TGF-{beta} and the Smad Signaling Pathway Support Transcriptomic Reprogramming during Epithelial-Mesenchymal Cell Transition

doi:10.1091/mbc.E04-08-0658

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Originally published as MBC in Press, 10.1091/mbc.E04-08-0658 on February 2, 2005

Vol. 16, Issue 4, 1987-2002, April 2005

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TGF- ${beta}$ and the Smad Signaling Pathway Support Transcriptomic Reprogramming during Epithelial-Mesenchymal Cell Transition

Ulrich Valcourt^*, Marcin Kowanetz^*, Hideki Niimi, Carl-Henrik Heldin, and Aristidis Moustakas

Ludwig Institute for Cancer Research, SE-751 24 Uppsala, Sweden

Submitted August 3, 2004; Accepted January 21, 2005
Monitoring Editor: Keith Yamamoto

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Epithelial-mesenchymal transition (EMT) contributes to normaltissue patterning and carcinoma invasiveness. We show that transforminggrowth factor (TGF)- ${beta}$ /activin members, but not bone morphogeneticprotein (BMP) members, can induce EMT in normal human and mouseepithelial cells. EMT correlates with the ability of these ligandsto induce growth arrest. Ectopic expression of all type I receptorsof the TGF- ${beta}$ superfamily establishes that TGF- ${beta}$ but not BMP pathwayscan elicit EMT. Ectopic Smad2 or Smad3 together with Smad4 enhanced,whereas dominant-negative forms of Smad2, Smad3, or Smad4, andwild-type inhibitory Smad7, blocked TGF- ${beta}$ –induced EMT.Transcriptomic analysis of EMT kinetics identified novel TGF- ${beta}$ target genes with ligand-specific responses. Using a TGF- ${beta}$ typeI receptor that cannot activate Smads nor induce EMT, we foundthat Smad signaling is critical for regulation of all testedgene targets during EMT. One such gene, Id2, whose expressionis repressed by TGF- ${beta}$ 1 but induced by BMP-7 is critical for regulationof at least one important myoepithelial marker, ${alpha}$ -smooth muscleactin, during EMT. Thus, based on ligand-specific responsivenessand evolutionary conservation of the gene expression patterns,we begin deciphering a genetic network downstream of TGF- ${beta}$ andpredict functional links to the control of cell proliferationand EMT.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The TGF- ${beta}$ superfamily of secreted polypeptides has diverse rolesduring metazoan embryonic development and adult tissue homeostasis(Piek et al., 1999a; Siegel and Massagué, 2003). TGF- ${beta}$ ligands signal through complexes of type II and type I receptorserine/threonine kinases, which induce Smad and alternativesignaling pathways (Shi and Massagué, 2003). Receptor-regulatedSmads (R-Smads) are phosphorylated by type I receptors and oligomerizewith Smad4 (CoSmad). In the nucleus, R-Smads and Smad4 regulategene transcription. Inhibitory Smads (I-Smads), Smad6 and Smad7,are negative signal regulators that block R-Smad phosphorylationand induce type I receptor dephosphorylation and/or proteasomaldegradation (Shi and Massagué, 2003).

The superfamily is divided into the TGF- ${beta}$ /activin/nodal branch,hereafter abbreviated as TGF- ${beta}$ , and the BMP/growth and differentiationfactor branch, hereafter referred to as BMP, based on theirdownstream R-Smad pathways (Miyazawa et al., 2002). TGF- ${beta}$ activatesSmad2 and Smad3, whereas BMP activates Smad1, Smad5, and Smad8.These pathways show cell type specificity but many coexist inone cell type (Chang et al., 2002). Currently, no systematicstudies of multiple TGF- ${beta}$ pathways in distinct cell types haveyet been performed. This approach is important for the understandingof major physiological responses to these factors, i.e., cellproliferation, apoptosis or differentiation (ten Dijke et al.,2002; Siegel and Massagué, 2003).

Epithelial-mesenchymal transition (EMT) is the process by whichan epithelial cell becomes a more motile mesenchymal cell (Condeelisand Segall, 2003; Grünert et al., 2003). EMT operates duringearly embryonic cell layer movements and later during organogenesis(Tosh and Slack, 2002). During EMT, cell-cell junctions arealtered, cells lose epithelial polarity, express the mesenchymalmarkers vimentin and ${alpha}$ -smooth muscle actin ( ${alpha}$ -SMA), and the resultingreorganization of the actin cytoskeleton supports cell migration.EMT is also important during tumor progression by stimulatinginvasiveness and metastasis (Condeelis and Segall, 2003; Grünertet al., 2003). In vivo verification of EMT is hard to assessdue to the transient and reversible nature of the process anddue to the lack of analytical tools that distinguish carcinomacells undergoing EMT from neighboring stromal fibroblasts.

During embryonic development and in cell culture systems, EMTis triggered by various growth factors, fibroblast growth factorand hepatocyte growth factor/scatter factor being the most extensivelystudied (Thiery, 2002). TGF- ${beta}$ acts as a tumor suppressor by inhibitingepithelial cell growth, but it also promotes tumor progressionin vivo (Siegel and Massagué, 2003; Tang et al., 2003).For example, TGF- ${beta}$ induces differentiation of squamous carcinomainto invasive spindle cell carcinoma in vivo and Smad2 playscritical roles in this process (Cui et al., 1996; Portella etal., 1998; Oft et al., 2002). TGF- ${beta}$ stimulates EMT in vitro inNamru murine mammary gland (NMuMG) and mouse proximal tubulekidney epithelial cells, in immortalized human keratinocytesHaCaT, as well as, in human colonic and hepatocellular carcinomas(Miettinen et al., 1994; Zavadil et al., 2001; Bates and Mercurio,2003; Xu et al., 2003; Brown et al., 2004). In NMuMG cells,TGF- ${beta}$ –mediated EMT involves the TGF- ${beta}$ type I and type IIreceptor complexes and Smad3 (Piek et al., 1999b). In addition,signaling inputs of the p38 mitogen-activated protein kinase(Bhowmick et al., 2001b; Bakin et al., 2002; Yu et al., 2002),the phosphoinositide-3'-kinase-Akt pathway (Bakin et al., 2000),and the RhoA GTPase (Bhowmick et al., 2001a) contribute to EMTof NMuMG cells in response to TGF- ${beta}$ . Thus, EMT in response toTGF- ${beta}$ involves multiple intracellular effectors and the roleof the Smad pathway in this cellular response has been disputedrepeatedly (Bhowmick et al., 2001a, 2001b; Bakin et al., 2002;Thiery, 2002; Yu et al., 2002; Grünert et al., 2003). Thisis in contrast to the process of epithelial growth suppressionby TGF- ${beta}$ where the central role of Smads is firmly established(ten Dijke et al., 2002; Siegel and Massagué, 2003).It is therefore important to systematically analyze the roleof Smads during EMT. There is also a growing interest in identifyinggene targets that execute EMT, in order to effectively interveneagainst this process, in the context of invasive/metastaticcarcinomas.

In the present study, we investigated the effects of variousTGF- ${beta}$ superfamily members on the EMT process of several normalmouse and human epithelial cell types. Based on our previousreport on the role of the type I receptor kinase ALK-5 in EMT(Piek et al., 1999b), we analyzed for the first time the roleof all type I receptor kinases and Smads of the superfamily.Using a cDNA microarray screen, we uncovered several new candidategenes possibly involved in TGF- ${beta}$ -mediated EMT. We therefore describean extensive dissection of the signaling and genetic networkthat supports EMT.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Cell Culture, Adenoviruses, Reagents, and Ligands
Human HaCaT keratinocytes, primary normal human mammary epithelialcells (HMEC), normal human epidermal keratinocytes (NHEK) ofadult origin, and murine mammary epithelial NMuMG cells havebeen described previously (Kowanetz et al., 2004). NMe cells,a clonal epithelial derivative of NMuMG were provided by K.Vershueren (Leuven; Comijn et al., 2001). Immortalized normalhuman mammary epithelial cells, MCF-10A were obtained from ATCCand immortalized human lung epithelial cells, HPL1 (clones Aand D) were donated by T. Takahashi (Nagoya; Masuda et al.,1997).

Adenoviruses expressing: a) the control protein ${beta}$ -galactosidase(Ad-LacZ), the C-terminally hemaglutinin (HA)-tagged constitutivelyactive ALK-1(QD), -2(QD), -3(QD), -6(QD), and ALK-4(TD), -5(TD),-7(TD) receptors, the HA-tagged kinase-inactive ALK1–7(KR)receptors, the N-terminally Flag-tagged Smad1–7 proteins,the C-terminally deleted form of Smad4 (Smad4 515-ter), andthe dominant-negative Smad3 (Smad3(D407E)) were donated by K.Miyazono (Tokyo; Fujii et al., 1999); b) N-terminally Flag-taggedconstitutively active (T204D) and L45 loop-mutated ALK-5 (caALK-5mL45,here referred to as ALK5(TD)mL45) was provided by V. Kaartinen(Los Angeles; Dudas et al., 2004); c) the CAGA₉-MLP-Luciferasepromoter-reporter module was from S. Dooley (Aachen; Dooleyet al., 2001); and d) GFP was based on the bicistronic Adeasyviral system from B. Vogelstein (Baltimore; He et al., 1998).Adenoviruses were amplified and titrated as previously described(Piek et al., 1999b).

The small-molecular-weight inhibitor SB431542 was a gift fromN. J. Laping (GlaxoSmithKline Pharmaceuticals) and has beenshown to inhibit selectively the ALK-4/-5/-7 protein kinaseactivity (Inman et al., 2002).

Recombinant mature TGF- ${beta}$ 1 was purchased from PeproTech EC (London,United Kingdom) or provided by N. Ferrara (Genentech, San Francisco,CA), and recombinant mature TGF- ${beta}$ 2 and - ${beta}$ 3 were provided by R&DSystems (Minneapolis, MN), and recombinant mature BMP-7 wasfrom K. Sampath (Curis, Cambridge, MA). Recombinant mature activin-Awas donated by Y. Eto (Ajinomoto, Tokyo, Japan).

Transient Cell Infections and Gene Reporter Assays
Adenoviral transient infection of cells, using the multiplicitiesof infection (MOIs) specified in the figure legends or tables,were performed as previously described (Piek et al., 1999b).Luciferase reporter assays were performed with the enhancedluciferase assay kit from BD PharMingen (San Diego, CA), accordingto the protocol of the manufacturer. A Smad3/Smad4-specificluciferase reporter, CAGA₉-Luc was used. This reporter contains9 repeats of the Smad-binding element found in the plasminogenactivator inhibitor 1 promoter and is an excellent read-outsystem for testing Smad3/Smad4 activation (Dennler et al., 1998;Dooley et al., 2001).

Transient and Stable Transfections
NMuMG or NMe cells were transiently transfected with siRNAsusing Lipofectamine 2000 (Invitrogen, Carlsbad, CA) accordingto the manufacturer's protocol and as described (Kowanetz etal., 2004). The two mouse Idb2-specific siRNAs used were describedrecently (Kowanetz et al., 2004). Twenty-four hours after transfection,cells were stimulated with BMP-7 for the times indicated inthe figures and before extraction of total proteins or totalRNA. For the establishment of stable NMuMG clones expressinginducible wild-type Smad2 or the dominant-negative form of Smad2(Smad2SA), N-terminally Flag-tagged wild-type Smad2 and Smad2SAwere provided subcloned into the inducible vector pMEP4 (Invitrogen)by S. Souchelnytskyi (Uppsala; Souchelnytskyi et al., 1997).Empty vector pMEP4, wild-type Smad2 or Smad2SA were transfectedinto NMuMG cells using Lipofectamine 2000 (Invitrogen) accordingto the manufacturer's protocol. Two days after transfection,cells were subcultured in the presence of 400 µg/ml hygromycin-B(Calbiochem, La Jolla, CA), and pools of antibiotic-resistantcells or individual cell clones were derived. For inductionof transfected Smad2 and immunofluorescence or Western blotassays, cells growing continuously in the presence of hygromycin-Bwere cultured in the presence of 10 µM CdCl₂ (Sigma, St.Louis, MO) for 24 h, at which point vehicle or TGF- ${beta}$ 1 was addedfor another 24–48 h in the presence of hygromycin-B andinducer.

Immunoblotting and Immunofluorescence Microscopy
Total proteins from infected and/or stimulated NMuMG cells wereextracted and subjected to SDS-PAGE and analyzed by Westernblotting as described previously (Kurisaki et al., 2003). Mousemonoclonal anti-Flag (M2 and M5), mouse anti- ${alpha}$ -smooth muscleactin (A2547) and mouse anti- ${beta}$ -tubulin (T8535) antibodies werepurchased from Sigma-Aldrich, mouse monoclonal anti-hemagglutinin(HA, 12CA5) from Roche (Nutley, NJ), mouse monoclonal anti-E-cadherin(C20820 [GenBank] ) from BD Transduction Laboratories (Lexington, KY),rat monoclonal anti-ZO-1 (MAB1520) from Chemicon International(Temecula, CA), and mouse monoclonal anti-Smad1/2/3 (H2) andrabbit polyclonal anti-Id2 (C-20) from Santa Cruz Biotechnology(Santa Cruz, CA). Rabbit polyclonal anti-phospho-Smad3 antibodywas a gift from Michael Reiss (New Brunswick). Rabbit polyclonalanti-phospho-Smad1 and anti-phospho-Smad2 antibodies were producedin house. Secondary anti-mouse-IgG and anti-rabbit-IgG coupledto horseradish peroxidase (HRP) were from Amersham Biosciences(Piscataway, NJ). The enhanced chemiluminescence detection systemwas purchased from Santa Cruz Biotechnology.

For morphological analysis, cell monolayers were stimulatedwith TGF- ${beta}$ 1/2/3, BMP-7, or activin-A, and/or infected with adenovirusesas indicated in the figure legends. Fixed cell preparationswere stained with tetramethyl-rhodamine isothiocyanate (TRITC)-labeledphalloidin (Sigma-Aldrich) or processed for immunofluorescencemicroscopy as described (Kowanetz et al., 2004). For immunofluorescence,primary antibodies were those listed above, and fluoresceinisothiocyanate (FITC)-conjugated rabbit anti-mouse-IgG antibodywas from DAKO (Carpinteria, CA) and TRITC-conjugated goat anti-rat-IgGantibody was from Jackson ImmunoResearch Laboratories (WestGrove, PA).

Thymidine Incorporation Assays
Cells were cultured, stimulated with growth factors, and labeledmetabolically as described before (Kowanetz et al., 2004). Thedata are plotted as average values with SEs of triplicate repeatsper independent experiment. Each independent experiment wasrepeated at least twice.

cDNA Microarray Analysis
The cDNA microarray analysis was performed with RNAs isolatedfrom NMuMG cells cultured in the presence of 10% fetal bovineserum for 2, 8, or 36 h in the presence or absence of TGF- ${beta}$ 1(10 ng/ml) and from three independent cell cultures. Total RNAextraction and cDNA probe labeling was performed as described(Kowanetz et al., 2004). Equal amount of labeled cDNA probesper pair was hybridized to cDNA microarray chips (Mver1.1.1)from the Sanger/LICR/CRUK Consortium (http://www.sanger.ac.uk/Projects/Microarrays/fordetails and hybridization protocols). This microarray chip contained11,500 unique single-stranded cDNA elements of 1.5-kb averagelength spotted on glass, which represent roughly 8850 uniquemouse genes. Hybridizations were carried out in quadruplicateor quintuplicate, using the RNAs from the three independentcultures and including the dye swap control. Microarray scanning,image analysis, and primary spot intensity statistical analysiswas performed as described (Kowanetz et al., 2004). Regulatedgenes were selected based on the average ratio value $≥$ 1.7 forup-regulated genes and $≤$ 0.57 for down-regulated genes. In addition,regulated genes had to be expressed at least on three arraysout of four (or on four arrays out of five, for the 8- and 36-htime points) and with a t test value for the ratios within replicatescorresponding to p < 0.05. Statistically significant geneswere clustered based on their expression values using the K-meansstatistical algorithm that is incorporated into the GeneSpring6.0 data mining software (Silicon Genetics, Redwood City, CA).For all time points, we considered as 0-h time point the conditionof duplicate cell cultures treated in an identical manner asthe TGF- ${beta}$ 1–treated samples, with the only difference beingthat we replaced TGF- ${beta}$ 1 with vehicle. Functional classificationof the highly regulated genes was performed manually based onexhaustive searches in PubMed (http://www.ncbi.nlm.nih.gov/PubMed/).All files containing the raw data of the microarray analysishave been deposited to ArrayExpress (http://www.ebi.ac.uk/arrayexpress/)at the European Bioinformatics Institute (Hinxton) and are publiclyavailable with Acc. No. E-MEXP-139.

Semiquantitative RT-PCR and Quantitative Real-time RT-PCR
Total RNA from NMuMG cells was extracted and analyzed as previouslydescribed (Kowanetz et al., 2004), using specific primers designedaccording to sequences available in the databanks or publishedby other authors (Supplementary Table 1). Primers for mouseglyceraldehyde-3'-phosphate dehydrogenase (Gapdh) were usedto ascertain that an equivalent amount of cDNA was synthesized.Controls where reverse transcriptase was omitted (-RT) and wherecDNAs were replaced with water were performed in order to demonstratethe specificity of the reactions.

DNase RQI-digested RNA from HaCaT and HMEC cells was reverse-transcribedas described (Kurisaki et al., 2003). PCR was performed in atotal volume of 25 µl with SYBR Green PCR Master Mix (AppliedBiosystems, Foster City, CA), 1 µl (24 ng) of cDNA, anda 200 nM concentration of each primer (Supplementary Table 2).Primers were designed with the computer program Primer Express(Applied Biosystems), using parameters recommended by the manufacturer.Reactions were carried out in an ABI-prism 7000 sequence detector(Applied Biosystems) in triplicate, using the following conditions:an initial denaturation step consisted of 2 min at 50°Cand 10 min at 95°C, followed by 40 cycles of 15 s at 95°Cand 1 min at 60°C. Levels of gene expression in each samplewere determined with the comparative Ct method (after validationassays for each gene primer set), using GAPDH gene as an endogenouscontrol. For each condition, the ground condition (-TGF- ${beta}$ 1) wasset as 1 and expression data are presented as bar graphs ofaverage expression values plus SD.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

EMT Correlates with Growth Arrest Induced by TGF- ${beta}$ in Normal Human and Mouse Epithelial Cells
We investigated the potencies of different members of the TGF- ${beta}$ superfamily (TGF- ${beta}$ 1, - ${beta}$ 2, - ${beta}$ 3, activin-A or BMP-7) to induce EMTand growth inhibition in epithelial cells of different origins.Primary human mammary epithelial cells (HMEC), normal humanand mouse mammary epithelial cells (MCF-10A and NMuMG), immortalizednormal lung epithelial cells (HPL1), primary normal human epidermalkeratinocytes (NHEK), and immortalized normal human keratinocytes(HaCaT) were analyzed (Figure 1A). TGF- ${beta}$ 1, - ${beta}$ 2, and - ${beta}$ 3 inducedcharacteristic features of EMT in the mammary and lung cells:formation of actin stress fibers (Figure 1A), down-regulationand delocalization of E-cadherin and elongated (spindle-like)cell morphology (unpublished results). This effect was lesspronounced in normal keratinocytes NHEK and HaCaT (Figure 1A).Signs of cell scattering were weakly obvious after prolongedstimulation of keratinocytes for several days (unpublished results).Activin-A did not induce EMT in mammary cells or keratinocytes,but caused scattering and spindle-like morphology of HPL1 cells(Figure 1A). Finally, BMP-7 did not induce EMT or scatteringof any cell type tested (Figure 1A). BMP-7 induced thin stressfibers and led to increased cell volume but preserved the cuboidalarchitecture of HMEC and HPL1 cells.

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Figure 1. TGF- ${beta}$ induces EMT and growth inhibition in human and mouse normal epithelial cells. (A) Actin cytoskeleton direct fluorescence microscopy of HMEC, MCF-10A, NMuMG, HPL1 (clone D), NHEK, and HaCaT cells treated with vehicle (control), TGF- ${beta}$ 1 (2.5 ng/ml), TGF- ${beta}$ 2 (2.5 ng/ml), TGF- ${beta}$ 3 (2.5 ng/ml), activin-A (10 ng/ml), or BMP-7 (150 ng/ml) for 36 h. Bars represent 10 µm and the magnification power of each series of photomicrographs is shown above the bars. (B) Dose-response growth inhibition assays performed in HMEC, NMuMG, NHEK, and HaCaT cells in response to TGF- ${beta}$ 1 (black bars) and BMP-7 (gray bars). The percentage of radiolabeled thymidine incorporated after TGF- ${beta}$ 1 or BMP-7 treatment is plotted relative to the level of vehicle-treated cells (set as 100%; open bars). Error bars represent SEs of the mean derived from triplicate determinations per experiment.

We also analyzed whether the six cell types were growth-inhibitedbecause this is a common response of epithelial cells to TGF- ${beta}$ (ten Dijke et al., 2002). Cells were treated with differentdoses of TGF- ${beta}$ 1 or BMP-7, and growth inhibition was estimatedby incorporation of [³H]thymidine (Figure 1B and unpublishedresults). All the epithelial cells tested were growth-inhibitedby TGF- ${beta}$ 1, whereas BMP-7 had a weak effect even at high doses,as expected (Kowanetz et al., 2004). We conclude that normalkeratinocytes exhibit strong growth suppression but relativelyweaker scattering/EMT responses to TGF- ${beta}$ , whereas normal mammaryand lung epithelial cells show both growth inhibition and EMTin relatively good correlation. Furthermore, ligands (such asTGF- ${beta}$ 1) that induce potent EMT also elicit potent growth suppression,whereas ligands (such as BMP7) that induce weak growth arrestare essentially incapable of promoting EMT in normal epithelialcells.

Only type I Receptors of the TGF- ${beta}$ Branch Are Able to Drive EMT in NMuMG Cells
The differential responsiveness of epithelial cells to variousTGF- ${beta}$ members might reflect the repertoire of receptors expressedby those cells or the differential activation of intracellularpathways downstream of the receptors. We investigated thesetwo possibilities in NMuMG cells, because these cells exhibitthe ligand-specific EMT response and thus represent a suitablein vitro model (Figure 1A). We analyzed by RT-PCR the expressionof all seven TGF- ${beta}$ superfamily type I receptors, also known asactivin receptor-like kinases (ALK-1 to -7), and four type IIreceptors (Figure 2A). NMuMG cells express Alk-5 (TGF- ${beta}$ receptortype I), Alk-2 (activin receptor type IA), and Tgfbr2 (TGF- ${beta}$ receptor type II) mRNA. This is in accordance with previousreceptor-ligand cross-linking experiments (Miettinen et al.,1994; Piek et al., 1999b). However, NMuMG cells did not expressdetectable Alk-1 (endothelial TGF- ${beta}$ type I receptor) mRNA. AlthoughNMuMG cells did not undergo EMT in the presence of BMP-7 oractivin-A, they did express at high levels Alk-3 (BMP receptortype IA), and Bmpr2 (BMP receptor type II) mRNA. However, theydid not express detectable Alk-6 (BMP receptor type IB) mRNA.They also expressed high levels of Acvr2 (activin receptor typeIIA) and Acvr2b (activin receptor type IIB), lower mRNA levelsof Alk-4 (activin receptor type IB) but did not express anyAlk-7 (activin receptor type IC) mRNA. Thus, the inability ofactivin-A or BMP-7 to induce robust EMT in NMuMG cells (Figure 1A)cannot be explained by the lack of expression of receptorsfor these ligands.

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Figure 2. All three type I receptors of the TGF- ${beta}$ branch are capable of eliciting EMT. (A) Expression of TGF- ${beta}$ superfamily type I and type II receptors in NMuMG cells. The expression of genes encoding the ALK and type II receptors was analyzed by RT-PCR. Lane M shows markers of molecular size (in kbp, kb). (B) Immunoblot analysis of phospho-Smad2 (Smad2-P) and ${alpha}$ -SMA levels in NMuMG cells. Cells were stimulated with the indicated ligands for 36 h, under the same conditions as in Figure 1A, and total cell extracts were analyzed with antibodies for the indicated proteins (arrows). (C) Effect of constitutively active ALK-3, -4, and -5 receptors on EMT. NMuMG cells were infected with control adenovirus LacZ (Ad-LacZ; MOI 100) or adenoviruses (MOI 100) expressing constitutively active forms of the BMP, activin, or TGF- ${beta}$ type I receptors, and the localization of E-cadherin and ZO-1 was assessed 36 h later. (D) NMuMG cells were infected either with the control adenovirus (Ad-LacZ, MOI 200) or with the adenoviruses expressing the dominant-negative versions of the indicated type I receptors (Ad-ALK(KR), MOI 200) and were treated with vehicle (Control) or TGF- ${beta}$ 1 (2.5 ng/ml) for 36 h. Direct fluorescence microphotographs of the actin cytoskeleton are shown. Bars, (C) and (D) 10 µm; the magnification power of each series of photomicrographs is shown above the bars. (E) NMe cells were infected with Ad-LacZ (MOI 100) or Ad-ALK-5(TD) (MOI 100) and then left unstimulated or stimulated with TGF- ${beta}$ 1 (5 ng/ml), in the presence of vehicle (dimethylsulfoxide) or SB431542 inhibitor (10 µM), and the EMT process was analyzed 48 h later. The levels of endogenous ${alpha}$ -SMA, E-cadherin (E-cadh.), phosphorylated Smad2 (Smad2-P) and Smad3 (Smad3-P), total Smad2 and Smad3, exogenous ALK5(TD), and ${beta}$ -tubulin were determined by immunoblotting. Relevant protein bands (arrows) and background bands (asterisk) are marked.

To confirm the relative inability of activin-A in causing EMTof NMuMG cells, we measured the levels of phosphorylated Smad2,which is an immediate intracellular effector of the pathwaydownstream the type I receptors (Figure 2B). TGF- ${beta}$ 1–3 inducedpotent phospho-Smad2 levels within 30 min of stimulation (unpublishedobservations) that were sustained up to 36 h, at which pointcells exhibit full EMT. In contrast, activin-A showed the samebackground response as vehicle or the negative control used,BMP-7. The Smad2 phosphorylation level reflects directly theEMT process as verified by immunoblot analysis of an establishedmarker of EMT, ${alpha}$ -SMA (Figure 2B). Thus, the relative failureof activin-A in inducing EMT in NMuMG cells correlates withthe poor activation of the Smad pathway, and it must reflecta defective signaling component proximal to the receptors ora very low level of functional receptor.

We then tried to test whether ectopic expression of activinand BMP type I receptors in NMuMG cells could rescue the observedinability of these ligands to induce EMT. We used an adenoviralsystem to transduce transiently all 7 type I receptors of thesuperfamily (in a constitutively active mutant form). EMT wasfollowed by immunofluorescence microscopy of the adherens junctionmarker E-cadherin and the tight junction marker ZO-1 (Figure 2Cand Supplementary Figure 1A). The exogenous type I receptorswere expressed in >95% of the infected cells (SupplementaryFigure 1B), at high levels (Supplementary Figure 1C). Stainingof LacZ-transduced cells demonstrated that infection per sedid not alter epithelial differentiation. Overexpression ofconstitutively active receptors of the BMP branch did not affectthe epithelial phenotype (Figure 2C for ALK-3(QD) and SupplementaryFigure 1A for ALK-1(QD), -2(QD), and -6(QD)). In contrast, constitutivelyactive activin, TGF- ${beta}$ and nodal type I receptors ALK-4(TD), -5(TD),-7(TD) induced a clear EMT (Figure 2C and Supplementary Figure1A). The constitutively active type I receptors were signalingproperly because they induced endogenous Smad1 (BMP receptors)or Smad2 (TGF- ${beta}$ receptors) phosphorylation even at the time (36–48h) at which EMT is fully manifested (Supplementary Figure 1C).Thus, among all type I receptors of the TGF- ${beta}$ superfamily, onlythose of the TGF- ${beta}$ branch were able to induce EMT in NMuMG cells.The activin type I receptor (ALK-4) is therefore sufficientto elicit EMT of NMuMG cells under conditions of ectopic expression.

To test the possibility that endogenous ALK-4 could also contributeto EMT, we overexpressed in NMuMG cells dominant-negative versionsof all type I receptors of the TGF- ${beta}$ superfamily and stimulatedcells with TGF- ${beta}$ 1 (Figure 2D and Supplementary Figure 2A). Dominantnegative ALK-1 to -7(KR) have a lysine to arginine mutationin the kinase active site, which obliterates their enzymaticactivity. Overexpression of ALK-3(KR) receptor (Figure 2D) orALK-1(KR), -2(KR), -6(KR), and -7(KR) (Supplementary Figure2A) did not block EMT induced by TGF- ${beta}$ 1. Only ALK-5(KR), andto a lower extent ALK-4(KR), were able to inhibit EMT inducedby TGF- ${beta}$ 1 (Figure 2D). The exogenous type I receptors were distributedin >95% of the infected cells (Supplementary Figure 2B) andwere expressed at high levels (Supplementary Figure 2C). Moreover,as a specificity control for the dominant-negative activityof the ectopic receptors, we showed that ALK-5(KR), but neitherALK-2(KR) nor ALK-3(KR), were able to block Smad2 phosphorylationinduced by TGF- ${beta}$ 1 (Supplementary Figure 2D). Thus, all the aboveexperiments establish that in addition to ALK-5, also ALK-4and ALK-7 are capable of inducing EMT in NMuMG cells; however,the latter receptor is not expressed at all in NMuMG cells.

We confirmed the above data on type I receptor specificity byusing a low-molecular-weight inhibitor (SB431542), which selectivelyinactivates the ALK-4, -5, and -7 receptors (Inman et al., 2002).NMuMG and their clonal derivatives, NMe cells were treated withTGF- ${beta}$ 1 or infected with the constitutively active ALK-5 adenovirus,in the presence or absence of the SB431542 compound. TGF- ${beta}$ 1 induced ${alpha}$ -SMA expression and robustly down-regulated E-cadherin levels,and SB431542 blocked these effects (Figure 2E). We found thesame results of SB431542 at the morphological level (SupplementaryFigure 3). These experiments also indicated that TGF- ${beta}$ is secretedby NMuMG cells and acts in an autocrine and/or paracrine mannerbecause after treating control cells with the inhibitor, weobserved a stronger epithelial phenotype with more polarizedcuboidal morphology (Figure 2E and Supplementary Figure 3).We confirmed that SB431542 could indeed block the activity ofthe endogenous and exogenous ALK-5 receptors, as it abolishedthe basal and TGF- ${beta}$ 1– or ALK-5(TD)–mediated phosphorylationof Smad2 and Smad3 in NMuMG cells (Figure 2E). Thus, the combinedexperiments with constitutively active type I receptors andSB431542 suggest that EMT of NMuMG cells can be mediated bythe TGF- ${beta}$ branch of pathways in the superfamily.

The Endogenous Smad Pathway Plays Critical Roles in TGF- ${beta}$ –induced EMT
The only signaling effectors known so far to be shared by ALK-4,-5, and -7 receptors are Smad2 and Smad3 (Miyazawa et al., 2002).We previously provided evidence that Smad3, when overexpressedtogether with ALK-5(TD), could enhance synergistically the EMTresponse of NMuMG cells (Piek et al., 1999b). However, thoseexperiments did not establish whether endogenous Smad pathwaysare indeed implicated in the EMT response, a question of importance,as described in the Introduction. Overexpression of a dominant-negativeSmad3(D407E) (Goto et al., 1998) reverted the TGF- ${beta}$ 1 effect ina dose-dependent manner and fully blocked EMT at the highestdose of adenovirus tested (Figure 3, A and B, and SupplementaryFigure 4A). As a control of the potency of dominant-negativeSmad3, we found that Smad3(D407E) partially blocked the dose-dependentgrowth inhibition of NMuMG cells by TGF- ${beta}$ 1 (Supplementary Figure4B). Smad3(D407E) also interfered with the activation of endogenousSmads in NMuMG cells, because it blocked dose-dependently theinducibility of a Smad3/Smad4-specific luciferase reporter,CAGA₉-Luc, by TGF- ${beta}$ 1 (Supplementary Figure 4C). Similar inhibitoryeffects were measured in stably transfected NMuMG cells witha dominant-negative Smad2 mutant (Smad2SA) whose two C-terminalserines were replaced with alanines (Figure 3, C and D, andSupplementary Figure 4D). Empty-vector and wild-type Smad2 transfectedclones served as controls. In mixed pools of transfected NMuMGcells and in two distinct clones per transfectant, we consistentlyobserved only minor enhancement of morphological EMT by wild-typeSmad2 and efficient blocking of the response by Smad2SA (Figure 3Cand Supplementary Figure 4E). Furthermore, induction of Smad2SAeffectively blocked ${alpha}$ -SMA levels in response to TGF- ${beta}$ 1 (Figure 3D).As a control, Smad2SA was shown to block effectively endogenousphospho-Smad2 but not as potently phospho-Smad3 activation byTGF- ${beta}$ 1 (Figure 3D and Supplementary Figure 4F).

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Figure 3. Endogenous Smad pathways mediate EMT in NMuMG cells. (A) NMuMG cells were infected either with Ad-LacZ (MOI 300) or with increasing doses of Ad-Smad3(D407E) (triangle: MOI 20, 100, 300) and were treated with vehicle (Control) or TGF- ${beta}$ 1 (2.5 ng/ml) for 36 h. Localization of ZO-1 was visualized by immunofluorescence. (B) Flag-tagged Smad3(D407E) levels measured by immunoblotting using extracts from cells treated as in A. (C) E-cadherin immunofluorescence microscopy of individual NMuMG stable clones transfected with empty vector pMEP4 (Mock), pMEP4-Smad2, and pMEP4-Smad2(SA). Transfected cells were induced (+) or not (-) with CdCl₂ and subsequently treated with vehicle (Control) or 5 ng/ml TGF- ${beta}$ 1 for 36 h. (D) Immunoblot analysis of endogenous ${alpha}$ -SMA in pools of NMuMG cells stably transfected with empty vector (Mock) or Smad2(SA) and treated under identical conditions as in C. Control immunoblots of endogenous phospho-Smad2 (Smad2-P), exogenous Flag-tagged Smad2 (F-Smad2), and endogenous ${beta}$ -tubulin, which serves as loading reference are also shown. (E) Immunofluorescence microscopy of E-cadherin in NMuMG cells infected with Ad-LacZ (MOI 100) or with Ad-Smad7 (MOI 100) and treated with vehicle (Control) or TGF- ${beta}$ 1 (5 ng/ml) for 36 h. Bars, (A, C, and E) 10 µm; the magnification power of each series of photomicrographs is shown above the bars. (F) Smad7 blocks ${alpha}$ -SMA protein synthesis induced by TGF- ${beta}$ 1. NMuMG cells were infected with Ad-LacZ (MOI 100) or increasing doses of Ad-Smad7 (triangle: MOI 30, 100), and then treated with vehicle (-) or with 5 ng/ml TGF- ${beta}$ 1 (+) for 48 h. The levels of ${alpha}$ -SMA, phosphorylated Smad2 (Smad2-P), exogenous Flag-Smad7 (F-Smad7), and total Smad2 and Smad3 were determined by immunoblotting. In B, D, and F the relevant protein bands are marked with arrows, and an asterisk marks background bands.

We obtained similar but weaker effects using a C-terminallydeleted Smad4(515-ter) (Supplementary Figure 5, A and B). Smad4(515-ter)is found in pancreatic tumors and acts as a dominant-negativeprotein, which is verified here by its effects on TGF- ${beta}$ –inducedgrowth inhibition (Supplementary Figure 5D) and CAGA₉-Luc reporteractivity (Supplementary Figure 5E). The weaker effect of Smad4(515-ter)compared with Smad3(D407E) or Smad2SA is due to the low expressionlevel of the former protein (Supplementary Figure 5C), whichresults from its documented unstable nature (Maurice et al.,2001).

We also tested the inhibitory Smads, Smad6, and Smad7, whichblock endogenous R-Smad activation by type I receptors and canalso mediate receptor degradation (Shi and Massagué,2003). Smad7 overexpression inhibited completely EMT inducedby TGF- ${beta}$ 1 (Figure 3E and Supplementary Figure 6A), as well asthe changes induced by ALK-4(TD), ALK-5(TD), and ALK-7(TD) (SupplementaryFigure 7A). Moreover, Smad7 blocked in a dose-dependent manner ${alpha}$ -SMA induction (Figure 3F). As controls, we showed that Smad7fully blocked NMuMG growth inhibition by TGF- ${beta}$ 1 (SupplementaryFigure 6B) and diminished both the basal and TGF- ${beta}$ 1,-inducedphosphorylation of Smad2 (Figure 3F). In contrast, Smad6, whichmainly blocks the BMP signaling pathways, was not able to blockEMT mediated either by TGF- ${beta}$ 1 or by constitutively active typeI receptors ALK-4, -5, -7 (Supplementary Figure 7A), supportingthe observed Smad effector specificity during EMT.

As a last test of the signaling specificity among TGF- ${beta}$ superfamilypathways that are capable to elicit EMT in NMuMG cells, we ectopicallyexpressed either each R-Smad alone, or together with Smad4,in the presence or absence of constitutively active type I receptors(these data are summarized in Supplementary Figure 7A). We usedALK-4/-5/-7(TD) receptors for the activation of Smad2 and Smad3proteins, and ALK-1/-2/-3/-6(QD) receptors for Smad1 and Smad5.None of the R-Smads when expressed alone transiently via theadenovirus system were able to drive EMT. However, Smad3, andmore weakly Smad2, in combination with Smad4 could induce EMTas previously described (Piek et al., 1999b). In addition, onlySmad2 and Smad3 (together with Smad4) were able to efficientlysynergize with a low dose of each of the three type I receptors,ALK-4(TD), -5(TD), and -7(TD). In contrast, none of the BMP-specificSmad1 or Smad5 could support similar effects on EMT when coexpressedwith several constitutively active type I receptors. We verifiedthe synergistic contribution of Smads together with constitutivelyactive type I receptors on EMT by monitoring the expressionlevels of ZO-1, E-cadherin, and ${alpha}$ -SMA. We present only limiteddata for the effect of Smad3 alone or in combination with Smad4and in the absence or presence of increasing MOI of the ALK-4(TD)receptor (Supplementary Figure 7B). The combined data on thethree protein markers recapitulate rather faithfully the microscopicanalysis of EMT in NMuMG cells (Supplementary Figure 7A).

All the above data showed that interfering with the endogenousSmads using dominant-negative Smad mutants and inhibitory Smadsresulted in inhibition of EMT induced by TGF- ${beta}$ 1 in NMuMG cells.Overexpressing Smad2 and Smad3 could also lead to EMT, whereasthe BMP-specific Smad1 and Smad5 could not. We conclude thatall three Smad proteins of the TGF- ${beta}$ pathway, Smad2, Smad3, andSmad4, are involved in EMT.

Transcriptome Analysis of TGF- ${beta}$ 1–mediated EMT in NMuMG Cells
To understand the mechanisms by which TGF- ${beta}$ 1 alters cellulardifferentiation and leads to EMT in mammary epithelial cells,we used a transcriptomic approach. We focused on the early (2h) and intermediate (8 h) transcriptional events triggered byTGF- ${beta}$ 1 (and leading to EMT) in NMuMG cells. Besides, in orderto define (possibly new) markers of EMT, we analyzed genes differentiallyexpressed in NMuMG cells showing clear EMT after long stimulationwith TGF- ${beta}$ 1 (36 h). Of $~$ 9000 unique genes represented on the mousecDNA chip of 11,500 cDNA elements used, we found 344 independentgenes regulated by TGF- ${beta}$ 1, among which 205 (60%) were up-regulatedand 139 (40%) were down-regulated (Figure 4A; SupplementaryTables 3 and 4). Many of the regulated genes (38%) do not haveany annotation or known function. Among the regulated geneswith clear annotation (213 genes out of 344), we identified28 previously studied TGF- ${beta}$ gene targets and 22 additional genesthat are shared with recent microarray screens of the TGF- ${beta}$ responsein various cell types. The rest 163 gene targets of the pathwayhave not been previously reported. We clustered the regulatedgenes according to their expression profile (K-means method)and inside each cluster we classified the genes according totheir functional annotation (Figure 4, B and C; SupplementaryTables 3 and 4). It is likely that genes that represent markersof EMT belong to clusters 3 and 4, whereas genes that induceEMT are in clusters 1 and 2. This is based on the kinetics ofphenotypic change induced by TGF- ${beta}$ , because no obvious morphologicalchange, alteration in cell-cell adhesion, or tight junctionintegrity can be observed in NMuMG cells earlier than 8–12h poststimulation.

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Figure 4. Summary and clustering of highly regulated genes by TGF- ${beta}$ 1 in NMuMG cells. (A) Venn diagrams of gene expression itemized in three ways, up-regulated genes (left), down-regulated genes (middle), and total regulated genes (right). The three time points (2, 8, and 36 h) are indicated outside each circle, and gene numbers are shown within each section. (B and C) Clustering of highly regulated genes. Up-regulated (B) and down-regulated (C) genes upon TGF- ${beta}$ 1 stimulation were clustered according to their expression profile using the K-means algorithm. Graphs represent the average values of normalized ratios of all genes per cluster plotted with their SEs (ratios of gene expression have no unit). The number of genes belonging to each cluster is indicated.

Among the annotated up-regulated genes, 18% encode functionslinked to the extracellular matrix/cell adhesion/cytoskeletonand are regulated mostly at the late time point. This is inagreement with the EMT process as fibroblastic cells start tosynthesize an extracellular matrix and increase their migratoryproperties. Many cytoskeletal genes are also in agreement withthe observed dramatic reorganization of the cytoskeleton. Wecould also observe changes that support the well-establishedmodel of TGF- ${beta}$ auto-induction (van Obberghen-Schilling et al.,1988). Accordingly, this group includes genes such as the up-regulatedLtbp1, Cd44, Itgb5, Bmp1, and Tgfbr1 that link directly to processesof TGF- ${beta}$ activation and signaling. Approximately 34% of the annotateddown-regulated genes encode functions linked to metabolism/transport/foldingand are regulated between 8 and 36 h (clusters 3 and 4). A substantialproportion of these (15 genes) encode functions linked to redoxregulation and hypoxia regulatory factors. Genes encoding proteinslinked to cell cycle/transcription/apoptosis/development correspondedroughly to 9% of the annotated regulated genes, 63% of thembeing up-regulated and 37% down-regulated, and were enrichedin the corresponding immediate-early clusters 1 and 2. In additionto the known transcriptional program that underlies the growthinhibitory response of epithelial cells to TGF- ${beta}$ (Siegel andMassagué, 2003), we identified a new set of strong candidategenes for the cytostatic program (up-regulated Hrasls3, N4wbp4/Pmepa1,Cks-2, Drp, Gas1, Cfh, and down-regulated Igfbp5, Cxcl1, Ccnd2,Pold1), and few new regulators of the apoptotic response (up-regulatedBag3, Capn2, Tgfb1i4/Tsc-22, Pea15). This functional group alsoincludes several transcription factors, some of which may possiblyregulate genes of the EMT program, including the architecturaltranscription factor Hmga2, the hypoxia-induced factor Hif1a,the Krüppel factor Klf4/Gklf and the Ets family memberEhf. Ongoing studies aim at analyzing the hypothesis that theseproteins are directly involved in EMT.

Functional Validation of TGF- ${beta}$ Target Genes Based on Pathway Specificity, Smad Requirement, and Contribution to EMT
To validate the microarray experiment, we chose a set of highlyregulated genes (Table 1) based on several criteria: 1) highintensity of gene expression (Lmcd1, Ssb-1, Pdgfa, N4wbp4/Pmepa1,Hmga2, and Cxcl1), 2) known TGF- ${beta}$ responsive genes (Tgif, Idb2,Idb3, Myc, and Timp3), 3) known markers of epithelial cells(Krt1–19), and 4) late and possibly novel markers of EMTbased on our literature screen (Zyx, Msn, Muc1, Igfbp5, andFbln2). We assessed the expression of these genes with RT-PCR(Figures 5, A and B, and 7A; unpublished results for Tgif; andKowanetz et al. (2004) for Idb3). In general, we found a verystrong concordance between microarray values of gene expressionand levels measured by semiquantitative RT-PCR for all the genestested.

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Table 1. Selected genes chosen for functional validation

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Figure 5. Differential response of selected gene targets to TGF- ${beta}$ 1 versus BMP-7. Semiquantitative RT-PCR analysis showing the mRNA steady-state levels of 14 selected genes. NMuMG cells were treated (+) or not (-) with 5 ng/ml TGF- ${beta}$ 1 for 2, 8, or 36 h (A and B) or cells were treated with 300 ng/ml BMP-7 for 2, 8, or 48 h (C and D). Expression of down-regulated (A) and up-regulated (B) genes is shown. The classification to down-regulated (C) and up-regulated (D) genes in the BMP-7 experiments is based on gene responsiveness to TGF- ${beta}$ 1. Gapdh serves as a control of equivalent cDNA synthesis, and water and minus RT controls show the specificity of the reactions.

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Figure 7. Id2 inhibits BMP-7 from regulating ${alpha}$ -SMA expression. (A and B) Semiquantitative RT-PCR analysis showing the mRNA steady state levels of Idb2 and control Gapdh. NMuMG cells were treated with vehicle (-), 5 ng/ml TGF- ${beta}$ 1 for 2, 8, and 36 h (A) or 300 ng/ml BMP-7 (+) for 2, 8, and 48 h (B). Water and minus RT controls show the specificity of the reactions. (C) Knockdown of Id2 allows BMP-7 to cause EMT and enhance ${alpha}$ -SMA protein synthesis in a time-dependent manner. NMe clonal cells were transfected with control (siRNA-luc) or specific (siRNA-Id2) and then treated with vehicle (0) or with 300 ng/ml BMP-7 for 8 or 36 h. The levels of endogenous ${alpha}$ -SMA, Id2, and ${beta}$ -tubulin were determined by immunoblotting.

Because we have shown that BMP-7 or BMP type I receptors failto induce EMT (Figures 1 and 2), we hypothesized that genescoregulated by both TGF- ${beta}$ 1 and BMP-7 might not be involved inthe EMT process. We therefore compared the expression of thesame set of genes in the presence of BMP-7 (Figure 5, C and D).BMP-7 did not affect the expression levels of any of thedown-regulated genes tested (Figure 5C). The same was true forall the up-regulated genes tested except Timp3 and Pdgfa, whoseexpression was not induced by BMP-7 at the late time point (48h), a characteristic difference from the TGF- ${beta}$ 1 response (Figure 5C).Furthermore, some of the up-regulated genes showed a transientinduction by BMP-7 at 2 h, which was considerably weaker andnot sustained later compared with the TGF- ${beta}$ 1 response. This mayreflect a transient and physiologically irrelevant responseto the acutely high dose of BMP-7 (150 or 300 ng/ml) used inmost of these experiments. This was done in order to ensuremaximal responsiveness by BMP-7. These experiments allow usto conclude that the differential response of genes to TGF- ${beta}$ versus BMP may prove useful as a means of validation of candidatetargets that play key roles in EMT.

To rapidly validate the involvement of R-Smad activation downstreamof TGF- ${beta}$ 1 in regulation of the selected genes, we used a doublemutant type I receptor that exhibits constitutively active kinasefunction and lacks critical amino acids in its L45 loop, thedocking site for R-Smads. This receptor (ALK5(TD)mL45) is completelyinactive in terms of phosphorylating R-Smads (Figure 6A), butotherwise can elicit downstream signaling via Smad-independentpathways (Yu et al., 2002; Itoh et al., 2003). The ALK5(TD)mL45adenoviral vector was equally ineffective in inducing EMT ofNMuMG cells (unpublished results), or ${alpha}$ -SMA levels (Figure 6A),as the previously published retroviral vectors carrying thesame or equivalent mutations in the L45 loop (Yu et al., 2002;Itoh et al., 2003). This insufficiency correlated tightly withthe failure of this mutant to induce phospho-Smad2 levels. ALK5(TD)mL45receptor rendered NMuMG cells more polarized, mimicking theeffect of the ALK-4/-5/-7 kinase inhibitor described in Figure 2E.Indeed, using ${alpha}$ -SMA as a quantitative marker of EMT, we showedthat increasing MOI of the ALK5(TD)mL45 adenovirus led to agradual decrease of background ${alpha}$ -SMA levels, thus enhancing theevidence that low level of constitutive endogenous TGF- ${beta}$ signalingoperates in NMuMG cells (Figure 6B). These experiments indicatethat the ALK5(TD)mL45 receptor can act as a dominant-negativemutant against endogenous (autocrine) TGF- ${beta}$ receptor signaling.

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Figure 6. Role of the L45 loop of the TGF- ${beta}$ type I receptor in EMT and gene regulation. (A) ALK5(TD)mL45 fails to induce ${alpha}$ -SMA protein synthesis. NMuMG cells were infected with Ad-LacZ (MOI 100) or increasing doses of Ad-ALK5(TD) or Ad-ALK5(TD)mL45 (triangles: MOI 50, 100), or alternatively they were treated with vehicle (-) or with 5 ng/ml TGF- ${beta}$ 1 (+) for 48 h. The levels of endogenous ${alpha}$ -SMA, phosphorylated Smad2 (Smad2-P), and Smad2 and Smad3 and exogenous ALK5(TD) receptors were determined by immunoblotting. The two different receptors are detected using anti-HA and anti-Flag immunoblotting as shown. (B) ALK5(TD)mL45 reduces ${alpha}$ -SMA protein synthesis. NMuMG cells were infected with Ad-LacZ (MOI 100) or increasing doses of Ad-ALK5(TD)mL45 (triangle: MOI 2, 5, 20, 50, 100) for 48 h. The levels of endogenous ${alpha}$ -SMA, exogenous ALK5(TD)mL45 receptor and total Smad2 and Smad3 were determined by immunoblotting. In A and B relevant protein bands (arrows) and background bands (asterisk) are marked. (C) Semiquantitative RT-PCR analysis showing the mRNA steady state levels of nine selected genes from Table 1. NMuMG cells were infected with Ad-LacZ, Ad-ALK5(TD), or Ad-ALK5(TD)mL45 (MOI 100) and then treated with vehicle (-) or with 5 ng/ml TGF- ${beta}$ 1 (+) for 36 h. Gapdh serves as a control of equivalent cDNA synthesis, and water and minus RT controls show the specificity of the reactions.

Next, we measured mRNA expression of the selected genes of Table 1in NMuMG cells stimulated with TGF- ${beta}$ 1 (as control), cells infectedwith Ad-ALK5(TD) or with Ad-ALK5(TD)mL45 (Figure 6C). AlthoughALK5(TD) gave the same response as TGF- ${beta}$ 1, the ALK5(TD)mL45 receptorgave essentially background response, similar to vehicle. Thisis clearly shown for Muc1, Krt1–19, Msn, Fbln2, Hmga2,Lmcd1, N4wbp4/Pmepa1, Pdgfa, and Ssb1 (Figure 6C). The levelsof Hmga2 do not show any regulation by the positive controlALK5(TD) as this gene does not respond after 36 h post-TGF- ${beta}$ 1treatment (Figure 5B), and adenoviral transduction of ALK5(TD)mimics a long-term stimulation (>36 h) with TGF- ${beta}$ 1. Thus,all of the selected genes appear to require an intact L45 loopin the TGF- ${beta}$ type I receptor in order to be properly regulated,suggesting a role of R-Smad activation in their regulation.

One of the target genes identified in this screen, which alsoshowed a distinct mode of regulation by TGF- ${beta}$ 1 versus BMP-7 isthe inhibitor of differentiation Idb2 that encodes for the knownprotein Id2 (Table 1). We have recently established the functionalrole of Id2 (and Id3) in regulation of EMT mediated by TGF- ${beta}$ (Kowanetz et al., 2004). Id2 (and Id3) must be down-regulatedby TGF- ${beta}$ in order for EMT to occur, whereas BMP fails to induceEMT because of the robust induction of the levels of Id proteins.Figure 7, A and B, shows the patterns of Idb2 gene expressionin response to TGF- ${beta}$ 1 and BMP-7 in NMuMG cells. This patternis conserved in many epithelial cell types including HMEC, NHEK,and HaCaT cells and is also faithfully reflected at the proteinlevel (Figure 7C and Kowanetz et al., 2004). To functionallylink one of the EMT markers used throughout this study, ${alpha}$ -SMA,with the Smad-regulated Idb2, we analyzed NMuMG or clonal NMecells transiently transfected with Id2-specific siRNAs thatcould down-regulate endogenous Id2 by 75% and stimulated thecells with BMP-7 (Figure 7C). Under conditions of Id2 knockdown,BMP-7 is capable of inducing significant ${alpha}$ -SMA levels, in a time-dependentmanner, much like TGF- ${beta}$ 1 under normal conditions. This is infull agreement with the fact that partial knockdown of Id2 issufficient to allow BMP-7 to elicit EMT (Kowanetz et al., 2004).We conclude that Id2 could play a primary role in regulatingsome of the genes identified in our primary transcriptomic screen,and we are in the process of testing this hypothesis using morecomplex cDNA microarray analyses.

Evolutionary Conservation of Gene Expression Patterns Downstream of TGF- ${beta}$
In the first part of this study we established that TGF- ${beta}$ canelicit EMT in several epithelial cell types of both mouse andhuman origin (Figure 1A). Two common characteristics of thesecell types were their relatively normal phenotype (as opposedto carcinoma cells) and their ability to be growth inhibitedby TGF- ${beta}$ (Figure 1B). We reasoned that an additional criterionfor validation of the gene targets obtained through our microarrayscreen should be evolutionary conservation of the expressionpatterns, at least between mouse and human epithelial cellsthat exhibit robust EMT responses. We therefore validated theselected gene list in two human cell types, HMEC and HaCaT cellsby monitoring gene expression at 8 and 36 h post-TGF- ${beta}$ 1 treatment(Figure 8A), because higher degree of regulation was obtainedin these two time points in NMuMG cells (Figure 5). HMEC respondto TGF- ${beta}$ 1 with robust EMT, whereas HaCaT could only exhibit weakscattering and cytoskeletal responses (Figure 1A). To controlfor the ability of TGF- ${beta}$ 1 to signal in these two cell types,we measured and confirmed the proper induction of phospho-Smad2levels at comparable levels between the two human cell types(Figure 8, B and C).

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Figure 8. Patterns of gene regulation by TGF- ${beta}$ 1. (A) Expression patterns of 10 selected genes from those tested in Figure 5. Quantitative real-time RT-PCR analysis performed with HMEC and HaCaT cells stimulated (gray bars) or not (white bars) with TGF- ${beta}$ 1 (5 ng/ml) for 8 and 36 h. Normalized values of relative gene expression (arbitrary units) are plotted in bar graphs as described in Materials and Methods. Smad2 phosphorylation status in HMEC (B) and HaCaT (C) cells in response to TGF- ${beta}$ 1 under the identical conditions used for the RT-PCR analysis. Immunoblots for phospho-Smad2 (Smad2-P) and total Smad2 and Smad3 are shown. The relevant protein bands are marked with arrows and an asterisk marks background bands.

This analysis revealed several genes that showed a unique regulatorypattern in mammary epithelial cells, which is conserved amongmice and humans, and is not observed in human keratinocytes.A few genes with a common pattern among mammary cells and keratinocyteswere also observed. Of 14 tested genes, the patterns of generegulation that were observed are summarized in Table 2. Wetherefore suggest that Muc1, Fbln2, Hmga2, Lmcd1, Ssb1, Zyx,and Msn are all newly identified targets of the TGF- ${beta}$ pathwaywhose expression patterns across species, and in response tovarious ligands of the superfamily, suggests that they mightplay functional roles in the process of EMT. We currently testthis prediction experimentally for these seven genes. The comparativeapproach of gene expression we have undertaken, so far has revealedsignificant gene targets and our future aim is to exploit thesetargets in order to establish the process of EMT in normal humanepithelial cells at the molecular level.

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Table 2. Expression patterns of 14 selected target genes

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The role of epithelial plasticity in normal embryogenesis andin carcinoma invasiveness and metastasis is a topic of intensecurrent research (Condeelis and Segall, 2003; Grünert etal., 2003). This emphasizes the need for identification of factorsthat mediate cancer metastasis. EMT characterizes changes inepithelial plasticity and probably represents a transitory stageof carcinoma cell evolution toward aggressive malignancy (Radiskyet al., 2001; Thiery, 2002; Grünert et al., 2003). Changesin epithelial plasticity during carcinoma progression are controlledby epigenetic, environmental, and cell communication mechanisms(Radisky et al., 2001). In this context, secreted growth factorsare of paramount importance, and the TGF- ${beta}$ superfamily includesmany members that contribute to regulation of epithelial plasticityand growth (ten Dijke et al., 2002; Siegel and Massagué,2003). One major task in the analysis of the TGF- ${beta}$ pathway istherefore the molecular dissection of components that contributeto processes such as cell cycle arrest or EMT.

Here we provide a comprehensive analysis of most componentsof the TGF- ${beta}$ superfamily signaling pathways using appropriatemodel cell systems and furthermore identify a group of novelgene targets of this pathway that potentially link basic TGF- ${beta}$ biology to epithelial cell invasiveness. A major conclusionis that EMT is a physiological response of both normal mouseand human epithelial cells to TGF- ${beta}$ . We observed a more robustscattering and depolarization in mammary and lung epithelialcells than in keratinocytes (Figure 1A), which may reflect thedevelopmental history of each tissue type. Despite this, allcell types tested here, as well as several others such as kidney,prostate or lens epithelial cells, undergo EMT (reviewed inGotzmann et al., 2004). The observations in normal keratinocytesare in agreement with another report, which analyzed HaCaT cellEMT in response to TGF- ${beta}$ 1 (Zavadil et al., 2001). Malignant keratinocytesexpressing Ras oncogenes exhibit stronger EMT and architecturaldepolarization, which is mediated by TGF- ${beta}$ and appears more similarto the response described here for normal mammary cells (Portellaet al., 1998). The data also suggest that TGF- ${beta}$ is sufficientto elicit a transient but fully developed EMT response in normalepithelial cells without the need for predisposing oncogenictransformation as documented for the Ras oncogene (Janda etal., 2002; Oft et al., 2002; Grünert et al., 2003). Wealso demonstrate that the in vitro EMT response of normal epithelialcells is conserved between mice and humans. Our data suggestthat NMuMG cells represent a faithful in vitro cell model ofEMT despite the fact that these cells carry no autonomous tumorigenicpotential.

Although the role of TGF- ${beta}$ on modulation of epithelial plasticityand tumor progression has become a major point of current research(ten Dijke et al., 2002; Siegel and Massagué, 2003),the contribution of the other members of the TGF- ${beta}$ superfamilyto such processes remains poorly studied. Using adenovirus-mediatedexpression of all type I receptors of the superfamily we coulddelineate for the first time that only signaling pathways thatbelong to the TGF- ${beta}$ /activin/nodal branch can induce EMT (Figure 2C,Supplementary Figure 1). The low-molecular-weight inhibitorof the three receptor kinases ALK-4, -5, -7, gave evidence forconstitutive autocrine TGF- ${beta}$ signaling that maintains low levelgene expression in NMuMG cells (Figure 2E). Although all threeALK-4(TD), -5(TD), and -7(TD) receptors induced EMT in NMuMGcells, only ALK-5(KR) (and partially ALK-4(KR)) were able toblock TGF- ${beta}$ 1-induced EMT (Figure 2D). This reflects the factthat all three constitutively active receptors can activaterobust Smad2/Smad3 signaling, whereas only ALK-5(KR) can efficientlyinterfere with the function of the endogenous TGF- ${beta}$ receptorcomplex. Because overexpressed activin type I receptor (ALK-4)is able to elicit EMT, we conclude that the failure of activin-Ato induce EMT and Smad2 phosphorylation in NMuMG cells may reflecta suboptimal level of ALK-4 on the cell surface in this celltype.

A corollary from the comprehensive receptor analysis was thatspecific R-Smads, i.e., Smad2 and Smad3, might be involved inthe process of EMT. Indeed, we previously reported a role forSmad3 downstream of TGF- ${beta}$ in NMuMG cell responses (Piek et al.,1999b). We extended our analysis to essentially all Smad componentsof the superfamily, Smad1–7, with the sole exception ofSmad8 for technical reasons (Figure 3, Supplementary Figures4–7). The new results strongly implicate the endogenousSmads of the TGF- ${beta}$ branch in signal transduction that orchestratesthe EMT response. However, a previous report that used stablytransfected NMuMG clones with wild-type Smad7 or a differentdominant negative Smad3 mutant than Smad3(D407E), failed toobserve effects on EMT in response to TGF- ${beta}$ (Bhowmick et al.,2001a). In our hands it has been impossible to obtain stableclones of epithelial cells that express wild-type or mutantSmads constitutively (unpublished results). We either had torely on inducible expression systems (Figure 3C) or on transientadenoviral infections (Figure 3A). Thus, it is possible thatNMuMG clones selected for survival in the continuous presenceof high levels of exogenous mutant Smad3 or Smad7 might adaptby exhibiting differential responses to TGF- ${beta}$ . The data describedhere are in good agreement with several recent reports on therole of Smad4 in mammary EMT and on the ability of transcriptionfactors YY1 and c-ski, which interact and inactivate Smad proteinfunction, to block specifically EMT of NMuMG cells (Kurisakiet al., 2003; Li et al., 2003; Takeda et al., 2004). The dominant-negativeSmad2 and Smad3 mutants used unfortunately have not allowedus to pinpoint possible differential effects between the twoR-Smads of the TGF- ${beta}$ pathway. This is in part due to the factthat these mutants interfere at least partially with both Smad2and Smad3 activation by TGF- ${beta}$ receptors. This has been previouslyestablished for mutant Smad3(D407E) (Goto et al., 1998) butnot for mutant Smad2SA. In the stable clones expressing Smad2SAwe could measure robust phospho-Smad3 levels induced by TGF- ${beta}$ 1(Supplementary Figure 4F). However, this finding does not necessarilyexclude the possibility that the mutant interferes with othercritical signaling effects, e.g., proper receptor-Smad endocytosisand trafficking. The fact that ectopic expression of Smad2 (orSmad3) alone could not elicit robust EMT in NMuMG cells (Figure 3C,Supplementary Figure 7) suggests that the Smad pathway asa whole is needed for this response, in addition to the cooperatingnon-Smad effectors.

The evidence supporting participation of Smads in the establishmentof EMT by TGF- ${beta}$ is also corroborated by the analysis of the ALK-5receptor with mutations in its L45 loop (Figure 6), a resultin full agreement with previous reports that examined the roleof the L45 loop of ALK-5 on EMT of NMuMG cells (Yu et al., 2002;Itoh et al., 2003). Despite this, other evidence has supportedthe role of alternative signaling pathways in the same phenotypicresponse (B

TGF- and the Smad Signaling Pathway Support Transcriptomic Reprogramming during Epithelial-Mesenchymal Cell Transition

TGF- ${beta}$ and the Smad Signaling Pathway Support Transcriptomic Reprogramming during Epithelial-Mesenchymal Cell Transition