Functional role of {alpha}-actinin, PI 3-kinase and MEK1/2 in insulin-like growth factor I receptor kinase regulated motility of human breast carcinoma cells

doi:10.1242/jcs.00104

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doi: 10.1242/10.1242/jcs.00104

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Journal of Cell Science 115, 4149-4165 (2002)
Copyright © 2002 The Company of Biologists Limited
doi: 10.1242/jcs.00104

Research Article

Functional role of ${alpha}$ -actinin, PI 3-kinase and MEK1/2 in insulin-like growth factor I receptor kinase regulated motility of human breast carcinoma cells

Marina A. Guvakova¹^,*, Josephine C. Adams²^,3 and David Boettiger¹

^¹ Department of Microbiology, University of Pennsylvania, 3610 Hamilton Walk, 211 Johnson Pavilion, Philadelphia PA 19104, USA
^² MRC-Laboratory for Molecular Cell Biology and Department of Biochemistry and Molecular Biology, University College London, Gower Street, London WC1E 6BT, UK
^³ Department of Cell Biology, Building NC1, Lerner Research Institute, Cleveland Clinic Foundation, 9500 Euclid Avenue, Cleveland, Ohio 44195, USA

^* Author for correspondence (e-mail: guvakova{at}mail.med.upenn.edu)

Accepted 19 August 2002

Summary

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Summary
Introduction
Materials and Methods
Results
Discussion
References

Within epithelial tissue, cells are held together by specializedlateral junctions. At particular stages of development and inpathological processes such as metastasis, cells break downthe intercellular junctions, separate from the epithelial sheetand migrate individually. Despite the importance of these processes,little is understood about the regulatory mechanisms of activecell separation. In view of the effects of insulin-like growthfactor I (IGF-I) on mammary gland development and cancer, wedeveloped a model using MCF-7 human breast cancer cells in whichthe process of cell separation can be induced by IGF-I. Theseparation was enhanced in MCF-7 cells overexpressing the IGF-IRand blocked in the cells expressing a dead-kinase mutant ofthis receptor. Activation of the IGF-IR resulted in a rapidformation of motile actin microspikes at the regions of cell-cellcontacts, disorganization of mature adherens junctions and theonset of cell migration. In cell separation, the signaling betweenthe IGF-IR kinase and actin required phosphatidylinositol 3(PI 3)-kinase-generated phospholipids but not MAP kinases andwas mediated by ${alpha}$ -actinin. The activity of MEK1/2 kinases wasneeded for consecutive cell migration. This work also defineda new function for ${alpha}$ -actinin. Upon IGF-IR activation, green fluorescence protein(GFP)-labeled ${alpha}$ -actinin concentrated at the base of actin microspikes.Deletion of the N-terminal actin-binding domain of ${alpha}$ -actininprevented this redistribution, indicating that this domain is necessary.Delection of the C-terminal tail of ${alpha}$ -actinin reduced the numberof microspikes, showing that ${alpha}$ -actinin has a role in the developmentof microspikes and is not passively reorganized with filamentous actin.We suggest that the signaling pathway from the IGF-IR kinasethrough the PI-3 kinase to ${alpha}$ -actinin participates in the rapidorganization of actin into microspikes at the cell-cell junctionsand leads to active cell separation, whereas signaling throughERK1/2 MAP kinases controls cell migration following cell separation.

Key words: IGF-IR signaling, ${alpha}$ -actinin, Actin cytoskeleton, Breast cancer cell migration

Introduction

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Summary
Introduction
Materials and Methods
Results
Discussion
References

Differentiated epithelial cells are organized in contiguouslayers that protect the underlying connective tissue from theexternal environment and comprise the parenchyma of the innerorgans such as the glands. The lateral membranes of these adherentcells are connected via highly specialized adhesive junctionswhose formation and maintenance is critically dependent on linkageto the cytoskeleton: tight and adherens junctions are linkedto the cortical actin, whereas desmosomes are connected to thenetwork of intermediate filaments (Cowin and Burke, 1996; Daviesand Garrod, 1997). This unique tissue architecture allows epithelialcells to remain relatively static, except for during cell separationand migration that occur in development, tissue regenerationand metastasis (Gumbiner, 1996).

Some mechanistic aspects and common sequential changes thatprecede cell separation have been determined using animal andcellular models (reviewed in Hay, 1995; Thiery and Chopin, 1999; Savagner,2001). For example, epithelial colonies can be induced to separateby treatment with physiological peptides, including hepatocytegrowth factor/scatter factor (HGF/SF), neuregulin, members ofthe fibroblast growth factor (FGF), epidermal growth factor(EGF) and transforming growth factor (TGF) families (Stokerand Perryman, 1985; Savagner et al., 1997; Chausovsky et al.,1998; Müller et al., 1999). Peptides with cell scatteringfunction induce a disruption of intercellular junctions, a reorganizationof the actin cytoskeleton and an increase in local cell motility.These effects are mediated by receptor tyrosine kinases (Sachset al., 1996), of which the most extensively studied is Met,the receptor for HGF/SF (reviewed in Furge et al., 2000). Activationof Met has a strong effect on scattering and invasiveness ofthe rodent mammary epithelial cells and various human carcinomacell lines, and similar disorganization is believed to leadto metastasis (Wiedner et al., 1990; Liang et al., 1996; Fironet al., 2000). It is less clear, however, whether HGF/SF andMet control motile behavior of human breast tumor cells. Noscattering response to HGF/SF has been seen in human breastcarcinoma cell lines in vitro (Stoker et al., 1987); in breasttissue biopsies, the intensity of Met staining was lower intumor tissue than in normal cells adjacent to mammary ducts (Tsarfatyet al., 1992).

Another member of the receptor tyrosine kinase family is thereceptor for IGF-I, a protein of particular interest for thebiology of the human mammary gland. There is a general requirementfor IGF-I in terminal end bud formation and ductal morphogenesisin the developing gland (Kleinberg et al., 2000). In humans,the IGF-IR is expressed by both normal and tumor mammary cells;yet the level of the receptor expression and its tyrosine kinaseactivity is higher in malignant compared with benign and normaltissues (Happerfield et al., 1997; Resnik et al., 1998). The signalingmechanisms evoked by IGF-IR kinase are well documented (reviewedby LeRoith, 2000). Ligand-induced activation of the IGF-IR causesthe sequential phosphorylation of three conservative tyrosineswithin the catalytic domain, followed by phosphorylation ofthe cytoplasmic domain of the receptor, recruitment of adaptermolecules and initiation of signaling cascades. The two best-characterizedpathways triggered by the activation of this receptor are thePI3-kinase signaling via the insulin receptor substrates (IRSs)and the MAP kinase pathway via adaptor molecules Shc. AlthoughIGF-I may have a pleiotropic effect on cell proliferation, differentiationand migration (Leventhal and Feldman, 1997; Lee et al., 1998; Chernickyet al., 2000), the range of IGF-IR activities is criticallydependent on the cell context (Baserga, 1999). There is good evidencethat in cultured mammary epithelial cells the IGF-IR stimulatesnot only proliferative but also motile cell responses (Kohnet al., 1990; Doerr and Jones, 1996; Mira et al., 1999). Wehave recently reported that IGF-I treatment of breast cancercells overexpressing IGF-IR results in a disruption of the epithelialsheet, implying a role for this receptor in concomitant reorganizationof the actin cytoskeleton and cellular junctions (Guvakova andSurmacz, 1999).

The most prominent epithelial structures relying on the actincytoskeleton are adherence junctions. The core of these junctionsis composed of transmembrane E-cadherins and cytoplasmic ${alpha}$ ,ß-and ${gamma}$ -catenins (reviewed by Gumbiner, 2000). ${alpha}$ -catenin directlyor via actin-binding proteins ${alpha}$ -actinin and vinculin couplescadherin-catenin complexes to microfilaments (Knudsen et al.,1995; Nieset et al., 1997; Vasioukhin et al., 2000). Such alinkage is essential for the stabilization of intercellularadhesion and the maintenance of mammary epithelial tissue (Tsukataniet al., 1997). On the basis of the correlation between upregulationof the IGF-IR in breast tumors and the effects of the overexpressedIGF-IR on the actin cytoskeleton, we hypothesize that high levelsof IGF-IR activity can induce destabilization of cell-cell contacts.We report a novel signaling effect of the IGF-IR kinase in coupling ${alpha}$ -actinin and actin-containing microspikes by a PI 3-kinase-dependentmechanism at an early stage of epithelial cell separation.

Materials and Methods

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Summary
Introduction
Materials and Methods
Results
Discussion
References

Cell culture and reagents
MCF-7 human breast cancer cell line (ATCC, HTB-22) and its derivativeswere all grown in Dulbecco's Modified Eagle Medium: NutrientMixture F-12 (Ham) 1:1 (D-MEM/F-12) containing 5% calf serum(CS), penicillin and streptomycin at 37°C in 5% CO₂. Forovernight serum starvation, MCF-7 cells were incubated in phenolred-and serum-free D-MEM/F-12 containing 0.5 mg/ml bovine serumalbumin (BSA). The derivation of a clonal line of MCF-7 that overexpressedthe wild-type human IGF-IR 18-fold has been previously described (Guvakovaand Surmacz, 1997). This line is referred as MCF-7/IGF-IR/WTin this study. D-MEM/F-12, phenol-red-free D-MEM/F-12, CS andGeneticin (G418) were purchased from Gibco BRL, Life Technologies.LY 294002, PD 98059 and the Akt inhibitor were from Calbiochem,UO126 from Promega and human recombinant IGF-I from Bachem.

Molecular cloning and cell transfection procedures
MCF-7/IGF-IR/DK kinase-deficient cells were generated usinga IGF-IR ß subunit with mutations in the activationloop of the catalytic domain (three tyrosine residues, Y1131,Y1135, and Y1136 were substituted by phenylalanines). This DNAwas a gift from D. Leroith, NIH (Kato et al., 1994). The mutantIGF-IR cDNA was subcloned from the pBluscript II KS+ vectorinto the EcoRI and XbaI sites of the pcDNA3 expression vector (InvitrogenCorp., San Diego, CA) under the control of the CMV promoter.MCF-7 cells expressing the mutant receptor were derived by calcium-phosphate-precipitation-mediatedtransfection with a plasmid encoding the mutant hIGF-IR followedby selection in 2.5 mg/ml G418. Surface expression of the IGF-IRwas confirmed by fluorescence-activated cell sorting (FACS) usinga monoclonal antibody against the ${alpha}$ subunit of the IGF-IR anda secondary FITC-conjugated goat anti-mouse antibody (Vector).Stable clones expressing approximately 1.0x10⁶ IGF-IRs per cellwere isolated.

For functional analysis of ${alpha}$ -actinin, new DNA constructs encodingthe truncated ${alpha}$ -actinins with enhanced green fluorescent protein(EGFP) tagged to the C-terminus were generated. A full-lengthchicken sarcomeric ${alpha}$ -actinin (GenBank^TM accession number X59247)was obtained from J. Sanger (University of Pennsylvania) (Dabiriet al., 1997). A 230 amino-acid N-terminal truncation, includingresidues 1-24 in the potential site for regulation of high-affinitybinding of ${alpha}$ -actinin to actin (Xu et al., 1998) and residues 108-189in the actin-binding site determined by mutagenesis (Hemmingsat al., 1992), was produced by excision of a unique 5' Eco47III-EcoRV restrictionenzyme fragment, followed by blunt-end religation of the truncated plasmidDNA. In this mutant ${alpha}$ -actinin RNA, the authentic methionine startcodon is removed, and the translation is initiated at the AUGcodon for methionine 231. The deletion of the C-terminal tailof ${alpha}$ -actinin was generated by excision of a SacI fragment fromthe plasmid encoding full-length ${alpha}$ -actinin, followed by religationof the fragment into the SacI site of pEGFPN1 vector. The authenticinitiating codon is retained in this mutant. The removed regionencodes 168 amino acids, including a large part of a vinculin-bindingsite [residues 713-749 (McGregor et al., 1994)] and both EF-handCa²⁺-binding motifs (Baron et al., 1987). The proper deletionswere confirmed by restriction mapping of the N- and C- terminalregions of ${alpha}$ -actinin cDNA. The position of the truncated ${alpha}$ -actininsin frame with EGFP was verified using the Vector NTI version 3.0program (InforMax, Inc.).

In transient transfection experiments, 5x10⁴ MCF-7/IGF-IR/WTor MCF-7/IGF-IR/DK cells were plated into a 35 mm glass-bottomedculture dish (MatTek Corporation, Ashland, MA). The next day, thecells were transfected with plasmids encoding EGFP- ${alpha}$ -actinin constructsor the pEGFP-N1 control vector (Clontech) using LipofectaminePlus Reagent (Gibco, BRL). After 3 hours, the cells were washedin D-MEM/F-12 and incubated overnight in the conditioned mediumof MCF-7/IGF-IR/WT cells to improve the survival of the transfectants.The living cells were used in experiments 48 hours after transfection,when approximately 40% of cells produced fluorescently labeledprotein.

Western blotting and immunoprecipitation
Cells were lysed in buffer containing 50 mM Hepes pH 7.5, 150mM NaCl, 1.5 mM MgCl, 1 mM EGTA, 10% glycerol, 20 µg/mlaprotinin, 1 mM phenylmethylsulfonyl fluoride, 2 mM Na orthovanadateand either 1% Triton X-100 or 1% SDS. For western blots, 20µg of total protein was resolved by SDS-polyacrylamidegel electrophoresis (SDS-PAGE) and transferred to Hybond ECLnitrocellulose (Amersham Pharmacia Biotech). In a series ofexperiments, the blots were probed with antibodies against IGF-IR(rabbit polyclonal anti-IGF-IR ß subunit, Santa Cruz,SC); IRS-1 (rabbit polyclonal anti-IRS-1, Upstate BiotechnologyInc., UBI, Lake Placid, NY); ${alpha}$ -actinin (mouse IgG clone AT6/172,UBI and goat polyclonal anti- ${alpha}$ -actinin antobodies, SC); ${alpha}$ -catenin(rabbit polyclonal antibodies, Sigma); GFP (mouse monoclonalantibody, Clontech Laboratories, Inc.); phospho-Akt (rabbit anti-phospho-Akt(Ser 473), rabbit anti-phospho-Akt (Thr 308), New England Biolab,NEB); Akt (rabbit anti-Akt, NEB); phospho MAPK (mouse monoclonalE10, anti-phospho-p44-42 MAPK (Thr 202/Tyr 204), NEB); ERK1/ERK2(rabbit polyclonal k23 anti-ERK1, SC), and phospho-tyrosine-containingproteins (mouse monoclonal PY-20 anti-phosphotyrosine, SC).For immunoprecipitation of ${alpha}$ -actinin, 500 µg of total proteinfrom 1% SDS cellular extracts was incubated with 4 µgof anti- ${alpha}$ -actinin monoclonal IgG₁, clone AT6/172 (UBI) and 50µl anti-mouse IgG-agarose beads (Sigma) in HNTG buffer(20 mM Hepes pH 7.5, 150 mM NaCl, 0.1% Triton X-100, 10% glycerol)overnight at 4°C. The immunoprecipitated proteins were resolvedby SDS-PAGE and blotted with anti- ${alpha}$ -actinin and PY 20 antibodies.To visualize primary antibody-bound protein, the secondary antibodiesconjugated to horseradish peroxidase (1:10,000 dilution; Calbiochem)and the ECL detection solutions (Amersham Pharmacia, UK) wereapplied. The chemiluminescent intensity of the bands was digitizedusing the Image Analyser LAS-1000 plus system and the ImageReader LAS-1000 Lite version 1.0 software (Fuji). When severalproteins were to be detected on the same membrane, nitrocellulosewas incubated in stripping buffer (100 mM 2-mercaptoethanol,2% SDS, 62.5 mM Tris-HCl pH 6.7) for 30 minutes at 50°C,then washed three times in washing buffer (100 mM Tris pH 7.5,1M NaCl, 1% Tween-20), blocked in 5% BSA in PBS and re-probed.The relative activity of the protein kinase B (PKB/Akt) andmitogen-activated protein (MAP) kinases was quantified as theratio of phosphorylated protein to the corresponding total proteindetected on the same blot.

Indirect immunofluorescence microscopy
To visualize filamentous actin (F-actin), cells grown on 22mm (no. 1) glass coverslips were fixed with 3.7% formaldehydein PBS for 15 minutes, permeabilized with 0.05% Triton X-100in PBS for 5 minutes and stained with tetramethylrhodamine Bisothiocyanate (TRITC)-phalloidin (1 µg/ml) (Sigma) for30 minutes. Changes in the intracellular distribution of ${alpha}$ -actinin wereassessed in formaldehyde-fixed cells using an anti- ${alpha}$ -actinin antibody(clone BM-75.2; Sigma) (1:200) followed by fluorescein isothiocyanate (FITC)-conjugatedgoat anti-mouse antibody (Vector). Distribution of ${alpha}$ -cateninwas assessed in formaldehyde-fixed cells using an anti- ${alpha}$ -cateninantibody (Sigma) (1:200) followed by a Rhodamine-Red-conjugatedgoat anti-rabbit antibody (Jackson ImmunoReseasrch Laboratories,Inc). Fascin was visualized in methanol-fixed cells using antibody55k-2 as described previously (Guvakova et al., 2002). The sampleswere examined under a Nikon Eclipse E600 MRC 1024 confocal laser-scanning(Bio-Rad) microscope with a Plan Apo 60x/1.4 oil objective lens(Nikon). Images were acquired using the Bio-Rad LaserSharp 2000 softwarerun under the OS/2 Warp ConnectTM operating system. Images were collectedas stacks of xy optical sections (z-series) taken at differentfocal planes within the sample.

Transmission electron microscopy
Cells were grown to confluence in regular culture medium on60 mm tissue culture dishes (Falcon). Following overnight serumstarvation, cells were either stimulated with 50 ng/ml IGF-Ifor 15 minutes or kept in serum-free medium at 37°C untilfixing. Cells were fixed in fresh fixative (1% glutaraldehyde,1% OsO₄ in 0.05M phosphate buffer, pH 6.2) for 45 minutes at4°C (Tilney and Tilney, 1994), washed three times in waterat 4°C to remove phosphate, stained with 1% uranyl acetateovernight in the dark at 4°C, dehydrated in ethanol and2-hydroxypropyl methacrylate and then embedded in an epon substituteLX-112 (Ladd Research Industries Inc, VT). Sections were cutwith a diamond knife and examined with a Philips 200 electronmicroscope (Philips Scientific, Mahwah, NJ). Photographs weretaken of sections mounted on uncoated grids. Images of the scannedphotographs were processed as Adobe Photoshop files for thefigures presented.

Four-dimensional imaging of EGFP- ${alpha}$ -actinin dynamics in live cells
Cells grown in glass-bottomed dishes in D-MEM/F-12 containing15 mM HEPES buffer were placed within a chamber heated at 37°Cmounted on the stage of a Nikon Eclipse TE 300 confocal laser-scanning(Bio-Rad) microscope. Multiple replicate fields of cells wereobserved over 10 minutes in serum-starved cultures or were followedfor 10 minutes in the presence of 50 ng/ml IGF-I. For the IGF-Itime course study, four-dimensional (4D) data sets (sequencesof z-series collected over time) were acquired using the acquisitionfunction of the LaserSharp 2000 (Bio-Rad) software. Digitalconfocal images were captured in real time as a z series (z-step=0.5µm) throughout the thickness of each cell. The 4D serieswas reconstructed into a 3D projection sequence using the LaserSharpprocessing function. Single sections were selected for exportinto Photoshop files for the figures presented.

Time-lapse video microscopy
MCF-7, MCF-7/IGF-IR/WT or MCF-7/IGF-IR/DK cells were platedat low density in DMEM/F-12 in Slideflasks (Nunc, Denmark) andallowed to adhere, spread over and establish cell-cell contacts.Time-lapse video microscopy was carried out in a 37°C environmentalchamber using a Zeiss Axiovert 100 microscope linked by a SonySS-M37OCE CCD camera to a video recorder driven by an EOS BAC 900animation controller. Recordings were made at a rate of 10 framesper minute over a 60-80 minute period for each sample. Eachsample contained between 46 to 102 cells per field, and allconditions were analyzed in three independent experiments. Alterationsin cell motility and shape were measured from traces of thevideo images documenting (a) paths of the cell centroid, whichwere used to calculate cell velocities as movement over time;(b) the changes in cell outline over time, from which the percentageof cells with edge ruffles was calculated; and (c) the appearanceof apical ruffles, which appeared as dynamic phase dark ridgesat the nuclear and perinuclear regions of the apical cell membrane.In experiments involving IGF-I treatment, video recording wasstarted within 1 minute of adding the growth factor. A QuickTime moviewas generated from video records using the Improvision Openlabsoftware package.

Results

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Summary
Introduction
Materials and Methods
Results
Discussion
References

The development of a cell model to study the role of the IGF-IR in motility of human epithelial cells
In the present study, we examined the effects of signaling fromthe IGF-IR kinase on motile behavior of human mammary epithelialcells. For this purpose, we have used parental MCF-7 cells,an MCF-7 cell line overexpressing the wild-type IGF-IR [MCF-7/IGF-IR/WT (Guvakovaand Surmacz, 1997)] and novel clonal lines expressing a kinase-deadform of the IGF-IR (designated MCF-7/IGF-IR/DK). Quantitativewestern blotting was used to compare the level of the IGF-IRin parental MCF-7 cells with clonal lines, which overexpressed eitherthe active or kinase-inactivated IGF-IR. In both transfectedcell lines, the receptor was about 20-fold higher than the endogenouslevel in parental MCF-7 cells (Fig. 1a).

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Fig. 1. IGF-IR expression levels and signaling in MCF-7-derived cell lines. (a) Expression of the IGF-IR was detected in MCF-7, MCF-7/IGF-IR/WT and MCF-7/IGF-IR/DK cells by western blotting of 20 µg of total protein with an antibody against the C-terminus of the IGF-IR ß subunit. The arrows show the position of the ß subunit in the mature receptor (95 kDa) and its precursors: prepro-(190 kDa) and pro-receptor (185 kDa). (b) Top panel: phosphotyrosine blot of MCF-7/IGF-IR/WT and MCF-7/IGF-IR/DK cells stimulated with 50 ng/ml IGF-I. Cell lysates were collected from serum-starved cells before (0 min) and after stimulation with IGF-I for 5, 15 and 60 minutes. Arrows show the position of the IGF-IR ß subunit (95 kDa) and IRS-1 (175 kDa). Protein molecular weight markers are indicated in kDa on the left of the blot. Lower panel: quantification of sample loading by western blot for the IGF-IR.

To compare receptor signaling over time in transfected cells, phosphorylationof the IGF-IR and IRS-1 was examined in the wild-type and kinase-deadtransfectants treated with IGF-I. Cells expressing the wild-type IGF-IRhad higher tyrosine phosphorylation of both the IGF-IRßsubunit and IRS-1 between 5 and 60 minutes following IGF-I treatment.By contrast, MCF-7/IGF-IR/DK cells showed a complete lack oftyrosine phosphorylation of either the IGF-IRß subunitor IRS-1 (Fig. 1b). These data establish that IGF-IR signalingis blocked in MCF-7/IGF-IR/DK cells at the first step of receptorkinase activation and IRS-1 phosphorylation.

The requirement for the IGF-IR kinase in the disorganization of the epithelial sheet
We next compared migratory behavior of the parental MCF-7 cellline and its derivative clones in response to IGF-I. Parentalcells treated with IGF-I became migratory and pulled apart fromone another at cell-cell contacts within colonies. Cell surfaceschanged markedly, exhibiting intensive membrane ruffling overthe apex and at the cell margins. When clones were treated with IGF-I,MCF-7/IGF-IR/WT but not MCF-7/IGF-IR/DK cells developed protrusions, separatedfrom one another and became motile in the direction of intense peripheralruffling. The MCF-7/IGF-IR/WT cells initially located at theedges of colonies became most motile; these cells detached completelyfrom neighboring cells and migrated freely as single cells untilthey came into contact with other cells (Movie 1; availableat jcs.biologists.org/supplemental).

To estimate the differences in cell migratory behavior in responseto IGF-I, we compared ruffling activity and cell movement ratesin MCF-7/IGF-IR/WT and MCF-7/IGF-IR/DK cells. Before stimulation,small zones of minor membrane ruffles at the free edges of cellswere observed occasionally in both cell types, but apical membraneactivity was undetectable. Stimulation with IGF-I resulted ina dramatic increase in the membrane ruffling of MCF-7/IGF-IR/WTover the period of 1 hour and that correlated temporally with cell-cellseparation (Fig. 2A). 100% of IGF-I-stimulated MCF-7/IGF-IR/WTcells developed prominent apical membrane activity, and thepercentage of cells with peripheral, phase dark ruffling activitydoubled (Fig. 2Ba-c). The rates of cell motility were relatedto the initial position of cells within colonies and variedbetween 20.7±2.4 µm/hour (mean±s.e.m.) forcells located inside the colonies and 59.7±7.6 µm/hour(mean±s.e.m.) for cells at the periphery of colonies.

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Fig. 2. (A) IGF-I induces membrane ruffling in separating MCF-7/IGF-IR/WT cells. Phase-contrast images of serum-starved MCF-7/IGF-IR/WT cells before and after stimulation with 50 ng/ml IGF-I for indicated times. The thin arrows show examples of apical ruffles. Thick arrows indicate nascent gaps at the sites of cell-cell detachment. Bar, 10 µm. (B) Inhibition of membrane ruffling and cell motility in dead-kinase expressing cells. Phase-contrast images of MCF-7/IGF-IR/WT (a,b) and MCF-7/IGF-IR/DK (d,e) cells. Cells were serum-starved (a,d) or stimulated with 50 ng/ml IGF-I for 60 minutes (b,e). Examples of sporadic lateral ruffles in serum-starved cells are indicated by arrows in a and d. As MCF-7/IGF-IR/WT cells moved apart, they extended long, fine cytoplasmic processes with the lamellipodia at the ends (arrows in b). Bar, 10 µm. (c,f) Quantification of cells with ruffles at free edges and over the cell apex, and migratory cells observed during time-lapse filming in MCF-7/IGF-IR/WT (c) and MCF-7/IGF-IR/DK (f) cells. Cells were incubated overnight in serum-free medium (SFM) and then stimulated with 50 ng/ml IGF-I (IGF-I).

In sharp contrast, MCF-7/IGF-IR/DK cells showed no increasein cortical ruffling upon IGF-I stimulation, and less than 20%of MCF-7/IGF-IR/DK cells developed apical membrane protrusions(Fig. 2Bd-f). Furthermore, only 17% of the cells showed anymotile activity with mean velocities 3.8±1.6 µm/hourinside the colonies and 13.9±1.9 µm/hour at thecolony margins. These results established that in MCF-7 cellsIGF-IR tyrosine kinase activity was essential for the formationof apical membrane projections, the increase of lateral rufflingand separation of cells followed by migration.

The IGF-IR kinase regulates concomitant reorganization of ${alpha}$ -actinin and F-actin at cell-cell contacts
In MCF-7 cells, the activation of the IGF-IR causes reorganizationof the actin cytoskeleton (Guvakova and Surmacz, 1999). Here,we used indirect immunofluoresence to assess whether in separatingcells reorganization of F-actin in cell-cell contacts is coupled tothe distribution of ${alpha}$ -catenin and ${alpha}$ -actinin, two principle actin-bindingproteins that connect microfilaments to adherens junction receptorcomplexes. In serum-starved MCF-7/IGF-IR/WT cells, ${alpha}$ -catenin and ${alpha}$ -actinin formed continuous lines along the borders of mature cell-cellcontacts, where F-actin was also localized extensively (Fig. 3Aa,e,i).Within 5 minutes of IGF-I stimulation, about 30-35%of cells had punctuated instead of continuous distribution of ${alpha}$ -catenin, which indicated the onset of the disruption of adherensjunctions. By contrast, ${alpha}$ -actinin appeared highly concentratedat cell margins, and the short actin-enriched projections appearedat cell-cell contacts (Fig. 3Ab,f,j). The formation of the cortical ${alpha}$ -actinin and F-actin structures correlated temporally with theloosening of cell-cell contacts and membrane ruffling documentedby time-lapse video microscopy. By 15 minutes, the majorityof the cells (up to 85%) had discontinuous ${alpha}$ -catenin stainingat cell-cell borders. In sharp contrast, ${alpha}$ -actinin and F-actincontinue to highly concentrate within marginal membrane protrusions(Fig. 3Ac,g,k). At 60 minutes, ${alpha}$ -catenin localized diffuselyin the cytoplasm and in the rare remaining cell-cell contacts,whereas ${alpha}$ -actinin and F-actin concentrated at the edges of multiplemembrane protrusions (Fig. 3Ad,h,l). These findings indicatedthat IGF-I-induced separation of MCF-7 cells was associatedwith the progressive reduction of ${alpha}$ -catenin and the increase of ${alpha}$ -actinin and F-actin at cell-cell contacts.

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Fig. 3. (A) The effects of IGF-IR activation on redistribution of ${alpha}$ -catenin, ${alpha}$ -actinin and F-actin. Serum-starved (0 min) MCF-7/IGF-IR/WT cells were treated with 50 ng/ml IGF-I for 5, 15 and 60 minutes, then fixed in 3.7% formaldehyde and stained with a polyclonal antibody to ${alpha}$ -catenin (a-d), a monoclonal antibody to ${alpha}$ -actinin (e-h) or TRITC-phalloidin for F-actin (i-l). Arrows show examples of ${alpha}$ -catenin disappearance from cell-cell contacts (a-c), relocalization of ${alpha}$ -actinin to the cellular borders (e-h) and reorganization of F-actin and microspike development (i-l) induced by IGF-I. Inset in e, examples of ${alpha}$ -actinin localized at the tips of stress fibers seen at the free edge of the spread cell. Bar, 10 µm. (B) IGF-I-stimulated reorganization of ${alpha}$ -actinin and F-actin is blocked when the IGF-IR kinase is inactive. Localization of ${alpha}$ -actinin (staining with antibody to ${alpha}$ -actinin) (a-c) and F-actin (staining with TRITC-phalloidin) (d-f) was examined in MCF-7/IGF-IR/DK cells that were serum starved (0 min) and exposed to 50 ng/ml IGF-I for 5 and 60 minutes. Confocal images are representative of three experiments. Bar, 10 µm.

The reduction of ${alpha}$ -catenin in cell-cell contacts can be achieved experimentallyby lowering the concentration of extracellular calcium ions. Thisprocess is thought to be associated with unclustering and/or internalizationof Ecadherin-catenin complexes (Kusumi et al., 1999). When confluentMCF-7/IGF-IR/WT cells were shifted to PBS containing 0.5 mMEDTA or PBS free of calcium, ${alpha}$ -catenin quickly translocated fromcell-cell contacts to the cytoplasm before dissociation of thecells. This procedure, however, did not stimulate the assemblyof cortical structures containing ${alpha}$ -actinin and F-actin or cellmotility (data not shown). We propose that IGF-IR-mediated reorganizationof the actin cytoskeleton at cell-cell contacts is specificfor the process of `active cell separation' followed by migration asopposed to experimentally induced `passive cell dissociation'unrelated to cell movement.

To determine the role of the IGF-IR kinase activity in activecell separation, we analyzed the effect of IGF-I on localizationof ${alpha}$ -actinin and F-actin in MCF-7/IGF-IR/DK cells, in which thedominant-negative receptor no longer activated IGF-IR signaling.In these cells, IGF-I treatment did not alter localization ofeither ${alpha}$ -actinin or F-actin over a 60 minute period (Fig. 3B).The cells continued to have apico-basal polarity and to be organizedin tight patches. Thus, in MCF-7 cells, both disorganizationof cell-cell contacts and the concomitant concentration of ${alpha}$ -actininand F-actin at cell peripheries are dependent on the catalyticactivity of the IGF-IR kinase.

IGF-I activates colocalization of ${alpha}$ -actinin with highly ordered actin microspikes
To examine in detail the sites of ${alpha}$ -actinin and F-actin colocalizationbefore and after IGF-I stimulation, we used double immunofluorescencestaining (Fig. 4A). In serum-starved MCF-7/IGF-IR/WT cells, ${alpha}$ -actinin co-distributed with F-actin in a circumferential band,small cytoplasmic aggregates and the tips of the stress fiber-likefilaments (Fig. 4Ac). Within 5 minutes of IGF-I stimulation,F-actin appeared to be depleted from the cytoplasm and was insteadconcentrated in short ( $~$ 2 µm) bundles that form highlyordered arrays of spikes at cell peripheries (Fig. 4Ad). Atthe same time, ${alpha}$ -actinin showed a striking enhancement in itscolocalization with F-actin at the basal portions of actin bundleswithin microspikes. Notably, there was no ${alpha}$ -actinin in the extremitiesof microspikes where F-actin persisted in the tight bundles (Fig. 4Af).These experiments revealed that IGF-I activates localizationof ${alpha}$ -actinin at the base of actin microspikes organized in wellordered arrays in lateral zones of separating cells.

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Fig. 4. (A) Colocalization of ${alpha}$ -actinin with F-actin in microspikes during IGF-I-induced cell separation. MCF-7/IGF-IR/WT cells, untreated (a-c) or stimulated with 50 ng/ml IGF-I for 5 minutes (d-f), were fixed in 3.7% formaldehyde and co-stained for F-actin with TRITC-phalloidin and for ${alpha}$ -actinin with a monoclonal antibody to ${alpha}$ -actinin. The images of middle sections acquired by confocal laser-scanning microscopy illustrate staining for F-actin in red (a,d) and ${alpha}$ -actinin in green (b,e). In overlays (c,f), sites of ${alpha}$ -actinin and F-actin colocalization appear in yellow. Insets in d-f: examples of F-actin and ${alpha}$ -actinin-containing microspikes from the zone of the intercellular membrane ruffles pointed to by arrow (d-f). Bar, 10 µm. (B) Ultra-structural analysis of IGF-I-induced microspikes in MCF-7/IGF-IR/WT cells. (a) Examples of adherens junction (aj), desmosome (d) and intermediate filaments (if) proximate to desmosomes are indicated in confluent serum-starved cells. The longitudinal section of continuous contacts between lateral membranes is shown in the upper inset. (b) Cross-sections through microspikes (MS) formed in the cells stimulated with 50 ng/ml IGF-I for 15 minutes. Individual bundles of actin in the core of MS formed by opposing cells are pointed out by a row of arrows; gaps between single microspikes are labeled with asterisks. A membrane site resembling an immature or disassembling desmosome in close proximity to intermediate filaments is labeled d. In the inset, the horizontal section through apical zones of IGF-I-stimulated cells is shown. N, nucleus. Bar, 250 nm. In insets, bar, 5 µm.

To examine more deeply the structure of microspikes in the separating cells,we repeated the IGF-I stimulation experiments, this time processing cellsfor transmission electron microscropy (TEM). Confluent serum-starved cellshad intercellular contacts typical of polarized epithelium (Fig. 4Ba).Within 15 minutes of IGF-I stimulation, finger-like projectionsformed in the lateral zones of the opposing cells (Fig. 4Bb). Thatcorrelated temporally with appearance of ${alpha}$ -actinin-actin microspikesidentified by immunofluorescence. The average diameter of the membrane-flankedindividual projection was 0.24±0.03 µm (mean±s.e.m.),the lengths of projections measured from tip to base variedfrom 0.27 µm to 1.21 µm. The shorter projectionswere in close contact with each other, whereas the elongatedones were separated by gaps. Clearly, the core of each projectionconsisted of a strap of bundled actin oriented perpendicularlyto the cell-cell contact zones. Actin bundles traversed projections,extended through the cell body and embedded in the actin meshwork,which coincided well with positioning of the cortical cytoskeletonrelatively to the apical membrane and cell nucleus. The average lengthof the individual actin strap was 1.94±0.15 µm (mean±s.e.m.).That agreed well with the estimated lengths of actin bundlesvisualized by immunofluorescence. Thus, the ultra-structuralanalysis confirmed that lateral projections induced by IGF-Iin separating cells are actin-enriched microspikes.

In living cells ${alpha}$ -actinin microspikes appear as motile apico-lateral structures
To study the dynamics of ${alpha}$ -actinin in living cells, we took advantage ofconfocal laser-scanning microscopy and examined the spatialand temporal effects of IGF-I on full-length ${alpha}$ -actinin taggedwith EGFP. The interior details from multiple focal planes wererecorded as they changed over time (4D imaging). For thoroughanalysis of ${alpha}$ -actinin localization, the representative sectionsare shown in Fig. 5.

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Fig. 5. (A) The development of ${alpha}$ -actinin motile projections in living MCF-7/IGF-IR/WT cells stimulated with IGF-I. Dynamics of EGFP- ${alpha}$ -actinin in live MCF-7/IGF-IR/WT cells transiently transfected with WT ${alpha}$ -actinin-EGFP encoding plasmid. (A-C) The representative laser confocal fluorescence images taken at the apical, middle and basal focal planes in serum-starved cells (a,d,g) stimulated with 50 ng/ml IGF-I for 5 minutes (b,e,h) or for 9 minutes (c,f,i) are shown. Circled is an example of a cell that is flattening, separating and moving from the adjacent cells in response to IGF-I treatment. The optical section from the apical region was taken about 2.0 µm from the top of cells. The example of the lateral single projection that extended and folded over the cell apex is indicated by arrow in a-c. The middle optical sections were collected from the focal plane about 6.5 µm from the top of cells. Basal images were taken close to the substratum level (about 1.5 µm from the glass surface). Bar, 10 µm.

(B) Reorganization of ${alpha}$ -actinin is blocked in living MCF-7/IGF-IR/DK cells treated with IGF-I. The images illustrate the localization of ${alpha}$ -actinin in live MCF-7/IGF-IR/DK cells transfected with EGFP-labeled ${alpha}$ -actinin before (0 min) and after IGF-I stimulation (shown for 1 and 5 minutes). The representative images derived by 3D projection of 20 consecutive apical and middle optical sections are shown. Bar, 10 µm.

Typically, without IGF-I treatment, ${alpha}$ -actinin lined the bordersof the adjacent MCF-7/IGF-IR/WT cells. The thin band of ${alpha}$ -actininappeared close to the lateral cell membranes in the most apicaloptical section and through the cell thickness of 10-12 µm. ${alpha}$ -actinin was also localized within small aggregates scatteredthroughout the cytoplasm and in the fine dotted or streak-likefocal structures about 2.5 µm above the substrate surface(Fig. 5Aa,d,g). Once cells were stimulated with IGF-I, the aggregatesof ${alpha}$ -actinin cleared off the cytoplasm and an increased amountof ${alpha}$ -actinin became associated with cell boundaries where thenascent projections were formed. Within a few minutes, the propellingmicrovilli-like projections containing ${alpha}$ -actinin extended andretracted laterally and upward; the most elongated projections (of6-10 µm in length) bent across the cell apex (Fig. 5Ab,c).The short (of 2-4 µm in length) ${alpha}$ -actinin projections werealso seen through a series of the middle optical sections spanning10 µm in height (Fig. 5Ae,f). Within 5 minutes, some cellsvanished from view in the most apical sections and then fromthe series of lateral sections (compare circled areas in Fig. 5Aa with b,d and e).In the same cells, ${alpha}$ -actinin motile rufflesformed along the boundaries of the basal membrane. These basalruffles resembled growth-factor-induced ruffles described inKB cells (Kadowaki et al., 1986). In parallel, the initiallyminute ${alpha}$ -actinin-containing focal structures enlarged and orientedin the direction of cell spreading (Fig. 5Ag-i, circled). By9 minutes of IGF-I stimulation, these focal structures appearedcloser to the substratum than they were in the untreated cells(1.5 µm compared with 2.5 µm from the substratelevel). Thus, we found that in separating living cells, ${alpha}$ -actininis localized in the dynamic apico-lateral microspikes besidesfocal adhesions and the edges of the basal ruffles.

In MCF-7/IGF-IR/DK cells, despite the continuous treatment withIGF-I, ${alpha}$ -actinin remained predominantly localized to lateralmembranes of cells tightly adhered to each other. Only minortime-dependent redistribution of ${alpha}$ -actinin occurred in the cytoplasmand at the cell borders (Fig. 5B); these changes were typicalof all live MCF-7-derived cells regardless of IGF-I stimulation.Taken together these observations clearly show that activationof the IGF-IR causes a time-dependent accumulation of ${alpha}$ -actinin-EGFPin the apico-lateral microspikes of separating cells.

The development of ${alpha}$ -actinin mutants for molecular genetic analysis of the requirements for ${alpha}$ -actinin in microspikes
In the ${alpha}$ -actinin molecule, the N-terminal head contains highly conservativeactin- and phospholipid-binding sites, the central rod domainis composed of four spectrin-like repeats implicated in dimerizationof ${alpha}$ -actinin monomers and interaction with other proteins andthe C-terminal end of the rod provides binding sites for ionsof calcium as well as proteins (Hemmings et al., 1992; Matsudaira, 1994;McGregor et al., 1994; Fukami et al., 1996). The characterizationof ${alpha}$ -actinin mutants has been particularly difficult in non-musclecells owing to the rapid lethality of cells expressing the mutantproteins (Scultheiss et al., 1992; Hijikata et al., 1997). To definethe contribution of individual domains to the function of ${alpha}$ -actininin microspikes, we have constructed new pEGFP N1-vector-based plasmidsencoding the mutant ${alpha}$ -actinins as C-terminal chimeras with EGFP (Fig. 6A),and that allowed us to monitor fusion proteins soon aftertransfection. 230 amino-acid residues in the N-terminus weredeleted to yield a mutant ${alpha}$ -actinin lacking the entire actin-bindingregion ( ${Delta}$ N). To inactivate ${alpha}$ -actinin in the C-terminus ( ${Delta}$ C), thelast 168 amino acids were removed (described in the Materialsand Methods).

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Fig. 6. (A) Schematic diagram of ${alpha}$ -actinin-EGFP fusion monomers. The WT, ${Delta}$ N and ${Delta}$ C ${alpha}$ -actinins are expressed as C-terminal chimeras with EGFP. The primary sequence of the WT ${alpha}$ -actinin consists of the N-terminal conservative actin-binding region (residues 1-245), a central domain of four spectrin-like repeats implicated in dimerization of ${alpha}$ -actinin and interaction with other proteins including ${alpha}$ -catenin (residues 246-712), and the C-terminal domain containing the vinculin-binding site (residues 713-749) and the two EF-hand binding Ca²⁺ motifs (residues 770-817). Numbering of residues includes the initiating methionine. (B) Expression levels of ${alpha}$ -actinin-EGFP fusion proteins in MCF-7/IGF-IR/WT cells. Expression of EGFP was detected in transiently transfected MCF-7/IGF-IR/WT cells by western blotting of 20 µg of total protein with an antibody against GFP. Upper panels, the representative western blot shows the levels of exogenous EGFP (27 kDa) and ${alpha}$ -actinin-EGFP chimeras (WT, 130 kDa, ${Delta}$ N, 104 kDa, ${Delta}$ C, 109 kDa) expressed as transgenes 48 hours after transfection (asterisks indicate the position of chimera). Lower panel, the same blot was stripped and re-probed with an antibody against ${alpha}$ -actinin to detect endogenous (100 kDa) and exogenous EGFP- ${alpha}$ -actinins whose positions on the blot are indicated by asterisks. Note that the endogenous ${alpha}$ -actinin and ${Delta}$ N ${alpha}$ -actinin-EGFP overrun in a 100 kDa band. (C) Intracellular localization of WT, ${Delta}$ N, ${Delta}$ C ${alpha}$ -actinin-EGFP fusion proteins in serum-starved and IGF-I-stimulated MCF-7/IGF-IR/WT cells. MCF-7/IGF-IR WT cells were transfected with plasmid encoding WT or ${Delta}$ N or ${Delta}$ C ${alpha}$ -actinin-EGFP. 24 hours after transfection, serum-starved cells were either fixed in 3.7% formaldehyde (a-c) or stimulated with 50 ng/ml IGF-I for 15 minutes and then fixed (d-f). The representative images of the middle optical sections acquired by confocal laser-scanning microscopy show (top panel, a-c) the WT and ${Delta}$ C ${alpha}$ -actinins incorporated into the mature cell-cell junctions (pointed by arrow) and ${Delta}$ N ${alpha}$ -actinin stained in the cytoplasm and nucleus. Lower panel, d-f: the images show the formation of ${alpha}$ -actinin-EGFP-containing spikes (arrows in d); diffuse staining for ${Delta}$ N ${alpha}$ -actinin-EGFP (e), aggregation of ${Delta}$ C ${alpha}$ -actinin-EGFP and formation of the defective microspikes (f). Bar, 10 µm.

MCF-7/IGF-IR/WT cells were transfected with plasmid DNA encodingeither control EGFP or EGFP chimeras with a full-length wild-type(WT), mutant ${Delta}$ N and ${Delta}$ C ${alpha}$ -actinin. Cell extracts were resolved electrophoretically,and proteins transferred on the membrane were probed sequentiallywith antibody to GFP and ${alpha}$ -actinin. Western immunoblotting hasconfirmed protein expression and the expected molecular weightsof exogenous EGFP (27 kDa), WT (127 kDa), ${Delta}$ N (104 kDa) and ${Delta}$ C(109 kDa) EGFP- ${alpha}$ -actinins (Fig. 6B).

Both head and tail domains of a-actinin are required for the development of highly ordered microspikes
To visualize the dynamics of ${alpha}$ -actinin-EGFP fusion proteins specific tothe regions of cell-cell contacts, we used confocal laser-scanning microscopyand collected stacks of images from the middle optical sections crossingnuclei. In serum-starved cells with mature cell-cell contacts,only the wild-type and ${Delta}$ C ${alpha}$ -actinins incorporated into pre-existing cell-celljunctions. Unlike the wild-type and ${Delta}$ C ${alpha}$ -actinin, ${Delta}$ N ${alpha}$ -actinin didnot associate with the circumferential actin ring and was insteadlocalized diffusely throughout the cell body (Fig. 6Ca-c).

In WT ${alpha}$ -actinin transfectants, IGF-I triggered the expected reorganizationof cell-cell contacts and the assembly of ${alpha}$ -actinin-actin microspikesin the lateral zones (Fig. 6Cd). ${Delta}$ N ${alpha}$ -actinin did not colocalizewith actin microspikes and remained diffused throughout thecell body (Fig. 6Ce). The number of ${Delta}$ C ${alpha}$ -actinin-transfected cellswith ${alpha}$ -actinin-actin spikes was half that of wild-type transfectants.Moreover, the spatial relationship between ${Delta}$ C ${alpha}$ -actinin and F-actinwas disturbed, as microspikes did not organize into well orderedarrays (Fig. 6Cf). In two independent experiments, the appearanceof microspikes was assessed quantitatively (Table 1). Collectively,these results demonstrate that in the ${alpha}$ -actinin molecule boththe head and tail regions are required for the function of microspikes.The N-terminal part of ${alpha}$ -actinin is necessary for associationof ${alpha}$ -actinin with actin bundles, whereas the C-terminal tailof the rod is needed for correct assembly and/or positioningof microspikes at cell peripheries.

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Table 1. Effects of ${alpha}$ -actinin mutants on microspikes

The mechanism of active cell separation and microspike assembly requires activities of PI 3-kinase-generated phospholipids
To address the role of IGF-IR kinase signaling in regulatingmicrospike assembly in relation to cell separation, we usedfour specific pharmacological inhibitors of PI 3-kinase andMAP kinase signaling pathways (Fig. 7). They are LY 294002,a specific inhibitor of the catalytic subunit of the PI 3-kinase;a D3-modified phosphatidylinositol (PI) ether lipid analog (alsocalled Akt inhibitor); PD 98059, a synthetic inhibitor of theMAP kinase-activating enzyme, MAPK/ERK kinase (MEK1); and UO126, an inhibitor of MEK1 and MEK2. In MCF-7/IGF-IR/WT cellstreated with LY 294002, the normal induction of phosphorylationof the PKB/Akt by putative PDK2 on serine 473 was downregulatedby 90% and 84% and by 3-phosphoinositide-dependent kinase 1(PDK1) on threonine 308 by 28% and 20%, and at 5 and 15 minutes,respectively. The 3D-modified PI-analog also downregulated signalingassociated with the activities of PI 3-kinase-generated phospholipids,although its effect on phosphorylation of PKB/Akt was much less.The relative phosphorylation of PKB/Akt on serine 437 was reducedby 8% and 19%, and on threonine 308 by 9% and 11% at 5 and 15 minutesof IGF-I stimulation (average of five experiments) (Fig. 7a).PD 98059 reduced the relative phosphorylation of ERK1/2 MAPkinases on threonine 202 and tyrosine 204 by 73% and 67% at5 and 15 minutes of IGF-I treatment (average of four experiments).UO 126 was a much more potent inhibitor of ERK1/2 MAPK kinases; itblocked completely IGF-I-stimulated and basal phosphorylationof these kinases (Fig. 7b and data not shown).

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Fig. 7. Effects of inhibitors on IGF-I-induced activation of the PI 3-kinase and MAP kinase signaling pathways. (a) Serum-starved cells (0). Cells not exposed to inhibitors (IGF-I) and pre-treated with 10 µM LY 294002 for 30 minutes (LY+IGF-I) or 40 µM PI analog for 3 hours (PI analog+IGF-I) were stimulated with 50 ng/ml IGF-I for the indicated times. Phosphorylation of PKB/Akt was detected with an antibody against phospho-Akt. For a loading control, the same blots were stripped and re-probed with an antibody against Akt (Materials and Methods). One of the re-probed blots is shown. (b). Serum-starved cells (0). Cells not exposed to inhibitors (IGF-I) and pre-treated with 50 µM PD 98059 (PD+IGF-I) or 50 µM UO 126 (UO+IGF-I) for 30 minutes were stimulated with 50 ng/ml IGF-I for the indicated times. The ERK1/2 MAPK phosphorylation was detected with specific phospho-MAPK antibodies. The same blot was stripped and re-probed with antibody against total ERK1/ERK2 (p44/p42) (Materials and Methods).

Pretreatment of MCF-7/IGF-IR/WT cells with 10 µM LY294002and 40 µM PI analog before the addition of 50 ng/ml IGF-Iblocked the formation of cortical microspikes and cell separationin response to IGF-I [compare Fig. 8A,b with c,d also with Guvakovaet al. (Guvakova et al., 2002)]. LY 294002- and PI-analog-pretreatedcells remained organized in tight colonies during at least 60and 30 minutes of the IGF-I treatment, respectively. By contrast,there was no apparent inhibitory effect of 50 µM PD 98059on cell separation; cells, exposed to this drug or not, appearedspindle-shaped, separated from each other and migrated within60 minutes of IGF-I stimulation. The formation of well ordered ${alpha}$ -actinin-actinmicrospikes was slightly disturbed by PD 98059 (compare Fig. 8A,b with e).The more potent inhibitor of MEK1 and MEK2, UO126, did not prevent IGF-stimulated concentration of ${alpha}$ -actininand actin in the peripheral microspikes (Fig. 8Af); however,it inhibited cell migration radically within first 60 minutesof IGF-I stimulation (data not shown).

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Fig. 8. A. The development of ${alpha}$ -actinin/actin microspikes by IGF-I is blocked by the inhibitors of PI-3 kinase signaling. MCF-7/IGF-IR/WT cells were serum-starved (a), serum-starved and then stimulated with 50 ng/ml IGF-I for 15 minutes (b), pretreated for 30 minutes with 10 µM LY 294002 (c), for 3 hours with 40 µM D3-PI analog (d), 30 minutes with 50 µM PD 98059 (e) or 30 minutes with 50 µM UO 126 (f) and then stimulated with 50 ng/ml IGF-I for 15 minutes. (a-f) Overlays of confocal images of cells stained with TRITC-phalloidin (red) and antibody against ${alpha}$ -actinin (green). Examples of actin/ ${alpha}$ -actinin microspikes are indicated by arrows. Images are representative of three experiments. Bar, 10 µm. (B) Differential effects of the PI analog and UO 126 on IGF-I-stimulated loss of adherens junctions and formation of microspikes. Serum-starved MCF-7/IGF-IR/WT cells were pretreated with 40 µM D3-PI analog for 3 hours, stimulated with 50 ng/ml IGF-I for 15 minutes in the presence of the inhibitor, fixed and stained with antibody to ${alpha}$ -catenin (a) or fascin (c) (Materials and Methods). In parallel, the same serum-starved cells were pretreated with 50 µM UO 126 for 30 minutes, stimulated with 50 ng/ml IGF-I for 15 minutes, then fixed and stained with an antibody to ${alpha}$ -catenin (b) or fascin (d). The relocation of ${alpha}$ -catenin from adherens junctions normally induced by IGF-I (compare with Fig. 3Aa-d) is blocked by the PI analog but not UO 126. Normal stimulation of fascin microspikes by IGF-I (inset in c, 50 ng/ml IGF-I, 15 minutes) is also blocked only by the PI analog. Confocal images are representative of four independent experiments. Bar, 10 µm. (C) The MEK1/2 inhibitor affects function of stress fibers in IGF-I-stimulated cells. Serum-starved cells not exposed to inhibitor (a) or pretreated with 50 µM UO 126 for 30 minutes (b) were stimulated with 50 ng/ml IGF-I for 15 minutes, then fixed and stained with TRITC-phalloidin. IGF-I normally promotes disassembly of stress fibers within 5 minutes followed by their re-assembly typically after 15 minutes. In cells pretreated with the MEK1/2 inhibitor, re-assembly of the prominent stress fibers is markedly inhibited. The representative images of optical sections collected at the basal level of the cells are shown. Bar, 10 µm.

MEK1/2 signaling downstream of the IGF-IR kinase is essential for migration of separated cells
The above findings prompted our suggestion that MEK1/2 signalingis unnecessary for initial steps of cell-cell separation butmay be essential for movement of the cells separated in responseto PI 3-kinase signaling. To test this idea, we compared theeffect of the PI analog and UO 126 on IGF-stimulated reorganizationof cell-cell contacts, this time monitoring distribution of ${alpha}$ -catenin, a molecular marker of adherens junctions, and fascin,a marker of the peripheral actin microspikes. In contrast to ${alpha}$ -actinin,fascin localizes along the length of actin bundles induced by IGF-Iand that allows visualizing microspikes without co-stainingfor F-actin (Guvakova et al., 2002). Pretreatment of cells withthe PI analog blocked IGF-I-stimulated redistribution of ${alpha}$ -cateninand thereby dissolution of adherens junctions. This inhibitoralso blocked the formation of microspikes containing fascin(Fig. 8Ba,c; inset in c, fascin microspikes induced by IGF-I).In sharp contrast, total inhibition of MEK1/2 activity by UO126 did not prevent a loss of ${alpha}$ -catenin from adherens junctionsand did not block the formation of fascin microspikes at cellperipheries (Fig. 8Bb,d). Strikingly, inhibition of MEK1/2 byUO 126 had a marked effect on stress fibers. Normally, activationof the IGF-IR in MCF-7 cells results in a rapid disassemblyof stress fibers followed by re-assembly of microfilaments after 15minutes of IGF-I stimulation. The latter coincides with advancinglong protrusions and moving the cell body [seen in Fig. 3Ai-land described in detail in (Guvakova and Surmacz, 1999)]. Pretreatmentwith UO 126 had no effect on disassembly of stress fibers; however,it prevented their re-assembly as well as the development ofthe long membrane protrusions after 15 minutes of IGF-I stimulation(compare Fig. 8Ca with b).

We conclude that separation of MCF-7 breast cancer cells inresponse to IGF-I is dependent on signaling from the activatedIGF-IR through the PI 3-kinase and its phospholipid products,and that signaling through MEK1/2 may be necessary for subsequentcell locomotion.

Discussion

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Summary
Introduction
Materials and Methods
Results
Discussion
References

The IGF system is essential for normal development of the mammarygland, and its disruption in human breast cancer leads to anexcess of IGF-IR signaling. The biological relevance of theenhanced catalytic activity of the IGF-IR kinase to breast tumorprogression has not been established. In this study, using acombination of molecular genetic, biochemical and pharmacologicalapproaches with a complementary monitoring of living cell behavior,we have identified a novel mechanism by which the IGF-IR kinase inducesseparation and migration of human breast carcinoma cells.

Cell motile responses mediated by the IGF-IR
It has previously been established that polypeptide growth factorsacting through receptor tyrosine kinases can induce transitionof cells from an epithelial to a motile fibroblastic phenotype,a phenomenon that resembles epithelial-mesenchymal transition,which occurs during development (Boyer and Thiery, 1993). IGF-I ismainly known as a mitogenic growth factor, and signaling throughthe IGF-IR in mammary epithelial cells has been chiefly studiedin respect to effects on cell proliferation and apoptosis (reviewedby Lee et al., 1998; Chernicky et al., 2000). Nevertheless,a role for the IGF-IR in motility of breast carcinoma cellshad been proposed more than a decade ago on the basis of theresults of the Boyden chamber assay (Kohn et al., 1990). Itshould be noted, however, that in this assay cells are artificiallyseparated from each other before examination, and it is therefore notpossible to analyze mechanisms of epithelial sheet disintegration.

In this study we examined in detail the effects of IGF-I onmotile behavior of cells within an epithelial sheet. We havenow demonstrated that, like other growth factors with scatteringfunction, IGF-I induced cell motile responses in a biphasicmanner, first causing separation and subsequently causing migrationof the cells. The phase of active separation lasted only for15-30 minutes and was unusually short compared with the 5-16hours reported for HGF/SF, FGF-1 and EGF (Stoker and Perryman,1985; Savagner et al., 1997; Müller et al., 1999). Duringthe separation phase, IGF-I stimulated highly dynamic activityof the entire cellular membrane: formation of apical ruffles andmotile apico-lateral microspikes, dissolution of adherence junctionsand an increase in basal membrane ruffling. Although the precisemechanism of such rapid morphological alterations is unknown,the appearance of dynamic microspikes at the cell-cell contactsand temporal correlation of this event with disintegration theadherens junction complex led us to suggest that microspikesfacilitate cell-cell detachment. In addition to acute cell separation,video tracking has revealed uncommonly fast rates of migrationof single MCF-7/IGF-IR/WT cells. Collectively these data establishfor the first time that activation of the IGF-IR can in theshort-term cause destabilization of cell-cell interactions,leading to quick separation and migration of breast cancer epithelialcells.

IGF-IR-mediated active cell separation: structural reorganizations
EGF modulates the interaction between the adherens junctionreceptor E-cadherin and the actin cytoskeleton, although associatedcytoskeletal reorganizations have not been characterized (Hazanand Norton, 1998). Our previous work has shown that in MCF-7cells, IGF-I induces rapid disassembly of stress fibers andextensive reorganization of the cortical actin (Guvakova andSurmacz, 1999). We have now demonstrated that disassembly ofthe cortical actin belt coincides with mobilization of ${alpha}$ -actininand actin into apicolateral microspikes and displacement of ${alpha}$ -catenin from the adherens junctions. This agreed with the recentreport that activation of the IGF-IR induces redistributionof E-cadherin and ß-catenin from the adherens junctionsinto the cytoplasm (Morali et al., 2001).

What drives ${alpha}$ -actinin into cell-cell contacts? As an actinbinding protein,intact ${alpha}$ -actinin shows a prominent colocalization with filamentousactin. Yet ${alpha}$ -actinin can bind to a number of molecules, in additionto actin (Crawford et al., 1992; Otey et al., 1993; Kroemkeret al., 1994; McGregor et al., 1994; Christerson et al., 1999)that perhaps determine the localization of ${alpha}$ -actinin. For example,in Cos and PtK2 cells, mutated ${alpha}$ -actinins with a deleted actin-bindingsite were not incorporated into stress fibers, although they localizedto ruffled membranes and adherens junctions (Hemmings et al.,1992; Hijikata et al., 1997). The prominent localization of ${alpha}$ -actinin to adherens junction has been related to the directassociation between the central rod domain of ${alpha}$ -actinin and theC-terminus of ${alpha}$ -catenin (Knudsen et al., 1995; Nieset et al.,1997). In epithelial culture, ${alpha}$ -actinin colocalizes with vinculinand the cadherin-catenin complex. In this study, we used GFP-labeled ${alpha}$ -actinin to follow distribution of ${alpha}$ -actinin in living cellsbefore and after IGF-I stimulation. Our results with a GFP-labeledmutant of ${alpha}$ -actinin, in which the ${alpha}$ -catenin-binding site was preservedwhile the actin-binding domain was removed, support the ideathat both ${alpha}$ -catenin and actin-binding sites of ${alpha}$ -actinin are essentialfor localization of this protein into the mature cell-cell junctions.The interaction of the C-terminal end of ${alpha}$ -actinin with vinculindoes not seem to be required because a GFP-tagged ${Delta}$ C ${alpha}$ -actininmutant in which the vinculin-binding site was disrupted didnot interfere with the ability of ${alpha}$ -actinin to localize to intercellularjunctions. The development of microspikes in response to IGF-Irequired at least two fully functional regions of the ${alpha}$ -actininmolecule. As expected, the head of ${alpha}$ -actinin was obligatory forbinding to actin spikes. The C-terminal tail of ${alpha}$ -actinin wasrequired for correct assembly and/or stabilization of microspikesbecause the truncation of this region reduced the number of ${alpha}$ -actinin/actinmicrospikes and caused their misalignment at the cell periphery.According to the previous suggestion, it is possible that the actin-bindingactivity of ${alpha}$ -actinin requires a ternary interaction with theC-tail as modifications in the EF-hand domain of ${alpha}$ -actinin have deleteriouseffects on the activity of its actin-binding domain (Witke etal., 1993; Dubreuil and Wang, 2000). Additionally, direct interactionof ${alpha}$ -actinin with vinculin, which is probably disturbed in the ${Delta}$ C ${alpha}$ -actinin mutant, might be required for correct organizationof microspikes. Thus our findings establish that functional ${alpha}$ -actinin is necessary for the development of microspikes and isnot passively reorganized following actin.

Our results, while supporting previous findings on IGF-I-stimulatedactin polymerization at the cell periphery (Kadowaki et al.,1986; Isumi et al., 1988), further demonstrate that activationof the IGF-IR coordinates reorganization of actin into peripheralmicrospikes. Localization of ${alpha}$ -actinin at the base rather thanat the tips of microspikes implies that other actin-crosslinking protein(s)compose the core of a spike. A good candidate for this roleis the 55 kDa actin-bundling protein fascin, which acts as acrosslinker, causing aggregation of actin into tight bundles (Edwardsand Bryan, 1995; Kureishy et al., 2002). In vitro, fascin and ${alpha}$ -actinin synergistically affect mechanical properties of actinfilaments (Tseng et al., 2001). In vivo, fascin plays a rolein extending the membrane during cell spreading and migration,and overexpression of fascin in pig epithelial cells causedthe disorganization of cell-cell contacts (Yamashiro et al.,1998). Fascin also acts as a negative regulator of cell-cellinteractions in rat mammary epithelial cells (Wong et al., 1999).Activation of the IGF-IR in MCF-7 cells induces rapid relocalizationof fascin from the cytoplasm to the peripheral actin microspikes(Guvakova et al., 2002). We reason now that the activated IGF-IRinduces cortical actin dynamics beneath the plasma membraneby increasing actin polymerization and promoting crosslinkingof actin by fascin to stabilize the cores of microspikes andby ${alpha}$ -actinin to properly position these nascent projections atthe cell periphery. Although the significance of microspikesin cell-cell separation remains hypothetical, one possibilityis that microspikes play an active cytomechanical role in thedestabilization of interactions between opposing cells. Alternatively,microspikes may be the form of cell-cell contacts that are transientand more flexible than adherens junctions and therefore providethe intermediate strength of adhesion between separating cells.

IGF-IR-regulated cell motility: signaling pathways
Cell-cell detachment and microspike formation was completelyblocked in MCF-7/IGF-IR/DK cells, clearly indicating the directcausative relationship between IGF-IR activation and ${alpha}$ -actininredistribution. Although it is conceivable that IGF-IR signalingaffects the phosphorylation status of ${alpha}$ -actinin, at least twolines of evidence imply that tyrosine phosphorylation of ${alpha}$ -actininis not relevant to the development of microspikes in MCF-7 cells.First, there was no detectable difference in the tyrosine phosphorylationof ${alpha}$ -actinin immunoprecipitated from cells stimulated with IGF-I(see Materials and Methods). Second, the WT ${alpha}$ -actinin-EGFP chimera,which lacked the only identified phopshotyrosine residue 12within the amino-acid motif QTNDY (Izaguirre et al., 2001),was nevertheless functionally active and localized to microspikes.

As relocalization of ${alpha}$ -actinin into cortical structures was detected after1-2 minutes of IGF-I stimulation, we predicted that the earlysignaling triggered by the ligand-receptor interaction promotesthe development of microspikes. In MCF-7 cells, activation ofthe IGF-IR kinase quickly drives the formation of a complexbetween the receptor and substrates IRS and Shc that bringsabout activation of the downstream cascades of serine/threonine kinasesand the PI 3-kinase. Interestingly, in different epithelialcells, different kinases play roles in cell motility. In MDCKcanine epithelial cells, activation of both the PI 3-kinaseand MAP kinase was found to be essential for the motile responseto HGF/SF (Royal and Park, 1995; Potempa and Ridley, 1998).The function of MAP kinases was delineated in scattering triggeredby HGF/SF in HT29 colon carcinoma cells and haptotaxis in FGcarcinoma cells and T47D breast carcinoma cells (Klemke et al., 1997;Herrera, 1998; Spencer et al., 2000), whereas pretreatment withthe MEK1 inhibitor, PD 98059, was dispensable for the chemotacticresponse of MCF-7 cells to IGF-I (Manes et al., 1999). Others havereported that IGF-I stimulates colonic epithelial cell migrationin a wound healing assay through multiple signaling pathwaysincluding PI 3-kinase, MAP kinases and PKC- ${gamma}$ and - ${delta}$ (Andre etal., 1999). In MCF-7 cells expressing the dominant-negativereceptors, activity of the PI-3 and

Research Article

Functional role of -actinin, PI 3-kinase and MEK1/2 in insulin-like growth factor I receptor kinase regulated motility of human breast carcinoma cells

Functional role of ${alpha}$ -actinin, PI 3-kinase and MEK1/2 in insulin-like growth factor I receptor kinase regulated motility of human breast carcinoma cells