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© The Rockefeller University Press, 0021-9525/1998//1749 $5.00
The Journal of Cell Biology, Volume 143, Number 6, , 1998 1749-1760

Release of cAMP Gating by the 6β4 Integrin Stimulates Lamellae Formation and the Chemotactic Migration of Invasive Carcinoma Cells

Department of Medicine, Beth Israel Deaconess Medical Center and Harvard Medical School, Boston, Massachusetts 02215

The 6β4 integrin promotes carcinoma in-vasion by its activation of a phosphoinositide 3-OH (PI3-K) signaling pathway (Shaw, L.M., I. Rabinovitz, H.H.-F. Wang, A. Toker, and A.M. Mercurio. Cell. 91: 949–960). We demonstrate here using MDA-MB-435 breast carcinoma cells that 6β4 stimulates chemotactic migration, a key component of invasion, but that it has no influence on haptotaxis. Stimulation of chemotaxis by 6β4 expression was observed in response to either lysophosphatidic acid (LPA) or fibroblast conditioned medium. Moreover, the LPA-dependent formation of lamellae in these cells is dependent upon 6β4 expression. Both lamellae formation and chemotactic migration are inhibited or "gated" by cAMP and our results reveal that a critical function of 6β4 is to suppress the intracellular cAMP concentration by increasing the activity of a rolipram-sensitive, cAMP-specific phosphodiesterase (PDE). This PDE activity is essential for lamellae formation, chemotactic migration and invasion based on data obtained with PDE inhibitors. Although PI3-K and cAMP-specific PDE activities are both required to promote lamellae formation and chemotactic migration, our data indicate that they are components of distinct signaling pathways. The essence of our findings is that 6β4 stimulates the chemotactic migration of carcinoma cells through its ability to influence key signaling events that underlie this critical component of carcinoma invasion.

Key Words: integrin • migration • cyclic AMP • phosphodiesterase • cytoskeleton

Abbreviations used in this paper: [cAMP]_i, intracellular cyclic AMP concentration; DIC, differential–interference contrast; Gi, inhibitory type G protein; IBMX, isobutylmethylxanthine; LPA, lysophosphatidic acid; PDE, phosphodiesterase; PI3-K, phosphoinositide 3-OH kinase.

Address correspondence to Arthur M. Mercurio, Beth Israel Deaconess Medical Center-Dana 601, 330 Brookline Ave., Boston, MA 02215. Tel.: (617) 667-7714. Fax: (617) 975-5531. E-mail: amercuri{at}bidmc.harvard.edu

CARCINOMA invasion is a complex process that involves directed migration and localized proteolysis (24). Although the mechanistic basis of invasion had been elusive, recent advances in molecular cell biology have facilitated a much more rigorous analysis of this important and critical component of cancer progression. In particular, insight into the function and regulation of cell adhesion receptors, as well as proteases, has fueled significant progress in our understanding of the invasive process. Studies aimed at defining specific signal transduction pathways that determine the behavior of invasive carcinoma cells are also contributing to an uncovering of the molecular basis of invasion.

Recent work by our group and others has implicated a key role for the 6β4 integrin in carcinoma invasion (3, 10, 32, 35, 40, 47). This integrin, which is a receptor for the laminins, is essential for the organization and maintenance of epithelial structure. In many epithelia, 6β4 mediates the formation of stable adhesive structures termed hemidesmosomes that link the intermediate filament cytoskeleton with the extracellular matrix (2, 12). The importance of this integrin in epithelial structure has been reinforced by the generation of β4-nullizygous mice that exhibit gross alterations in epithelial morphology and anchorage to the basement membrane (9, 46). In contrast to its function in normal epithelia, 6β4 can stimulate carcinoma migration and invasion through its ability to interact with the actin cytoskeleton and mediate the formation and stabilization of lamellae (32). This dynamic function of 6β4 in enhancing the migration of invasive carcinoma cells is quite distinct from its role in maintaining stable adhesive contacts in normal epithelia by associating with intermediate filaments. In fact, we have established that the ability of 6β4 to stimulate carcinoma migration and invasion depends upon its preferential activation of a phosphoinositide 3-OH kinase (PI3-K)¹/Rac signaling pathway that we (40) and others (18) have shown is necessary for invasion. In essence, our studies have defined an integrin-mediated mechanism of carcinoma invasion that involves the stimulation of carcinoma migration by the dynamic association of 6β4 with F-actin and the activation of a specific signaling pathway by this integrin.

Although we have established the involvement of 6β4 in the migration of invasive carcinoma cells, the nature of this migration has not been well defined. Moreover, signaling pathways distinct from PI3-K/Rac that are also regulated by 6β4 are likely to contribute to carcinoma migration. For these reasons, we sought to examine the migration mediated by 6β4 in more detail and to identify other signaling pathways regulated by this integrin that contribute to migration. The results obtained indicate that 6β4 stimulates the chemotactic migration of invasive carcinoma cells but that it has no influence on their haptotactic migration. Importantly, we demonstrate that the ability of 6β4 to suppress the intracellular cAMP concentration ([cAMP]_i) by activating a cAMP-specific phosphodiesterase (PDE) is essential for its enhancement of lamellae formation and chemotactic migration. Although PI3-K and cAMP-specific PDE activities are required for lamellae formation and chemotactic migration, we conclude that they are components of distinct signaling pathways.

	Materials and Methods

Top Abstract Materials and Methods Results Discussion References

 
Cell Culture and Antibodies
We used stable subclones of MDA-MB-435 human breast carcinoma cells that had been transfected with either the expression vector alone (mock transfectants), a full-length β4 cDNA (MDA/β4 transfectants), or a mutated β4 cDNA that lacked the entire cytoplasmic domain with the exception of four amino acids distal to the transmembrane sequence (MDA/β4-CYT). The characterization of these transfectants has been described previously (38, 40). Both the β4 transfectants and the β4-CYT transfectants expressed the 6β4 heterodimer on the cell surface as assessed by FACS^® analysis and immunoprecipitation of surface-labeled extracts (40). The surface expression of 6β4 in these transfectants was comparable to the expression seen in other breast carcinoma cell lines that express this integrin endogenously such as MDA-MB-231 cells (Shaw, L.M., unpublished observation). All MDA-MB-435 cells were cultured in Dulbecco's modified Eagle's medium (DME) with 10% fetal calf serum plus 1% L-glutamine, 1% penicillin, and 1% streptomycin (GIBCO BRL, Gaithersburg, MD). Clone A cells, originally isolated from a human, poorly differentiated colon adenocarcinoma (7) and were cultured in RPMI 1640 medium containing 10% fetal calf serum plus 1% L-glutamine, 1% penicillin, and 1% streptomycin.

NIH-3T3 cells were cultured in DME containing 10% newborn calf serum plus 1% L-glutamine, 1% penicillin, and 1% streptomycin. NIH-3T3 conditioned medium was prepared from normal culture medium incubated with cells for 2 d before harvest with cellular debris removed by centrifugation.

The following function blocking, integrin-specific monoclonal antibodies (mAb) were used: mAb 13 (mouse anti-β1; S. Akiyama, National Institutes of Health, Research Triangle Park, NC), G0H3 (rat anti-6; Immunotech, Westbrook, ME) and 2B7 (mouse anti-6, prepared by our laboratory [39]). Non-specific mouse IgG was purchased from Sigma Chemical Co. (St. Louis, MO).

Migration and Invasion Assays
Cells were harvested using trypsin, rinsed three times with serum-free DME containing 250 µg/ml heat-inactivated BSA (DME/BSA), and then resuspended in DME/BSA. For migration assays, the lower surface of the membrane in each Transwell chamber (6.5-mm-diam, 8 µm pore size; Costar, Cambridge, MA) was coated for 30 min with either 15 µg/ml laminin-1 purified from Englebreth-Holm-Swarm tumor (19), 15 µg/ml collagen I (Vitrogen^®; Collagen Biomaterials, Palo Alto, CA), or NIH-3T3 conditioned medium. For chemotaxis assays, either NIH-3T3 conditioned medium or lysophosphatidic acid (LPA) was added to the lower chamber. For haptotaxis assays, DME/BSA was added to the lower chamber. Cells (5 x 10⁴) suspended in DME/BSA were added to the upper chamber. After incubating for 4 h at 37°C, nonmigrating cells were removed from the upper chamber with a cotton swab and cells that had migrated to the lower surface of the membrane were fixed with 100% methanol and stained with 0.2% (wt/vol) crystal violet in 2% ethanol. Migration was quantified by counting cells per square millimeter using bright-field optics. For antibody inhibition experiments, cells were incubated with 20 µg/ml of antibody for 30 min and then added to the Transwell chambers. The effects of pertussis toxin, IBMX (Calbiochem-Novabiochem, La Jolla, CA), forskolin, and rolipram (Sigma Chemical Co.) on migration were assessed by preincubating the cells with these reagents for 30 min before assay and including them in the assay medium at the concentrations noted in the figure legends.

Invasion assays were performed as described previously (40). In brief, 10 µg of Matrigel (Collaborative Research, Bedford, MA) was diluted with cold water and dried onto each Transwell filter. The Matrigel was reconstituted with DME for 1 h before its use in the assays. Cells were prepared as above and then added to the upper chamber of each well. NIH-3T3 conditioned medium was added to the lower chamber. Cells were allowed to invade for 4 h and then cells that had invaded were stained and quantified as described above.

cAMP Assays
Culture dishes (35-mm) were coated overnight with 20 µg/ml of collagen I in PBS and then blocked with serum-free RPMI containing 250 µg/ml BSA (RPMI/BSA). Cells (1.5 x 10⁶) were then plated for 2 h and harvested by quickly removing the medium and extracting them directly with 80% (vol/vol) ethanol. Cell extracts were collected, cleared by centrifugation in a microcentrifuge for 10 min, dried in a SpeedVac (Savant Instruments, Farmingdale, NY) for 1.5 h, and then resuspended in 50 mM phosphate buffer, pH 6.2. The intracellular cAMP concentration was quantified using a cAMP enzyme-linked immunoabsorption assay (cAMP EIA; Cayman Biochemicals, Ann Arbor, MI) following the manufacturer's recommendation using nonacetylated cAMP as a standard and acetylcholine esterase-linked cAMP as a competitor. Values were corrected for cell number as determined from replicate plates. In some experiments, either 50 µM forskolin alone or forskolin plus 1 mM IBMX was added to cells 15 min before harvesting. To determine the cAMP content of cells under normal culture conditions, cells were plated in 35-mm dishes in DME plus 10% FCS, incubated for 18 h, and then processed as described above.

Phosphodiesterase Assays
cAMP PDE assays were performed according to the protocol of Sette et al. (37). In brief, cells were plated onto collagen I coated dishes as described for cAMP assays. Cells were then scraped from the dishes in a hypotonic lysis buffer (PDE lysis buffer: 20 mM Tris-HCl, pH 8.0, 1 mM EDTA, 0.2 mM EGTA, 50 mM sodium fluoride, 10 mM sodium pyrophosphate, 0.5 µg/ml leupeptin, 0.7 µg/ml pepstatin, 4 µg/ml aprotinin, and 2 mM PMSF) and then sonicated. Cellular debris was removed by centrifugation and the supernatants were assayed immediately for PDE activity. PDE activity of cell extracts (2–4 µg protein) was assayed in cAMP PDE assay buffer (20 mM Tris-HCl, pH 8.0, 10 mM MgCl₂, 1.25 mM β-mercaptoethanol, 0.14 mg/ml BSA, 1 µM cAMP, and 0.2 µCi [³H] cAMP) for 10 min at 34°C. The reaction was stopped by adding 40 mM Tris, pH 7.5, containing 10 mM EDTA and heating for 2 min at 100°C. The reaction products were then digested with 50 µg Crotalus atrox snake venom (Sigma Chemical Co.) for 30 min at 34°C, separated from substrate using SpinZyme acidic alumina devices (Pierce Chemical Co., Rockford, IL), and quantified using a scintillation counter (Wallace, Gaithersburg, MD). Values were corrected for protein content and are reported as pmol cAMP hydrolyzed/min per milligram of protein. Protein content of cell extracts was determined using the Bio-Rad protein reagent (Hercules, CA) with BSA as a protein standard. Where noted, cells were incubated either for 30 min with 50 µM forskolin or 100 nM wortmannin or for 5 min with 100 nM LPA before harvest. For rolipram inhibition of PDE activity, 100 nM rolipram was added to cell extracts for 5 min before assaying for PDE activity.

Assessment of Lamellae Formation
Glass coverslips were coated overnight at 4°C with 20 µg/ml collagen I or laminin-1 and then blocked with BSA (0.25% in RPMI). The MDA-MB-435 transfectants were trypsinized and rinsed as described above, and then plated onto the coverslips for 2 h. As noted, cells were then treated with either 1 mM IBMX or 0.2% DMSO for 30 min. Subsequently, the cells were either treated with 100 nM LPA for 5 min or left untreated and then fixed for 10 min with 4% paraformaldehyde containing 10 mM Pipes, pH 6.8, 2 mM EGTA, 2 mM MgCl₂, 7% sucrose, and 100mM KCl. The coverslips were rinsed three times with PBS and mounted in glycerol. For the analysis of clone A cells, the cells were treated with IBMX or DMSO for 30 min, plated on laminin-1–coated coverslips, incubated for 45 min at 37°C, and then fixed. Clone A cells were then rinsed three times with PBS and incubated with blocking solution containing 1% BSA/5% normal donkey serum for 30 min. Cells were incubated with 20 µg/ml TRITC-labeled phalloidin in blocking solution for 30 min. Cells were rinsed four times with PBS over 30 min and then mounted in glycerol containing 1x PBS, pH 8.5, and 0.1% propylgallate. All cells were imaged with a Nikon Diaphot 300 inverted microscope (Tokyo, Japan) using either Nomarski differential–interference contrast (DIC) or phase–contrast optics. Images were captured with a charge-coupled device camera (Dage-MTI, Michigan City, IN), a frame grabber (Scion, Frederick, MD) and a 7600 Power Macintosh computer (Apple Computer, Cupertino, CA). Images were analyzed and lamellar area quantified using IPLab Spectrum image analysis software (Signal Analytics, Vienna, VA) using the criteria for defining lamellae used previously by our group (32). Lamellae were defined as broad, flat cellular protrusions rich in F-actin and devoid of membrane-bound vesicles. The lamellar area of each cell was determined using both phase contrast optics and FITC-phalloidin staining.

Analysis of PDE Expression
To determine the relative expression of PDE in the cells used in this study, cell extracts (40 µg of protein) were resolved by SDS-PAGE (8%), transferred to nitrocellulose, and then immunoblotted with PDE4-specific antibodies provided by M. Conti (Stanford University, Stanford, CA) (15). Immune complexes were detected with horseradish peroxidase-conjugated secondary antibodies and visualized using SuperSignal chemiluminescent substrate (Pierce Chemical Co.).

Analysis of PI3-K Activation
The activation of PI3-K by the integrin 6β4 was assessed as described previously (40). In brief, cells were trypsinized and rinsed as above, resuspended in RPMI/BSA at a concentration of 2 x 10⁶ cells/ml and incubated for 30 min with integrin-specific antibodies or in buffer alone. Either IBMX (1 mM), forskolin (50 µM) or DMSO (0.2%) was added for 10 min before plating the cells onto tissue culture dishes coated with goat anti–rat IgG Ab. After incubation for 30 min at 37°C in the presence of IBMX, forskolin, or DMSO, the cells were washed twice with cold PBS and solubilized at 4°C for 10 min with 20 mM Tris, pH 7.4, 137 mM NaCl, 1% NP-40, 10% glycerol, 1 mM sodium orthovanadate, 2 mM PMSF, and 5 µg/ml of aprotinin, pepstatin, and leupeptin. Equivalent amounts of protein from each extract were incubated for 3 h at 4°C with the antiphosphotyrosine mAb, 4G10 (Upstate Biotechnology, Lake Placid, NY) and protein A–Sepharose (Pharmacia Biotech, Piscataway, NJ). The Sepharose beads were washed twice with lysis buffer then twice with 10 mM Hepes, pH 7.0, and 0.1 mM EGTA. Beads were then resuspended with kinase buffer plus 100 µM ATP, 25 µM MgCl₂, 10 µCi [-³²P]ATP, and 10 µl sonicated brain lipids and incubated for 10 min at room temperature. The reaction was stopped using 60 µl 2N HCl and 160 µl chloroform/methanol (1:1). Lipids were resolved using potassium oxalate-coated thin layer chromatography plates.

	Results

Top Abstract Materials and Methods Results Discussion References

 
Expression of the 6β4 Integrin in MDA-MB-435 Cells Enhances Their Chemotactic Migration
The possibility that expression of the 6β4 integrin influenced the rate of either haptotactic or chemotactic migration was assessed. For this purpose, stable transfectants of MDA-MB-435 cells were used that expressed either the 6β4 integrin (MDA/β4) or a deletion mutant of 6β4 (MDA/β4-CYT) that retains only four amino acids of the β4 cytoplasmic domain, immediately proximal to the transmembrane domain (40). As shown in Fig. 1 A, subclones of the MDA/β4 transfectants (5B3 and 3A7) exhibited a rate of haptotactic migration toward laminin-1 that was slightly lower than the rate observed for subclones of the mock transfectants (6D7 and 6D2). In marked contrast, expression of 6β4 induced a substantial increase in the rate of chemotaxis of these cells towards conditioned medium from NIH-3T3 cells (Fig. 1 B). The rate of chemotaxis of the MDA/β4 transfectants (5B3 and 3A7) was 15– 20-fold greater than that of the mock transfectants (6D7 and 6D2) over a 4-h time period. These data indicate that expression of 6β4 potentiates chemotactic migration of MDA-MB-435 cells without substantially altering their rate of haptotaxis.

View larger version (42K): [in this window] [in a new window] [Download PPT slide]   Figure 1 Expression of the 6β4 integrin in MDA-MB-435 carcinoma cells stimulates chemotaxis but not haptotaxis. The migration of the MDA/β4 (5B3 and 3A7) MDA/β4-CYT (3C12, 1E10), and MDA/mock (6D2 and 6D7) transfectants toward laminin-1 (haptotaxis; A), 3T3 conditioned medium (chemotaxis; B), or LPA (chemotaxis; C and D) was assessed using a modified Boyden chamber. The lower surfaces of Transwell membranes were coated with either laminin-1 (A), conditioned medium (B), or collagen I (C and D), and then either BSA (A) 3T3 conditioned medium (B) or LPA (C and D) was added to the lower chambers. Cells (105 [A and B] or 5 x 104 [C and D]) were placed in the upper chambers. After 4 h at 37°C, cells that did not migrate were removed from the upper chamber with a cotton swab and cells on the opposite side of the membrane were fixed, stained, and quantified manually as described in the Materials and Methods. (A) Haptotaxis toward laminin-1; (B) chemotaxis toward NIH-3T3 conditioned medium; (C) dose response of MDA-MB-435 subclones 5B3 (β4 transfected; solid circles) and 6D7 (mock transfected; open squares) chemotaxis toward LPA; (D) Chemotaxis toward 100 nM LPA. Data are reported as fold increases over haptotactic migration on collagen I in the absence of LPA. Data (all panels) are shown as mean ± standard deviation from triplicate determinations.

The increased chemotaxis observed for the MDA/β4 transfectants in response to LPA was evident on both collagen I (Fig. 1, C and D) and laminin-1 (data not shown), indicating that 6β4-enhanced migration is independent of the matrix protein used for traction. This possibility was examined further by preincubating the MDA/β4 transfectants with function-blocking mAbs before their use in the chemotaxis assays. As shown in Fig. 2 A, inhibition of 6 integrin function with the mAb 2B7 did not block the chemotaxis of the MDA/β4 transfectants on collagen I towards LPA. However, this mAb inhibited the haptotaxis of MDA-MB-435 cells toward a laminin-1 gradient (Fig. 2 B), a process that is dependent on the 6β1 integrin (38). Chemotaxis toward LPA was inhibited completely, however, by preincubating the cells with the β1 integrin-specific mAb 13 (Fig. 2 A). Collectively, these data indicate that the stimulation of chemotaxis by expression of 6β4 can be independent of the adhesive functions of 6β4, and that the adhesive interactions required for 6β4-enhanced chemotaxis on collagen I are mediated through β1 integrins.

View larger version (45K): [in this window] [in a new window] [Download PPT slide]   Figure 2 Inhibition of 6β4-stimulated migration by integrin-specific antibodies. MDA/β4 (5B3; A, gray bars) or mock transfectants (6D7; B, stippled bars) were incubated with the indicated function blocking mAbs for 30 min before their use in a chemotaxis assay using 100 nM LPA on collagen I (A) or a haptotaxis assay on laminin-1–coated wells (B) as described in Fig. 1. Nonspecific mouse IgG was used as a negative control. Data are reported as the percentage of migration observed for the IgG control ± standard deviation from triplicate determinations.

Expression of the 6β4 Integrin Is Required for the Formation of Lamellae in Response to LPA

View larger version (77K): [in this window] [in a new window] [Download PPT slide]   Figure 3 The 6β4 integrin is required for the LPA-dependent formation of lamellae in MDA-MB-435 cells. MDA/β4 (A and B) and mock transfectants (C) were plated onto coverslips that had been coated with 20 µg/ ml collagen I. Cells were allowed to adhere for 2 h at 37°C and then treated with LPA for 5 min. (B and C) or left untreated (A). The cells were visualized using Nomarski DIC optics. Note the large lamellae that are formed in response to LPA stimulation of the MDA/β4 transfectants. (D) The effect of LPA on lamellar area was quantified using IPLab Spectrum imaging software. Data are shown as mean lamellar area ± standard error in which n > 20. Bar, 10 µm.

View larger version (17K): [in this window] [in a new window] [Download PPT slide]   Figure 4 Forskolin stimulation of adenyl cyclase inhibits LPA-mediated chemotaxis differentially in the MDA/β4 and mock transfectants. (A) MDA/β4 transfectants (5B3; solid circles) or mock transfectants (6D7; open squares) were treated with the indicated concentration of forskolin for 30 min before their addition to the upper wells of the Transwell chambers. Cells were assayed for LPA-mediated chemotaxis on collagen I as described in Fig. 1. The dashed line depicts the basal level of migration of both subclones in the absence of LPA. (B) In a separate experiment, the same cells were treated with forskolin for 30 min before assaying for LPA chemotaxis (solid symbols) or laminin haptotaxis (open symbols). Data are reported as the percent migration of cells not treated with forskolin ± standard deviation of triplicate determinations.

Expression of the 6β4 Integrin in MDA-MB-435 Cells Influences cAMP Metabolism

View larger version (47K): [in this window] [in a new window] [Download PPT slide]   Figure 5 Intracellular cAMP content of the MDA-MB-435 transfectants. The MDA/β4 (3A7, 5B3), MDA/β4-CYT (3C12, 1E10) and MDA/mock transfectants (6D2, 6D7) were plated in DME containing 10% FCS. After 18 h, cells were harvested and cAMP content was measured using a cAMP EIA protocol as described in Materials and Methods. Data shown represent the mean of 10 sample determinations ± standard error. The difference in the [cAMP]i between the MDA/β4 and the mock transfectants is significant (P < 0.001; asterisk), but the difference between the mock and the β4-CYT transfectants is not significant (P = 0.2). (B and C) Differential effects of forskolin stimulation on the [cAMP]i in the MDA/β4 and mock transfectants. The [cAMP]i was assayed in the 5B3 (solid bars) and 6D7 (stippled bars) clones plated on collagen I and treated for 15 min with either 50 µM forskolin (B) or forskolin and 1 mM IBMX (C). Note that the MDA/β4 transfectants (5B3) are more resistant to a forskolin-stimulated increase in [cAMP]i than the mock transfectants (6D7). The inhibition of PDE activity with IBMX shown in C reveals that 6β4 expression results in an increase in PDE activity and not a decrease in cAMP synthesis. Data shown are the mean values ± standard error obtained from multiple experiments.

To establish more directly that expression of the 6β4 integrin can regulate cAMP-dependent PDE activity, the activity of this enzyme was assayed in cell extracts obtained from the MDA/mock and β4 transfectants. As shown in Fig. 6 A, the MDA/β4 transfectants exhibited a significantly higher rate of PDE activity than the mock transfected cells. Moreover, the PDE activity of the MDA/ β4 transfectants was markedly increased (51% for 5B3 and 45% for 3A7) in response to forskolin stimulation compared with the mock transfectants (29% for 6D7; Fig. 6 A). The difference in PDE activity between the MDA/β4 and mock transfectants was eliminated by rolipram, a type IV PDE-specific (PDE 4) inhibitor (Fig. 6 B). These data indicate that a cAMP-dependent PDE 4 activity is influenced by 6β4 expression in MDA-MB-435 cells. Also, this activity is likely responsible for the observed decrease in [cAMP]_i and the resistance to forskolin-mediated inhibition of LPA chemotaxis observed in the MDA/β4 transfectants.

View larger version (92K): [in this window] [in a new window] [Download PPT slide]   Figure 6 Assay of cAMP-specific PDE activity. (A) MDA/β4 (3A7 and 5B3) or mock transfectants (6D7) plated on collagen I were treated with 50 µM forskolin or 100 nM LPA as noted. Cells were harvested and the cytosolic fraction was assayed for PDE activity as described in Materials and Methods. The PDE activity of the MDA/β4 transfectants was compared with the MDA/mock transfectants for statistical significance: *, P < 0.002; , P < 0.01. (B) Extracts from cells treated as in A were incubated with 100 µM rolipram before assaying for PDE activity to determine how much of the activity in A constitutes cAMP-specific PDE (PDE 4). Data shown are mean ± standard error of four separate determinations (A and B). ns, not significant; , P = 0.02. (C) Relative expression of PDE 4B in the MDA-MB-435 transfectants. Extracts (40 µg protein) obtained from the MDA/β4 (3A7 and 5B3) and mock (6D2 and 6D7) transfectants, as well as purified PDE 4 proteins (short form of variants A, B, and D; 10 ng each; provided by M. Conti) were resolved by SDS-PAGE and immunoblotted with a PDE 4B-specific Ab. Arrows, long and short forms of PDE 4B.

PDE Activity Is Necessary for Chemotaxis, Invasion, and Lamellae Formation
The importance of PDE for chemotactic migration was examined by treating the MDA/mock and β4 transfectants with IBMX before their use in the chemotaxis assay. As shown in Fig. 7 A, IBMX inhibited LPA-stimulated chemotaxis with maximal inhibition observed at 1 mM. Similar results were obtained with the cAMP-specific PDE inhibitor, rolipram (data not shown). We also examined the involvement of PDE in carcinoma invasion by treating cells with IBMX before their use in a standard Matrigel invasion assay. A substantial inhibition of invasion was observed in the presence of IBMX in comparison to the solvent control (Fig. 7 B).

View larger version (19K): [in this window] [in a new window] [Download PPT slide]   Figure 7 cAMP specific-PDE activity is required for the chemotactic migration and invasion of MDA-MB-435 cells. The MDA/ β4 (5B3; squares) or mock transfectants (6D7; circles) were treated with varying concentrations (A) or 1 mM (B) IBMX for 30 min before their use in either an LPA chemotaxis assay (A) or a Matrigel chemoinvasion assay (B). Data shown represent mean values ± standard deviation of triplicate determinations.

View larger version (38K): [in this window] [in a new window] [Download PPT slide]   Figure 8 cAMP specific-PDE activity is required for LPA-dependent formation of lamellae in the MDA/β4 transfectants. The MDA/β4 transfectants (5B3) were plated on collagen I–coated coverslips. After 2 h, the cells were either left untreated (A and C) or treated with 1mM IBMX (B and D) for 30 min. Subsequently, the cells were either left untreated (A and B) or treated with 100 nM LPA for 5 min (C and D). The cells were then fixed and visualized using Nomarski DIC optics. (E) The effect of LPA and IBMX on lamellar area was quantified using IPLab Spectrum imaging software. Bars represent mean lamellar area ± standard error in which n > 20. Of note, IBMX inhibited the LPA-dependent formation of lamellae by 70%.

View larger version (81K): [in this window] [in a new window] [Download PPT slide]   Figure 9 Lamellae formation in clone A colon carcinoma cells requires PDE activity. Clone A colon carcinoma cells were either treated with solvent alone (A and B) or 1 mM IBMX in solvent (C and D) and then plated on laminin-1–coated coverslips. After 45 min the cells were fixed and stained for F-actin using TRITC-phalloidin. (A and C) Phase–contrast images; (B and D) fluorescence images. Bar, 10 µm.

View larger version (41K): [in this window] [in a new window] [Download PPT slide]   Figure 10 (A) Evaluation of PI3-K involvement in PDE activity. The MDA/β4 transfectants were incubated for 30 min in the presence of either forskolin or wortmannin, or both in combination, before assay of PDE activity as described in Materials and Methods. (B) Evaluation of the cAMP regulation of PI3-K activity. The MDA/β4 and mock transfectants were incubated in suspension with either forskolin or IBMX or both for 10 min. Subsequently, these cells were either maintained in suspension or incubated with a β4 integrin-specific antibody and allowed to adhere to anti-mouse IgG-coated plates or laminin-1–coated plates for 30 min. Aliquots of cell extracts that contained equivalent amounts of protein were incubated with the anti-phosphotyrosine mAb 4G10 and protein A–Sepharose for 3 h. After washing, the beads were resuspended in kinase buffer and incubated for 10 min at room temperature. The phosphorylated lipids were resolved by thin layer chromatography. Arrows, position of the D3-phosphoinositides.

	Discussion

Top Abstract Materials and Methods Results Discussion References

Although integrins can regulate a number of signaling pathways (4), their ability to influence cAMP metabolism has not been studied extensively. An earlier study, however, did provide evidence that the simultaneous engagement of β2 integrins and tumor necrosis factor (TNF) receptors decreases the [cAMP]_i in neutrophils (30). Interestingly, the reduction in [cAMP]_i observed in response to β2 integrin and TNF receptor engagement in neutrophils is similar to the level of [cAMP]_i suppression that we observed in response to 6β4 expression (30%). This level of suppression of the total [cAMP]_i is quite impressive given that localized gradients of [cAMP]_i are probably required to facilitate chemotactic migration, as well as for other cell functions that are gated by cAMP. For example, localized gradients of cAMP have been implicated in regulating the direction of growth cone turning (41). It is also important to note that we observed an inverse correlation between the [cAMP]_i and the rate of chemotaxis (compare values in Fig. 4 A with Fig. 5 B). This observation reinforces the functional significance of 6β4 suppression of the [cAMP]_i.

A novel aspect of our study is the finding that integrins, and 6β4 in particular, can regulate the activity of a rolipram-sensitive, cAMP-specific PDE. This family of PDEs is defined as type IV PDE (PDE 4) and consists of a number of structural variants (6). Because all of these variants hydrolyze cAMP with a K_m comparable to the [cAMP]_i, it is thought that tissue-specific expression and the state of activity of these variants are the major determinants of their responsiveness to extracellular stimuli (6). Indeed, the major focus of work in this area has been hormonal regulation of PDE activity. Regulation of PDE activity can occur rapidly in response to hormone stimulation through a mechanism that involves PKA-dependent phosphorylation of the enzyme (36, 37). In addition, long-term, hormonal stimulation can actually increase de novo synthesis of the cAMP-specific PDEs (6, 43). The data we obtained suggest that expression of 6β4 does not increase the expression of PDE 4B, a predominant PDE variant expressed by MDA-MB-435 cells. For this reason, regulation of PDE 4 activity by 6β4 expression may occur through a mechanism that involves PDE phosphorylation. Another possibility that has been proposed recently is that the subcellular localization of the cAMP-specific PDEs influences their function and activation (17). The possibility that 6β4 increases the association of PDE 4 with either the plasma membrane or cytoskeleton is certainly attractive and could account, at least in part, for its ability to influence cAMP metabolism. Interestingly, LPA stimulation by itself had no effect on either PDE activity or the [cAMP]_i in MDA-MB-435 cells. This observation reinforces our hypothesis that a major function of 6β4 is to release cAMP gating of LPA-stimulated chemotaxis.

In previous studies, we established that an important function of 6β4 in invasive carcinoma cells is its ability to stimulate the formation of lamellae (32). This function of 6β4 is highlighted by the observation in the present study that LPA was able to induce significant lamellae formation only in MDA-MB-435 cells that expressed 6β4 (Fig. 3). Importantly, our finding that PDE activity is necessary for lamellae formation promoted by 6β4 expression implies that a localized suppression of the [cAMP]_i plays an important role in controlling the signaling and cytoskeletal events that are required for lamellae formation. This hypothesis agrees with studies that have shown an inhibitory effect of cAMP on the organization of the actin cytoskeleton (11, 13, 21, 22). Moreover, the formation of lamellae is a dynamic process that is linked to the mechanism of cell migration. Therefore, it is likely that temporal fluxes in the [cAMP]_i regulated by 6β4 contribute to the chemotactic migration of carcinoma cells.

Of particular relevance to our work, Butcher and colleagues (23) reported that cAMP is a negative regulator of leukocyte migration signaled through the classical chemoattractants. In this model, cAMP impedes or gates RhoA-mediated leukocyte integrin activation and adhesion. Our results support their conclusion that cAMP inhibits chemotactic migration. Importantly, we also provide evidence for an integrin-mediated mechanism of regulating the [cAMP]_i to facilitate migration. Our findings support the work of the Butcher group because LPA is a potent activator of Rho (29) and, in fact, we have observed that the expression of a dominant-negative Rho can inhibit both LPA-stimulated chemotactic migration and invasion of MDA-MB-435 cells (O'Connor, K.L., and A.M. Mercurio, unpublished observation). Thus, a possibility worth investigating is that LPA-mediated activation of Rho is gated by cAMP and that 6β4 releases cAMP gating by increasing cAMP-specific PDE activity and thereby enhances Rho activation. A likely target of Rho activation is the actin cytoskeleton (44), which is consistent with the reported effects of cAMP on the cytoskeleton (11, 13, 21, 22), as well as our demonstration that cAMP inhibits lamellae formation. Although Rho has been linked to stress fiber formation and not lamellae formation in fibroblasts (25), much less is known about Rho function in epithelial-derived cells. In fact, our preliminary data suggest that LPA-induction of lamellae formation in the MDA/β4 transfectants is inhibited by expression of a dominant-negative Rho. Other integrins, especially the β1 integrins that mediate the adhesive interactions required for chemotactic migration, are another potential target of Rho (25, 34). It is worth noting in this context that expression of 6β4 has been shown to alter the function of collagen I–binding integrins in breast carcinoma cells (42).

The ability of 6β4 to promote lamellae formation and carcinoma invasion is dependent upon its preferential activation of a PI3-K and Rac signaling pathway (40). Our current finding that the release of cAMP gating by 6β4 is also required for these events raised the issue of a possible link between cAMP and the PI3-K/Rac pathway. Such a link was suggested, for example, by the finding that the interleukin-2 dependent activation of PI3-K is inhibited by cAMP (28). In our experiments, however, pharmacological stimulation of cAMP levels had no effect on the ability of 6β4 to activate PI3-K even under conditions in which the [cAMP]_i increased 30-fold over basal levels. Our data also indicate that PI3-K probably does not function upstream of cAMP-specific PDE because wortmannin did not inhibit the activity of this enzyme. We conclude from these findings that PI3-K and cAMP-specific phosphodiesterase function in tandem to promote lamellae formation and chemotactic migration but they are components of distinct signaling pathways.

An interesting finding in the present study is that the ability of 6β4 to stimulate chemotactic migration and suppress the [cAMP]_i can be independent of the adhesive function of this integrin. Although the laminins are the only known matrix ligands for 6β4 (26), expression of this integrin also stimulated chemotactic migration on a collagen I matrix and this migration was not inhibited by an 6-function blocking mAb. The possibility that the effects of 6β4 expression on migration result from a decrease of 6β1 expression is discounted by the fact that expression of the 6β4 CYT integrin had no effect on either chemotaxis, cAMP levels or PDE activity even though expression of this mutant integrin eliminates 6β1 expression in these cells (38). The observation that the ability of 6β4 to promote chemotactic migration can be independent of its adhesive function is in agreement with several recent studies by our group and others that have revealed ‘ligand-independent' functions for the 6 integrins in carcinoma cells (3, 5, 8). Insight into the possible mechanism of this phenomenon was provided by a recent study that demonstrated self-association of the β4 cytoplasmic domains, a process that could initiate intracellular signaling events independently of ligand binding (33). One important implication of these findings is that the ability of 6β4 to influence cAMP metabolism and stimulate the chemotactic migration of carcinoma cells need not be limited to sites of contact with laminin-containing matrices. This possibility is supported by the numerous studies that have implicated 6β4 as a major determinant of carcinoma invasion and progression (10, 35, 47).

In summary, we have demonstrated that the 6β4 integrin can stimulate lamellae formation and chemotactic migration of invasive carcinoma cells by increasing the activity of a rolipram-sensitive cAMP specific-PDE and lowering the [cAMP]_i. This cAMP specific-PDE functions in tandem with a PI3-K/Rac pathway, that is also regulated by 6β4, and is required for carcinoma invasion and lamellae formation. The essence of our findings is that the 6β4 integrin stimulates the chemotactic migration of carcinoma cells through its ability to influence key signaling events that underlie this critical component of carcinoma invasion.

	Acknowledgments

 
This work was supported by grants from the United States Army Medical Research and Material Command to K. O'Connor (DAMD17-98-1-8033), L.M. Shaw (DAMD17-97-1-7313), and A.M. Mercurio (DAMD17- 96-1-6199) and a grant from the National Institutes of Health to A.M. Mercurio (CA-44704).

Submitted: 24 September 1998

Revised: 27 October 1998

We would also like to thank M. Conti and S. Iona (Stanford University, Stanford, CA) for their generous contribution of the PDE 4 antibodies, as well as S. Akiyama for the β1 integrin antibody. We also thank R. Falcioni, (Regina Elena Cancer Institute, Rome, Italy), R. Bachelder, I. Rabinovitz, and D. Senger (all three from Beth Israel Deaconess Medical Center, Boston, MA) for their comments and discussions regarding the manuscript.

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