N-CAM Binding Inhibits the Proliferation of Hippocampal Progenitor Cells and Promotes Their Differentiation to a Neuronal Phenotype

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The Journal of Neuroscience, May 15, 2000, 20(10):3631-3640

N-CAM Binding Inhibits the Proliferation of Hippocampal Progenitor Cells and Promotes Their Differentiation to a Neuronal Phenotype
Marie-Claude Amoureux¹, Bruce A. Cunningham¹, Gerald M. Edelman¹^,², and Kathryn L. Crossin¹
¹ Department of Neurobiology, The Scripps Research Institute, La Jolla, California 92037, and ² The Skaggs Institute for Chemical Biology, La Jolla, California 92037

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell adhesion molecules (CAMs) play important roles during the development of the nervous system. On the basis of our previousobservations that binding of the neural CAM (N-CAM) inhibits astrocyteproliferation and alters gene expression, we hypothesized thatN-CAM may influence the balance between the proliferation andthe differentiation of neural progenitor cells. Rat and mousehippocampal progenitor cells were cultured and showed dependenceon basic FGF for proliferation, immunoreactivity for nestin, thepresence of limited numbers of differentiated cells, and the abilityto generate glial cells and neurons under different culture conditions.Addition of soluble N-CAM reduced cell proliferation in a dose-dependentmanner with no evidence of apoptosis. The inhibition of proliferationby N-CAM was accompanied by an induction of differentiation tothe neuronal lineage, as indicated by a twofold increase in thepercentage of microtubule-associated protein 2-positive cellseven in the presence of mitogenic growth factors. Experimentsusing hippocampal cells from N-CAM knock-out mice indicated thatN-CAM on the cell surface is not required for these effects, suggestingthe existence of heterophilic signaling. These results supporta role for N-CAM and N-CAM ligands in the inhibition of proliferationand the induction of neural differentiation of hippocampal neuralprogenitorcells.

Key words: neural stem cells; progenitors; neural cell adhesion molecule (N-CAM); inhibition of proliferation; neuronal differentiation; N-CAM knock-out; N-CAM heterophile

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neural stem cells have been the object of increasing attention for their potential use in cell replacement or gene therapy(Pincus et al., 1998). Extensive neurogenesis occurs throughoutdevelopment, but only recently has it been demonstrated that theadult brain of vertebrates also contains a source of proliferativestem cells (Richards et al., 1992; Barnea and Nottebohm, 1996;Kempermann et al., 1997, 1998a,b; Palmer et al., 1997). Attemptsto define a neural stem cell have been made, but the lack of appropriatelyspecific markers and the pace of new discoveries (Doetsch et al.,1999; Johansson et al., 1999) leave only two unambiguous criteria:self-renewal and multipotentiality. Cells from different regionsof the CNS of primates and rodents have been isolated and shownto proliferate in the presence of growth factors (Reynolds andWeiss, 1992, 1996; Reynolds et al., 1992; Ray and Gage, 1994;Williams and Price, 1995; Gritti et al., 1996). The cells cangenerate cells of glial and neuronal lineages in vitro in thepresence of particular neurotrophic factors (Ahmed et al., 1995;Ghosh and Greenberg, 1995; Temple and Qian, 1995; Vicario-Abejonet al., 1995; Kahn et al., 1997; Williams et al., 1997; Arsenijevicand Weiss, 1998; Koblar et al., 1998; Zigova et al., 1998) orin vivo after transplantation (Chuah et al., 1991; Campbell etal., 1995; Craig et al., 1996; Carpenter et al., 1997; Winkleret al., 1998). The role of cell surface molecules other than receptorsfor neurotrophic factors and growth factors remains an importantsubject forstudy.

The neural cell adhesion molecule (N-CAM) is one of many CAMs and extracellular matrix (ECM) proteins that mediate cell interactionsand modulate developmental processes including neuronal migration,neurite extension, and gene expression. CAMs also participatein neural regeneration, neurite fasciculation, and synaptogenesisin the mature nervous system (for review, see Edelman and Crossin,1991; Lynch et al., 1991; Doherty and Walsh, 1996). N-CAM maybe important in neural stem cell biology on the basis of recentstudies of the rostral migratory pathway, in which neural stemcells migrate to populate the olfactory bulb. Polysialic acid(PSA), a large, negatively charged sugar moiety carried by N-CAMthat reduces its adhesive efficacy (Seki and Arai, 1991), N-CAM,and laminin are abundantly expressed along this pathway from thesubventricular zone to the olfactory bulb (Key and Akeson, 1991;Lois and Alvarez-Buylla, 1994; Lois et al., 1996; Thomas et al.,1996), suggesting that the place-dependent expression of thesemolecules may contribute to neural stem cell migration and differentiation.Indeed, the PSA-rich rostral migratory pathway has been proposedto promote neural stem cell migration to the olfactory bulb (Rousselotet al., 1995). Various N-CAM knock-out mouse models (Tomasiewiczet al., 1993; Cremer et al., 1994; Holst et al., 1998) and a PSA-depletedmouse model (Ono et al., 1994) present a similar phenotype thatincludes a reduced olfactory bulb, which has been attributed todecreased migration of the subventricular zone cells to theirtarget. PSA-N-CAM is also found in other areas where neural proliferationoccurs, such as the hippocampus (Seki and Arai, 1991), raisingthe possibility that the decreased membrane contacts in the presenceof PSA-N-CAM (Rutishauser et al., 1988; Acheson et al., 1991)are favorable toneurogenesis.

The involvement of neural CAMs in the control of neural stem cell proliferation and differentiation has not been studied directly.We reported previously that N-CAM binding inhibits astrocyte proliferationin vitro and in vivo after a lesion (Krushel et al., 1995, 1998;Sporns et al., 1995) and decreases the proliferation of otherN-CAM-expressing cell lines (Krushel et al., 1998). We hypothesizedthat N-CAM, acting in conjunction with growth factors, may playa role in influencing the balance between proliferation and differentiationof neural stem cells. The present study investigated the effectof N-CAM on hippocampal progenitor cell proliferation and differentiation.The findings suggest that N-CAM and its ligands play a role incontrolling the proliferation of neural progenitor cells and directingtheir differentiation toward a neuronallineage.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hippocampal progenitor cell culture. Hippocampi were dissected from embryonic day 17 (E17) to E18 rat embryos or E16 to E17mouse embryos into HBSS without calcium or magnesium and containingpenicillin (50 U/ml), streptomycin (100 µg/ml), and glutamine(2 mM) (Life Technologies, Gaithersburg, MD). The tissue was collectedby centrifugation for 2 min at 500 × g, and the buffer was removed.To dissociate the tissue into single cells, we incubated it for20 min at 37°C in 0.15% trypsin, 1 mM EDTA (Life Technologies),and 0.1 mg/ml DNase I (Sigma, St. Louis, MO). A mixture of HBSS,BSA (0.1%), trypsin inhibitor (0.025 mg/ml; Sigma), and DNaseI (0.1 mg/ml) was added before pelleting the tissue for 5 minat 500 × g. The dissociated tissue was incubated in this samemixture for 1 min and triturated with glass Pasteur pipettes ofnarrowing diameter. The resulting dissociated cells were centrifugedand resuspended in Neurobasal medium supplemented with penicillin,streptomycin, glutamine, and the synthetic mixture B27 (Life Technologies)(NB/B27), in the presence of 20 ng/ml basic FGF (bFGF; Sigma).The cells were plated on a poly-L-lysine and laminin substratefor proliferation as well as differentiationassays.

Preparation of N-CAM, extracellular N-CAM, and recombinant N-CAM domains. N-CAM was purified from early postnatal rat brainsor chicken brains as described previously (Hoffman et al., 1982;Sporns et al., 1995) and was shown to contain the polysialic acidcharacteristic of N-CAM from young brain tissue. ExtracellularN-CAM was obtained by digestion of chicken brain membranes withthe Staphylococcus aureus V8 protease as described previously(Cunningham et al., 1983) and subsequently subjected to immunoaffinitypurification using an antibody specific to the extracellular partof N-CAM. The various N-CAM recombinant proteins were producedin Escherichia coli and purified as reported previously (Ranheimet al., 1996).

Proliferation assay. Hippocampal cells were plated at a density of 20,000 cells/ml; 100 µl per well was seeded in 96-wellplates (Packard, Meridian, CT) coated with poly-L-lysine and laminin(Sigma). After 2 d in NB/B27 supplemented with 20 ng/ml bFGF,the cells were treated with various N-CAM protein reagents for48 hr. During the last 24 hr of this period, 5-bromo-2'-deoxyuridine(BrdU; 10 µM) was added. At the end of the 48 hr, cells were fixedin 4% paraformaldehyde (PFA) for 30 min. BrdU was quantified usingthe chemiluminescence cell proliferation ELISA-BrdU kit (BoehringerMannheim, Indianapolis, IN) according to the protocol providedby the manufacturer. In some experiments, cells were pretreated(1 hr) with heparin, heparinase, chondroitin sulfate, glycosidases[N-glycosidase endo F and O-glycosidase (Boehringer Mannheim)],or an anti-FGF receptor (Upstate Biotechnology, Lake Placid,NY).

Apoptosis assay. Hippocampal cells were plated at a density of 20,000 cells/ml on eight-chamber glass slides coated with poly-L-lysineand laminin in NB/B27 medium containing 20 ng/ml bFGF for 2 d(0.25 ml per well). After 48 hr of treatment with N-CAM (10 µg/ml),cells were fixed with 4% PFA (Sigma). The TUNEL assay was usedto assess apoptosis. Briefly, fragmented DNA was extended by theterminal deoxynucleotide transferase (250 U/ml; Boehringer Mannheim)that incorporated chromatide bodipy-FL-14-dUTP (5 µM; MolecularProbes, Eugene, OR). To reveal nuclear DNA, the cells were counterstainedwith 4,6-diamidino-2-phenylindole (DAPI) (Sigma) applied at 1µg/ml for 2 min at room temperature. The nuclei of healthy cells(blue) and the nuclei of apoptotic cells (green) were countedusing a fluorescencemicroscope.

Immunocytochemistry for BrdU, microtubule-associated protein 2, GFAP, and nestin. For all antibody staining, cells were fixedwith 4% PFA. For BrdU immunostaining, fixed cells were treatedfor 5 min with 0.05N NaOH. Nonspecific binding sites were blockedwith 5% goat serum in PBS, and the cells were permeabilized with1% Triton X-100 (Sigma). All steps were performed at room temperature.Nestin monoclonal antibody (PharMingen, San Diego, CA) and microtubule-associatedprotein 2 (MAP2) monoclonal antibody (Sigma) were diluted 1:1000.BrdU monoclonal antibody (Dako, Carpinteria, CA) was diluted 1:20.For GFAP staining, polyclonal anti-GFAP (Dako) was applied ata dilution of 1:2000. MAP2 and GFAP antibodies were applied simultaneously.Primary antibodies were incubated with the cells for 1 hr. Afterwashing three times for 10 min with 0.1% Triton X-100, the secondaryantibodies [Texas Red-anti-mouse for MAP2 (1:500) and FITC-anti-rabbitfor GFAP (1:500); both from Molecular Probes] were applied andincubated for 1 hr, and the slides were washed as described above.Nestin and BrdU antibodies were revealed using the biotin $---$ avidin-horseradishperoxidase vectastain system (Vector Laboratories, Burlingame,CA) and DAB in tablets as a substrate (Sigma). BrdU- and nestin-positivecells were observed in bright field. For MAP2 and GFAP labeling,cell nuclei were counterstained with DAPI, and the microscopeslides were mounted with Slowfade-mounting media (Molecular Probes)and observed by fluorescencemicroscopy.

Differentiation assay. Hippocampal cells were grown on poly-L-lysine- and laminin-coated eight-chamber glass slides (BectonDickinson, Bedford, MA) in NB/B27 medium in the presence of bFGF(20 ng/ml), at a density of 5000 cells per well for 4 d. At thattime, the medium was changed, and the cells were treated for 3additional days with N-CAM or with various N-CAM fragments, BDNF,neurotrophin-3 (NT-3), PDGF, insulin-like growth factor (IGF-I),CNTF, or FCS in NB/B27 with bFGF and at the concentrations indicatedin the figure legends. As a control, BDNF was also added in theabsence of bFGF to stimulate neuronal differentiation under theconditions reported previously (Vicario-Abejon et al., 1995).At the end of the seventh day, cells were fixed and processedfor MAP2 and GFAP immunocytochemistry as described above. Allthe cells were counterstained with DAPI to reveal cell nuclei.For each treatment, five fields were counted for total cells (DAPI),neuronal cells (MAP2⁺), and astrocytes (GFAP⁺). The results of the five fields were averaged and correspondedto a minimum number of 200 cells. The percentage of MAP2⁺ or GFAP⁺ cells was thencalculated.

Binding of N-CAM and N-CAM fragments in vitro to live progenitor cells from N-CAM knock-out mice. Hippocampal cells from N-CAMknock-out (KO) mouse embryos (Holst et al., 1998) were grown onpoly-L-lysine and laminin substrate in glass multichamber slides(Becton Dickinson) for 1-2 d in NB/B27 medium in the presenceof bFGF (20 ng/ml). They were treated with various N-CAM proteinreagents for 2 hr at 37°C. The cells were washed with PBS, fixedwith 4% PFA, and processed using immunocytochemistry for the bindingof N-CAM and N-CAM fragments. A rabbit polyclonal antibody directedagainst the extracellular domain of N-CAM that recognizes bothrat and chicken N-CAM (anti-N-CAM 527) was used at 3 µg/ml. Specificantibodies for each N-CAM domain were used at 10 µg/ml (Ranheimet al., 1996). The secondary antibody was an FITC-anti-rabbitantibody (Molecular Probes) (1:500). In some instances, cellswere pretreated (1 hr) with heparin, heparinase, chondroitin sulfate,or glycosidases (N-glycosidase endo F and O-glycosidase) (allfrom BoehringerMannheim).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Characterization of the rat hippocampal progenitor cell culture system

As described in the introductory remarks, several studies have provided culture conditions that support the growth and expansionof hippocampal neural progenitors. These conditions were adaptedfor the present study, and the resulting cultures were characterized.Four hours after plating rat hippocampal cells in bFGF-supplementedmedium, some cells either formed "neurospheres" in the absenceof a substrate that supported adhesion or formed colonies in thepresence of a substrate that supported adhesion. After 4 d ona poly-L-lysine and laminin substrate, the cells grew in loosecolonies of individually identifiable cells (Fig. 1A). At thistime, ~70% of the cells incorporated BrdU over 24 hr (Fig. 1B).bFGF or a combination of both epidermal growth factor (EGF) andbFGF supported cell proliferation, whereas EGF alone was an effectivebut less potent mitogen (data not shown). The cells were unipolaror bipolar with short extensions (Fig. 1A), and 95% of the cellsexpressed nestin, an intermediate filament protein present inneural stem cells and progenitors (Lendhal et al., 1990) (Fig.1C). These cells could be subcultured for up to 6 months in thepresence of bFGF.

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Figure 1. Characterization of primary E17-E18 rat hippocampal progenitor cells. A, Bright-field view of proliferating rat hippocampal cells cultured on poly-L-lysine- and laminin-coated substrates in NB/B27 medium in the presence of 20 ng/ml bFGF after 4 d in culture. B, C, BrdU incorporation (B) and immunolabeling (C) of the intermediate filament protein nestin. D, Phenotype of cells cultured for 4 d in NB/B27 + 20 ng/ml bFGF followed by 2 d of culture in the same medium without bFGF to stimulate differentiation. Cells were double-labeled for GFAP (FITC; green) and MAP2 (Texas Red; red) and counterstained with the nuclear stain DAPI (blue). Magnification: A, 10×; B $---$ D, 40×.

To stimulate differentiation, cells grown for 4 d in medium with bFGF were shifted to medium without bFGF and grown for anadditional 2 d. Following the convention established in otherstudies (Ghosh and Greenberg, 1995; Arsenijevic and Weiss, 1998),cells of the neuronal lineage were identified by MAP2 expression,and cells of the astrocyte lineage were identified by GFAP expression.Immunostaining for MAP2 and GFAP revealed many cells expressingeach differentiation marker (Fig. 1D; 25% GFAP⁺ and 70% MAP2⁺). S100 antibodies stained all GFAP⁺ cells and no others. Approximately 1% of the cells expressedthe oligodendrocyte marker 04 (data not shown). In the later-passagecells, cell phenotypes stimulated by growth factor removal werein approximately the same proportion as those in primary cultures.These observations suggest that the proliferating cells presentin the original culture correspond to multipotential neural progenitorcells.

Inhibition of rat progenitor cell proliferation by N-CAM and an extracellular N-CAM fragment

We found previously that N-CAM inhibited astrocyte proliferation in vitro and in vivo after a lesion and that the third immunoglobulindomain of N-CAM (Ig III) was effective at reducing astrocyte proliferation(Krushel et al., 1995, 1998; Sporns et al., 1995). We thereforeasked whether this effect occurred in other proliferative cellsof the nervous system, including neural progenitor cells, whichhave been demonstrated to express N-CAM (Rousselot et al., 1995;Mayer-Proschel et al., 1997) (M.-C. Amoreaux and K. L. Crossin,unpublished observations). Purified N-CAM inhibited neural progenitorcell proliferation stimulated by bFGF in a dose-dependent manner,reaching a maximum of 94% at a dose of 10 µg/ml (Fig. 2A). A concentrationof N-CAM > 1.25 µg/ml was necessary to obtain measurable inhibition,and the IC₅₀ was determined to be ~1.5 µg/ml. Preabsorption ofthe N-CAM solution with beads coated with monoclonal antibodyagainst N-CAM abolished the inhibitory activity (Fig. 2B), indicatingthat the effect was specifically caused by N-CAM. The inhibitoryactivity of N-CAM was also observed when N-CAM was coated ontothe dish in addition to the poly-lysine and/or laminin substrate(data not shown). N-CAM (10 µg/ml) could also inhibit EGF-stimulatedprogenitor proliferation by 72 ± 16%, indicating that the effectof N-CAM is not attributable to a particular mitogen. RecombinantN-CAM Ig III fragment and an extracellular fragment of nativeN-CAM purified from V8 protease-treated brain membranes (Cunninghamet al., 1983) were also tested in this assay (Fig. 2B). The nativeextracellular domain inhibited cell proliferation, whereas therecombinant Ig III domain did not. It was surprising that neitherIg III (Fig. 2B) nor an antibody against N-CAM (data not shown)inhibited proliferation, because both of these reagents were effectivein inhibiting astrocyte proliferation (Sporns et al., 1995; Krushelet al., 1998). In the absence of bFGF, BrdU incorporation wasvery low after 2 d and was unaffected by N-CAM treatment (datanot shown).

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Figure 2. Inhibition of rat hippocampal progenitor cell proliferation by N-CAM. A, Dose response of the effect of N-CAM on rat hippocampal progenitor cell proliferation measured by BrdU incorporation stimulated by 20 ng/ml bFGF. The values indicated on the graph represent the relative BrdU incorporation compared with that of untreated cultures. Values represent the average ± SD of a minimum of two experiments. B, BrdU incorporation stimulated by 20 ng/ml bFGF measured after treatment with N-CAM, the extracellular domain of N-CAM, the recombinant Ig III domain of N-CAM, or N-CAM preabsorbed on an N-CAM monoclonal antibody as described in Materials and Methods. The values are normalized to the BrdU incorporation in untreated cultures. Each value represents the average ± SEM of a minimum of three experiments (***p < 0.001; Student's t test).

N-CAM does not induce cell death

A possible explanation for the decrease in BrdU incorporation is that N-CAM reagents induced cell death. Indeed, a previousstudy suggested that N-CAM cross-linking induced by the applicationof an N-CAM antibody resulted in apoptosis of cortical neuronsin vitro (Azizeh et al., 1998). Apoptosis was measured by TUNELlabeling with fluorescent nucleotides with or without N-CAM treatmentfor 2 d (Fig. 3). The percentage of TUNEL-positive cells was measuredas a fraction of the total cells revealed by the DAPI nuclearstain. Few cells underwent apoptosis in either condition: 5.4%(± 4.6%) for untreated and 8.0% (± 3.0%) for N-CAM-treated cultures.Moreover, no pyknotic nuclei were observed in either condition.Therefore the large decrease in BrdU incorporation in the presenceof N-CAM could not be explained by an increase in cell death.

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Figure 3. Absence of apoptotic cell death after N-CAM treatment. Hippocampal cells were plated in NB/B27 with 20 ng/ml bFGF for 48 hr and treated for 2 additional days with 10 µg/ml N-CAM. Apoptosis was assessed using the TUNEL method as described in Materials and Methods. Green fluorescent nuclei correspond to apoptotic cells in which the terminal transferase has incorporated fluorescent dUTP (Bodipy-dUTP) into fragmented DNA. All the cells were counterstained with the nuclear stain DAPI shown in blue. A minimum of 10 independent fields was used to assess the percentage of apoptotic cells (see Results).

N-CAM binding leads to increased progenitor cell differentiation

Because proliferation was altered by N-CAM binding, we hypothesized that neural progenitor differentiation might also be affected.To address this possibility, we quantified the number of differentiatedcells by immunocytochemistry using antibodies to MAP2 and GFAP(see Fig. 1D). bFGF was maintained in the medium (NB/B27) to preservethe conditions under which N-CAM affected proliferation. WhenN-CAM was added (10 µg/ml) to rat hippocampal progenitor cells,~85% of the cells expressed MAP2, a 2.3 (± 0.3)-fold (n = 7) increaseover control cells. N-CAM treatment also resulted in a reductionin the number of GFAP-expressing cells from 12 to 2% of the totalcells (Fig. 4A). This effect on differentiation could not be mimickedwith any recombinant Ig N-CAM domains (Ig I-II, Ig III, Ig IV,or Ig V domains) applied at concentrations up to 50 µg/ml (datanot shown).

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Figure 4. Stimulation of differentiation of rat and mouse hippocampal neural progenitor cells toward a neuronal phenotype by N-CAM. A, Quantitation of differentiation of rat hippocampal progenitor cells. Cells were grown for 4 d on poly-L-lysine- and laminin-coated glass multichamber slides in NB/B27 media in the presence of bFGF alone (20 ng/ml) and then treated for 3 d with N-CAM (10 µg/ml) or left untreated. In each experiment, the number of MAP2⁺ cells and GFAP⁺ cells is shown as a percentage of the total number of cells. A minimum of 200 cells in five different fields per condition were counted. The values are expressed as the average ± SD from a representative experiment. B, Immunocytochemistry for MAP2 (Texas Red) and GFAP (FITC) showing N-CAM induction of MAP2⁺ cells and CNTF or FCS induction of GFAP⁺ cells in mouse progenitor cell culture after treatment for 3 d with N-CAM (10 µg/ml), CNTF (100 ng/ml), or FCS (10%). Cells were counterstained with DAPI.

To control for possible species differences in neural progenitors (Kempermann et al., 1998a) as well as to characterize amouse progenitor culture that could be used with cells from geneticallyaltered animals, we assessed the effect of N-CAM on the differentiationof mouse progenitor cells (Figs. 4B, 5). In medium supplementedwith bFGF, many cells were MAP2⁺ (~40%), but in contrast to rat progenitor cells cultured underidentical conditions, few mouse cells expressed GFAP (12% in ratvs 0.33% in mouse) (Figs. 4B, 5). However, in agreement with thefindings using rat cultures, N-CAM treatment significantly increasedthe percentage of MAP2⁺ cells (Figs. 4B, 5). Although N-CAM did not affect the percentageof astrocytes from mouse progenitor cell cultures (Fig. 5A), aGFAP⁺ population could be induced by the addition of CNTF or FCS (Figs.4B, 5A). In the mouse cultures, it is clear that the increaseof MAP2⁺ cells cannot be caused by an effect on astrocyte proliferation,because this number of GFAP⁺ cells was low and did not vary after treatment with N-CAM. Wheneither CNTF or FCS was added 2 d after N-CAM, the number of astrocytesincreased (78-fold by CNTF, from 0.33 to 26%, and 69-fold by FCS,from 0.33 to 23%), but the number of MAP2⁺ cells was the same as when N-CAM was added alone (data not shown).These findings suggest that MAP2⁺ cells induced by N-CAM did not dedifferentiate and that N-CAMand CNTF or FCS may act on separate populations. Together theexperiments on mouse and rat cultures indicate that N-CAM increasesthe differentiation of progenitor cells to a neuronal lineagein addition to its ability to reduce astrocyte proliferation.

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Figure 5. Comparison of the effect of N-CAM, BDNF, NT-3, IGF-I, PDGF, and CNTF on the differentiation of hippocampal progenitor cells. A, The protocol was exactly the same as that used in Figure 4. BDNF, NT-3, IGF-I, PDGF, and CNTF were used at 100 ng/ml, N-CAM was used at 10 µg/ml, and factors were added in the presence of bFGF (20 ng/ml) after 4 d of culture of mouse hippocampal progenitor cells (***p < 0.001; *p < 0.05; Student's t test). B, Cells were cultured for 4 d in the presence of bFGF, after which BDNF (100 ng/ml) or N-CAM (10 µg/ml) was added without bFGF and the cultures were grown for an additional 3 d. The counting was also done as described in Figure 4, and the values represent the average ± SD from a representative experiment (**p < 0.01; *p < 0.05; Student's t test).

Comparison of the effects of N-CAM and growth factors on the differentiation of mouse and rat hippocampal neural progenitor cells

The effect of N-CAM on the differentiation of hippocampal progenitor cells was compared with that of growth factors reportedto stimulate the differentiation of neural progenitor cells towardspecific lineages. In the presence of bFGF (Fig. 5A), the separateaddition of either BDNF, NT-3, PDGF, or IGF-I did not significantlyenhance neuronal differentiation of the hippocampal progenitorcells over that seen in untreated cultures, but N-CAM treatmentresulted in significant differentiation. In contrast, in the absenceof bFGF (Fig. 5B), the addition of BDNF alone increased the numberof MAP2⁺ cells, consistent with previous reports (Ahmed et al., 1995;Vicario-Abejon et al., 1995). Therefore, in the presence of themitogen bFGF, N-CAM is at least as potent an inducer of neuronaldifferentiation as the growth factors reported previously to affectstem cell differentiation in the absence ofbFGF.

N-CAM affects the proliferation and differentiation of progenitor cells lacking N-CAM

We investigated whether N-CAM homophilic binding was required for N-CAM to affect the proliferation and differentiation ofneural progenitor cells using cell cultures derived from micelacking N-CAM (Holst et al., 1998). Cells were prepared from E16to E17 heterozygous (+/ $-$ ) and homozygous ( $-$ / $-$ ) N-CAM KO mice.Cells from N-CAM +/ $-$ animals expressed N-CAM at their surface,whereas those from N-CAM $-$ / $-$ animals did not (data not shown),and cells from either origin incorporated BrdU after multiplepassages, indicating that they could be subcultured and remainproliferative. They were further characterized as describedbelow.

N-CAM and recombinant N-CAM fragments were added to the culture medium containing bFGF (20 ng/ml), and proliferation was measuredby BrdU incorporation. N-CAM strongly reduced the proliferationof progenitor cells derived from N-CAM +/ $-$ mice or N-CAM $-$ / $-$ mice(Fig. 6). N-CAM recombinant fragments (Fig. 6) or a polyclonalantibody against N-CAM (data not shown) had little effect, incontrast to studies on astrocytes in which N-CAM fragments andantibodies all reduced cell proliferation (Sporns et al., 1995;Krushel et al., 1998). N-CAM also effectively induced the differentiationof N-CAM KO hippocampal progenitor cells to the same extent asin N-CAM wild-type or rat cell cultures. The percentage of MAP2⁺ cells was increased from 18 ± 7.0 to 51 ± 7.5%. These data stronglysupport the involvement of a heterophilic ligand in the effectsof N-CAM on neural progenitor cell proliferation and differentiation.

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Figure 6. Inhibition of proliferation of hippocampal progenitor cells from N-CAM heterozygous (+/ $-$ ) and knock-out ( $-$ / $-$ ) mice. Neural progenitor cells were prepared from the hippocampi of N-CAM heterozygous (+/ $-$ ) or N-CAM knock-out ( $-$ / $-$ ) mice and incubated with 10 µg/ml N-CAM, Ig I-II, or Ig III, after 2 d in culture as described in Materials and Methods. BrdU incorporation was measured over the last 24 hr of treatment. Each value represents the average ± SEM of a minimum of three experiments (***p < 0.001; Student's t test).

Mechanism of action of N-CAM: evidence of a heterophilic ligand

To establish an assay for evaluating heterophilic binding, N-CAM and recombinant domains of N-CAM were allowed to bind tolive cells lacking N-CAM. The bound molecules were revealed afterfixation and detection with specific antibodies (Ranheim et al.,1996) (Fig. 7). N-CAM and the extracellular domain of N-CAM boundto the KO cells in vitro, whereas Ig III showed no binding (Fig.7). Preabsorption of the N-CAM solution with N-CAM antibodieslinked to beads removed the binding molecules (Fig. 7). The proteinswere revealed without permeabilization of the cells, indicatingthat they were bound to the cell surface. Addition of 0.02% sodiumazide, which blocks internalization processes, did not alter thepattern of N-CAM binding, further suggesting that N-CAM-positivestaining is located at the cell surface.

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Figure 7. Binding of N-CAM and extracellular N-CAM to live hippocampal progenitor cells from N-CAM knock-out mice. Cells were treated with N-CAM, the extracellular domain of N-CAM, and the recombinant Ig III domain (10 µg/ml) for 2 hr at 37°C. The cells were washed with PBS, fixed with 4% PFA, and processed for immunocytochemistry using antibodies for N-CAM and N-CAM domains and FITC-labeled secondary antibodies as described in Materials and Methods. Nuclei were revealed by counterstaining with DAPI.

Because heparin, heparan sulfate proteoglycans (HSPG), and chondroitin sulfate proteoglycans (CSPG) have been shown to interactwith N-CAM (Cole et al., 1986; Friedlander et al., 1994), heparinand chondroitin sulfate were tested as competitors for N-CAM bindingto the surface of live KO cells. Heparinase was also used to preventpossible interactions of exogenously added N-CAM with HSPG presenton the cell surface. Cells were preincubated with heparin, heparinase,or chondroitin sulfate before N-CAM treatment. None of the treatmentsprevented N-CAM binding (Fig. 8). Oligosaccharides were used totest whether carbohydrate binding was involved as has been suggestedfor N-CAM and L1 interactions (Horstkorte et al., 1993). Pretreatmentof N-CAM KO cells with N- and O-glycosidases had no effect onsubsequent N-CAM binding (Fig. 8).

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Figure 8. Saccharides and saccharide-modifying enzymes do not affect N-CAM binding to knock-out progenitor cells. Cells were pretreated (1 hr) with heparin (0.01 mg/ml), chondroitin sulfate (0.01 mg/ml), heparinase (0.01 U/ml), or glycosidases (4 U/ml; N-glycosidase endo F and O-glycosidase) and then treated with N-CAM (10 µg/ml) for 2 hr at 37°C. The cells were washed with PBS, fixed with 4% PFA, and processed for immunocytochemistry for N-CAM, as described in Materials and Methods.

To confirm that N-CAM was not interacting with heparin, HSPG, or CSPG to affect proliferation, the same reagents used in thebinding experiments were used in the proliferation assays (Fig.9). None of these molecules was able to reduce the inhibitoryactivity of N-CAM on progenitor cell proliferation (Fig. 9). Consistentwith the inability of heparin or heparan sulfate to affect proliferation,Ig I-II, which contains the Ig II domain responsible for the interactionof N-CAM with HSPG (Cole and Akeson, 1989), was inactive (Fig.6). These findings suggest that heparan sulfate or chondroitinsulfate proteoglycans or cell surface oligosaccharides were notinvolved in the binding of N-CAM to the cell surface, furthersupporting the presence of a novel N-CAM heterophile.

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Figure 9. N-CAM inhibitory activity on proliferation is not affected by known N-CAM heterophiles. The protocol was the same as that used in Figure 2, with N-CAM applied at 2 µg/ml. Cells were pretreated (1 hr) with heparin (0.01 mg/ml), chondroitin sulfate (0.01 mg/ml), heparinase (0.01 U/ml), anti-FGF receptor (1:200), or glycosidases (4 U/ml; N-glycosidase endo F and O-glycosidase). The values represent the BrdU incorporation in a representative experiment. Values are expressed as the average ± SD of a minimum of three measurements.

We also excluded the possibility that N-CAM could bind either of the mitogens bFGF or EGF and thereby influence cell proliferation.Preincubation of the culture medium with beads coated with N-CAMfollowed by treatment of the cells with the eluate showed no reductionin basal proliferation or in the ability of N-CAM to inhibit proliferation,suggesting that N-CAM was not interacting with and therefore depletingbFGF or EGF from the medium (data not shown). N-CAM has been reportedto interact with the FGF receptor (Williams et al., 1994; Dohertyand Walsh, 1996). An antibody against the FGF receptor that wasshown in these studies to block the N-CAM effect on neurite outgrowth(Williams et al., 1994; Doherty and Walsh, 1996) was used to testthe possible interaction of the FGF receptor with N-CAM. The applicationof the FGF receptor antibody alone reduced cell proliferationin a dose-dependent manner. When used at a concentration thatdid not dramatically affect proliferation but showed FGF receptorimmunostaining (data not shown), the inhibition of proliferationby N-CAM was not prevented by the addition of this FGF receptorantibody (Fig. 9).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have investigated the effect of N-CAM on neural progenitor cell proliferation and differentiation. In previous studies,we found that N-CAM affected the proliferation of astrocytes andNF- $kappa$ B signaling in both astrocytes and neurons. We therefore hypothesizedthat N-CAM might have a significant effect on neural progenitorcells. The studies reported here support this idea but indicatethat the mechanism of N-CAM action is significantly different.In astrocytes and neurons, N-CAM apparently can signal via N-CAMitself by a mechanism that is influenced by the first three Igdomains. Its effect on neuronal precursors, however, appears toinvolve signaling via an as yet unidentified heterophilic ligand.In the presence of either bFGF or EGF, both of which favor proliferationof neural progenitor cells, addition of N-CAM decreased cell proliferation.The inhibition of proliferation by N-CAM was not restricted tohippocampal progenitor cells but also occurred in neonatal cerebellarrat progenitor cell cultures and normal human neural progenitorcells (M.-C. Amoreaux and K. L. Crossin, unpublished observations).N-CAM binding to the surface of several neural cell types cantherefore inhibit theirproliferation.

In addition to inhibiting cell proliferation, N-CAM efficiently promoted neuronal differentiation in the presence of bFGF.Previous studies have shown that a variety of neurotrophins andgrowth factors, including BDNF, NT-3, CNTF, leukemia inhibitoryfactor, IGF-I, and PDGF, enhance neural stem cell differentiationafter bFGF removal (Ahmed et al., 1995; Ghosh and Greenberg, 1995;Temple and Qian, 1995; Vicario-Abejon et al., 1995; Kahn et al.,1997; Williams et al., 1997; Arsenijevic and Weiss, 1998; Koblaret al., 1998; Zigova et al., 1998). However, the present resultsdemonstrate that these factors had little effect in the presenceof bFGF, in contrast to the robust effect of N-CAM. One of thereported effects of neurotrophins is to decrease the amount ofapoptosis of cortical progenitors and to promote neuronal survivalin the absence of growth factors (Kirschenbaum and Goldman, 1995;Wade et al., 1999). Because little apoptosis was observed in thepresence of bFGF, the possible effects of N-CAM on cell survivalwere not measurable in our experimental paradigm. However, thepreviously reported ability of BDNF to enhance neural differentiationin the absence of bFGF was also observed in this study and mightreflect the survival-promoting activity of BDNF in the absenceof bFGF or the ability of BDNF to enhance differentiation (Ahmedet al., 1995). Moreover, it has been suggested that differentmitogens promote the proliferation or the survival of particularprogenitor populations (Lillien, 1998). In the case of N-CAM,a specific mitogen did not seem to be critical, because N-CAMinhibited both bFGF- and EGF-stimulated proliferation. Moreover,N-CAM was equally effective in promoting neuronal differentiationin the presence or absence of bFGF. These results indicate thatN-CAM did not achieve its effects on proliferation and differentiationby acting on a specific subpopulation of progenitors or by influencingparticular growth factor receptor signaling as reported in otherin vitro systems (Williams et al., 1994; Doherty and Walsh, 1996).

The increased number of MAP2⁺ cells stimulated by the presence of N-CAM could result from several mechanisms. It is likelythat N-CAM decreased the number of GFAP⁺ cells in rat cell culture at least partially because of its inhibitoryeffect on astrocyte proliferation as shown in previous studies(Sporns et al., 1995; Krushel et al., 1998), although it is possiblethat N-CAM treatment could have induced these cells to becomeMAP2⁺ neuroblasts as reported previously for subventricular zone GFAP⁺ stem cells (Doetsch et al., 1999). In any case, the increasein the number of MAP2⁺ cells induced by N-CAM in rat neural progenitors was much greaterthan could be accounted for simply by the decrease in GFAP⁺ cells. The use of mouse progenitor cells allowed us to verifythis conclusion unambiguously. Cultures of these cells displayedalmost no GFAP⁺ cells (0.33%) compared with that in rat hippocampal cells (12%)in the same culture conditions. The increase of MAP2⁺ cells after N-CAM treatment of mouse cells resulted thereforefrom the differentiation of MAP2/GFAP cells that were present. It is also unlikely that the increasein the ratio of MAP2⁺ cells could have been caused by a stimulation of the proliferationof the MAP2⁺ neuroblast population in view of the dramatic global inhibitoryeffect of N-CAM on proliferation. In addition, N-CAM did not stimulateproliferation in the absence of bFGF. It can therefore be concludedthat N-CAM acts on a stage in the differentiation process ratherthan by producing a secondary effect on MAP2⁺ or GFAP⁺cells.

The relationship between the inhibition of proliferation and the increase in differentiation observed here requires furtherstudy. There is no clear evidence that the two events, cell cyclearrest and differentiation, are interdependent in neural stemand progenitor cells, and indeed, evidence to the contrary exists.For example, the degree of primitivity of a stem cell seems notto be correlated with its mitotic properties. Some neural stemcells are mitotically quiescent, whereas others divide rapidly;intermediary progenitors proliferate faster than do pluripotentstem cells (Morrison et al., 1997). Interestingly, the same situationis true for hematopoietic stem cells, in which the most primitivestem cells are highly quiescent but can be maintained in long-termculture (Hao et al., 1996). In addition, even though a fractionof the neural stem cells of the subventricular zone undergoesapoptosis in vivo (Morshead and van der Kooy, 1992), many neuralstem cells remain quiescent and yet do not differentiate (Morsheadet al., 1994). It is probable that various cell cycle-controllingfactors are involved in a multistep manner to lead a cell to exitthe cell cycle and enter a differentiation program (Robertsonand Levitt, 1999; Scheffler et al., 1999). These observationsfurther support the idea that N-CAM may instructively induce progenitordifferentiation, independent of its effect onproliferation.

The present study raises the possibility that N-CAM is an endogenous regulator of progenitor cell proliferation and differentiation.Membrane-associated factors have been suggested previously toplay a role in the control of progenitor cell proliferation. Forexample, stem cells grown as neurospheres seem to proliferatefaster than the same cells plated on a substrate (Reynolds andWeiss, 1996). Other studies indicate that contact with some celltypes favors proliferation whereas interactions with other celltypes are inhibitory to proliferation (Temple and Davis, 1994).Removal of PSA from oligodendrocyte preprogenitors, which increasescell-cell interactions, has also been reported recently to increasethe differentiation of these cells (Nait-Oumesmar et al., 1999).Delta and Notch are also cell membrane proteins (ligand and receptor,respectively) that control progenitor differentiation. Their interactionprevents Notch-expressing cells from differentiating by inhibitingthe production of neurogenic transcriptional regulators (Ohtsukaet al., 1999). Whether an increase of neurogenic gene expressionin progenitor cells occurs after N-CAM binding remains to beinvestigated.

These results indicate that molecular signaling events underlying the cell-cell interaction mediated by N-CAM may participatein progenitor cell proliferation and differentiation. The mechanismby which N-CAM modulates neural differentiation remains to bedetermined. N-CAM may generate intracellular signals directlyby interacting with a heterophilic receptor or may perturb preexistingendogenous molecular interactions and thereby prevent rather thanmimic the normal signaling events generated by N-CAM interactions.It is possible that N-CAM activates the same intracellular pathwaysin progenitor cells as do the neurotrophins, which bind to theirtyrosine kinase receptors, the Trks (Lachyankar et al., 1997).Recent studies suggest that N-CAM signaling involves nonreceptortyrosine kinase activation (Beggs et al., 1997; Choi et al., 1999)and that this activation may influence multiple intracellularsignaling cascades. Because N-CAM counteracts the mitogenic effectsof bFGF (Ray and Gage, 1994; Gritti et al., 1996) (present results),it is also likely that N-CAM signal pathways alter signaling viathe FGF receptor, which has been reported to interact with N-CAMin other cellular systems (Doherty and Walsh, 1996). Such a mechanismof antagonism of growth factor receptor signals has been suggestedin previous studies (Ghosh and Greenberg, 1995). Distinct signalingpathways from N-CAM, Trks, and Notch may each influence the balancebetween stimulatory and inhibitory signals leading todifferentiation.

Identification of the ligand to which N-CAM binds to exert its effects on progenitor cells will help to define the mechanismof N-CAM action. Binding of N-CAM to live cells from N-CAM KOmice provides an assay to evaluate cellular extracts for suchheterophiles. Moreover, the tissue from knock-out animals providesan excellent source of protein to identify heterophiles withoutinterference from N-CAM homophilic binding. Possible heterophilicligands, such as membrane proteins, particularly homologs of N-CAMsuch as O-CAM (Schwob and Gottlieb, 1988; Yoshihara et al., 1997),basement membrane proteins, ECM proteins, the protein core ofproteoglycans, or new peptide ligands (Ronn et al., 1999), maybind exogenous N-CAM. However, we present evidence that the previouslyproposed heterophilic ligands for N-CAM, including the heparanor chondroitin sulfate part of proteoglycans or FGF receptorsat the cell surface (Cole et al., 1986; Friedlander et al., 1994;Williams et al., 1994; Doherty and Walsh, 1996), are not the ligandsby which N-CAM alters progenitor cell proliferation ordifferentiation.

Whether N-CAM binding affects the genesis or differentiation of neural progenitors in vivo is of critical interest, and resolutionof this issue may suggest mechanisms of controlling stem cellstates during development and in adult animals after transplantation.PSA-N-CAM is present endogenously in neurogenic regions, suchas the hippocampus (Seki and Arai, 1991) and subventricular zone(Key and Akeson, 1991; Thomas et al., 1996). Limited cell-cellinteractions because of the presence of PSA-N-CAM could, in concertwith growth factors, control neural progenitor cell proliferationand differentiation. The specific spatiotemporal distributionof N-CAM and N-CAM ligands may turn out to represent significantfactors in the genesis of cells of the nervoussystem.

  FOOTNOTES

Received Dec. 28, 1999; revised Feb. 23, 2000; accepted March 1, 2000.

This work was supported by United States Public Health Service Grants HD 16550 and HD 09635, a grant from the Mathers Foundation,and support from The Skaggs Institute for Chemical Biology. Wethank Drs. Frederick S. Jones, Leslie A. Krushel, Joseph A. Gally,and Ralph J. Greenspan for critical comments on this manuscriptand Ms. Anna M. Tran and Ms. Elizabeth L. Kao for their excellenttechnical assistance. Drs. Bruce A. Cunningham and Kathryn L.Crossin are consultants to BectonDickinson.
Correspondence should be addressed to Dr. Kathryn L. Crossin, Department of Neurobiology, The Scripps Research Institute,10550 North Torrey Pines Road, SBR-14, La Jolla, CA 92037. E-mail:kcrossin{at}scripps.edu.

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