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Angiogenesis, Metastasis, and the Cellular Microenvironment

Src Regulates Actin Dynamics and Invasion of Malignant Glial Cells in Three Dimensions¹

¹ Brain Tumor Research Center, Montreal Neurological Institute and Hospital, Department of Neurology and Neurosurgery, McGill University, Montreal, Quebec, Canada and ² Hospital for Sick Children and Department of Molecular Genetics and Microbiology, University of Toronto, Toronto, Ontario, Canada

Requests for reprints: Rolando Del Maestro, Brain Tumor Research Center, Montreal Neurological Institute and Hospital, Department of Neurology and Neurosurgery, McGill University, 3801 University Room BT-205, Montreal, Quebec, Canada H3A 2B4. Phone: 514-398-8293; Fax: 514-398-3971. E-mail: rolando.delmaestro{at}mcgill.ca

	Abstract

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 
Malignant glioma is the major brain tumor in adults and has a poor prognosis. The failure to control invasive cell subpopulations may be the key reason for local glioma recurrence after radical tumor resection and may contribute substantially to the failure of the other treatment modalities such as radiation therapy and chemotherapy. As a model for this invasion, we have implanted spheroids from a human glioma cell line (U251) in three-dimensional collagen type I matrices, which these cells readily invade. We first observed that the Src family kinase-specific pharmacologic inhibitors PP2 and SU6656 significantly inhibited the invasion of the cells in this assay. We confirmed this result by showing that expression of two inhibitors of Src family function, dominant-negative-Src and CSK, also suppressed glioma cell invasion. To characterize this effect at the level of the cytoskeleton, we used fluorescent time-lapse microscopy on U251 cells stably expressing a YFP-actin construct and observed a rapid change in actin dynamics following addition of PP2 in both two-dimensional and three-dimensional cultures. In monolayer cultures, PP2 caused the disappearance of peripheral membrane ruffles within minutes. In three-dimensional cultures, PP2 induced the loss of actin bursting at the leading tip of the invadopodium. The inhibition of Src family activity is thus a potential therapeutic approach to treat highly invasive malignant glioma.

	Introduction

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 
Grade IV astrocytoma or glioblastoma multiforme is distinct in that it rarely metastasizes outside the brain (reviewed in ref. 1). However, despite the advances in surgical and radiotherapy techniques and the development of new chemotherapeutic regimens and reagents, patient prognosis remains poor. This is due to the presence in glioblastoma multiforme of subpopulations of highly invasive cells that disseminate into the surrounding brain parenchyma and result in tumor recurrence at the edges of the resection cavity and/or at distant sites in the brain.

In our attempts to characterize the determinants of glioma cell invasion, we have developed and characterized a model where glioma cell aggregates are implanted in a solid collagen type I matrix (2-4). This method approximates the in vivo environment of tumor invasion more accurately than standard two-dimensional migration assays while allowing for convenient monitoring of invasion rates and individual cell behavior (5). The benefits of three-dimensional systems have become evident in light of recent observations concerning the difference in behavior between cells migrating on a two-dimensional plane and cells invading a matrix (6-8). Strategies that efficiently impair migration in monolayers have been ineffective when used to modulate invasion due to the capacity of these cells to adapt their behavior and continue their ability to invade.

The three-dimensional matrix model system can be readily manipulated by addition of different soluble reagents in the matrix; we have therefore used this system to assess the ability of available pharmacological agents to inhibit glioma invasion.³ We found that among the most effective agents that decreased the invasion rates of glioma cells were the Src family kinase inhibitors PP2 and SU6656. We confirmed these results by showing that expression of two inhibitors of Src family function, dominant-negative (DN)-Src and CSK, also suppressed glioma cell invasion. In monolayer cultures, addition of PP2 resulted in the rapid and selective disappearance of peripheral membrane ruffles. This seems to correspond in the three-dimensional collagen matrix to a loss of actin bursting activity at the tip of the invadopodia. Taken together, these results suggest that Src protein kinases are involved in glioma cell invasion by regulating actin dynamics.

	Results

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 
Inhibition of Glioma Cell Invasion in Three Dimensions by Src Inhibitors
Src inhibitors have been shown to suppress the invasion of prostate, colon, and ovarian cancer cells (9-11). Similarly, our screen of inhibitors of glioma invasion in three-dimensional matrices indicated that among the most effective inhibitory agents was the Src family kinase inhibitor PP2. When spheroids of the human glioma cell line U251 were implanted into the collagen gel, the cells rapidly invaded the matrix radially and the extent of invasion can be assessed by measuring the diameter between the fronts of invading cells. Addition of the Src family kinase inhibitor PP2 to the medium inhibited this invasion in a dose-dependent manner (Fig. 1A). PP3, an analogue of PP2, was used as a negative control because it exhibits the same nonspecific effects as PP2 without inhibiting the Src family kinases (12, 13). In our assay, PP3 did not significantly alter the invasion of the U251 cells from the spheroid into the collagen matrix even at high concentrations (Fig. 1A). Similar results were obtained with PP2 and PP3 using spheroids of C6 astrocytoma rat cells, showing that this effect is not specific to the U251 human glioma cells (data not shown).

View larger version (25K): [in this window] [in a new window] [Download PPT slide]   FIGURE 1. Effects of the Src inhibitors on glioma invasion. A. Dose-dependent decrease in the invasion of U251 spheroids in a three-dimensional collagen matrix with PP2 but not with PP3 (n = 8 spheroids per condition). **, P < 0.01, compared with control (two-factor mixed-design ANOVA). B. Similar effect observed with SU6566 (SU). C. Single-cell invasion distances of U251 glioma cells between 24 and 48 hours after implantation measured using time-lapse videomicroscopy. Measurements were separated in 100 µm intervals. Bars, % cells whose invasion distance fell within that interval in each experiment. D. Effect of addition in the matrix of 10 µmol/L PP2 on the distribution seen in C. The great majority of the cells (70%) do not invade >50 µm in that interval (n = 3 movies, an average of 40 cells measured for each). **, P < 0.01, significantly higher than control; , P < 0.01, significantly lower than control.

To confirm that the effect of PP2 on tumor cell invasion was at the level of the rate of cell movement, we measured the rate of invasion of individual cells into the collagen matrix using time-lapse videomicroscopy. U251 spheroids were implanted into three-dimensional collagen gels and allowed to invade so that individual invading cells at a distance from the main spheroid mass could be identified and monitored. At 24 hours postimplantation, the gel was overlaid with either medium or medium containing 10 µmol/L PP2 and placed into a chamber attached to a microscope. A computer-controlled camera was used to take bright-field pictures of the invading cells every 4 minutes for 24 hours. After this time, a video was generated, which allowed the tracing of the invasion paths of each of the cells from the commencement of invasion. The distances calculated using the Northern Eclipse program are shown in Fig. 1C and D. The results are shown as a distribution of cells invading different distance intervals. In normal conditions (Fig. 1C), some cells invade very little or not at all (<50 µm) in the period assessed, whereas others invade large distances in the same period (>450 µm). Addition of 10 µmol/L PP2 caused a significant shift of the distribution toward small invasion distances (Fig. 1D), confirming that the inhibition of the tumor spread observed in Fig. 1A is due to a reduction of the cell invasion velocity into the collagen matrix. However, these results do not detect the effects of Src inhibition in the percentage of glioma cells participating in invasion, because only the cells that detached from the spheroid after the first 24 hours, when no inhibitors are present, are measured.

The Src inhibitors used in this study inhibit all of the Src family kinases. Three of these kinases, Src, Fyn, and Yes, were expressed in glioma cells as shown by probing lysates of U251 cells with antibodies to these proteins (Fig. 2A, top, and B). c-Src also has a neuronal-specific splice form (N-Src), which contains an insert of 6 amino acids. To determine which Src protein was expressed in U251 cells, we generated a N-Src-specific antibody by immunizing rabbits with a polypeptide composed of the 6 N-Src-specific amino acids. The resulting antibody specifically immunoprecipitated N-Src (data not shown). Lysates from U251 cells were immunoprecipitated with anti-N-Src and probed in Western blots with an antibody that recognizes both c-Src and N-Src. Figure 2A shows that U251 cells express c-Src (top) but not N-Src (bottom). As controls, human 293 cells, which express c-Src, and a fragment of human normal cortex obtained from a surgical operation, which expresses N-Src, are shown. The significance of this absence of N-Src from glioma and the expression patterns of this splice form in different populations of neural stem cells (see ref. 16) and different stages of differentiation are currently under investigation. Taken together, those results indicate that the targets of our inhibitors are expressed in the cell line used.

View larger version (28K): [in this window] [in a new window] [Download PPT slide]   FIGURE 2. U251 glioma cells express Src, Fyn, and Yes but not N-Src. A. Western blot (WB) of total cell lysates obtained from 293 cells, normal human brain, and U251 cells probed for Src (top). Immunoprecipitation (IP) of the same lysates using a N-Src-specific antibody probed with the Src antibody, which recognizes both N-Src and c-Src, showing that N-Src is expressed in normal human brain but not in the human glioblastoma cell line U251 (bottom). B. Western blot of total cell lysate from U251 cells probed for Yes and Fyn antibodies. C. Efficient inhibition of Src activity by the inhibitor PP2. Total cell lysates of U251 cells expressing activated Src were probed with an anti-phosphotyrosine antibody to confirm the disappearance of the signal when increasing concentrations of PP2 are added.

PP2 Decreases the Proliferation Rate of Glioma Cells
We then asked whether the inhibition of glioma invasion by PP2 was due to a toxic or apoptotic effect of the Src inhibitor on the tumor cells. U251 cells grown in monolayers were trypsinized, counted, and plated in six-well plates (day 0). At day 1, cells were treated with 10 µmol/L PP2 or 5 µmol/L SU6656 and the cells were counted every 2 days. Figure 3A shows a significant decrease in the proliferation rates of glioma cells following treatment with PP2 or SU6656. The calculated doubling times of the cultures were 36, 44, and 60 hours for control, PP2-treated, and SU6656-treated cells, respectively. During the proliferation assay, no significant cell death or de-adhesion was observed (data not shown). In addition, when the cells were labeled with terminal deoxynucleotidyl transferase dUTP nick end labeling, which stains apoptotic nuclei, <3% of both control and treated cells showed staining within their nuclei (data not shown), indicating that the decrease in the number of cells treated with the Src inhibitor was not due to cell death.

View larger version (13K): [in this window] [in a new window] [Download PPT slide]   FIGURE 3. Effects of PP2 on U251 glioma cells proliferation. A. Decrease in the proliferation rates of glioma cells by PP2 and SU6656. At day 0, 50,000 cells were plated in six-well plates and the inhibitors were added at day 1 (arrow). Cells were counted every 2 days by trypsinizing the cells and feeding them in a Coulter particle counter. **, P < 0.01, compared with control (two-factor ANOVA). B. Decrease in the proliferation index of the cultures with PP2 but not with PP3 as measured by the ratio of Ki67-positive nuclei 4 days after addition of the inhibitors. **, P < 0.01, compared with control (ANOVA).

Overexpression of DN-Src and CSK Decreases the Invasion Rates of Individual Glioma Cells
To confirm the role of Src in regulating the rate of glioma invasion, we expressed two inhibitors of Src family function, DN c-Src and CSK, in U251 cells. The DN-Src mutant used encodes two mutations, lysine to arginine at amino acid 255 and tyrosine to phenylalanine at position 527, that renders the enzyme catalytically inactive and locked in an open conformation and effective in sequestering Src family kinase activators and substrates, therefore interfering with the activity of all Src family members. CSK phosphorylates Src, Fyn, and Yes on a COOH-terminal tyrosine, inactivating those enzymes (19). To express DN-Src and CSK in glioma cells, we cloned the genes encoding these proteins into recombinant adenovirus vectors, which we showed previously allows efficient and nontoxic expression of genes in glioma cell lines (20). The adenovirus vector used, pAdTrack, also expresses the green fluorescent protein (GFP) on a separate cytomegalovirus promoter, which allows for identification of the infected cells.

U251 spheroids were incubated in suspension with the recombinant adenoviruses prior to implantation. During the first 24 hours, the cells invaded the matrix; after that time, infected cells commenced expressing the recombinant gene products. This method eliminates the possible effects of adenoviral infection on spheroid formation or cell detachment from the main tumor mass. The cells were then filmed during the second 24 hours and their individual invasion distances were assessed. Once the distances were recorded, a GFP fluorescence image was overlaid on the first image of migrating cells to identify which cells expressed DN-Src/GFP, CSK/GFP, or GFP. Because we routinely infect 50% of the cells in a spheroid, the uninfected cells provide an internal control for each experiment.

In cells expressing GFP alone, no significant effect on invasion was observed as compared with noninfected cells in the same spheroid (Fig. 4A). In contrast, expression of DN-Src or CSK significantly reduced the invasion distances of the cells (Fig. 4B and C), confirming that the results obtained with PP2 and SU6656 were indeed due to inhibition of Src family member activity. These results as well as the results from Fig. 1C and D are summarized in Table 1. Table 1 also shows the maximum invasion distance for an individual cell observed in all the conditions. Treatment of cells with PP2 as well as overexpression of DN-Src or CSK not only resulted in a significant decrease in the average invasion distances of the glioma cells in the three-dimensional collagen matrix but also eliminated the subpopulation of the most highly invasive cells.

View larger version (32K): [in this window] [in a new window] [Download PPT slide]   FIGURE 4. Expression of DN-Src and CSK in the cells invading the collagen matrix. A. Infection of the cells with a GFP-expressing adenovirus (bottom) did not significantly alter their invasion velocity compared with control, noninfected cells in the same spheroids (top). B. Expression of a DN mutant of c-Src significantly decreased U251 invasion distances. C. Expression of CSK also, to a lesser extent, shifted the distribution toward smaller invasion distances (n = 3 movies, an average of 20 cells measured for each). **, P < 0.01, significantly higher than control; , P < 0.05; , P < 0.01, significantly lower than control.

Figure 5A shows one of the YFP-actin expressing cells grown in a monolayer. Different structures can be seen, such as stress fibers and a large lamellipodium at the leading front of the cell (arrow). After addition of 10 µmol/L PP2, we observed within minutes the rapid disappearance of the lamellipodium. This loss was selective and not due to general actin disassembly because stress fibers did not disappear even after longer periods (data not shown). To quantify this effect and to confirm that this was not due to aberrant effects of overexpressing YFP-actin, the disappearance of actin-rich ruffles was measured after PP2 treatment of U251 cells. Under phase microscopy, the ruffles appear as dark borders at the cell periphery (Fig. 5B, arrows). Cells were counted as "ruffle positive" if they contained at least one of these ruffles. At time 0, PP2 was added to a final concentration of 5 µmol/L. Figure 5C shows the rapid decrease in ruffle-positive cells in the population that becomes significant after 1 minute of PP2 addition (5 µmol/L). A similar effect was observed with SU6656 (data not shown). To confirm that this is not a response of the cells to fluid perturbation caused by the addition of PP2 to the culture, the same experiment was repeated without inhibitor (data not shown) or the negative control PP3 with no effect observed (Fig. 5C).

View larger version (50K): [in this window] [in a new window] [Download PPT slide]   FIGURE 5. Effect of PP2 on peripheral membrane ruffles in glioma cells. A. Fluorescent time-lapse videomicroscopy images of a single U251 stably expressing a YFP-actin construct before and after addition of 10 µmol/L PP2 show a selective disappearance of the peripheral membrane ruffle (arrow). Bar, 20 µm. B and C. Quantification of this effect using low-magnification time-lapse videomicroscopy of untransfected U251 cells. Under phase, the peripheral lamellipodia appear as phase-dark ruffles (arrows) and disappear after addition of PP2 (B). Bar, 50 µm. Quantification shows that this effect is specific to PP2 and becomes significant 2 minutes after addition of PP2 at time 0 (n = 8 movies, an average of 40 cells counted for each). **, P < 0.01 compared with PP3 (two-factor mixed-design ANOVA). D and E. Effects of the recombinant adenoviruses on the number of cells with membrane ruffles in the population (n = 3, an average of 95 cells counted for each). *, P < 0.05; **, P < 0.01, compared with control (ANOVA). Images show typical fields 24 hours after addition of the virus. Bar, 50 µm.

PP2 Causes a Rapid Loss of Actin Bursting at the Invading Tip of U251 Cells in Three Dimensions
We then analyze whether the loss of lamellipodia observed in monolayer cultures treated with PP2 similarly affected actin dynamics in cells invading a three-dimensional matrix. Spheroids from the YFP-actin–overexpressing U251 cells were generated and implanted into solid collagen matrices. After 24 hours, cell invasion by randomly invading cells was quantified by time-lapse fluorescent microscopy. These cells adopted a different morphology compared with the same cells grown in monolayers, exhibiting rounded cell bodies and long protrusions extending away from the main tumor mass (Fig. 6A). As in Fig. 5A, the same cells were monitored before and after the addition of PP2. Cells in the three-dimensional matrix did not form long membrane ruffles, but a close-up of the tip of the invadopodium revealed the presence of pulsating bursts of actin (Fig. 6B). Quantification of the fluorescence in this region shows that this bursting occurred at a regular frequency (every 10 minutes for this particular cell) and disappeared shortly after addition of 5 µmol/L PP2 (Fig. 6C).

View larger version (32K): [in this window] [in a new window] [Download PPT slide]   FIGURE 6. Effect of PP2 on the actin dynamics in U251 in the three-dimensional collagen matrix. A. YFP-actin image of a cell invading away from the spheroid (bottom). Bar, 20 µm. B. High-magnification zoom of the invading tip of the cell showing a "burst" of actin. Bar, 2 µm. C. Quantification of the fluorescence intensity in the area in A shows that this bursting occurs at regular interval in this cell and is abrogated by the addition of 5 µmol/L PP2 on the collagen gel (dashed line).

	Discussion

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

To obtain these results, we have implanted glioma spheroids in three-dimensional collagen matrices. This model was chosen because it reflects many of the characteristics of glioma invasion of normal neural tissue in vivo, such as process extension, probing, degradation of the extracellular matrix, and adhesion to and detachment of the cell from the matrix. Collagen type I was chosen for its capacity to form solid gels at 37°C, which is not the case for other matrix components such as collagen type IV (4). The resulting matrix is free of growth factors and other types of extracellular components that could influence our experiments. Addition of other components to the matrix-like fibronectin or laminin, for example, had little effect on glioma invasion in this system and was not included here (4). An environment more similar to the situation encountered by glioma cells in vivo could be obtained by coculturing the glioma spheroids with rat brain aggregates (29-32). However, this type of experiment does not allow for the live qualitative and quantitative analysis of single invading glioma cells and will be part of future experiments designed to test the efficiency of Src inhibition on the control of glioma infiltration in vivo.

The involvement of Src in cell migration has led to recent interest in investigating the potential of Src as a target to block invasion in different types of cancer. Stable overexpression of DN-Src or CSK in carcinoma cells greatly decreased the potential of those cells to metastasize in vivo (33). In prostate cancer cells, invasion has been shown to correlate with FAK/Src signaling (34). The invasion of these cells was blocked by PP2 (34) as well as two novel Src inhibitors, CGP77675 and CGP76030 (10). The latter inhibitors were also shown to decrease proliferation of prostate cancer cells. In colon cancer cells, PP2 minimally affected proliferation but strongly inhibited invasion (11). Ovarian cancer cell invasion was also inhibited by addition of PP2 (9). In the case of colon and ovarian cancer cells, PP2 was shown to exert its effects at the level of extracellular matrix degradation by blocking urokinase-type plasminogen activator receptor expression (11) or transforming growth factor-ß–induced urokinase-type plasminogen activator expression (9), respectively. Although we did not investigate these pathways in our glioma cells, time-lapse microscopy studies have shown effects of Src inhibition on glioma cell invasion at the level of peripheral actin dynamics (Figs. 5 and 6). Recent literature suggests potential targets for Src in these events. The small G-protein Rac, for example, has been long implicated in lamellipodia regulation (35). Src, by phosphorylating its substrate p130cas, creates binding sites for the protein Crk (36), which then recruits DOCK180, a member of a novel family of proteins that directly activate Rac (37, 38). However, we have shown recently that in glioma cells Rac is an important survival-inducing protein and that inhibition of its activity results in apoptosis of most glioblastoma cell lines and primary cells derived from human tumor samples (20). Another interesting candidate for a Src substrate affecting invasion is the F-actin binding cortactin. Phosphorylation of cortactin by Src is required for the formation of sphingosine-1-phosphate–induced membrane ruffling, and this effect is independent of Rac (24). In NIH-3T3 cells, expression of an inhibiting truncation of the Cbl proto-oncogene resulted in the formation of dorsal membrane ruffles that were also blocked by the PP2 inhibitor (39). Interestingly, unlike what we showed in Fig. 5 for U251 cells, PP2 did not inhibit the formation of peripheral actin ruffles in this system. We are currently characterizing the Src invasion pathway and particularly investigating whether other proteins that we have found to mediate glioma invasion such as Rho kinase (ROCK) are regulated by Src activity.

Our results suggest that in glioma cells Src is not mutated to become constitutively active. Indeed, CSK, which inhibits the activity of wild-type but not oncogenic Src, mimicked to some extent the effects of the Src inhibitors and DN-Src and suggests that the endogenous Src regulatory mechanisms are still functional. However, we could not determine whether the endogenous Src was hyperactivated in glioma cells, as the basal activity of the Src family members was difficult to detect. Src family activity may be concentrated in a subset of glioma cells (e.g., the most invasive cells) or elevated at the leading edge of those cells.

Several groups have suggested that, because cells use similar intracellular processes to migrate and to divide, inhibition of one process would result in an increase of the other ("Go or Grow" hypothesis; refs. 40-42). We have shown recently that this hypothesis does not describe the behavior of individual medulloblastoma cells in two-dimensional or three-dimensional collagen matrix invasion models (7). Recent data have also shown that targeting of one of these pathways in glioma cells does not necessarily result in overactivation of the other (43, 44). Here, we show that inhibition of Src kinases results in a decrease of both glioma cell proliferation (Fig. 3) and invasion (Fig. 1). The effect of Src inhibition on the cell cycle might therefore be of concern if the Src inhibitors are used to treat glioma together with chemotherapeutic agents that depend on inducing cytotoxicity of proliferating cells. In addition, it is not known what the effect of Src inhibition is on nontransformed human astrocytes, although PP2 can inhibit the proliferation of normal rodent astrocytes (45).

The future treatment of high-grade glioma will depend on the ability of treatment modalities to target the highly infiltrative cells that escape surgical resection of the main tumor mass (46), whether by manipulating their survival (20, 47, 48), their extracellular guidance cues (29), or their intracellular invasion machinery (44, 49).⁴ The three-dimensional collagen type I matrix has shown to predict, to some extent, the invasion of glioma cells into fetal and adult astrocytes aggregates (29) while allowing for the identification and characterization of proteins and agents that suppress invasion. We propose, based on our results using the three-dimensional collagen matrix, that Src inhibition following surgical removal of malignant glioma is a potential therapeutic avenue to prevent reoccurrence of this tumor.

	Materials and Methods

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 
Cell Culture
The human glioblastoma cell line U251 and the rat astrocytoma cell line C6 were purchased from American Type Culture Collection (Rockville, MD) and maintained in DMEM supplemented with 10% fetal bovine serum and penicillin/streptomycin in a humidified 37°C incubator containing 5% CO₂. A sample of normal human cortex was obtained from a surgical specimen (resected for tumor exposure) at the Montreal Neurological Institute and Hospital following guidelines.

Hanging drop aggregates were prepared as described previously (5, 7, 50). Briefly, 20 µL drops of DMEM/10% fetal bovine serum containing 30,000 cells each were deposited on the lid of a 100 mm Petri dish. The lid was then inverted and placed in the incubator for 3 days. The aggregates are then transferred into another dish coated with 2% agar in normal DMEM for 2 days.

Three-Dimensional Collagen Matrices
The glioma spheroids were implanted into three-dimensional collagen gels as described previously (4, 7). Briefly, a liquid bovine type I dermal collagen solution (3.0 mg/mL, Cohesion, Palo Alto, CA) was supplemented with one-tenth volume of 10 x DMEM. The pH of the solution was adjusted to 7.4 using 0.1 mol/L NaOH. This collagen preparation was aliquoted into 24-well plates (500 µL/well) and a glioma spheroid was added in each well while the solution was still viscous. The gel was solidified by incubating the plates at 37°C for 30 minutes before being overlaid with 500 µL of supplemented DMEM with or without pharmacologic inhibitors. If an inhibitor was added, its concentration was doubled in the overlay solution to take into account the volume of the gel. The Src inhibitors used (PP2, PP3, and SU6656) were purchased from Calbiochem (San Diego, CA) and resuspended in DMSO to a final concentration of 10 mmol/L. The extent of cell dispersion was measured every 2 days using a calibrated micrometer in the ocular of an inverted light microscope (5).

Single-Cell Invasion Distance Measurements
U251 spheroids were implanted as described above and allowed to invade for 24 hours. The plate was then placed in an inverted Axiovert 25 microscope (Carl Zeiss, Kirkland, Quebec, Canada) equipped with an environment chamber where temperature and CO₂ content were maintained by a heated stage and a CO₂ monitor (Carl Zeiss). Images of the invading cells were captured every 4 minutes for the next 24 hours by a Retiga 1300 CCD digital camera (Qimaging, Vancouver, British Columbia, Canada) controlled by the Northern Eclipse 6.0 time-lapse videomicroscopy software (Empix Imaging, Mississauga, Ontario, Canada). The individual images were then compiled into a movie (7). Every individual cell that detached from the main spheroid mass after the first 24 hours was numbered and their individual paths were traced on the screen by following them throughout the movie. The resulting traces were then measured using a calibrated Curve Measurement feature in the Northern Eclipse software. For measurements in the presence of PP2, the inhibitor was added a few minutes before starting the capture of the images.

Immunoprecipitation and Western Blotting
The c-Src antibody (clone 327) has been provided generously by Dr. Joanne Brugge (Harvard Medical School, Boston, MA). The rabbit polyclonal anti-Yes antibody was purchased from Upstate (Charlottesville, VA), whereas the mouse monoclonal anti-Fyn antibody was from Santa Cruz Biotechnology (Santa Cruz, CA). The N-Src-specific polyclonal antibody was generated by injecting rabbits with a synthetic peptide composed of residues NNTRKVDVREGD, the 6 amino acids specific to N-Src plus 3 amino acids on each side to help antigenicity, coupled to MA-peptide. For immunoprecipitation, cells or frozen tissue sample were lysed in radioimmunoprecipitation assay buffer [50 mmol/L Tris-HCl (pH 7.2), 150 mmol/L NaCl, 0.1% SDS, 0.5% sodium deoxycholate, 1% NP40]. The lysate was incubated with 4 µL of the N-Src-immunized whole rabbit serum and 30 µL of protein A-Sepharose (Amersham Biosciences, Piscataway, NJ) for 90 minutes at 4°C. The beads were washed three times with radioimmunoprecipitation assay buffer and resuspended in SDS-PAGE loading dye. Western blots were done following common procedures. The proteins were subjected to SDS-PAGE and transferred to nitrocellulose membranes. The membranes were blocked [150 mmol/L NaCl, 25 mmol/L Tris (pH 8.1), 5% milk, 0.05% Triton X-100] and incubated with the respective primary antibodies. The horseradish peroxidase–conjugated antibodies (Bio-Rad, Hercules, CA) were used at a 1:5,000 dilution and detected by chemiluminescence.

The PP2 inhibitor was tested by infecting U251 cells with activated Src-expressing adenoviruses (see below). At the time of infection, different concentrations of the inhibitor was added to the supernatant. At 24 hours postinfection, the cells were harvested and lysed as described above and the total cell lysate was probed with the anti-phosphotyrosine antibody 4G10.

Cell Proliferation Assays
Proliferation was measured by plating 5 x 10⁴ U251 cells/well of six-well plates and counting the cells every 2 days. At day 1, for treated wells, 10 µmol/L PP2 or 5 µmol/L SU6656 were added. The medium containing the inhibitors was replaced every 2 days.

The proliferative population of U251 was determined by indirect immunofluorescence against the nuclear protein Ki67. Briefly, cells treated for 4 days with the PP2 or PP3 inhibitors were fixed 15 minutes in 4% paraformaldehyde, permeabilized with 0.1% Triton/PBS, and blocked 45 minutes in 0.5 % bovine serum albumin in PBS. The cells were then incubated for 1 hour with anti-Ki67 (1:200, PharMingen, San Diego, CA), washed, and incubated with Cy3-labeled goat anti-mouse antibodies (1:400, Jackson ImmunoResearch, West Grove, PA). Before mounting and examination by fluorescence microscopy, the cells were counterstained for 2 minutes with Hoechst 33258 (Sigma, St. Louis, MO).

Recombinant Adenoviruses
The DN and activated Src adenoviruses used in this study have been described previously (17). The CSK adenovirus was obtained using the same method, the pAdEasy recombination system (Stratagene, La Jolla, CA; 51). The rat CSK cDNA was a generous gift from Dr. Jean-François Côté (McGill University, Montreal, Quebec, Canada). Briefly, CSK was cloned in the GFP-expressing shuttle vector pAdTrack, recombined with the adenoviral vector pAdEasy by co-electroporation in bacteria, linearized, transfected, and amplified in 293A cells. The viruses were purified by centrifugation on CsCl gradients, dialyzed, and titered in 293A cells.

The invasion distance assay described above was modified the following way: Prior to implantation into the collagen matrix, the U251 spheroids were incubated with 10⁶ plaque-forming units of the respective viruses in 1 mL complete DMEM for a few hours. The viruses are then washed and the spheroid was implanted. After 24 hours, a GFP image of the spheroid is taken and saved. A movie is then taken and the invasion distances of individual cells were measured as described above. When all the numbers have been compiled, the GFP image is overlaid on the first phase image of the movie to determine which of the cells were infected and the results were allocated accordingly.

YFP-Actin U251 Cells
The actin cytoskeleton of live U251 cells was imaged using the pEYFP-actin construct from Clontech (Palo Alto, CA). The construct was transfected using LipofectAMINE Plus (Invitrogen, Gaithersburg, MD) in U251 cells, which were then selected in 0.6 mg/mL G418 (Life Technologies, Gaithersburg, MD) until clones could be seen. Three clones expressing high amounts of YFP-actin, as seen under fluorescence microscopy, were isolated and expanded. Movies in two and three dimensions were made, taking pictures every 30 seconds of the same cells before and after addition of the PP2 inhibitor. For monolayers, the cells were placed without cover in the conditioned chamber of the microscope in a minimal amount of complete DMEM. At time 0, the volume is doubled with prewarmed complete DMEM containing the inhibitor at a 2x concentration. For collagen gels, the medium overlaying the gel is removed before the beginning of the movie. The plate is placed without cover on the microscope, and at time 0, 500 µL prewarmed complete DMEM containing the inhibitor at 2x concentration is pipetted onto the gel.

	Acknowledgements

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 
We thank Drs. Joan Brugge and Jean-François Côté for the generous gifts of the Src antibody and CSK cDNA, respectively, and A-M. Osiceanu for critical reading of the article.

	Notes

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 
¹ Alex Pavanel and Franco Di Giovanni Funds for Brain Tumor Research (R.F. Del Maestro), Canadian Cancer Society and National Cancer Institute of Canada (D.R. Kaplan), National Cancer Institute of Canada Terry Fox Studentship (A. Angers-Loustau), Canadian Institute for Health Research doctoral research award (T.E. Werbowetski), Harold Johns and Canadian Cancer Society research scientist award and Canada Research Chair (D.R. Kaplan), Montreal Neurological Institute Killam Scholarship, and William Feindel Chair in Neuro-Oncology (R.F. Del Maestro).

Note: A. Angers-Loustau was cosupervised by R.F. Del Maestro and D.R. Kaplan.

³ R. Hering et al., submitted for publication.

⁴ Hering et al., submitted for publication.

Received July 26, 2004; revised September 15, 2004; accepted September 27, 2004.

	References

Top Notes Abstract Introduction Results Discussion Materials and Methods Acknowledgements References

 

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