Electric Field-directed Cell Motility Involves Up-regulated Expression and Asymmetric Redistribution of the Epidermal Growth Factor Receptors and Is Enhanced by Fibronectin and Laminin

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Vol. 10, Issue 4, 1259-1276, April 1999

Electric Field-directed Cell Motility Involves Up-regulated Expression and Asymmetric Redistribution of the Epidermal Growth Factor Receptors and Is Enhanced by Fibronectin and Laminin

Min Zhao,^* Andrew Dick, John V. Forrester, and Colin D. McCaig^*

Departments of ^*Biomedical Sciences and Ophthalmology, Institute of Medical Sciences, University of Aberdeen, Aberdeen AB25 2ZD, Scotland

Submitted March 24, 1998; Accepted February 4, 1999
Monitoring Editor: W. James Nelson

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Wounding corneal epithelium establishes a laterally oriented, DC electric field (EF). Corneal epithelial cells (CECs) culturedin similar physiological EFs migrate cathodally, but this requiresserum growth factors. Migration depends also on the substrate.On fibronectin (FN) or laminin (LAM) substrates in EF, cells migratedfaster and more directly cathodally. This also was serum dependent.Epidermal growth factor (EGF) restored cathodal-directed migrationin serum-free medium. Therefore, the hypothesis that EGF is aserum constituent underlying both field-directed migration andenhanced migration on ECM molecules was tested. We used immunofluorescence,flow cytometry, and confocal microscopy and report that 1) EFexposure up-regulated the EGF receptor (EGFR); so also did growingcells on substrates of FN or LAM; and 2) EGFRs and actin accumulatedin the cathodal-directed half of CECs, within 10 min in EF. Thecathodal asymmetry of EGFR and actin staining was correlated,being most marked at the cell-substrate interface and showingsimilar patterns of asymmetry at various levels through a cell.At the cell-substrate interface, EGFRs and actin frequently colocalizedas interdigitated, punctate spots resembling tank tracks. Cathodalaccumulation of EGFR and actin did not occur in the absence ofserum but were restored by adding ligand to serum-free medium.Inhibition of MAPK, one second messenger engaged by EGF, significantlyreduced EF-directed cell migration. Transforming growth factor $beta$ and fibroblast growth factor also restored cathodal-directedcell migration in serum-free medium. However, longer EF exposurewas needed to show clear asymmetric distribution of the receptorsfor transforming growth factor $beta$ and fibroblast growth factor.We propose that up-regulated expression and redistribution ofEGFRs underlie cathodal-directed migration of CECs and directedmigration induced by EF on FN andLAM.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Directed cell movements are fundamental in tissue construction and reconstruction. DC electric fields (EFs) exist where cellmigrations occur: in embryonic development and during wound healingof skin and cornea (Jaffe and Vanable, 1984; Chiang et al., 1992;Shi and Borgens, 1995; Robinson and Messerli, 1996). EFs equivalentto the field strength in vivo induce directed movement of culturedcells. Consequently, a physiological EF may be one guidance cueused by migrating cells (Robinson, 1985; Nuccitelli, 1988; McCaigand Zhao, 1997).

After corneal wounding, growth factor and cytokine levels increase in tear fluid and in stroma layers, and a provisional ECMis elaborated (Gipson and Inatomi, 1995; Virtanen et al., 1995;Sheardown and Cheng, 1996; Tervo et al., 1997; Vesaluoma et al.,1997a,b). How EFs interact with growth factors and different substratumcomponents in directing cell migration is unknown but relevant,because growth factors alone have chemotactic and chemokineticeffects on cells, and EFs may create extracellular gradients ofrelevant molecules (Messerli and Robinson, 1997).

Cell-substratum adhesion is important in cell migration (Palecek et al., 1997). For instance, the ECM influences EF-directedmigration of human keratinocytes (Sheridan et al., 1996). Fibronectin(FN) normally is not present beneath corneal epithelial cells(CECs) but appears after injury and persists until migration iscomplete (Fujikawa et al., 1984). Local FN also increases rapidlyafter human photorefractive keratectomy (Virtanen et al., 1995)and experimental corneal wounding (Cai et al., 1993; Espaillatet al., 1994; Vitale et al., 1994). Some data suggest that FNstimulates corneal epithelial migration in vivo and in vitro (Nishidaet al., 1983, 1984; Mooradian et al., 1993; Gundorova et al.,1994; Gipson and Inatomi 1995), but not all reports agree (Newtonet al., 1988). Laminin (LAM) may not be essential for migrationduring corneal wound healing (Fujikawa et al., 1984) but is importantin CEC-substrate adhesion (Ohji et al., 1993) and is expressedin corneal epithelial wound healing in vitro (Kurpakus et al.,1990). Integrins are expressed on CECs. Among them, $alpha$ 2 $beta$ 1, $alpha$ 3 $beta$ 1,and $alpha$ $nu$ $beta$ 1 bind LAM, collagen, and FN. Epithelial expression of $beta$ 1 integrins increased as FN in the wound increased and decreasedas wound healing was completed (Murakami et al., 1992; Elner andElner, 1996). $alpha$ 6 $beta$ 4 is synthesized and redistributed in wound healing(Kurpakus et al., 1991) and binds LAM (Sonnenberg et al., 1993),whereas LAM promotes reorganization of filamentous actin (F-actin)in CECs (Svoboda, 1992; Khoory et al. 1993). In addition, theECM contains a complex array of fixed charges and the ionic chargeof a substrate modulates corneal cell integrin expression, cellspreading, and cell migration. For example, the expression of $alpha$ 6 and $beta$ 4 integrin proteins and their mRNAs on CECs is down-regulatedby hydrogel surfaces lacking positively charged amine moieties(Wu and Trinkaus-Randall, 1997), whereas corneal epithelia andfibroblast show differential spreading behavior on differentlycharged surfaces (Bergethon et al., 1989). Because EFs, LAM, FN,and growth factors coexist after corneal injury, they may interactto modulate cell motility. We show that bovine CECs cultured onFN or LAM in a physiological EF migrated faster and more directlycathodally. Both responses were serumdependent.

Epidermal growth factor (EGF) stimulated CEC motility (Tao et al., 1995), and overexpression of EGF receptor (EGFR) enhancedkeratinocyte motility (McCawley et al., 1997). Cultured bovineand human CECs migrated cathodally in a physiological EF and requiredserum or EGF, basic fibroblast growth factor (bFGF), or transforminggrowth factor $beta$ 1 (TGF- $beta$ 1) in serum-free medium to do so (Zhaoet al., 1996a,b, 1997). Therefore, signal transduction throughgrowth factor receptors may underlie EF-directed CEC migration,although the mechanisms are notclear.

EF-induced reorganization of charged surface receptors and of the cytoskeleton seems to be involved (Poo et al., 1979; Onumaand Hui, 1988; Brown and Loew, 1994; McCaig and Zhao, 1997). EF-inducedextracellular gradients of growth factors or FN or LAM also maybe important (Robinson and Messerli, 1996; Messerli and Robinson,1997). Thus reorganization of cell surface receptors or extracellularmolecules to induce a gradient of either receptor or ligand, respectively,is likely an initial event, which activates cells asymmetricallyand drives subsequent cytoskeletal reorganization and directedcellmigration.

We tested whether EGFR expression and distribution were regulated by an EF or by ECM proteins in a manner that could underliedirected CEC migration. Flow cytometry was used to monitor membraneexpression of EGFRs. Not only did EF increase expression of EGFRs,so also did a substratum of FN or LAM. Using semiquantitativeconfocal microscopy, we have asked whether actin and the receptorsfor the three growth factors (EGF, TGF- $beta$ 1, and FGF), which restoredfield-directed migration in serum-free medium (Zhao et al., 1996a,b),become asymmetrically distributed. Actin and all three receptorsaccumulated cathodally after EF exposure, with the EGFR and actinshowing patterned colocalization at the cell-substrate interfaceand early cathodal asymmetry, consistent with a role in directingcell migration. We also used PD98059, which prevents the phosphorylationof MAPK kinase (MEK; MAPK is an element of the EGF signaling pathway),and this reduced directed migration of CECs in EFs plus EGF. Wepropose that EF-directed migration of CECs uses the well-recognizedligated EGFR as a proximal element, with downstream signaling,and that up-regulated expression and redistribution of EGFRs andcoordinate redistribution of actin underlie cathodal-directedmigration. The intracellular location and markedly slower field-inducedasymmetry of the FGF receptor and the TGF receptor II (TGFR II)suggest that they may be less important in instigating field-directedCECmigration.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Antibodies, Growth Factors, and Reagents

The monoclonal mouse anti-human EGFR (catalog number E2760), FITC- and TRITC-conjugated secondary antibodies (catalog numbersF2883 and T6778), and normal rabbit and sheep serum were fromSigma (Poole, United Kingdom). Rhodamine phalloidin and fluorescein-conjugatedEGF (fluorescein EGF; E3478) were from Molecular Probes Europe(Leiden, The Netherlands). Polyclonal rabbit anti-chicken FGFreceptor (FGFR) antibody (catalog number 06-177), which reactswith bovine FGFR, and polyclonal rabbit anti-human TGF- $beta$ typeII receptor (catalog number 06-277) were from Upstate Biotechnology(TCS Biologicals, Buckingham, United Kingdom). Cy5-labeled goatanti-rabbit immunoglobulin G (IgG; catalog number PA45004) wasfrom Amersham (Arlington Heights, IL). PD98059 (MEK1 inhibitor;9900S) was from New England Biolabs (Beverly,MA).

Cell Cultures and EF Stimulation

Primary cell cultures of bovine CECs were prepared by standard methods (Zhao et al., 1996a). For immunofluorescence studythe chamber base was an acid-washed glass coverslip, or slide,stuck down with silicone grease (MS4; Dow Corning, Auburn, MI)in a plastic culture dish. Cells were cultured at a cell densityof ~24 × 10⁴ cells/ml for migration and immunofluorescence experiments andat ~100 × 10⁴ cells/ml for flow cytometry experiments. FN (McIntosh et al.,1988), and LAM (from mouse sarcoma, Sigma) were diluted usingPBS. One milliliter of diluted solution was pipetted into thegalvanic culture chamber (see Zhao et al., 1996a, their Figure1), left for 2 h (37°C, 5% CO₂), washed off, and rinsed threetimes with PBS. Cells adhered to the base for 16~24 h (37°C; 5%CO₂), before a roof of number 1 cover glass (Chance Propper, Warley,England) was added and sealed with silicone grease. Final dimensionsof the chamber, through which current was passed, were 22 × 10× 0.2 mm for migration and immunofluorescence microscopy and 64× 10 × 0.2 mm for flow cytometryexperiments.

For experiments labeling EGFR in live cells, slide chambers were mounted directly on the microscope stage immediately afterpreparing the cells and adding the coversliproof.

Quantification of Cell Behavior

Cells were tracked and analyzed with an image analyzer (Zhao et al., 1996a). Mean migration rate and directedness were quantifiedover 5 h (Gruler and Nuccitelli, 1991; Zhao et al., 1996a). Theangle that each cell moved with respect to the imposed EF vectorwas measured. The cosine of this angle is 1 if the cell moveddirectly along the field lines toward the cathode, 0 if the cellmoved perpendicular to the EF vector, and $-$ 1 if the cell moveddirectly toward the positive pole of EF. Averaging the cosines( $Sigma$ iCOS $theta$ /N, where $theta$ is the angle between the field vector andthe cellular translocation direction, and N is the total numberof cells) yields average directedness of cellmovement.

Inhibition of MEK Activation and Phosphorylation

Cells were washed and incubated for 1 h with 50 µM PD98059 diluted in serum-free medium before EF application. Immediatelybefore EF exposure, serum-free medium with 25 ng/ml EGF and 50µM PD98059 was substituted into the EF chamber. Control cultureslackedPD98059.

Flow Cytometry Analysis

Cells were exposed to EF at 37°C, 5% CO₂ for 12~16 h or for ~3 h in room air for FN or LAM experiments. After EF exposure,cells were washed thoroughly with PBS (Ca²⁺ and Mg²⁺ free), then 4 ml of Versene solution (Dow Chemical, Midland,MI) was added and incubated for 10-20 min at 37°C. In some experimentstrypsin (final concentration, 0.05%) was added. Harvested cellswere washed twice in cold serum-free DMEM. Cells were suspendedin 5-10 ml of serum-free DMEM and revitalized for 15 min at 37°C.Harvested samples included no less than 10⁶ cells/ml. Cells were washed twice with ice-cold FACS buffer.All subsequent staining was done at 4°C or on ice. Cells wereincubated with antibodies against EGFRs for 30 min, washed twicewith FACS buffer, and incubated with FITC-conjugated secondaryantibody (1:128) for 30 min. After two washes, the pellet wassuspended with 400 µl of FACS buffer for immediate flow cytometryor with 400 µl of FACS fix (1% formaldehyde) when flow cytometrywas performed the next day. Appropriate isotype control includedOX21 to determine the level of nonspecific binding of IgG mAbsto CECs. Additional controls included cells alone and FITC-conjugatedsecondary antibody. Cell viability was determined either by trypanblue or with propidium iodide (Sigma) after treatment with FACSperm(Becton Dickinson, San Jose, CA) after secondary antibody incubation.Cell viability was consistently 85-95% for flow cytometric analysis.Cytofluorometric analysis was performed using a FACScaliber (BectonDickinson) flow cytometer equipped with a 488-nm argon line. Alinear forward scatter versus linear side scatter display wasused to set a broad gate that eliminated small debris and largeaggregates for collection of fluorescent list mode data. The datawere collected and computer analyzed using CellQuest analysissoftware (Becton Dickinson). For each sample a minimum of 10,000gated events were analyzed, and mean fluorescence intensity ofthree subpopulations wasdetermined.

Confocal Fluorescence Microscopy Analysis

Cells were washed three time with PBS, fixed with acetone (4°C for 10 min), air dried at room temperature for 30 min, andrehydrated with PBS (with 1% BSA). All antibodies were dilutedin PBS with 1% BSA and used as follows: monoclonal anti-EGFR at1:80; polyclonal anti-FGFR, 1:50; polyclonal anti-TGFR II, 10µg/ml; monoclonal anti-FGFR, 1:20; and monoclonal anti-TGFR, 1:20.Dilutions for secondary antibodies were: sheep anti-mouse IgGFITC conjugate (Fab'), 1:250; goat anti-rabbit IgG TRITC conjugate,1:300; and goat anti-rabbit IgG Cy5 conjugate, 30 µg/ml. For triplestaining, cells were incubated with primary antibodies againstEGFR in a humid chamber at 37°C for 30 min and washed twice withPBS, 10 min each. The cells were incubated with FITC-conjugatedsheep anti-mouse IgG (Fab') for 30 min and then washed twice withPBS. Cells were incubated with anti-TGFR or anti-FGFR for 30 minand washed twice (the last time with 10% normal goat serum). Cy5-conjugatedanti-rabbit IgG was mixed with rhodamine-phalloidin (5 U/ml) andadded to the cells for 30 min at 37°C. For double labeling, onlyone of anti-EGF, or anti-TGFR or anti-FGFR and appropriate secondaryantibodies was used. This staining was used also in some experimentswith triple staining to make sure the triple-staining resultswere not caused by excessive cross-reaction. For negative controlstaining, only the secondary antibodies were incubated with thecells. No positive staining was observed with secondary antibodiesalone. When monoclonal anti-TGFR or anti-FGFR was used, anti-mouseIgM (µ-chain specific) FITC conjugate (Sigma) was used with rhodamine-phalloidin.After washing twice with PBS, slides were mounted in Vectorshield(Vector Laboratories, Peterborough, United Kingdom) and viewedwith a Bio-Rad (Hercules, CA) MRC 1024 confocalmicroscope.

For live cell labeling, antibodies were diluted in serum-free DMEM. After two washes (10 min each) with serum-free DMEM, cellswere incubated with primary antibodies at 37°C for 30 min, washedtwice, and incubated with secondary antibodies. A coverslip roofwas attached, and appropriate medium replaced the washing solution(as described above, Cell Cultures and EF Stimulation). Slideswere mounted on the confocal microscope, and EF was applied asbefore.

For fluorescein-conjugated EGF labeling, cells were washed with ice-cold PBS after 3 h of EF application (150 mV/mm) and kepton ice or in an ice-cold environment thereafter. Cells were incubatedwith ice-cold serum-free medium with fluorescein EGF (100 ng/ml)for 1 h, washed with ice-cold PBS, and immediately viewed on anice-cold stage with fluorescent and confocalmicroscopes.

To quantify the asymmetric distribution of growth factor receptors or F-actin, fluorescence intensity was measured for cathodal-and anodal-facing sides. Well-spread, positively stained cellsshowing asymmetric distribution of staining were selected. Theimages were typically three to five frame averaged. A cell projectionor a section of cell was divided into left (cathodal) and right(anodal) halves by a vertical line through the center of the cellor center of the nucleus perpendicular to the EF vector. In cellswith well-defined cathodal patches of fluorescence, the polygonselection function was used, and the complete, positively stainedarea was measured. Measurements also were made using the samepolygons from the anodal half, opposite from the cathodal patches(along the axis of the EF). Polygons were drawn with Bio-Rad LaserSharp2.1a and avoided including areas near cell boundaries, where fluorescenceintensity was near background. Freehand polygonal areas were drawnalso to determine membrane-juxtamembrane region labeling, as opposedto intracellular labeling. An asymmetric index was calculated:Ai = (Cfi $-$ Afi)/(Cfi + Afi) for each cell or cell section, whereCfi represents mean cathodal side fluorescence intensity, andAfi is mean anodal side fluorescence intensity. Acellular areasin the same image were measured as background and subtracted fromcellular measurements. This method avoids potential artifactsattributable to differential expression and detection of givenproteins within different cells. A cell with uniform fluorescencestaining will have an Ai of 0. A cell with fluorescence stainingtotally restricted to the cathodal half will have an Ai of 1,whereas a cell stained only in the anode-facing half will havean Ai of $-$ 1. Therefore, Ai values >0 indicate cathodal accumulationof fluorescence staining, with stronger cathodal staining givingAi values progressively closer to 1. The average Ai from a groupof cells gives an objective estimate of fluorescence stainingasymmetry across thegroup.

Statistical analyses were made using unpaired, two-tailed Student's t test or Welch's unpaired t test when SDs were significantlydifferent from each other. Data are expressed as mean ± SEM, unlessstatedotherwise.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

FN and LAM Enhance Cathodally Directed Migration of CECs

CECs cultured without applied EFs migrated randomly, with directedness near 0 (Zhao et al., 1996a). In EFs, both single cellsand sheets of cells moved cathodally (Zhao et al., 1996a,b). Cathodal-directedmotility increased on FN or LAM (Figure 1; compare with Zhao etal., 1996a, their Figure 3) and was concentration dependent. Concentrations>100 and <0.01 µg/ml did not enhance cathodal directedness (Figure2). At most concentrations, LAM more effectively stimulated directednessthan FN (Figures 1 and 2). Directional migration of CECs requiredserum (Zhao et al., 1996a). CECs on a range of FN or LAM concentrationsin serum-free DMEM (150 mV/mm) lost all cathodal directedness(Figure 1).

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Figure 1. Typical translocation of bovine CECs over 5 h in EF (150 mV/mm). Substrate and serum dependency are illustrated. Each point represents a single cell, located initially (0 h) at the center of the circular graph with final location plotted after 5 h in EF. The radius of each circle is 200 µm, and average cell length is ~20 µm. The average cosine (directedness) of the distribution ± SEM and the number of cells plotted are indicated at upper right of each distribution. (for distributions for unstimulated cells and cells exposed to EF alone, see Zhao et al., 1996a

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Figure 2. FN or LAM significantly increased cathodal directedness of migration. The enhancement was concentration dependent. **, p < 0.01; *, p < 0.05 compared with that on the noncoated substratum in same EFs (shown at right). Directedness of 0 indicates random migration; directedness of 1 indicates all cells migrated directly cathodally; and $-$ 1 indicates direct anodal migration of all cells along the field vector. For methods of determining directedness, see Zhao et al. (1996a)

. Number of cells for each point, 43~221.

LAM and FN Increased the Rate of Cell Migration in EF

FN or LAM alone did not alter cell speed (Figure 3A), which remained low, ~5 µm/h in serum-free medium. Serum increased cellspeed on uncoated plastic and on FN or LAM substrates (Figure3B), although high concentrations of FN (100 µg/ml) suppressedthe migration rate in serum (Figure 3B). Cells on noncoated dishesin EF moved at 11.6 ± 0.8 µm/h (n = 183) but moved faster on FNor LAM in the same EF (150 mV/mm; Figure 3, B and C). This alsowas concentration dependent. On FN (0.1-100 µg/ml), enhanced rateswere constant, ~16 µm/h, although at 100 µg/ml enhanced cathodaldirectedness was lost (compare Figures 2 and 3C). LAM also increasedthe migration rate at 0.1 µg/ml, but higher concentrations wereless effective. Only when FN or LAM and EF were present togetherdid migration rate increase significantly (Figure 3).

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Figure 3. Migration rate of CECs cultured in: serum-free DMEM (A) without EF (

) and with EF at 150 mV/mm (

) and DMEM plus 10% FBS (B) without EF (

) and with EFs at 150 mV/mm (

). **, p < 0.01 compared with that on the noncoated substratum without EF. (C) Coating concentration dependency of migration rate in serum-containing DMEM at 150 mV/mm. *, p < 0.05 compared with noncoated substratum in same EFs (shown at right). Number of cells for each point, 38~221.

The synergistic effect of ECM and EF on migration rate also depended on serum. Cells on FN or LAM in EF but no serum migratedslowly, like those with no EF, no substrate coating, and no serum(Figure 3, compare A andB).

Inhibition of MEK Significantly Reduced EF-directed Cell Migration

The MAPK inhibitor PD98059 significantly reduced both the migration rate and directedness of CECs in EF. Migration rate droppedfrom 6.6 ± 0.4 µm/h in serum-free medium plus EGF to 4.5 ± 0.3µm/h (n = 170-198; four experiments; p < 0.0001) after drug exposure.Drug-treated cells therefore migrated at the same rate as thosein serum-free medium plus EFs (Zhao et al., 1996a; 4.8 ± 0.8 µm/h),indicating that the effect of adding EGF on the migration rateof CECs in EFs was completely abolished. Directedness also droppedsignificantly from 0.78 ± 0.02 to 0.60 ± 0.04 (n = 170-198; fourexperiments; p < 0.001) in PD98059 but remained substantial. Treatmentwith PD98059 also reduced the migration rate of CECs on LAM orFN significantly (p < 0.001, two experiments) from control of16.7 ± 0.54 µm/h (n = 123) to 11.8 ± 1.18 µm/h (n = 45) on FNand 16.3 ± 0.98 µm/h to 8.33 ± 0.8 µm/h (n = 90) on LAM (coatingconcentration, 0.1 and 10 µg/ml, respectively). However, the directednessremained unchanged for cells on both substrata exposed to EFs(our unpublishedresults).

EF Exposure Increased Expression of EGFR

With negative isotype and second antibody control as background, positively stained cells were recognized as total expressionof EGFR and gated as M1 (with background gated events set to <1%of total population). Within gate M1, two peaks of EGFR-labeledCECs were distinguished (Figure 4A) and further divided and gatedas M2 and M3. Gate M2 represents a lower amount of EGFR expressedon the cell surface, recognized by dim fluorescence, which wedefined as EGFR^Low. Gate M3 represents a high amount of EGFR expressed on the cellsurface, recognized by bright fluorescence, which we defined asEGFR^High. The cells for these experiments were cultured on plastic for~16 h before EF application. After a further ~16 h in a physiologicalEF (100-150 mV/mm; 37°C, 5% CO₂, 95% humidity), the percentageof membrane EGFR-positive cells increased significantly (Figure4B). The EGFR^Low-expressing cells increased most (p < 0.05), from control valueof 16.1 ± 1.4% (n = 5) to 22.0 ± 1.8% (n = 8 at 100-150 mV/mm),making a significant (p < 0.05) increase in the total percentageof positive cells, from control value of 25.3 ± 1.6% (n = 5 withno EFs) to 34.3 ± 2.8% (n = 8 at 100-150 mV/mm). However, averageEGFR^High remained unchanged (11.1 ± 1.3%; n = 8; at 100-150 mV/mm versus9.3 ± 1.5%; n = 5; with no EFs), although a few experiments showeda dramatic increase in the percentage of EGFR^High cells. Mean fluorescence intensity, corresponding to the numberof EGFRs per cell, did not increase (our unpublished results).Interestingly, up-regulation did not occur in cells exposed tohigher EFs (200-300 mV/mm; n = 4): percents of EGFR total, EGFR^Low, and EGFR^High were 25.7 ± 2.1, 19.0 ± 1.2, 7.1 ± 0.7%, respectively. Serumstarvation might be expected to increase the membrane expressionof EGFR, but we found no significant increase (EGFR total, 29.0± 2.0%; EGFR^Low, 16.4 ± 1.2%; EGFR^High, 12.6 ± 1.5%; n = 7).

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Figure 4. Representative fluorescent intensity flow cytometric histograms show the effect of LAM or FN with or without EF on membrane expression of EGFR on CECs. Isotype-matched negative control, OX21 as primary mAb, background fluorescence was similar with secondary Ab as negative control. M1 (positively stained cells) was set where the expression of gated events was <1% in isotype-matched negative control. (A) Control (without substratum coating, no EF) cells showed a population of positively stained cells, region M1, which can be further divided into a low peak (region M2) representing a subpopulation of low EGFR expression (EGFR^Low) and a higher peak (region M3) representing a subpopulation of high EGFR expression (EGFR^High) expression. (B) After 12 h in EF (100 mV/mm), positively stained cells increased, as shown by gated events in M1 as total, M2 as EGFR^Low expression cells (p < 0.01), and M3 as EGFR^High expression cells. The cells were cultured on plastic without substratum coating. (C) Withdrawal of serum from culture medium and exposed to EF (100 mV/mm) for 13 h shows a significant decrease in EGFR expression (p < 0.05 for EGFR^High). The cells were cultured on plastic without substratum coating. (D) Addition of EGF (25 ng/ml) in serum-free medium and EF (100 mV/mm) for 13 h; EGFR^Low expression was significantly up-regulated; compare with C. Also see text for detailed numerical data. (E) Significant increases in total EGFR expression and more dramatically in EGFR^High were evident for CECs cultured on substratum of LAM (1 µg/ml) followed by 3 h of EF exposure at 100 mV/mm.

Culturing CECs in serum-free medium plus an EF (100-150 mV; n = 3; 200-300 mV; n = 4) did not induce EGFR up-regulation (Figure4C; our unpublished results). To test whether receptor up-regulationby a small EF depends on the ligand, cells in serum-free mediumwith added EGF were assessed. Up-regulation of membrane expressionof EGFR by EF (100 mV/mm) plus specific ligand was virtually identicalto that seen in EF plus 10% fetal calf serum: total expression,33.14 ± 0.46% (n = 2; p = 0.09); up-regulation was seen largelyfor EGFR^Low: 22.07 ± 0.02% (p < 0.01) (Figure 4D); whereas EGFR^High remained unchanged (11.48 ± 0.48%) compared with serum-free mediumand 0 mV/mm. Addition of EGF alone to serum-free medium (no EF)did not increase EGFR expression (p = 0.91).

FN or LAM Substratum Increased Expression of Membrane EGFR

The effects of FN or LAM alone or in combination with EFs in modulating EGFR expression on CECs also were tested. To minimizepossible effects of secreted ECM, which occurs 18~24 h after seedingCECs (Sugrue and Hay, 1982; Ohji et al., 1993), CECs culturedfor ~15 h on plastic or on substratum of FN or LAM were exposedto EF for 3 h (100 mV/mm) in separateexperiments.

Membrane EGFR expression of CECs cultured on plastic for ~15 h followed by 3 h of EF exposure remained unchanged comparedwith that of the cells not stimulated with EF (Table 1).

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Table 1. Effects of EF and fibronectin or laminin on membrane expression of EGF receptors on corneal epithelial cells

CECs on FN or LAM alone (1 µg/ml coating concentration) for ~18 h, however, did show significantly higher total expressionof membrane EGFR even without applied EFs. There were no significantchanges in EGFR^Low or EGFR^High for those cells (Table 1).

FN or LAM (~15 h) plus 3 h of EF exposure in medium with or without serum did not further up-regulate total membrane EGFRexpression. (Cells were cultured in DMEM with 10% serum for ~15h before EF exposure and serum-free exposure. Only during the3-h EF exposure was serum-free DMEM used.) However, analyzingEGFR^Low and EGFR^High subpopulations in the cells revealed an interesting issue. EGFR^High tended to be higher for the cells cultured on FN or LAM thanon plastic whether EFs were applied (Table 1). When those cellson substrata of FN or LAM were further subjected to 3 h of 100mV/mm, significant increases in EGFR^High became evident. This was particularly true for the cells culturedon FN followed by 3 h in serum-containing medium at 100 mV/mmand cells cultured on LAM followed by 3 h at 100 mV/mm in a mediumwith or without serum (Table 1). A dramatic increase in EGFR^High was evident for the cells cultured on LAM followed by 3 h ofexposure to 100 mV/mm in serum-free medium (Figure 4E).

Mean receptor numbers per cell (mean fluorescence intensity) did not change, with EF, FN or LAM, or EF plus FN or LAM (ourunpublishedresults).

Three Growth Factor Receptors and Actin Are Redistributed by a Physiological EF

Mean fluorescence intensity of probes for growth factor receptors and for actin on the cathodal- and anodal-facing halvesof CECs was assessed, and asymmetric indices (Ai) for 10-20 singlecells were calculated (see MATERIALS ANDMETHODS).

Early EF-induced Redistribution of EGFR and Actin Are Serum Dependent

With no EF, most cells showed no asymmetry of EGFRs or actin staining (Figure 5, a and a'). After exposure to an EF (150 mV/mm)in serum-containing medium, EGFR and actin staining redistributedand accumulated at the cathode-facing side of the cells (Figure5, c and c') (38% of 587 cells showed clear asymmetry of receptors).Figure 6 shows the dynamic cathodal accumulation of EGFR in alive cell. After 10 min in an EF (300 mV/mm), EGFR had accumulatedcathodally. The increase of cathodal EGFR staining was more obviousat 20 min with a concomitant decrease in anodal staining. In serum-freemedium, however, no cathodal accumulation of EGFR or actin wasobserved for cells exposed for 3 h to EFs of 150 mV/mm (Figure5b) or for live cells exposed to an EF of 300 mV/mm (our unpublishedresults).

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Figure 5. Confocal images of CECs double labeled for actin filaments (red) and EGFR (green). Colocalization is indicated by yellow. (a) Cell cultured without EF, no obvious asymmetric distribution of EGFR or F-actin. (b) Cell cultured in serum-free medium at 150 mV/mm, no obvious asymmetric distribution of EGFR or F-actin. (C) Cell cultured in EF in serum. Obvious accumulation of EGFR and F-actin cathodally was evident. (a'-c') Fluorescence intensity in arbitrary units along a line drawn across the cells in a-c, respectively. Asymmetry of both actin and EGFR is evident both visually and digitally only for the cell in c. Figure 6. (A) Confocal images of a live CEC labeled with EGFR antibodies, showing dynamic accumulation of EGFR at the cathode facing side (arrows) when exposed to 300 mV/mm for a 20-min duration, cultured in DMEM with 10% FBS. Bar, 20 µm. (B) Asymmetry of EGFR and F-actin in a cell exposed to 150 mV/mm for 3 h. (B') Representative vertical section (through the line drawn across the cell in B) shows actin and EGFR staining in an interdigitating pattern in punctate spots near the cell-substratum interface.

Ai was used to quantify EGFR and actin asymmetry (see MATERIALS AND METHODS for details). An Ai value close to 0 indicatessymmetric distribution. Increasing asymmetric accumulation isindicated by a higher value of Ai from 0 to 1. There are two importantpoints. 1) EF-induced asymmetry was voltage dependent; there wasa higher Ai at higher field strength. Cells exposed to EF for3 h had Ai values for EGFR of 0.19 ± 0.06 at 150 mV/mm and 0.30± 0.09 at 250 mV/mm, both significantly higher than the control: $-$ 0.06 ± 0.05 (p < 0.05; average of 10-20 cells). 2) EF-inducedasymmetry was serum dependent. In serum-free medium, the Ai valuefor EGFR was $-$ 0.01 ± 0.04 at 150 mV/mm, showing no obvious asymmetry.Even exposure to 250 mV/mm did not increase the Ai of EGFR significantly(0.16 ± 0.08; p = 0.08 compared with no field control). Ai foractin was 0.34 ± 0.07 (n = 10) when cultured in 150 mV/mm with10% FBS, whereas Ai failed to rise when cultured in serum-freemedium (Ai = 0.06 ± 0.26; n = 21) at the same field strength.When exposed to 300 mV/mm in 10% FCS, Ai for EGFR in live cells(n = 7) was $-$ 0.02 ± 0.01 at 0 min, 0.07 ± 0.05 at 10 min, and0.37 ± 0.13 at 20 min (p < 0.05 when compared with that at 0 min),whereas cells cultured in serum-free medium did not show significantchanges in Ai at the same field strength. To test whether growthfactors might facilitate cathodally directed growth factor receptoraccumulation, we added TGF- $beta$ 1 to serum-free culture medium (1.5pg/ml). This is one of the growth factors that partially restoredEF-induced directional migration of CECs in serum-free medium(Zhao et al., 1996a). Clear cathodal accumulation of EGFR andTGFR and rhodamine-phalloidin staining for actin filaments wereobserved (our unpublished results). We have not done the equivalentexperiment with EGFRligand.

Redistributed receptors were capable of binding EGF, because there was marked cathodal accumulation of EGFR-fluorescein EGFcomplexes after 3 h of EF exposure (Figure 7a). The Ai valuesalso show voltage and serum dependency of the cathodal accumulationof this ligand-receptor complex (Figure 7b).

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Figure 7. Marked cathodal accumulation of EGFR on live CECs revealed by fluorescein EGF binding. (A) Cells were exposed to EF for 3 h at 150 mV/mm and labeled as described in MATERIALS AND METHODS. (B) Ai of EGFR (in 10-20 cells for each group) as revealed by fluorescein EGF binding (see MATERIALS AND METHODS for details). An Ai value >0 indicates higher fluorescence intensity on the cathodal facing side; values close to 1 indicate extreme cathodal asymmetry of EGFR. *, p < 0.001 when compared with that of the cells in serum-free medium or cells not exposed to EF.

Membrane and Intracellular Asymmetry of EGFR and F-actin

Cathodal asymmetry was also analyzed using horizontal and vertical optical sections to reveal the subcellular distributionof receptor and actin staining. Qualitative observations and Aicalculations of single horizontal sections from base to top togetherindicate that well-spread cells showed greater cathodal asymmetryof EGFR in basal layers, whereas for less-spread cells, a higherAi was evident in the middle or top layers. EGFRs accumulatedcathodally both at the leading edge and intracellularly; the latterwas largely perinuclear. We analyzed these separately. Intracellularand membrane-juxtamembrane regions were selected (see MATERIALSAND METHODS), and Ai values were calculated. The most marked cathodalasymmetry was found for membrane-associated staining for EGFRand for F-actin. The greatest asymmetry of membrane EGFR occurredin serum-containing medium at 150 mV/mm (Ai = 0.40 ± 0.06 comparedwith $-$ 0.03 ± 0.06 for control cells [no EF]; n = 10; p = 0.0002).EF exposure also induced asymmetry of EGFR staining intracellularly(Ai = 0.18 ± 0.04; no EF = 0.03 ± 0.04; n = 10; p = 0.04). MembraneF-actin (at the leading edge) also accumulated cathodally afterEF exposure, (Ai = 0.28 ± 0.03; no EF = 0.08 ± 0.06; p < 0.01).Intracellular Ai for F-actin also suggested cathodal asymmetry(0.23 ± 0.05) but was not statistically different from no EF controlvalues of 0.07 ± 0.12.

Close Colocalization of EGFR and F-actin

Both F-actin and EGFRs accumulated cathodally and frequently were observed colocalized or adjacent to each other (Figure 5,c and c'). These observations were quantified by optically sectioning10 cells (EF 150 mV/mm; 3 h) and assessing the Ai for both EGFRand for actin in parallel in each of 96 optical sections. Themean Ai was very similar for each probe (0.38 ± 0.07 for EGFR,0.34 ± 0.07 for actin). The paired values were highly correlated(R = 0.72; p < 0.001, two-tailed Pearson correlation test), indicatinga high degree of colocalization. A representative Ai as a functionof position (base to top) in one cell is shown in Figure 8. Asimilar pattern with a high correlation between Ai for F-actin(Figure 8A) and Ai for EGFR (Figure 8B) was observed in 9 of 10cells. EGFR and actin therefore were asymmetric to a similar extentin similar locations. This asymmetry in cathodal- and anodal-facinghalf cells was further refined. Asymmetrical distribution of EGFRand actin associated with either membrane, or intracellular locationsalso were assessed and showed marked correlation, perhaps indicatingcausal relationships. The Ai for membrane EGFR was highest andwas highly correlated with the Ai for intracellular EGFR and formembrane F-actin and intracellular F-actin (R = 0.32, 0.62, and0.53, respectively; p < 0.004). The Ai for membrane-associatedF-actin also correlated well with that for intracellular EGFRand for intracellular F-actin (R = 0.23 and 0.61, respectively;p < 0.05).

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Figure 8. Ai of F-actin and EGFR from serial optical sections through a single cell, showing close correlation of the subcellular localization of F-actin (A) and EGFR (B). An Ai value >0 indicates higher fluorescence intensity on the cathodal facing side; therefore, values close to 1 indicate extreme cathodal asymmetry of F-actin or EGFR. Each section is 0.5 µm thick.

At the cell-substratum interface, EGFR and actin staining frequently were colocalized and interdigitated, to form "tank track"-likerepeats of red (actin filament) and green (EGFR) staining (Figure6, B and B'). This intriguing interdigitated pattern of EGFR andactin staining close to the cell-substrate interface was obviousin 9 of 10cells.

EF-induced Asymmetry of FGFR and TGFR II

Like EGF, bFGF and TGF- $beta$ 1 also partially restored cathodally directed migration of CECs in serum-free medium (Zhao et al.,1996a). Perhaps the receptors for these growth factors also redistributeand accumulate cathodally. CECs in EF for 3 h (150 mV/mm) didnot show a clear asymmetry of FGFR or TGFR, although a weak cathodalasymmetry of TGFR was seen after contrast enhancement (our unpublishedresults). After 12-16 h in EF (37°C), however, both TGFR and FGFRshowed pronounced EF-induced cathodal redistribution (Figure 9).Asymmetry of TGFRs occurred in single cells (Figure 9A, verticalsections, V1 and V2) and grouped cells (Figure 9B, V3). Markedperinuclear asymmetry of TGFR is evident in basal (Figure 9B')and middle (Figure 9B") optical sections of the cells. Long (~16-h)EF exposure also induced marked cathodal asymmetry of FGFR (Figure9D), whereas control cells (no EF) showed no obvious asymmetryof FGFR (Figure 9C). Longer EF exposure therefore revealed cathodalperinuclear asymmetry for both TGFR and FGFR.

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Figure 9. Confocal images of CECs exposed to EF of 150 mV/mm for 12-16 h and double labeled with rhodamine-phalloidin for F-actin (red) and antibodies against growth factor receptors (green): TGFR (top panel) or FGFR (lower panel). Colocalization is indicated by yellow. (A) Two single cells showing stronger staining at the cathodal side for both TGFR and F-actin. (V1 and V2) Vertical sections along the line V1 and V2 in A. (B) Grouped cells also show accumulation of TGFR staining at the cathodal side (arrows). (V3) Vertical section cut along line V3 in B shows asymmetric accumulation of TGFR at the cathodal facing side. (B' and B") TGFR and F-actin asymmetry in the basal and middle sections of B. (C) Two control cells (no EF exposure) show F-actin and FGFR staining. (D) Striking asymmetric distribution of the FGFR (green) and actin (red) observed in two cells after 16 h in EF of 150 mV/mm.

Asymmetry of TGFR and FGFR also was quantified. After 16 h of EF exposure at 150 mV/mm, the Ai for TGFR increased to 0.17± 0.08 (n = 9), significantly higher (p = 0.013) than no EF control,0.05 ± 0.11 (n = 13). A striking increase in Ai for FGFR stainingwas found after 16 h of exposure to EF of 150 mV/mm: 0.61 ± 0.08(n = 14); p < 0.01 compared with control. However, a short duration(3 h) of EF exposure did not increase Ai of FGFR: Ai values forFGFR were 0.02 ± 0.05 for the control; $-$ 0.01 ± 0.05 for the cellsexposed to 150 mV/mm in DMEM with 10% FCS; 0.03 ± 0.06 for thecells exposed to 250 mV/mm in DMEM with 10% FCS; and 0.06 ± 0.04for the cells exposed to 150-250 mV/mm in serum-free medium (n= 10-20cells).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Corneal wounding induces secretion of EGF and FN, the latter acting as a transient matrix for epithelial migration (Gipsonand Inatomi, 1995). Endogenous, laterally oriented EFs also areinduced after corneal injury (Chiang et al., 1992), and culturedCECs migrate cathodally in similar, physiological EFs (Zhao etal., 1996a,b). (We used field strengths two- to threefold greaterthan those measured in vivo [42 mV/mm], but these are underestimates[Chiang et al., 1992]. The theoretical maximum in vivo is as muchas 500 mV/mm.) When these elements were combined, both the speedand the extent of cathodal directedness increased on FN or LAM,and both events were serum dependent. Because EGF restored cathodal-directedmigration in serum-free medium, we tested the hypothesis thatEGFR activation may be an early event in EF-directed CEC migration.EF, FN, or LAM each up-regulated membrane expression of EGFRs(all enhance cathodal directedness), whereas EGFRs and polymerizedactin redistributed to accumulate cathodally, with a time courseand a pattern of colocalization consistent with a role in directingcell migration cathodally. Additionally, up-regulation of EGFRsand asymmetric redistribution of EGFRs and actin all requiredserum.

Enhancement of Migration Speed: Serum Dependency

FN or LAM with or without serum and FN or LAM with EF but no serum did not increase rates of cell movement. Only cells grownon FN or LAM with EF and serum showed an increased speed of migration.Cells may migrate in response to chemotactic (growth factor) and/orhaptotactic (ECM protein) stimuli, which may be spatially distributedin concentration gradients. However, multiple stimuli such asFN or LM with EF and growth factors alter speed of migration aswell as directionality (see below). This may indicate that thecoordinated interaction of these stimuli alters the kinetics ofthe migratory response signaling pathway, perhaps via intracellularregulation of second messenger responses, e.g., via rates of phosphorylationand dephosphorylation of receptors. Such interactions seem likely.For instance, human CECs migrate on FN only in the presence ofEGFR activation, and migration on FN is inhibited by antibodiesto EGF (Maldonado and Furcht, 1995). Similarly, anti-FN antibodiesinhibit EGF-stimulated migration of rabbit CECs, indicating thatmigration may require activation of both growth factor receptorsand the integrin receptors for FN (Nishida et al., 1990). FN significantlypotentiates activation of MAPK by EGF in fibroblast cells (Miyamotoet al., 1996) and endothelial cells (Short et al., 1998) and onlydoes so if the integrins are both aggregated and occupied by ligand(Miyamoto et al., 1996). ECM and EGF may interact to activateMAPK at the level of integrin aggregation, integrin occupancy,and growth factor binding (Miyamoto et al., 1996). The presentstudy shows that additionally there may be regulation of EGFRsby ECM (see Up-regulation of EGFR by FN and LAM). Serum dependencyof faster, ECM- and field-induced cell speed may represent a requirementfor EGF and the induction of a shift to more optimal levels ofcell-substratum adhesiveness (Palecek et al., 1997).

There may be changes also in the total number of receptors expressed on migrating cells, making more receptors available tobind excess ligand. Adding serum to cultured fibroblasts increasedgene expression for FN, FN receptors, actin, and tropomyosin within15 min (Ryseck et al., 1989). EGF increased synthesis and secretionof FN and may control integrin expression in CECs, because $alpha$ 2 $beta$ 1, $alpha$ 3 $beta$ 1, and $alpha$ $nu$ $beta$ 1 integrins all increased in wounded CECs (Elnerand Elner, 1996). Additionally, growth factors, FN, and a singleelectrical pulse (at a field strength 100- to 250-fold strongerthan used here; Pazmany et al., 1995) all induced early activationof growth-related genes. Whether immediate early gene expressionis increased by the much smaller and constant physiological EFused here is notknown.

Enhancement of Cathodal Directedness

LAM or FN did not induce directed migration. On FN or LAM plus EF, migration was more sharply focused directly toward thecathode. LAM was more effective than FN, although below and abovea range of concentrations, enhancement of directedness was lost(Figures 1 and 2). LAM plus EF also enhanced migration rate, andsimilar concentrations were effective, suggesting common mechanisms(compare Figures 2 and 3C). By contrast, FN- plus EF-enhancedmigration rates persisted at concentrations that no longer enhancedcathodal directedness (100 µg/ml; Figures 2 and 3C), suggestingseparate underlyingmechanisms.

It is perhaps not surprising that the MAPK inhibitor PD98059 did not reduce the directedness of CECs cultured on FN or LAMin EFs to the same extent as it reduced the migration rate. MEK1is a downstream element in EGF signaling. It is quite likely thatthe asymmetry of EGFR serves as a steering wheel, whereas themotor machinery activated through MAPK-phosphorylating myosinmoves the cells on ECM (Klemke et al., 1997).

Potential Mechanisms: Up-regulation of EGFR by EF

The EGFR is up-regulated by its ligand EGF and by TNF and down-regulated in vitro by increasing cell density (Holley et al.,1977; Earp et al., 1986; Palombella et al., 1987). Additionally,LAM down-regulates both the EGFR and insulin-like growth factorI receptor on rat enterocytes (Wolpert et al., 1996). Up-regulationof EGFRs by an EF or by FN or LAM is a novel observation and addsto the tight regulation of this receptor. The mechanisms underlyingEGFR up-regulation by EF or by ECM proteins in CECs are unclear.However, because EGFR expression was determined 12-16 h afterEF or ECM exposure, there would be time for nuclear transcriptionand new protein synthesis to occur, as well as recruitment ofpreexisting receptors. DC fields do regulate gene expression,e.g., c-fos, jun, and c-myc (Lin et al., 1994; Pazmany et al.,1995; Sauer et al., 1997). In addition, EGFR up-regulation wasvoltage dependent, occurring only at EF close to the physiologicalwound field strength. Higher EFs were ineffective. Wounding corneaor skin also induced and up-regulated expression of EGFR (Wenczaket al., 1992; Murata et al., 1993) and induced laterally orientedDC EF (Chiang et al., 1992). Perhaps the EF is causal in up-regulatingthe EGFR invivo.

Interestingly, EF did not up-regulate EGFRs in serum-free medium, but this did occur if the ligand EGF was present. This implicatesthe ligated EGFR as a proximal element in EF-induced receptorup-regulation. EGFR regulation probably involves ligand-receptorinteraction and EF-induced, ligand-bound receptor clustering (seeRedistribution of EGFR and Actinbelow).

Up-regulation of EGFR by FN and LAM

CECs on FN or LAM also increased membrane expression of EGFR (Table 1). We do not know whether the EGFR is actively synthesizedin our experimental system. If this is the case, one potentialmechanism is that ECM may stimulate TGF- $beta$ 1 gene transcription(Streuli et al., 1993), which in turn up-regulates EGFR transcriptionand expression in fibroblasts (Thompson et al., 1988). Integrinreceptors and growth factor receptors (such as EGF) act synergisticallyby common signaling pathways (Schlaepfer et al., 1994; Miyamotoet al., 1996), and expression of integrin receptors in CECs isspecifically regulated by ECM ligands (Grushkin-Lerner et al.,1997). Perhaps EGFRs and integrin receptors are up-regulated inparallel by FN, LAM, or EF. Additionally, enhanced exportationfrom intracellular pools of EGFR to the cell membrane cannot beexcluded.

The discovery that both EF and FN up-regulated EGFR may be significant given that both stimuli are early responses to cornealwounding. However, their effects on EGFR up-regulation were notadditive, suggesting that they operate by a common and saturablemechanism.

Redistribution of EGFR and Actin

Asymmetric redistribution of EGFR was demonstrated in both live and fixed CECs exposed to EFs using either antibody againstEGFR (Figures 5, 6, and 8B) or the physiological ligand for theEGFR (Figure 7). The dynamics of receptor redistribution in livecells also was demonstrated (Figure6A).

EFs also induced cathodal accumulation and colocalization of EGFR and actin. Both AC and DC fields redistribute cell surfacereceptors (including the EGFR) and the actin cytoskeleton (Pooand Robinson, 1977; Luther et al., 1983; Giugni et al., 1987;McCaig and Dover, 1991; Cho et al., 1994, 1996; Brown and Loew,1996), although the mechanisms differ, because redistributionin an AC field is not along the field vector (Cho et al., 1996).We propose that EGFR redistribution cathodally leads to localizedactin polymerization at the EGFR-plasma membrane interface andthat these events respectively trigger and mediate cathodal-directedCEC migration. The EGFR is an actin-binding protein (den Hartighet al., 1992), and EGF induces rapid remodeling of the actin cytoskeleton.In human epidermal carcinoma cells, actin polymerization is localizedto activated EGFRs in the plasma membrane and is not associatedwith internalized EGFRs (Rijken et al., 1995). Moving the EGFRcathodally, therefore, may be a key event, with downstream consequencesof asymmetry of actin polymerization. Both receptor and actinasymmetries were serum dependent. Ligated EGFRs may have considerablygreater lateral mobility within the plasma membrane than unboundreceptors. The IgE-Fc $epsilon$ receptor complex accumulated strongly cathodallyon leukemic rat basophils, whereas ligand-free Fc $epsilon$ receptors showedminimal cathodal accumulation in DC fields 10 times those usedhere (McCloskey et al., 1984). Because neither EGFR nor F-actinaccumulated cathodally in serum-free medium, EGFR redistributionmight be both sufficient and necessary for subsequent actin asymmetry.(We cannot exclude the possibility that cathodal redistributionof some other receptor also might induce actin accumulation cathodally.)Intracellular EGFRs accumulated cathodally also, perhaps reflectinginitial asymmetry of membrane EGFRs and asymmetric internalization.Significantly, EGFRs also accumulated cathodally in cell sheets,and sheets of cells migrate cathodally (Zhao et al., 1996b). Thisis important because corneal wound healing involves migrationof cell sheets, which maintain intercellular linkages (Dua andForrester, 1989; Gipson and Sugrue, 1994). EF-induced F-actinredistribution to the leading edge of single cells also may facilitateactin cable formation at the leading edge of healing cornea, aprocess that underlies the coordinated movement of cell sheets(Danjo and Gipson, 1998).

In mouse fibroblasts, EGFR activation disassembles focal contacts, and the extent of this is correlated with increasing migrationspeed (Xie et al., 1998). EF-directed, faster migration of CECson FN or LAM also may involve polarized focal contact disassemblyand integrin receptor redistribution (see above). We have no dataon integrin expression in migratory CECs, although the $alpha$ 5 $beta$ 1 FNreceptor redistributed on fibroblasts in a DC EF, with smalleraggregates accumulating cathodally and larger aggregates accumulatinganodally (Brown and Loew, 1996). Also, the LAM receptor $alpha$ 6 $beta$ 4 redistributesand spreads out in wounded corneal epithelium (in an endogenous,wound-induced EF) to break up and decrease focal adhesion in preparationfor cell migration (Gipson and Inatomi, 1995). Additionally, ACfield-directed migration of human macrophages was inhibited byantibodies to the $beta$ 2 but not the $beta$ 1 integrin subunit (Cho et al.,1997). Irrespective of the integrins involved, close colocalizationof EGFR, actin polymerization, and integrin receptor turnoverat dynamic substrate contact points are likely to underpin cathodalmigration. An interesting pattern of interdigitated, colocalizedEGFR clusters and F-actin was observed (Figure 6B'), particularlycathodally at the cell-substrate interface in CECs. The relationshipof this to directed cell migration or focal adhesion disassemblyis notknown.

Our data indicate asymmetries both on the membrane and intracellularly. The intracellular asymmetry of EGFR and F-actin suggestsa causal relationship between the asymmetries of membrane EGFRand membrane-associated F-actin and those of intracellular EGFRand F-actin. Live cells showed cathodal accumulation of EGFR within10 min in an EF (Figure 6A). Binding with EGF (Figure 7A) mayinitiate asymmetric cell signaling and EF-directed cell migration.As activated membrane EGFRs, the internalized receptors that remainassociated with EGF are also capable of phosphorylating endogenoussubstrates (Sorkin, 1996). Therefore, signals from activationof EGFRs may be expected from both membrane and intracellularEGFR-EGF complexes, and both are distributed asymmetrically inEFs. Asymmetry of intracellular proteins will not result directlyfrom EF exposure (because of the high resistance of the cell membrane);therefore, the new observations of cathodal accumulation of intracellularEGFR probably indicate asymmetric internalization of EGFR. Onesignaling pathway used by the EGFR to engage cell migration involvesMAPK (Klemke et al., 1997). The MAPK inhibitor PD98059 significantlyreduced EF-directed cell migration, further supporting the notionof asymmetric signaling triggered by asymmetric receptoractivation.

The TGFR and FGFR also accumulated cathodally but less strikingly and more slowly than the EGFR (Figure 9). TGF and bFGF partiallyrestored EF-directed migration in serum-free medium over 5 h (Zhaoet al., 1996a). Whether the mechanism involves receptor accumulationcathodally isunclear.

Physiological Significance

The basic mechanism of EF-directed cell motility and its relevance in corneal wound healing are key issues. EF-directed CECmigration may begin with cathodal redistribution of EGFRs andculminate with asymmetric polymerization of the actin cytoskeleton.Manipulations that enhanced cell speed and cathodal directedness,EF and EF plus FN or LAM, each up-regulated the EGFR and redirectedboth EGFR and actin cathodally. Higher, nonphysiological EFs,which did not up-regulate the EGFR, resulted in slower speed,although directedness was maintained (Zhao et al., 1996a,b). Becausegrowth factor receptor asymmetry can induce directed cell movement,perhaps enhanced directedness requires enhanced receptor asymmetry.The EGFR is widely expressed and tightly regulated and appearsto control many aspects of cell motility (Xie et al., 1998; Wareet al., 1998). It is satisfying and significant that a physiologicalEF may initiate directed cell movement by using EGFRsignaling.

Wounding collapses the transcorneal potential difference (PD) and creates a laterally directed EF (Chiang et al., 1992). CECscultured in a similar EF migrate directionally. However, thereis a question of polarity (Figure 10). The inside positive transcornealPD drives current (flow of positive charge) below the epitheliallayers, out the wound with a return path in the thin tear fluidfilm (Chiang et al., 1992). Direct measurements of the resultantlateral fields indicate that the higher resistance path, and theone across which the greater voltage drop is measured, is thetear fluid. In that layer, the wound is positive relative to distantsites (Figure 10); yet in culture CECs migrate cathodally. At subepithelialstromal levels, the resistance to current flow was much lower,establishing only a very small lateral fields, wound site negative(Chiang et al., 1992). However, what has not been determined experimentallyis the more relevant lateral fields immediately below the upperepithelial layer, where the tight junctons exist and across whichthe transcorneal PD is established (Klyce, 1972; Wolosin, 1988).Immediately below the migrating surface epithelia, cells are tightlypacked, with little extracellular space. Tissue resistance maybe substantial and may establish larger lateral fields with thewound negative. Several epithelial cell types maintain a normaltransepithelial resistance, with functional tight junctions upto a wound border (Hudspeth, 1982), whereas for newly apposedcells, tight junctions are formed within 15 min. In healing stratifiedcorneal epithelium, maintenance of functional tight junctionsis indicated by the presence of tight junction-specific proteinoccludin and ZO-1 just one cell back from the leading edge (Danjoand Gipson, 1998). Thus the upper aspect of a migrating sheetof epithelium may "see" the wound as an anode, whereas the lowersurface would see a cathode at the wound. In support of this,several reports have demonstrated suprabasal cells rolling overthe basal cells to assume a position at the leading edge of healingtongue in reepithelialization (Krawczyk, 1971; Garlick and Taichman,1994). This is consistent with a role for EF in directing cornealcell movement into a wound but may involve a complex push-pulltype of EF-induced behavior on the upper and lower surfaces, respectively,of a migrating corneal epithelial sheet (Figure 10).

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Figure 10. Model illustrating potential role of lateral EF in directing corneal epithelial migration at a wound edge. Beyond ~1 mm away from a wound, the transcorneal PD indicated at the left (+25 mV inside positive) is supported by the high resistance of the tight junctions in the upper sheet of epithelial cells. At the wound the PD collapses to zero, FN has replaced the normal basement membrane, and the upper sheet of epithelial cells rapidly slides down to make contact with the transient basement membrane within ~1 h (Kuwabara et al., 1976

). Direct measurements indicate that the lateral fields in the tear fluid are higher than those in the stroma. However (see DISCUSSION), the relevant subepithelial voltage drop immediately below the top sheet of corneal epithelium has not been measured and is likely to be substantial, given the tight packing of these differentiated and flattened cells. The lower surface of the cells of a sliding sheet therefore would be migrating toward a cathode. In corneal epithelial wounds, the tight junction-specific protein occludin is present just one cell back from the leading edge (Danjo and Gipson, 1998

	ACKNOWLEDGMENTS

We thank The Wellcome Trust and Dr. James Alexander Mearns' Trust for financial support, G. Flett for preliminary experiments,Dr. A.M. Rajnicek for helpful discussion, and Dr. J. Zhang (LawrenceBerkeley National Laboratory, University of California, Berkeley,CA) for help with initial staining methods. We thank our refereesfor their valuable comments and suggestions. This work was supportedby The Wellcome Trust and Dr. James Alexander Mearns' Trust, UnitedKingdom.

	FOOTNOTES

Corresponding authors. E-mail addresses: c.mccaig{at}abdn.ac.uk, m.zhao{at}abdn.ac.uk.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERNCES

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