The Catalytic Activity of the Src Family Kinases Is Required to Disrupt Cadherin-dependent Cell-Cell Contacts

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Vol. 11, Issue 1, 51-64, January 2000

The Catalytic Activity of the Src Family Kinases Is Required to Disrupt Cadherin-dependent Cell-Cell Contacts

Dewi W. Owens,^* Gordon W. McLean,^* Anne W. Wyke,^* Christos Paraskeva, E. Kenneth Parkinson,^* Margaret C. Frame,^*^§ and Valerie G. Brunton^*

^*The Beatson Institute for Cancer Research, CRC Beatson Laboratories, Glasgow G61 1BD, United Kingdom; and Department of Pathology and Microbiology, University of Bristol, School of Medical Sciences, Bristol BS8 1TD, United Kingdom

Submitted March 26, 1999; Revised November 3, 1999; Accepted November 10, 1999
Monitoring Editor: Joan Brugge

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Despite the importance of epithelial cell contacts in determining cell behavior, we still lack a detailed understanding ofthe assembly and disassembly of intercellular contacts. Here weexamined the role of the catalytic activity of the Src familykinases at epithelial cell contacts in vitro. Like E- and P-cadherin,Ca²⁺ treatment of normal and tumor-derived human keratinocytes resultedin c-Yes (and c-Src and Fyn), as well as their putative substratep120^CTN, being recruited to cell-cell contacts. A tyrosine kinase inhibitorwith selectivity against the Src family kinases, PD162531, anda dominant-inhibitory c-Src protein that interferes with the catalyticfunction of the endogenous Src kinases induced cell-cell contactand E-cadherin redistribution, even in low Ca²⁺, which does not normally support stable cell-cell adhesion. Time-lapsemicroscopy demonstrated that Src kinase inhibition induced stabilizationof transiently formed intercellular contacts in low Ca²⁺. Furthermore, a combination of E- and P-cadherin-specific antibodiessuppressed cell-cell contact, indicating cadherin involvement.As a consequence of contact stabilization, normal cells were unableto dissociate from an epithelial sheet formed at high densityand repair a wound in vitro, although individual cells were stillmotile. Thus, cadherin-dependent contacts can be stabilized bothby high Ca²⁺ and by inhibiting Src activity in low (0.03 mM) Ca²⁺ invitro.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Adherens junctions are among the principal types of cell-cell contacts between epithelial cells. They consist of calcium-dependenttransmembrane proteins of the cadherin superfamily, cell-celladhesion receptors that are linked to the actin cytoskeleton byanother group of proteins, the cytoplasmic catenins (reviewedby Cowin and Burke, 1996). The cadherin-catenin multiprotein complexesregulate a variety of fundamental biological processes, includingproliferation, differentiation, and cellular invasion (reviewedby Takeichi, 1991, 1993).

Despite the obvious importance of cadherin function as a determinant of cell behavior and cell fate, the regulation of assemblyand disassembly of cadherin-mediated cell-cell adhesions and therecruitment of signaling molecules to complexes at these adhesionsare not well understood. Recent work has indicated that in epithelialcells, the Rho family of small GTPases, in particular Rho andRac, are required for the formation of cadherin-mediated adhesionsand the stabilization of cadherins at these sites, mediated bytheir effects on the actin cytoskeleton (Braga et al., 1997).Consistent with a role for actin cytoskeletal remodeling in cadherin-mediatedcell-cell adhesion, high extracellular Ca²⁺ leads to the accumulation of actin at cell-cell contacts (Bragaet al., 1997). In addition to the small GTPases, protein kinasesmay also contribute to the regulation of cadherin-mediated cell-celladhesions with several reports, suggesting that recruitment of $beta$ -catenin is regulated by phosphorylation (Hinck et al., 1994;Balsamo et al., 1996; Rubinfeld et al., 1996).

Control of the disassembly of cadherin-mediated cell-cell adhesions is particularly relevant to cancer development. Earlystudies identified a clear trend among epithelial cancers, withthe more invasive tumor types expressing lower amounts of cadherins(Shimoyama and Hirohashi, 1991; Shiozaki et al., 1991; Takeichi,1991). In particular, loss of E-cadherin, the major adhesion moleculeof epithelia, is often associated with cancer progression (Birchmeieret al., 1993; Birchmeier and Behrens, 1994; Takeichi, 1993). Furthermore,when functional E-cadherin complexes are reestablished in epithelialtumor cells that have lost normal adherens junctions, E-cadherinspecifically acts as a suppressor of cancer cell invasion (Frixenet al., 1991; Vleminckx et al., 1991). More recently, a causalrole has been demonstrated for loss of E-cadherin-mediated cell-celladhesion during the adenoma to carcinoma transition in a transgenicmodel of pancreatic carcinogenesis (Peri et al., 1998), indicatingthat disruption of cadherin-mediated cell-cell adhesions is requiredfor tumor progression in vivo. In addition, a germ line mutationin the gene encoding E-cadherin, which gives rise to a truncatedprotein product, was recently shown to be responsible for familialtransmission of gastric cancer (Guilford et al., 1998).

There are also several lines of evidence that tyrosine phosphorylation may play a role in disruption of cell-cell adhesions.First, treatment of Madin-Darby canine kidney cells with vanadateleads to a concomitant increase in phosphotyrosine and deteriorationof cellular adherens junctions (Volberg et al., 1992). Second,v-Src activity in chick cells and rat 3Y1 cells perturbs cadherin-mediatedcell-cell adhesion (Matsuyoshi et al., 1992; Hamaguchi et al.,1993). Third, stimulation of tyrosine phosphorylation of the E-cadherin- $beta$ -catenincomplex by a temperature-sensitive v-Src protein in Madin-Darbycanine kidney cells correlates with loss of epithelial differentiationand gain of invasive potential (Behrens et al., 1993). Fourth,Ras-transformed breast epithelial cells have less developed adherensjunctions and increased tyrosine phosphorylation of junction components(Kinch et al., 1995). Fifth, migratory growth factors such ashepatocyte growth factor (or scatter factor) and epidermal growthfactor (EGF) induce dispersion or scattering of normal and malignantepithelial cells, most likely by tyrosine phosphorylation of cadherin-associatedproteins (Shibamoto et al., 1994; Sato et al., 1995). Furthermore,EGF-induced scattering of the rat bladder carcinoma cell lineNBT-11 requires the activity of both Src and Ras, although theseapparently induce their scattering effects by distinct mechanisms(Boyer et al., 1997).

Despite the wealth of data that tyrosine phosphorylation in general, and oncogenic Src kinases in particular, can affect theintegrity of cadherin-mediated cell-cell adhesions, a recent studyhas reported that tyrosine phosphorylation and the Src familykinases are associated with the formation of cell-cell adhesionsbetween mouse keratinocytes (Calautti et al., 1998). In particular,keratinocytes derived from fyn-deficient mice are impaired inthe formation of cell-cell junctions in vitro, as are epidermalcells in the skin of mice with a double disruption in the srcand fyn genes (Calautti et al., 1998). One reason for the apparentdiscrepancy may lie in the fact that the Src family kinases aremultidomain proteins that have adaptor or protein-protein interactionfunctions involving the Src homology domains, as well as catalyticactivity. Because gene disruption leads to ablation of all aspectsof cellular protein function, fyn and src null cells have proveduseful tools to demonstrate that the protein products of thesegenes are required for cell-cell junction assembly (Calautti etal., 1998). However, additional, more subtle, interventionistapproaches are required to determine the role of specific Srcactivities in the dynamic regulation of epithelial cell-cell adhesions.This notion is reinforced by the findings that in fibroblasts,where the Src family kinases are predominantly located in cell-extracellularmatrix (ECM) focal adhesions, disruption of the src gene leadsto reduced cell spreading and impaired focal adhesion assembly(Kaplan et al., 1995), whereas inhibition of the catalytic activityby a dominant interference results in impaired focal adhesionturnover and reduced cell motility (Fincham and Frame, 1998).

These findings prompted us to specifically investigate the role of the catalytic activity of the Src family kinases in humanprimary epithelial cells, which could be grown in serum-free,low-Ca²⁺ medium. We found that c-Yes (and the other ubiquitously expressedkinases c-Src and Fyn) and their putative substrate p120^CTN were recruited to cadherin-mediated cell-cell contacts in normalepidermal keratinocytes in response to elevating the extracellularCa²⁺. Furthermore, pharmacological and molecular inhibition of theSrc catalytic activity promoted the stability of cell-cell contactsand recruitment of E-cadherin to regions of contact, even in lowCa²⁺. In addition, a mixture of E- and P-cadherin-specific antibodiessuppressed intercellular contact. Thus, in keratinocytes in vitro,inhibition of the catalytic activity of the Src kinases promotesthe stability of cadherin-dependent cell-cell contacts, implyingthat Src kinase activity is normally required to disassemble cell-cellcontacts. Taken together with the findings of Calautti et al.(1998), our data further imply that, although activities of Srcother than its kinase may be required for assembly of epithelialcell-cell junctions, the induction of its catalytic activity afterrecruitment triggers the destabilization and disassembly of cadherin-dependentcell-cellcontacts.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell Culture

Normal Human Keratinocytes. Human epidermal keratinocytes (HEKs) were prepared from human foreskin tissue essentially as described by Parkinson et al.(1986), except that type I S trypsin inhibitor (Sigma, St. Louis,MO) was used instead of FCS-containing medium to neutralize trypsin.The cells were plated in keratinocyte growth medium (KGM; modifiedMCDB 153 medium [Clonetics, San Diego, CA] containing the followingsupplements: 0.4% bovine pituitary extract, 10 ng/ml epidermalgrowth factor, 0.5 µg/ml hydrocortisone, 5 µg/ml insulin, 50 ng/mlamphotericin-B and 50 µg/ml gentamicin). CaCl₂ solution was addedto give a final Ca²⁺ concentration of 0.03 mM (low Ca²⁺) or 1 mM (high Ca²⁺). HEKs were routinely maintained in low-Ca²⁺ KGM in a humid 37°C/5% CO₂ incubator and were always subculturedbefore reaching confluence. All experiments were performed usingcultures between passages 2 and 5. Cytochalasin D (Sigma) wasprepared as a 5 mg/ml stock solution in DMSO and was used at afinal concentration of 5 µg/ml. PD162531 (a gift from A. Kraker,Parke-Davis, Ann Arbor, MI) was prepared as a 10 mM stock solutionin DMSO and used at a final concentration of 2 µM.

Malignant Human Keratinocytes. SCC-13 cells (a gift from J.G. Rheinwald, Dana-Farber Cancer Institute, Boston, MA; to E.K.P) were maintained in Dulbecco'smodified Eagle's medium (Life Technologies, Gaithersburg, MD)supplemented with 10% FCS, 2 mM L-glutamine, and 0.4 µmg/ml hydrocortisoneon lethally irradiated 3T3 feeder cells. SCC-13/ecSrc-KD is acell clone derived from SCC-13, which can be induced to expresskinase-defective (KD) avian c-Src (K295M) with the ecdysone analoguemuristerone A (No et al., 1996). Kinase-defective c-Src was clonedas an XbaI fragment from pCA10-K (a gift from K. Kaplan, Massachusetts Institute of Technology,Boston, MA) into the pIND vector (Invitrogen, San Diego, CA).The resulting plasmid (pIND-295) was introduced into SCC-13 cellsin combination with pRXR (Invitrogen) using N-1-(2,3-dioleoyloxy)propyl]-N,N,N,-trimethylammoniummethyl sulfate liposomal transfection reagent (Boehringer Mannheim,Indianapolis, IN). Stable cell lines were selected using a combinationof 800 µg/ml G418 and 250 µg/ml zeocin and were tested for theirability to express kinase-inactive c-Src in response to inductionwith 10 µM muristerone A by immunoblotting with avian-specificmAb EC-10 (Upstate Biotechnology, Lake Placid, NY). For experimentsinvolving manipulation of the extracellular Ca²⁺ concentration, SCC-13 cells were temporarily maintained in KGM.For the experiments to monitor drug selectivity, SCC13 cells weregrown in KGM in the absence of EGF for 16 h before stimulationwith 2 ng/ml EGF for 10min.

Time-Lapse Video Microscopy

HEKs were seeded at low density in low-Ca²⁺ KGM and were treated with 2 µM PD162531 (DMSO for controls) or were transferredto high-Ca²⁺ medium. The cells were visualized using a phase-contrast microscopeequipped with a heated stage, and images were recorded at 10-minintervals using a charge-coupled device camera. The relative ratesof cell motility of individual cells were calculated by computertracking of individual cells that did not come into contact ineach frame of the time-lapse series and computing distance traveledin a given time using Openlab software (Improvision, Coventry,United Kingdom). The average speed of a number of cells grownin low Ca²⁺, low Ca²⁺ with PD162531, or high Ca²⁺ was calculated using Excel (Microsoft, Redmond, WA), and themean speed in low Ca²⁺ was designated as 100%.

Wound-healing Assay

HEKs or SCC-13/ecSrc-KD cells were grown to confluence in six-well plates (Costar, Cambridge, MA) in low-Ca²⁺ KGM. Monolayers were wounded using a plastic micropipette tip,and the cells were rinsed with low-Ca²⁺ KGM before visualization using a phase-contrast microscope. Thecells were treated with either 2 µM PD162531 (DMSO for controls)or 10 µM muristerone A or were transferred to high-Ca²⁺ medium and returned to a 37°C incubator for 16 h before recordingwoundrepair.

Protein Immunoblotting and Immunoprecipitation

Cells were lysed in 10 mM Tris, pH 7.4, 1% Triton X-100, 150 mM NaCl, 1 mM EDTA, 10 mM inorganic tetrasodium pyrophosphate,2 mM PMSF, 100 µM Na₃VO₄, 0.5 mM NaF, and 0.1% aprotinin (Sigma).Extracts were assayed for protein content using the Micro BCAprotein assay kit (Pierce, Rockford, IL) after clarification byhigh-speed centrifugation at 4°C. Lysates were boiled in high-SDSsample buffer and separated by discontinuous SDS-PAGE under reducingconditions before transfer to nitrocellulose. Proteins were detectedby probing with 0.125 µg/ml anti-E-cadherin mAb (TransductionLaboratories, Lexington, KY), 0.25 mg/ml anti-Yes mAb (TransductionLaboratories), 0.1 µg/ml anti-Src mAb 327 (Calbiochem, La Jolla,CA), or 1 µg/ml anti-avian Src mAb EC10 (Upstate Biotechnology)diluted in 5% nonfat milk in PBS/0.2% (vol/vol) Tween 20. Detectionof bound antibody was by reaction with horseradish peroxidase-conjugatedsecondary antibody (Amersham, Little Chalfont, United Kingdom),and visualization was by enhanced chemiluminescence(Amersham).

To test the selectivity of PD162531, SCC-13 keratinocytes were deprived of EGF for 16 h and 2 ng/ml EGF was added back for10 min. c-Src or EGF receptor was immunoprecipitated using 1 µgof anti-Src mAb 327 or 5 µg of anti-EGF receptor mAb (UpstateBiotechnology), respectively, and immunoprecipitated proteinswere collected and washed as described above, separated by 7%SDS-PAGE, and immunoblotted using 1 µg/ml anti-phosphotyrosinePY20 (Transduction Laboratories) in the case of EGF receptor oreither 0.1 µg/ml anti-Src mAb 327 or 0.5 µg/ml immunoglobulinG (IgG) specific for c-Src that is phosphorylated at tyrosine419 of the human sequence (phospho-423-Y; BioSource International,Camarillo,CA).

Immune Complex Kinase Assays

Src Family Kinases. Lysates were prepared in Src lysis buffer (10 mM 1,4-piperazinediethanesulfonic acid, pH 6.8, 50 mM NaCl, 3 mM MgCl₂, 300mM sucrose, 0.5% Triton X-100, 10 mM sodium pyrophosphate, 2 mMphenylmethylsulfonyl fluoride, 100 µM Na₃VO₄, and 0.1% aprotinin),and c-Src, c-Yes, and c-Fyn were then immunoprecipitated using0.5 µg of antisera (c-Src, mAb 327, c-Yes, and c-Fyn; Santa CruzBiotechnology, Santa Cruz, CA). Immunoprecipitates were washedfive times in lysis buffer, followed by one wash in kinase buffer(100 mM 1,4-piperazinediethanesulfonic acid, pH 6.8, 20 mM MnCl₂,10 µM Na₃VO₄), and then resuspended in 10 µl of kinase buffer.The immune complexes were incubated with [ $gamma$ -³²P]ATP (1 µM, 5 µCi; Amersham; specific activity, 3000 Ci/mmol)and 0.3 mM Src substrate peptide (Upstate Biotechnology) in thepresence or absence of 100 nM PD162531. After incubation at 30°Cfor 10 min, the reaction was stopped by addition of excess unlabeledATP and chilling on ice. The reaction mixes were spotted ontoWhatman (Maidstone, United Kingdom) P81 paper discs, and the discswere then washed three times in 10% trichloroacetic acid. Thediscs were transferred to scintillation vials, and the radioactivitywas determined. Control reactions without peptide were alsoperformed.

EGF Receptor Kinase. Lysates were prepared in EGF receptor lysis buffer (20 mM HEPES, pH 7.5, 150 mM NaCl, 10% glycerol, 1% Triton X-100, 1.5 mMMgCl₂, 1 mM EGTA, 10 mM sodium pyrophosphate, 2 mM phenylmethylsulphonylfluoride, 100 µM Na₃VO₄, and 0.1% aprotinin). The EGF receptorwas then immunoprecipitated from clarified lysates with 5 µg anti-EGFreceptor mAb (Upstate Biotechnology). The immunoprecipitates werewashed twice with HNTG buffer (20 mM HEPES, pH 7.5, 10% glycerol,and 0.1% Triton X-100) containing 500 mM NaCl and then three timeswith HNTG buffer containing 150 mM NaCl and resuspended in 10µl of HNTG buffer containing 150 mM NaCl. The immune complexeswere incubated with 5 mM MnCl₂, 100 µM Na₃VO₄, and 10 ng/ml EGFon ice for 5 min in the presence or absence of 100 nM PD162531.After addition of [ $gamma$ -³²P]ATP (1 µM, 5 µCi; Amersham; specific activity, 3000 Ci/mmol),the immune complexes were incubated at 30°C for 10 min, and thereaction was then stopped by addition of Laemmli sample buffer(double strength). The products were separated by 7% SDS-PAGE,and phosphorylation of the EGF receptor was detected by autoradiographyand quantitated bydensitometry.

Confocal Immunofluorescence Microscopy

Cells were grown on chamber slides (Nunc, Naperville, IL) and fixed and permeabilized in methanol for 20 min on ice (HEK andSCC-13). Cells were then blocked with 10% FCS in 120 mM NaCl,6 mM KCl, 1.2 mM MgCl₂, 1 mM CaCl₂, and 25 mM HEPES, pH 7.4, andincubated with primary antibodies diluted in this blocking solutionfor 1 h at room temperature: 1 µg/ml anti-E-cadherin mouse mAb,2.5 µg/ml anti-p120^CTN mAb (Transduction Laboratories), 2.5 µg/ml anti-c-Yes Mab (TransductionLaboratories), 1:100 anti-Src mAb N2-17 ascites fluid (a giftfrom Dr. T. Hunter, The Salk Institute, San Diego, CA), 1:100anti-Fyn (Santa Cruz), or 1:100 anti-vinculin (Sigma). Bound antibodywas detected using 15 µg/ml FITC-labeled anti-mouse IgG (JacksonImmunoResearch, Stratatech Scientific, Luton, United Kingdom)and visualization was via a confocal microscope (MRC600; Bio-Rad,Hercules,CA).

Cadherin Blocking Experiments

Cells were grown on chamber slides in 200 µl of medium containing low Ca²⁺, and either PD162531 was added or cells were transferred to highCa²⁺. For 1 h before addition of PD162531, a mixture of anti-E-cadherinand anti-P-cadherin antibodies was added. For blocking experimentsthe antibodies used were anti-E-cadherin (DECMA-1; Sigma; at 1:20final dilution) and anti-P-cadherin (NCC-CAD-299; Worthington,Freehold, NJ) at 100 µg/ml final concentration). Cells were visualizedby phalloidin staining of their polymerizedactin.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Ca²⁺-induced Translocation of c-Yes (and c-Src and Fyn) to Epithelial Cell-cell Contacts Requires the Actin Cytoskeleton

Although c-Src protein expression is required for optimal cell spreading and focal adhesion assembly in fibroblasts (Kaplanet al., 1995), our previous work demonstrated that Src proteinsare recruited into newly assembling focal adhesions by an actin-dependentprocess that does not require Src catalytic activity (Finchamet al., 1996; Fincham and Frame, 1998). In particular, v-Src proteinis recruited to cell-ECM focal adhesions in fibroblasts from whereit induces focal adhesion turnover during oncogenic transformationand cell motility (Fincham and Frame, 1998). These data, togetherwith the ability of v-Src to induce disruption of cadherin-mediatedcell-cell adhesions in epithelial cells (Matsuyoshi et al., 1992;Volberg et al., 1992; Behrens et al., 1993; Hamaguchi et al.,1993; Takeda et al., 1995) and the enrichment of rat liver hepatocyteadherens junctions for Src family kinases (Tsukita et al., 1991),led us to examine the subcellular localization of the endogenousSrc kinases in normal and malignant human epithelial cells inlow and high Ca²⁺ and the role of their combined catalytic activities. Specificimmunostaining for all three ubiquitous kinases, c-Yes, c-Src,and Fyn, was diffuse in the cytoplasm of normal epidermal keratinocytesmaintained in low-Ca²⁺-containing medium (confocal images shown for c-Yes in Figure1A). Elevating the extracellular Ca²⁺ induced c-Yes (and c-Src and Fyn) to translocate to regions ofcell-cell contact (shown for c-Yes in Figure 1B) in a manner thatwas indistinguishable from Ca²⁺-induced relocalization of both E- and P-cadherin to the cellperiphery (our unpublished results). Ca²⁺-induced translocation of the Src kinases to cell-cell contactswas sensitive to 5 µg/ml cytochalasin D (shown for c-Yes in Figure1C), implying that their recruitment to contacts required an organizedactin cytoskeleton. This, together with the requirement for thecytoskeletal modulators Rho and Rac in Ca²⁺-induced relocation of E-cadherin (Braga et al., 1997), impliesa general role for the actin cytoskeleton in the recruitment ofcomponents of cell-cell contacts, including the endogenous Srckinases. In addition to c-Yes (and c-Src and Fyn), their putativesubstrate p120^CTN also underwent Ca²⁺-induced translocation to cadherin-mediated cell-cell contacts(Figure 1E). We also found that the Src kinases were similarlyredistributed in a tumor-derived keratinocyte cell line (SCC-13;Rheinwald and Beckett, 1981). Thus, the Src family kinases undergoCa²⁺-induced, actin-dependent translocation to cadherin-mediated cell-cellcontacts in normal and tumor-derived human epithelial cells.

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Figure 1. c-Yes and p120^CTN translocate to cell-cell adhesions in epithelial cells in response to high Ca²⁺. Shown are confocal immunofluorescence micrographs of primary human epidermal keratinocytes, HEKs (A-E), and SCC-13 (F and G) cells stained with anti-c-Yes (A, B, C, F, and G) or anti-p120^CTN (D and E). HEKs were maintained in low Ca²⁺ (A and D) or transferred to high Ca²⁺ for 24 h (B, C, and E). SCC-13 cells were transferred to low-Ca²⁺-containing medium for 24 h (F) and were subsequently transferred to high Ca²⁺ for 24 h (G). Cytochalasin D was added to HEKs at a concentration of 5 µmg/ml as they were transferred to high Ca²⁺ (C). Bars, 25 µm.

Because we, and others, have shown that c-Src and v-Src are translocated to newly forming focal adhesions in fibroblasts (Kaplanet al., 1995; Fincham et al., 1996), we addressed whether c-Yes,(or c-Src or Fyn) could also be detected in keratinocyte cell-matrix(ECM) focal adhesions. For this, we used immunofluorescence confocalmicroscopy to scan through cells until vinculin-stained focaladhesions at the bottom of the cells were observed in low andhigh Ca²⁺ (our unpublished results). When cells stained with c-Yes (orc-Src or Fyn) were similarly scanned, we could not detect anystaining in focal adhesion structures (our unpublished results).Thus, the predominant recruitment of these kinases to sites ofcell-cell contact in primary human keratinocytes treated withhigh extracellular Ca²⁺, and the absence of detectable levels in keratinocyte focal adhesions,is in contrast to the situation in fibroblasts, where the Srckinases are predominantly in cellular focal adhesions. However,we cannot exclude the possibility that c-Yes, c-Src, or Fyn maybe present in keratinocyte cell-ECM adhesions at levels that arenot detectable byimmunofluorescence.

A Selective Inhibitor of the Src Family Kinases and a Dominant Inhibitory c-Src Protein Stimulate Cell-Cell Contact in Low Ca²⁺

To determine the physiological role of the catalytic activity of the cellular Src kinases in epithelial cells, we inhibitedtheir activity in two ways. First, we used a pharmacological tyrosinekinase inhibitor, PD162531, which selectively inhibits Src familykinases (provided by A. Kraker, Parke-Davis). Treatment of normalepidermal keratinocytes with 2 µM PD162531 in low-Ca²⁺-containing medium had no effect on cell growth (our unpublishedresults) but resulted in the formation of tightly packed clustersof cells (Figure 2A, right panel). In addition, treatment of thecells with PD162531 stimulated E-cadherin redistribution fromrelatively diffuse cytoplasmic staining in low-Ca²⁺-containing medium (Figure 2B, left panel) to cell-cell contactsinduced by the drug (Figure 2B, right panel). Similar effectsof PD162531 were observed after treatment of the tumor-derivedSCC-13 keratinocytes (our unpublished results). To confirm theselectivity of PD162531 in vivo, we compared its effects on EGFreceptor (EGF-R) autophosphorylation (because EGF is the majorgrowth factor present in serum-free KGM medium) and c-Src autophosphorylation,after SCC13 keratinocytes that had been grown in EGF-deprived,low-Ca²⁺ KGM medium had been treated with 2 ng/ml EGF for 10 min. Theaddition of 2 µM PD162531 suppressed phosphorylation of c-Srcon tyrosine 419, the presumed site of Src autophosphorylation(equivalent to tyrosine 416 in the avian sequence; Smart et al.,1981), as judged by reduced reactivity of immunoprecipitated c-Srcwith an antibody raised against a peptide containing tyrosine419 in its phosphorylated form (Figure 2C, upper panel). In contrast,EGF-R tyrosine phosphorylation was not substantially altered bydrug treatment (Figure 2C, lower panel). These findings indicatethat PD162531 is likely to be a more selective inhibitor of theSrc family kinases in vivo than previously used agents, such asherbimycin A, genistein, or tyrphostins. However, although thesedata are supportive of selectivity against Src in vivo, it isbased on the assumption that tyrosine 419 phosphorylation is theresult of autophosphorylation, and we note that this has not formallybeen proven in vivo.

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Figure 2. The Src-selective inhibitor PD162531 induces cell-cell contact and E-cadherin redistribution. (A) Phase-contrast images; (B) E-cadherin confocal immunofluorescence micrographs of HEKs maintained in low Ca²⁺ and treated with 0.02% DMSO (vol/vol) as controls (left panels) or with 2 µM PD162531 for 24 h (right panels). Bars, (A) 200 µm; (B) 25 µm. (C) SCC-13 tumor-derived keratinocytes, which also responded to PD162531, were grown in KGM serum-free medium and were deprived of exogenous EGF for 16 h, before restimulation with 2 ng/ml EGF (+ EGF) for 10 min in the absence ( $-$ ) or presence (+) of 2 µM PD162531. Presumed c-Src autophosphorylation was monitored by immunoprecipitating cell lysates with anti-Src (mAb 327) and immunoblotting using anti-Src (phospho-423-Y) as probe (upper left panel). Control immunoprecipitations were blotted with anti-Src (mAb 327; upper right panel). EGF-R autophosphorylation was monitored by immunoprecipitating untreated ( $-$ EGF) or EGF-treated (+ EGF) cell lysates with anti-EGF-R and immunoblotting with anti-phosphotyrosine. (D) In vitro kinase activities were measured as described in MATERIALS AND METHODS in the presence and absence of 100 nM PD162531. The kinase activities in the presence of drug are expressed as a percentage of untreated activities.

We also confirmed by immune complex kinase assays that PD162531 potently inhibited the tyrosine kinase activity of all threeubiquitous family members c-Yes, c-Src, and Fyn in vitro, at concentrationsthat were not inhibitory to EGF-R autophosphorylation in vitro(shown for 100 nM PD162531 in Figure 2D); furthermore, althoughPD162531 also has some activity against the receptors for bothbasic fibroblast growth factor (bFGF) and platelet-derived growthfactor (PDGF), the drug is at least 8 and 50 times more potentat inhibiting the Src family kinases than the bFGF receptor andthe PDGF receptor in vitro, respectively (Kraker, Parke-Davis,personal communication). Thus, treatment of normal keratinocyteswith a tyrosine kinase inhibitor that exhibits selectivity forthe Src family kinases induced cell-cell contact, even in lowCa²⁺ that does not normally support stable cadherin-mediated cell-celladhesion (Figure 2, A and B, left panels). That this effect ofPD162531 was not mediated by inhibition of either PDGF receptoror bFGF receptor is supported by the facts that cultured keratinocytesdo not express the PDGF receptor (Ansel et al., 1993), and thatat the concentration used, the drug did not have any effect oncell growth, although bFGF is known to positively influence keratinocytegrowth (Sarret et al., 1992).

To complement the pharmacological approach, and to more rigorously test the role of Src kinase activity, we generated SCC-13cells that expressed an ecdysone-inducible, kinase-inactive c-Srcprotein (SCC-13/ecSrc-KD). Kinase-inactive mutants of Src havebeen widely used and effectively block the functioning of thecatalytic activity of the endogenous cellular Src family by actingin a dominant-negative manner (Twamley-Stein et al., 1993; Finchamand Frame, 1998). Treatment of SCC-13/ecSrc-KD keratinocytes with10 µM muristerone A, an analogue of ecdysone, efficiently inducedexpression of the exogenous avian kinase-inactive c-Src protein(Figure 3A, upper panel). The extent of overexpression was severalfold,as judged by immunoblotting control and muristerone A-treatedcells with an antibody (mAb 327) that recognizes both endogenousand exogenous c-Src-KD protein (Figure 3A, lower panel). MuristeroneA treatment of these cells in low Ca²⁺ also induced cell-cell contact, resulting in areas of clusteredcells (Figure 3B, right panel), an effect similar to that inducedby the Src inhibitor PD162531 in normal keratinocytes (Figure2A). In contrast, parental SCC-13 cells were unaffected by muristeroneA (our unpublished results). Furthermore, muristerone A stimulatedredistribution of cytoplasmic E-cadherin in SCC-13/ecSrc-KD cellsto regions of cell-cell contact (Figure 3C, right panel). Thus,induction of a dominant-inhibitory, kinase-inactive c-Src proteinin tumor-derived keratinocytes had an effect similar to that ofthe Src-selective inhibitory drug PD162531 in normal keratinocytes,by stimulating the formation of cell-cell contacts at which E-cadherinwas present.

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Figure 3. Induction of a kinase-defective (KD) c-Src protein also induces cell-cell contact and E-cadherin redistribution. (A) Immunoblot using avian-specific mAb EC10 to detect only exogenous c-Src-KD expression in SCC 13 parental cells and SCC-13/ecSrc-KD transfectant cells that were untreated (uninduced), treated with ethanol alone (control), or treated with 10 µM muristerone A for 24 h (upper panel). Both endogenous and exogneous Src expression were monitored by immunoblotting with anti-Src (mAb 327) that reacts with both human and avian Src (lower panel), (B) Phase-contrast images; (C) E-cadherin confocal immunofluorescence micrographs of SCC-13/ecSrc-KD cells maintained in low Ca²⁺ and untreated (left panels) or treated with 10 µM muristerone A for 24 h (right panels). Bars, (B) 200 µm; (C) 25 µm.

One explanation for these data is that cell-cell contacts were being transiently assembled and disassembled as cells cameinto contact during routine keratinocyte cell culture and thatthis dynamic regulation was perturbed either by Ca²⁺ addition or by inhibition of Src kinase activity, both stimulistabilizing transiently assembled cell-cell contacts. If true,this implicates Src catalytic activity in cell-cell contact disassemblyin both normal keratinocytes (HEKs) and in malignant keratinocytesthat retain expression of E-cadherin (such as SCC-13). Treatmentof keratinocytes with PD162531 or muristerone A had no significanteffect on cell growth at the concentrations used, and the effectof the Src inhibitor on cell-cell contact was completely reversible(our unpublished results), indicating that Src kinase inhibitionwas not toxic to culturedkeratinocytes.

Inhibiting Src Kinase Activity Stabilizes Cell-Cell Contacts

To test the prediction that Src catalytic activity is required to disassemble transiently formed cell-cell contacts in lowCa²⁺, we carried out time-lapse phase-contrast imaging of low-densitykeratinocytes. We found that as cells collided in untreated culturesand formed transient associations, they were subsequently ableto free themselves from one another (Figure 4A, upper panel).In contrast, when exposed to the Src-inhibitory drug PD162531or high Ca²⁺, cells that collided remained in contact with one another, evenafter several hours (Figure 4A, middle and lower panels). Quantitationof the time individual cells remained in contact with other cellsduring a 6-h treatment period is shown (Figure 4B). In addition,if the above explanation is correct, individual cells must remainmotile to make contacts and cluster when Src catalytic activityis inhibited. Therefore, using time-lapse microscopy and computer-basedtracking of individual cells in sequential time-lapse images,we established that individual cells remained motile when treatedwith high Ca²⁺ or with the Src-selective inhibitor PD162531 (Figure 4C, andas exemplified by the cells marked with white arrows that havemoved between frames a and b under all three conditions shown,Figure 4A). However, in the presence of the PD162531 Src inhibitor,there was a drop in the rate of cell motility of individual cellsby ~40-50% (Figure 4C). Although the reason for this reductionwas not clear, because we were unable to detect any of the ubiquitous,Src kinases in cell-ECM adhesions, this was consistent with previousreports that Src activity is required for optimal cell motilityin fibroblasts (Hall et al., 1996; Fincham and Frame, 1998) andsuggests that low levels of the Src kinases may be present infocal adhesions or in the smaller focal complexes associated withlamellipodia.

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Figure 4. The Src-inhibitory drug PD162531 stabilizes cell-cell contacts. (A) Phase-contrast time-lapse images of low-density HEKs (in low Ca²⁺), which were treated with 0.02% DMSO (control, upper panel) or 2 µM PD162531 (middle panel) or transferred to high-Ca²⁺ medium (lower panel). Treatment with PD162531 or high Ca²⁺ began at 0 h and was continuous for the duration of the experiment. Individual cells are indicated by arrows. Bars, 50 µm. (B) The mean time that individual keratinocytes grown under different conditions spent in contact with other cells in the culture was determined by observing time-lapse images frame by frame. The duration of each intercellular contact formed by every cell in the time-lapse field (typically ~20 cells per experiment) was recorded and expressed as a percentage of the experiment time (6 h), and the mean contact time was plotted as percentage of time in contact. Thus, a value of 100% would indicate that all cell-cell contacts persisted for the duration of the experiment. (C) The migration of individual cells that did not come into contact with other cells (typically approximately six cells per experiment) was quantitated using Openlab software, and the mean pixels per frame value for control cells in low Ca²⁺ was defined as 100%. (D) c-Yes confocal immunofluorescence micrograph of HEKs maintained in low Ca²⁺. Specifically shown here is the contact region between two cells that have collided. Bars, 25 µm.

Thus, our data indicate that inhibition of Src catalytic activity induced cell clustering, most likely as a result of stabilizingtransient cell-cell contacts at which E-cadherin was present (Figures2 and 3). One potential problem with the conclusion that Src kinaseactivity is required for disruption of these transiently formedcell-cell contacts is that c-Yes, c-Src, and Fyn were apparentlylocated throughout the cytoplasm of isolated cells in low Ca²⁺ (Figure 1). However, upon further examination of immunofluorescencestaining of c-Yes in cells that had come into contact in low Ca²⁺, we noted that c-Yes was redistributed to the regions of transientcontact (Figure 4D). Thus, although c-Yes was cytoplasmic in isolatedcells in low Ca²⁺, it was located at sites of contact formed as a result of collisionbetween motile cells. Our data indicate that the catalytic activityof the Src family kinases at these sites is required for disruptionof transient cell-cell contacts in low Ca²⁺.

The Stabilization of Cell-Cell Contacts as a Result of Src Kinase Inhibition Involves Cadherins

Because E-cadherin redistributed to sites of cell-cell contact upon inhibition of Src catalytic activity, we sought to determinewhether the cadherins were involved in contact stabilization.Thus, cells were pretreated for 1 h with a mixture of E- and P-cadherin-specificantibodies. Cell clustering and strong actin staining at the peripheryof cells in the clusters were monitored by phalloidin reactivity.Although some random cell clustering occurs in HEK cultures inlow Ca²⁺ (Figure 5, top left panel), tight clustering was dramaticallystimulated by transfer to high Ca²⁺ or by treatment with the PD162531 Src-inhibitory drug (Figure5, top right and bottom left panels, respectively). However, inthe presence of both E- and P-cadherin-specific blocking antibodies,cell-cell contact and cell clustering were suppressed (Figure5, bottom right panel). This suppressive effect was specific tothe cadherin antibodies because equivalent concentrations of nonimmuneIgG had no effect on cell clustering, and $beta$ 1-integrin-specificantibodies induced cell detachment (our unpublished results).These data indicate that the cadherins have a role in the stabilizationof the intercellular contacts induced as a result of Src kinaseinhibition.

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Figure 5. The contacts stabilized as a result of Src kinase inhibition are cadherin dependent. Immunofluorescence images of cells stained with phalloidin-FITC are shown for HEKs in low Ca²⁺ (top left), high Ca²⁺ (top right), and low Ca²⁺ in the presence of the Src-inhibitory drug PD162531 (bottom panels) in the absence (left panel) and presence of a mixture of E- and P-cadherin-specific antibodies (right panel). Bars 100 µm.

Inhibiting Src Catalytic Activity Suppresses Repair of a Wounded Epithelial Monolayer

We next tested whether inhibition of the endogenous Src kinases affected the ability of cells present at the edge of a woundedkeratinocyte monolayer to break their intercellular contacts andmove freely out of the epithelial sheet and repair the wound.Confluent keratinocyte monolayers were wounded, and cell migrationinto the denuded area of individual cultures that were equivalentlywounded was monitored microscopically. Untreated HEKs had extensivelymigrated into the wound as individual rounded cells after 16 h[Figure 6A, low Ca²⁺ (16 h)]. Wound repair was unaffected by the presence of mitomycinC (our unpublished results), indicating that cell division wasnot a major component of the wound repair process. In contrast,HEKs treated with the Src-selective inhibitor PD162531, or withhigh extracellular Ca²⁺, were substantially impaired in their ability to migrate as individualcells into the wound [Figure 6A, PD162531 (16h) and high Ca²⁺ (16h), respectively], although the denuded area was narrowedas a consequence of forward movement of the edge of the epithelialsheet [compare low Ca²⁺ (16h) with PD162531 (16h)]. Thus, because individual keratinocyteswere motile under conditions that did not permit wound repair(Figure 4), we conclude that it was the freeing of individualcells from their epithelial neighbors in the sheet that was impairedin cells treated with the PD162531 Src inhibitor or with highextracellular Ca²⁺. Dose-response analysis confirmed that drug-induced impairmentof wound repair occurred at the same concentration range of PD162531as inhibition of Src Tyrosine-419 phosphorylation (Figure 6B),consistent with the drug having its biological effects via Srcinhibition. This was further supported by the impaired wound repairby individual cells dissociating from the epithelial sheet, whichwas observed in confluent SCC-13/ecSrc-KD cell cultures treatedwith muristerone A or with high Ca²⁺ (Figure 6C). These data indicate that the catalytic activityof the endogenous cellular Src kinases is required to induce disruptionof established cell-cell contacts that have formed in an epithelialsheet at high density and is necessary for cell dispersion andefficient repair of a wounded keratinocyte monolayer in vitro.

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Figure 6. The Src-inhibitory drug PD162531 and overexpression of the dominant-negative c-Src protein suppress keratinocyte wound healing in vitro. Phase-contrast photomicrographs show four individual HEK monolayers (A) or SCC-13/ecSrc-KD cells (B and C) grown to confluence in low Ca²⁺ and then wounded (example shown at t = 0) and either treated for 16 h (16h) with 0.02% DMSO (low Ca²⁺, 0 µM), 0.1, 1, 2, or 10 µM PD162531 as indicated (low Ca²⁺ + PD162531), or 10 µM muristerone A [low Ca²⁺ muristerone A (16h)] or transferred to high Ca²⁺ for 16 h [high Ca²⁺ (16h)]. Bars, 200 µm. White bars represent relative distances between the two edges of apposing epithelial sheets. Presumed c-Src autophosphorylation at the indicated drug concentrations was monitored by immunoprecipitating cell lysates with anti-Src (mAb 327) and immunoblotting using anti-Src (phospho-423-Y) as probe (B).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell motility is controlled, at least in part, by a cycle of cell attachment and detachment. In epithelial sheets where thecells themselves, rather than the underlying matrix, bear mostof the mechanical stress, this almost certainly involves the assemblyand disassembly of intercellular contacts. There is considerablecircumstantial evidence implicating tyrosine phosphorylation inthe disassembly of cadherin-mediated cell-cell contacts. Muchof this evidence is derived from experiments using the v-Src oncoprotein,which induces tyrosine phosphorylation of $beta$ -catenin, as well asp120^CTN (Reynolds et al., 1989) and E-cadherin (Papkoff, 1997), withconcomitant loss, or substantial weakening, of cadherin-mediatedadhesion (Matsuyoshi et al., 1992; Behrens et al., 1993; Hamaguchiet al., 1993; Shibamoto et al., 1994; Takeda et al., 1995). Inaddition, growth factors such as EGF and hepatocyte growth factorinduce tyrosine phosphorylation and dispersion or scattering ofresponsive epithelial cells (Weidner et al., 1991; Shibamoto etal., 1994). However, to date there is no direct experimental evidencethat tyrosine kinases are important for the E-cadherin-expressingtumor cell disaggregation that is required for invasion, and theidentity of putative endogenous cellular kinases that might bedirectly responsible has not beenestablished.

In the work presented here, we provide evidence that the catalytic activities of one or more of the endogenous cellular Srcfamily kinases are required for the disassembly of cell-cell contactsduring their dynamic regulation in normal and malignant humankeratinocytes in vitro. In normal skin in vivo, disruption ofepithelial cell-cell contacts is relevant to wounded epidermis,in which c-Yes locates at regions of cell-cell contact (Kreugeret al., 1991). In cultured human keratinocytes treated with highextracellular Ca²⁺, c-Yes (and c-Src and Fyn), as well as their putative substratep120^CTN, were recruited to cell-cell adhesions (Figure 1) in a mannerthat was indistinguishable from the translocation of both E- andP-cadherin. Furthermore, Ca²⁺-induced translocation of the Src kinases was blocked when theactin cytoskeleton was disrupted by cytochalasin D (Figure 1),implying that their recruitment to cadherin-mediated cell-celladhesions is an actin-dependent process, which requires reorganizationof the actin cytoskeleton. Consistent with this, Dsrc41, the Drosophilaclose relative of vertebrate c-Src, colocalizes with actin fibersand DE-cadherin in vivo during the development of Drosophila eyes(Takahashi et al., 1996). One possibility, previously suggestedby Braga et al. (1997), is that the Rho family of small GTPasesinduces the recruitment of cytoplasmic proteins to regions ofcontact between epithelial cells, mediated by their effects onthe actin cytoskeleton. The possibility that c-Yes and the otherSrc kinases are recruited in this way is consistent with our previousfindings that recruitment of v-Src to its site of action at thecell periphery of fibroblasts is also an actin-dependent processthat requires the activity of Rho proteins (Fincham et al., 1996).However, in contrast to fibroblasts, we were unable to detectany of the ubiquitous cellular Src family kinases in keratinocytefocaladhesions.

When normal epidermal keratinocytes were treated with an Src-selective tyrosine kinase inhibitor, PD162531, or tumor-derivedkeratinocytes were induced to express a dominant-negative, kinase-defectivec-Src protein, the cells clustered as a consequence of the formationof cell-cell contacts (Figures 2 and 3, respectively), an effectthat was accompanied by translocation of E- and P-cadherin tothe sites of intercellular contact. Thus, both pharmacologicaland molecular inhibition of the endogenous cellular Src familykinases were sufficient to induce the formation of cell-cell contactsat which the cadherins were present, even in low Ca²⁺. Using time-lapse microscopy, we demonstrated that when keratinocytesin low Ca²⁺ came into contact as they moved around in low-density culture,they formed transient cell-cell adhesions that were rapidly disassembledas cells broke apart. In cultures treated with the Src-inhibitorydrug PD162531, or with high Ca²⁺, cells also formed cell-cell contacts, but they were impairedin their ability to sever these contacts (Figure 4). The findingthat c-Yes accumulated at transiently formed cell-cell contactsin low Ca²⁺ from its cytoplasmic location in isolated cells (Figure 4) isconsistent with the proposed role in the regulation of cell-cellcontacts. Furthermore, we demonstrated that a combination of E-and P-cadherin-specifc antibodies was able to suppress contactformation induced by inhibition of cellular Src catalytic activity(Figure 5). Thus, our data provide the first clear demonstrationthat cellular Src activity at cadherin-dependent cell-cell contactsplays an important role in contact disruption. However, becauseall three ubiquitous members of the Src family are similarly locatedat intercellular contacts and are inhibited by both the Src-inhibitorydrug and dominant-negative c-Src protein, we are unable to concludewhether individual members of the Src family proteins have uniquefunctions at intercellularcontacts.

Because the experiments presented here were carried out using adherent keratinocytes, we were unable to draw conclusions aboutthe relative adhesive strength of intercellular contacts formedby inhibition of Src kinase activity and elevation of the extracellularCa²⁺. Although it would be possible, in principal, to measure adhesivestrength between keratinocytes in suspension, this would not necessarilyrelate to the strength or mode of regulation of intercellularcontacts formed between adherent keratinocytes in which the cellularcytoskeleton and adhesive properties are substantially different.This would be particularly true if the effects of inhibiting Srckinase activity were mediated by altered regulation of cytoskeletaldynamics. Thus, because the adhesive strength is unclear, we haveused "contacts" and not "adhesions" to describe the cadherin-dependentcell-cell junctions formed as a result of Src kinase inhibition.One possibility is that such contact formation is a prerequisitefor Ca²⁺-dependent, cadherin-mediated adhesion, and that the state ofcatalytic activation of one or more of the Src family kinasesat these contact sites determines whether transient contacts aredisassembled or are stabilized before formation of stronger cadherin-mediatedadhesions.

Because we, and others, have shown that the Src kinases are important components of the pathways that regulate cell motilityin fibroblasts (Hall et al., 1996; Fincham and Frame, 1998), wealso examined whether cells that formed stable cell-cell contactsas a result of Src inhibition were able to migrate into a woundin vitro. Normal keratinocytes treated with the PD162531 Src inhibitor,or tumor-derived keratinocytes induced to overexpress kinase-defectivec-Src, were unable to break free from their epithelial neighborsand migrate as individual cells into the denuded area of a confluentcell sheet (Figure 6). We confirmed using time-lapse microscopythat individual cells remained motile when the PD162531 Src inhibitorwas present, although the rate of cell motility was reduced by~40-50%, presumably as a result of interference with a relativelysmall amount of the Src kinases present in focal adhesions orfocal complexes. Thus, inhibition of the endogenous cellular Srckinase activity in keratinocytes leads to substantially impairedwound repair in vitro, at least in part as a result of the stabilizationof cell-cellcontacts.

Epithelial cancer cells can be divided into two classes with respect to cadherin-mediated cell-cell adhesion. One class havedysfunctional adhesions as a consequence of genetic loss or mutationof at least one adhesion component, and many of these cells haveundergone an epithelial to mesenchymal transition; consequently,they are relatively unrestrained in dissociating from the tumorand have the potential to invade freely into surrounding tissue.The other class have retained normal levels of functional cell-celladhesion components, yet many such cells are still able to freethemselves from the stable epithelia and invade and metastasize.Although the mechanisms used by the latter class of tumor cellsto deregulate stable cadherin-mediated contacts are not well understood,we have also found that release of individual cancer cells frominteraction with their neighbors requires the activity of theSrc family kinases at sites of cell-cell adhesion (Figure 6) andis a prerequisite for growth factor-induced invasion of epithelialcancer cells from a monolayer into Matrigel in vitro (our unpublishedresults). Taken together with the findings of others, we postulatethat migratory growth factors that induce epithelial cell dispersiondo so by stimulating Src-induced disassembly of cadherin-mediatedcell-cell contacts, a likely requirement for epithelial cancercell invasion. In this way, the aberrant regulation of a normalSrc-mediated process in epithelial cells may contribute to invasivebehavior. In this regard, activating mutations of the c-src genehave recently been associated with late-stage human colorectalcancers (Irby et al., 1999).

The mechanisms by which Src-induced tyrosine phosphorylation induces cadherin-mediated contact disassembly are not known,although it seems likely that phosphorylation of one or more crucialsubstrates triggers disruption. Although $beta$ -catenin is a candidatefor a triggering substrate, its role remains unclear because v-Src-inducedweakening of cadherin-mediated adhesions can occur in cells inwhich $beta$ -catenin is not involved in adhesion (Takeda et al., 1995).Other candidate substrates include the ERM proteins (ezrin/radixin/moesin)and ZO-1, which have been implicated as determinants of cadherin-dependentadhesion strength (Takeda et al., 1995; Imamura et al., 1999),and p120^CTN, which has recently been shown to bind to the juxtamembrane intracellulardomain of C-cadherin that is responsible for cadherin clusteringand adhesion strengthening (Yap et al., 1998). Although it isnot yet clear how p120^CTN contributes to cadherin clustering, it is possible that tyrosinephosphorylation may negatively regulate some p120^CTN-induced clustering function. Another possibility is that thecatalytic activity of the Src kinases at cadherin-mediated cellcontacts disrupts or destabilizes the actin cytoskeleton thatis required for adhesion maintenance (Braga et al., 1997). Insupport of the latter possibility, there is evidence that inhibitionof serine/threonine kinases inhibits epithelial cell-cell junctiondissociation by influencing the contractility of associated cytoskeleton(Citi et al., 1994). In addition to the mechanism of Src kinase-induceddisruption of cell-cell contacts, it remains to be establishedwhether Src activity at cadherin-mediated adhesions influencesthe downstream signaling pathways that originate at these intracellularsites.

In conclusion, our results demonstrate that the catalytic activity of the endogenous cellular Src family kinases disruptsepithelial cell-cell contacts during their dynamic regulationin low Ca²⁺ in vitro and is also required to free cells from the constraintsof their epithelial connections during in vitro wound repair.In contrast, the study by Calautti et al., (1998) demonstratedthat cells lacking c-Src and Fyn are impaired at forming cell-celljunctions in vitro and in vivo. This is summarized in the modelin Figure 7. Taken together, these findings indicate that in ananalogous manner to focal adhesion regulation in fibroblasts,aspects of Src function other than the catalytic activity, mostlikely adaptor functions associated with the Src homology domains,are required for epithelial cell-cell junction assembly, whereasthe kinase activity is required for subsequent cell-cell contactdisruption. This implies that the Src kinases are recruited tocadherin-dependent cell-cell contacts as they form, and subsequentstimulus-induced enzymatic activation may trigger cell-cell contactdisassembly. Our work further predicts that if clinically usefulanticancer drugs that specifically target the kinase activityof the Src family are developed, these will be of particular benefitin the treatment of potentially invasive tumors that have notlost functional cadherins or catenins.

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Figure 7. Model depicting the likely biological consequences of modulating Src kinase activity in E-cadherin-expressing epithelial cells. The weakening of intercellular contact stability may facilitate processes such as epithelial wound repair or cancer cell invasion.

	ACKNOWLEDGMENTS

We thank John Wyke, Val Fincham, Malcolm Finbow, and John Pitts for their helpful comments on this work and for critical readingof the manuscript. Thanks also to K. Kaplan for the plasmid-encodingkinase-inactive c-Src, to A. Malliri for help with time lapse,to A. Kraker and Parke-Davis for the PD162531 tyrosine kinaseinhibitor (and for allowing us access to information on its selectivity),and to T. Hunter and N. Carter for the N2-17 mAb against c-Src.This work was supported by the Cancer Research Campaign, UnitedKingdom (M.C.F., E.K.P., C.P., A.W.W., and G.W.M.) and by theMedical Research Council, United Kingdom (V.G.B. and D.W.O.).

	FOOTNOTES

These authors contributed equally to thiswork.

^§ Corresponding author. E-mail address: m.frame{at}beatson.gla.ac.uk.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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				J. Qi, J. Wang, O. Romanyuk, and C.-H. Siu Involvement of Src Family Kinases in N-Cadherin Phosphorylation and beta-Catenin Dissociation during Transendothelial Migration of Melanoma Cells Mol. Biol. Cell, March 1, 2006; 17(3): 1261 - 1272. [Abstract] [Full Text] [PDF]

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				A. M. Carothers, K. A. Melstrom Jr., J. D. Mueller, M. J. Weyant, and M. M. Bertagnolli Progressive Changes in Adherens Junction Structure during Intestinal Adenoma Formation in Apc Mutant Mice J. Biol. Chem., October 12, 2001; 276(42): 39094 - 39102. [Abstract] [Full Text] [PDF]

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