Hepatocyte Growth Factor Releases Mink Epithelial Cells from Transforming Growth Factor beta 1-Induced Growth Arrest by Restoring Cdk6 Expression and Cyclin E-Associated Cdk2 Activity

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Molecular and Cellular Biology, May 1999, p. 3654-3663, Vol. 19, No. 5
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Hepatocyte Growth Factor Releases Mink Epithelial Cells from Transforming Growth Factor $beta$ 1-Induced Growth Arrest by Restoring Cdk6 Expression and Cyclin E-Associated Cdk2 Activity

Minna Tsubari, Jussi Taipale, Erja Tiihonen, Jorma Keski-Oja, and Marikki Laiho^*

Department of Virology, Haartman Institute, University of Helsinki, Helsinki, Finland

Received 22 May 1998/Returned for modification 14 July 1998/Accepted 22 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Transforming growth factor $beta$ (TGF- $beta$ ) potently suppresses Mv1Lu mink epithelial cell growth, whereas hepatocyte growth factor(HGF) counteracts TGF- $beta$ -mediated growth inhibition and inducesMv1Lu cell proliferation (J. Taipale and J. Keski-Oja, J. Biol.Chem. 271:4342-4348, 1996). By addressing the cell cycle regulatorymechanisms involved in HGF-mediated release of Mv1Lu cells fromTGF- $beta$ inhibition, we show that increased DNA replication is accompaniedby phosphorylation of the retinoblastoma protein and alternativeregulation of cyclin-Cdk-inhibitor complexes. While TGF- $beta$ treatmentdecreased the expression of Cdk6, this effect was counteractedby HGF, followed by partial restoration of cyclin D2-associatedkinase activity. Notably, HGF failed to prevent TGF- $beta$ inductionof p15 and its association with Cdk6. However, HGF reversed theTGF- $beta$ -mediated decrease in Cdk6-associated p27 and cyclin D2-associatedCdk6, suggesting that HGF modifies the TGF- $beta$ response at the levelof G₁ cyclin complex formation. Counteraction of TGF- $beta$ regulationof Cdk6 by HGF may in turn affect the association of p27 withCdk2-cyclin E complexes. Though HGF did not differentially regulatethe total levels of p27 in TGF- $beta$ -treated cells, p27 immunodepletionexperiments suggested that upon treatment with both growth factors,less p27 is associated with Cdk2-cyclin E complexes, in parallelwith restoration of the active form of Cdk2 and the associatedkinase activity. The results demonstrate that HGF intercepts TGF- $beta$ cell cycle regulation at multiple points, affecting both G₁ andG₁-S cyclin kinaseactivities.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Cell cycle progression of eukaryotic cells is controlled by sequential activation of cyclin-cyclin-dependent kinase (Cdk)complexes. Formation of complexes and regulation of their activityis highly specific, and distinct complexes drive cell cycle progressionin the G₁ (cyclins D1 to D3 in complex with Cdk4 or Cdk6), G₁-S,and S phases (cyclin E-Cdk2 and cyclin A-Cdk2 or -cdc2) and inmitosis (cyclin B-cdc2) (32, 37, 44). Cdk's are activatedby association of the cyclin subunit and by stimulatory phosphorylationof a conserved threonine residue (Thr¹⁶⁰ in Cdk2) by Cdk-activating kinase (CAK) (9, 13, 35, 48).A steric model of the Cdk2-cyclin A complex indicates that associationof the cyclin subunit with the kinase leads to reorientation ofthe catalytic cleft and reveals the Thr¹⁶⁰ phosphorylation site (19). In addition, activation of the kinaserequires dephosphorylation of an inhibitory tyrosine residue bycdc25 phosphatase (11, 30). Kinase activity is negativelyregulated by cyclin-dependent kinase inhibitors (CDKIs). CDKIshave been grouped into two families related to p21^Cip1/Waf1 and p16^Ink4a/MTS1 (12, 46). In contrast to p16 family members (p15, p16, p18,and p19), which associate only with the Cdk's, the members ofthe p21 family (p21, p27, and p57) associate with both cyclinand Cdk subunits (15). The crystal structure of Cdk2-cyclinA in complex with p27 indicates that p27 binds to the catalyticcleft of Cdk2, thus inactivating the kinase (42). Of the CDKIs,p21, p27, and p15 are regulated by growth factors (7, 16,25, 39).

One of the targets of the Cdk complexes in G₁-S-phase transition is the retinoblastoma tumor suppressor protein, pRb (21).pRb, and its relatives p107 and p130, bind to and inhibit theE2F family of transcription factors (52). They also directlyinteract with and regulate the activity of cyclin E-Cdk2 complexes(55). Binding sites for E2F have been found in several genesessential for cell cycle progression from G₁ to S phase (44).The activity of pRb is regulated by its phosphorylation status,and the hypophosphorylated form of pRb associates with E2F. Inlate G₁ phase, pRb is phosphorylated by cyclin D- and cyclin E-dependentkinases (45, 52), and these phosphorylations induce the dissociationof pRb from E2F and allow transcription of genes required forprogression into Sphase.

Transforming growth factor $beta$ 1 (TGF- $beta$ 1) is a member of large family of growth factors involved in regulation of cellular growthand differentiation (21, 50). TGF- $beta$ is the only known growthfactor that reversibly arrests the growth of epithelial, endothelial,and hematopoietic cells in the G₁ phase of the cell cycle withoutpermanently differentiating them. TGF- $beta$ treatment of mink lungepithelial cells prevents efficiently the phosphorylation of pRb(24). Inhibition of pRb phosphorylation by TGF- $beta$ is a resultof complex regulation of the activities of Cdk's and their inhibitors.TGF- $beta$ increases the expression of p15, which binds Cdk4/6-cyclinD complexes (16). Binding of p15 to Cdk4/6-cyclin D complexesleads to dissociation of p27 from these complexes and subsequentbinding of p27 to Cdk2-cyclin E complexes and results in G₁ growtharrest (40, 41). Concomitantly, TGF- $beta$ reduces the amount ofthe active, faster-migrating form of Cdk2 (22). TGF- $beta$ preventsalso the association of cyclin D1 with Cdk4, apparently by upregulationof p15 in human mammary epithelial cells (43). In addition,inhibition of Cdk activity by TGF- $beta$ is suggested to be mediatedby a decrease in the level of Cdk4 in Mv1Lu cells (10) and incdc25A Cdk-activating phosphatase in p15-deficient mammary epithelialcells (18).

Hepatocyte growth factor (HGF) is derived from mesenchymal cells and acts as a growth stimulator for epithelial cells. Inaddition, HGF stimulates the motility and invasiveness of epithelialand endothelial cells (2, 4, 31). We have previously shownthat HGF releases epithelial and endothelial cells from TGF- $beta$ -inducedgrowth arrest (49). To address the underlying mechanisms, wehave analyzed the effects of TGF- $beta$ and HGF on the cellular levelsof Cdk's, cyclins, their specific inhibitors, and complex formationin Mv1Lu mink lung epithelial cells. We find here that HGF relievesTGF- $beta$ -mediated growth arrest by inhibition of TGF- $beta$ -mediated downregulationof Cdk6. These events lead to expression of Cdk6-cyclin D2 complexesat levels comparable to those in control cells and partial rescueof cyclin D2-associated kinase activity. Despite induction ofp15 and relocalization of p27 inhibitor to Cdk6 and Cdk2 complexes,respectively, Cdk2-cyclin E-associated kinase activity is fullyrecovered in cells treated with both growth factors. Our datasuggest that in cells treated with both growth factors, only asubpopulation of Cdk6 is inactivated by binding to p15, whilethe rest of Cdk6 remains in complex with cyclin D2 or cyclin D2-p27,thus possibly harvesting a part of p27 from that that forms complexeswith Cdk2 and cyclin E. The decrease in the available p27 resultsin activation of Cdk2-cyclin E complexes sufficient for cellproliferation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and reagents. Mv1Lu mink lung epithelial cells (CCL-64; American Type Culture Collection, Manassas, Va.) were grown in Dulbecco's modifiedEagle medium (DMEM) containing 10% fetal calf serum (FCS) (Gibco-BRL,Rockville, Md.). In all assays, except when otherwise stated,the cells were treated with 100 pM TGF- $beta$ 1, 220 pM HGF, or bothin DMEM containing 10% FCS for 16 h. TGF- $beta$ 1 was purified fromoutdated human platelets (51), and recombinant human HGF waspurchased from R&D Systems (Minneapolis, Minn.). 5-Bromo-2'-deoxyuridine(5-BrdUrd) was purchased from Sigma (St. Louis, Mo.).

Antibodies. Antibodies used in immunoblotting assays for Cdk2 (M2), Cdk4 (C-22), and Cdk6 (C-21); cyclins D1 (H-295), D2 (C-17), and E(M-20); and p15 (C-20) and pRb (C-15) were from Santa Cruz Biotechnology(Santa Cruz, Calif.). p27 antibody was from Transduction Laboratories(Lexington, Ky.). Antibodies used to immunoprecipitate Cdk2 (M2),Cdk6 (C-21), cyclin D2 (C-17), and p27 (C-19) were also from SantaCruz Biotechnology; cyclin E (no. 06-459) was from Upstate Biotechnology(Lake Placid, N.Y.); and polyclonal p27 antibody was generousgift from J. Massagué (Sloan-Kettering Institute, New York, N.Y.).Monoclonal antibodies against cyclin D1 (DCS-11) and Cdk6 (DCS-83)were generous gifts of Jiri Bartek (Danish Cancer Society, Copenhagen,Denmark). Mouse monoclonal antibody against 5-BrdUrd was fromAmersham Life Sciences (Amersham, United Kingdom). Biotin-conjugatedswine anti-rabbit and swine anti-mouse antibodies were from DAKO(Glostrup,Denmark).

Flow cytometry and 5-BrdUrd assays. Fluorescence-activated cell sorting (FACS) and 5-BrdUrd analyses were carried out essential as described earlier (14). Briefly,for FACS analysis, cells were trypsinized, pelleted by centrifugation,washed with phosphate-buffered saline (PBS) (140 mM NaCl in 10mM sodium phosphate buffer, pH 7.4), and fixed with ice-cold 100%methanol at $-$ 20°C overnight. For DNA staining, the cells werewashed with PBS, resuspended in PBS containing 50 µg of RNaseA (Sigma) per ml, and incubated at 37°C for 30 min. The DNA wasstained with 50 µg of propidium iodide (Sigma) per ml at 4°C overnight,and the DNA content was analyzed by FACScan (Becton Dickinson).The data were analyzed by the ModFIT program. For 5-BrdUrd analysis,cells grown on coverslips were incubated for 1 h with 50 µM 5-BrdUrdand fixed with 3.5% paraformaldehyde at room temperature for 20min. After permeabilization of the cell membranes with 0.5% NonidetP-40 (NP-40) in PBS for 5 min, DNA was denatured with 1.5 M HClfor 30 min, washed with PBS, and stained with monoclonal antibodyagainst 5-BrdUrd followed by rhodamine-conjugated anti-mouse antibody(DAKO). Nuclei were stained with Hoechst 33258 (2 µg/ml) (Sigma).The proportion of 5-BrdUrd-positive nuclei of all Hoechst 33258-stainednuclei was calculated by immunofluorescencemicroscopy.

Immunoblotting and immunoprecipitation analysis. For immunoblotting analysis of total cell lysates, cells were lysed with 50 mM Tris-Cl buffer, pH 6.8, containing 100 mM dithiothreitol(DTT), 2% sodium dodecyl sulfate (SDS), and 10% glycerol and incubatedat 95°C for 10 min. DNA was sheared by sonication, and the proteinconcentrations were measured by the Bradford assay (3). Bromophenolblue was added (0.1% final concentration), and 10 µg of proteinper lane was separated by SDS-polyacrylamide gel electrophoresis(PAGE) followed by transfer to an Immobilon-P membrane (Millipore,Bedford, Mass.). The proteins were detected by immunoblottingwith the indicated antibodies by using biotin-avidin amplificationand enhanced chemiluminescence detection (Amersham Life Sciences).For immunoprecipitation studies, the cells were lysed with NP-40lysis buffer (50 mM Tris-Cl, pH 7.5, containing 150 mM NaCl, 0.5%NP-40, 50 mM NaF, 1 mM sodium orthovanadate, 1 mM phenylmethylsulfonylfluoride, 0.1 mg of leupeptin per ml, 0.1 mg of E-64 per ml, and0.1 mg of soybean trypsin inhibitor per ml) on ice for 20 minand the lysate was clarified by centrifugation. The protein concentrationswere measured by the Bio-Rad D_c protein assay kit (Bio-Rad, Hercules,Calif.). For immunoprecipitation, cell lysates containing equalamounts of proteins were precleared with protein A-Sepharose (Pharmacia,Uppsala, Sweden) or with GammaBind-G Sepharose (Pharmacia) forpolyclonal and monoclonal antibodies, respectively, for 4 h, followedby incubation on ice overnight with the indicated antibodies.The immunocomplexes were precipitated with protein A-Sepharoseor GammaBind-G Sepharose at 4°C for 40 min, washed six times withNP-40 lysis buffer, and separated by SDS-PAGE, followed by transferto Immobilon-P membranes. The following percentages of polyacrylamidein SDS-PAGE were used for the detection of individual proteins:7.5% for pRb; 10% for cyclin E; 12.5% for Cdk4, Cdk6, and cyclinD1-2; and 15% for Cdk2, p15, andp27.

For immunodepletion analysis, lysates were incubated for three sequential cycles with polyclonal anti-p27 antibodies on icefor 2 h followed by precipitation with protein A-Sepharose. Aftereach precipitation, the lysates were recovered by centrifugationand subjected to the next precipitation cycle. Finally, the lysateswere incubated with anti-cyclin E antibody and precipitated withprotein A-Sepharose followed by kinase assay. Quantitation ofproteins after immunoblotting analysis was carried out by ScionImage (Scion Corp.), version $beta$ eta2.

For metabolic labeling, cells were incubated with 150 µCi of [³⁵S]methionine-cysteine labeling mix (Promix; Amersham Life Sciences)per ml in methionine-cysteine-free medium containing 10% dialyzedFCS for 2 h. To determine the half-life of Cdk6, cells were labeledwith [³⁵S]methionine-cysteine labeling mix in methionine-cysteine-freemedium containing 10% dialyzed FCS for 2 h, as above, followedby three washes with growth medium and chases for the indicatedtimes in the presence of growth factors. Cells were lysed in 10mM Tris-HCl, pH 7.5, containing 1% SDS and boiled for 5 min. ForCdk6 immunoprecipitation, equal amounts of denatured cell lysateswere diluted 1:10 into RIPA buffer (final concentration of 50mM Tris-HCl, pH 7.5 containing 1% NP-40, 0.5% sodium deoxycholate,0.1% SDS, 50 mM NaF, 1 mM sodium orthovanadate, 1 mM phenylmethylsulfonylfluoride, 0.1 mg of leupeptin per ml 0.1 mg of E-64 per ml, and0.1 mg of soybean trypsin inhibitor per ml) followed by immunoprecipitation,as describedabove.

Northern analyses. mRNA was isolated by using oligo(dT)-cellulose column chromatography (Calbiochem). mRNA (3 µg per lane) was separated on a1% agarose-formaldehyde gel and transferred to a Hybond-N membranein 20× SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate).RNA was detected by probing with a human Cdk6 XmnI cDNA fragmentlabeled with [ $alpha$ ³²P]dCTP by random priming (Ready-To-Go; Pharmacia). Full-lengthCdk6 cDNA was a kind gift of J. LaBaer and E.Harlow.

Kinase assays. Kinase assays were carried out essentially as described by Matsushime et al. (29). Briefly, cells were lysed with NP-40lysis buffer and immunoprecipitations were carried out as describedabove, except that beads were washed four times with NP-40 lysisbuffer followed by two washes with 50 mM HEPES-Cl, pH 7.5, containing1 mM DTT. The beads were suspended in 30 µl of kinase buffer (50mM HEPES-Cl [pH 7.5], 10 mM MgCl₂, 1 mM DTT, 2.5 mM EGTA, 0.1mM sodium orthovanadate, 1 mM NaF, 20 µM ATP, and 10 µCi of [ $gamma$ -³²P]ATP [3,000 Ci/mmol] [Amersham Life Sciences]) containing 1 µgof histone H1 (Boehringer, Mannheim, Germany) or 2 µg of glutathioneS-transferase (GST)-Rb (17) as a substrate. The reaction mixturewas incubated at 30°C for 30 min with occasional mixing of thebeads. Phosphorylated proteins were visualized by autoradiographyafter separation by SDS-12.5% PAGE. Quantitations of the autoradiogramswere carried out with a Fujifilm BAS-2500 Image Analyser and MacBAS2.5. Kinase activities resulting from nonimmune rabbit serum orrabbit or mouse immunoglobulin G were subtracted in eachassay.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

HGF counteracts TGF- $beta$ -Induced G₁ arrest of Mv1Lu mink lung epithelial cells. We have previously found that HGF releases Mv1Lu cells from TGF- $beta$ -mediated growth arrest and induces anchorage-independentgrowth of Mv1Lu cells (49). To analyze the effects of TGF- $beta$ and HGF on cell cycle distribution of Mv1Lu cells, exponentiallygrowing Mv1Lu cells were incubated with TGF- $beta$ (100 pM), HGF (220pM), or both in growth medium for 16 h. Subsequently, the cellswere fixed and stained with propidium iodide, and the DNA contentswere analyzed by flow cytometry (FACS). FACS analysis indicatedthat in TGF- $beta$ -treated cells, the fraction of G₁-phase cells hadincreased to 76%, compared to 46% in control cells (Fig. 1A).The cell cycle distribution of HGF-treated cells was similar tothat of control cells. Treatment of the cells with both TGF- $beta$ and HGF decreased the fraction of growth-arrested cells, as shownby an increase of S-phase cells to 29%, compared to 17% in TGF- $beta$ -treatedcells (Fig. 1A), and a decrease in the fraction of G₁-phase cellsfrom 76 to 57%. To further analyze the effects of these growthfactors on DNA synthesis, we measured the DNA replication activityof the cells by 5-BrdUrd incorporation followed by immunostaining.Upon TGF- $beta$ -treatment, only 7% of cells replicated their DNA, comparedto 43% in control cells (Fig. 1B). HGF slightly induced DNA synthesis,as 52% of cells were 5-BrdUrd positive. DNA replication was resumedin cultures treated with both TGF- $beta$ and HGF, and 29% of the cellsincorporated 5-BrdUrd (Fig. 1B). HGF thus prevents the TGF- $beta$ -inducedG₁ block in Mv1Lu cells.

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FIG. 1. Effects of TGF- $beta$ and HGF on cell cycle distribution of Mv1Lu cells. Exponentially growing Mv1Lu cells were treated with 100 pM TGF- $beta$ , 220 pM HGF, or both in DMEM containing 10% FCS for 16 h. (A) Flow cytometry analysis. Inset: percentages of cells in different cell cycle phases. 2n and 4n, diploid and tetraploid DNA contents, respectively. (B) 5-BrdUrd incorporation. Cells were labeled with 5-BrdUrd during the last hour of the 16-h incubation, and 5-BrdUrd incorporation was detected by immunostaining. The results are expressed as percent 5-BrdUrd-positive nuclei of Hoechst 33258-stained nuclei. The results are averages of five independent experiments; standard deviations are shown.

Inhibition of retinoblastoma protein phosphorylation by TGF- $beta$ is prevented by HGF. In TGF- $beta$ -treated, G₁-arrested Mv1Lu cells, pRb is rendered in its underphosphorylated form (24). To study whether HGF modulatesthe effects of TGF- $beta$ on pRb phosphorylation, we analyzed by immunoblottingthe phosphorylation status of pRb in Mv1Lu cells treated withTGF- $beta$ and/or HGF for 16 h. In the TGF- $beta$ -treated cells, the majorityof pRb was in its faster-migrating, underphosphorylated form (Fig.2), whereas in cells grown in the presence of HGF, the migrationof pRb was similar to that in control cells (Fig. 2). In the presenceof both growth factors, pRb was predominantly in its phosphorylatedform, but a single faster-migrating underphosphorylated form wasalso detectable (Fig. 2). These alterations in pRb phosphorylationpatterns reflect the observed effects on cell growth and indicatethat the HGF-induced signal that prevents TGF- $beta$ mediated growtharrest acts at or before pRb phosphorylation.

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FIG. 2. Effects of TGF- $beta$ and HGF on phosphorylation of pRb. Mv1Lu cells were treated with TGF- $beta$ (100 pM) and HGF (220 pM), as indicated, and incubated for 16 h, and the cells were lysed with Laemmli sample buffer. Total cellular lysates (10 µg) were separated by SDS-7.5% PAGE and transferred to an Immobilon-P membrane, followed by immunoblotting against pRb. The hypophosphorylated (pRb^hypo-P) and hyperphosphorylated (pRb^P) forms of pRb are indicated (arrows).

TGF- $beta$ inhibition of Cdk6 synthesis is counteracted by HGF, whereas TGF- $beta$ induction of p15 remains intact. pRb is phosphorylated in G₁ by cyclin D complexes (5, 20, 26, 53). To study how HGF signaling interacts with TGF- $beta$ signaling to prevent the shift of pRb to its underphosphorylatedform, we analyzed the effects of TGF- $beta$ and HGF on the levels onG₁ Cdk's (Cdk4 and Cdk6), cyclins D1 and D2, and their respectiveinhibitors (p15, p27, p21). Exponentially growing Mv1Lu cellswere incubated in medium containing TGF- $beta$ and HGF for 16 h. Concordantwith previously published results (41), analysis of total cellularextracts by immunoblotting with specific antibodies indicatedthat TGF- $beta$ induced expression of p15 and did not affect the levelof Cdk4, cyclin D1 or D2, or p27 (Fig. 3A). Additionally, althoughp21 CDKI has been suggested to mediate TGF- $beta$ growth inhibition(7), its levels in Mv1Lu cells were found to be low and werenot affected by TGF- $beta$ (41) or TGF- $beta$ and HGF (data not shown).Although HGF antagonized TGF- $beta$ -induced growth arrest, it did notprevent TGF- $beta$ -mediated induction of p15 (Fig. 3A). On the otherhand, TGF- $beta$ decreased the expression of Cdk6 present in totalcell lysates by 75% (±14% [n = 3]) compared to controls, whereasconcomitant HGF treatment restored expression (Fig. 3A). The resultswere confirmed in metabolically labeled cells treated with therespective growth factors for 16 h. TGF- $beta$ decreased the synthesisof Cdk6 by 44%, whereas HGF alone had no effect (Fig. 3B). Inthe presence of both growth factors, Cdk6 synthesis was restored(Fig. 3B). Analysis for Cdk6 mRNA expression showed the presenceof multiple transcripts all expressed at low levels, as describedpreviously (6), none of which was significantly affected byTGF- $beta$ treatment of the cells (Fig. 3C) or by HGF or their combination(not shown). Chase experiments were performed to address whetherTGF- $beta$ regulates Cdk6 expression by affecting the half-life ofthe protein. Mv1Lu cells were incubated in the presence of growthfactors for 16 h and labeled for the last 2 h with [³⁵S]methionine-cysteine, followed by washing off of the label andchasing for the indicated time in the presence of each growthfactor. The results show that whereas the half-life of Cdk6 incontrol cells was 7 h, it was decreased in TGF- $beta$ -treated cellsto 4 h (Fig. 3D). HGF, on the other hand, prevented the turnoverof Cdk6 by increasing the half-life to 10 h (Fig. 3D). Concomitanttreatment of the cells with TGF- $beta$ and HGF led to partial restorationof Cdk6 turnover (half-life, 5.5 h [Fig. 3D]). We conclude fromthe above experiments that TGF- $beta$ decreases Cdk6 expression byinhibiting Cdk6 synthesis and by increasing its turnover and thatHGF opposes both of these effects.

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FIG. 3. Growth factor effects on G₁ Cdk's, cyclins, and their inhibitors. (A) Mv1Lu cells were treated with growth factors, as indicated, and cell lysates were prepared, followed by immunoblotting analysis as described in the legend to Fig. 2. The proteins were detected by using the indicated antibodies. (B) Mv1Lu cells were treated with growth factors for 16 h and labeled for the last 2 h with [³⁵S]methionine-cysteine, followed by analysis of cell lysates by immunoprecipitation with a Cdk6 antibody. The autoradiograms were quantitated by PhosphorImager analysis. (C) Northern analysis of cells treated with TGF- $beta$ was performed for the indicated times by using human Cdk6 as a probe, followed by quantitation of the signals by PhosphorImager analysis. Fold changes in the three most abundant mRNA transcripts are shown below. Black bars, 2.4 kb; shaded bars, 1.8 kb; white bars, 1.1 kb. (D) Chases of metabolically labeled Mv1Lu cells were performed as described in Materials and Methods. Signals from Cdk6 immunoprecipitates were quantitated by PhosphorImager analysis. The relative levels of Cdk6, compared to the amount of Cdk6 present at time zero (set at 1) in cells treated with the respective growth factor, are plotted. The results are means of two independent experiments.

HGF opposes TGF- $beta$ -mediated downregulation of cyclin D2-associated Cdk6 and Cdk6-associated p27. The changes in the G₁ cyclin-Cdk complexes and their interaction with inhibitors were studied by immunoprecipitation followedby immunoblotting. As cyclin D2 is the predominant cyclin in Mv1Lucells (10, 41), cyclin D2 complexes were analyzed in furtherexperiments. Cell lysates of Mv1Lu cells incubated in medium containingTGF- $beta$ and HGF for 16 h were immunoprecipitated with Cdk6 or cyclinD2 antibodies followed by immunoblotting with antibodies specificfor CDKIs or Cdk6, as indicated. The results showed that TGF- $beta$ induced the association of p15 with Cdk6 by 2.8-fold, and a similarlevel of association was found in cells treated with both growthfactors (Fig. 4A). Upon TGF- $beta$ treatment, the association of Cdk6with cyclin D2 was decreased by over 90%, as well as the bindingof p27 to Cdk6 (Fig. 4A). The latter effects probably reflectthe presence of lesser amounts of Cdk6 in TGF- $beta$ -treated cells,as well as displacement of p27 from Cdk6 complexes by p15, assuggested earlier (41). HGF treatment alone had no major effectson cyclin D2 and Cdk6-associated p27, p15 bound to Cdk6, or Cdk6complexed with cyclin D2 (Fig. 4A). However, HGF restored theassociation of Cdk6 with cyclin D2 and Cdk6 binding to p27 fromTGF- $beta$ -exerted negative regulation (Fig. 4A). The presence of higheramounts of Cdk6 and Cdk6-associated proteins in these complexesfits well with the counteraction of HGF on Cdk6 regulation byTGF- $beta$ (Fig. 3A).

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FIG. 4. Effects of growth factors on complex formation of G₁ Cdk's, cyclins, and associated kinase activities. (A) Immunoblotting analysis of immunoprecipitated complexes. Immunoprecipitations (IP) were carried out first with antibodies against Cdk6 and cyclin D2, followed by separation by SDS-PAGE. The proteins were then transferred to an Immobilon-P membrane, followed by Western blotting (WB) with the indicated antibodies. The signals were quantitated with Scion Image, as described in Materials and Methods, and fold changes compared to controls are shown below each analysis. (B) Cyclin D2-associated kinase activity was determined by using GST-Rb as a substrate. Kinase activities were quantitated by PhosphorImager, the kinase activity given by nonimmune serum was subtracted, and the activities were compared to the level in control cells, which was set at 100.

To address directly whether HGF is able to bypass the TGF- $beta$ -mediated cell cycle block through altered regulation of G₁ cyclincomplexes, we analyzed the regulation of cyclin D2-associatedGST-Rb kinase activity by growth factors. Cyclin D2-associatedGST-Rb kinase activity in control and HGF-treated cells was 14%of that of Cdk2-associated GST-Rb kinase activity (not shown).In TGF- $beta$ -treated cells, there was virtually no cyclin D2-associatedkinase activity (Fig. 4B). In cells treated with both growth factors,HGF was able to partly rescue the kinase activity, although itstill remained low (37% of control) (Fig. 4B). This suggests thatHGF may override the TGF- $beta$ block by mechanisms other than solelyregulation of G₁ cyclin-Cdkcomplexes.

The results indicate that HGF fails to prevent TGF- $beta$ -induced accumulation of p15 and its association with Cdk6. Though thetotal levels of Cdk6 decline in TGF- $beta$ -treated cells, there appearsto be enough Cdk6 to bind available p15, thus suggesting the presenceof lesser amounts of p15 than Cdk6 in TGF- $beta$ -treated cells. Incontrast, HGF prevents TGF- $beta$ -mediated decrease of free and cyclinD2-bound Cdk6. The restoration of Cdk6 expression in cells treatedwith both factors could also lead to its binding of more p27,thus harvesting a part of p27 from that bound to Cdk2complexes.

HGF counteracts TGF- $beta$ regulation of Cdk2. Cdk2-cyclin E complexes phosphorylate pRB in late G₁ phase (1, 26). TGF- $beta$ treatment decreases the activity of Cdk2-cyclinE complexes by enhancing the association of p27 to these complexes(39-41). Concomitantly, TGF- $beta$ decreases the amount of the faster-migrating,active form of Cdk2 (22, 41). Both of these events lead toa decrease in Cdk2-associated kinase activity. To study whetherthe changes in phosphorylation of pRb effected by TGF- $beta$ and HGFin Mv1Lu cells are due to altered regulation of Cdk2 and cyclinE complexes, we analyzed the effects of growth factors on Cdk2and cyclin E protein expression and their association with theinhibitorp27.

Immunoblotting analysis of total cell lysates of growth factor-treated cells revealed no changes in the expression of Cdk2or cyclin E (Fig. 5A). However, as shown before (22), TGF- $beta$ decreased the amount of the faster-migrating, active form of Cdk2(Fig. 5A) whereas HGF had no effect on the migration of Cdk2 comparedto control cells (Fig. 5A). Interestingly, when cells were treatedwith both growth factors, the TGF- $beta$ -mediated decrease in the faster-migratingform of Cdk2 was efficiently prevented by HGF (Fig. 5A).

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FIG. 5. Effects of TGF- $beta$ and HGF on expression and complex formation of Cdk2 and cyclin E. Mv1Lu cells were treated with the indicated growth factors, and cell lysates were prepared. (A) Immunoblotting analysis of Cdk2 and cyclin E. The different forms of Cdk2 are indicated (Thr¹⁶⁰ phosphorylated form of Cdk2 is designated cdk2^T160P). (B) Complex formation of cyclin E and Cdk2 was detected by immunoprecipitation (IP), followed by Western blotting (WB) analysis with the indicated antibodies. Fold changes compared to controls are shown below each analysis.

The effects of TGF- $beta$ and HGF on complexes of Cdk2, cyclin E, and p27 were studied by immunoprecipitation followed by immunoblottinganalysis. Growth factor treatments had no effect on the amountof cyclin E-associated Cdk2 (Fig. 5B). The amount of p27 in complexeswith Cdk2 or cyclin E was induced 1.4- and 2.5-fold, respectively,by TGF- $beta$ treatment (Fig. 5B). HGF alone decreased the amount ofp27 associated with Cdk2 by over half but had little effect onthe association of p27 with cyclin E (Fig. 5B). In cells treatedwith both growth factors, the amount of p27 bound to Cdk2 or cyclinE was similar to that found in cells treated with TGF- $beta$ alone(Fig. 5B). These findings suggest that HGF alleviates the decreasein the faster-migrating form of Cdk2 induced by TGF- $beta$ , whereasit has only a slight effect on the formation of complexes betweenp27 and Cdk2 or cyclin E in response to TGF- $beta$ .

HGF restores TGF- $beta$ -suppressed Cdk2 and cyclin E kinase activities towards histone H1 and GST-Rb. Association of p27 CDKI with Cdk2 complexes, induced by TGF- $beta$ , inactivates kinase activity (40, 41). The regulation ofCdk2-cyclin E complexes by growth factors was studied with histoneH1 and GST-Rb as substrates. Cells were treated with TGF- $beta$ andHGF, as described above, and cellular lysates were immunoprecipitatedwith Cdk2 and cyclin E antibodies, followed by kinase assays (29).The Cdk2-associated kinase activity towards histone H1 in TGF- $beta$ -treatedcells was 30% of control, whereas HGF induced the kinase activityby 1.6-fold (Fig. 6A, lanes 2 and 3). In cells treated with bothTGF- $beta$ and HGF, Cdk2-associated kinase activity was 90% of control(Fig. 6A, lane 4). Similarly, GST-Rb was used as a substrate forCdk2 and cyclin E-associated kinase activities (Fig. 6B). In TGF- $beta$ -treatedcells, Cdk2-associated kinase activity was 14% of control (Fig.6B, lane 2), whereas HGF treatment had no major effect on kinaseactivity (Fig. 6B, lane 3). In cells treated with both factors,HGF counteracted the TGF- $beta$ effect on Cdk2 kinase activity towardsGST-Rb and restored it to levels similar to those in control cells(Fig. 6B, lane 4). Accordingly, cyclin E-associated kinase activitytowards GST-Rb in TGF- $beta$ -treated cells was 30% of control (Fig.6B, lane 6), whereas HGF alone stimulated the activity only slightly(Fig. 6B, lane 7). However, HGF restored TGF- $beta$ -repressed cyclinE-associated kinase activity (Fig. 6B, lane 8).

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FIG. 6. Cdk2- and cyclin E-associated kinase activities of TGF- $beta$ - and HGF-treated Mv1Lu cells. Cells were treated with the indicated growth factors, followed by lysis in NP-40 buffer. Immunoprecipitations with the indicated antibodies and kinase assays were carried out as described in Materials and Methods. (A) Cdk2-associated kinase activity with histone H1 as a substrate. (B) Cdk2 (lanes 1 to 4)- and cyclin E (lanes 5 to 8)-associated kinase activities with GST-Rb as a substrate. The figures show relative kinase activities compared to control cells (set at 100). (C) Sparsely seeded cells were pretreated with TGF- $beta$ (400 pM) for 16 h, followed by addition of HGF (220 pM) without removal of TGF- $beta$ , and incubations were continued for the indicated times (4 to 36 h). Untreated control cells are included (lanes 1 and 14). In wash, cells treated with TGF- $beta$ for 16 h were washed four times with growth medium, followed by addition of fresh medium. The cells were lysed, followed by Cdk6 and Cdk2 immunoblotting and determination of Cdk2-associated kinase activity towards histone H1. Relative kinase activities after subtraction of the kinase activity given by nonimmune serum are shown compared to cells treated with TGF- $beta$ for 16 h (set at 100) (lane 1). 5-BrdUrd incorporation was analyzed for the last hour of each incubation. The results are expressed as percent 5-BrdUrd-positive nuclei of Hoechst 33258-stained nuclei.

We next wanted to address whether HGF can bypass TGF- $beta$ -mediated growth arrest under conditions in which cells are first arrestedin G₁ by a 16-h incubation with TGF- $beta$ , followed by addition ofHGF without the removal of TGF- $beta$ . After addition of HGF to thecells, the cells were further incubated for 4 to 36 h, followedby analysis of Cdk6 and Cdk2 (by immunoblotting), Cdk2-associatedkinase activity towards histone H1, and DNA replication in cells.Addition of HGF to TGF- $beta$ -arrested cells for 12 h was sufficientto induce an increase in DNA replication of the cells (from 9to 23%), with a significant portion of the cells replicating theirDNA by 24 h after HGF addition (59%) (Fig. 6C). In contrast, attemptsto wash TGF- $beta$ away followed by addition of fresh growth mediumwere without effect on DNA replication in cells even after a 36-hincubation. Concomitant analyses of Cdk6, Cdk2, and Cdk2-associatedkinase activity showed that, firstly, HGF restored Cdk6 expressionwithin 12 h after addition. Secondly, immunoblotting analysesof Cdk2 indicated that while in TGF- $beta$ -treated cells Cdk2 remainedin its slower-migrating form, in HGF-treated cells Cdk2 showeda significant shift to its faster-migrating form by 24 h, kineticsthat paralleled entry of the cells into S phase (Fig. 6C, lane10). Furthermore, HGF stimulated kinase activity by twofold at12 h after addition of HGF to the TGF- $beta$ -arrested cells (Fig. 6C,lane 8), which remained at the same level of induction at 24 and36 h after exposure to HGF (Fig. 6C, lanes 10 and 12). The resultsshow that HGF releases Mv1Lu cells from TGF- $beta$ -mediated growtharrest with concomitant upregulation of Cdk6 and increased Cdk2-cyclinEactivities.

Regulation of cyclin E-associated kinase activity towards histone H1 is not affected by p27 immunodepletion. The observed growth factor regulation of Cdk2 and cyclin E activities could result from complexes devoid of p27. To studyfurther the action and regulation of p27 present in Cdk2-cyclinE complexes by TGF- $beta$ and HGF, we immunodepleted lysates of growthfactor-treated cells with polyclonal anti-p27 antibodies. Afterthree immunodepletion cycles with anti-p27 antibody, the lysateswere either directly resolved by SDS-PAGE or immunoprecipitatedwith cyclin E or p27 followed by immunoblotting analysis. Thedepletion steps removed all detectable p27, cyclin E-associatedp27, and p27-associated Cdk2 but did not significantly affectthe total levels of cyclin E or Cdk2 (Fig. 7B, lanes 5 to 8).p27 immunodepletion removed 40 and 20% of cyclin E-bound Cdk2present in control cells and in HGF-treated cells, respectively(Fig. 7B, lanes 5 and 7), whereas in TGF- $beta$ -treated cells cyclinE-associated Cdk2 was lost almost totally, reflecting the higheramounts of p27 bound to this complex upon TGF- $beta$ treatment (Fig.7B, lane 6). Instead, in cells treated with both growth factors,30% of cyclin E-bound Cdk2 was left after immunodepletion, suggestingthat less p27 remains attached with cyclin E-Cdk2 complexes.

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FIG. 7. (A) Growth factor regulation of cyclin E-associated kinase activity following p27 immunodepletion. Sparsely seeded cells were treated with TGF- $beta$ (100 pM) and HGF (220 pM), as indicated, followed by lysis in NP-40 buffer. Lysates were immunoprecipitated with cyclin E antibody (lanes 1 to 4) or with three subsequent cycles of polyclonal p27 antibody, followed by cyclin E immunoprecipitation (lanes 5 to 8). Kinase assays towards histone H1 were carried out as described in Materials and Methods. Relative kinase activities after subtraction of the kinase activity given by nonimmune serum compared to control cells (set at 100) are indicated. (B) Effects of p27 immunodepletion steps on cyclin E, Cdk2, p27, and their complexes. In parallel with experiment represented by panel A, cell lysates before and after three immunodepletion cycles with anti-p27 antibody were analyzed by immunoprecipitation (IP) with the indicated antibody, followed by immunoblotting (WB). Total cyclin E and p27 were analyzed by immunoblotting. Fold changes compared to controls are shown below each analysis.

Histone H1 kinase assays, carried out in parallel with the above experiment, indicated that TGF- $beta$ decreased the cyclin E-associatedkinase activity to close to basal levels in both p27-depletedand nondepleted lysates (Fig. 7A, lanes 2 and 6). Depletion ofp27 from cells treated with both growth factors had no effecton the activity (Fig. 7A, lanes 4 and 8). In control cells, kinaseactivity was somewhat increased by p27 immunodepletion. However,in repeated immunodepletion experiments, the increase varied between1.1- and 1.4-fold. The p27 depletion assays suggest that thoughp27 is associated with Cdk2-cyclin E complexes in cells treatedwith both TGF- $beta$ and HGF and part of these complexes is removed,there appears to be enough active complex present in cells forcellularproliferation.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Cancer cells escape cellular growth control by ignoring growth inhibitory signals, such as TGF- $beta$ . The TGF- $beta$ signal transductionpathway is well studied, and many of the components that are involvedin the TGF- $beta$ signaling pathway are mutated or have altered functionsin malignant cells (28, 50). However, little is known abouthow cells respond to simultaneous inhibitory and stimulatory growthfactors and on what level these signals are integrated. Mv1Lucells are extremely sensitive to growth inhibition by TGF- $beta$ , andthis growth regulation has been extensively studied (10, 22,24, 38, 40, 41). We found earlier that HGF prevents TGF- $beta$ -inducedgrowth arrest in Mv1Lu mink lung epithelial cells and in endothelialcells (49). This finding gave us an in vivo model system forstudy of the TGF- $beta$ growth arrest and cell cycle regulatory mechanismsthat allow cells to escape TGF- $beta$ -induced G₁ block. Flow cytometryanalyses and 5-BrdUrd incorporation studies indicated that HGFdecreased the number of Mv1Lu cells arrested in G₁ phase by TGF- $beta$ .The observed fourfold increase in DNA synthesis in cells treatedwith both TGF- $beta$ and HGF, compared to TGF- $beta$ -treated cells, is inline with the observation that most of pRb is phosphorylated aftertreatment of cells with both growth factors. As TGF- $beta$ is a verypotent growth inhibitor of Mv1Lu cells (50% effective dose, $<=$ 5pM), rescue from TGF- $beta$ growth arrest by HGF was significant, albeitnot complete. Concomitant with the rescue of TGF- $beta$ -induced G₁arrest by HGF, we found that HGF opposed the TGF- $beta$ effects byinhibiting the TGF- $beta$ -mediated decrease in Cdk6 expression andthe decrease of Cdk6 association with p27 and cyclin D2. However,HGF was unable to interfere with TGF- $beta$ induction of p15 and itscomplex formation with Cdk6. The results suggest that as a consequenceless p27 associates with and inhibits Cdk2 activity, leading torestoration of Cdk2-cyclin E-associated kinase activity suppressedby TGF- $beta$ . Significantly, HGF was able to restore Cdk6 expressionand the Cdk2-associated kinase activities and cell proliferationin cells that were already growth arrested by TGF- $beta$ .

Growth factor interactions can be integrated by intracellular signaling pathways. Epidermal growth factor and HGF can antagonizethe effects of bone morphogenetic protein by inducing phosphorylationof Smad1 via the extracellular signal-regulated kinase-mediatedpathway. Phosphorylation leads to the inhibition of bone morphogeneticprotein signaling (23), suggesting that opposing signals aremodulated at the level of Smad proteins. Smad1 is not involvedin TGF- $beta$ signaling (28), but similar mechanisms utilizing Smad2and Smad3 could affect the ability of HGF to alter the growthinhibitory effect by TGF- $beta$ . Indeed, recent work shows that HGFcan phosphorylate and activate Smad2, although to a lesser extentthan can TGF- $beta$ (8). Our data, however, indicate that HGF doesnot inhibit, nor act synergistically with, TGF- $beta$ , because HGFdoes not alter the level of induction of p15 or extracellularmatrix components such as fibronectin and thrombospondin (49)or PAI-1 (not shown) by TGF- $beta$ . Our results are consistent withthe hypothesis that HGF does not interfere, in general, with theTGF- $beta$ signal transduction pathways but that the signals involvinggrowth regulation are integrated at the level of Cdkcomplexes.

This is the first study in which the regulation of endogenous p15 protein by TGF- $beta$ has been detected in Mv1Lu cells. The findingscorrelate with prior observations of increases in p15 mRNA byTGF- $beta$ in Mv1Lu and HaCaT human keratinocyte cells (16, 41)and p15 protein in HMEC human mammary epithelial cells (43).TGF- $beta$ enhanced the association of endogenous p15 with Cdk6 complexes,but the induction of p15 and its association with Cdk6 was notprevented by HGF. Accordingly, cyclin D2-associated Rb kinaseactivity was decreased by TGF- $beta$ and by concomitant treatment withTGF- $beta$ and HGF. Interestingly, TGF- $beta$ was found to decrease theexpression of Cdk6 and its association with cyclin D2, both ofwhich were prevented by HGF. A similar decrease in Cdk6 by TGF- $beta$ was found in metabolically labeled Mv1Lu cells (Fig. 3B) (41).The restoration of Cdk6 expression in cells treated with bothgrowth factors correlated with the partial rescue of cyclin D2-associatedkinase activity towards GST-Rb. This suggests that though p15induction is unperturbed in cells treated with both growth factorsand it avidly forms complexes with Cdk6, its levels are not highenough to fully prevent the activity of Cdk6-cyclin D2 complexes.The observed decrease in cyclin D2-activity may be attributedto partial inhibition of a fraction of Cdk6 by p15. In addition,the levels of p15 may not be sufficient to sequester all Cdk6present in the cells. This in turn leads to the presence of activeCdk6-cyclin D2 complexes that can harvest p27 from binding toCdk2. Thus, the decrease in Cdk6 expression may contribute importantlyto the induction, maintenance, and adaptation of cells to TGF- $beta$ -mediatedgrowtharrest.

Cyclin E and Cdk2 protein levels per se were unaffected by growth factor treatments. Kinase assays of TGF- $beta$ -treated cellsshowed that Cdk2 and cyclin E-associated activities were decreased,while HGF rescued these TGF- $beta$ -mediated effects. This finding isin line with the observed phosphorylation status of pRb and withthe notion that there were fewer cells in G₁ in the TGF- $beta$ - andHGF-treated population than in TGF- $beta$ -treated cells. TGF- $beta$ decreasedthe amount of the faster-migrating form of Cdk2, and HGF counteractedthis effect. The TGF- $beta$ -mediated decrease in the faster-migratingform of Cdk2 is in accordance with earlier studies (22, 41,47). The possibility remains that the decrease in the amountof active Cdk2 could be associated with modulation of CAK activityin growth factor-treated cells. Regulation of endogenous Cdk7-cyclinH activity by TGF- $beta$ and HGF was not observed in our study (datanot shown), but this does not exclude the presence of other uncharacterizedCAKs.

As shown earlier for TGF- $beta$ (40, 41), total p27 levels were not affected either by TGF- $beta$ or by HGF. Instead, as shown bythe immunodepletion assay with p27 antibodies, TGF- $beta$ enhancedthe association of p27 with Cdk2 and cyclin E complexes and HGFprevented this interaction partially, suggesting that less p27is associated with the Cdk2-cyclin E complex in cells treatedwith both growth factors (Fig. 7B). Further, the immunodepletionassay suggests that the kinase activity of Cdk2-cyclin E complexesdevoid of p27 may be sufficient for cellular proliferation. Thoughthe binding of p27 to the Cdk2-cyclin E complex is generally thoughtto inhibit kinase activity, p27 itself and its association withthe complex is under modulation. For example, it has been suggestedthat Myc activates Cdk2-associated kinase activity by phosphorylationof p27, resulting in enhanced p27 degradation (33), and by inhibitionof p27 binding to newly formed Cdk2-cyclin E complexes (36).Additionally, the viral oncoproteins E1A and E7 bind and sequesterp27 from Cdk2-cyclin E complexes, leading to activation of thecomplex (27, 54). Though we have no direct evidence that HGFcauses alternative regulation of p27 protein levels, we cannotexclude the possibility that upon HGF treatment p27 loses high-affinitybinding to Cdk2-cyclin E or that the steric complex between p27,Cdk2, and cyclin E would be in a conformation facilitating activationof Cdk2 kinaseactivity.

Based on our results, we suggest that HGF modifies the TGF- $beta$ response by regulation of Cdk6 complexes, thus also affectingthe activity of Cdk2 complexes, and that these modifications serveas means of hindering the growth inhibition exerted by TGF- $beta$ .Firstly, HGF prevents a decrease in Cdk6 but not an increase inp15 by TGF- $beta$ . Though the level of p15 is increased, it may notbe sufficient to sequester all Cdk6 present in the cells, andactive Cdk6-cyclin D2 complexes can harvest p27 from binding toCdk2. The observed decrease in cyclin D2 activity may also beattributed to partial inhibition of a fraction of Cdk6 by p15.Secondly, HGF could relieve the TGF- $beta$ growth arrest by directlymodulating Cdk2 kinase activity or the association of p27 withthe kinase complex. However, we cannot rule out the possibilitiesthat the HGF effect is not solely mediated by the alternativeregulation of Cdk6 and that the release of Cdk2-cyclin E activityfrom suppression by p27 occurs through increased binding of Cdk6complexes to p27. Here we have addressed the regulation of onlya set of kinases and their inhibitors, based on their abundancein Mv1Lu cells. We cannot exclude the possibility that regulationof other kinases, cyclin partners, or inhibitors contributes tosome of the observed effects. The hypothesis that TGF- $beta$ growtharrest involves additional mechanisms besides action of p15 andp27 CDKIs is strengthened by genetic and biochemical evidence,as cells from mice nullizygous for p27 (34) and mammary epithelialcells that lack p15 are growth inhibited by TGF- $beta$ (18). Thesemodels imply that for TGF- $beta$ growth suppression to take place,TGF- $beta$ must affect multiple cell cycle components. Our data indicatethat regulation of Cdk6 levels is important for TGF- $beta$ growth inhibition.The decrease in Cdk6 can contribute to TGF- $beta$ growth arrest bydownregulation of cyclin D2-associated kinase activity and byensuring that sufficient amounts of p27 are liberated to associatewith and inhibit Cdk2-cyclin E activity. Furthermore, the presentdata indicate that positive and negative growth signals are integratedat the level of Cdkregulation.

	ACKNOWLEDGMENTS

We thank Joan Massagué and Jiri Bartek for generous gifts of antibodies, Tomi Mäkelä for critical review of the manuscript,and Annamari Heiskanen for fine technicalassistance.

This work was supported by the Academy of Finland, the Ida Montin Foundation, Novo Nordisk Foundation, Sigrid Juselius Foundation,Finnish Cancer Foundation, and BiocentrumHelsinki.

	FOOTNOTES

^* Corresponding author. Mailing address: Haartman Institute, Department of Virology, University of Helsinki, P.O. Box 21 (Haartmaninkatu3), FIN-00014 Helsinki, Finland. Phone: 358-9-1912-6509. Fax:358-9-1912-6491. E-mail: Marikki.Laiho{at}Helsinki.FI.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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47. Slingerland, J. M., L. Hengst, C. H. Pan, D. Alexander, M. R. Stampfer, and S. I. Reed. 1994. A novel inhibitor of cyclin-Cdk activity detected in transforming growth factor $beta$ -arrested epithelial cells. Mol. Cell. Biol. 14:3683-3694[Abstract/Free Full Text].

48. Solomon, M. J., T. Lee, and M. W. Kirschner. 1992. Role of phosphorylation in p34cdc2 activation: identification of an activating kinase. Mol. Biol. Cell 3:13-27[Abstract].

49. Taipale, J., and J. Keski-Oja. 1996. Hepatocyte growth factor releases epithelial and endothelial cells from growth arrest induced by transforming growth factor- $beta$ 1. J. Biol. Chem. 271:4342-4348[Abstract/Free Full Text].

50. Taipale, J., J. Saharinen, and J. Keski-Oja. 1998. Extracellular matrix associated transforming growth factor- $beta$ : role in cancer cell growth and invasion. Adv. Cancer Res. 75:87-133[Medline].

51. van den Eijnden-van Raaij, A. J., I. Koornneef, and E. J. van Zoelen. 1988. A new method for high yield purification of type $beta$ transforming growth factor from human platelets. Biochem. Biophys. Res. Commun. 157:16-23[Medline].

52. Weinberg, R. A. 1995. The retinoblastoma protein and cell cycle control. Cell 81:323-330[Medline].

53. Zarkowska, T., and S. Mittnacht. 1997. Differential phosphorylation of the retinoblastoma protein by G1/S cyclin-dependent kinases. J. Biol. Chem. 272:12738-12746[Abstract/Free Full Text].

54. Zerfass-Thome, K., W. Zwerschke, B. Mannhardt, R. Tindle, J. W. Botz, and P. Jansen-Dürr. 1996. Inactivation of the Cdk inhibitor p27^KIP1 by the human papillomavirus type 16 E7 oncoprotein. Oncogene 13:2323-2330[Medline].

55. Zhu, L., E. Harlow, and B. D. Dynlacht. 1995. p107 uses a p21^Cip1-related domain to bind cyclin/Cdk2 and regulate interactions with E2F. Genes Dev. 9:1740-1752[Abstract/Free Full Text].

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Hepatocyte Growth Factor Releases Mink Epithelial Cells from Transforming Growth Factor 1-Induced Growth Arrest by Restoring Cdk6 Expression and Cyclin E-Associated Cdk2 Activity

Hepatocyte Growth Factor Releases Mink Epithelial Cells from Transforming Growth Factor $beta$ 1-Induced Growth Arrest by Restoring Cdk6 Expression and Cyclin E-Associated Cdk2 Activity