BF-1 Interferes with Transforming Growth Factor beta  Signaling by Associating with Smad Partners

doi:10.1128/MCB.20.17.6201-6211.2000

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Molecular and Cellular Biology, September 2000, p. 6201-6211, Vol. 20, No. 17
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

BF-1 Interferes with Transforming Growth Factor $beta$ Signaling by Associating with Smad Partners

Changlin Dou,¹ Jun Lee,¹ Bo Liu,¹ Fang Liu,¹^, Joan Massague,¹^,² Shouhong Xuan,¹^, and Eseng Lai¹^,^*

Cell Biology Program, Memorial Sloan-Kettering Cancer Center,¹ and Howard Hughes Medical Institute,² New York, New York 10021

Received 24 January 2000/Returned for modification 10 March 2000/Accepted 30 May 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The winged-helix (WH) BF-1 gene, which encodes brain factor 1 (BF-1) (also known as foxg1), is essential for the proliferationof the progenitor cells of the cerebral cortex. Here we show thatBF-1-deficient telencephalic progenitor cells are more apt toleave the cell cycle in response to transforming growth factor $beta$ (TGF- $beta$ ) and activin. We found that ectopic expression of BF-1in vitro inhibits TGF- $beta$ mediated growth inhibition and transcriptionalactivation. Surprisingly, we found that the ability of BF-1 tofunction as a TGF- $beta$ antagonist does not require its DNA bindingactivity. Therefore, we investigated whether BF-1 can inhibitSmad-dependent transcriptional responses by interacting with Smadsor Smad binding partners. We found that BF-1 does not interactwith Smads. Because the identities of the Smad partners mediatinggrowth inhibition by TGF- $beta$ are not clearly established, we examineda model reporter system which is known to be activated by activinand TGF- $beta$ through Smads and the WH factor FAST-2. We demonstratethat BF-1 associates with FAST-2. This interaction is dependenton the same region of protein which mediates its ability to interferewith the antiproliferative activity of TGF- $beta$ and with TGF- $beta$ -dependenttranscriptional activation. Furthermore, the interaction of FAST-2with BF-1 is mediated by the same domain which is required forFAST-2 to interact with Smad2. We propose a model in which BF-1interferes with transcriptional responses to TGF- $beta$ by interactingwith FAST-2 or with other DNA binding proteins which functionas Smad2 partners and which have a common mode of interactionwithSmad2.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The neocortex develops from the progenitor cells of the rostral neural plate, the telencephalic neuroepithelial cells. Followinga period of uniform proliferation, cerebral cortical progenitorsgenerate neurons asynchronously beginning at E11 in the mouse.The progenitors undergo asymmetric cell divisions in which onedaughter cell leaves the cell cycle to differentiate while theother continues to divide. The fraction of cells with asymmetricdivisions increases steadily over a period of several days. Towardthe end of the neurogenetic period (E17), both daughter cellsdifferentiate, resulting in depletion of the progenitor pool (2,32). The duration of the neurogenetic period is an importantdeterminant of the number of neurons generated within the cerebralcortex. Thus, the mechanisms which regulate the proliferationof progenitor cells and the timing of their withdrawal from thecell cycle are of central importance in the development of thebrain.

The progenitor cells of the telencephalon are identifiable as early as the eight-somite stage (E8.5) by the expression ofthe Winged-Helix (WH) protein brain factor 1 (BF-1) (also knownas foxg1) (11, 29). WH proteins are a family of putative transcriptionalregulators with diverse roles in development, characterized bya highly conserved DNA binding structure, the WH domain (14,15). We have previously shown that the BF-1 gene plays a criticalrole in the development of the cerebral hemispheres of the brain.Targeted disruption of the BF-1 gene in mice leads to severe defectsin the development of telencephalic structures, e.g., the cerebralcortex and basal ganglia. The loss of BF-1 results in an acceleratedrate of neuronal differentiation and the shortening of the neurogeneticperiod in the embryonic cerebral cortex (37). Although BF-1is expressed by E8.5 in telencephalic progenitors, the disruptionof the BF-1 gene has no apparent effect on the behavior of cerebralcortical progenitor cells until about E11.5, after neuronal differentiationhas begun. These observations suggested that BF-1 may regulatethe response of cerebral cortical progenitors to environmentalcues which act at this stage in development to control their withdrawalfrom the cellcycle.

Transforming growth factor $beta$ (TGF- $beta$ ) and related peptides inhibit the proliferation of many types of epithelial cells in theembryo and are present in the developing brain during the periodof neurogenesis (6, 7, 26). TGF- $beta$ ligands signal throughcell surface receptor kinases, which phosphorylate cytoplasmicSmad proteins. Receptor-specific Smad proteins (24) associatewith Smad4, translocate to the nucleus, and direct transcriptionalactivation by interacting with a DNA binding partner. For theactivin-responsive genes Mix.2 and goosecoid, these partners havebeen identified as the WH proteins FAST-1 (foxh1) and FAST-2 (foxh2),respectively (3, 18, 21). While a number of other DNA bindingpartners of Smad proteins have been discovered, the identitiesof the partners which mediate most TGF- $beta$ responses remainunknown.

We find that isolated telencephalic progenitor cells from BF-1^/ mutant embryos have an increased sensitivity to growth inhibitionby TGF- $beta$ and activin compared with cells from their normal littermates.BF-1^/ mutant embryos yield a limited number of neuroepithelial cells,making biochemical studies impractical. To investigate the mechanismsby which BF-1 regulates cellular responses to TGF- $beta$ , we developedcell lines with inducible expression of BF-1 and used an in vitrotranscriptional reporter system in these cells. The mink lungepithelial cell line Mv1Lu was selected because the TGF- $beta$ signaltransduction pathway is well characterized in this line. Usingthis model system, we found that BF-1 antagonizes the antiproliferativeactivity of TGF- $beta$ and inhibits TGF- $beta$ -dependent transcriptionalactivation. Unexpectedly, we discovered that the DNA binding activityof BF-1 is not required for these functions, raising the possibilitythat BF-1 might act by interacting with components of the TGF- $beta$ signaling pathway. We provide evidence that BF-1 can form a complexin the cell with the Smad partner FAST-2. Studies to characterizethe functional regions of the BF-1 protein revealed a common domainwhich is required to antagonize the antiproliferative activityof TGF- $beta$ , to inhibit TGF- $beta$ -dependent transcriptional activation,and to interact with FAST-2. These observations, together withthe identification of the domain in the FAST-2 protein which mediatesits interaction with BF-1, lead to a model in which BF-1 interfereswith multiple TGF- $beta$ responses by associating with DNA bindingproteins which function as Smadpartners.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Constructs. Site-directed mutagenesis (pALTER; Promega) of the mouse BF-1 cDNA (33) was used to create a PvuII restriction site at thebeginning of the translated sequence, permitting the insertionof BF-1 into the expression vectors pFlag-CMV2 (Eastman Kodak)and Myc-tagged CS2 vector, beginning with the second amino acid.The BF-1(NH-AA) mutant (see Results) was generated by site-directedmutagenesis, creating a novel StuI site. Mutated plasmids werecompletely sequenced. Myc-tagged FAST-2 constructs were preparedby inserting FAST-2 cDNA clones 1.2 (encoding amino acids 9 to401) and 12.1 (encoding amino acids 52 to 401) into the CS2 vectordownstream of Myc epitopes (21). A3-luc reporter constructswere kindly provided by M. Whitman (3, 4). All other constructshave been described previously (12, 22, 35).

Isolation and culture of primary neuroepithelial cells. The genetic background of the mice used in these studies (C57BL6) differs from that of the mice used in earlier studies (mixed129 and C57BL6). While no significant differences are noted inthe brain phenotype, the gestation period of the mice is 1 daylonger, with mice being born at E19.5 instead of E18.5. This isassociated with slower development of the embryos. Embryos atE13.5 are comparable in size and developmental stage to thosepreviously obtained at E12.5, while embryos at E10.75 are equivalentto those previously obtained atE10.

Telencephalic neuroepithelial cells were isolated from E10.75 mouse embryos by a method modified from that of Kilpatrick andBartlett (16). Embryos from BF-1^+/ × BF-1^+/ heterozygote matings were dissected in ice-cold phosphate-bufferedsaline. The epidermis of the head was removed, and the head wastreated with pancreatin-trypsin on ice for 30 to 45 min. The mesenchymewas separated from the neural tube, and the neuroepithelium ofthe telencephalon was dissected. The isolated neuroepitheliumwas treated with 0.025% trypsin and 0.001% DNase I for 7 min todissociate the cells. The cells were washed with Dulbecco's modifiedEagle's medium (DMEM)-10% fetal bovine serum (FBS) followed byDMEM-F12 (1:1) supplemented with 2 mM L-glutamine, 6 mg of glucoseper ml, N2 supplements, and 1% FBS. They were then plated ontopoly-L-lysine- and laminin-coated 48-well plates at 10,000 to40,000 cells/well in DMEM-F12 supplemented with 20 ng of fibroblastgrowth factor 2 per ml of FGF-2 and TGF- $beta$ or bone morphogeneticprotein 4 (BMP4) at 100 pM as indicated in duplicatewells.

Luciferase and $beta$ -gal assays. Mv1Lu cells were transfected with Lipofectamine (GIBCO BRL) and treated with 100 pM TGF- $beta$ 1 (R&D Systems) for 18 to 24 h. Luciferaseactivity was measured with a luciferase assay kit (Promega), and $beta$ -galactosidase ( $beta$ -gal) activity was measured with a chemoluminescencedetection kit from Tropix. In some cases, cell lysates were alsoanalyzed by Western blotting to check the expression of transfectedvectors under differentconditions.

RT-PCR. Total RNA from neuroepithelium or cell lines was prepared with Tri-reagents and reverse transcribed with random hexamers andSuperscript II reverse transcriptase (GIBCO-BRL). TGF- $beta$ receptormRNAs were amplified with the primer pairs 5'-GTC CGC AGC TCCTCA TCG TGT TG-3' and 5'-GGT GGT GCC CTC TGA AAT GAA AG-3' forTGF $beta$ RI and 5'-CCC GGG GCA TCG CTC ATC TC-3' and 5'-AAT TTC TGGGCG CCC TCG GTC TCT-3' for TGF $beta$ RII. Glyceraldehyde-3-phosphatedehydrogenase was amplified using the primers 5'-GTG GCA AAG TGGAGA TTG TTG CC-3' and 5'-GAT GAT GAC CCG TTT GGC TCC-3', and activinreceptor type IIB was amplified using 5'-TCC CTA CGG CCA TGT GGACAT CCA-3' and 5'-ATG CAG GTA TGA GAG GCC TCG TGA-3'. Amplificationwas performed for 30cycles.

Generation of BF-1-inducible Mv1Lu cell lines. To construct a vector in which the BF-1 coding sequence is under the control of the tetracycline operator, the SstI-StuI fragmentof BF-1 cDNA clone mN3 (33), which encodes the full-length BF-1protein, was inserted to the XbaI site of pUHD-10-3-hygromycinplasmid (28). The pUHD-10.3-hygromycin-BF-1 plasmid was transfectedwith Lipofectamine into Mv1Lu (14tTA) cells, in which the tTAexpression vector is stably integrated. The transfected cellswere cultured in selection medium containing 1 mg of G418 (GIBCOBRL) per ml and 0.3 mg of hygromycin (Boehringer Mannheim) perml. The medium was changed every 2 days for 2 weeks. The colonieswere ring-cloned, and each colony was analyzed by Western blottingwith polyclonal antibody against the BF-1 N terminus (BNF1; 1:1,000).Of 32 clones we analyzed, 8 had high levels of BF-1 expression,10 had moderate levels of BF-1, and 14 had undetectable BF-1 expression.Clone 8 is one of the high-level expressers. A mutant form ofBF-1, BF-1(NH-AA), and several Flag-tagged BF-1 constructs werealso transfected into 14tTA cells to yield various stable celllines. Lines with comparable protein expression as monitored byWestern blotting with anti-Flag antibody were selected for furtherstudies.

Mv1Lu cells were maintained in minimal essential medium supplemented with 2 µg of tetracycline per ml and 10% FBS along withantibiotics and L-glutamine. COS1 cells were cultured in high-glucoseDMEM (DMEM HG) supplemented with 10% FBS, L-glutamine, and antibiotics(excludingtetracycline).

[³H]thymidine incorporation assay. (i) Mv1Lu cells. Cells in 24-well plates were labeled with [³H]thymidine (2 µCi/well) (Amersham) in serum-free medium for 2 h. At the end ofthe labeling step, the cells were washed with phosphate-bufferedsaline and lysed in 0.5 ml of 0.5% sodium dodecyl sulfate. Celllysates were mixed with an equal volume of 20% cold trichloroaceticacid and left on ice for at least 30 min. The mixture was filteredthrough a fiberglass filter and washed sequentially with 10% trichloroaceticacid and 95% ethanol. Filters were then dried and counted in 5ml of EconoFluor 2 (DuPont) scintillation fluid. Counts from triplicatewells were averaged andplotted.

(ii) Primary neuroepithelial cells. Cells in a 48-well plate were cultured for 18 h and then labeled with [³H]thymidine (2 µCi/well in 200 µl) in growth medium for 6 h. Thecells were washed and lysed as described above. Counts from duplicatewells were averaged andplotted.

Contact release assay. Mv1Lu cells were cultured to confluence and then maintained at confluence for another 5 days to achieve quiescence in thepresence of 2 µg of tetracycline per ml. The cells were then replatedat a 1:5 ratio to release them from contact inhibition. [³H]thymidine incorporation was measured 15 h after replating. Whenadded, TGF- $beta$ 1 at a final concentration of 100 pM was suppliedat the time of replating. Induction of BF-1 was achieved by withdrawalof tetracycline 48 h prior toreplating.

T2 RNase protection assay. Total RNA was prepared from BF-1-induced and uninduced Mv1Lu cells by using Tri-reagent as specified by the manufacturer (MolecularResearch Center, Inc.). Total RNA (10 µg) in 100 µl of 70% ethanolwas mixed with ³²P-labeled p15ink4b riboprobe (10⁹ cpm/µg) and 3,000 cpm of low-specific-activity (10⁷ cpm/µg) mouse glyceraldehyde-3-phosphate dehydrogenase (Ambion)internal control riboprobe. The mixture was precipitated with70% ethanol and redissolved in 25 µl of 80% formamide 1× hybridizationbuffer [40 mM piperazine-N,N'-bis(2-ethanesulfonic acid) (PIPES;pH 6.4), 400 mM NaCl, 1 mM EDTA]. Hybridization was performedby first denaturing the mixture at 80°C for 10 min and then hybridizingit overnight at 60°C. At the end of the hybridization, 300 µlof T2 RNA endonuclease (GIBCO BRL) digestion buffer (50 mM sodiumacetate [pH 4.6], 100 mM NaCl, 2 mM EDTA) was added to the hybridmixture, which was then incubated for 2 h at 30°C. The digestedproducts were ethanol precipitated, denatured, and resolved ina 7 M urea-6% polyacrylamidegel.

Gel mobility shift assay. Proteins comprising the BF-1 binding domain (BD) and BF-1 BD mutation (NH-AA) were made by in vitro translation using reticulocytelysates (GIBCO BRL). The DNA binding assay was performed with1 ng of radiolabeled S2 probe essentially as described previously(33).

Immunoprecipitation and immunoblotting. COS1 cells were cotransfected with various Flag- or Myc-tagged expression vectors by the DEAE-dextran method. Cells receivingTGF- $beta$ treatment were also transfected with a constitutively activeTGF- $beta$ receptor, T $beta$ R-I (T204D) (35). At 40 to 48 h after transfection,the cells were treated with low-serum medium (DMEM-HG plus 0.2%FBS), plus or minus 0.5 nM TGF- $beta$ , for 1 h and then lysed in 1ml of TNE buffer (10 mM Tris [pH 8.0], 0.15 M NaCl, 1 mM EDTA,1% NP-40) plus protease inhibitors. Cell lysates were preclearedwith protein A- and G-coupled agarose beads and incubated withMyc (9E10; Santa Cruz Biotechnology) or M2 Flag (Eastman Kodak)monoclonal antibodies for 3 h. Immunoprecipitates and aliquotsof cell lysates before immunoprecipitation were separated on sodiumdodecyl sulfate-7 or 12% polyacrylamide gel and transferred toan Immobilon-P membrane. The membrane was then probed with Flag(0.8 µg/ml) or Myc (50 ng/ml) antibody and incubated with horseradishperoxidase-conjugated goat anti-mouse antibody and detected bychemiluminescence(Pierce).

Immunodetection of retinoblastoma protein (Rb) was performed with anti-Rb monoclonal antibody G3-245 (1 µg/ml; Pharmingen)and horseradish peroxidase-conjugated goat anti-mouse immunoglobulinG (Pierce) and chemiluminescence detection(Pierce).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Telencephalic progenitor cells lacking BF-1 are more responsive to growth inhibition by TGF- $beta$ and activin. To test the possibility that BF-1 regulates the response of neural progenitors to extracellular signals, we examined [³H]thymidine incorporation in cells isolated from the dorsal telencephalonof E10.75 BF-1^/ mutant embryos and littermates. Cells from embryos at E10.75were selected for study because at this age the BF-1^/ mutants are indistinguishable from wild-type (WT) and BF-1^+/ heterozygous embryos. The dorsal telencephalic neuroepitheliumwas dissected, separated from the adjacent mesenchyme, dissociatedinto single cells, and plated. We routinely obtained populationsof cells in which >80% were derived from the telencephalon, asmonitored by staining for $beta$ -gal activity in the BF-1^+/ heterozygote and the BF-1^/ mutant (Fig. 1A). Cells from these embryos expressed $beta$ -gal underthe control of the BF-1 promoter. Therefore, the $beta$ -gal stainingshows that the cells are of telencephalic origin. The variabilityin staining intensity between cells may reflect the gradient ofBF-1 expression within the telencephalon. The higher overall stainingintensity in the mutant cells can be attributed to the fact thateach cell has two copies of the $beta$ -gal gene whereas the heterozygouscells have only one copy.

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FIG. 1. Telencephalic neuroepithelial cells from BF-1 homozygous mutant embryos are more sensitive to growth inhibition by TGF- $beta$ . (A) Neuroepithelial cells isolated from E10.75 BF-1^+/ heterozygous and BF-1^/ mutant embryos were cultured for 24 h and stained with 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside (X-Gal) and nuclear fast red. Cells staining blue are telencephalic neuroepithelial cells with activated BF-1 promoter. Strong and weak staining indicates cells with high and low BF-1 promoter activity, respectively. Bar, 25 µm. (B) RT-PCR for TGF- $beta$ receptor type I and II and activin receptor type IIB from RNA isolated from neuroepithelial cells. (C) Neuroepithelial cells isolated from WT, BF-1^+/ and BF-1^/ embryos were cultured in the presence or absence of TGF- $beta$ or BMP4 (both at 100 pM) for 24 h. Control medium included 1% FBS and 20 ng of FGF-2 per ml. [³H]thymidine was added during the last 6 h, and the amount of [³H]thymidine incorporated was determined as described in Materials and Methods. The [³H]thymidine counts from duplicate wells of a representative experiment were normalized to the cell number. (D) The inhibition of [³H]thymidine incorporation by TGF- $beta$ , activin, or BMP4 (mean ± standard error) is reported.

FGF-2 promotes the survival and proliferation of neuroepithelial cells (16). [³H]thymidine incorporation is similar in WT and in BF-1^+/ heterozygotes and BF-1^/ homozygous mutants in telencephalic progenitors in the presenceof both FGF-2 and 1% FBS (Fig. 1C, columns 1, 4, and 7). Verylittle [³H]thymidine incorporation was observed when cells were culturedin media with FGF-2 or serum alone (data not shown). These resultsshow that at E10.75, the loss of BF-1 function does not substantiallyalter the ability of the cerebral cortical progenitors to proliferatein response to growth factors. Next, we investigated the responseof cerebral cortical progenitors to TGF- $beta$ , activin, and BMP4.We found that telencephalic progenitor cells from WT and BF-1^+/ heterozygotes were not growth inhibited by TGF- $beta$ (Fig. 1C andD) while those from BF-1^/ mutant embryos showed a 40% inhibition of [³H]thymidine incorporation in response to TGF- $beta$ . Activin also hada greater antiproliferative activity on mutant cells, reducing[³H]thymidine incorporation by 66% versus 33 to 40% in progenitorcells isolated from normal littermates (Fig. 1D). By comparison,BMP4 inhibited [³H]thymidine incorporation to a similar level in all three populationsof cells (Fig. 1C and D). We showed by RT-PCR that receptors forTGF- $beta$ and activin were present in the telencephalic neuroepitheliumat this stage in development in WT as well as BF-1^/ mutant embryos (Fig. 1B).

BF-1 antagonizes TGF- $beta$ -mediated growth arrest in cultured cells. To facilitate studies of how BF-1 controls cellular responses to TGF- $beta$ , we developed a model system, a mink lung epithelialcell line (Mv1Lu) with tetracycline transactivator (9)-inducibleexpression of BF-1 (clone 8). Another line (clone 7), which doesnot express ectopic BF-1, was used as a control. Expression ofBF-1 did not alter the growth rate (data not shown), indicatingthat ectopic BF-1 does not directly stimulate cell proliferationand is not toxic to the cells. However, BF-1 expression resultedin reduced responsiveness to growth inhibition by TGF- $beta$ (Fig.2A). BF-1 expression also overcame the ability of TGF- $beta$ to blockreentry into the cell cycle in cells released from contact inhibition(Fig. 2B, upper panel). Growth inhibition by TGF- $beta$ is associatedwith its ability to block Rb hyperphosphorylation (19). We observedthat ectopic expression of BF-1 in Mv1Lu cells resulted in thehyperphosphorylation of Rb even when these cells were exposedto TGF- $beta$ (Fig. 2B, middle panel).

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FIG. 2. (A) BF-1 blunts the growth-inhitory activity of TGF- $beta$ . (Inset) Western blot analysis with anti-BF-1 antibody. BF-1 is expressed in clone 8 (lane 2) upon tetracycline withdrawal but not in clone 7 (lane 4). Exponentially growing cells not expressing BF-1 are growth inhibited by TGF- $beta$ . Induction of BF-1 (clone 8, $-$ Tet) results in a reduced response to TGF- $beta$ . [³H]thymidine incorporation in cells exposed to TGF- $beta$ is expressed as a percentage of that in cells not exposed to TGF- $beta$ . (B) [³H]thymidine incorporation in cells released from contact inhibition in the presence or absence of TGF- $beta$ is shown in the top panel. Cells were cultured for 5 days at contact density to achieve quiescence. BF-1 expression was induced by withdrawal of tetracycline for 48 h prior to replating cells with or without TGF- $beta$ (100 pM) for 15 h. When BF-1 is expressed, [³H]thymidine incorporation is increased 10-fold (compare lanes 2 and 4). Hyperphosphorylation of Rb in BF-1-expressing cells treated with TGF- $beta$ is shown in the middle panel. Western blot analysis with anti-Rb antibody was performed to determine the amount of hyperphosphorylated (Rb-P) and hypophosphorylated (Rb) forms of Rb in these cells. BF-1 overcomes inhibition of Rb phosphorylation by TGF- $beta$ (lanes 2 and 4); an RNase protection assay for p15ink4b is shown in the bottom panel. Induction of p15ink4b by TGF- $beta$ is reduced in the presence of BF-1 (lane 4). (C) A 2-amino-acid substitution in the WH domain of BF-1 disrupts DNA binding activity. The DNA binding domain (WH domain) of BF-1 or the WH domain with the NH-AA mutation was expressed by translation in reticulocyte lysates. A gel mobility shift assay demonstrates high-affinity binding of the WT BF-1 protein to the S2 double-stranded oligonucleotide (lane 1). This binding activity is abolished by the NH-AA mutation (lane 2). (D) BF-1(NH-AA) antagonizes TGF- $beta$ -mediated cell cycle arrest (top panel). Cells cultured with tetracycline to repress BF-1(NH-AA) are inhibited from reentering S phase by TGF- $beta$ upon replating at low density (lanes 1 and 2). When BF-1(NH-AA) expression is induced, TGF- $beta$ is unable to inhibit [³H]thymidine incorporation. BF-1(NH-AA) inhibits the induction of p15ink4b expression by TGF- $beta$ (bottom panel). An RNase protection assay for p15ink4b expression is shown. TGF- $beta$ induction of p15ink4b expression is reduced in the presence of BF-1(NH-AA) (compare lanes 2 and 4).

A mutation of BF-1 which abolished DNA binding does not alter its ability to antagonize TGF- $beta$ . Because BF-1 has previously been shown to function as a transcriptional repressor (20), we tested whether DNA binding activitywas essential for inhibiting the activity of TGF- $beta$ . Based on thestructure of HNF-3 $gamma$ complexed with DNA (5), we designed a mutationin the WH domain of BF-1 of two residues, N165 and H169, predictedto be involved in critical contacts with DNA. Mutation of thesetwo amino acids to alanine (NH-AA mutant) abolished DNA bindingactivity in reticulocyte lysates expressing the mutant bindingdomain (Fig. 2C).

To examine the role of DNA binding in BF-1 function, we generated an Mv1Lu cell line in which BF-1 containing the NH-AA mutation,BF-1(NH-AA), was expressed under the control of the tetracyclinetransactivator. The mutant BF-1 protein was expressed at levelscomparable to the expression of WT BF-1 in clone 8 (describedabove) but lacked DNA binding activity (data not shown). We foundthat the mutant protein is active in antagonizing TGF- $beta$ activity.Expression of BF-1(NH-AA) promoted entry into S phase in the presenceof TGF- $beta$ (Fig. 2D, upper panel, lane 4), suggesting that BF-1interferes with TGF- $beta$ activity through a mechanism independentof DNAbinding.

BF-1 inhibits TGF- $beta$ -dependent gene expression. To determine whether BF-1 interferes with TGF- $beta$ -dependent gene expression, we examined the effect of ectopic BF-1 on the inductionof the cyclin-dependent kinase (CDK) inhibitor p15. Increasedexpression of p15 in response to TGF- $beta$ results in the inhibitionof CDK activity and blockade of Rb phosphorylation by G₁ cyclin-dependentkinases (10, 28). In Mv1Lu cells expressing BF-1 (Fig. 2B,lower panel) and BF-1(NH-AA) (Fig. 2D, lower panel), inductionof p15 mRNA levels by TGF- $beta$ was inhibited. The regulation of thep15 promoter is not well understood. Therefore we examined a well-characterizedTGF- $beta$ -responsive promoter, the A3-luc reporter, as a model togain further insight into how BF-1 may be interfering with TGF- $beta$ activity. A3-luc has previously been shown to be activated inMv1Lu cells by TGF- $beta$ or activin in a Smad2-Smad4- and FAST-2-dependentmanner (4, 22). We found that BF-1 inhibited TGF- $beta$ -inducedtranscriptional activation of the A3-luc reporter gene by about75 to 85% without inhibiting the expression of FAST-2 (Fig. 3A).The BF-1(NH-AA) mutant also blocked the activation of the A3-lucreporter (Fig. 3C).

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FIG. 3. Transcriptional activation by TGF- $beta$ is inhibited by BF-1. (A) The A3-luc reporter construct, Rous sarcoma virus (RSV)- $beta$ -gal, and Myc-FAST-2 were cotransfected into Mv1Lu cells with or without BF-1 expression vector. The cells were treated with 100 pM TGF- $beta$ for 24 h before being harvested for luciferase and $beta$ -gal assays. Luciferase activity was normalized to cotransfected RSV- $beta$ -gal expression. The mean and standard error from duplicate wells is plotted. Very little luciferase activity is detected in the absence of FAST-2 (lane 1). FAST-2 causes a 40-fold transcriptional activation by TGF- $beta$ (lane 2). Increasing amounts of cotransfected BF-1 (50 and 100 ng) inhibit FAST-2-mediated A3 luc reporter expression (lanes 3 and 4). In the lower panel, cell lysates from the same experiment were subjected to Western blotting with anti-Myc antibody to monitor the expression levels of FAST-2. (B) BF-1 does not inhibit VD-luc reporter expression. VD-luc reporter, RSV- $beta$ -gal, and VD receptor were cotransfected into Mv1Lu cells in the presence or absence of BF-1. The cells were treated with VD (10 nM) or left untreated for 24 h before being harvested. Data were analyzed and plotted in the same way as described for panel A. (C) Inhibition of TGF- $beta$ - and FAST-2-dependent activation of A3-luc by levels of BF-1 which do not interfere with cell proliferation (see also Fig. 2B). Clone 8 (Fig. 2A) Mv1Lu cells were cultured with tetracycline (lanes 1, 3, and 4) or without tetracycline to induce BF-1 expression (lane 2). Inhibition by induced BF-1 is comparable to that achieved by cotransfection with an expression plasmid for WT BF-1 (lane 3) or BF-1(NH-AA) (lane 4).

In our studies with transfected cells, we limited the levels of expressed BF-1 so that transcription was not globally repressed.Under these conditions, BF-1 did not inhibit either the basalor vitamin D (VD)-dependent transcriptional activation of a VDreceptor-responsive promoter (Fig. 3B). In contrast, BF-1 wasobserved to reduce expression from the A3-luc reporter by 25 to40% in the absence of TGF- $beta$ . This effect was dependent on thepresence of the FAST-2 response elements (Fig. 3A and C). We alsofound that the induced BF-1 levels achieved by tetracycline withdrawalin clone 8 Mv1Lu cells are sufficient to inhibit A3-luc activationby TGF- $beta$ (Fig. 3C, lanes 2 and 3). These levels of BF-1 did notinterfere with normal cell growth, indicating that transcriptionis not globally inhibited in these stably transfected cells. Takentogether, these results suggest that inhibition of TGF- $beta$ -dependenttranscriptional activation by BF-1 is mediated through a specificmechanism.

BF-1 associates with FAST-2. To investigate DNA binding-independent mechanisms of BF-1 action, we looked for interactions between BF-1 and components ofTGF- $beta$ signal transduction pathways. Because BF-1 is a nuclearprotein, we focused our attention on proteins which can act inthe nucleus. We detected no interaction between BF-1 and Smad1,Smad2, Smad3, or Smad4 (data not shown), and so we investigatedwhether BF-1 might interact with the DNA binding partners of Smadproteins. Because we could demonstrate an effect of BF-1 on FAST-2and TGF- $beta$ -dependent transcriptional activation of the A3-luc reporter,we looked for an interaction between BF-1 and FAST-2. Flag-taggedBF-1 and Myc-tagged FAST-2 were found to coimmunoprecipitate whenexpressed together in COS cells with either anti-Flag (Fig. 4A)or anti-Myc (Fig. 4B) antibody. The expression levels of eachof the constructs were monitored by Western analysis. Controlswith other epitope-tagged proteins and alternately tagged BF-1and FAST-2 demonstrated that the interaction was not mediatedby the epitope tags (data not shown). The efficiency of coimmunoprecipitationfor BF-1 and FAST-2 was similar to that observed for Smad2 andFAST-2 (Fig. 4A, lanes 2 and 5). The interaction between BF-1and FAST-2 was reduced upon exposure of the cells to TGF- $beta$ (lanes2 and 3), while the Smad2-FAST-2 interaction was enhanced (lanes4 and 5). To delineate the region of the FAST-2 protein whichis required for association with BF-1, we examined the abilityof BF-1 to coimmunoprecipitate a series of truncated FAST-2 proteins(Fig. 4B). Deletions which disrupted the C-terminal Smad interactiondomain abolished the association with BF-1.

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FIG. 4. BF-1 associates with FAST-2. (A) Comparison of the association between FAST-2 and BF-1 with the association of FAST-2 and Smad-2. Flag-tagged BF-1, Flag-tagged Smad2, and Myc-tagged FAST-2 were transfected into COS cells as indicated. BF-1 and Smad2 coimmunoprecipitate with FAST-2 with similar efficiencies in the absence of TGF- $beta$ . TGF- $beta$ treatment reduces the association of FAST-2 with BF-1 and enhances its association with Smad2. (Top panel) Cell lysates were immunoprecipitated with anti-Flag antibody and blotted with anti-Myc antibody. (Middle panel) Western blot of cell lysates with anti-Myc antibody. (Bottom panel) Western blot of cell lysates with anti-Flag antibody. (B) Flag-tagged BF-1 was transfected into COS1 cells alone or with several different Myc-tagged FAST-2 constructs. (Top panel) Western blot of cell lysates immunoprecipitated with anti-Myc antibody and probed with anti-FLAG antibody. (Middle panel) Western blot of cell lysates with anti-Flag antibody. (Bottom panel) Western blot of cell lysates with anti-Myc antibody. (C) Requirement of amino acids 314 to 372 in BF-1 for antagonism of TGF- $beta$ activity and association with FAST-2. Myc-tagged FAST-2 alone or with different Flag-tagged BF-1 constructs was transfected into COS1 cells. (Top panel) Western blot of cell lysate immunoprecipitated with anti-Flag antibody and probed with anti-Myc antibody. (Middle panel) Western blot of cell lysates with anti-Myc antibody. (Bottom panel) Western blot of cell lysates with anti-Flag antibody.

The same region of the BF-1 protein is required to antagonize TGF- $beta$ activity and to associate with FAST-2. To evaluate whether the activities of BF-1 (i) to antagonize the antiproliferative activity of TGF- $beta$ , (ii) to inhibit transcriptionalactivation by TGF- $beta$ , and (iii) to associate with FAST-2 are related,we compared the structural requirements of each of these functions.Examination of a series of stable cell lines in Mv1Lu, expressingmutants of the BF-1 protein, revealed that a region of BF-1 adjacentto the WH domain (amino acids 276 to 372) was required to antagonizegrowth inhibition by TGF- $beta$ (Fig. 5B and 6). This region of BF-1was also required for inhibition of TGF- $beta$ and FAST-2-dependenttranscriptional activation from the A3-luc reporter (Fig. 5C and6). Each of the BF-1 polypeptides was Flag tagged to permit quantitationof their expression levels (Fig. 5A). The Flag epitope did notalter the activity of the full-length BF-1 protein (compare Fig.3C and Fig. 5C). We then determined which region of BF-1 was requiredfor association with FAST-2. The DNA binding activity of BF-1was not required for its interaction with FAST-2 (Fig. 4C, lane10). However, mutations of BF-1 which abolish its ability to antagonizeTGF- $beta$ activities, e.g., growth inhibition and stimulation of A3-luctranscription, also destroy its ability to associate with FAST-2(Fig. 4C, lanes 12 to 15; summarized in Fig. 6). Further studiesshowed that deletion of amino acids 276 to 313 in BF-1 did notaffect its ability to antagonize TGF- $beta$ -mediated transcriptionalactivation or to associate with FAST-2 (Fig. 6). These resultsnarrow the critical domain in BF-1 required for interference withTGF- $beta$ signaling to amino acids 314 to 372. Our data do not excludethe possibility that BF-1 and FAST-2 interact through an intermediaryprotein.

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FIG. 5. Four Mv1Lu cell lines with inducible expression of different Flag-tagged BF-1 constructs (A) were used in growth inhibition (B) and A3-luc reporter (C) assays. (A) Expression of Flag-tagged BF-1 (F-BF-1) (lanes 1 and 2) and three deletion mutants of BF-1 (F- $Delta$ 373-480 [lanes 3 and 4], F- $Delta$ 276-372 [lanes 5 and 6], and F- $Delta$ 1-149 [lanes 7 and 8]) was induced by tetracycline withdrawal and monitored by Western blotting. (B) Inhibition of [³H]thymidine incorporation by TGF- $beta$ is antagonized by Flag-tagged BF-1 and F- $Delta$ 1-149 (lanes 2 and 8) and partially antagonized by F- $Delta$ 373-480 (lane 4). F- $Delta$ 276-372 is inactive in this assay (lane 6). (C) Activation of the A3-luc reporter by TGF- $beta$ in Mv1Lu cells cotransfected with FAST-2 is inhibited by Flag-tagged BF-1 and F- $Delta$ 1-149 (lanes 2 and 8) and partially inhibited by F- $Delta$ 373-480 (lane 4). F- $Delta$ 276-372 is inactive in this assay (lane 6).

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FIG. 6. Schematic diagram of BF-1 constructs used in the experiments in Fig. 4 and 5B and C. The relative efficiency of each construct in coimmunoprecipitating FAST-2 is compared with their ability to inhibit TGF- $beta$ -stimulated A3 luc reporter expression and to antagonize the growth-inhibitory activity of TGF- $beta$ . ++, strong activity; +, low to moderate activity; $-$ , no activity; nd, not determined. The asterisk indicates that the BF-1(NH-AA) protein in this stable cell line is not Flag tagged.

BF-1 can interfere with the association between FAST-2 and Smad2. Because the interaction between FAST-2 and BF-1 is dependent on the Smad interaction domain of FAST-2, we examined whetherBF-1 could affect the ability of FAST-2 to associate with Smad2.When Myc-tagged BF-1 $Delta$ 1-119 was cotransfected with Myc-tagged FAST-2and Flag-tagged Smad2 in COS cells, a reduction in the amountof Flag-tagged Smad protein which is coimmunoprecipitated withMyc-tagged FAST-2 was observed (Fig. 7A). The full-length BF-1protein was also capable of interfering with the formation ofthe FAST-2-Smad2 complex. When Myc BF-1 was cotransfected withMyc-tagged FAST-2- and Flag-tagged Smad2, the amount of Myc-taggedFAST-2 which coimmunoprecipitated with Flag-tagged Smad2 was reduced(Fig. 7B).

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FIG. 7. BF-1 interferes with the formation of the FAST-2-Smad2 complex. (A) Interference by BF-1 $Delta$ 1-119. (Top panel) Flag blot of proteins immunoprecipitated with Myc antibody. Flag-tagged Smad2 (F-Smad2) coimmunoprecipitates with Myc-lagged FAST-2 when cotransfected into COS cells. Formation of this complex is enhanced by TGF- $beta$ . Coexpression of Myc-tagged BF-1 $Delta$ 1-119 reduces the amount of Flag-tagged Smad2 which is coimmunoprecipitated with Myc-tagged FAST-2. (Middle and bottom panels) Western blots of cell lysates indicate the relative amounts of Flag-tagged Smad2 (middle) and Myc-tagged FAST-2 or Myc-tagged BF-1 $Delta$ 1-119 (bottom). (B) Interference by BF-1. (Top panel) Myc blot of proteins immunoprecipitated with Flag antibody. Coexpression of Myc-tagged BF-1 reduces the amount of Flag-tagged Smad2 which is coimmunoprecipitated with Myc-tagged FAST-2. (Middle and bottom panels) Western blots of cell lysates indicate the relative amounts of Myc-tagged FAST-2 or Myc-tagged BF-1 (middle) and Flag-tagged Smad2 (bottom).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

BF-1 antagonizes TGF- $beta$ activity through a DNA binding-independent mechanism. We demonstrate that the WH transcription factor BF-1 functions as an antagonist of TGF- $beta$ . This conclusion is based on resultsof both (i) loss-of-function studies in primary neuroepithelialcell cultures and (ii) gain-of-function studies in a cell linewith inducible expression of BF-1. Cerebral cortical progenitorcells isolated from BF-1^/ mutant embryos are more responsive to growth inhibition by TGF- $beta$ and activin than are cells isolated from their normal littermates.These differences are observed in progenitor cells isolated fromembryos at E10.75. At this stage, no differences are observedin the morphology of the telencephalon between BF-1^/ mutant embryos and their normal littermates. Bromodeoxyuridinelabeling reveals no differences in the rate of proliferation inthe cerebral cortical progenitor population (37). Isolated BF-1^/ mutant cells have a similar proliferative response to mitogensin vitro as do cells obtained from WT and BF-1^+/ heterozygotes. Thus, the altered response to the antiproliferativeactivity of TGF- $beta$ and activin is the earliest phenotype we detectedin the BF-1^/ mutant cerebral corticalprogenitor.

We also examined the activity of BF-1 in Mv1Lu cell lines generated to express BF-1 and mutant forms of BF-1. We find thatectopic expression of BF-1 in mink lung epithelial cells doesnot significantly alter their rate of proliferation. However,BF-1 expression results in a reduction in the response of thesecells to the antiproliferative activity of TGF- $beta$ . BF-1 inhibitsthe ability of TGF- $beta$ to block the hyperphosphorylation of theRb protein and to stimulate the expression of the CDK inhibitorp15. BF-1 can also antagonize transcriptional activation by TGF- $beta$ of a FAST-2-dependent reporter gene, A3-luc.

A 2-amino-acid mutation (NH-AA) within the third $alpha$ -helix of the WH domain abolishes the ability of BF-1 to bind to a high-affinitysite on double-stranded DNA. However, this mutation does not alterthe ability of BF-1 to inhibit TGF- $beta$ -mediated growth arrest andTGF- $beta$ -dependent transcriptional activation. This result suggestedthat BF-1 may have functions which do not require DNA binding.Other transcription factors also have important functions whichare independent of their ability to bind to DNA. Truncated formsof eve and msx-1, which disrupt their DNA binding domains, canfunction as transcriptional repressors (1, 34). In addition,mice with a DNA binding-defective glucocorticoid receptor areviable whereas glucocorticoid receptor-deficient mice die shortlyafter birth (27). We cannot exclude the possibility that theBF-1(NH-AA) mutant can bind to DNA sequences other than knownBF-1 sites. However, because we have targeted the mutations tocritical residues in the binding helix of BF-1, any DNA bindingactivity of the BF-1(NH-AA) mutant is likely to utilize an atypicalmode of interaction with DNA. We favor the interpretation thatBF-1 may be antagonizing TGF- $beta$ function through a DNA binding-independentmechanism.

Association of BF-1 with a Smad partner. The activity of a DNA binding-defective form of BF-1 raised the possibility that BF-1 could be interfering with TGF- $beta$ functionby interacting with components of the TGF- $beta$ signaling pathway.Several mechanisms have previously been described in which TGF- $beta$ signal transduction is negatively regulated by interference withSmad transcriptional complexes. Smad6 associates with Smad1, therebyblocking signaling through the activating Smads (13, 25).The homeodomain protein evi has been suggested to antagonize TGF- $beta$ signals by undergoing a direct interaction with Smad3 (17).The homeodomain protein TGIF and the oncoproteins Ski and SnoNact as transcriptional corepressors (23, 30, 31, 36).In these examples, negative regulation is achieved through interactionswith Smad proteins. We did not obtain any evidence for interactionsbetween BF-1 and Smadproteins.

We find that BF-1 forms a complex with FAST-2 in cells. We provide evidence that the region of the BF-1 protein which is requiredfor its interaction with FAST-2 is also essential for its abilityto inhibit TGF- $beta$ -stimulated A3-luc expression and to antagonizethe antiproliferative activity of TGF- $beta$ . These results suggesta common mechanism for these three activities of BF-1. However,FAST-2 is not known to mediate the antiproliferative activityof TGF- $beta$ . BF-1 antagonizes this activity of TGF- $beta$ in Mv1Lu cellswhich do not express FAST-2. Furthermore, the low expression levelsof FAST-2 in the telencephalic neuroepithelium (C. Dou et al.,unpublished results) suggest that other DNA binding partners ofSmad proteins mediate TGF- $beta$ family signals in the developing brain.Thus, it is likely that BF-1 interferes with TGF- $beta$ responses whichare not mediated by FAST-2.

The finding that BF-1 associates with the same region of FAST-2 (the Smad interaction domain) which mediates its ability tointeract with Smad proteins suggests a mechanism by which BF-1can interfere with both FAST-2-dependent and FAST-2-independentTGF- $beta$ responses. We propose that BF-1 interacts with a subsetof DNA binding proteins which are characterized by sharing withFAST-2 a mode of interaction with Smad proteins (Fig. 8A and B).Thus, BF-1 interferes with TGF- $beta$ -stimulated transcriptional activationof the A3-luc reporter through its association with FAST-2. However,the antiproliferative responses of Mv1Lu cells and neuroepithelialcells to TGF- $beta$ and/or activin are likely to be mediated throughother DNA binding proteins. While transcriptional activation ofthe CDK inhibitor p15 has been identified as an important componentof the antiproliferative response in Mv1Lu cells (28), the correspondingtranscriptional targets in many other cells remain unknown andthe DNA binding proteins which recruit Smad complexes to thesepromoters have not yet been identified. We suggest that some ofthese DNA binding proteins (X in Fig. 8B) will associate withSmad2 through a structure which resembles that found in FAST-2.This model also predicts that BF-1 will not interfere with allTGF- $beta$ responses, e.g., transcriptional regulation mediated throughDNA binding partners which associate with Smad proteins througha distinct structural motif (Y in Fig. 8C). Our competition modelfurther predicts that BF-1 will reduce the amount of transcriptionallyactive Smad complex for any level of TGF- $beta$ signal. BF-1 can havean inhibitory activity in the absence of TGF- $beta$ , for a nonzerobasal level of Smad partner in the nucleus. We suggest that thisis a plausible explanation for the modest repression of the A3-lucreporter by BF-1 observed in FAST-2-transfected cells in the absenceof added TGF- $beta$ .

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FIG. 8. BF-1 interferes with multiple TGF- $beta$ responses by interference with FAST-2 and other Smad2 partners. (A) In this model, we propose that BF-1 associates with FAST-2 through a specific motif within the Smad interaction domain of the FAST-2 protein to inhibit TGF- $beta$ - and FAST-2-dependent transcriptional activation from the A3-luc reporter gene. ARE, activin response element. (B) BF-1 also interferes with other TGF- $beta$ responses such as the transcriptional activation of the p15 gene. The specific Smad2 partner for this and other responses remains to be established. We postulate that BF-1 will interact with a subset of these DNA binding partners, i.e., those that share with FAST-2 a mode of interaction with Smad2. (C) This model also predicts that other DNA binding partners which interact with Smad2 through a distinct mechanism will not be susceptible to interference by BF-1.

The homeodomain proteins Mixer and Milk were recently found to mediate activin- and TGF- $beta$ -induced transcription of the Xenopusgoosecoid promoter (8). These proteins associate with Smad2through a common motif, called the Smad interaction motif. Thismotif is also found within the Smad interaction domain of FAST-2.The expression pattern of Mixer and Milk suggests that they arenot likely to function in the developing brain. However, theiridentification as Smad partners supports the concept that multipleDNA binding proteins can recruit Smad2 to distinct promoter elementsthrough a common mechanism. Thus, the potential interaction targetsof BF-1 may include not only WH factors related to FAST-2 butalso members of other families of transcriptionalregulators.

	ACKNOWLEDGMENTS

We thank Abeel Mangi and Gabriela Balas for valuable assistance with these studies, M. Whitman and L. Freedman for providingreporter constructs, and R. Benezra and S. Li for critical reviewof themanuscript.

This work was supported by grants from the NIH to E.L. (HD29584), C.D. (F32NS10313), and MSKCC (Cancer Center SupportGrant).

	FOOTNOTES

^* Corresponding author. Mailing address: Box 83, 1275 York Ave., New York, NY 10021. Phone: (212) 639-2556. Fax: (212) 717-3053.E-mail: e-lai{at}ski.mskcc.org.

Present address: Center for Advanced Biotechnology and Medicine, Rutgers University, Piscataway, NJ08854.

Present address: Columbia University, New York, NY10016.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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BF-1 Interferes with Transforming Growth Factor Signaling by Associating with Smad Partners

BF-1 Interferes with Transforming Growth Factor $beta$ Signaling by Associating with Smad Partners