Integrin alpha 5/beta 1 Mediates Fibronectin-dependent Epithelial Cell Proliferation through Epidermal Growth Factor Receptor Activation

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Vol. 11, Issue 7, 2485-2496, July 2000

Integrin $alpha$ 5/ $beta$ 1 Mediates Fibronectin-dependent Epithelial Cell Proliferation through Epidermal Growth Factor Receptor Activation

Scott K. Kuwada,^* and Xiufen Li

Division of Gastroenterology, University of Utah and Salt Lake City Veterans Affairs Medical Center, Salt Lake City, Utah 84132

Submitted January 13, 2000; Revised March 14, 2000; Accepted April 25, 2000
Monitoring Editor: Joan Brugge

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Human integrin $alpha$ 5 was transfected into the integrin $alpha$ 5/ $beta$ 1-negative intestinal epithelial cell line Caco-2 to study EGF receptor(EGFR) and integrin $alpha$ 5/ $beta$ 1 signaling interactions involved in epithelialcell proliferation. On uncoated or fibronectin-coated plastic,the integrin $alpha$ 5 and control (vector only) transfectants grew atsimilar rates. In the presence of the EGFR antagonistic mAb 225,the integrin $alpha$ 5 transfectants and controls were significantlygrowth inhibited on plastic. However, when cultured on fibronectin,the integrin $alpha$ 5 transfectants were not growth inhibited by mAb225. The reversal of mAb 225-mediated growth inhibition on fibronectinfor the integrin $alpha$ 5 transfectants correlated with activation ofthe EGFR, activation of MAPK, and expression of proliferatingcell nuclear antigen. EGFR kinase activity was necessary for bothMAPK activation and integrin $alpha$ 5/ $beta$ 1-mediated cell proliferation.Although EGFR activation occurred when either the integrin $alpha$ 5-transfectedor control cells were cultured on fibronectin, coprecipitationof the EGFR with SHC could be demonstrated only in the integrin $alpha$ 5-transfected cells. These results suggest that integrin $alpha$ 5/ $beta$ 1mediates fibronectin-induced epithelial cell proliferation throughactivation of theEGFR.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Epithelial cells receive important cues from the environment through soluble growth factors and insoluble extracellular matrixproteins. The receptors chiefly responsible for this binding arethe growth factor receptors and integrins, respectively. The signalingtriggered by these receptors effect changes in critical cell functionsas diverse as proliferation, differentiation, and survival (Pignatelliand Bodmer, 1989; Streuli et al., 1991; Roskelley et al., 1994;Sastry et al., 1996; Giancotti, 1997; Somasiri and Roskelley,1999). With regard to cell cycle progression and proliferation,coordinated input from both growth factor receptors and integrinsis necessary (Clark and Brugge, 1995; Zhu and Assoian, 1995, 1996;Wary et al., 1996, 1998; Schwartz and Baron, 1999).

How growth factor and integrin signal transduction pathways are actually integrated in controlling cell functions is not wellunderstood. Most studies have used mesenchymal cells and bolusesof exogenous growth factors to stimulate growth factor receptoractivity. Such acute conditions are not usually found in normaltissue. Epithelial cells are usually regulated by autocrine growthfactor loops (Ferriola et al., 1991, 1992; Bishop et al., 1995;Damstrup et al., 1999). Autocrine growth factor activation ofthe EGF receptor (EGFR) is best described as a steady-state systemas it approximates normal cell physiology in vivo (Wiley and Cunningham,1981). Epithelial cells would rarely be exposed in vivo to acuteand large concentrations of growth factors. In addition, the exposureof cells to boluses of EGF family growth factors usually resultsin only transient activation of the EGFR. The use of epithelialcells is clinically relevant in that they are the frequent targetsof diseases, such as adenocarcinoma, in which aberrant growthis a characteristicfinding.

Both integrins and the EGFR activate common members of the RAS-ERK signal transduction pathway (Pages et al., 1993; Chen etal., 1994; Lange-Carter and Johnson, 1994; Kelleher et al., 1995;Morino et al., 1995; Zhu and Assoian, 1995, 1996; Miyamoto etal., 1996). Growth factor-induced cell proliferation is mediatedby the MAPKs, also known as extracellular signal-regulated kinases(ERKs) (Pages et al., 1993; Aliaga et al., 1999). Although integrinsand the EGFR can activate ERK independently, the emerging pictureis that ERK activation must exceed a threshold to drive cell proliferation.Exceeding this threshold requires input from both integrins andgrowth factor receptors (Zhu and Assoian, 1995, 1996; Schwartzand Baron, 1999). How integrin and growth factor receptor signalingare integrated proximal to ERK is not wellunderstood.

At present, there are three known mechanisms by which integrins can activate ERKs, and all three mechanisms involve RAS asthe activator of downstream MAPKs. The first mechanism is throughthe activation of Fyn by Shc, which is initially recruited byactivated integrins via caveolin (Wary et al., 1998). Interestingly,although integrins $alpha$ 1, $alpha$ 2, $alpha$ 3, $alpha$ 5, and $alpha$ V interact with caveolin,only $alpha$ 1/ $beta$ 1, $alpha$ 5/ $beta$ 1, or $alpha$ V can recruit Shc and activate Fyn (Waryet al., 1996, 1998). Shc then recruits Grb2 and SOS, the latterof which activates the RAS-ERK pathway. The second mechanism ofERK activation is through integrin-mediated focal adhesion kinaseactivation, which results in the recruitment of Grb2 (Schlaepferet al., 1994, 1998; Hanks and Polte, 1997), which in turn recruitsSOS and consequently leads to RAS activation. The third mechanismis integrin-mediated EGFR activation (Moro et al., 1998; Li etal., 1999), which also causes activation of Shc, Grb2, andRAS.

Epithelial cells express a large repertoire of various integrin receptors, and the redundancy of specific extracellular matrixproteins bound by these integrins complicates investigation. However,integrin $alpha$ 5/ $beta$ 1 possesses high-affinity binding only to fibronectin(Hemler, 1990). The Caco-2 intestinal epithelial cell line usedlacks detectable expression of the classic fibronectin receptor,integrin $alpha$ 5/ $beta$ 1, and EGFR expression and function have been characterizedextensively in this cell line (Hidalgo et al., 1989; Bishop andWen, 1994; Bishop et al., 1995; Tong et al., 1998; Kuwada et al.,1999). Although adding EGF family ligands, such as EGF, does notgreatly stimulate Caco-2 cell proliferation, interrupting autocrineEGF family growth factor activation of the EGFR can diminish cellproliferation significantly (Damstrup et al., 1999; Kuwada etal., 1999). Caco-2 cells were transfected with integrin $alpha$ 5 tostudy signaling interactions between integrin $alpha$ 5/ $beta$ 1 and the EGFRthat are involved in the control of epithelial cellproliferation.

We asked specifically whether integrin $alpha$ 5/ $beta$ 1-mediated EGFR activation occurs in epithelial cells and what role this playsin cell proliferation. We found that integrin $alpha$ 5/ $beta$ 1 mediates fibronectin-inducedEGFR activation, which leads to EGFR-mediated activation of MAPKsand cellproliferation.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Antibodies and Kinase Inhibitors

Antibodies used were integrin $alpha$ 2 mAb (Becton-Dickinson, Franklin Lakes, NJ); integrin $alpha$ 3 mAb (Becton-Dickinson); integrin $alpha$ V mAb, phosphoserine mAb, EGFR mAb, rabbit anti-mouse immunoglobulinG (Zymed, San Francisco, CA); integrin $alpha$ 5 subunit (mAb 16, Becton-Dickinson;and polyclonal antibody, Chemicon); PY-20 mAb, phospho-p44/42MAPK E10 mAb, Shc polyclonal antibody, Grb2 mAb, ERK1 mAb, MEK1,proliferating cell nuclear antigen (PCNA) mAb (Transduction Laboratories,Lexington, KY); and alkaline phosphatase-conjugated goat anti-rabbitantibody (Jackson Immunoresearch, West Grove, PA). The MEK1 inhibitorPD 98059 (Calbiochem, La Jolla, CA) and the EGFR kinase inhibitorCompound 32 (PD 153035; Calbiochem) were solubilized inDMSO.

Integrin $alpha$ 5 Gene Construct

The human integrin $alpha$ 5 gene (in the plasmid pECE) was obtained as a generous gift from Dr. Erkki Ruoslahti. The SalI-XbaI fragmentencompassing the integrin $alpha$ 5 gene was cloned into the XhoI andXbaI sites of the vector pcDNA3 (Invitrogen, Carlsbad, CA), whichhas a G418 resistancegene.

Cell Lines, Tissue Culture, and Transfection

Caco-2 cells were obtained as a gift from Dr. Robert J. Coffey, Jr., and maintained in DMEM (ICN Biomedical, Costa Mesa, CA)supplemented with fibronectin-free 10% FBS (Hyclone, Logan, UT),glutamine, penicillin, and streptomycin in a 37°C humidified tissueculture incubator with a 5% CO₂ environment. The cells were culturedon uncoated or fibronectin-coated (10 µg/ml; Sigma Chemical, St.Louis, MO) 35-mm bacterial plastic dishes (Falcon), 35-mm tissueculture dishes (Greiner), and 96-well tissue culture plastic dishes(Greiner). When mAb 225 (Imclone) and integrin mAb (Becton-Dickinson)were used, they were mixed with dispersed cells to a final concentrationof 10 and 5 µg/ml, respectively, just before cell plating. Compound32 (PD 153035), solubilized in DMSO, was added to cell culturemedium to achieve a final concentration of 4 µM (controls receivedan equal concentration of DMSOalone).

Caco-2 cells were transfected with the pcDNA3 vector alone or with the human integrin $alpha$ 5-pcDNA3 construct by a calcium phosphatemethod. Caco-2 cells between passages 90 and 95 were grown to~70% confluence on 100-mm dishes. Ten to 40 µg of plasmid DNApreparations (Wizard Preparations, Promega, Madison, WI) wereadded to sterile 1× TE buffer to a total volume of 500 µL. Fiftymicroliters of sterile 2.5 M CaCl₂ in 10 mM HEPES, pH 7.2 wasadded to the plasmid DNA and mixed thoroughly. The calcium-DNAsolution was then dripped into 0.5 ml of sterile 2× HEBS bufferwith vigorous mixing every three drops. The mixture was incubatedat room temperature for 30 min. The entire mixture was then addedto the 10 ml of culture medium bathing the cells. The medium wasaspirated off the next day, the cells were washed twice with PBS-EDTA,and fresh medium was added. Forty-eight hours after the transfectionprocedure, the cells were dispersed in trypsin and replated in10 ml of medium containing 1.5 mg/ml G418 (LD curves demonstratedthat a G418 final concentration of at least 1.2 mg/ml was neededto kill all Caco-2 cells in culture). Approximately 25-30 cellcolonies were obtained, and the individual clones were removedwith trypsin with the use of cloning cylinders (Bellco). The individualcolonies were plated on 12-well plates in medium containing 1.5mg/ml G418. Once confluent colonies were obtained in 12-well plates,the cells were replated on 10-cm dishes. During all steps, thecell culture medium was exchanged every 2d.

For the soft agar proliferation assay, a 1.6% low-melting-point agar solution (in water) was microwaved until boiling andthen cooled in a 37°C water bath. The agar solution was mixed1:1 with 2× medium, and 1 ml of this solution was plated in 35-mmtissue culture plastic dishes. A total of 20,000 cells were addedto a solution containing 2× medium and 1× medium in a 1:2 ratio(3 ml total volume per dish). Then, 1 ml of liquid 1.6% agar solution(at 37°C) was added to the cell mixture, which was vortexed gentlyto disperse the cells. One milliliter of the cell mixture waslayered onto the bottom of the dish and left at room temperatureuntil the agar solidified. The cells were placed in a 37°C incubatorwith 5% CO₂ and photographed eachday.

Expression of Integrins by Caco-2 Cells

Flow cytometry and immunoblotting were used to evaluate cells for the expression of various integrins. For flow cytometricanalysis of integrin expression, cells were dispersed in 0.25%trypsin in PBS-EDTA and washed twice in PBS-EDTA. The cells werethen mixed at 37°C with integrin $alpha$ 5 mAb (Becton-Dickinson) ata dilution of 1:500 in blocking buffer A (1% radioimmunoassay-gradeBSA [Bio-Rad, Richmond, CA] in PBS) for 60 min. The cells werewashed twice in blocking buffer A, mixed with a 1:1000 dilutionof FITC-labeled rabbit anti-mouse mAb (Jackson Immunoresearch)in blocking buffer A, and incubated at 37°C for 30 min. The cellswere washed twice in PBS-EDTA and assayed with a flow cytometer(Becton-Dickinson). Integrin expression was determined to be thepercentage of FITC-positive cells. The gate setting was determinedby the fluorescence intensity of the same cells stained with FITC-conjugatedsecondary antibodyonly.

For immunodetection of integrin $alpha$ 5 expression, cells were cultured for 2 d on plastic dishes and then prepared according tothe immunoprecipitation protocol described below. For immunoprecipitation,2 µg of integrin $alpha$ 5 mAb (Becton-Dickinson) was added to each tubeof lysate, and the primary antibody used for immunodetection wasintegrin $alpha$ 5 polyclonal antibody (Chemicon) used at a 1:1000 dilutionin blocking bufferB.

Immunoprecipitation and Immunodetection

For immunoprecipitation, cells were lysed in 4°C lysis buffer (50 mM HEPES, 150 mM NaCl, 1.5 mM MgCl₂, 1 mM EGTA, 100 mM NaF,10 mM Na₂PO₄, 1 mM Na₃VO₄, 10% glycerol, 1% Triton X-100, and1 µg/ml each of aprotinin, leupeptin, chymostatin, and pepstatin)and clarified at 12,000 rpm at 4°C for 15 min. The lysates werethen normalized for protein concentration to a total volume of1 ml in lysis buffer. Antibody (1-2 µg) was added to each tubeof lysate, which was then incubated on a rocker at 4°C for 2 h.The antibodies were immunoprecipitated with 50 µl of a slurryof protein A/G-Sepharose beads (Calbiochem) for 1 h on a rockerat 4°C. The beads were washed twice with lysis buffer and thenboiled in sample buffer (125 mM Tris-HCl, pH 6.8, 20% glycerol,4% SDS, 2% $beta$ -mercaptoethanol, 10 µg/ml bromphenol blue) for 3min. The beads were pelleted by brief centrifugation, and thesupernatants were loaded on SDS-PAGE gels (7.5 or 10% acrylamide).The proteins were transferred to nitrocellulose and then incubatedin blocking buffer B (1% BSA [Bio-Rad], 100 mM Tris-Cl, pH 7.4,0.9% NaCl, 0.1% Nonidet) overnight at 4°C.

For immunodetection, the blocked blots were probed with primary antibody for 2 h at 4°C on a rocker. The blots were washedtwice for 10 min each in blocking buffer B and then incubatedwith a 1:2000 dilution of a rabbit anti-mouse secondary antibody(for monoclonal primary antibodies). After two washes in blockingbuffer B, the blots were finally incubated either with a 1:5000dilution of alkaline phosphatase-conjugated rabbit anti-mouseantibodies (Jackson Immunoresearch) or 50 ng/ml ¹²⁵I-protein A in blocking buffer B. Alkaline phosphatase was detectedby a colorimetric reaction with the use of a 5-bromo-4-chloro-3-indolylphosphate/nitroblue tetrazolium kit (Zymed). ¹²⁵I-protein A-labeled blots were detected with the use of a MolecularImager FX (Bio-Rad).

Cell Proliferation Assay

Cells were dispersed and plated at 40,000 cells per well in 96-well dishes. At various days in culture, the cells were gentlywashed twice with 100 µl per well of ice-cold blocking bufferA and twice with 100 µl per well of ice-cold PBS. The cells werefixed for 10 min in 100% ice-cold methanol (100 µl per well) andthen allowed to air-dry. The cells were stained with 100 µl perwell of 0.1% crystal violet in water for 10 min and then washedgently four times with double-distilled water and four times withPBS. The plates were then air-dried completely. The stained cellswere solubilized in 1% sodium deoxycholate, and the plates wereread at 590 nm in a spectrophotometer. The absorption at 590 nmis proportional to the number of attached cells (our unpublishedresults).

Signal Transduction

Cells were incubated in cell culture medium supplemented with mAb 225 (10 µg/ml final concentration), mAb integrin $alpha$ 5 (Becton-Dickinson;5 µg/ml final concentration), PD 98059 (20-100 µM final concentration),or Compound 32 (4 µM final concentration) for various numbersof days. The degree of activation for immunoprecipitated EGFR,Shc, and Grb2 proteins was determined by immunodetection of antiphosphotyrosinewith PY-20 mAb (1:2000 dilution in blocking buffer B; see Immunoprecipitationand Immunodetection for details). Activation of ERK1 and ERK2was determined by immunodetection of cell lysates with phospho-MAPKE10 mAb (1:2000 dilution in blocking buffer B). Activation ofMEK1 was determined by immunodetection of MEK1 immunoprecipitateswith phosphoserine mAb (1:1000 dilution in blocking buffer B).Loading control experiments were performed by immunodetectionof immunoprecipitates or lysates with EGFR mAb (1:500 dilutionin blocking buffer B), Shc polyclonal antibody (1:5000 dilutionin blocking buffer B), Grb2 mAb (1:2000 dilution in blocking bufferB), ERK1 mAb (1:2000 dilution in blocking buffer B), and MEK1mAb (1:1000 dilution in blocking buffer B). PCNA expression wasdetermined by immunodetection of cell lysates with PCNA mAb (1:5000dilution in blocking bufferB).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Expression of Integrins in Caco-2 Cells

Caco-2 cells expressed integrins $alpha$ 2, $alpha$ 3, $alpha$ 4, $beta$ 1, $beta$ 3, $beta$ 4, and $alpha$ V, but not $alpha$ 5, by indirect immunofluorescence microscopy (ourunpublished results). Flow cytometry with two different mAbs raisedagainst the human $alpha$ 5 integrin subunit failed to detect $alpha$ 5 integrinsubunit expression in Caco-2 cells (Figure 1A, left panel), whereasanother colonic epithelial cell line, SW-620, was positive forintegrin $alpha$ 5 expression by flow cytometry (Figure 1A, right panel).

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Figure 1. (A) Flow cytometry of Caco-2 and SW-620 cells demonstrating integrin $alpha$ 5 expression (gray areas). (B) Flow cytometry of Caco-2 cell lines, A105 and A9, stably transfected with integrin $alpha$ 5 (gray areas). The cells were stained with an integrin $alpha$ 5 mAb and FITC-conjugated goat anti-mouse antibodies or with FITC-labeled goat anti-mouse antibodies alone (controls; unshaded areas). The ordinate represents the number of cells counted (in thousands) and the abscissa the fluorescein intensity. (C) Immunoblots of integrin $alpha$ 5 immunoprecipitates from Caco-2 cells stably transfected with vector alone (B6 and B7) and integrin $alpha$ 5. A single ~120-kDa band (arrow), corresponding to the heavy chain of integrin $alpha$ 5, was obtained under reducing conditions. (D) Integrin $alpha$ 3, $alpha$ 4, and $alpha$ V subunit expression in the control and integrin $alpha$ 5-transfected cells determined by flow cytometry. The transfectants were stained with integrin $alpha$ 3, $alpha$ 4, and $alpha$ V mAbs followed by FITC-conjugated goat anti-mouse antibodies. For each integrin subunit, the fluorescence intensity was expressed as a percentage of the controls (stained with FITC-conjugated goat anti-mouse antibodies alone).

Caco-2 cells were transfected with the human integrin $alpha$ 5 subunit or vector alone (controls). Two stable integrin $alpha$ 5 transfectants(A105 and A9) and two stable control transfectants (B6 and B7)were isolated after selection in G418 and used in all subsequentexperiments. Integrin $alpha$ 5 expression was confirmed in the transfectantsby flow cytometry (Figure 1B) and Western blot analysis of integrin $alpha$ 5 immunoprecipitates (Figure 1C). Because other integrin receptorsubunits are involved in fibronectin binding ( $alpha$ 3/ $beta$ 1, $alpha$ 4/ $beta$ 1, and $alpha$ V), the expression of integrin $alpha$ 3, $alpha$ 4, and $alpha$ V was compared betweenthe integrin $alpha$ 5 transfectants and control cells by flow cytometry(Figure 1D). The integrin $alpha$ 5 transfectants and control cells expressedthe integrin $alpha$ 3, $alpha$ 4, and $alpha$ V subunits at similar levels exceptfor clone B6, which expressed lower levels of integrin $alpha$ V, whichprobably represents minor clonalvariation.

Fibronectin Overcomes Inhibition of EGFR-mediated Cell Proliferation

Autocrine growth factor signaling by the EGFR has been shown to be important in Caco-2 cell proliferation. We have shown thatexogenously applied EGF family growth factors have little effecton Caco-2 cell proliferation. This may be because the cells alreadyexpress EGF family ligands (amphiregulin, TGF $alpha$ , EGF, and HB-EGF).(Damstrup et al., 1999; Kuwada et al., 1999). However, incubatingCaco-2 cells with EGFR-blocking antibodies significantly reducescell proliferation by interrupting autocrine growth factor binding(Damstrup et al., 1999; Kuwada et al., 1999).

The Caco-2 integrin $alpha$ 5 transfectants grew at similar rates as the control cells on plastic (Figure 2, A and B) or fibronectin-coatedplastic (Figure 2, C and D). In the absence of exogenous fibronectin,both the integrin $alpha$ 5 transfectants (Figure 2A) and control cells(Figure 2B) demonstrated significant inhibition of cell proliferationin the presence of 10 µg/ml of the antagonistic EGFR mAb 225,which inhibits ligand binding to the EGFR, resulting in diminishedEGFR tyrosine kinase activity (Gill et al., 1984). On fibronectin-coatedplastic, however, the integrin $alpha$ 5 transfectants grew at nearlythe same rate in the absence or presence of mAb 225 (Figure 2C).In contrast, the control cells were growth inhibited to a similardegree by mAb 225 on uncoated or fibronectin-coated plastic (Figure2, compare B and D). In addition, mAb 225 inhibited fibronectin-inducedexpression of the cell cycle protein PCNA in the control cellsbut not in the integrin $alpha$ 5-transfected cells at d 2 in culture(Figure 3). Thus, the inhibition of autocrine EGFR-mediated cellcycle progression and proliferation was overcome in the integrin $alpha$ 5/ $beta$ 1-expressing cells in the presence of exogenous fibronectin.This ability of the integrin $alpha$ 5/ $beta$ 1-expressing cells to overcomeEGFR inhibition appeared to occur early during the 7-d cell proliferationstudies when the Caco-2 cells were subconfluent. This may reflectmore of a role for integrin $alpha$ 5/ $beta$ 1-mediated cell proliferationwhen Caco-2 cells are rapidly proliferating and not yet fullydifferentiated.

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Figure 2. Proliferation assays of control and integrin $alpha$ 5-transfected cells on plastic in the presence (

) or absence (

) of mAb 225. (A) Integrin $alpha$ 5-transfected cells cultured on plastic. (B) Control cells cultured on plastic. (C) Integrin $alpha$ 5-transfected cells cultured on fibronectin-coated plastic. (D) Control cells cultured on fibronectin-coated plastic. Cell counts were estimated with the use of a crystal violet staining method. The ordinate represents the optical density at 590 nm and the abscissa the number of days in culture. Cells were plated at 50,000 cells per well in 96-well plates at day 0. Each data point represents the average ± SEM of triplicate experiments.

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Figure 3. Immunoblot of PCNA performed on lysates of control and integrin $alpha$ 5-transfected cells cultured for 2 d on uncoated or fibronectin (Fn)-coated plastic in the absence of presence of mAb 225 (10 µg/ml). All lanes represent equal total protein concentrations.

To determine whether EGFR kinase activity was essential to the ability of the integrin $alpha$ 5-transfected cells to overcome mAb225-mediated growth inhibition on fibronectin, we performed parallelproliferation studies with the use of the tyrphostin Compound32. Compound 32 directly inhibits EGFR tyrosine kinase activityby competing for the ATP-binding site. Compound 32, used at afinal concentration of 4 µM, caused a significant inhibition ofcell proliferation for the integrin $alpha$ 5-transfected (Figure 4A)and control (Figure 4B) cells on plastic and inhibited EGFR autophosphorylation(our unpublished results). Unlike the case for mAb 225, culturingthe integrin $alpha$ 5-transfected cells on fibronectin-coated plasticcould not reverse the growth inhibition caused by compound 32(Figure 4A). These results suggested that EGFR kinase activitywas necessary for the integrin $alpha$ 5-transfected cells to overcomemAb 225-mediated growth inhibition in the presence of fibronectin.This implied that fibronectin might induce EGFR activation.

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Figure 4. Proliferation assays of control and integrin $alpha$ 5-transfected cells cultured on uncoated or fibronectin-coated plastic in the presence or absence of 4 µM Compound 32. (A) Integrin $alpha$ 5-transfected cells cultured on plastic without (

) and with ( $triangle$ ) Compound 32 or on fibronectin without (

) and with ( $black-diamond$ ) Compound 32. (B) Control cells cultured on plastic without (

) and with ( $triangle$ ) Compound 32 or on fibronectin without (

) and with ( $black-diamond$ ) Compound 32. Each data point represents the mean ± SEM for experiments performed in triplicate.

Integrin $alpha$ 5/ $beta$ 1-mediated Activation of the EGFR

Recent reports showed that the EGFR could be activated by integrin-mediated fibronectin binding (Moro et al., 1998), evenin the absence of growth factors (Li et al., 1999). Therefore,we examined whether the EGFR was activated by adhesion to fibronectinin the integrin $alpha$ 5-transfected and control cells. We found thatthe EGFR was activated in both the control and integrin $alpha$ 5-transfectedcells when adhered to fibronectin but not to plastic (Figure 5A).

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Figure 5. Control (B6) and integrin $alpha$ 5-transfected (A105) cells were cultured for 2 d on uncoated or fibronectin-coated plastic in the presence or absence of mAb 225 (10 µg/ml). Immunoprecipitates of EGFR, Shc, and Grb2 were obtained from lysates normalized for total protein and resolved by SDS-PAGE. Immunoblotting was then performed. (A) Phosphotyrosine (top panels) and EGFR (bottom panels) immunoblots of EGFR immunoprecipitates. (B) Phosphotyrosine (top panels) and Shc (bottom panels) immunoblots of Shc immunoprecipitates. (C) Phosphotyrosine (top panels) and Grb2 (bottom panels) immunoblots of Grb2 immunoprecipitates.

The EGFR can activate Shc and Grb2, signaling proteins important in EGFR-mediated cell proliferation (Rozakis-Adcock et al.,1993; Sasaoka et al., 1994). Thus, we examined their levels oftyrosine phosphorylation in the control and integrin $alpha$ 5-transfectedcells (Figure 5, B and C). The levels of tyrosine phosphorylationof Shc and Grb2 were similar between the integrin $alpha$ 5 transfectantsandcontrols.

Although the levels of tyrosine phosphorylation of total cellular Shc protein were similar under the various conditions, onlya small proportion of total cellular Shc may be recruited by activatedEGFR. Therefore, the levels of EGFR protein associated with Shcwere studied in the control and integrin $alpha$ 5-transfected cells.The control and integrin $alpha$ 5 transfectants were grown on eitheruncoated or fibronectin-coated plastic for 2 d and then lysed.The presence of EGFR protein, tyrosine phosphorylated EGFR, andShc protein was detected in Shc immunoprecipitates. Although Shcwas immunoprecipitated from all the cell lysates under the variousconditions at equal levels (Figure 6A, left panel), EGFR proteincoprecipitated with Shc only in the integrin $alpha$ 5-transfected cellscultured on fibronectin-coated plastic (Figure 6B, right panel).Furthermore, EGFR protein that coprecipitated with Shc in theintegrin $alpha$ 5-transfected cells was tyrosine phosphorylated (Figure6C, right panel), which is consistent with previous reports thatShc binds only to activated EGFR (Pelicci et al., 1992; Ruff-Jamisonet al., 1993; Sasaoka et al., 1994). Thus, the interaction ofShc with the EGFR was exclusive to the integrin $alpha$ 5 transfectantsthat were cultured on fibronectin.

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Figure 6. Shc (A), EGFR (B), and phosphotyrosine (C) immunoblots were performed on Shc immunoprecipitates from control and integrin $alpha$ 5-transfected cells grown for 2 d on uncoated (P) or fibronectin-coated (Fn) plastic. Shc immunoprecipitation was performed on the different lysates that had been normalized for total protein. Each of the immunoprecipitates was then divided into three aliquots, which were used to generate the different immunoblots in A, B, and C. Panel A shows that equal amounts of Shc were immunoprecipitated from the different cell lysates.

Integrin $alpha$ 5/ $beta$ 1 and EGFR-mediated MAPK Activation

Activated EGFR and integrin $alpha$ 5/ $beta$ 1 can recruit both Shc and Grb2. Grb2 then recruits SOS, which activates RAS and leads tothe recruitment of Raf to the cell membrane. Raf then activatesMEK1, which in turn activates ERK1 and ERK2. Because MAPKs areimportant mediators of growth factor-induced cell proliferation(Pages et al., 1993; Cowley et al., 1994), we examined the abilityof integrin $alpha$ 5/ $beta$ 1 to activate ERK1 andERK2.

Integrin $alpha$ 5-transfected and control cells were cultured on uncoated or fibronectin-coated plastic dishes in the absence orpresence of mAb 225 for 8 d. At various times from 2 to 8 d inculture, the cells were lysed and Western blots with an activatedMAPK mAb were performed. Between 2 and 5 d in culture, significantdifferences in constitutive MAPK activation were seen betweenintegrin $alpha$ 5-transfected and control cells. When the control cellswere cultured on uncoated or fibronectin-coated plastic, the activationof ERK1 and ERK2 was significantly inhibited in the presence ofmAb 225 (Figure 7A, top left panel). Constitutive ERK1 and ERK2activation in the integrin $alpha$ 5 transfectants grown on plastic wasinhibited by mAb 225 (Figure 7A, top right panel). However, whenthe integrin $alpha$ 5-transfected cells were cultured on fibronectin-coatedplastic, ERK1 and ERK2 constitutive activation levels were notdecreased by the presence of mAb 225 (Figure 7A, top right panel).

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Figure 7. Control (B6 and B7) and integrin $alpha$ 5-transfected (A105 and A9) cells were cultured on uncoated or fibronectin-coated plastic in the presence or absence of mAb 225 for 2-4 d, after which they were lysed and normalized for total protein. (A) Immunoblots of phospho-MAPK (top panels) and ERK1 (bottom panels) were made from clones B6 and A105. Arrows indicate phosphorylated ERK1 and ERK2, both of which were detected by the phospho-MAPK mAb. (B) Immunoblots of phospho-MAPK (top panels) and ERK1 (bottom panels) were made from clones B7 and A9. (C) Immunoblots of phosphoserine (top panels) and MEK1 (bottom panels) were made from MEK1 immunoprecipitates from clones B6 and A105. Densitometry results of the bands are reported as ratios of the band densities of phospho-MAPK or phosphoserine to the respective loading controls.

Similarly, constitutive ERK1 and ERK2 activation was inhibited by mAb 225 in the control cell line B7, but not in the integrin $alpha$ 5-transfected cell line A9, when they were cultured on fibronectin(Figure 7B). When the integrin $alpha$ 5-transfected and control cellswere cultured on fibronectin in the presence of mAb 225 and anantifunctional integrin $alpha$ 5 mAb, ERK1 and ERK2 activation was unchangedin the control cells but was inhibited in the integrin $alpha$ 5 transfectants(our unpublished results). This demonstrated that the integrin $alpha$ 5/ $beta$ 1-fibronectin interaction was specifically responsible forthe activation of ERK1 and ERK2 in the integrin $alpha$ 5 transfectantsin the presence of mAb225.

Because MEK1 activates ERK1 and ERK2, we examined MEK1 activation. Activated (serine-phosphorylated) MEK1 was detected whenthe control cells (Figure 7C, top left panel) and integrin $alpha$ 5transfectants (Figure 7C, top right panel) were cultured on uncoatedor fibronectin-coated plastic. However, when the cells were culturedon fibronectin-coated plastic in the presence of mAb 225, activatedMEK1 was not detected in the control cells (Figure 7C, top leftpanel) but was detected in the integrin $alpha$ 5 transfectants (Figure7C, top rightpanel).

To determine whether MAPK activation was important to cell proliferation, the integrin $alpha$ 5 transfectants and controls weregrown on fibronectin-coated or uncoated plastic in the presenceor absence of the MEK inhibitor PD98059 for 8 d. In the presenceof 50 or 100 µM PD98059, the growth of the control cells and integrin $alpha$ 5 transfectants was significantly inhibited on plastic and fibronectin(our unpublished results). Treatment of the control cells andintegrin $alpha$ 5 transfectants with PD98059 (20 µM) significantly decreasedERK1 and ERK2 activation (our unpublished results). These resultsdemonstrated the overall importance of ERK1 and ERK2 activationto the proliferation of the integrin $alpha$ 5 transfectants and controlcells.

To determine whether EGFR kinase activity was necessary for ERK1 and ERK2 activation, the integrin $alpha$ 5-transfected and controlcells were grown in the presence of Compound 32 for 48 h, afterwhich ERK1 and ERK2 activation were determined. For both the integrin $alpha$ 5-transfected and control cells, Compound 32 resulted in thenear-total inhibition of activated ERK1 and ERK2 in the presenceor absence of fibronectin (our unpublishedresults).

These data suggested that ERK1 and ERK2 activation was dependent on the following: 1) EGFR kinase activity in both the integrin $alpha$ 5-transfected and control cells, and 2) autocrine EGFR activationin the control cells but not in the integrin $alpha$ 5-transfectedcells.

Because focal adhesion kinase (FAK) could potentially mediate integrin activation of MAPK, FAK tyrosine phosphorylation wasalso studied in the transfectants. No significant differencesin FAK tyrosine phosphorylation were seen for the control or integrin $alpha$ 5-expressing cells cultured on plastic or fibronectin-coatedplastic in the absence or presence of mAb 225 (our unpublishedresults).

Anchorage-independent Proliferation

A previous study showed that the expression of integrin $alpha$ 5 in the HT-29 colon cell line resulted in growth inhibition in theabsence of exogenous fibronectin (Varner et al., 1995). Therewas no growth arrest in the integrin $alpha$ 5-transfected versus controlCaco-2 cell lines in the absence of fibronectin. This may havebeen due to the fact that Caco-2 cells express fibronectin (Figure8A) and HT-29 cells reportedly do not. Our results seemed paradoxicalin that although the integrin $alpha$ 5-transfected cells expressed endogenousfibronectin, the reversal of mAb 225-mediated growth inhibitioncould occur only in the presence of exogenous fibronectin. Mostof the endogenous fibronectin protein recovered from the Caco-2transfectants was associated with the cells themselves (our unpublishedresults). The exogenous fibronectin was presented to the cellson a fixed, rigid, and planar surface. It has been reported thatexogenous fibronectin results in more robust cell adhesion inhuman epithelial cells (Wang et al., 1999). Furthermore, recentstudies have shown that extracellular matrix substrates can elicitcompletely different cellular responses depending on whether theyare presented to cells in a rigid or malleable form (Bissell andGuzelian, 1980; Bissell et al., 1987; Ben-Ze'ev et al., 1988;Garcia et al., 1999). This may be due to the ability of a rigidextracellular matrix to provide forces of tension to cellularstructures, which can effect specific signal transduction activity(Miyamoto et al., 1995, 1998). Fibronectin deposited on the cellsurface or presented to the cell in its malleable form, on theother hand, cannot provide fixed points against which cellularstructures can be anchored and tensioned.

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Figure 8. (A) Fibronectin immunoblot of control (B6 and B7) and integrin $alpha$ 5-transfected (A9 and A105) cell lines cultured on plastic for 4 d. (B) Photomicrographs (×40) of control (B7) and $alpha$ 5-transfected (A105) cell lines grown in soft agar for 6 d. Cells were seeded at the same density on d 1, and the assays were performed in triplicate.

To study this, we cultured the Caco-2 transfectants in soft agar in which any endogenous fibronectin could not be depositedas a rigid extracellular matrix. In soft agar, the integrin $alpha$ 5-transfectedcells were growth inhibited compared with the control cells (Figure8B). These results are similar to those in HT-29 colonic epithelialcells expressing integrin $alpha$ 5/ $beta$ 1 (Varner et al., 1995). Interestingly,the shape of Caco-2 cells cultured in soft agar is round (Figure8B), although they become columnar when cultured on a rigid surface(Hidalgo et al., 1989). Cell shape is important in determiningcell proliferation (Folkman and Moscona, 1978), and integrin-extracellularmatrix interactions are important transducers of changes in cellshape (Ingber, 1990). It appears that although Caco-2 cells expressfibronectin, only fibronectin presented to the cell as a rigidsubstrate can stimulate cell proliferation, presumably by bothclustering and activating fibronectin receptors. Thus, Caco-2cells transfected with integrin $alpha$ 5 are capable of depositing fibronectinon plastic, which may be sufficient to prevent integrin $alpha$ 5/ $beta$ 1-mediatedgrowth inhibition in thesecells.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Expression of human integrin $alpha$ 5 in Caco-2 cells resulted in significant differences in Caco-2 cell proliferation and signaltransduction events. Fibronectin reversed the growth inhibitionby mAb 225 for the integrin $alpha$ 5-transfected cells but not the controlcells. The reversal of mAb 225-mediated growth inhibition wasassociated with the activation of EGFR, MEK1, ERK1, and ERK2 andthe expression of PCNA. Furthermore, the fibronectin-mediatedactivation of ERK1 and ERK2 was specific to integrin $alpha$ 5/ $beta$ 1. Directinhibition of EGFR tyrosine kinase activity by Compound 32 decreasedcell proliferation and ERK1 and ERK2 activation. These effectsof Compound 32 could not be reversed by fibronectin. These resultssuggested that EGFR tyrosine kinase activity was necessary forthe fibronectin-induced and integrin $alpha$ 5/ $beta$ 1-mediated activationof ERK1 and ERK2 as well as cell proliferation. Furthermore, theinhibition of MAPK activity significantly decreased the proliferationof the control and integrin $alpha$ 5-transfected Caco-2cells.

Although tyrosine phosphorylation of the EGFR was seen in both the control and integrin $alpha$ 5-transfected cells cultured on fibronectin,the EGFR coprecipitated with Shc only in the integrin $alpha$ 5 transfectantsand in the presence of fibronectin. This suggests that the clusteringof integrin $alpha$ 5/ $beta$ 1 receptors by fibronectin resulted in the accessof activated EGFR to Shc. Integrins $alpha$ 1/ $beta$ 1 and $alpha$ 5/ $beta$ 1, but not other $beta$ 1-containing integrin receptors, are coupled to the Ras-ERK pathwaythrough Shc (Wary et al., 1996, 1998). Integrin clustering byfibronectin and integrin $alpha$ 5 antibodies leads to the formationof large signaling complexes containing many substrates of theEGFR, including Grb2 and Shc (Mainiero et al., 1995, 1997; Miyamotoet al., 1995, 1998; Wary et al., 1996, 1998). In addition, integrinscan cluster and coprecipitate with EGFRs (Miyamoto et al., 1996;Moro et al., 1998), and we were able to coprecipitate the EGFRwith integrin $alpha$ 5 from our integrin $alpha$ 5-transfected cells as well(our unpublished results). Although the activated EGFR can recruitboth Grb2 and Shc, the latter appears to be the preferred substratethrough which the EGFR activates SOS and then RAS (Sasaoka etal., 1994). Thus, fibronectin not only activates the EGFR butmay result in the spatial juxtaposition of Shc with activatedEGFRs. This suggests that integrins may play an important spatialregulatory role in controlling interactions between the EGFR andcertain substrates. Finally, on fibronectin, ERK1, ERK2, and MEK1were constitutively activated in the control and integrin $alpha$ 5-transfectedcells but were inhibited by mAb 225 only in the control cells.This suggests that the activation of ERK1 and ERK2 may have occurredthrough somewhat different mechanisms in the two celltypes.

Two recent studies that support our results demonstrated activation of the EGFR itself by integrin ligation. In one study,B82L fibroblasts migrated in response to EGF only when the cellswere adhered to fibronectin (Li et al., 1999). Furthermore, migrationof these cells was dependent on integrin-mediated activation ofan intact EGFR in a ligand (growth factor)-independent manner,thus placing the EGFR downstream of integrins for migratory signaling.In another study, when NIH 3T3 cells transfected with the humanEGFR were adhered to fibronectin, activation of EGFR, Shc, andERK1 occurred (Moro et al., 1998). This integrin-mediated activationof the EGFR occurred in the absence of growth factors and wasnecessary for cell survival and entry into S phase of the cellcycle in the presence of exogenous EGF or serum. Treatment ofthe cells with the EGFR-specific tyrphostin AG1478 or cotransfectionwith a dominant-negative mutant EGFR nearly abolished activationof EGFR, Shc, and ERK1 in response to adhesion to fibronectin.This again placed the EGFR downstream of integrins in integrin-mediatedERK1 activation. However, integrin-mediated activation of theEGFR alone was insufficient to drive cell proliferation in theabsence of exogenous growth factors, suggesting that integrinspotentiated growth factor-mediated activation ofERK1.

The mechanism by which integrin-mediated EGFR activation occurs is currently unknown. It is possible that EGFR activationoccurs through a ligand-dependent process such as intracrine EGFRactivation (Kennedy et al., 1993; Cao et al., 1995). However,intracrine EGFR activation has been described in only a few celltypes, and a growth factor-independent mechanism is more attractivebecause integrin-mediated EGFR activation occurred in cells devoidof any detectable EGF family growth factor expression (Moro etal., 1998; Li et al., 1999). Another potential mechanism is integrin-inducedactivation of the EGFR through heterodimerization with anothermember of the erbB family of receptors (Gamett et al., 1997; Graus-Portaet al., 1997). Caco-2 cells express erbB-2 receptors (our unpublisheddata), and heterodimerization of the EGFR with erbB-2 could leadto the transactivation of the EGFR even in the absence of EGFRligand-induced activation (Gamett et al., 1997; Worthylake etal., 1999). In addition, certain colon cancer cells have beenreported to express heregulins that stimulate cell proliferation(Vadlamudi et al., 1999). Heregulins can bind to erbB-3 and erbB-4receptors, which can in turn activate erbB-2, allowing it to heterodimerizewith and activate the EGFR. Whether integrins can induce heregulinexpression or its binding to erbB3 or erbB4 is unknown. Furthermore,there are no reports yet supporting integrin-stimulated heterodimerizationof erbB receptors. Further studies will be necessary to determinewhether integrins can cause the activation of erbB-2, thus leadingto heterodimerization and activation of theEGFR.

In summary, our results show that the EGFR-RAS-MAPK pathway can be activated downstream of integrin $alpha$ 5/ $beta$ 1 and stimulate epithelialcell proliferation. This adds to a growing body of literaturesupporting the view that the EGFR-RAS-MAPK pathway can be usedas an important signaling pathway by other receptors to controlor modulate critical cell functions attributed to EGRF-mediatedsignaling (Daub et al., 1996; Rosen and Greenberg, 1996; Zwicket al., 1997; Li et al., 1998). Thus, the EGFR appears to playan important role in integrating environmental cues as diverseas cytokines, UV light, and extracellular matrix proteins (Sachsenmaieret al., 1994; Daub et al., 1996, 1997; Moro et al., 1998; Li etal., 1999) to achieve regulation of cell migration, survival,and proliferation. The fine level of integration and orchestrationof signaling performed by the EGFR is underscored by the tumorigeniceffects caused by the aberrant expression and/or functioning ofproteins at all levels of the EGFR-Ras-ERK signal transductioncascade (Gerosa et al., 1989; Ishitoya et al., 1989; Cook et al.,1992; Itakura et al., 1994; Mansour et al., 1994; Rajkumar andGullick, 1994; Hirono et al., 1995; Normanno et al., 1995; Huanget al., 1996; Stumm et al., 1996; Bucci et al., 1997; Kuttan andBhakthan, 1997; Sekine et al., 1998).

	ACKNOWLEDGMENTS

The authors acknowledge Dr. H. Steven Wiley for his generous support and technical advice on this project and Dr. Erkki Ruoslahtifor providing the human integrin $alpha$ 5 gene. This work was supportedby the Office of Research and Development, Department of VeteransAffairs, and by grants from the National Institute of Diabetes,Digestive, and Kidney Diseases, the Huntsman Cancer Institute,the Glaxo Institute for Digestive Health, and the American CancerSociety.

	FOOTNOTES

^* Corresponding author. E-mail address: scott.kuwada{at}hsc.utah.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Integrin 5/1 Mediates Fibronectin-dependent Epithelial Cell Proliferation through Epidermal Growth Factor Receptor Activation

Integrin $alpha$ 5/ $beta$ 1 Mediates Fibronectin-dependent Epithelial Cell Proliferation through Epidermal Growth Factor Receptor Activation