Fibroblast Growth Factor 2 (FGF-2) Promotes Acquisition of Epidermal Growth Factor (EGF) Responsiveness in Mouse Striatal Precursor Cells: Identification of Neural Precursors Responding to both EGF and FGF-2

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The Journal of Neuroscience, October 1, 1998, 18(19):7869-7880

Fibroblast Growth Factor 2 (FGF-2) Promotes Acquisition of Epidermal Growth Factor (EGF) Responsiveness in Mouse Striatal Precursor Cells: Identification of Neural Precursors Responding to both EGF and FGF-2
Francesca Ciccolini¹^,² and Clive N. Svendsen¹
¹ Medical Research Council Cambridge Centre for Brain Repair, Cambridge CB2 2PY, England, and ² Medical Research Council Laboratory of Molecular Biology, Cambridge CB2 2QH, England

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Epidermal growth factor (EGF) and fibroblast growth factor 2 (FGF-2) induce the proliferation of neural precursor cells isolatedfrom specific regions of the embryonic and adult brain. However,the lineage relationship between the EGF- and FGF-2-responsivecells is unknown. In this study we used phosphorylation of thetranscription factor cAMP response element-binding protein asa functional readout to identify cells responding to EGF and FGF-2.In primary cultures of mouse embryonic day 14 (E14) striatum,maintained in vitro for 24 hr, 12% of the cells responded to FGF-2,whereas no response to EGF could be detected. Seventy-five percentof these FGF-2-responsive cells were $beta$ tubulin III (TuJ1)-positiveneurons, and 25% expressed nestin, a marker for neuroepithelialprecursors. After growth factor treatment for 6 d, a populationof nestin-positive cells responding to both EGF and FGF-2 wereidentified. The 6-d-old cultures also contained a small numberof TuJ1-positive cells that responded to FGF-2 only. Priming ofstriatal cells for 24 hr with FGF-2 but not with EGF was sufficientto induce the appearance of EGF- and FGF-2 responsive cells afteronly 2 d in vitro. Thus, neural precursor cells from the mouseE14 striatum initially responding to FGF-2 only acquire EGF responsivenesslater during in vitro development. At this stage EGF and FGF-2act on the same cells. The acquisition of EGF responsiveness ispromoted by FGF-2.

Key words: stem cells; progenitors; growth factors; CREB phosphorylation; embryonic brain; neural development

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The discovery of neural precursors with the ability both to self-renew and to generate progenitors for neurons, astrocytes,and oligodendrocytes in vitro (Cattaneo and McKay, 1991; Reynoldsand Weiss, 1992; Temple and Davis, 1994) provides a powerful modelfor examining cellular mechanisms underlying the development ofthe CNS. Neural precursors could also provide a source of tissuefor clinical transplantation programs that may in the future leadto novel therapeutic approaches for treating neuronal loss associatedwith neurodegenerative conditions such as Parkinson's and Huntington'sdiseases (Lindvall, 1997; Svendsen, 1997).

A number of growth factors support the proliferation of neural precursor cells and the differentiation of their progenitors.In particular, epidermal growth factor (EGF) and fibroblast growthfactor 2 (FGF-2) have been found to stimulate the division ofembryonic or adult CNS precursors (for review, see Gage et al.,1995; Kilpatrick et al., 1995; McKay, 1997; Weiss et al., 1996).However, their relative importance in inducing a mitogenic responseis controversial. EGF has been shown to induce the proliferationof multipotent precursor cells from either embryonic or adultmouse striatum, leading to formation of cell clusters termed neurospheres(Reynolds and Weiss, 1992; Reynolds et al., 1992), whereas FGF-2may act on lineage-restricted progenitors present in these EGF-generatedneurospheres (Vescovi et al., 1993). Other studies, however, haveshown that FGF-2 can also induce the proliferation of multipotentprecursor cells from adult striatum (Gritti et al., 1996), spinalcord (Weiss et al., 1996a; Shihabuddin et al., 1997), or bothadult and embryonic hippocampus and embryonic cortex (Gensburgeret al., 1987; Ray et al., 1993; Johe et al., 1996; Qian et al.,1997). These studies could indicate the existence of a distinctpopulation of multipotent precursor cells responding to eitherEGF or FGF-2. Alternatively, it is possible that these cells respondto both EGF and FGF-2 and that their proliferative response toeither growth factor depends on experimental conditions.

To investigate whether EGF and FGF-2 act on the same or distinct cell populations and to analyze the lineage relationshipbetween growth factor-responsive cells, we characterized individualEGF- and FGF-2-responsive cells derived from mouse embryonic day14 (E14) striatum. Because it has been difficult to assess growthfactor receptor expression in individual cells, we have developeda new approach to functionally detect cells responding to EGFor FGF-2. Both growth factor receptors act on classical receptortyrosine kinases that induce the activation of the Ras/extracellularsignal-regulated kinase (ERK) pathway (Marshall, 1995). One wellcharacterized intracellular consequence of this event is the phosphorylationof the transcription factor cAMP response element-binding protein(CREB) on serine 133 (Ginty et al., 1994; Xing et al., 1996).This phosphorylation can be detected immunocytochemically usingan antibody that specifically recognizes the phosphorylated formof CREB (phospho-CREB) (Ginty et al., 1993). In this study CREBphosphorylation was used as a functional readout for EGF and FGF-2cell responsiveness and was combined with the characterizationof the cellular phenotype in double-immunostaining experimentsusing antibodies to either nestin, as a marker for precursor cells,or TuJ1, as a marker for neurons.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Culture of primary embryonic striatal cells. Striata from E14 CD1 albino mouse embryos (plug day = 1.0) (Charles River Laboratories,Wilmington, MA) were dissected and transferred into ice-cold culturemedium consisting of: DMEM/F12 (1:1; Life Technologies, CostaMesa, CA), glucose (0.6%), glutamine (2 mM), NaHCO₃ (3 mM), HEPESbuffer (5 mM) (all from Sigma, St. Louis, MO), and 2% B27 supplement(Life Technologies). The tissue was gently triturated with a fire-polishedPasteur pipette, and 10⁶ cells were plated at a density of 200,000 cells/ml in Corning(Corning, NY) T25 culture flasks or Nunc (Naperville, IL) four-welldishes in the above culture medium in the presence of EGF (Sigma)and/or FGF-2 (R & D Systems, Minneapolis, MN) at a concentrationof 20 ng/ml each. Half of the medium was replaced every 3 d withfresh medium containing the same concentration of growth factors.After 6 or 7 d, neurospheres were collected by centrifugation,resuspended in fresh medium, and triturated with a fire-polishedPasteur pipette as described above. This procedure gave rise toa mixture of single cells and small neurospheres. The number ofviable cells in each culture was determined by the trypan blueexclusion technique.

To assess the effects of the different growth factor treatments on the size and number of neurospheres, mouse E14 striatalcells were plated onto 24 well plates (Nunc; 100,000 cells perwell) and grown for 6 d in culture medium containing growth factorsas described above. For each growth factor condition the totalnumber of neurospheres, categorized into small, medium, and largesize, was determined.

Antibodies. The following antibodies were used at the indicated dilution: mouse monoclonal antibody to nestin (PharMingen,San Diego, CA; 1:1000); mouse monoclonal antibody to $beta$ -tubulintype III (TuJ1; Sigma; 1:1000); mouse monoclonal antibody to galactocerebrocidase (Gal-C; a gift from Dr. Neil Scolding, NeurologyUnit, Cambridge University, England; 1:30); rabbit polyclonalantibody to glial fibrillary acidic protein (GFAP; Dako, HighWycombe, UK; 1:500); rabbit polyclonal antibody to CREB phosphorylatedon serine 133 (Upstate Biotechnology, Lake Placid, NY; 1:1500),and mouse monoclonal antibody to bromodeoxyuridine (BrdU) (BoehringerMannheim, Indianapolis, IN; 1:10).

Differentiation of the neurospheres. Mouse E14 striatal cells were grown for 6-7 d in the presence of EGF and/or FGF-2. Fromeach culture 30-50 neurospheres were collected, rinsed in culturemedium, and resuspended in culture medium containing 1% fetalcalf serum (FCS). Cells were plated onto poly-L-lysine-laminin-coatedchamber slides (Nunc), and their phenotype was determined immunocytochemicallyafter 14 d using antibodies to TuJ1, GFAP, and Gal-C.

Growth factor stimulation. Striatal cells were plated (50,000 cells/cm²) either immediately after dissection or after 6 d of growth invitro in the presence of EGF and/or FGF-2 onto poly-L-lysine-laminin-coatedchamber slides (Nunc) in culture medium without EGF and FGF-2.Cells were stimulated 24 hr after plating with EGF or FGF-2 (20ng/ml each) or with a combination of both growth factors (20 ng/mleach). In some experiments a higher growth factor concentration(40 ng/ml each) was used, which gave identical results. Cellswere fixed after 7 min and processed for immunocytochemistry.

To analyze the effects of 24 hr growth factor starvation and growth on a poly-L-lysine-laminin substrate on striatal cellproliferation, cells were plated immediately after dissectiononto poly-L-lysine-laminin-coated four-well plates (Nunc; 100,000cells per well). For each growth factor condition (EGF and/orFGF-2) two sets of cultures were established and compared: culturesto which growth factors were added at the time of plating andcultures to which growth factors were added 24 hr after plating.After 5-6 d, clusters of growing cells were counted, and after7 d, cells were incubated with 0.025% trypsin (Sigma) for 5 min,followed by addition of 10% FCS, and the total number of viablecells was determined.

Measurement of BrdU incorporation. The rate of BrdU incorporation was determined by adding 10 µM BrdU (Boehringer Mannheim)to cultures of striatal cells grown for 1, 3, and 6 d either inthe presence of EGF and/or FGF-2 (20 ng per ml each) or in theabsence of exogenous growth factors. One hour after BrdU additioncells were collected, washed twice with culture medium, resuspendedin culture medium, and plated onto poly-L-lysine-laminin-coatedchamber slides (Nunc). Twenty minutes after plating cells werefixed and processed for immunocytochemistry. For BrdU-phospho-CREBdouble-immunostaining experiments, striatal cells grown for 6d in growth factor-containing culture medium were collected bycentrifugation and plated onto poly-L-lysine-laminin-coated chamberslides in culture medium (without exogenous growth factors) containing10 µM BrdU. After 24 hr cells were stimulated with growth factorsand processed for immunocytochemistry using the phospho-CREB andBrdU antibodies.

Immunocytochemistry. Cells were fixed in 4% paraformaldehyde in PBS containing 4% sucrose for 10 min, washed several timesin PBS, permeabilized in NP-40 (0.05% in PBS) for 5 min, and blockedin goat serum (1.5% in PBS) for 30 min, all done at room temperature.Gal-C immunostaining was performed as described above, exceptthat the cells were fixed for 20 min in ice-cold methanol. Afterfixing the cells were incubated with primary antibodies overnightat 4°C. FITC-labeled secondary antibodies were used to visualizethe signal. In double-immunostaining experiments, primary rabbitpolyclonal antibodies were detected using a biotin-conjugatedgoat anti-rabbit secondary antibody and Cy3-conjugated streptavidin(Vector Laboratories, Burlingame, CA); primary mouse monoclonalantibodies were detected using FITC-conjugated goat anti-mouseantibody (Vector).

Cell counts and statistical analysis. To determine the number of growth factor-responsive cells, photographs of immunostainedcells were taken using a high-resolution digital camera (Nikon).The number of cells showing nuclear phospho-CREB immunoreactivitywas determined by counting the immunopositive and the total numberof cells in four visual fields (100-400 cells per field). Forantigens other than CREB, immunopositive cells were counted infour to seven visual fields (100-200 cells per field). The meansand SEs of at least three independent experiments were calculated,and statistical significance test (ANOVA with post hoc Newman-Keuls)analyses were performed using a statistical package (Graphpad,Prism).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

EGF and FGF-2 have distinct biological effects on cultures of mouse embryonic striatal cells

Primary mouse E14 striatal precursor cells were grown in the presence of EGF and/or FGF-2 for 7 d, leading to the formationof neurospheres. The size and the number of neurospheres obtainedwere dependent on the growth factor added: EGF treatment gaverise to fewer and smaller neurospheres when compared with FGF-2and EGF plus FGF-2 treatment (Fig. 1A-D, Table 1). No neurosphereswere found in control cultures grown in the absence of exogenousgrowth factor. Analysis of the total number of cells obtainedfrom 7-d-old neurosphere cultures revealed the smallest cell numberin EGF-treated cultures and an intermediate number with FGF-2,whereas EGF plus FGF-2 had a synergistic effect on growth andproduced the highest number of cells (Fig. 1E). We next determinedthe rate of BrdU incorporation in control and growth factor-treatedcultures after 1, 3, and 6 d in vitro. One-day-old striatal culturesshowed a similar rate of BrdU incorporation irrespective of thegrowth factor conditions (Fig. 1F). After 3 d in vitro, culturesgrown in the presence of FGF-2 and EGF plus FGF-2 contained significantlymore dividing cells than EGF-treated and control cultures (Fig.1G). After 6 d in vitro the same percentage of BrdU-labeled cellswas found in all growth factor-treated cultures, whereas veryfew cells incorporated BrdU in control cultures (Fig. 1H). However,because cultures grown in EGF contained significantly less cellsthan those treated with FGF-2 and EGF plus FGF-2 (Fig. 1E), EGFtreatment actually gave rise to approximately three to five timesless BrdU-labeled cells than the other growth factor conditions.In addition, at each time point analyzed and in all growth factorconditions all the BrdU-immunopositive cells expressed nestina marker for neuroepithelial precursors (data not shown).

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Figure 1. Effects of different growth factor conditions on mouse E14 striatal cells. A-D, Photographs of neurospheres present in cultures grown for 7 d without EGF and FGF-2 (A) or in the presence of EGF (B), FGF-2 (C), or EGF plus FGF-2 (D). E, Number of viable cells in cultures of striatal cells grown as neurospheres for 7 d in the presence of the indicated growth factors. Data represent the means of seven independent experiments. F-H, Rate of BrdU incorporation in striatal cells grown in vitro for 1 (F), 3 (G), and 6 (H) d in the presence of the indicated growth factors. Data represent the means of four different experiments. E, ^#Significantly different from EGF and FGF (p < 0.001). G, *Significantly different from EGF and control (p < 0.001).


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Table 1. Effects of growth factor treatment on size and number of neurospheres

Because these cultures represent a heterogeneous population of cells at different stages of neuronal and glial development,we next determined their phenotype immunocytochemically usingantibodies to different marker proteins. These markers were nestin,TuJ1 (neurons), GFAP (astrocytes), and Gal-C (oligodendrocytes).Analysis of the cells 24 hr after striatum dissection revealedthat the majority of the cells were either nestin-positive (nestin⁺) or TuJ1 positive (TuJ1⁺), whereas very few cells expressed GFAP or Gal-C (Table 2).In cultures grown for 7 d in the presence of either EGF or EGFplus FGF-2 and analyzed 24 hr after dissociation of the neurospheresand plating, the majority of cells were nestin⁺, whereas only a small percentage expressed TuJ1 (Table 2). Thepercentage of TuJ1⁺ cells in cultures grown for 7 d in FGF-2 was significantly higherthan in cultures grown in either EGF or EGF plus FGF-2 (Table2; p < 0.001). However, when absolute numbers of TuJ1⁺ cells were compared, the difference was significant only betweenEGF and FGF-2 grown cultures. The glial cell content of 7-d-oldcultures was small (<1% of the cells were Gal-C-positive cells;no detectable GFAP staining) (Table 2). Approximately 25% ofthe cells did not stain with any of the antibodies used irrespectiveof the growth factor treatment. Terminal deoxynucleotidyl transferase-mediatedbiotinylated UTP nick end-labeling staining indicated that thesecells may have been undergoing apoptotic cell death (data notshown). Differentiation of the cells derived from 6- to 7-d-oldcultures gave rise to a percentage of neurons and glial cellsthat did not vary with the growth factor conditions used duringthe first week in vitro (Table 2). These results demonstratethat nestin⁺ precursor cells and TuJ1⁺ neurons are the two main cell types found in cultures of mouseE14 striatum grown for 7 d in EGF and/or FGF-2. These differencesin proliferative responses, and in the relative abundance of precursorcells and neurons, indicate that EGF and FGF-2 have distinct biologicaleffects on these cells. To investigate whether this reflects theexistence of distinct subsets of cells differentially respondingto either growth factor, we next analyzed EGF and FGF-2 responsivenessat the single-cell level.


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Table 2. Effects of growth factor conditions on expression of differentiation markers in E14 striatal cells

Striatal precursor cells respond to FGF-2 but not to EGF at early stages of in vitro development

Binding of EGF and FGF-2 to their receptors activates the Ras/ERK signaling cascade culminating in the phosphorylation ofthe transcription factor CREB on serine 133 (Ginty et al., 1994;Xing et al., 1996). We used an antibody specific for CREB phosphorylatedon serine 133 (Ginty et al., 1993) to identify individual cellsresponding to EGF (E^res), FGF-2 (F^res), and both EGF and FGF-2 (E/F^res). Because CREB phosphorylation induced with growth factor stimulationwas analyzed in cells grown attached to a substrate for 24 hrin the absence of EGF and FGF-2, we first investigated whetherthis procedure affected proliferation or differentiation. We comparedthe growth factor-induced proliferative response in sister culturesexposed to the exogenous growth factors either immediately or24 hr after plating (for details see Materials and Methods). After7 d of culturing no significant differences were found in eitherthe total numbers of cells or the numbers of cell clusters formedin corresponding cultures (Table 3): EGF gave rise to the smallest,FGF-2 to intermediate, and EGF plus FGF-2 to the highest cellcounts and numbers of clusters (Table 3), irrespective of thetime of growth factor addition. In addition, growth factor starvationfor 24 hr did not change the expression of differentiation markers:the numbers of nestin⁺ and TuJ1⁺ cells found 1 hr after plating were virtually identical to thoseobserved 24 hr after plating (data not shown). These results showthat the conditions used to analyze growth factor-induced CREBphosphorylation did not alter proliferation or differentiationof growth factor-responsive precursors.


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Table 3. Effects of 24 h growth factor starvation on proliferation of mouse E14 striatal cells

We next analyzed CREB phosphorylation in mouse E14 striatal cells 24 hr after dissection and plating in culture medium withoutEGF or FGF-2 (Fig. 2). Without stimulation with exogenous growthfactors, only 1% of the cells showed nuclear phospho-CREB immunoreactivity.Compared with unstimulated cultures, addition of EGF did not increasethe number of phospho-CREB-positive cells. In contrast, stimulationwith FGF-2 or with a combination of EGF and FGF-2 induced CREBphosphorylation in 10-12% of the cells. These results indicatethat mouse E14 striatal cells, cultured in vitro for 24 hr, contain10-12% F^res cells, whereas no E^res cells appear to be present at this time. In control experimentscells were stimulated with 10 µM forskolin, an activator of adenylatecyclase, which causes CREB phosphorylation in a receptor-independentmanner by increasing intracellular levels of cAMP, leading toactivation of cAMP-dependent protein kinase (Gonzalez and Montminy,1989). We found that virtually all cells were phospho-CREB-positivewith forskolin treatment (data not shown).

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Figure 2. FGF-2-induced CREB phosphorylation in mouse E14 striatal cells cultured in vitro for 24 hr. A, Examples of phospho-CREB immunostaining (right panels) and corresponding phase-contrast pictures (left panels) of unstimulated cells (unst.) or after stimulation with the indicated growth factors. Arrows indicate phospho-CREB-immunopositive cells. Scale bar, 10 µm. B, Quantitative analysis of CREB phosphorylation in unstimulated cells (U) and in cells stimulated with EGF (E), FGF-2 (F), or a combination of EGF and FGF-2 (E/F). Data represent the means of five independent experiments. For each condition >5000 cells were counted. *Significantly different from unstimulated (p < 0.001).

We next characterized the phenotype of the F^res cells. Previous studies have shown that FGF-2 can act on differentiating neuronalcells (Ray and Gage, 1994; Bouvier and Mytilineou, 1995; Ghoshand Greenberg, 1995). To determine whether the F^res striatal cells were precursors or differentiating neurons, weperformed double-immunostaining experiments using the phospho-CREB-specificantibody together with antibodies to either nestin or TuJ1. Examplesof double-immunostaining experiments are shown in Figure 3; quantitativeanalysis of the data are illustrated in Figure 4. We found that75% of the F^res cells (8% of total cells) were TuJ1⁺, whereas the remaining F^res cells (3-5% of the total cells) were nestin⁺ (Fig. 4A,B). These results identify two distinct populationsof F^res cells in mouse E14 embryonic striatum: TuJ1⁺ neurons and nestin⁺ precursors. Neither of these cell types responded to EGF at thisstage of in vitro development.

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Figure 3. FGF-2-induced CREB phosphorylation in precursor cells and neurons present in mouse E14 striatal cells cultured in vitro for 24 hr. Examples of double immunostaining after stimulation of the cells with the indicated growth factors are shown. Phospho-CREB and nestin immunoreactivity (left panels) and phospho-CREB and TuJ1 immunoreactivity (right panels) are shown. Phospho-CREB immunoreactivity is viewed through rhodamine filters. Nestin and TuJ1 immunoreactivity is viewed through fluorescein filters. Arrows indicate double-immunopositive cells; arrowheads indicate cells immunopositive only for phospho-CREB; unst., unstimulated cells. Scale bar, 15 µm.

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Figure 4. Characterization of FGF-2-responsive mouse E14 striatal cells cultured in vitro for 24 hr. Quantitative analysis of phospho-CREB and nestin (A) or phospho-CREB and TuJ1 (B) double-immunopositive cells in unstimulated cultures (U) or in cultures stimulated with EGF (E), FGF-2 (F), or with a combination of both EGF and FGF-2 (E/F). Data represent the means of four independent experiments. For each condition a total of 3000 cells were counted. *Significantly different from U (p < 0.001).

Identification of single cells responding to both EGF and FGF-2 at later stages of in vitro development

We next examined responsiveness to EGF and FGF-2 in cells isolated from mouse embryonic striatum and grown for 6 d in thepresence of EGF and/or FGF-2. Figure 5 shows examples of double-immunostainingexperiments; quantification of the data are shown in Figure 6.We found that, irrespective of the growth factor conditions duringthe expansion phase, both EGF and FGF-2 elicited a response ina similar percentage of nestin⁺ cells (Figs. 5, 6), whereas the TuJ1⁺ cells responded to FGF-2 and not to EGF (Fig. 6B). To investigatewhether EGF and FGF-2 acted on dividing cells, 6-d-old striatalcultures were labeled with BrdU in culture medium (without exogenousgrowth factors) for 24 hr before growth factor stimulation. Analysisof cells immunopositive for both BrdU and phospho-CREB revealedthat, irrespective of the growth factor condition during the 6d in vitro, >50% of the BrdU-positive cells (56 ± 7%, 57 ± 6.6%,and 63 ± 7% in EGF, FGF-2, and EGF plus FGF-2 grown cultures,respectively) were also phospho-CREB-immunopositive after eitherEGF or FGF-2 stimulation (Fig. 7). These data underestimate thenumber of dividing growth factor-responsive cells: some cells,although proliferatively active, may be in a particular phaseof the cell cycle during the 24 hr starvation period that preventsthem from incorporating BrdU.

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Figure 5. EGF- and FGF-2-induced CREB phosphorylation in precursor cells and neurons present in mouse E14 striatal cultures grown for 6 d in the presence of EGF plus FGF-2. A, B, Left panels, Examples of phospho-CREB immunostainings in unstimulated (unst.) cells and after stimulation with the indicated growth factors. Right panels, Nestin (A) and TuJ1 (B) immunoreactivity within the same visual fields. Arrows indicate double-immunopositive cells. Scale bar, 15 µm.

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Figure 6. Characterization of growth factor-responsive cells in cultures of striatal precursor cells grown for 6 d in the presence of EGF (6 DIV EGF) and FGF-2 (6 DIV FGF-2) or in the presence of both (6 DIV EGF+FGF-2). Quantitative analysis of the double-immunopositive cells (A, phospho-CREB and nestin; B, phospho-CREB and TuJ1) in unstimulated cultures (U) and in cultures stimulated with EGF (E), FGF-2 (F), or a combination of EGF and FGF-2 (E/F). Data represent the means of three independent experiments. For each condition >1000 cells were counted. A, *Significantly different from U (p < 0.01); ^#Significantly different from E and F (p < 0.05) and from U (p < 0.001). B, *Significantly different from unst. (p < 0.001). The differences in the numbers of TuJ1 and phospho-CREB double-immunopositive cells in U and E are not significant.

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Figure 7. BrdU and phopho-CREB double immunostaining. Examples of phospho-CREB immunostainings in unstimulated cultures (unst.) and after stimulation with the indicated growth factors (top panels) and BrdU-immunopositive precursors within the same visual fields (bottom panels). Arrows indicate double-immunopositive cells. Scale bar, 5 µm.

To analyze whether EGF and FGF-2 stimulated the same or distinct subsets of nestin⁺ cells, we next determined the number of phospho-CREB-positivecells after stimulation with a combination of EGF and FGF-2. Wefound that in cultures grown for 6 d with FGF-2 or EGF plus FGF-2,stimulation of the cells with either growth factor or with a combinationof both induced a response in a similar number of nestin⁺ cells (Fig. 6A). This indicates that EGF and FGF-2 act on thesame cell population (E/F^res cells). In contrast, in EGF-grown cultures the number of cellsstimulated with both EGF and FGF-2 was significantly greater thanthe number of cells responding to either growth factor alone (Fig.6A; p < 0.05). This result suggests that, under these growth conditions,E/F^res cells as well as E^res and F^res cells are present in the cultures. Given the difference in totalcell counts obtained after 7 d after each growth factor treatment(Fig. 1B), the absolute number of E/F^res cells was three to seven times smaller in EGF-grown culturesthan in cultures grown in the presence of FGF-2. We next investigatedthe role of FGF-2 in the generation of E/F^res cells.

Priming of neural precursor cells with FGF-2 induces the appearance of a cell population responding to both EGF and FGF-2 after 2 d in vitro

Exogenous FGF-2 could increase the number of E/F^res cells by promoting the division of F^res precursor cells that will subsequently acquire EGF responsivenessin an FGF-2-independent manner. Alternatively, FGF-2 may, in additionto inducing proliferation, promote the transition of growth factorresponsiveness from F^res to E/F^res. To distinguish between these two possibilities, mouse E14 striatalcells were primed for 24 hr with either EGF or FGF-2 after striatumdissection. Cells were then plated onto poly-L-lysine-laminin-coatedchamber slides and analyzed for EGF and FGF-2 responsiveness afteran additional 24 hr in vitro in the absence of exogenous growthfactors. In FGF-2-primed cultures, the same percentage of nestin⁺ cells, representing ~5% of the total number of cells, showedphospho-CREB nuclear immunostaining after stimulation with eitherEGF or FGF-2 alone or with a combination of both (Fig. 8B), demonstratingthat EGF and FGF-2 stimulated the same precursor cells (E/F^res cells). F^res cells, which were present at 24 hr after dissection, were nolonger detected (Fig. 8B; for a comparison, also see Fig. 4A),indicating that they had acquired EGF responsiveness after FGF-2treatment. In contrast, this transition in growth factor responsiveness,from F^res to E/F^res, was not observed in EGF-primed cultures, which, similar to 24hr after dissection, contained cells responding to FGF-2 but notto EGF (i.e., F^res cells) (Fig. 8A). Priming with either EGF or FGF-2 did not affectthe TuJ1⁺ cells, which remained responsive to FGF-2 only (Fig. 8C,D; fora comparison, also see Fig. 4B). These results demonstrate acquisitionof growth factor responsiveness on single neural precursors: cellsinitially responding to FGF-2 only acquire EGF responsivenessat later stages of in vitro development. FGF-2 but not EGF canpromote this transition.

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Figure 8. Characterization of growth factor-responsive cells in cultures of striatal precursor cells primed for 24 hr with EGF (A, C) or FGF-2 (B, D). Graphical representation of the percentage of double-immunopositive phospho-CREB and nestin (A, B) and phospho-CREB and TuJ1, (C, D) cells in unstimulated cultures (U) and in cultures stimulated with EGF (E), FGF-2 (F), or a combination of EGF and FGF-2 (E/F). Data represent the means of three independent experiments. For each condition a total of 600 cells were counted. A, B, *Significantly different from U (p < 0.01). C, D, *Significantly different from U (p < 0.001).

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Phospho-CREB-specific antibodies: a tool for characterization of growth factor-responsive cells in heterogeneous populations of neural precursor cells

Previous studies have used clonal analysis to show that single neural precursors divide in response to EGF or FGF-2 and subsequentlydifferentiate into multiple neural phenotypes (Kilpatrick andBartlett, 1993; Gage et al., 1995; Qian et al., 1997). However,clonal analysis cannot detect the response of single cells togrowth factor signals. In this study we used a novel approachto characterize, at the single-cell level, EGF- and FGF-2-responsivecells in cultures of mouse E14 striatum. Phosphorylation of CREBon serine 133 is one of the intracellular events following activationof receptor tyrosine kinases (Ginty et al., 1994; Xing et al.,1996). Using an antibody recognizing this phosphorylated formof CREB, we identified EGF- and FGF-2-responsive cells by immunostaining.This antibody also recognizes the phosphorylated form of the transcriptionfactor ATF1, which is closely related to CREB. This cross-reactivity,however, does not represent a limit for our experimental approach,because the antibody was used as an activation marker. Alternativemethods, such as RT-PCR and immunocytochemistry, have been usedpreviously to detect growth factor receptor expression in neuralprecursors at the level of mRNA (both EGF and FGF receptors) andprotein (FGF receptor only) (Reynolds et al., 1992; Vescovi etal., 1993; Qian et al., 1997). However, it has been difficultto assess growth factor receptor expression in individual cells,which may be because of their low abundance and/or lack of suitableantibodies. Analysis of CREB phosphorylation, rather than immunodetectionof growth factor receptor molecules, has several advantages. Itprovides a detection method to analyze the response to differentgrowth factors acting on receptor tyrosine kinases. It is a verysensitive method because CREB phosphorylation is the result ofa cascade of intracellular biochemical events in which the initialsignal is amplified. Therefore, it allows identification of cellsexpressing very few growth factor receptors that would be difficultto detect by conventional immunocytochemical staining. A potentialdrawback of this approach is that cells responding to growth factorswithout activating the classical Ras/ERK pathway leading to CREBphosphorylation will remain undetected. However, all availableevidence suggests that activation of receptor tyrosine kinases,in particular that of EGF and FGF-2 receptors, is linked to Ras/ERKsignaling cascades (Marshall, 1995). Cells that do not expressCREB would also remain undetected with this assay for growth factorresponsiveness. However, CREB is widely expressed in the CNS (Herdegenet al., 1997), and immunostaining of the cells analyzed in thisstudy shows that virtually all cells express CREB protein (datanot shown).

EGF responsiveness arises later during in vitro development

The majority of the cells in primary striatal cultures were either nestin⁺ or TuJ1⁺ at any given time analyzed in this study. Nestin has been widelyaccepted as a marker of neuroepithelial precursor cells (Lendahlet al., 1990), and TuJ1 has been recognized as a neuronal marker(Menezes and Luskin, 1994), although low levels of TuJ1 can befound also in immature oligodendrocyte. We found that TuJ1⁺ cells responded to FGF-2, irrespective of the growth conditionsand the length of in vitro culturing. This is consistent withthe previous observation that rat embryonic cortical neurons respondto FGF-2 but not EGF (Ghosh and Greenberg, 1995). In contrast,growth factor responsiveness of the nestin⁺ cells changes during in vitro development. After 1 d in vitro,E14 striatal cultures contain nestin⁺ cells responding to FGF-2, whereas EGF-responsive cells are undetectable.This provides a possible explanation for the previous observationthat precursors derived from rodent embryonic striatum proliferatein response to EGF only after 4-5 d in vitro (Reynolds et al.,1992; Svendsen et al., 1995). Our results indicate that this lackof EGF-induced proliferation is attributable to the absence ofEGF-responsive cells rather than to the inability of the cellsto divide at early stages of in vitro development. After 7 d invitro a population of cells had acquired EGF responsiveness andwas stimulated by both EGF and FGF-2 (E/F^res cells). These cells represented the majority, if not all, ofthe dividing cells in 7-d-old cultures. The change in growth factorresponsiveness occurred under all culture conditions; however,FGF-2 and EGF plus FGF-2-treated cultures contained three andseven times, respectively, more E/F^res cells than EGF-grown cultures. This difference in E/F^res cell number correlates with the total cell counts and the numberand size of neurospheres after 7 d in vitro. There is also a closecorrelation between the time of appearance of the E/F^res cells and the increase in the rate of BrdU incorporation. Thissuggests that the E/F^res cells are critical for neurosphere formation. It is possiblethat the E/F^res cells, which constitute 15-20% of the cell population, representthe fraction (18.7%) of cells derived from primary neurospheresthat was previously found to generate secondary neurospheres inresponse to EGF (Reynolds and Weiss, 1996).

Although the differentiation potential of the E/F^res cells remains to be investigated directly, several lines of evidence suggestthat E/F^res cells represent multipotent precursors. First, EGF and FGF-2support the proliferation of striatal multipotent neural precursors,and E/F^res cells are the principal population of growth factor-responsiveprecursors found under all growth conditions analyzed. Second,the relative abundance of E/F^res cells present in neurospheres correlates with the percentageof neurons and glial cells obtained after differentiation.

In EGF-treated cultures, two other cell populations are present: E^res cells and F^res cells. The F^res cells could be similar to those found after 24 hr in vitro thathave not yet acquired EGF responsiveness. The nature of the E^res cells is less clear. Because EGF receptor mRNA is expressed inmany differentiating cell populations of the embryonic brain (Kornblumet al., 1997), one possible explanation for the presence of E^res cells in EGF- but not FGF-2-grown cultures is that they may representmore lineage-restricted progenitors with a limited or slow proliferativeactivity. Therefore, these cells could be overgrown by more rapidlydividing cells present in FGF-2-containing cultures. Alternatively,the E^res cells may originate from F^res cells that only temporarily acquired responsiveness to both growthfactors (i.e., E/F^res cells) but have lost FGF-2 responsiveness in the absence of FGF-2in the culture medium.

FGF-2 promotes acquisition of EGF responsiveness during neural precursor development

Our priming experiments indicate that FGF-2 promotes the appearance of an EGF response in cells originally responding to FGF-2only. A short (24 hr) exposure to FGF-2 induced the appearanceof E/F^res cells after 2 d, whereas F^res nestin⁺ cells were no longer detected. EGF was unable to promote thistransition in growth factor responsiveness, which may explainwhy the number of E/F^res cells after 7 d in vitro was lower in EGF-grown cultures thanin cultures exposed to FGF-2. The here-described role for FGF-2in promoting a change in growth factor responsiveness resemblesa previous observation by Cattaneo and McKay (1990), who foundthat rat embryonic precursors proliferated in response to nervegrowth factor (NGF) after a 2 d exposure to FGF-2, whereas untreatedcultures did not respond to NGF.

Exogenous FGF-2 is not essential for the acquisition of EGF responsiveness in striatal cells, because E/F^res cells were also identified in EGF-grown cultures, although insmall numbers. Although this could indicate that the acquisitionof EGF responsiveness is a default pathway during in vitro development,the finding that the neural precursor cultures derived from embryoniccerebrum may secrete FGF-2 suggests that endogenous FGF-2, ora related molecule, may be responsible for changing growth factorresponsiveness (Kilpatrick and Bartlett, 1995). This hypothesisis supported by the observation that EGF is virtually ineffectivein inducing proliferation of primary striatal cells grown at clonaldensity (Reynolds and Weiss, 1996). Under these conditions secretedFGF-2, or a similarly acting growth factor, may not reach a concentrationhigh enough to be biologically effective.

One possible function of this FGF-2-induced change in growth factor responsiveness could be that it allows the cells to proliferatemore actively. Indeed, we found that EGF plus FGF-2 had a synergisticeffect, compared with EGF or FGF-2 alone, on total cell countsand on the number and size of neurospheres, which is consistentwith previous observations (Weiss et al., 1996a; Svendsen et al.,1997). The acquisition of EGF responsiveness could also affectneural cell differentiation. For example, the appearance of EGFresponsiveness in cultures of mouse E17 cerebrum coincides withthe appearance of glial-restricted precursors. These precursorsare absent in similar cultures from E10 cerebrum, which appearto lack EGF responsiveness (Kilpatrick and Bartlett, 1995). Otherstudies have shown that overexpression of EGF receptor altersthe differentiation characteristics of rat retinal precursorsand of cortical progenitors of the ventricular zone (Lillien,1995; Burrows et al., 1997).

The mechanism through which FGF-2 induces EGF responsiveness could be the result of induction of EGF receptor mRNA and protein.The promoter of the EGF receptor gene contains several putativeregulatory elements that function either as repressors or activatorsof transcription (Hou et al., 1994; Johnson, 1996). Whether FGF-2stimulates a transcriptional activator, inhibits a repressor,or alternatively, induces an EGF response by a post-transcriptionalmechanism remains to be investigated.

Conclusions

Neural precursor cells initially responding to FGF-2 only become responsive to EGF later during in vitro development. Thischange in growth factor responsiveness is promoted by FGF-2 andleads to the appearance of a population of precursor cells respondingto both EGF and FGF-2. A model illustrating our findings is shownin Figure 9.

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Figure 9. Model illustrating the generation of neural precursors responding to both EGF and FGF-2 during in vitro development. Neural precursors responding to FGF-2 (F^res) after 1 d in vitro (DIV) acquire EGF responsiveness later during in vitro development, giving rise to precursors responding to both growth factors (E/F^res). The effects of the different growth factor conditions on this transition are illustrated: FGF-2, but not EGF, promotes the change in growth factor responsiveness; EGF plus FGF-2 has a synergistic effect on the growth of E/F^res cells. The numbers of E/F^res cells indicate their approximate growth rate under the different culture conditions.

  FOOTNOTES

Received May 15, 1998; revised July 21, 1998; accepted July 21, 1998.

This work was funded by the European Community and the Wellcome Trust. We thank Dr. Hilmar Bading for discussion and helpwith this manuscript and Dr. Neil Scolding for the Gal-C antibody.
Correspondence should be addressed to Dr. Francesca Ciccolini, Medical Research Council Cambridge Centre for Brain Repair,Forvie Site, Robinson Way, Cambridge CB2 2PY, England.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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