From the Departments of Medicine and Pathology, and the Molecular Biology Program, University of Colorado Health Sciences Center, Denver, Colorado 80262
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ABSTRACT |
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Progesterone has biphasic effects on proliferation of breast cancer cells; it stimulates growth in the first cell cycle, then arrests cells at G1/S of the second cycle accompanied by up-regulation of the cyclin-dependent kinase inhibitor, p21. We now show that progesterone regulates transcription of the p21 promoter by an unusual mechanism. This promoter lacks a canonical progesterone response element. Instead, progesterone receptors (PRs) interact with the promoter through the transcription factor Sp1 at the third and fourth of six Sp1 binding sites located downstream of nucleotide 154. Mutation of Sp1 site 3 eliminates basal transcription, and mutation of sites 3 and 4 eliminates transcriptional up-regulation by progesterone. Progesterone-mediated transcription is further prevented by overexpression of E1A, suggesting that CBP/p300 is required. Indeed, in HeLa cells, Sp1 and CBP/p300 associate with stably integrated flag-tagged PRs in a multiprotein complex. Since many signals converge on p21, cross-talk between PRs and other factors co-localized on the p21 promoter, may explain how progesterone can be either proliferative or differentiative in different target cells.
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INTRODUCTION |
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Progesterone is a paradoxical hormone having either growth stimulatory effects or growth inhibitory and differentiative effects, depending on the tissue in question and the dose and treatment regimen (1, 2). In the uterus for example, progesterone inhibits epithelial growth and has differentiative effects (3). It is therefore used to counteract the proliferative and carcinogenic effects of unopposed estrogens in women prescribed hormone replacement therapy (4). In the breast, the role of progesterone is more complex. The hormone is required for terminal growth and differentiation of the mammary gland (2). Therefore, mice lacking progesterone receptors (PRs)1 exhibit incomplete mammary gland ductal branching and failure of lobulo-alveolar development (5). In animal models of mammary carcinogenesis, progesterone, depending on the regimen used, can either inhibit or promote tumor formation (2). On the other hand, in animals with established PR-positive mammary tumors, progesterone is usually proliferative, and progesterone antagonists inhibit tumor growth (6). Despite this, in humans, second-line high dose progestin therapy effectively suppresses the growth of hormone-dependent PR- and estrogen receptor-positive breast cancers that have acquired resistance to the antiestrogen tamoxifen (6).
How can these contradictory effects of progesterone be reconciled? Recent studies have dealt with the effects of progesterone on mitosis and key cell cycle regulatory proteins in cultured human breast cancer cells (1, 7-9). Treatment of such cells with progestins produces biphasic effects. Studies focusing on the initial growth stimulatory component show that progestin-induced entry of cells into S-phase is accompanied by transient increases of cyclin D1 and cyclin-dependent kinase 4 activity (1, 7). Indeed, cyclin D1 is a critical component of the mitogenic response to progestins, and its overexpression in transgenic mice produces lobulo-alveolar changes in the mammary gland usually associated with progestational effects in pregnancy (8). Growth stimulation by progestins is restricted to one cycle, however, and is followed by growth arrest at the G1/S boundary of the second cycle (1, 7, 9). Cells then enter a period of resistance to growth regulatory effects of additional progesterone, accompanied by hypophosphorylation and profound down-regulation of pRb, loss of cyclins D, A, and B, and sequential increases first, in the levels of the cyclin-dependent kinase inhibitor p21 (p21Waf1, Cip1, Kip1, Sdi1) followed by increases in the cyclin-dependent kinase inhibitor p27 (1).
The control of proliferation and differentiation by many hormones and growth factors is linked by events that occur at the G1/S boundary of the cell cycle (10, 11). Recent studies implicate growth arrest accompanied by up-regulation of p21 not only in inhibiting proliferation but in promoting differentiation (12). Elevated p21 levels are associated with phorbol ester-, retinoic acid-, and vitamin D-induced differentiation in the myelomonocytic cell line U937, with butyrate-induced differentiation in WiDr cells, MyoD-induced differentiation of myoblasts, and thrombopoietin-induced differentiation of the megakaryoblastic leukemia cell line, CMK (12-18). In each case, the differentiating agents were also shown to induce transcription in a p53-independent manner from the p21 promoter fused to a reporter gene.
We therefore asked whether the up-regulation of p21 protein levels
induced by progesterone involves transcriptional regulation of the p21
promoter. We find that this promoter lacks a canonical progesterone
response element (PRE). Instead, progesterone activates the gene
through a novel mechanism that involves interactions between PRs and
CBP/p300, with the transcription factor Sp1, at Sp1 DNA binding sites
lying just upstream of the TATA box. Since other agents, such as
phorbol esters, butyrate, Ca2+, BRCA-1, and TGF- also
induce p21 from this region of the promoter (13, 16, 19-21), this
model may provide a means of analyzing cross-talk between steroid
hormones and other signal transduction pathways.
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MATERIALS AND METHODS |
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Cell Lines and Reagents-- Wild-type PR-positive T47DCO breast cancer cells were previously described (22). HeLa cells stably expressing flag-tagged PR A or B will be described elsewhere.2 Cells are routinely cultured in 75-cm2 plastic flasks and incubated in 5% CO2 at 37 °C in a humidified environment. The stock medium consists of Eagle's minimum essential medium with Earle's salts (MEM), containing L-glutamine (2 mM) buffered with sodium bicarbonate (4 mg/liter) and HEPES (4.8 mg/liter), insulin (6 ng/ml), and 5% fetal calf serum (HyClone, Logan, UT) without antibiotics. For routine subculturing, cells are diluted 1:20 into new flasks once per week, and the medium is replaced every 2-3 days. Cells are harvested by incubation in Hanks' solution-EDTA for 15 min at 37 °C.
Antibodies were obtained from the following sources. Anti-mouse polyclonal CBP-CT and anti-human monoclonal p300 were from Upstate Biotechnology, Lake Placid, NY; anti-p21 and anti-Sp1 were from Santa Cruz Biotechnology, Santa Cruz, CA; anti-PR AB-52 and B-30 were produced in our laboratories (23); and secondary antibodies were from Bio-Rad. Various p21 promoter and expression vectors were obtained as follows: the wild-typeTransfection and Transcription--
T47D breast cancer cells (1 million) were plated and grown in 100-mm cell culture plates in MEM
supplemented with 5% fetal calf serum. Transfection of plasmid DNA by
calcium phosphate coprecipitation was usually performed 24 h after
plating using 3 µg of the luciferase-fused reporter construct (23), 3 µg of the -galactosidase expression plasmid PCH110 (Amersham
Pharmacia Biotech) to correct for transfection efficiency, and
BluescriptTM carrier plasmid (Stratagene, La Jolla, CA) for
a total of 20 µg of DNA as described previously (23). 16 h
later, transfection was completed when the medium was aspirated, and
the cells shocked at room temperature for 2 min with 2 ml of
phosphate-buffered saline containing 20% glycerol. Cells were washed
twice with serum-free MEM to remove the glycerol, then 10 ml of MEM
containing 5% fetal calf serum were added per dish either with 30 nM progesterone or ethanol vehicle. Cells in duplicate
plates were harvested 48 h later in 250 µl of lysis solution
(Analytical Luminescence Laboratories, Ann Arbor, MI), and 100 µl of
lysate was analyzed for luciferase activity using the Enhanced
Luciferase Assay Kit and a Monolight 2010 Luminometer (Analytical
Luminescence Laboratories, Ann Arbor, MI) as described by the
manufacturer. A further 100 µl of lysate was assayed for
-galactosidase activity as described previously (25) to normalize
for transfection efficiency. In Fig. 1, T47D cells were treated with
progesterone or ethanol for 48 h prior to transfection, then
re-treated with progesterone or ethanol for a second 48-h period as
shown. HeLa cell transfection was carried out as above with the
exception that 90,000 cells were plated in 60-mm dishes in 5%
charcoal-stripped phenol red-free MEM. HeLa cells were not glycerol
shocked and were harvested for analysis 24 h after hormone
treatment.
In Vivo Association among PRs, Sp1, and CBP/p300-- HeLa cells were stably transfected with flag epitope-tagged PR B (f:PRB) or A (f:PRA) or the wild-type PR isoforms. In the presence of transiently transfected PRE2-TATAtk-chloramphenicol acetyltransferase reporter and the synthetic progestin R5020, the flag-tagged and wild-type receptors produce equal chloramphenicol acetyltransferase activity (not shown). For co-immunoprecipitation assays, nuclear extracts were prepared from HeLa f:PR cells or PR-negative HeLa cells treated with or without 100 nM R5020 for 1 h. The PRs were immunoprecipitated using an anti-flag M2 affinity gel (Eastman Kodak Co.), washed twice with TEDG (10 mM Tris, pH 7.4, 1 mM EDTA, 1 mM dithiothreitol, 10% glycerol), twice with 0.3 M KCl in TEDG, twice with 0.1% Nonidet P-40 in TEDG and then eluted from the gel using 0.2 mg/ml flag peptide (Kodak). The PRs and associated eluted proteins were resolved by SDS-polyacrylamide gel electrophoresis on 7.5% gels, transferred to nitrocellulose, and immunoblotted with the antibodies against PRs, Sp1, or CBP/p300 described above. The protein bands were detected by enhanced chemiluminescence (Amersham Corp.).
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RESULTS |
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Progesterone Activates the p21 Promoter through an Sp1 Site-- We recently demonstrated that in PR-positive T47D breast cancer cells, a pulse of progesterone induces one round of cell division. The cells then enter a period of prolonged growth arrest, during which they are resistant to the proliferative effects of a second dose of progesterone (1). The cells are not resistant to other mitogenic signals, however, because they can reenter the mitotic cell cycle in response to epidermal growth factor. Furthermore, during the arrested state the cells express functional PRs, which following treatment with a second dose of progesterone can activate transcription of a synthetic promoter/reporter (1) and can promote cellular differentiation and accumulation of lipid vesicles (26). Cells arrested by one dose of progesterone express high levels of p21, and the levels rise further following a second dose of progesterone given 48 h after the first (1).
To determine whether progesterone regulates p21 transcriptionally, a luciferase reporter gene driven by 2320 nt of the p21 promoter (Fig. 1A) was transfected into PR-positive T47DCO cells that had been pre-treated with ethanol or 30 nM progesterone for 48 h, then re-treated with ethanol or progesterone for another 48 h (Fig. 1B). Luciferase activity increased 2.3-fold in cells harvested 48 h after progesterone treatment, and 11.7-fold in cells receiving two sequential 48 h progesterone treatments. If progesterone is removed after 48 h, but the cells are not harvested for another 48 h, luciferase transcription continues and rises to 6.3-fold above controls. Since the half-life of progesterone is 3-4 h (27) and of luciferase is 90 min (28), we speculate that secondary signals prolong p21 transcription.
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Involvement of CBP/p300 in PR Regulation of the p21
Promoter--
Recently, Missero et al. (30) demonstrated
that keratinocyte differentiation associated with an increase in p21
levels is abolished by overexpression of the E1A oncoprotein. E1A binds CBP/p300, therefore titration of CBP/p300 into the keratinocytes restored p21 expression (30). To determine whether CBP/p300 is
important in the induction of p21 by progesterone, HeLa cells were
cotransfected with empty-, wild-type E1A-, or mutant E1A-containing expression vectors, the 2320 bp or the truncated
154 bp p21 promoter, and the PRA expression vector, and the cells were
treated with vehicle or progesterone (Fig.
4). In the absence of excess E1A,
progesterone induces luciferase transcription, but when wild-type E1A
is overexpressed, progesterone-regulated transcription is abolished
from either promoter. In contrast, an E1A mutant (E1A del 2-36; Ref.
30) lacking the N-terminal region required to bind CBP/p300, cannot
block progesterone-regulated transcription from the
2320 bp promoter.
This mutant also increases basal transcription of the p21 promoter,
which is similar to its effects on p15 promoter activity previously
described (31). Interestingly, overexpression of wild-type E1A also
abolishes progesterone regulation of the PRE2-TATAtk promoter, yet fails to alter
progesterone-regulated transcription of the Sp1-Luc (32) promoter (not
shown). This suggests that the ability of E1A overexpression to block
progesterone-induced transcription is promoter specific and not
necessarily Sp1-dependent.
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PR Bind Sp1 and p300-- Since the PR-dependent induction of p21 involves Sp1 and CBP/p300 in a region of the p21 promoter lacking a PRE, we postulated that PRs are tethered to the promoter through Sp1 and/or CBP/p300. To test this hypothesis, HeLa cells were stably transfected with expression vectors encoding flag-tagged PR A or B. The cells were treated or not with the progestin R5020, and nuclear extracts were prepared. PRs and associated proteins were immunoprecipitated from nuclear extracts with an anti-flag M2 affinity gel, then eluted from the resin with a flag peptide, and detected by immunoblotting. Fig. 5A (top) shows expression of the PR A- or B-isoforms in nuclear extracts from untreated or R5020-treated PR-positive HeLa cells. Low levels of A receptors can be immunopurified from nuclear extracts with anti-flag resin even in the absence of ligand (lane 2), and the levels increase further after ligand addition (lane 1). In the absence of ligand, no B receptors can be precipitated from nuclear extracts (lane 4), but high levels are purified following ligand treatment (lane 3). Fig. 5A (bottom) shows that Sp1 co-immunoprecipitates with the anti-flag antibody and is eluted by the flag peptide only from extracts that contain PRs. Similarly, no Sp1 is present in immunoprecipitates of nuclear extracts from PR-negative HeLa cells (not shown).
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DISCUSSION |
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In breast cancer cells, a transient pulse of progesterone has biphasic effects; it accelerates proliferation in the first cell cycle then arrests cells at the G1/S boundary of the second cycle (1, 9). A second dose of progesterone prolongs the growth arrest. We have proposed that the arrested cells are poised to enter a proliferative or differentiative pathway, depending on the nature of other cellular signals. This model calls for the convergence and integration of signals from the cell surface and cytoplasm with those in the nucleus. Since the progesterone-induced growth arrest is accompanied by a 10-15-fold increase in the levels of p21 (1) and this protein is a key player in determining cell fate (12), we speculated that integration of divergent signals occurs at the p21 promoter. To that end we sought to understand the mechanisms by which progesterone regulates the levels of p21.
We show here that a transient pulse of progesterone increases
transcription from the p21 promoter 2-3-fold (Figs. 1 and 2), which
rises to approximately 12-fold in cells receiving a second hormone dose
(Fig. 1). The progestin-responsive element maps to the Sp1-3 and Sp1-4
sites located between 84 and
65 nt. This suggests that progesterone
induction is p53-independent, since the two p53 binding sites are
located much further upstream at
1.4 and
2.3 kilobases (33). This
also rules out involvement of sites for two other nuclear receptors in
the progestin response, the retinoid-sensitive region, which maps to
1.2 kilobases (14) and the vitamin D site at
770 nt (15). The
proximal p21 promoter contains six Sp1 binding sites and a TATA box.
The region comprising Sp1-1 and Sp1-2 is involved in
12-O-tetradecanoylphorbol-13-acetate-mediated p21 induction
in U937 cells (13) and in BRCA-1-mediated p21 induction in SW480 colon
cancer cells (20). The region comprising Sp1-3 is required for p21
induction by TGF-
(21), butyrate (16), and Ca2+ (19).
Butyrate sensitivity also requires Sp1-5 and Sp1-6 in conjunction with
Sp1-3, with Sp1-3 being critical. We have mapped the
progesterone-responsive region to 20 nt comprising Sp1-3 and Sp1-4 and
show, furthermore, that Sp1-3 is required for basal promoter activity
in HeLa cells. This explains the data of Biggs et al. (13)
who demonstrated that deletion of
120 to
61 (which includes Sp1-3)
from the full-length promoter abolishes
12-O-tetradecanoylphorbol-13-acetate- and p53-mediated
induction. This would be expected if basal promoter function is
destroyed. We conclude that if Sp1-3 is required for basal promoter
activity, then progesterone response specificity requires Sp1-4, but
clearly both sites are important. To our knowledge, no other p21
regulator has been mapped to Sp1-4.
The mechanisms underlying Sp1-mediated induction of p21 transcription
are unknown. Phosphorylation of the protein is unaffected by
12-O-tetradecanoylphorbol-13-acetate or butyrate treatment (13), and footprinting studies demonstrate that Sp1 is constitutively bound to the DNA (13). We find that deletion of the TATA box does not
abolish the response to progesterone, an observation also reported by
Dotto et al. (21) in mapping the TGF--responsive element.
Sp1 is known to interact with the N terminus of the TATA-binding protein-associated factor dTAF110 in the TFIID complex, and
this interaction may account for the ability of Sp1 to activate
transcription from TATA-less promoters (34-36). Interestingly, the DNA
binding domain of PRs interacts with dTAF110 at its C
terminus (37). Thus, PRs and Sp1 may bind dTAF110
concurrently as shown in Fig. 6 and
suggests a mechanism for PR regulation of the p21 promoter.
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CBP/p300 may be a similar coregulator. It is necessary for
p21-dependent differentiation of keratinocytes (30, 31) and p21-dependent cell cycle arrest and differentiation of
muscle cells induced by MyoD (17). Although CBP/p300 was originally identified as a cAMP-response element binding protein, recent reports
have demonstrated that many transcription factors including steroid
receptors bind this protein (38). In this study we demonstrate that PRs
can bind CBP/p300 and that, in conjunction with Sp1, CBP/p300 is
required for induction of the p21 promoter by progesterone. This
suggests that CBP/p300 is an integral component of the basal transcription machinery of this promoter and/or that PRs recruit CBP/p300 to this transcription complex (Fig. 6). The former is more
likely since p21 promoter regulation by TGF- in keratinocytes is
also CBP/p300-dependent (31).
In sum, we have demonstrated a novel mechanism by which PRs can regulate gene transcription through a promoter that lacks canonical PREs. Instead, we suggest that PRs are brought to the DNA by binding to Sp1. It is possible that other Sp1-responsive genes (39, 40) can be similarly regulated. Furthermore, we have demonstrated this unusual regulation using the promoter of the p21 gene. This cyclin-dependent kinase inhibitor is a key intermediary protein in the pathway that determines whether cells proliferate or differentiate (10, 11), and it is therefore a target of regulation by multiple signaling molecules. We speculate that the proliferative versus differentiative fate of progesterone target cells is controlled by interactions between PRs and other transcription factors colocalized on the p21 promoter.
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ACKNOWLEDGEMENTS |
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We thank Bert Vogelstein, Len Freedman, Joseph Biggs, Andrew Kraft, and Xiao-Fan Wang for gifts of p21 promoter constructs, Bill Wood for the PA3-luciferase vector, Peggy Farnham for the pGL2-Sp1-Luc promoter construct, and Richard Goodman for the CBP/p300 expression vectors. Thank you also to Roger Powell, Carol Lange, M. Greg Abel, and J. Dinny Graham in our laboratory for advice and training. A special thanks to Joe Biggs for his helpful insights.
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FOOTNOTES |
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* This work was supported by Grants CA26869 and DK48238 from the National Institutes of Health, Grant DAMD17-94-5-4026 from the U. S. Army Medical Research Materiel Command, the National Foundation for Cancer Research, and the Core Laboratories of the University of Colorado Cancer Center.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Depts. of Medicine and
Pathology, and the Molecular Biology Program, University of
Colorado Health Sciences Center, 4200 E. 9th Ave., Campus Box B151, Denver, CO 80262. Tel.: 303-315-8443; Fax: 303-315-4525; E-mail:
kate.horwitz{at}uchsc.edu.
1
The abbreviations used are: PR, progesterone
receptor; PRE, progesterone response element; TGF-, transcription
growth factor-
; MEM, Eagle's minimum essential medium with Earle's
salts; nt, nucleotides; bp, base pair(s).
2 J. K. Richer, manuscript in preparation.
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REFERENCES |
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