Cell Culture

SCp2 cells and the mouse mammary carcinoma cell line SCg6 (Desprez et al., 1993; Lochter et al., 1977) were routinely maintained and passaged in serum-containing medium as described (Desprez et al., 1993). Selected clonal cell lines p2S6, p2S7, and p2S10, which inducibly expressed SL-1, and the cell line p2C, which was established in the same manner as the p2S cell lines but did not express the SL-1 transgene, were routinely grown in serum-containing medium with 100 μg/ml Geneticin and 4.8 μM Tet to maintain selection pressure and to silence transgene expression. The same medium, but without Tet, was also used for long-term induction of SL-1 for longer than 13 d.

All other experiments were performed in chemically defined medium consisting of DME/F12, 5 μg/ml insulin, 5 μg/ml transferrin, 5 ng/ml selenium (added as ITS medium supplement; Sigma Chemical Co.), and 50 μg/ml gentamicin with or without 4.8 μM Tet. In some experiments, a reconstituted basement membrane (Matrigel; Collaborative Biomedical Products, Bedford, MA) was added at a final concentration of 150–200 μg/ml (Streuli et al., 1995). To study milk protein expression, Matrigel and the lactogenic hormones prolactin (3 μg/ml; Sigma Chemical Co.), and hydrocortisone (1 μg/ml; Sigma Chemical Co.) were added for 6 or 7 d. The hydroxamic acid MMP inhibitor 3-(N-hydroxycarbamoyl)-2(R)-isobutylpropionyl-l-tryptophan methylamide (GM6001) and an inactive structural homologue (N-tert-butyloxycarbony)-l-leucine-l-tryptophan (GM1210) (gifts from Dr. R. Galardy, Glycomed Corporation, Alameda, CA) (Grobelny et al., 1992) were dissolved at a concentration of 100 mM in DMSO and added to the culture medium at a final concentration of 100 μM. GM6001 is a general inhibitor of all MMPs with dissociation constant of enzyme–inhibitor complexes (K _i) values <100 nM (Grobelny et al., 1992; Gijbels et al., 1994).

Conditioned medium was generated by incubating subconfluent cultures in 10-cm dishes with 5 ml of chemically defined medium for 2 d. Conditioned medium was then mixed at a 1:1 ratio with fresh culture medium before addition to SCp2 cells.

For indirect immunofluorescence, cells were plated at a density of 30,000 cells/cm² onto poly-l-lysine–treated glass coverslips as described (Lochter et al., 1997).

For coculture of SCp2 and p2S cells, both cell types were mixed at a 1:1 ratio, plated at a density of 30,000 cells/cm² onto poly-l-lysine–coated glass coverslips and maintained for 6 d in chemically defined medium. Before mixing the two cell types, SCp2 cells were labeled for 50 min at 37°C with 40 μg/ml of the lipophilic, red fluorescent dye, 1,1′-dioctadecyl-3,3,3′,3′-tetramethylindocarbocyanine perchlorate (DiI; Molecular Probes, Eugene, OR) in serum-containing medium with 1.6% ethanol as described (Honig and Hume, 1986).

Invasion assays were performed for 2–4 d in modified Boyden chambers (Collaborative Biomedical Products) coated with Matrigel as described (Lochter et al., 1997).

Analysis of Cellular Morphology and Indirect Immunofluorescence

For analysis of cellular morphology, cells were maintained for 12 d on glass coverslips, fixed, and then stained with toluidine blue as described (Lochter et al., 1991).

For indirect immunofluorescence, cells cultured on glass coverslips were fixed with methanol/acetone (1:1) for 15 min at −20°C, washed twice with PBS, and then blocked by incubation with 15% FBS in PBS for 1 h at ambient temperature. Cells were then reacted for 1 h at ambient temperature with mouse monoclonal antibody against E-cadherin (C20820) (1:100 dilution; Transduction Laboratories, Lexington, KY), mouse monoclonal antibody against β-catenin (1:100 dilution; Transduction Laboratories), mouse monoclonal antibody against vimentin (1:200 dilution; Sigma Chemical Co.), or rabbit polyclonal antibody cocktail against cytokeratins (1:20 dilution; Dako Corp., Carpintera, CA) in 15% FBS in PBS. After three washes with PBS, cells were incubated at ambient temperature for 30 min with Texas red–conjugated, goat anti–mouse IgG (Caltag Laboratories, Burlingame, CA) or donkey anti–rabbit IgG (Amersham Corp., Arlington Heights, IL) antibodies, or FITC-conjugated, goat anti–mouse IgG (Caltag Laboratories), or donkey anti–rabbit IgG (Amersham Corp.) antibodies, all at a 1:100 dilution in 15% FBS in PBS. Cells were then washed twice with PBS, incubated with 4′,6-diamidino-2-phenylindole (DAPI) for 1 min to visualize nuclei, and washed two more times with PBS and once with water before mounting with Vectashield (Vector Laboratories, Inc., Burlingame, CA).

For immunofluorescence analysis of cocultured SCp2 and p2S cells, cells were permeabilized for 30 s with digitonin and fixed as described (Crowley and Horwitz, 1995). This procedure insured that cells were permeabilized without removing DiI from cell membranes. Subsequent immunostaining was performed as described above.

Zymograms, Immunoblots, and Immunoprecipitations

For zymograms on conditioned medium, subconfluent cells maintained in 10-cm dishes were preinduced to express SL-1 for 1 d. 5 ml of chemically defined medium was then added to the cells, collected 2 d later, and concentrated 20-fold with Centricon filter units (Amicon Corp., Danvers, MA) according to the manufacturer's instructions. Casein and gelatin zymography was subsequently performed as described (Fisher and Werb, 1995; Lochter et al., 1997). Identification of all gelatinolytic bands shown in Fig. ​Fig.77 as MMPs (not shown) was achieved by incubation of gels with 1,10-phenanthroline and GM6001 (Fisher and Werb, 1995).

Open in a separate window

Figure 7

Activation and induction of endogenous MMPs by SL-1. Negative images of gelatin zymograms of medium conditioned by SCp2, p2C, p2S7, and p2S10 cells maintained for 3 d in the presence (+) or absence (−) of Tet. Positions of molecular mass markers are indicated.

For immunoblots, cells grown in 10-cm dishes were lysed with radioimmunoprecipitation assay (RIPA) buffer (30 mM NaCl, 50 mM Tris-HCl, pH 7.4, 5 mM ethylenediamine tetraacetic acid, 1% NP-40, 1% deoxycholic acid, 0.1% SDS) containing 20 μg/ml aprotinin (Sigma Chemical Co.) and 1 mM 4-(2-aminoethyl)benzenesulonylfluoride (Calbiochem-Novabiochem Corp., La Jolla, CA). Extraction of cells with Triton X-100 was performed as described (Näthke et al., 1994). Samples containing 10 μg of protein were separated on 8% SDS–polyacrylamide slab gels under reducing conditions (Laemmli, 1970) and transferred onto Immobilon-P membranes (Amersham Corp.). Membranes were then blocked for 1 h with TBST (50 mM Tris, pH 7.5, 100 mM NaCl, 0.1% Tween 20) containing 5% skim milk powder, and then incubated for 1 h at ambient temperature with monoclonal antibody against E-cadherin (C20820; 1:5,000 dilution) or β-catenin (1:5,000 dilution) in the same solution. Blots were then washed with TBST and treated with horseradish peroxidase–conjugated, sheep anti–mouse IgG antibodies (Amersham Corp.) in 5% skim milk powder in TBST. Bands were visualized with an enhanced chemiluminescence detection kit (Amersham Corp.) according to the manufacturer's instructions. For immunoblots for detection of β-casein, RIPA extracts from an equivalent of 10⁵ cells were resolved on 12% SDS–polyacrylamide gels and 4% BSA was used as a blocking reagent. β-casein was detected with a rabbit polyclonal antibody against mouse milk proteins followed by horseradish peroxidase–conjugated, donkey anti–rabbit IgG antibodies (1:1,500 dilution; Amersham Corp.). Immunoblots with mouse monoclonal antibody HA.11 directed against the hemagglutinin epitope tag (1:50 dilution, BAbCO, Richmond, CA) were performed on medium conditioned for 1 or 2 d by an equivalent of 10⁶ cells.

Immunoprecipitations on cell lysates were carried out with cells that had been metabolically labeled for 16 h with 200 μCi [³⁵S]methionine (Amersham Corp.) per ml culture medium. For biotinylation of cell surface proteins, cells were washed three times with PBS and once with Hepes-buffered saline (135 mM NaCl, 5 mM KCl, 0.5 mM Na₂HPO₄, 10 mM Hepes, pH 7.5) after radiolabeling. Cells were then incubated for 1 h at 4°C with 100 μg/ml Sulfo-NHS-Biotin (Pierce Chemical Co., Rockford, IL) in Hepes-buffered saline. Radiolabeled cells that were or were not cell surface biotinylated were washed three times with chemically defined medium, and then lysed in NP-40 lysis buffer (150 mM NaCl, 50 mM Tris, pH 7.5, 1% NP-40). Antibodies to integrin subunits β1, β4, and α6 (all from PharMingen, San Diego, CA), antibody to the extracellular domain of E-cadherin (ECCD-2) (a gift from Dr. Takeichi, Kyoto University, Kyoto, Japan [Shirayoshi et al., 1986]), and antibody C20820 to the cytoplasmic domain (Transduction Laboratories) were added to cell lysates at a final concentration of 10 μg/ml, and then incubated overnight at 4°C. Subsequently, protein G–agarose (Sigma Chemical Co.) was added and incubation was carried out for 1 h at 4°C. Protein G–agarose beads were washed three times with NP-40 lysis buffer and twice with 50 mM Tris, pH 7.5. Immunoprecipitants were separated on 5% SDS–polyacrylamide gels under nonreducing conditions for integrins, or on 8% SDS–polyacrylamide gels under reducing conditions for E-cadherin. Gels were either dried and processed for autoradiography, or blotted onto Immobilon-P membranes, blocked with 5% skim milk in TBST, and then incubated with peroxidase-conjugated streptavidin (1:100 dilution; Amersham Corp.) before detection of biotinylated proteins with the ECL detection system. For detection of E-cadherin cleavage products released from SCp2 cells by conditioned medium from p2S cells, SCp2 cells were incubated with conditioned medium for 12 h at 37°C. The culture medium was then supplemented with BSA at a final concentration of 1 mg/ml and processed for immunoprecipitation as described above.

ELISA

Cells were plated at a density of 6,000 cells per well into 96-well plates. After designated culture periods, cells were fixed with methanol/acetone (1:1) for 15 min at −20°C and washed twice with PBS. Plates were then incubated for 1 h at ambient temperature with 15% FBS in PBS and subsequently for 1 h at ambient temperature with polyclonal antibody against cytokeratins (1:1,000 dilution), mouse monoclonal antibody against E-cadherin (1:5,000 dilution; C20820), mouse monoclonal antibody against β-catenin (1:5,000 dilution), or mouse monoclonal antibody against γ-catenin (1: 5,000 dilution; Transduction Laboratories). After three washes with PBS, plates were incubated for 1 h at ambient temperature with horseradish peroxidase–conjugated, donkey anti–rabbit IgG antibodies (1:2,500 dilution; Amersham Corp.) or sheep anti–mouse IgG antibodies (1:2,500 dilution; Amersham Corp.) in PBS containing 15% FBS. Plates were then washed six times with PBS and developed with 100 μl/well 1 mg/ml azino-bis-ethylbenzthiazolinesulfonic acid, and 0.1 μl/ml H₂O₂ in 100 mM sodium acetate, 50 mM sodium phosphate, pH 4.2, for 30 min at 37°C. Absorbance was measured at 405 nm.

SL-1 Triggers Cleavage of E-cadherin and Regulates β-Catenin Expression

Because cell scattering and invasion requires dissolution of stable cell–cell contacts (for review see Birchmeier et al., 1996; Gilles and Thompson, 1996), we examined whether SL-1 affected cell–cell adhesion systems maintained by the major epithelial adhesion molecule E-cadherin. Both E-cadherin and its intracellular binding partner β-catenin were present at cell–cell contacts in p2S cells maintained in the presence of Tet (Fig. ​(Fig.2,2, a and b). However, by 6 d after induction of SL-1 there was a marked decrease in both of these molecules at cell–cell junctions (Fig. ​(Fig.2,2, a and b). SL-1 disrupted the integrity of cell–cell junctions in cells maintained both in the absence and presence of Matrigel (Fig. ​(Fig.2,2, a and b). E-cadherin and β-catenin localization at sites of cell–cell contact was unaffected by Tet in control SCp2 and p2C cells (not shown).

Open in a separate window

Figure 2

Subcellular localization of E-cadherin and β-catenin after SL-1 induction. (a–b) P2S10 cells were maintained for 6 d in the absence (a) or presence (b) of Matrigel and in the presence (+ Tet) or absence (− Tet) of Tet. Cells were analyzed by indirect immunofluorescence for distribution of E-cadherin and β-catenin (red in a, green in b). Cells were counterstained with DAPI to visualize nuclei (blue). (c) SCp2 cells were labeled with DiI (red) and cocultured with p2S10 cells for 6 d in the presence (+ Tet) or absence (− Tet) of Tet. Cells were then permeabilzed with digitonin, fixed, and then immunostained for E-cadherin (green). Cells were counterstained with DAPI (blue). Bars: (a and b) 10 μM; (c) 25 μm.

To exclude the possibility that the effects observed with SL-1 were observable only in the p2S cell clones selected, SCp2 cells were labeled with the lipophilic red fluorescent dye DiI and cocultured with p2S cells in the absence of Tet on tissue culture plastic. E-cadherin (Fig. ​(Fig.22 c) and β-catenin (not shown) immunofluorescence was dramatically reduced after brief detergent extraction in both the SCp2 cells that did not express the SL-1 transgene and p2S cells that expressed SL-1. Thus, the phenotypic alteration induced by SL-1 was not cell autonomous and could also be induced in trans. Furthermore, these data show that the effects of SL-1 are because of its extracellular activity.

We observed an increased detergent solubility of E-cadherin and β-catenin in cells exposed to SL-1, which suggests a reduced association with the cytoskeleton (Näthke et al., 1994). Total E-cadherin protein, as determined by immunoblotting, was not altered, but the Triton X-100– resistant, E-cadherin pool was greatly diminished upon SL-1 induction in p2S cells for 6 d (Fig. ​(Fig.3).3). For β-catenin, both total and Triton X-100–resistant pools were reduced 6 d after induction of SL-1 (Figs. ​(Figs.33 and ​and44 a). This reduction in β-catenin levels required the proteolytic activity of SL-1, because it was prevented by GM6001, but not by its inactive structural homologue GM1210 (Fig. ​(Fig.44 b). A significant reduction of β-catenin levels occurred first 4 d after SL-1 induction (Fig. ​(Fig.44 a and not shown). When p2S cells were maintained in the presence of Matrigel, β-catenin expression also decreased as a result of SL-1 induction, albeit to a lesser extent than in the absence of Matrigel (Fig. ​(Fig.44 a). Results similar to β-catenin were obtained also for γ-catenin (Fig. ​(Fig.44 a; and not shown). With prolonged induction of SL-1 in p2S cells by culture for 2 mo on tissue culture plastic without Tet, β-catenin levels declined further and E-cadherin expression was repressed (Fig. ​(Fig.4,4, a and c).

Open in a separate window

Figure 3

Total and cytoskeleton-associated E-cadherin and β-catenin after SL-1 induction. P2C, p2S7 and p2S10 cells were cultured for 6 d on tissue culture plastic in the presence (+) or absence (−) of Tet. They were then either directly lysed in RIPA buffer (total) or briefly extracted with Triton X-100 before cell lysis in RIPA buffer (TX-100-resistant) before analysis of expression of E-cadherin and β-catenin by immunoblotting.

Open in a separate window

Figure 4

Expression of E-cadherin and β-catenin in p2S cells cultured in the absence and presence of Matrigel. (a) Quantification of E-cadherin (○), β-catenin (), and γ-catenin () expression by ELISA on p2S10 cells maintained on plastic and induced to express SL-1 for 2, 4, and 6 d (2d, 4d, and 6d) or 2 mo (2m), or on p2S10 cells induced to express SL-1 for 6 d in the presence of Matrigel. Results are expressed as percent increase or decrease in expression of cells maintained in the absence of Tet as compared to cells maintained in the presence of Tet. Means and standard deviations from three independent experiments are shown. (b) Quantification of β-catenin expression by ELISA on p2C (white bars), p2S7 (gray bars), and p2S10 (black bars) cells maintained on tissue culture plastic for 6 d in the presence (+ Tet) or in the absence (− Tet) of Tet with no further additives (none) or with GM6001 or its inactive homologue GM1210. Results are normalized with expression levels obtained in the presence of Tet set to 100. Means and standard deviations from three independent experiments are shown. (c) Immunoblots for total E-cadherin (E-cad) and β-catenin (β-cat) expressed by p2C and p2S10 cells maintained for 6 d (6d) or 2 mo (2m) in the presence (+) or absence (−) of Tet. (d) [³⁵S]methionine-labeled SCp2 cells were treated for 12 h with conditioned medium from p2S10 cells induced (− Tet) or not induced (+ Tet) to express SL-1 for 6 d. The conditioned medium from p2S10 cells maintained without Tet was either supplemented (+ GM) or not supplemented (− GM) with GM6001. E-cadherin was subsequently immunoprecipitated from the cell culture medium with a monoclonal antibody against the extracellular (ECCD-2) or intracellular (C20820) domain of E-cadherin. The amount of cleaved E-cadherin detected in the medium, however, constituted only a minor part of the total E-cadherin produced by p2S cells (not shown). (e) Cell surface proteins of [³⁵S]methionine-labeled p2S10 cells maintained for 6 d in the presence of Tet (6d +), or for 6 d (6d −), or 2 mo (2m −) in the absence of Tet were biotinylated, immunoprecipitated with antibodies against E-cadherin, and then visualized with peroxidase-conjugated streptavidin (cell surface). Autoradiograms of total immunoprecipitated E-cadherin protein (total), on the same membranes as used for immunoblotting, are shown for comparison.

Because MMPs have cell surface substrates in addition to ECM substrates, we asked whether proteolytic removal of the extracellular domain of E-cadherin by SL-1 occurred. Indeed, after exposure of SCp2 cells to medium conditioned by p2S cells maintained in the absence of Tet, soluble 95- and 80-kD fragments reacting with ECCD-2 were recovered from the medium (Fig. ​(Fig.44 d). Consistent with this finding, cell surface E-cadherin was slightly reduced in p2S cells induced to produce SL-1 for 6 d (Fig. ​(Fig.44 e). E-cadherin cleavage did not occur in the presence of GM6001, indicating that E-cadherin is either a direct substrate of SL-1 or that SL-1 activates or induces other MMPs that could degrade E-cadherin. A 40-kD form of E-cadherin was precipitated from the medium regardless of whether SL-1 was induced or not (Fig. ​(Fig.44 d).

Cell–ECM contacts are also altered during epithelial cell scattering (for review see Adams and Watt, 1993; Gilles and Thompson, 1996). We therefore examined the impact of SL-1 on expression of integrin subunits β1, β4, and α6, which have been implicated in functional differentiation of mammary epithelial cells (Streuli et al., 1991; Boudreau et al., 1995; Weaver et al., 1997). The α6 integrin subunit was selectively coimmunoprecipitated with β4, but not with β1, indicating that p2S cells expressed α6β4, but not α6β1 integrin (Fig. ​(Fig.55 a), whether SL-1 was induced or not. Expression of total β1, β4, and α6 was not altered by SL-1, even after 2 mo of induction (Fig. ​(Fig.55 a). However, there was a reproducible, transient modulation in cell surface expression of the α6 integrin subunit that appeared to be decreased at day 6 after SL-1 induction, but not 2 mo after SL-1 induction (Fig. ​(Fig.55 b). Thus, integrin alterations appeared to be minor, whereas E-cadherin biochemistry changed dramatically after SL-1 induction.

Open in a separate window

Figure 5

Effect of SL-1 induction on expression of integrins. (a) Cell lysates of [³⁵S]methionine-labeled p2S10 cells maintained for 6 d in the presence of Tet (6d +), or for 6 d (6d −), or 2 mo (2m −) in the absence of Tet were immunoprecipitated with antibodies against integrin subunits β1, β4, and α6. Positions of molecular mass markers of 220, 97.4, and 66 kD are indicated. (b) Cell surface proteins of [³⁵S]methionine-labeled p2S10 cells maintained for 6 d in the presence of Tet (6d +), or for 6 d (6d −), or 2 mo (2m −) in the absence of Tet were biotinylated, immunoprecipitated with antibodies against integrin subunits β4 and α6, and visualized with peroxidase-conjugated streptavidin (cell surface). Autoradiograms of total immunoprecipitated β4 and α6 protein (total), on the same membranes as used for immunoblotting, are shown for comparison.

SL-1 Induction Leads to Alterations in Expression of Intermediate Filament Cytoskeleton Proteins

Epithelial cells that are migratory and invasive often downregulate their expression of cytokeratins and upregulate vimentin (for review see Birchmeier et al., 1996; Gilles and Thompson, 1996). The p2S cells contained cytokeratin intermediate filaments in the presence of Tet, and did not express vimentin (Fig. ​(Fig.6,6, a and b). Upon induction of SL-1, p2S cells began to express vimentin, even when cultured with Matrigel (Fig. ​(Fig.6,6, a and b). Some cells expressed vimentin alone, whereas others coexpressed vimentin with various levels of cytokeratins (Fig. ​(Fig.6,6, a and b), suggesting dual expression of vimentin and cytokeratins during transition to the complete loss of cytokeratins. In p2S cells that were maintained on tissue culture plastic and induced to express SL-1 for 6 d, cytokeratin expression decreased to ~50% of control, as measured by ELISA assay (Fig. ​(Fig.66 c). Furthermore, ~30% of the cells became vimentin positive, as determined by counting the number of cells reacting with antibodies against vimentin (Fig. ​(Fig.66 d). Addition of GM6001 at the time of Tet removal inhibited this phenotypic transition (not shown). After 2 mo of SL-1 induction, ~80% of the cells were vimentin positive, whereas total cytokeratin expression decreased to 15% of control levels (Fig. ​(Fig.6,6, c and d). The transition from a cytokeratin cytoskeleton to a vimentin cytoskeleton in p2S cells occurred even in the presence of a basement membrane, albeit more slowly. When Tet was removed for 6 d in cultures containing Matrigel, ~15% of the cells became vimentin positive, and total cytokeratin expression decreased to ~70% of control levels (Fig. ​(Fig.6,6, c and d). Taken together these results show that, both in the presence and absence of a basement membrane, SL-1 induction leads to inhibition of expression of epithelial cytokeratins concomitant with expression of the mesenchymal intermediate filament protein vimentin.

Open in a separate window

Open in a separate window

Open in a separate window

Open in a separate window

Figure 6

Effect of SL-1 induction on cytokeratin and vimentin expression. (a–b) P2S10 cells were maintained for 6 d in the absence (a) or presence (b) of Matrigel and in the presence (+ Tet) or absence (− Tet) of Tet. Cells were analyzed by indirect immunofluorescence for expression of cytokeratins (red) and vimentin (green). Cells were counterstained with DAPI (blue) to visualize nuclei. Note that in the presence of Matrigel most cells are round and form multicellular aggregates. (c) Quantification of cytokeratin expression by ELISA on p2C (•), p2S7 (), and p2S10 () cells maintained on plastic and induced to express SL-1 for 2, 4, and 6 d (2d, 4d, and 6d), or 2 mo (2m), or on cells maintained in the presence of Matrigel for 6 d. Results are expressed as the percent increase or decrease in cytokeratin expression of cells maintained in the absence of Tet as compared to cells maintained in the presence of Tet. Means and standard deviations from three independent experiments are shown. (d) Quantification of the number of vimentin expressing p2C (circles), p2S7 (triangles) and p2S10 (squares) cells maintained on plastic or in the presence of Matrigel, and induced (black symbols) or not induced (white symbols) to express SL-1 for the times indicated above. Results are expressed as the percentage of cells displaying vimentin immunoreactivity. Means and standard deviations from three independent experiments are shown.

SL-1 Alters Endogenous MMPs and Induces KGF Expression in p2S Cells

The observation that SL-1 induced a cascade of apparent epigenetic changes in p2S cells, characterized by induction of vimentin and downregulation of cytokeratins and β-catenin, raises the question of whether the regulation of other genes important for mammary epithelial function also changed in response to SL-1 action. Because a SL-1 transgene induces endogenous MMP expression in mice (Alexander et al., 1996), and inhibition of SL-1 expression in mammary carcinoma cells also reduces the synthesis of other MMPs (Lochter et al., 1997), we first determined whether other MMP activities were altered after SL-1 induction. We observed that endogenous gelatinase B was activated as early as 3 d after removal of Tet from the culture medium (Fig. ​(Fig.7).7). Moreover, additional gelatinolytic bands of 58 and 51 kD were upregulated, the latter corresponding to the molecular weight of collagenase-3 (Fig. ​(Fig.7).7). Interestingly, endogenous SL-1 was a late gene induced by the SL-1 transgene, not present at day 6, but appearing between 2 and 8 wk after SL-1 induction (not shown).

Cell scattering and loss of E-cadherin–mediated cell adhesion can be induced in other types of epithelial cells by growth factors such as KGF, HGF, and transforming growth factor-β (TGF-β) (Weidner et al., 1990; Miettinen et al., 1994; Savagner et al., 1994; Kitagawa et al., 1996). We therefore asked whether the SL-1–induced scattering and dedifferentiation are secondary to an induction of these scattering and/or dedifferentiation factors. If this were the case, the conditioned medium from p2S cells induced to express SL-1 should contain factors that could lead to a loss of differentiation in SCp2 cells even when MMP function is inhibited by GM6001. Consistent with the coculture experiment (Fig. ​(Fig.22 c), treatment of SCp2 cells for 6 d with medium conditioned by p2S cells generated in the absence of Tet for 6 d, resulted in reduction of β-catenin and cytokeratin levels (Fig. ​(Fig.88 a). Significantly, these alterations were also observed, albeit to a lesser extent, when the experiment was performed in the presence of GM6001 (Fig. ​(Fig.88 a), suggesting that SL-1 induces secreted factors that are not themselves MMPs. We thus determined whether KGF, HGF, or TGF-β were produced by p2S cells. Neither KGF nor HGF mRNA was expressed by p2S cells cultured in the presence of Tet (Fig. ​(Fig.88 b). In contrast, expression of SL-1 for 3 d led to induction of KGF, but not HGF mRNA (Fig. ​(Fig.88 b). TIMP2 mRNA, which was used as a positive control in this assay, was unchanged. KGF mRNA expression was maintained in cells induced to express SL-1 for 2 mo (Fig. ​(Fig.88 b). However, recombinant KGF, alone, was unable to alter β-catenin or cytokeratin expression in p2S or SCp2 cells (not shown), suggesting that additional factors were needed for the effects observed with conditioned medium. TGF-β, as measured by the mink lung cell assay, was secreted in a latent form by p2S cells (not shown). Total amounts of secreted TGF-β or its activation were not significantly altered by SL-1 expression (not shown). Taken together, these data indicate that the regulation of at least one growth factor gene (KGF) is downstream from SL-1 action, but that KGF alone is not sufficient for the phenotypic conversion observed.

Open in a separate window

Open in a separate window

Figure 8

Induction of KGF by induction of SL-1. (a) Quantification of cytokeratin (keratin) and β-catenin expression by ELISA on SCp2 cells that had been incubated for 6 d with medium conditioned by p2C (white bars), p2S7 (gray bars), or p2S10 (black bars) cells maintained in the presence (+ Tet) or absence (− Tet) of Tet. GM6001 or GM1210 were added or not added (none) to conditioned medium from cells maintained in the absence of Tet. Results are expressed as the percent increase or decrease in cytokeratin or β-catenin expression compared to SCp2 cells maintained with conditioned medium from p2C cells cultured in the presence of Tet. Means and standard deviations from three independent experiments are shown. (b) Southern hybridization of RT-PCR products obtained with primers specific for HGF, KGF, or TIMP2 on total RNA prepared from p2C, p2S7, and p2S10 cells maintained for 3 days in the presence of Tet (3d +), or 3 d (3d −) or 2 months (2m −) in the absence of Tet, or from the mouse mammary carcinoma cell line SCg6 (g6).

We are grateful to D. Lam for excellent technical assistance, and to F. Wang, R. Schwarz, and D. Callaghan for helpful technical advice.

This work was supported by funds from the U.S. Department of Energy, Office of Health and Environmental Research (contracts DE-AC03-76-SF00098 and DE-AC03 76-SF01012), and the National Cancer Institute (grant CA 57621), by the Institutional National Research Service Award (5T32 ES07106) (to S. Galosy), and by postdoctoral fellowships from the European Molecular Biology Organization and the California Breast Cancer Research Program (to A. Lochter), and the National Institutes of Health (to J. Muschler).