1 Cell Biology, Zoological Institute, Technical University of Braunschweig, 38106 Braunschweig, Germany
2 Cell Biology, German Research Centre for Biotechnology (GBF), 38124 Braunschweig, Germany
3 The Randall Division, King's College London, London SE1 1UL, UK
4 Institute of Immunology, Witten/Herdecke University, 58448, Witten, Germany
Author for correspondence (e-mail: wolfgang.ziegler{at}medizin.uni-leipzig.de)
Accepted 18 January 2005
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Summary |
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Key words: Cell-matrix adhesion, Cell motility, Microfilaments, Phosphatidylinositol-4,5-bisphosphate, Vinculin
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Introduction |
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Vinculin activation requires release of an intramolecular head-to-tail interaction. This intramolecular bond blocks the association of the free, not the membrane-associated, form of vinculin with most of its protein ligands (Critchley, 2000). The recently solved structure of vinculin suggests that binding sites for vinculin ligands are structurally distinct but conformationally linked, and activation of vinculin ligand binding requires the simultaneous binding of several ligands (Bakolitsa et al., 2004
; Borgon et al., 2004
). In vitro, the intramolecular bond can be released by charging either the vinculin head (Vh) with appropriate talin peptides (Bass et al., 2002
; Izard et al., 2004
) or the vinculin tail (Vt) with acidic phospholipids such as phosphatidylinositol-4,5-bisphosphate (PIP2) (Hüttelmaier et al., 1998
; Weekes et al., 1996
). Binding of PIP2 to vinculin was suggested to promote adhesion-site targeting of vinculin (Gilmore and Burridge, 1996
), and biochemical evidence argues strongly for a competition between acidic-phospholipid and actin-filament binding to the vinculin tail (Steimle et al., 1999
).
PIP2 acts as a central regulator of actin dynamics and adhesion-site turnover (Nayal et al., 2004; Yin and Janmey, 2003
), and many cytoskeletal proteins involved in cell adhesion bind to PIP2 (Sechi and Wehland, 2000
). Both activation and integrin binding of talin are dependent on the local availability of PIP2 (Martel et al., 2001
). Elevated local concentrations of PIP2 can be a consequence of either release from proteins sequestering acidic phospholipids or generation by lipid kinases (Caroni, 2001
; Doughman et al., 2003
). Type I
661 phosphatidylinositol-4-phosphate 5-kinase (PIP 5-kinase), a lipid kinase that can raise local PIP2 levels by phosphorylating the ubiquitous precursor molecule phosphatidylinositol 4-phosphate, is recruited to talin in nascent adhesions and triggers adhesion site growth (DiPaolo et al., 2002
; Ling et al., 2002
). Conversely, strong overexpression of the same kinase leads to breakdown of adhesion sites as a consequence of imbalanced local PIP2 levels (Ling et al., 2002
).
To elucidate the significance of acidic phospholipid binding to vinculin for its intracellular localization, its influence on adhesion-site dynamics and cell motility, we have mutated one or both lipid-binding sites in vinculin while leaving its actin-binding ability largely intact. Expression of full-length vinculin variants in B16-F1 mouse melanoma cells revealed that the targeting and velocity of incorporation of these mutants into adhesion sites were not affected. By contrast, adhesion-site turnover was grossly slowed down in cells expressing a vinculin mutant defective in both lipid-binding sites, associated with a delay in cell spreading and locomotion. These dominant negative effects of this mutant were seen on several different extracellular matrices. Furthermore, disassembly of adhesion sites and detachment of cells, seen as a consequence of increased cellular PIP2 levels in cells overexpressing PIP 5-kinase, were suppressed. Our results emphasize that vinculin targeting to and incorporation into adhesion sites is independent of lipid binding, whereas adhesion site turnover strongly depends on the vinculin-PIP2 interaction.
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Materials and Methods |
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Protein expression, purification and characterization
Recombinant Vt(858-1066) variants were expressed and purified as described (Ziegler et al., 2002). Circular dichroism spectroscopy (J-810 Spectropolarimeter; Jasco) confirmed the
-helical character of Vt variants (Miller et al., 2001
). Vh(1-258) bearing an N-terminal glutathione-S-transferase (GST) tag was expressed in Escherichia coli strain M15, purified on glutathione-Sepharose beads according to manufacturer's instructions (Amersham Biosciences) and used bound to beads in pull-down experiments. Protein concentrations were determined using a BCA assay (Sigma) and identical molar amounts of Vt protein were used in all experiments. However, the Coomassie dye take of Vt proteins was not identical (e.g. 70% and 40% of wild-type (wt) Vt for Vt-H3 and Vt-LD, respectively) and resulted in relatively faint bands of these proteins on Coomassie-stained gels. A comparable effect on the dye take was observed for similar lipid-binding-site mutants of ezrin (Barret et al., 2000
).
Vesicle pull-down assay and statistic analysis
Sucrose-loaded large unilamellar vesicles (SLVs) were generated using a mini-extruder (Avanti Polar Lipids) according to manufacturer's instructions, mixed with Vt protein and sedimented. In brief, vesicles containing the phospholipids phosphatidylcholine (PC), phosphatidylserine (PS) (45%) (Sigma) and PIP2 (7%) (Merck Biosciences) from bovine brain, in molar ratios 4.8:4.5:0.7, were prepared by solubilizing dried phospholipid films in buffer 1 (600 mM sucrose, 100 mM NaCl, 40 mM Tris-HCl pH 7.5 and 3 mM MgCl2). Vesicles were subjected to repeated freeze-thaw cycles (five times) and thereafter to extrusion (11 times) using 0.2 µm filters in a mini-extruder. Vesicles suspension was diluted 1:5 in buffer 2 (100 mM NaCl, 40 mM Tris-HCl pH 7.5, 3 mM MgCl2) and vesicles were collected by high-speed centrifugation, 100,000 g for 30 minutes in an Airfuge (Beckman Instruments). Vesicles were washed again and finally suspended in buffer 2 (1 mg ml1 total lipid). Proteins were diluted in buffer 2 (5 µM protein, final concentration), precentrifuged at 20,000 g for 15 minutes to remove any protein aggregates and incubated with SLVs (0.5 mg ml1 final concentration) at 37°C for 15 minutes. After incubation, protein-vesicle mixtures were centrifuged at 20,000 g for 15 minutes. Pellet and supernatant fractions were separated and proteins retrieved from supernatants by methanol-chloroform precipitation (Wessel and Flügge, 1984). Pellet and supernatant were subjected to SDS-PAGE and Coomassie-stained bands analysed by densitometry (EASY RH apparatus and EASY Image Plus Software; Herolab). Statistical significance of differences in all data sets (unless stated otherwise) was tested by variance analysis (post hoc Bonferroni/Dunn) using Statview 5.0® (SAS Institute). Images were compiled in Adobe® Photoshop® (v.6).
Vinculin tail interaction with Vh (D1) and actin filaments
The interaction of Vt variants with the Vh domain 1 (D1, amino acids 1-258) fragment was tested in a GST pull-down assay. GST-Vh (D1) protein bound to glutathione-Sepharose beads was equilibrated in phosphate buffer (50 mM NaH2PO4, pH 7.4, 0.2 mM EGTA) and incubated with Vt proteins (6 µM) for 30 minutes at 37°C. Beads were then washed three times with phosphate buffer. Pellet fractions were analysed on Coomassie-stained SDS-PAGE gels. The interaction of Vt variants with actin filaments was tested by high-speed cosedimentation at various molar ratios of actin and Vt, as described (Ziegler et al., 2002). Prepolymerized actin was used at a 3 µM final concentration. Pellets and supernatants were analysed by densitometry of Coomassie-stained gels (see above). Images were compiled in Adobe Photoshop (v.6).
Cell lines and stable transfection
B16-F1 mouse melanoma cells (ATCC CRL-6323) were cultured in Dulbecco's modified Eagle's medium (DMEM) plus 4.5 g l1 glucose (Invitrogen), 10% foetal calf serum (FCS) (PAA Laboratories), 2 mM glutamine at 37°C and 7% CO2. Superfect® (Qiagen) was used according to the manufacturer's recommendation for transient and stable transfections. Cells expressing vinculin variants tagged with green fluorescent protein (GFP) were sorted using a cell sorter (MoFlo; Dako Cytomation) and cultured in the presence of 1 mg ml1 G418 (Invitrogen) to generate stably expressing populations. Following the second round of sorting, cell populations kept under selection pressure were used up to passage six for experiments. Protein expression levels were determined by semiquantitative immunoblotting using a monoclonal vinculin antibody (hVin; Sigma) and densitometry (see above). Blots were scanned and images were compiled in Adobe Photoshop (v.6). For experiments with murine myc-tagged PIP 5-kinase (Rozelle et al., 2000
), wild-type B16-F1 cells or cells stably expressing GFP-vinculin-wt or GFP-vinculin-LD were transfected on coverslips using Superfect (Qiagen) 16 hours after attachment to fibronectin and processed for immunofluorescence as specified below.
Immunofluorescence and video microscopy
After 6 hours of attachment to laminin, cells were fixed with 4% paraformaldehyde (PFA) solution in PBS for 15 minutes, permeabilized with a mixture of 0.1% Triton X-100 in PFA for 60 seconds and blocked with 1% bovine serum albumin (BSA) in PBS. Cell adhesions and actin filaments were stained with mouse anti-paxillin (BD Biosciences) and tetramethylrhodamine isothiocyanate (TRITC) tagged anti-mouse IgG (Sigma) antibodies, and with Alexa-350-coupled phalloidin (Molecular Probes), respectively. In PIP-5-kinase experiments with wild-type B16-F1 cells, actin filaments were stained with Alexa-594-coupled phalloidin and endogenous vinculin using mouse anti-vinculin antibody (Sigma) and Alexa-488-labelled anti-mouse IgG (Molecular Probes). To detect PIP-5-kinase expression, anti-myc antibody 9E10 (Abcam) was used that had been directly coupled to Alexa 350 (Molecular Probes) according to manufacturer's instructions. B16-F1 cells co-expressing PIP5-kinase [or myc-tagged L61-Rac (Lamarche et al., 1996)] with GFP-tagged vinculin variants were stained using a mixture of Alexa-594/phalloidin, and Alexa-350-tagged anti-myc antibody or anti-BiPro 4A6 antibody (Rüdiger et al., 1997
) and Alexa-350-labelled anti-mouse IgG (Molecular Probes). Coverslips were mounted using Mowiol® (Aventis). Specimens were examined in a Zeiss Axiovert S100TV microscope using a 100x Plan-Neofluar oil objective (NA 1.3) or a 63x Plan-Neofluar oil objective (NA 1.25) and photographed with a TE/CCD-1000 TKB camera (Princeton Scientific Instruments). To determine the ratio of polarized cells in B16F1 populations, phalloidin-stained cells displaying a clear lamellipodium and trailing edge were scored as motile, cells with several lamellipodia or no clear orientation as ambiguous and cells without lamellipodia as unpolarized. Phalloidin staining was used to improve the visualization of lamellipodia and the orientation of cells. Numbers of polarized, unpolarized and ambiguous cells were counted manually in representative fields (n>600 cells per vinculin variant). Video microscopy was performed as described earlier (Rottner et al., 1999a
). All acquisitions and movies were controlled using IPLab software (Scanalytics). Movies were processed by Scion Image software (v.1.6) (Scion). Figures were assembled for presentation using Adobe Photoshop (v.6) and Adobe Illustrator® (v.9).
Adhesion and spreading of cells and migration in collagen matrix
12-well plates (Nunc) were coated with either laminin (25 µg ml1) or fibronectin (50 µg ml1) (Sigma) and incubated at room temperature for 1 hour. Alternatively, they were coated with collagen I (1 mg ml1; Cohesion Technologies) and allowed to polymerize for 3 hours. B16-F1 cells expressing GFP-vinculin variants were harvested in trypsin-EDTA. 1.5x104 cells were seeded in each well. For analysis of adhesion, cells were allowed to attach for 10 minutes at 37°C for laminin and fibronectin or 90 minutes for collagen. Nonadherent cells were removed by washing the wells three times with PBS. Cells were fixed in 4% PFA in PBS. The number of cells in ten random microscopic fields (450-550 cells) was counted using a Nikon Eclipse TE 300 with a 10x Plan-Fluar objective (NA 0.3). For analysis of spreading, cells were treated as described above and allowed to attach for 15 minutes at 37°C on laminin or fibronectin. After washing and fixation, cells were stained with TRITC-phalloidin (Sigma) and mounted on slides. Cells were examined in a Zeiss Axiophot microscope using a 40x Plan Neo-Fluar oil objective (NA 1.3) and photographed with a RTE/CCD-1300 Y/HS camera (Roper Scientific). Three subpopulations of cells were counted: spread cells with clear peripheral lamellipodia, non-spread cells (which were just attached) and ambiguous cells that fell in neither of the two categories.
The migratory capacities of the B16-F1 populations expressing GFP-vinculin variants were analysed by time-lapse video microscopy as described (Niggemann et al., 1997). In brief, cells were harvested in trypsin-EDTA and 6x104 cells in 50 µl medium were mixed with 100 µl of a carbonate-buffered collagen solution (1.67 mg ml1 bovine dermal type-I collagen). The suspension was filled into self-constructed chambers and the collagen was allowed to polymerize at 37°C for 30 minutes. Migration of the cells was recorded for 15 hours in a 1920-fold time-lapse mode. The paths of 30 randomly selected cells were calculated at 15 minute intervals by computer-assisted cell tracking using custom-made software (Niggemann et al., 1997
), and migratory parameters (number of motile cells, velocity, persistence) were calculated from these data.
Analysis of individual adhesion sites (confocal microscopy and FRAP)
Microscopy
B16-F1 cells were microinjected (InjectMan NI 2; Eppendorf) with constructs encoding GFP-vinculin-wt or the -LD mutant. Constructs were allowed to express for 3 hours before mounting coverslips into a chamber containing gassed growth medium. The chamber was placed onto a temperature-regulated 37°C microscope stage 15 minutes before viewing. Time-separated confocal 12-bit images were collected using a Zeiss LSM 510 META confocal laser scanning microscope system with a 63x Plan-Apochromat oil objective (NA 1.4). GFP was excited with the 488 nm line of the argon laser, and reflected and emitted light were separated using a 470-500 nm band-pass filter (for interference reflection microscopy) and a 505 nm long-pass filter (for viewing GFP emission). Line scans were performed with fourfold averaging per pixel. When bleaching, the 488 nm laser line output was set to 100% using 50 iterations. Two images (lines) were scanned before bleaching to determine the pre-bleach intensity of GFP-vinculin. After bleaching, line scans were collected for 3 minutes and stacked together to form a two-dimensional image, a so-called kymograph, in which the x-axis is distance along the line scan and the y-axis represents time with t=0 at the top.
Image analysis
To determine speed of focal-adhesion translocation, adhesions in time-lapse sequences were manually tracked using the Motion Analysis package (Kinetic Imaging). The software calculated the speeds after appropriate calibration. Fluorescence recovery in time-lapse fluorescence recovery after photobleaching (FRAP) sequences was analysed using the Lucida Image Analysis package (Kinetic Imaging). Because focal adhesions had a tendency to translocate, it was not possible to perform a simple spot analysis. Instead, kymographs were produced along the axis of the adhesion sites and the direction of translocation. Five line scans were then taken along the kymograph time axis taking into account any translocation. The average of this was normalized with respect to the initial fluorescence intensity. Normalized values were subtracted using the first post-bleach intensity, which also resulted in background subtraction. The data were then inversely plotted to produce a straight-line graph with positive gradient. The x-axis intercept was used to determine the time constant for fluorescence recovery (i.e. the time taken to recover to a level of 50%). Statistics of data in this paragraph were performed applying an unpaired two-tailed Student's t-test (with Welch correction) using InStat3® (GraphPad Software).
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Results |
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Vt mutants defective in lipid binding still bind protein ligands
The lipid-binding sites in helix 3 and the C-terminus overlap with attachment sites for protein ligands [e.g. for filamentous actin (Hüttelmaier et al., 1997) and for the vinculin head (Vh) (Izard et al., 2004
; Miller et al., 2001
)]. To analyse the consequences of the mutations described above on ligand binding, we performed a pull-down assay and a high-speed cosedimentation assay to probe for Vh or F-actin binding, respectively (Fig. 1D,E). Because the intramolecular head-to-tail interaction controls the ligand-binding properties of vinculin (Critchley, 2000
; Bakolitsa et al., 2004
), our vinculin mutants were designed to leave the head-to-tail interaction intact. In order to demonstrate this, we tested the interaction of Vt mutants with a GST-Vh [domain 1 (D1), 1-258] fusion protein. GST-Vh(D1) immobilized on glutathione-Sepharose beads was incubated with an excess of Vt protein and sedimented by centrifugation. As shown in Fig. 1D, the head-to-tail interaction was found to be functional for all Vt mutants. Cosedimentation with F-actin at a molar ratio of actin:Vt of 5:1 displayed >95% binding for all Vt mutants compared with wild-type Vt (data not shown), indicating that overall F-actin binding is well conserved. When a molar ratio of actin:Vt of 2:1 was used, a ratio that represents the maximal binding capacity of F-actin [0.3-0.5 moles of Vt per mole of actin (Johnson and Craig, 1995
)], a decrease in binding of Vt mutants H3 and LD to 65% compared with the wild type was observed (Fig. 1E). In conclusion, the general conformation and overall binding specificities for protein ligands of the Vt domain were found to be largely intact in the lipid-binding-site mutants CT, H3 and LD.
Intracellular localization of vinculin variants is normal
B16-F1 mouse melanoma cells were transfected with full-length wild-type and mutant GFP-vinculin variants, and cell populations stably expressing the respective constructs were obtained by a combination of cell sorting and antibiotic selection. Expression of GFP-vinculin was stable for more than six passages. The resulting populations of cells expressing GFP-vinculin variants were used for a set of experiments to analyse alterations in protein localization, cell adhesion and migration. Protein expression patterns (Fig. 1F,G) were determined by semiquantitative western blotting of cell lysates from parental B16-F1 and transfected populations at different passages (1-5). A antibody against vinculin was used to monitor both endogenous vinculin and GFP fusion proteins (Fig. 1F). Comparison of the levels of recombinant to endogenous protein revealed ratios of exogenous to total vinculin varying from 0.3 to 0.45 (Fig. 1G). Cell populations stably expressing GFP-vinculin variants were generated several times with identical results.
Intracellular distribution patterns of GFP-vinculin fusion proteins in B16-F1 cells were analysed by counterstaining focal adhesions with anti-paxillin antibodies and actin filaments with phalloidin, in cells seeded onto laminin and fixed after 6 hours. Fig. 2 shows that wild-type GFP-vinculin as well as all lipid-binding mutants localized to focal adhesions, where they perfectly colocalized with paxillin to adhesion sites linked to actin filaments. The population of B16-F1 cells expressing GFP-vinculin-LD, however, displayed a high frequency of cells with abnormally long adhesive extensions. Furthermore, these cells contained more pronounced stress fibres and larger focal adhesions than populations expressing other vinculin variants (Fig. 2).
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Vinculin-LD interferes with the motility of B16-F1 cells
On laminin, B16-F1 cells display a motile phenotype that is characterized by highly polarized cells with wide lamellipodia at their leading edges (Ballestrem et al., 1998). This phenotype was also observed in a large proportion of cells expressing vinculin-wt or vinculin mutants CT and H3 6 hours after attachment to laminin (see also Fig. 2). By contrast, the number of cells displaying this phenotype when expressing vinculin-LD was significantly reduced compared with cells expressing GFP-tagged vinculin-wt (Fig. 3A-C). Classification of more than 600 cells for each population allowed us to quantify the defect of vinculin-LD-expressing cells in adopting a motile phenotype. Whereas 54% of vinculin-wt cells displayed a motile phenotype and only 24% did not, this ratio was inverted in the vinculin-LD cells with 12% polarized and motile cells, whereas 63% of the cells were spread but not polarized or with clear lamellipodia and therefore judged to be non-motile. Using time-lapse microscopy of single cells migrating on laminin, locomotory activity of vinculin-wt-expressing cells was confirmed, whereas not a single motile vinculin-LD-expressing cell was detected in this assay (see Fig. S1 in supplementary material).
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Vinculin-LD delays cell adhesion and spreading on different extracellular matrices
B16-F1 cells express receptors for the extracellular matrix proteins laminin (integrins 1ß1 and
6ß1), fibronectin (integrins
4ß1 and
5ß1) and collagen (integrin
1ß1) (Ballestrem et al., 1996
). Hence, we tested the effect of our vinculin variants for adhesion and spreading on these matrices. Populations of B16-F1 cells expressing wild-type or mutant GFP-vinculin were allowed to attach for various times. Comparable degrees of adhesion were reached on laminin and fibronectin 10 minutes after seeding, and on collagen after 90 minutes. Non-adherent cells were washed away and remaining cells counted in randomly selected microscopic fields. Cell adhesion was quantified as a proportion of adherent cells expressing the different vinculin variants (mean±s.d., n=4-6 independent experiments) compared with cells expressing GFP-vinculin-wt, using an average of 450-550 cells per test. As illustrated in Fig. 4A, vinculin-LD-expressing cells displayed a decrease in adhesion of 79% on collagen (after 90 minutes) and of 42% and 34% on laminin and fibronectin, respectively (after 10 minutes), compared with the vinculin-wt population.
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To analyse the effects of vinculin variants on spreading, cells were allowed to attach for 15 minutes on laminin or fibronectin, fixed and phalloidin stained. Based on shape and cytoskeletal staining, cells were divided in three groups: spread, non-spread and ambiguous cells (Fig. 4B). Spreading was expressed as a proportion of spread cells compared with the total number of adherent cells (mean±s.e., n=3 independent experiments), using more than 150 cells per test. As illustrated in Fig. 4B, vinculin-LD-expressing cells displayed a decrease in spreading of 31% and 46% on laminin and fibronectin, respectively (after 15 minutes), and six times more non-spread cells than cells expressing vinculin-wt or other vinculin variants. After 90 minutes of adhesion and spreading on laminin or fibronectin, differences in the number of adherent cells were decreased to less than 10%. Therefore, we conclude that vinculin-LD induces a delay in cell spreading compared with the other vinculin constructs rather than a defect in adhesion.
Vinculin-LD strongly impairs the migration of B16-F1 cells in collagen gels
Spontaneous migration of cells expressing mutant and wild-type GFP-vinculin was analysed in a three-dimensional collagen matrix. The cells were embedded in collagen and migration of cells (n=30) in one field was followed for 15 hours using time-lapse video microscopy. Differences in motility of vinculin-wt- and vinculin-LD-expressing cells became immediately evident upon comparison of representative tracks (Fig. 5A). Both the proportion of motile cells and their velocity were calculated from tracking data (Fig. 5B,C). After an initial phase of adhesion to the collagen matrix (also compare to spreading, Fig. 4), the number of motile cells remained constant and averages (mean±s.d.) were calculated for each of the populations between 6 hours and 15 hours (constant phase). A reduction of motility to 16% compared with the wild type (and other vinculin constructs) was observed in the vinculin-LD-expressing cell population (Fig. 5B). The velocity was determined from the relative movement of motile cells (Fig. 5C). During the constant phase of movement (6-15 hours), the average velocity (mean±s.d.) of vinculin-LD-expressing cells was reduced to 53% of the value of cells expressing exogenous vinculin-wt, revealing a strong inhibition of cell migration. This effect was observed on a background of endogenous vinculin (70% of total vinculin, also compare to Fig. 1F). The persistence of cell migration was analysed based on angle changes, showing no significant differences (data not shown). Values for vinculin-LD, however, were calculated based on a few rather short tracks, because most cells registered did not migrate at all.
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Vinculin-LD is correctly incorporated into adhesion sites but inhibits translocation and disassembly of adhesions
Localization of vinculin-LD was indistinguishable from that of vinculin-wt in B16-F1 cells, but the number of stress fibres and the number and size of adhesions appeared to be increased in vinculin-LD-expressing cells (see also Fig. 2). To test whether exchange rates of vinculin molecules in individual adhesion sites are altered in vinculin-LD-expressing cells, we used FRAP to measure the rate of re-incorporation of GFP-tagged vinculin variants after bleaching. The half-time of fluorescence recovery after photobleaching was about 45 seconds for both wild-type and lipid-binding-deficient vinculins (Fig. 6A) in adhesions that remained stable for more than 10 minutes. Hence, a lipid-binding deficiency of vinculin-LD does not interfere with its incorporation into and exchange rate for individual adhesion sites. To study further the impairment of cell migration in vinculin-LD-expressing cells (Figs 3, 5), we then analysed the overall turnover of adhesion sites. Confocal video microscopy of individual adhesions revealed a strong inhibition of retrograde sliding (translocation) in vinculin-LD-expressing cells (Fig. 6B). To estimate the average speed of adhesion-site movement towards the cell centre, more than 100 individual sites per vinculin variant were tracked. Adhesions in vinculin-LD-expressing B16-F1 cells translocated at 22% of the speed acquired by vinculin-wt-expressing cells, reflecting a prominent stabilization of adhesion sites by vinculin-LD. The influence of vinculin-LD on adhesion stability was further emphasized by the finding that the number of adhesion sites formed and disassembled during the observation period of 20 minutes was remarkably different from controls. In vinculin-wt-expressing cells, 27% of total adhesions were newly formed and 32% were disassembled, whereas only 9% were formed and 2% disassembled in cells expressing vinculin-LD. Thus, vinculin-wt-expressing cells showed a five times higher adhesion-site turnover than cells expressing the lipid-binding-deficient mutant. Hence, we conclude that cell signalling leading to turnover of adhesion sites requires the ability of vinculin to bind acidic phospholipids, whereas the basic exchange rates of vinculin molecules for a given adhesion (i.e. during adhesion-site maintenance) do not.
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Our results argue strongly for a lipid-dependent regulation of vinculin interactions in adhesion sites (Fig. 7). To test this model further, we asked whether a general increase in cellular PIP2 levels could trigger the release of vinculin from adhesions and whether this might be altered in vinculin-LD-expressing cells. We therefore overexpressed murine PIP 5-kinase (Tolias et al., 2000
), which leads to membrane localization of this kinase and high PIP2 levels (Doughman et al., 2003
), in B16-F1 cells co-expressing either the vinculin-wt or the vinculin-LD variant. In line with our model, increased PIP2 levels in these cells induced relocalization of vinculin-wt from adhesion sites to the perinuclear region. This effect was evident 8 hours after transfection of B16-F1 cells (data not shown). By 12 hours, cells expressing PIP 5-kinase
had lost vinculin-wt staining from adhesion sites and started to detach (Fig. 6C). By contrast, cells expressing GFP-vinculin-LD were more resistant to this treatment. Out of 60 cells co-expressing vinculin-LD and PIP 5-kinase
for 12 hours, 41 showed vinculin-LD localized to adhesion sites (Fig. 6C). Moreover, the effect of PIP-5-kinase-
overexpression was dependent on the enzymatic activity of PIP 5-kinase
and is contrast with that of PIP 5-kinase
, which also displaces talin as a kinase-dead variant (Ling, 2002), not competing with vinculin binding to adhesion sites. Thus, in cells expressing kinase-deficient (KD) PIP 5-kinase
(Shibasaki et al., 1997
), no relocalization was observed of vinculin-wt or -LD (Fig. 6C), indicating that lipid-kinase activity was required to displace vinculin from adhesions. These findings support the view that the connection between integrin-based adhesions and the actin cytoskeleton is regulated by PIP2 signals in a vinculin-dependent fashion.
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Discussion |
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Spreading of cells requires a high turnover of small, transient adhesion sites to allow (fast) outward movement of peripheral lamellipodia under the control of the small Rho-family GTPase Rac (Rottner et al., 1999b; Sheetz et al., 1999
). The spreading process is independent of force coupling to talin (Giannone et al., 2003
) and RhoA-controlled actomyosin contractility (Zaidel-Bar et al., 2003
), two mechanisms that are involved in adhesion-site maturation (Giannone et al., 2003
; Rottner et al., 1999b
). By contrast, spreading depends on non-receptor tyrosine kinases such as focal-adhesion kinase (FAK) and Src-family kinases (Von Wichert et al., 2003
). Tyrosine kinases are activated as a result of integrin binding to the extracellular matrix (Felsenfeld et al., 1999
; Wang et al., 2001
). In addition, tyrosine phosphorylation is a hallmark of adhesion sites (Zaidel-Bar et al., 2003
) and tight control of phosphorylation regulates the function of cytoskeletal proteins during cell spreading. For instance, in protein-tyrosine-phosphatase-2-deficient fibroblasts, FAK activity strongly reduces the residence lifetime of paxillin and vinculin in adhesion sites (Von Wichert et al., 2003
). Protein-tyrosine-phosphatase-2 deficiency leads to inhibition of cell spreading on fibronectin and vitronectin, as well as to the accumulation of immature adhesions lacking
-actinin (Von Wichert et al., 2003
). Effects of tyrosine kinase activity on vinculin recruitment to adhesion sites were also observed for cell adhesion to vitronectin, because vinculin is only recruited to force-activated vitronectin receptors in c-Src-deficient cells (Felsenfeld et al., 1999
; Galbraith et al., 2002
). Both examples suggest that tyrosine-kinase activity can negatively regulate the association of vinculin and paxillin with adhesion sites, leading to increased adhesion dynamics. This conclusion is further supported by the behaviour of vinculin-deficient fibroblasts, which show reduced spreading and less-stable focal adhesions accompanied by an increase in FAK activity and in locomotion (Xu et al., 1998a
).
From these findings, it can be concluded that lack of vinculin inhibits cell spreading owing to a disability of the affected cells to stabilize initial adhesions. This mechanism cannot, however, explain the severe spreading defect observed in vinculin-LD-expressing B16-F1 cells (this study), because these cells produce mature adhesion sites and display a strongly reduced migratory activity associated with a severely diminished movement of individual adhesion sites. The defect in spreading of B16-F1 cells does not result from a reduced speed of incorporation of the mutant vinculin and is observed in the presence of endogenous vinculin. Combining these observations with data showing that PIP2 and actin binding to the vinculin tail can compete with each other (Steimle et al., 1999), and with our results showing that the actin-binding ability of Vt-LD seems largely intact, we propose that incorporation of vinculin-LD into newly formed adhesion sites leads to an interaction with F-actin but does not respond to release signals from the cell membrane. Subsequently, an unregulated interaction between integrins and the actin cytoskeleton prevents the rapid turnover of adhesion sites, as would be required for cell spreading and in lamellipodia of migrating cells (Fig. 7). Furthermore, vinculin acts as a scaffold for other adhesion proteins (Critchley, 2000
) and these complexes might also be stabilized by the LD mutant.
Residence-lifetime analysis of vinculin in adhesion sites has shown that the half-time of recovery for GFP-vinculin is considerably shorter than overall lifetimes of adhesions in B16-F1 cells (this study). A similar relation between lifetimes was reported in fibroblasts (Von Wichert et al., 2003). Because the vinculin exchange rates within adhesion sites must be such that the protein can balance the stabilization and maturation of adhesions against dissipation, vinculin can contribute to a differential control of adhesion-site assembly and disassembly, as observed at different locations in motile cells (Ballestrem et al., 2001
; Von Wichert et al., 2003
; Wehrle-Haller and Imhof, 2002
). This control function is rendered inadequate by introducing a dominant negative mutant of vinculin that is incapable of transducing PIP2 signals to the destabilization of the adhesion structure.
In contrast to a previous report (Gilmore and Burridge, 1996), we did not find evidence for a PIP2-binding-dependent incorporation of vinculin into focal adhesions. Instead, our results are consistent with the assumption that vinculin acts as a sensor, thus converting local modulation of PIP2 levels to adhesion-site dynamics. Vinculin-LD is unable to execute this function. Finally, PIP2 might also influence the association of vinculin binding partners other than talin and F-actin like the actin-nucleator complex Arp2/3 (DeMali et al., 2002
) and protein kinase C
(Ziegler et al., 2002
).
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Acknowledgments |
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Footnotes |
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* Present address: IZKF-Interdisciplinary Centre for Clinical Research Leipzig, Faculty of Medicine, University of Leipzig, 04103 Leipzig, Germany
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References |
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