SM, Zerlin M, Hawkes R, Levine JM, Goldman JE (2001) Aldolase C/Zebrin II expression in the neonatal rat forebrain reveals cellular heterogeneity within the subventricular zone and early astrocytes differentiation. J Neurosci 21:6195-6205[Abstract/Free Full Text].
Stoykova A, Fritsch R, Walther C, Gruss P (1996) Forebrain patterning defects in Small eye mutant mice. Development 122:3453-3465[Abstract].
Tekki-Kessaris N, Woodruff R, Hall AC, Gaffield W, Kimura S, Stiles CD, Rowitch DH, Richardson WD (2001) Hedgehog-dependent oligodendrocyte lineage specification in the telencephalon. Development 128:2545-2554[Abstract/Free Full Text].
Thompson RJ, Kynoch PAM, Willson VJC (1982) Cellular localization of aldolase C subunits in human brain. Brain Res 232:489-493[Medline].
Voigt T (1989) Development of glial cells in the cerebral wall of ferrets: direct tracing of their transformation from radial glia into astrocytes. J Comp Neurol 289:74-88[ISI][Medline].
Walther EU, Dichgans M, Maricich SM, Romito RR, Yang F, Dziennis S, Zackson S, Hawkes R, Herrup K (1998) Genomic sequences of aldolase C (Zebrin II) direct lacZ expression exclusively in non-neuronal cells of transgenic mice. Proc Natl Acad Sci USA 95:2615-2620[Abstract/Free Full Text].
Wilson SW, Rubenstein JLR (2000) Induction and dorsoventral patterning of the telencephalon. Neuron 28:641-651[ISI][Medline].
Woodruff R, Tekki-Kessaris N, Stiles CD, Rowitch DH, Richardson WD (2001) Oligodendrocyte development in the spinal cord and telencephalon: common themes and new perspectives. Int J Dev Neurosci 19:379-385[ISI][Medline].

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