Epidermal Growth Factor Receptors Control Competence to Interpret Leukemia Inhibitory Factor as an Astrocyte Inducer in Developing Cortex

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The Journal of Neuroscience, April 15, 2003, 23(8):3385

Epidermal Growth Factor Receptors Control Competence to Interpret Leukemia Inhibitory Factor as an Astrocyte Inducer in Developing Cortex
Jane Viti, Angela Feathers, Jennifer Phillips, and Laura Lillien
Department of Neurobiology and Pittsburgh Cancer Institute, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania 15261

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Cortical progenitors begin to interpret leukemia inhibitory factor (LIF) and bone morphogenetic protein (BMP) as astrocyte-inducingsignals during late embryonic cortical development, coincidentwith an increase in their expression of epidermal growth factorreceptors (EGFRs). To determine whether the developmental changein EGFRs regulates the change in responsiveness to LIF and BMP,we analyzed cortical progenitors induced to express EGFRs prematurelyand progenitors from late embryonic EGFR-null cortex. Prematureelevation of EGFRs conferred premature competence to interpretLIF, but not BMP, as an astrocyte-inducing signal. EGFR-null progenitorsfrom late embryonic cortex did not interpret LIF as an astrocyte-inducingsignal but responded to BMP4. LIF responsiveness in EGFR-nullcells was rescued by the addition of EGFRs but not by the stimulationof fibroblast growth factor receptors. Astrocyte differentiationinduced by LIF depends on signal transducer and activator of transcription3 (STAT3). We show that the level of STAT3 increases during lateembryonic development in a subset of progenitors. EGFRs regulatethis change in STAT3 and increase STAT3 phosphorylation in responseto LIF. Increasing STAT3 prematurely with a retrovirus also increasedthe phosphorylation of STAT3 by LIF. In contrast to the findingwith EGFRs, however, increasing STAT3 did not cause LIF to induceastrocytes, although it reduced expression of the neurogenic factorPAX6 (paired box gene 6 ). Our findings show that developmentalchanges in EGFRs regulate the competence of progenitors to interpretLIF as an astrocyte-inducing signal. EGFRs elevate STAT3 expressionand increase its phosphorylation by LIF, but this is not sufficientto change LIF responsiveness to astrocyte induction, suggestingthat EGFRs also regulate LIF responsiveness downstream ofSTAT3.

Key words: EGF receptor; LIF; astrocyte; cortex; STAT3; stem cell; PAX6; BMP4

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

During late embryonic development, there is a shift in cell-type specification from neurogenesis to gliogenesis (for review,see Bayer and Altman, 1991). Several intrinsic molecules thatcontrol the choice between neurogenesis and gliogenesis have beenidentified. Paired box gene 6 (PAX6) and the bHLH (basic helix-loop-helix)factors neurogenin 1 (ngn1) and ngn2 promote a neuronal fate andinhibit the development of astrocytes (Sun et al., 2001; Heinset al., 2002). ngns achieve this control of cell fate in partby antagonizing the action of signal transducers and activatorsof transcription (STATs) (Sun et al., 2001), which promote thedevelopment of astrocytes (Bonni et al., 1997; Rajan and McKay,1998). Several extrinsic signals that induce the development ofastrocytes have been identified. These include leukemia inhibitoryfactor (LIF)/ciliary neurotrophic factor (CNTF), bone morphogeneticproteins (BMPs), and epidermal growth factor (EGF)-family ligands(Gross et al., 1996; Johe et al., 1996; Burrows et al., 1997).The timing of astrocyte development is regulated by changes inligand expression (Lillien et al., 1988; Stockli et al., 1991)and changes in the competence of progenitors to respond to theseligands in a specific manner (Mehler et al., 2000; Molne et al.,2000). Changes in competence are mediated at least in part bythe ratio of ngn1 to STATs in progenitors (Sun et al., 2001).

The competence of progenitors to interpret LIF/CNTF, BMPs, and EGF-family ligands as astrocyte-inducing signals can firstbe observed at approximately embryonic day 14.5 (E14.5) in miceand E16 in rats (Burrows et al., 1997; Mehler et al., 2000; Molneet al., 2000). Our previous work demonstrated that the changein responsiveness to EGF-family ligands reflects an increase inthe level of EGF receptors (EGFRs) expressed by progenitors betweenE13 and E16 in mice (E14.5-E16.5 in rats) (Eagleson et al., 1996;Burrows et al., 1997; Caric et al., 2001). The developmental changein EGFR expression is regulated by extrinsic signals, includingfibroblast growth factor 2 (FGF2), which induces EGFR expression(Lillien and Raphael, 2000). The change in responsiveness to BMPand LIF does not reflect an absence of functional receptors andsignal transduction machinery for these ligands in early corticalprogenitors (Molne et al., 2000; Takizawa et al., 2001). In fact,early progenitors are responsive to BMP and LIF but generate neuronsrather than astrocytes (Li et al., 1998; Molne et al., 2000).

Our previous work raised the possibility that EGFRs induce the development of astrocytes by regulating responses of progenitorsto heterologous extrinsic signals, such as LIF/CNTF and BMPs (Burrowset al., 1997). To test this idea, we introduced high levels ofEGFRs into cortical progenitors prematurely by retroviral transductionand asked whether this conferred competence to interpret LIF orBMP as astrocyte-inducing signals prematurely. We also assessedresponses to LIF and BMP in EGFR-null progenitors after the changein responsiveness to LIF and BMP should have occurred. We notedthat EGFRs regulated a developmental increase in the level ofSTAT3 and in the ability of LIF to induce STAT3 phosphorylation.To address the idea that EGFRs regulate responses to LIF by controllingthe level of STAT3, we increased STAT3 in progenitors prematurelyby retroviraltransduction.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Animals. EGFR-null mice in a CD1 background (Threadgill et al., 1995) were purchased from The Jackson Laboratory (Bar Harbor,ME). Homozygous null and wild-type littermates were obtained bybreeding heterozygotes. EGFR-null embryos were used at E16.5-E17.At this age, eyelids have fused in wild-type embryos but not inEGFR-null embryos. The genotype of embryos was confirmed by PCR.Only EGFR-null ( $-$ / $-$ ) and wild-type (+/+) embryos were used foranalysis.

Cultures. Timed pregnant CD1 or EGFR +/ $-$ females were killed with CO₂, and embryos were collected in HBSS (Invitrogen, Gaithersburg,MD) at E11-E11.5, E13-E13.5, or E16-E17. Embryonic age was determinedfrom crown-rump length and by examination of external features(Theiler, 1972). The dorsolateral cortex was dissected and culturedon nucleopore filters in serum-free medium in 35 mm dishes, asdescribed previously (Burrows et al., 1997). Progenitors wereinfected with replication-incompetent retroviruses by placinga 30 µl drop of medium containing virus on the filters. Theseviruses provide a means of introducing extra wild-type EGFR orSTAT3 (see below), in addition to serving as lineage markers.These viruses selectively infect dividing cells at the ventricularsurface (Burrows et al., 1997). The frequency of infection wasdetermined by counting the proportion of cells that express virallytransduced genes 1 d after infection. For example, 0.002 ± 0.0002%of the cells in an E13 explant were infected by either controlor EGFR viruses with titers of ~1 × 10⁷ colony-forming units (cfu)/ml. When viruses of lower (0.5 × 10⁷) and higher (2 × 10⁷) titers were compared, there was no significant difference incell fate (data not shown). Viral stocks with titers of 0.5-2× 10⁷ cfu/ml were selected for infection of explants in this study.Growth factors were added as noted. They were added daily to themedium, beginning 1 d after explants were cultured. Growth factorsincluded recombinant human FGF2 (10 ng/ml; R & D Systems, Minneapolis,MN), human BMP4 (10-100 ng/ml; R & D Systems); human TGF $alpha$ (10ng/ml; R & D Systems), and murine LIF [2000-10,000 U/ml; R & DSystems and Chemicon (Temecula, CA)]. To quantify effects on cell-typespecification among the infected cells after 4 d in vitro, explantswere dissociated [15 min in 0.1% trypsin (Sigma, St. Louis, MO)],and cells were allowed to attach to poly-D-lysine (PDL; Sigma)-coatedslides for 1 hr and then processed for immunocytochemistry (seebelow). To assay the ability of LIF to induce STAT3 phosphorylation,explants were infected at E11 or E13, cultured without exogenousgrowth factors for 4 d, and then dissociated and plated as describedabove. Cells were allowed to recover from dissociation for 3 hr,stimulated with LIF for 20 min, and then fixed and stained asdescribedbelow.

Viruses. Progenitors in explants were infected with control virus expressing either the histochemical marker $beta$ -geo (lacZ plusneomycin phosphatase) (Friedrich and Soriano, 1991) or enhancedgreen fluorescent protein (eGFP) (Clontech, Palo Alto, CA). TheeGFP viral vector was made by subcloning the internal ribosomeentry sequence (IRES)-eGFP sequence from IRES2-EGFP (Clontech)into the mouse mammary tumor virus vector pLIA (Bao and Cepko,1997), after removing the fragment encoding IRES-alkaline phosphatase.The resulting vector (pLIE) was used to generate a viral vectorthat coexpresses STAT3 (rat cDNA) (Ripperger et al., 1995) andeGFP. Eighty-five to 90% of infected E11.5 cortical progenitorsthat express eGFP coexpressed a high level of STAT3 (both detectedimmunocytochemically) (see Fig. 6A,B). The EGFR virus (Lillien,1995) coexpresses $beta$ -geo (Friedrich and Soriano, 1991) and wild-typehuman EGFR (Velu et al., 1989). Virus stocks were made by transfecting $psi$ -2 cells with the viral vectors (Cepko et al., 1993). In thecase of pLIE and pLIE-STAT3, cells were cotransfected with pSV2neo.Clones of transfected cells were selected in G418, screened forexpression of the virally transduced genes, and titered with 3T3cells (Cepko et al., 1993).

Immunocytochemistry. Cells on PDL slides were fixed in 4% PFA in either 0.1 M PO₄, pH 7.4, or 3% PIPES buffer at room temperaturefor 10 min. Cells were rinsed and blocked in PBS containing 10%FBS and 0.1% Triton X-100 for 10 min. For phospho-STAT3 staining,cells were also fixed in methanol for 10 min at $-$ 20°C. Cells wereincubated for 1 hr at room temperature in primary antibodies dilutedin this block. Antibodies included rabbit anti- $beta$ -galactosidase( $beta$ -gal) (Cortex Biochem, San Leandro, CA), rabbit or mouse anti-eGFP(Molecular Probes, Eugene, OR), chick anti-eGFP (Chemicon), mouseanti- $beta$ -gal (Promega, Madison, WI), mouse anti-S-100 $beta$ (Sigma),mouse anti-GFAP (Sigma), mouse anti-proliferating cell nuclearantigen (PCNA) (Sigma), sheep anti-EGFR (Upstate Biotechnology,Waltham, MA), mouse anti- $beta$ -tubulin (TuJ1; Covance Research Products,Berkeley, CA), rabbit anti-STAT3 (Cell Signaling Technology, Beverly,MA), rabbit anti-phospho-STAT3 (Tyr⁷⁰⁵; Cell Signaling Technology), mouse anti-PAX6 (Ericson et al.,1997) (Developmental Studies Hybridoma Bank, Iowa City, IA), mouseanti-RC2 (Misson et al., 1988) (Developmental Studies HybridomaBank), and rabbit anti-activated caspase 3 (Biovision, MountainView, CA). For phospho-STAT3 staining, cells were incubated inprimary antibodies overnight at 4°C. Cells were rinsed in PBSand incubated for 30 min in a mixture of secondary antibodies(Jackson ImmunoResearch, West Grove, PA): donkey anti-rabbit Cy3,donkey anti-sheep Cy3, donkey anti-rabbit Cy2, donkey anti-chickCy2, or donkey anti-mouse IgG or IgM Cy2. To characterize theantigenic phenotype of E15 and E17 cells, dorsolateral cortexwas dissected free of meninges, dissociated, plated on PDL slides,and stained as described for explants. Cells were rinsed and mountedin glycerol/PBS. Stained cells were analyzed with a Leica (Nussloch,Germany) DMR fluorescence microscope, and images were capturedwith a Sensys digital camera using IPLab and Photoshop software(Axon Instruments, Foster City, CA). One hundred cells per conditionwere counted per experiment. At least three experiments were performedfor each condition. Data are presented as mean ± SEM. Statisticalevaluation was performed using Student's t test and Statview software,with p < 0.05 consideredsignificant.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Premature elevation of EGFRs alters responses to LIF but not BMP

It has been reported that cortical progenitors from early embryonic rats and mice fail to differentiate into GFAP⁺ astrocytes when stimulated with either LIF/CNTF or BMPs in culture,although both factors induce astrocytes in cultures of older tissue(Gross et al., 1996; Johe et al., 1996; Li et al., 1998; Molneet al., 2000) (Fig. 1A,B). Rather than becoming astrocytes, progenitorcells infected with a control virus at E11 or E13 and then exposedto LIF or BMP4 differentiated into neurons, their normal fatein vivo at these ages (Fig. 1C).

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Figure 1. Premature expression of EGFRs induces a premature change in responsiveness to LIF. Progenitors in cortical explants were infected with either control virus or virus expressing EGFRs at E11, E13, or E16, and the proportion of infected cells ( $beta$ -gal⁺) (D, F) that express the astrocyte marker GFAP (A, B, G) or the neuron marker TuJ1 (C, E) was determined 4 d later. Cultures were grown in the absence ( $-$ ) or presence (+) of LIF (L) (A, C) or BMP4 (B) (B, C). EGFRs induce premature competence to interpret LIF as an astrocyte-inducing signal (A, F, G). Some EGFR-infected cells differentiate into neurons (C-E), but this is reduced compared with control-infected cells. Arrows point to double-labeled cells. D-G, E13 progenitors were infected with EGFR virus, grown without (D, E) or with (F, G) LIF, and then stained for $beta$ -gal (D) and TuJ1 (E) or $beta$ -gal (F) and GFAP (G). C, Comparisons are between EGFR virus and control virus. *p = 0.01; **p $<=$ 0.006; ***p < 0.0001.

To determine whether the developmental increase in EGFR expression between E13 and E16 plays a role in the temporal changein responsiveness to LIF and/or BMP, we elevated EGFRs prematurelyby infecting progenitors in explants with a retrovirus that transduceswild-type EGFRs and the histochemical marker $beta$ -gal. As a control,we used a virus transducing the marker alone. These viruses infectonly dividing cells, thereby serving as a method of marking progenitorsand following the fate of their progeny. The explants were grownin the absence or presence of LIF (2000 U/ml) or BMP4 (10 ng/ml)for 3 d, beginning 1 d after infection. The ability of the infectedcells to respond to these factors by generating astrocytes ratherthan neurons was analyzed by double-labeling cells with a $beta$ -galantibody to identify infected cells and with cell-type-specificantibodies for astrocytes (GFAP; S-100 $beta$ ) or neurons(TuJ1).

Premature elevation of EGFRs at E11 conferred premature competence to interpret LIF as an astrocyte-inducing signal in 15-20%of the infected cells (Fig. 1A,F,G). A larger proportion of thecells infected with EGFR virus generated astrocytes in responseto LIF at later stages, E13 and E16 (Fig. 1A). In contrast, prematureelevation of EGFRs did not confer competence to interpret BMP4as an astrocyte-inducing signal prematurely, although it increasedthe proportion of cells that exhibited this response to BMP4 later,at E16 (Fig. 1B). In the absence of exogenous ligands, prematureelevation of EGFRs reduced the differentiation of neurons at allages (Fig. 1C). These observations suggest that increased expressionof EGFRs is one of the molecular mechanisms used to regulate thetiming of a change in responsiveness to LIF, but not toBMPs.

EGFRs are required for the developmental change in responsiveness to LIF but not BMP4

The results of viral transduction experiments indicated that elevated EGFR expression is sufficient for the change in responsivenessto LIF but did not address the issue of necessity. To determinewhether EGFRs are required for the change in responsiveness toLIF or BMP4, explants of E16-E17 EGFR-null cortex were exposedto LIF or BMP4 (Fig. 2). At this age, wild-type progenitors markedby infection with control virus respond to LIF by expressing S-100 $beta$ ,an early marker of astrocytes (Fig. 2A,C,D), in addition to GFAP,a later marker of astrocytes (Fig. 1A). In contrast, EGFR-nullprogenitors did not express even the early astrocyte marker S-100 $beta$ after stimulation with LIF (Fig. 2A) but differentiated into neuronsinstead (data not shown). If EGFRs were added back to EGFR-nullprogenitors, LIF could induce their differentiation into GFAP⁺ astrocytes, as observed in wild-type progenitors (Fig. 2B). Incontrast to LIF, BMP4 could induce the late astrocyte marker GFAPin EGFR-null progenitors (Fig. 3). These findings provide additionalsupport for the hypothesis that the developmental change in responsivenessto LIF is controlled by EGFRs.

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Figure 2. The developmental change in responsiveness to LIF depends on EGFRs. Explants of E16-E17 cortex from EGFR-null mice ( $-$ / $-$ ) and wild-type littermates (+/+) were infected with control virus (A) or EGFR virus (B), and the proportion of infected cells ( $beta$ -gal⁺) (C) that express the early astrocyte marker S-100 $beta$ (A, D) or the late astrocyte marker GFAP (B) was determined after 3 d in the absence ( $-$ ) or presence (+) of LIF. Competence to generate astrocytes in response to LIF is lost by EGFR-null cells (A) and restored by infecting progenitors with EGFR virus (B). Arrows point to a double-labeled cell expressing $beta$ -gal (C) and S-100 $beta$ (D). *p = 0.03; **p = 0.001; ***p < 0.0001, comparing LIF with untreated cells.

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Figure 3. The developmental change in responsiveness to BMP4 does not depend on EGFRs. Explants of E16-E17 cortex from EGFR-null mice ( $-$ / $-$ ) and wild-type littermates (+/+) were infected with a control virus, and the proportion of cells that expressed the late astrocyte marker GFAP was determined after 3 d in the absence ( $-$ ) or presence (+) of BMP4. *p = 0.009, comparing BMP4 with untreated $-$ / $-$ cells.

Effects of FGF2 on LIF responsiveness require EGFRs

It has been suggested that FGF2 induces responsiveness to CNTF/LIF (Molne et al., 2000; Morrow et al., 2001). We have reportedthat FGF2 can induce elevated expression of EGFRs (Lillien andRaphael, 2000). Our results showing that EGFRs are required forLIF to induce astrocytes raised the question of whether EGFRswere also required for FGF2-dependent changes in LIF responsiveness.In wild-type E16 progenitors, FGF2 enhanced the proportion ofGFAP⁺ astrocytes, and the combination of FGF2 and LIF also increasedthe proportion of astrocytes (Fig. 4), as reported previously(Molne et al., 2000). In EGFR-null progenitors, FGF2 also promotedGFAP⁺ astrocyte differentiation to levels that were comparable withthose of wild-type progenitors; however, LIF failed to induceadditional GFAP⁺ astrocytes when combined with FGF2 (Fig. 4). These observationsindicate that FGFR activation cannot substitute for EGFRs in modulatingresponsiveness to LIF. Moreover, they suggest that the effectof FGF2 on LIF responsiveness requires EGFRs.

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Figure 4. FGF2-dependent change in responsiveness to LIF requires EGFRs. Explants of E16-E17 cortex from EGFR-null mice ( $-$ / $-$ ) and wild-type littermates (+/+) were infected with a control virus, and the proportion of infected cells that express the astrocyte marker GFAP was determined after 3 d in the absence ( $-$ ) or presence (+) of FGF2 or the combination of FGF2 and LIF. FGF2 alone increases astrocyte development in wild-type and EGFR-null cells but does not enhance astrocyte development in response to LIF in EGFR-null cells. *p $<=$ 0.0004.

STAT3 levels in progenitors increase during development

Responses to LIF are mediated by STAT1 and STAT3 (Bonni et al., 1997). It has been proposed that the relative concentrationof STATs and neurogenin determines whether progenitors becomeneurons or glia, with a high ngn/STAT ratio promoting a neuronalfate (Sun et al., 2001). STAT3 is expressed in the embryonic cortexbefore the change in LIF responsiveness occurs (Molne et al.,2000). At E17, however, there is cell-to-cell variability in thelevel of STAT3 expression, on the basis of fluorescence intensitymeasurements taken after staining with STAT3 antibody (Fig. 5A).Cells (n = 210) fell into three general categories: STAT3-negative/low(8% of cells; fluorescence intensity $<=$ 10 arbitrary units abovebackground), STAT3-moderate (82% of cells; fluorescence intensity10-60 arbitrary units above background), and STAT3-high (10% ofcells; fluorescence intensity >80 arbitrary units above background).At E17, ~7% of the progenitor population defined by PCNA expressionand 32% of the RC2⁺ population (radial glia, now thought to be progenitors) (Malatestaet al., 2000; Noctor et al., 2001) expressed a high level of STAT3(Fig. 5B,C). In contrast, at earlier embryonic stages (E11, E13,and E15), there were relatively few PCNA⁺ or RC2⁺ cells that expressed a high level of STAT3 immunoreactivity (Fig.5B,C).

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Figure 5. STAT3 expression changes during development and is regulated by EGFRs. A, E17 dorsolateral cortex was stained for STAT3. Note that four cells (arrows) express a high level of STAT3 immunoreactivity, whereas the majority express intermediate or low levels (see Results for quantification of the populations). The population of cells that expresses a high level of STAT3 appears at E15 and increases in size over 2 d, coexpressing the progenitor markers PCNA (B) or RC2 (C). D, Premature elevation of EGFRs induces a high level of STAT3 prematurely. Cells infected with the EGFR virus at E13 express the viral marker $beta$ -gal (E; arrows) and a high level of STAT3 (F; arrows). G, The size of the population of cells that expresses a high level of STAT3 is reduced in EGFR-null cortical explants ( $-$ / $-$ ), compared with wild type. *p $<=$ 0.02; **p < 0.0001.

At E17, approximately one-half of the cells that expressed a high level of STAT3 also expressed a high level of EGFRs (Table1). Approximately one-half of the STAT3^high cells expressed the early astrocyte marker S-100 $beta$ , but none expressedthe later marker GFAP. Few STAT3^high cells expressed the neuronal marker TuJ1, but most were PCNA⁺. At E15, 40-50% of the STAT3^high cells coexpressed PAX6, but this fell to <5% by E17. PAX6 isassociated with competence to generate neurons (Heins et al.,2002). The data in Table 1 and Figure 5 indicate that the populationof cells that expresses a high level of STAT3 is heterogeneous,increases in size between E15 and E17, and changes in a mannersuggesting that the potential of these cells to generate neuronsdeclines.


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Table 1. Antigenic phenotype of STAT3^high cells

EGFRs regulate STAT3 level

Although the subpopulations of embryonic cells that express high levels of EGFRs or STAT3 do not overlap completely, the timingof the changes in EGFR and STAT3 expression suggested that anincrease in EGFRs might induce elevated expression of STAT3, andthat this might underlie EGFR-dependent changes in LIF responsiveness.To determine whether EGFRs regulate the level of STAT3 expression,progenitors were infected with EGFR virus at E11, E13, and E16.At all ages, EGFRs increased STAT3 expression in approximatelyone-half of the infected cells (Fig. 5D-F). To determine whetherthe loss of EGFRs results in a failure of late embryonic cellsto express a high level of STAT3, we examined EGFR-null cellsmarked by control virus at E16.5 and cultured as explants for4 d. The proportion of control-infected cells that expressed ahigh level of STAT3 was reduced in EGFR-null cells (Fig. 5G).These observations suggest that EGFRs regulate the level of STAT3in embryonic corticalprogenitors.

Increased STAT3 expression is not sufficient to change LIF responsiveness

STAT3 has been shown to be required for astrocyte generation in response to LIF/CNTF (Bonni et al., 1997). Our data raisedthe possibility that EGFRs mediate changes in LIF responsivenessby increasing the level of STAT3. To determine whether a highlevel of STAT3 is sufficient to induce a change in responsivenessto LIF, E11.5 progenitors were infected with a virus that expressesSTAT3 and the reporter eGFP (Fig. 6A,B) or a virus that expresseseGFP alone. Infection with STAT3 virus did not confer competenceto interpret LIF as an astrocyte-inducing signal in E11.5 progenitors(Fig. 6C) or E13.5 progenitors (11 ± 1% for control virus vs 8.5± 0.5% for STAT3 virus). Instead, these cells differentiated intoneurons (data not shown). STAT3 did increase the proportion ofcells that expressed the early astrocyte marker S-100 $beta$ in theabsence of LIF (Fig. 6C), but these cells did not express thelater marker GFAP (data not shown). LIF has been reported to actsynergistically with BMP to induce GFAP⁺ astrocytes (Nakashima et al., 1999); however, premature elevationof STAT3 did not confer competence to interpret the combinationof BMP4 and LIF, or BMP alone, as astrocyte-inducing signals (datanot shown).

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Figure 6. Premature expression of a high level of STAT3 reduces PAX6 but does not change responsiveness to LIF. A retrovirus that coexpresses eGFP (A) and wild-type STAT3 (B) was used to infect progenitors in E11.5 cortical explants. C, Four days after infection, STAT3 virus increases the proportion of cells that express the early astrocyte marker S-100 $beta$ in the absence ( $-$ ) of LIF but does not cause more cells to respond to LIF as an astrocyte-inducing signal. +, Addition of LIF. The proportion of infected E11.5 cells (D; arrow) that express the neurogenic factor PAX6 (E; arrow) is reduced by STAT3 virus compared with a control virus (F). *p = 0.02; **p = 0.003. GFP, Green fluorescent protein.

Although increasing STAT3 did not change the way progenitors interpreted LIF, it did reduce the proportion of PAX6⁺ cells (Fig. 6D-F). STAT3 virus did not alter PCNA expressionsignificantly (data not shown), suggesting that the reductionin PAX6 did not simply reflect a reduction in dividing progenitors.A significant reduction in the proportion of PAX6⁺ cells was seen as early as 2 d after infection with STAT3 virus:6.9 ± 0.9% of STAT3-infected E12 cells were PAX6⁺, compared with 11.3 ± 1.3% of control-infected cells (n = 3;p = 0.04). As noted in Table 1, coexpression of PAX6 and STAT3declines between E15 and E17. Our findings suggest that elevatedSTAT3 may induce the decline in PAX6 expression. This could facilitatethe transition in cell fate specification from neurons to astrocytes,although expression of a high level of STAT3 is not sufficienton its own to alter responsiveness to LIF orBMP4.

LIF-induced STAT3 phosphorylation is enhanced by EGFRs and elevated STAT3

The induction of astrocytes by LIF is associated with the tyrosine phosphorylation and nuclear translocation of STAT3 (Bonniet al., 1997). We wondered whether increased STAT3 expressionfailed to confer astrocyte induction in response to LIF becauseof a limitation in STAT3 phosphorylation. To address this, weinfected progenitors at E11 and E13 with control, EGFR, or STAT3viruses and assessed the expression and nuclear localization ofphospho-STAT3 (Tyr⁷⁰⁵) 4 d later, after stimulation with LIF for 20min.

Cells infected with EGFR virus exhibited nuclear phospho-STAT3 staining after stimulation with LIF (Fig. 7A,B), as did cellsinfected with STAT3 virus (Fig. 7C,D). The proportion of phospho-STAT3⁺ cells observed after stimulation with LIF was greater among EGFR-infectedcells than control-infected cells at either E11 or E13 (Fig. 7E).The increase in phospho-STAT3 was greater at E13, although theproportion of EGFR-infected cells that express a high level ofSTAT3 is comparable at E11 and E13 (Fig. 5D). The difference inLIF-induced STAT3 phosphorylation at E11 and E13 is consistentwith the age-related difference in LIF-induced astrocyte developmentnoted in Figure 1. The ability of LIF to induce STAT3 phosphorylationappears to be developmentally regulated by an EGFR-independentmechanism that limits astrocyte development. Surprisingly, theproportion of STAT3 virus-infected cells that were phospho-STAT3⁺ after stimulation with LIF was comparable with that observedamong EGFR-infected cells (Fig. 7E). This suggests that the failureof STAT3 elevation to confer astrocyte induction in response toLIF does not reflect a limitation of its phosphorylation. Instead,astrocyte induction by LIF appears to be limited downstream ofSTAT3 phosphorylation. Elevated expression of EGFRs can overcomethis limitation to turn LIF into an astrocyte-inducing signal.

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Figure 7. LIF induces STAT3 phosphorylation. E13 explants were infected with EGFR virus (A, B) or STAT3 virus (C, D), dissociated 4 d later, stimulated with LIF for 20 min, and then stained with antibodies to phospho-STAT3 (A, C) and viral markers (B, D). E, The proportion of cells that respond to LIF by phosphorylating STAT3 (pSTAT3) is greater among EGFR-infected and STAT3-infected cells compared with control-infected cells at E11 and E13. $-$ , No LIF; +, addition of LIF. *p $<=$ 0.01; **p < 0.0001, comparing LIF with no LIF. More EGFR-infected and STAT3-infected cells responded to LIF at E13 than at E11 (p < 0.0025).

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Our previous work suggested that a developmental change in cortical progenitor expression of EGFRs contributed to the transitionfrom neurogenesis to gliogenesis (Burrows et al., 1997). Othershave shown that progenitor competence to interpret LIF/CNTF andBMP as astrocyte-inducing signals is acquired during late embryonicdevelopment in rat and mouse cortex (Li et al., 1998; Mehler etal., 2000; Molne et al., 2000). In the present study, we examinedthe relationship between the increase in EGFR expression and theacquisition of competence to interpret LIF and BMP as astrocyte-inducingsignals. We demonstrated that EGFRs regulate the change in responsivenessto LIF but not to BMPs (Fig. 8). To address the molecular mechanismunderlying this effect of EGFRs, we tested the idea that the expressionof STAT3, which mediates astrocyte differentiation, is regulatedby EGFRs and is sufficient for the effect of EGFRs on LIF responsiveness.We show that EGFRs upregulate levels of STAT3 and its phosphorylationin response to LIF, and that STAT3 misexpression downregulatesthe neurogenic factor PAX6. Increased STAT3 expression also enhancesLIF-induced phosphorylation of STAT3, but this does not inducethe change in LIF responsiveness to astrocyte induction. Our findingssuggest that EGFRs overcome a limitation downstream of STAT3 elevationand phosphorylation that allows LIF to induce astrocytes.

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Figure 8. Relationship between EGFR expression and responsiveness to LIF. Progenitors that express low (A) or no (D) EGFRs generate neurons when stimulated with LIF, whereas progenitors that express a high level of EGFRs (B, C) generate astrocytes in response to LIF.

How does increased EGFR expression alter LIF responsiveness?

Our observation that EGFR-null progenitors fail to undergo the normal developmental change in responsiveness to LIF suggeststhat the EGFR is required for this change to occur. This contradictsa previous study suggesting that EGFRs were not required. Thisinterpretation was based on the observation that an inhibitorof the EGFR tyrosine kinase did not prevent the developmentalchange in responsiveness to CNTF/LIF (Zhu et al., 2000). Mutantforms of the EGFR that lack intrinsic tyrosine kinase activityhave been shown to mediate signal transduction, as least in partby serving as a substrate for other kinases and a scaffold forthe assembly of signal transduction complexes (Wright et al.,1995; Yamauchi et al., 1997; Deb et al., 2001). In cortical progenitors,EGFRs might therefore regulate responsiveness to LIF by such akinase-independentmechanism.

It has been suggested that the process of gliogenesis can be separated into two steps that are regulated by distinct extrinsicsignals. Restriction to a glial fate could first be specifiedby a signal such as FGF2, followed by terminal differentiationinto astrocytes in response to CNTF/LIF (Morrow et al., 2001).Where does the EGFR fit in? EGFR activation per se does not restrictfate to gliogenesis (Reynolds and Weiss, 1992; Ferri and Levitt,1995; Burrows et al., 1997; Morrow et al., 2001). Instead, EGFRstimulation appears to block restriction to a neuronal fate (Fig.1C), maintaining progenitors in a multipotent state that allowsthe generation of both neuronal and glial progeny (Burrows etal., 1997; Morrow et al., 2001). We reported previously that EGFRsenhance proliferation in addition to promoting astrocyte development(Burrows et al., 1997). The impact of EGFRs on LIF responsivenesscould reflect mitotic expansion of multipotent cells that arecompetent to interpret LIF as an astrocyte-inducing signal. Wedid not observe a selective effect of EGFR virus on survival;for example, after 4 d in vitro, 1.4 ± 0.5% of control-infectedE13 cells expressed activated caspase 3, a marker of dying cells,compared with 1 ± 0.7% of EGFR-infected cells (n = 4). It is thereforenot likely that selective survival of a progenitor subpopulationunderlies the impact of EGFRs on LIFresponsiveness.

Previous work has shown that FGF2 promotes astrocyte differentiation in response to LIF (Molne et al., 2000; Morrow et al.,2001). The present study shows that this effect of FGF2 requiresEGFRs. We have shown previously that FGF2 induces expression ofa high level of EGFRs prematurely (Lillien and Raphael, 2000).Normally, during development, these signals may act sequentially,with FGF2 inducing an increase in EGFR expression, which thenalters responsiveness toLIF.

Regulation of STAT3 expression and phosphorylation

Early progenitors express STAT3 as well as functional LIF receptors (Molne et al., 2000), but we noticed an increase in thelevel of STAT3 expression among a subpopulation of progenitors,beginning at E15. Over 2 d, the size of the population that expresseda high level of STAT3 increased. At E17, approximately one-halfof the STAT3^high cells coexpressed a high level of EGFRs. These observations suggesteda causal relationship between EGFRs and the level of STAT3. Severallines of evidence support the idea that EGFRs contribute to thedevelopmental increase in STAT3 expression. First, a prematureelevation of EGFRs induced a premature increase in STAT3 expression.Second, the proportion of STAT3^high cells was reduced in late embryonic EGFR-null cortex. Not allSTAT3^high cells expressed a high level of EGFRs, suggesting that additionalmechanisms contribute to the regulation of STAT3expression.

It has been suggested that the choice between neurogenesis and gliogenesis depends at least in part on a competitive relationshipbetween the neurogenic factor ngn1 and STAT3 for limiting concentrationsof CREB binding protein/p300 (Sun et al., 2001). This hypothesisimplies that increasing the ratio of STAT3 to neurogenic factorsmight shift the balance and promote gliogenesis. Several observationssupport the idea that increased STAT3 expression contributes toneuron-astrocyte choice. The developmental increase in STAT3 leveloccurs during the transition from neurogenesis to gliogenesis.At E15, 40-50% of the STAT3^high cells coexpressed PAX6, which has been shown to promote a neuronalfate (Heins et al., 2002). Over 2 d, however, the proportion ofSTAT3^high cells that coexpressed PAX6 declined. When we bypassed the EGFRand increased STAT3 prematurely with a retrovirus, PAX6 expressiondeclined. The increase in STAT3 expression might therefore contributeto the transition from neurogenesis to gliogenesis by regulatingPAX6. PAX6 is a positive regulator of ngn2 (Scardigli et al.,2001; Heins et al., 2002), so it is possible that STAT3 upregulationcould indirectly reduce ngn2 expression by negatively regulatingPAX6.

In contrast to increased EGFR expression, increasing STAT3 with a retrovirus was not enough to change responsiveness to LIF,BMPs, or the combination of these factors. Activation of thresholdlevels of EGFRs therefore changes LIF responsiveness by additionalmechanisms, although elevated STAT3 could still be required forthe change in LIF responsiveness. Increasing STAT3 in the absenceof exogenous LIF induced a small increase in the early astrocytemarker S-100 $beta$ that was comparable with the response of control-infectedcells to LIF. Increased STAT3 expression might therefore sensitizecells to endogenous signal(s) that initiate astrocyte differentiation,but it does not appear to be sufficient to drive cells to a GFAP⁺ state. The endogenous signals responsible for this effect onS-100 $beta$ expression have not been identified but could includeLIF.

LIF activation of STAT3 signaling involves phosphorylation of STAT3 on tyrosine 705 (Bonni et al., 1997). We found that theability of LIF to induce STAT3 phosphorylation was enhanced byelevating EGFRs. Moreover, when we bypassed EGFRs and increasedthe level of STAT3 directly, the ability of LIF to induce STAT3phosphorylation was also enhanced. Because this was not enoughto cause LIF to induce astrocytes, something downstream of STAT3phosphorylation appears to be limiting. It has been noted thatmethylation of the GFAP promoter is developmentally regulatedand also serves to limit astrocyte development (Takizawa et al.,2001). Elevated EGFR expression is able to overcome limitationsdownstream of STAT3 phosphorylation to confer astrocyte inductionby LIF. It remains to be determined whether EGFRs achieve thisby altering methylation or antagonizing one of the inhibitorsof LIF signaling downstream of phospho-STAT3, such as PIAS3 (proteininhibitor of activated STAT3) (for review, see O'Shea et al.,2002).

Conclusions

Several lines of evidence implicate EGFRs in the generation of astrocytes. For example, astrocyte development is abnormalin EGFR-null mice (Kornblum et al., 1998), and misexpression ofEGFRs in vivo promoted astrocyte development prematurely (Burrowset al., 1997). Results from the present study demonstrate thatEGFRs can regulate the development of astrocytes by modulatingresponsiveness to heterologous signals such as LIF. Although EGFRscontribute to astrocyte generation, astrocytes can also be inducedby EGFR-independent mechanisms. For example, FGF2 and BMP4 inducedastrocyte development in EGFR-nullcells.

We observed developmental changes in the effectiveness of EGFR stimulation in eliciting changes in STAT3 phosphorylation andLIF responsiveness (Figs. 1A, 7E). Thus, additional developmentallyregulated events appear to restrict astrocyte generation in theearly embryonic cortex. Astrocyte induction by LIF/CNTF is inhibitedby a number of extrinsic and intrinsic molecules. These includePDGF (Park et al., 1999), C/EBP (CCAAT/enhancer-binding protein)(Menard et al., 2002), and SOCS (suppressor of cytokine signaling)family members (for review, see Turnley and Bartlett, 2000). Theability of EGFRs to change LIF responsiveness in early progenitorscould be limited by these molecules. EGFRs did not regulate changesin responsiveness to BMPs, indicating that astrocyte inductionby these molecules is controlled by distinct mechanisms that remainto beidentified.

  FOOTNOTES

Received Oct. 9, 2002; revised Jan. 15, 2003; accepted Feb. 5, 2003.

This work was supported by National Institutes of Health Grant RO1 NS38306. We thank Amy Sinor and Alexandra Gulacsi for theircomments on thismanuscript.

Correspondence should be addressed to Dr. Laura Lillien, Department of Neurobiology and Pittsburgh Cancer Institute, Universityof Pittsburgh School of Medicine, W1454 Biomedical Science Tower,Pittsburgh, PA 15261. E-mail: lillien+{at}pitt.edu.

  References

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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