17beta -Estradiol Potently Suppresses cAMP-induced Insulin-like Growth Factor-I Gene Activation in Primary Rat Osteoblast Cultures*

(Received for publication, February 12, 1997, and in revised form, May 16, 1997)

Thomas L. McCarthy Dagger §, Changhua Ji Dagger , Hong Shu Dagger , Sandra Casinghino Dagger , Kristina Crothers Dagger , Peter Rotwein and Michael Centrella Dagger

From the Dagger  Yale University School of Medicine, Section of Plastic Surgery, New Haven, Connecticut 06520-8041 and the  Division of Molecular Medicine, Oregon Health Sciences University, Portland, Oregon 97201-3098

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES


ABSTRACT

Insulin-like growth factor-I (IGF-I) is a key factor in bone remodeling. In osteoblasts, IGF-I synthesis is enhanced by parathyroid hormone and prostaglandin E2 (PGE2) through cAMP-activated protein kinase. In rats, estrogen loss after ovariectomy leads to a rise in serum IGF-I and an increase in bone remodeling, both of which are reversed by estrogen treatment. To examine estrogen-dependent regulation of IGF-I expression at the molecular level, primary fetal rat osteoblasts were co-transfected with the estrogen receptor (hER, to ensure active ER expression), and luciferase reporter plasmids controlled by promoter 1 of the rat IGF-I gene (IGF-I P1), used exclusively in these cells. As reported, 1 µM PGE2 increased IGF-I P1 activity by 5-fold. 17beta -Estradiol alone had no effect, but dose-dependently suppressed the stimulatory effect of PGE2 by up to 90% (ED50 ~0.1 nM). This occurred within 3 h, persisted for at least 16 h, required ER, and appeared specific, since 17alpha -estradiol was 100-300-fold less effective. By contrast, 17beta -estradiol stimulated estrogen response element (ERE)-dependent reporter expression by up to 10-fold. 17beta -Estradiol also suppressed an IGF-I P1 construct retaining only minimal promoter sequence required for cAMP-dependent gene activation, but did not affect the 60-fold increase in cAMP induced by PGE2. There is no consensus ERE in rat IGF-I P1, suggesting novel downstream interactions in the cAMP pathway that normally enhances IGF-I expression in skeletal cells. To explore this, nuclear extract from osteoblasts expressing hER were examined by electrophoretic mobility shift assay using the atypical cAMP response element in IGF-I P1. Estrogen alone did not cause DNA-protein binding, while PGE2 induced a characteristic gel shift complex. Co-treatment with both hormones caused a gel shift greatly diminished in intensity, consistent with their combined effects on IGF-I promoter activity. Nonetheless, hER did not bind IGF-I cAMP response element or any adjacent sequences. These results provide new molecular evidence that estrogen may temper the biological effects of hormones acting through cAMP to regulate skeletal IGF-I expression and activity.


INTRODUCTION

Although postmenopausal osteoporosis is one of the most prevalent age-related skeletal disorders, our understanding of the role of estrogen, which has a critical role in maintaining bone mass, remains incomplete. The principal laboratory animal model of postmenopausal osteoporosis is the ovariectomized (OVX)1 rat. One consistent observation with this model is an increase in the rate of bone remodeling after OVX-induced estrogen depletion (1-5). Furthermore, consistent with a cause and effect relationship, estrogen administration re-establishes a reduced rate of bone remodeling in the OVX rat.

Bone remodeling consists of two opposing events, i.e. bone resorption and formation (6). Skeletal integrity in adults relies on closely coupled remodeling where there is a balance between these catabolic and anabolic processes. Net bone loss in postmenopausal osteoporosis is thought to result from bone resorption that exceeds formation, even though both processes are accelerated in this condition (7-9). Recent data indicate the involvement of several interleukins (IL-1beta and IL-6) in estrogen deficiency-induced bone resorption (10-13). IL-6 has emerged as a pivotal factor in accelerated bone resorption in the estrogen-depeleted state, due in part to the apparent absence of bone loss in OVX mice carrying a knockout of the IL-6 gene (14). While progress has been made in understanding the interactions of estrogen and interleukins in regulating bone resorption, relatively little is known about factors involved in bone formation in the estrogen-depleted state. Recently, several groups reported elevated serum IGF-I levels that returned to normal following estrogen supplementation in OVX rats (15, 16). Similarly, postmenopausal women given estrogen experience a drop in serum IGF-I levels (17). The endocrine influence of elevated levels of circulating IGF-I is likely to include a positive effect on bone formation (18-21).

Local osteoblast-derived IGF-I also increases bone cell activity (18, 19, 22-26). The osteotropic hormone, parathyroid hormone (PTH), while stimulating resorption, also stimulates IGF-I synthesis by osteoblasts through a mechanism involving cAMP-dependent protein kinase A (22, 23, 27). PTH administered intermittently in vivo or in vitro increases osteoblast replication and matrix collagen synthesis (23, 28-32). An increase in IGF-I expression is in part responsible for the anabolic effect of PTH. In fetal rat calvarial bone explants, a brief exposure to PTH increases the rate of collagen synthesis, and neutralizing antibodies to IGF-I dramatically reduce this effect (23). Therefore, IGF-I appears to couple this aspect of bone remodeling.

Earlier studies examining the influence of estrogen on IGF-I expression by primary cultures of neonatal rat calvarial osteoblasts indicated a small stimulatory effect (~2-fold), thought to result from changes in the rate of gene transcription (33, 34). However, OVX increases IGF-I mRNA expression in the calvariae of growing rats, and this effect can be reversed by the estrogen agonist diethylstilbesterol (35, 36). These latter observations agree with the elevated serum IGF-I levels seen in OVX rats, indicated earlier (15, 16). Therefore, in vivo and in vitro findings together predict that estrogen may suppress IGF-I expression in skeletal tissue and that this may be focused on the stimulatory effect of agents that induce cAMP. This interpretation is consistent with the lower rate of bone remodeling seen in the estrogen replete versus estrogen-depleted animals.

In this study we wished to evaluate the effect of 17beta -estradiol on IGF-I promoter activity. Because we previously demonstrated a PKA-dependent increase in IGF-I transcription after exposure to PGE2 in fetal rat osteoblasts (37-40), we used this model to examine the influence of 17beta -estradiol alone and in combination with PGE2 on IGF-I promoter function. Furthermore, because other studies suggested that estrogen can suppress an increase in cAMP in response to PTH (33), we also examined the effect of 17beta -estradiol on PGE2-stimulated cAMP in these cultures. Although we find a potent regulatory effect of 17beta -estradiol on cAMP-dependent IGF-I expression, it occurs downstream of cAMP accumulation.


EXPERIMENTAL PROCEDURES

Cell Cultures

Primary osteoblast-enriched cell cultures were prepared from the parietal bones of 22-day-old Sprague-Dawley rat fetuses (Charles River Laboratories, Raleigh, NC). Animals were housed and euthanized by methods approved by the Yale University Animal Care and Use Committee. Cranial sutures were eliminated during dissection, and the bones were digested with collagenase for five sequential 20-min intervals. The cell population released during the last three digestions exhibits biochemical characteristics associated with differentiated osteoblasts, including PTH receptors, type I collagen synthesis, and a rise in osteocalcin expression in response to dihydroxyvitamin D3 (41, 42). Histochemical staining demonstrates that approximately 80% of the cells express alkaline phosphatase,2 although this itself is not entirely specific for osteoblasts. However, using these criteria, as well as differential sensitivity to transforming growth factor-beta , bone morphogenetic protein-2, various prostaglandins, and the ability to form mineralized nodules in vitro (43, 44), these cells are well distinguished from the less differentiated cells released during earlier collagenase digestions. Cells from the last three digestions were pooled and then plated at 4,800 per cm2 in Dulbecco's modified Eagle's medium (DMEM) containing 20 mM HEPES (pH 7.2), 0.1 mg/ml ascorbic acid, penicillin and streptomycin (all from Life Technologies Inc.) and 10% fetal bovine serum (Sigma). At the time of transfection, cultures were rinsed twice with phenol red-free, serum-free DMEM. All subsequent culturing was in phenol red-free DMEM, with (growth medium) or without (treatment medium) charcoal-stripped serum, prepared as described by Ernst and Rodan (34).

Plasmids

Rat IGF-I promoter 1 constructs have been described previously (45). A Rous sarcoma virus promoter-driven expression vector for both the human estrogen receptor (pRSV-hER; containing a glycine to valine substitution at position 400), and a recombinant luciferase reporter construct containing two tandem estrogen response elements (ERE from the vitellogenin gene) along with the minimal prolactin promoter ((ERE)2PRL36-Luc), were kindly provided by Dr. Stuart Adler (Washington University School of Medicine). All plasmids were propagated in Escherichia coli strain DH5alpha with ampicillin selection and were prepared with a Wizard Plus Maxiprep DNA purification kit (Promega Corp., Madison, WI) and the manufacturer's recommended protocol.

Transfection Studies

IGF-I promoter 1-luciferase reporter plasmids (1.25 µg/9.6-cm2 culture well) were co-transfected with pRSV-hER (1.25 µg/culture well). Cultures at 40% confluence were rinsed in serum-free medium and exposed to plasmids in the presence of 0.5% LipofectinTM (Life Technologies Inc.) for 3 h. The solution was then replaced with growth medium containing 5% charcoal-stripped fetal bovine serum, and cultures were re-incubated for 48 h. Subconfluent cultures were rinsed with serum-free medium and treated for the indicated times with vehicle (ethanol-diluted 1/1,000 or greater), PGE2, 17beta -estradiol, or 17alpha -estradiol (all from Sigma; each was dissolved in 95% ethanol), either individually or in combination. After treatment, medium was aspirated, and cultures were rinsed with phosphate-buffered saline and then lysed in 100 µl of 25 mM Tris phosphate (pH 7.8), 2 mM dithiothreitol (DTT), 2 mM 1,2-diaminocyclohexane-N,N,N',N'-tetraacetic acid, 10% glycerol, 1% Triton X-100 (cell lysis buffer, Promega Corp.). Nuclei were pelleted at 12,000 × g for 5 min, and supernatants were stored at -75 °C until assay. A commercial kit (Promega Corp.) was used to measure luciferase by single channel photon counting, and enzyme activity was corrected for protein content as determined by the Bradford assay (46).

cAMP Radioimmunoassay

Cultures were transiently transfected with pRSV-hER. After 48 h, cultures were rinsed twice with serum-free phenol red-free DMEM and exposed to control medium or 10 nM 17beta -estradiol for 30 min. Cultures were then treated for 5 min with 0.5 mM isobutylmethylxanthine, to inhibit endogenous phosphodiesterase activity, prior to a 10-min treatment (at room temperature) with control (ethanol vehicle), PGE2 (1 µM), 17beta -estradiol (0.1-10 nM), alone or in combination. Treatments were terminated by aspirating the medium, and the plates were immediately frozen at -75 °C. Cultures were extracted with n-propyl alcohol, and the samples were air-dried and then dissolved in 50 mM sodium acetate (pH 6.2). An aliquot was used to measure cAMP content using a highly specific commercial radioimmunoassay kit (Biomedical Technologies, Inc.). The amount of cAMP in each extract was determined from the linear portion of a standard curve and is expressed as picomoles of cAMP/2-cm2 culture, as reported previously (27).

Nuclear Protein Extracts

Control or pRSV-hER-transfected cultures were rinsed with serum-free medium and exposed to treatment solution for 4 h. Medium was aspirated, and cultures were rinsed twice with phosphate-buffered saline at 4 °C. All subsequent steps were performed on ice or at 4 °C. Cells were harvested with a cell scraper and gently pelleted, and the pellets were washed with phosphate-buffered saline. Nuclear extracts were prepared by the method of Lee et al. with minor modifications (39, 47). Cells were lysed in hypotonic buffer (10 mM HEPES (pH 7.4), 1.5 mM MgCl2, 10 mM KCl, 0.5 mM DTT) with phosphatase inhibitors (1 mM sodium orthovanadate, 10 mM sodium fluoride), protease inhibitors (0.5 mM phenylmethylsulfonyl fluoride, 1 µg/ml pepstatin A, 2 µg/ml leupeptin, 2 µg/ml aprotinin; Sigma), and 1% Triton X-100. Nuclei were gently pelleted. Nuclei were resuspended in hypertonic buffer containing 10 mM HEPES, pH 7.4, 0.42 M NaCl, 0.2 mM Na2EDTA, 25% glycerol, and the phosphatase and protease inhibitors indicated above. Soluble proteins released by a 30-min incubation at 4 °C were collected by centrifugation at 12,000 × g for 5 min, and the supernatant was collected and aliquoted for storage at -75 °C.

Electrophoretic Mobility Shift Assay

Using previously published methods (40, 48, 49), radiolabeled double-stranded probe (Universal DNA, Inc., Tigard, OR) was prepared by annealing complementary oligonucleotides, followed by fill-in of single-stranded overhangs with dCTP, dGTP, dTTP, and [alpha -32P]dATP, using the Klenow fragment of DNA polymerase I. Five to ten µg of nuclear extract protein was preincubated for 20 min on ice with 2 µg of poly(dI-dC) with or without unlabeled specific or nonspecific competitor DNAs in 60 mM KCl, 25 mM HEPES (pH 7.6), 7.5% glycerol, 0.1 mM EDTA, 5 mM DTT, and 0.025% bovine serum albumin. After the addition of 5 × 104 cpm of DNA probe (0.1-0.2 ng) for 30 min on ice, samples were applied to a 5% nondenaturing polyacrylamide gel that was pre-electrophoresed for 30 min at 12.5 V/cm at 25 °C in 45 mM Tris, 45 mM boric acid, 1 mM EDTA. Electrophoresis proceeded for 2.5 h under identical conditions. Dried gels were exposed to x-ray film at -75 °C with intensifying screens. Electrophoretic mobility supershift analysis was performed in select experiments using normal rabbit serum as a negative control and monoclonal anti-rhER antibody (Santa Cruz Biotechnologies Inc., Santa Cruz, CA) for its ability to produce a supershift of hER-bound probe. Sequences of sense strands of oligonucleotides used in the electrophoretic mobility shift assays are as follows: HS3D, 5'-GAGCAGATAGAGCCTGCGCAATCGAAATA-3' (the minimal binding sequence of the atypical cyclic response element within the HS3D footprint site of the rat IGF-I promoter 1 is underlined (40)) and ERE, 5'-GATCCAAAGTCAGGTCACAGTGACCTGATCAAAGA-3' (the estrogen response element is underlined in this sequence).

Reagents

17beta -Estradiol, 17alpha -estradiol, and PGE2 were obtained from Sigma and were 99% pure as determined by TLC.

Statistical Analysis

Data were assessed by one way analysis of variance with SigmaStat® software, with the Student-Newan-Keuls method for post hoc comparison.


RESULTS

The IGF-I gene has two promoters, and promoter 1 (P1) is used exclusively in cultures of fetal rat osteoblasts (38). Initial studies were conducted with osteoblast cultures transiently transfected with the longest IGF-I P1-luciferase reporter construct, IGF1711b/Luc (containing 1711 bp of upstream sequence, and the initial 328 bp of transcribed but untranslated exon 1), which we previously found to be most responsive to treatment with the cAMP-inducing agent PGE2 (39). To ensure expression of active estrogen receptors, cultures were co-transfected with the hER expression vector pRSV-hER. Incubation with 17beta -estradiol at 0.01-10 nM for 16 h did not alter basal IGF-I P1 activity (Fig. 1, left panel). As a positive control, parallel cultures were co-transfected with pRSV-hER and a recombinant reporter plasmid containing tandem copies of the consensus estrogen response element (ERE) from the vitellogenin gene, and a short segment of the prolactin promoter (plasmid (ERE)2PRL-Luc). Unlike the IGF-I P1 recombinant plasmid, treatment with 17beta -estradiol enhanced expression of this ERE-containing reporter gene up to 10-fold (Fig. 1, center panel). Co-transfection with pRSV-hER was required for all 17beta -estradiol-dependent responses, including activation of the (ERE)2PRL-Luc construct (data not shown).


Fig. 1. 17beta -Estradiol dose-dependently suppressed PGE2-stimulated IGF-I promoter 1 activity in osteoblast cultures expressing human estrogen receptor. IGF-I promoter 1 luciferase reporter plasmid, IGF1711b/Luc, was co-transfected with a Rous sarcoma virus promoter-driven expression vector encoding human estrogen receptor cDNA, pRSV-hER, into osteoblast cultures (9.6 cm2) using LipofectinTM. Parallel cultures were transfected with a recombinant luciferase reporter construct containing two tandem copies of the consensus ERE (from the vitellogenin gene) and a segment of the prolactin promoter ((ERE)2PRL-Luc) along with pRSV-hER. Cultures were grown in phenol red-free DMEM containing 5% FBS (charcoal-stripped) for 48 h. The growth medium was aspirated, and the cultures were rinsed with phenol red-free, serum-free DMEM. Cultures were treated with control medium (containing ethanol vehicle), PGE2 (1 µM), 0.01-10 nM 17beta -estradiol, or both agents for 16 h. 17alpha -Estradiol (10 nM) was tested in the absence or presence of PGE2 (1 µM) to test the response for estrogen isoform specificity. Cytoplasmic extracts were prepared and luciferase activity determined. Data are corrected for protein content. Transfections were performed in triplicate, and results are representative of three separate experiments. The mean ± S.E. for luciferase expression (counts/min/µg of protein) are shown. * indicates luciferase levels significantly different (p < 0.05) from control, and ** indicates levels significantly different (p < 0.05) from PGE2 treatment alone.
[View Larger Version of this Image (25K GIF file)]

Fetal rat osteoblasts respond to PGE2 with a rapid increase in IGF-I expression, mediated by PKA-dependent activation of IGF-I P1 (39). This occurs through an atypical CRE located at bp +202 to +209 of exon 1 (40), and PTH similarly requires this element to enhance IGF-I promoter function (data not shown). As we reported previously, PGE2 (1 µM, 16 h) increased IGF-I P1 activity 5-fold (39). While 17beta -estradiol alone was ineffective, co-treatment with PGE2 led to a dose-dependent suppression of IGF-I promoter activation over a concentration range of 0.1-10 nM (ED50 ~0.1 nM) (Fig. 1, left panel). This response required expression of hER (Fig. 1, right panel), and an active form of estradiol, since 17alpha -estradiol was 100-300-fold less potent than 17beta -estradiol at blocking PGE2-mediated IGF-I P1 activity (Fig. 1, left panel). By contrast, expression of the ERE-driven reporter gene was not inhibited by co-treatment with 17beta -estradiol and PGE2 (see Fig. 3).


Fig. 3. Co-localization of cAMP response element and estrogen inhibitory function within the shortest IGF-I promoter 1 construct. Osteoblast cultures were co-transfected with IGF1711b/Luc (containing 1711 bp of upstream sequence and 328 bp of 5'-transcribed and untranslated exon 1), IGF823/Luc (containing 823 bp of upstream sequence and 328 bp of 5'-transcribed and untranslated exon 1), or IGF122/Luc (containing 122 bp of upstream sequence and 328 bp of 5'-transcribed and untranslated exon 1; each construct is diagramatically shown in A), along with pRSV-hER, as described under "Experimental Procedures." Parallel cultures were transfected with recombinant luciferase reporter construct (ERE)2PRL-Luc, along with pRSV-hER. Cultures were grown 48 h, the growth medium was aspirated, and the cultures were rinsed with phenol red-free, serum-free DMEM. Cultures were treated with control medium (containing ethanol vehicle), PGE2 (1 µM), 10 nM 17beta -estradiol, or both agents for 16 h. Cytoplasmic extracts were prepared and luciferase activity determined. Data are corrected for protein content. Transfections were performed in triplicate, and results are representative of three separate experiments. The mean ± S.E. for luciferase expression (counts/min/µg of protein) are shown in B. * indicates luciferase levels significantly different (p < 0.05) from control, and ** indicates levels significantly different (p < 0.05) from PGE2 treatment alone.
[View Larger Version of this Image (33K GIF file)]

Time course experiments next were performed to examine the kinetics of inhibition of IGF-I P1 activity by 17beta -estradiol. Cells were treated with PGE2 (1 µM) or 17beta -estradiol (10 nM), alone or in combination for 3, 6, or 16 h. PGE2-activated expression of the IGF-I P1 reporter gene was rapidly blunted by 17beta -estradiol. Both the stimulatory effect of PGE2 on IGF-I promoter activity and the opposing, suppressive influence of 17beta -estradiol were observed within 3 h of hormone treatment. Both responses were maintained throughout a 16 h incubation, while the ERE-containing plasmid ((ERE)2PRL-Luc) was activated progressively by 17beta -estradiol (Fig. 2).


Fig. 2. 17beta -Estradiol suppression of PGE2-induced IGF-I promoter 1 activity occurred within 3 h of co-treatment and was sustained for 16 h. Osteoblast cultures were co-transfected with IGF1711b/Luc and pRSV-hER, as described under "Experimental Procedures" and in the legend to Fig. 1. Parallel cultures were transfected with a recombinant luciferase reporter construct (ERE)2PRL-Luc, along with pRSV-hER. Cultures were grown 48 h, the growth medium was aspirated, and the cultures were rinsed with phenol red-free, serum-free DMEM. Cultures were treated with control medium (containing vehicle), PGE2 (1 µM), 10 nM 17beta -estradiol, or both agents for 3, 6, or 16 h. Cytoplasmic extracts were prepared and luciferase activity determined. Data are corrected for protein content. Transfections were performed in triplicate, and results are representative of three separate experiments. The mean ± S.E. for luciferase expression (counts/min/µg of protein) are shown. * indicates luciferase levels significantly different (p < 0.05) from control, and ** indicates levels significantly different (p < 0.05) from PGE2 treatment alone.
[View Larger Version of this Image (38K GIF file)]

IGF-I P1 lacks a consensus ERE, and yet 17beta -estradiol suppressed cAMP-dependent promoter activation. Therefore, an effort was made to localize the region(s) of the promoter responsible for the opposing effect of estrogen on cAMP-mediated gene activation. Deletion of 5' flanking DNA from nucleotides -1711 to -123 (with respect to the most 5' transcription start site of rat IGF-I exon 1 (45)) did not alter either PGE2-stimulated promoter activation (39), or the opposing inhibitory effect of 17beta -estradiol (Fig. 3). All three of the plasmids tested retained the same 328 bp of exon 1, which preserves the unconventional CRE (located at bp +202 to +209) required for the stimulatory effect of PGE2 (40).

Next, several approaches were taken to determine the mechanism by which estrogen might suppress IGF-I promoter activation by PGE2. Previous conflicting reports suggested a possible inhibitory effect by estrogen on cAMP accumulation in response to PTH in osteoblasts (33, 50). We examined cAMP levels in cells that were treated with 1 µM PGE2 alone or in combination with 10 nM 17beta -estradiol (as in the promoter/reporter assays) and in cells preincubated with 17beta -estradiol for 30 min followed by PGE2 treatment. All cultures were transfected 48 h earlier with pRSV-hER and pretreated with isobutylmethylxanthine for 5 min to inhibit phosphodiesterase activity. In all experiments, cAMP accumulation increased by 60-fold after 10-min treatment with PGE2, even in the presence of 17beta -estradiol co-treatment or pretreatment (Fig. 4). In addition, regardless of the presence of 17beta -estradiol, PGE2-induced accumulation of cAMP was accompanied by pronounced morphological changes, as seen previously with these cells (data not shown). These results indicate that the adenylate cyclase pathway was intact and functional in cells exposed to 17beta -estradiol.


Fig. 4. 17beta -Estradiol does not alter PGE2-stimulated cAMP levels in cultures transfected with hER. Osteoblast cultures were transiently transfected with hER expression vector pRSV-hER. Forty-eight hours later, cultures were rinsed twice with serum-free phenol red-free DMEM and exposed to control medium or 10 nM 17beta -estradiol for 30 min. Cultures were treated for 5 min with 0.5 mM isobutylmethylxanthine (phosphodiesterase inhibitor) prior to a 10-min treatment (at room temperature) with control (ethanol vehicle), PGE2 (1 µM), 17beta -estradiol (0.1-10 nM), alone or in combination. Cultures were extracted with n-propyl alcohol and the cAMP content determined by radioimmunoassay. These data are the pooled results from two independent observation where n = 6. No statistical difference was detected between control and 17beta -estradiol treatment alone or PGE2 treatment in the absence or presence of 17beta -estradiol (co-treatment or 30-min pretreatment). * indicates comparably elevated cAMP levels that are significantly different (p < 0.05) from control.
[View Larger Version of this Image (43K GIF file)]

While cAMP levels were not altered by 17beta -estradiol, estrogen may interfere with other steps in the process of PKA-dependent IGF-I gene activation that lie downstream of the generation of cAMP. One possibility is that the ligand-activated ER may modulate the binding of cAMP-dependent transcription factor(s) to the IGF-I CRE. To examine this possibility, nuclear extracts prepared from control and PGE2-treated cells were tested in the electrophoretic mobility shift assay using a 32P-labeled double-stranded oligonucleotide containing the IGF-I CRE (designated HS3D, based on the notation for the footprinted site (45)). In agreement with our earlier observations, a gel-shifted doublet band was seen with this oligonucleotide using nuclear extracts from PGE2 (1 µM, 4 h)-treated cultures (40). The PGE2-inducible gel shift that occurred for extracts from cells previously transfected with the hER expression plasmid was identical to that for untransfected cultures (Fig. 5). In cells expressing hER, incubation with 17beta -estradiol alone did not induce nuclear protein binding to the HS3D oligonucleotide probe. However, the amount of nuclear protein complex that occurred with extract from hER tranfected cells co-treated with PGE2 and 17beta -estradiol was dose-dependently reduced in intensity compared with PGE2 treatment alone, but there was no change in the banding pattern. In contrast 17alpha -estradiol was not similarly inhibitory.


Fig. 5. PGE2-induced binding of nuclear protein(s) to the IGF-I promoter 1 CRE was suppressed by 17beta -estradiol co-treatment. Electrophoretic mobility shift experiments were performed as described under "Experimental Procedures" with nuclear extract from osteoblast cultures. Left panel, nuclear protein binding to 32P-labeled HS3D probe is shown. Nuclear extracts used in the first two lanes were from osteoblast cultures that were not transfected with hER; cultures were treated with control medium or PGE2 for 4 h to demonstrate the expected inducible gel shift. Nuclear extracts used in subsequent lanes were prepared from cultures that had been transfected with pRSV-hER 48 h prior to treatment, as indicated. Nuclear extracts of culture treated for 4 h with control (ethanol vehicle), 1 µM PGE2, 10 nM 17beta -estradiol alone, or in combination with 1 µM PGE2, were used, as indicated above each lane. Autoradiographic exposures were performed at -75 °C with an intensifying screen. This experiment was repeated three times with identical results. In the right panel are densitometric data (from duplicate experiments) from electrophoretic mobility shift experiments using nuclear extracts from cultures treated for 4 h with 1 µM PGE2 alone or in combination with 10, 1, 0.1 nM 17beta -estradiol, or 10 nM 17alpha -estradiol, to examine binding to 32P-labeled HS3D probe. 17beta -Estradiol dose-dependently reduced the intensity of the characteristic PGE2-induced complex (closed circles), while 17alpha -estradiol (closed square) was not similarly inhibitory.
[View Larger Version of this Image (40K GIF file)]

We then examined the possibility that ER directly associates with the IGF-I CRE and therefore competes with cAMP-stimulated transcription factor(s) for binding at this element. First, we tested recombinant hER (rhER) for its ability to bind a 32P-labeled consensus ERE oligonucleotide as a positive control and to determine if excess unlabeled HS3D oligonucleotide could compete for rhER binding. Without rhER, no gel-shifted band was detected with 32P-labeled ERE oligonucleotide. However, the association of rhER with 32P-labeled ERE oligonucleotide produced strong gel shift complexes that were significantly reduced in intensity by 50-fold molar excess of unlabeled homologous ERE, but were unaffected by excess unlabeled HS3D oligonucleotide. To confirm the specificity of the hER/ERE interaction further, a monoclonal anti-hER antibody was used in a supershift assay. As shown, normal rabbit serum was ineffective, while anti-hER antibody altered the mobility of the hER-dependent gel-shifted band (Fig. 6, left panel). Next, to examine binding of hER to the IGF-I promoter directly, two 32P-labeled double-stranded DNA probes generated from the -122 bp to +328 bp portion of rat IGF-I P1 were combined with recombinant hER. No gel shift complex was seen with either fragment. These findings indicate that no direct interactions occur between rhER and the regions of IGF-I P1 that contain or flank HS3D (Fig. 6, right panel), even though HS3D is required for stimulation of reporter gene expression by PGE2 and for the opposing influence of 17beta -estradiol.


Fig. 6. Purified recombinant human estrogen receptor (rhER) binds a consensus ERE, however, this hER/ERE interaction was not diminished by excess unlabeled HS3D (IGF-I CRE), nor does rhER bind to the IGF-I cyclic response element or adjacent sequences. Left panel, recombinant hER (Panvera Corp.) was tested in the electrophoretic mobility shift assay to demonstrate binding to a double-stranded consensus ERE containing oligonucleotide and to determine if the HS3D oligonucleotide used in Fig. 5 could compete with the ERE oligonucleotide for binding the rhER. Right panel, the promoter 1/exon 1 segment present in construct IGF122/Luc was also tested for direct binding of rhER. The promoter 1/exon 1 insert was cleaved out of the reporter construct with BamHI, PvuII, and HindIII, which produced two fragments that were gel-purified, 32P-end-labeled, and used in individual electrophoretic mobility shift assays (designated [32P]1/exon1 (-122 to +86) and [32P]p1/exon1 (+87 to +328)). Unlabeled, 100-fold molar excess ERE and HS3D oligonucleotide were tested as competitors in the electrophoretic mobility shift assays. Normal rabbit serum and monoclonal anti-rhER antibody (Santa Cruz Biotechnologies Inc., Santa Cruz, CA) were tested for their ability to produce a supershift of hER bound probe. The 32P-labeled double-stranded oligonucleotide probe used in each assay is indicated above each set. Lane 1, 32P-labeled probe alone; lane 2, 32P-labeled probe plus recombinant hER; lane 3, 32P-labeled probe plus recombinant hER plus, 100-fold excess unlabeled double-stranded ERE oligonucleotide; lane 4, 32P-labeled probe plus recombinant hER plus 100-fold excess unlabeled double-stranded HS3D oligonucleotide; lane 5, 32P-labeled probe plus recombinant hER plus 1 µg of normal rabbit serum; lane 6, 32P-labeled probe plus recombinant hER plus 1 µg of monoclonal anti-rhER antibody.
[View Larger Version of this Image (96K GIF file)]


DISCUSSION

Estrogen deprivation has long been associated with a decline in skeletal integrity, but its role in the normal maintenance of bone mass is still poorly understood. Several lines of evidence indicate that estrogen deficiency increases the total process of bone remodeling in such a way that the rate of bone resorption significantly outpaces formation and results in osteoporosis (1-5). Studies with OVX rats, where surgical estrogen depletion incurs a decrease in bone mass, strongly connect IL-1 and IL-6 to accelerated bone resorption. In vivo studies using an IL-1 receptor antagonist demonstrate a bone sparing effect similar to that observed with estrogen replacement therapy, while IL-6 knockout mice do not experience the OVX-induced bone loss seen in their heterozygous littermates (14, 51). In vitro studies indicate that both lymphokines are associated with activation of mature osteoclasts and stimulation of osteoclastogenesis. These results have increased our understanding of the high rates of bone resorption that follow the loss of endogenous estrogen. Nevertheless, little is still known about the mechanisms by which bone formation rates also increase, albeit to a lesser extent, under similar conditions.

Estrogen has a positive influence on the growth of some tissues, such as uterine tissue. In rats, OVX causes weight gain and increased longitudinal bone growth, both of which are reversed by estrogen treatment. Consistent with this, OVX increases the circulating levels of IGF-I, and estrogen treatment can normalize this change (15, 16). Similar results were observed in postmenopausal women (17). Liver is a primary source of serum IGF-I. In this regard, estrogen suppresses growth hormone-stimulated hepatic IGF-I synthesis in hypophysectomized and OVX animals, even though it increases serum growth hormone levels in OVX animals (52, 53). These latter findings may help explain some in vivo results with OVX rats. Interestingly, estrogen treatment is also associated with accelerated skeletal maturation and closure of growth plates in both rats and humans (54). Local IGF-I synthesis by bone cells is also induced by growth hormone and contributes significantly to longitudinal bone growth (4), predicting that estrogen can oppose its stimulatory effect on IGF-I synthesis in liver as well as peripheral tissue. OVX also alters several markers of osteoblast activity in intramembranous bone such as calvariae (the source of osteoblastic cells used in our studies). Within 1 week of OVX, transcript levels for osteocalcin, osteonectin, and IGF-I increase at this site. Subsequent treatment with the estrogen analog diethylstilbesterol rapidly decreases the appearance of these mRNAs, reduces periosteal mineral apposition rate, and also suppresses osteoblast number (8, 35, 36, 55).

Alterations in serum PTH levels have also been reported after OVX (5, 56). We first identified that IGF-I is one coupling factor in the bone-remodeling process. At least part of the anabolic action of PTH on skeletal tissue is mediated by its stimulatory effect on IGF-I expression by way of an increase in cAMP (22, 23). Since then we have examined the cellular and molecular mechanisms that regulate IGF-I synthesis in this system. We recently identified an atypical cAMP response element that controls PKA-dependent (PGE2- or PTH-activated) IGF-I gene expression in fetal rat bone cells (40). Even more recently we found that this can occur through activation of one of several previously characterized trans-activating factors that associate with this atypical CRE.3 Like PTH, PGE2 can prevent or significantly restore bone loss due to OVX or immobilization (57-59). PGE2 is synthesized locally in the skeleton following exposure to cytokines (transforming growth factor-beta and IL-1), hormones such as PTH, and mechanical strain (59). In osteoblasts, PGE2 also activates IGF-I expression through a PKA-dependent mechanism, where it stimulates IGF-I gene transcription, mRNA accumulation, and protein production (37-40).

Our current studies revealed that 17beta -estradiol alone does not directly alter IGF-I promoter activity. However, it suppresses PKA-dependent IGF-I gene activation in a rapid and sustained, estrogen receptor-dependent, isoform-specific, and dose-dependent way. The ED50 of 17beta -estradiol was ~0.1 nM, within its physiological concentration range (60), while 17alpha -estradiol was 100-300-fold less effective. This suppressive effect was not due to hormone toxicity, since the same doses of 17beta -estradiol stimulated expression of a reporter gene containing a consensus ERE. Furthermore, neither estrogen pretreatment or co-treatment altered cAMP accumulation, indicating that its effect on IGF-I expression occurs downstream of cAMP itself. Reporter gene expression, under control of the smallest fragment of IGF-I promoter DNA, which retains PKA sensitivity, was completely suppressed by 17beta -estradiol. This observation co-localizes the responsive sequences for each event to one element or a small region of DNA. The rat IGF-I promoter 1 contains no consensus ERE or CRE DNA sequences. However, electrophoretic mobility shift assays using the HS3D region of the IGF-I promoter, where the atypical IGF-I promoter CRE resides, revealed that 17beta -estradiol reduced the intensity of the cAMP-inducible gel shift. No additional bands or changes in relative mobility occurred with estrogen treatment. Therefore, interactions between hER and the cAMP-activated nuclear factor(s) or co-activator(s) appear to limit nuclear factor binding to the atypical IGF-I CRE within the HS3D region itself. Complex kinetics for the suppressive effect of 17beta -estradiol on PKA-activated IGF-I promoter function may indicate multiple actions of 17beta -estradiol on activation, binding, and synthesis of the responsible cAMP-activated transcription factor. Once we have identified with certainty the cAMP-activated transcription factor responsible for this effect, we will be better positioned to resolve the mechanism by which its binding is reduced at this element.

In contrast to our findings, earlier studies found that estrogen alone may enhance IGF-I mRNA levels ~2-fold in neonatal rat osteoblasts in vitro (33, 34). We do not yet understand this obvious difference with our results in fetal bone cells or with other in vivo studies where IGF-I mRNA in intramembranous bone increases after OVX (35, 36). Our findings clearly indicate that estradiol reduces nuclear factor binding to the atypical CRE found in the IGF-I promoter, which is much less evident in the basal state. Consequently, the ~2-fold stimulation by estrogen on basal IGF-I expression that was reported previously differs in context from our studies that focus on the ability of this hormone to suppress the more potent 5-10-fold increase in IGF-I expression that occurs in response to PKA activation. Transfection-mediated hER expression was required to observe an effect of estrogen in the studies we present here, including reporter gene expression by the positive estrogen responsive (ERE)2-PRL-Luc, indicating low to negligible levels of ER in our fetal osteoblast cultures. Unlike the earlier results of Ernst and Rodan (34), we have been unable to detect an effect of 17beta -estradiol on IGF-I transcript or promoter function in newly confluent or confluent and aged untransfected primary fetal rat osteoblasts. The reasons for these discrepancies are unclear, but may reflect differences in neonatal bone used by Ernst and Rodan (34) versus fetal bone used in our studies to prepare the primary cell cultures or subsequent culture conditions.

Other earlier studies identified the importance of an AP-1 binding site for the hER-dependent stimulatory effect of 17beta -estradiol on chicken IGF-I promoter activity in human hepatoma cells (61). Again, we could not detect any effect by 17beta -estradiol alone on rat IGF-I promoter activity with or without co-expression of hER in fetal rat bone cells. The minimal region of the IGF-I promoter, which is sensitive to both PGE2 and 17beta -estradiol, does not contain an identifiable AP-1 site (45). We further examined agents such as phorbol myristate acetate, shown to active AP-1, and IGF-I promoter activity was not enhanced (39). These results may reflect differences between rat and chicken IGF-I promoters, between human and rat cells used to assess promoter activity, between liver and bone cells or certain variations that may sometimes occur when promoters are examined in heterologous assay systems.

In contrast to the antagonistic effects that we observe within the IGF-I promoter, activation of PKA can synergistically enhance the stimulatory effect of estrogen on expression of reporter genes containing a conventional ERE (62), as we observed in osteoblasts for the (ERE)2PRL-Luc construct. Potentiation of estrogen action may occur with no detectable changes in ER expression, in estrogen binding to ER, or in ER binding to the ERE, but may result from changes in interactions among other components of the transcriptional apparatus. Additional signals modulated by growth factor receptors, induced by transforming growth factor alpha , epidermal growth factor, or IGF-I, also may activate ERE-containing promoters through estrogen receptor-dependent transcriptional events, possibly by activation of the Ras-mitogen-activated protein kinase signal transduction cascade (63). This latter finding further suggests participation by endogenously synthesized IGF-I in some estrogenic effects in skeletal tissue.

Osteoclastic bone resorption can also be regulated by local, osteoblast-derived factors whose expression is controlled by yet other local and systemic agents (64, 65). In this context, IL-6 expression is suppressed by estrogen (11-13), while it is induced by IGF-I (66). Consistent with other opposing effects of estrogen and agents that induce cAMP, estrogen may suppress PTH-stimulated osteoclast formation by interfering with a downstream event in the PKA-dependent signal pathway in osteoblasts (67). Furthermore, osteoporotic postmenopausal women with primary hyperparathyroidism are as effectively treated by estrogen replacement as they are by parathyroidectomy (68).

A recent case report may indicate the importance of estrogen in men as well as women. A 28-year-old male with an estrogen receptor mutation exhibited incomplete epiphyseal growth plate closure, continued longitudinal bone growth, and osteoporosis, even in the presence of high levels of serum estrogen and normal levels of testosterone (69). Furthermore, mice with insertional disruption of the estrogen receptor have decreased skeletal mineralization in both females and males (70). Therefore, a functional estrogen signal pathway may be needed for proper skeletal maturation and balanced bone remodeling sequence in either sex.

In conclusion, while 17beta -estradiol alone had no effect on IGF-I promoter function, it rapidly and significantly reduced PGE2-mediated promoter activation. This effect was estradiol isomer-selective and ER-dependent. While recombinant hER does not bind directly to the region encompassing the atypical IGF-I CRE, 17beta -estradiol significantly reduced the activation or binding of the transcription factor(s) responsible for cAMP inducible binding to this element. These findings provide new molecular evidence that estrogen may temper PGE2- and PTH-regulated IGF-I actions in bone and may help to explain the additional aspects of altered bone remodeling that occurs with estrogen depletion. These results may have implications for therapeutic regimens for postmenopausal osteoporosis that include combinations of agents to activate bone formation while suppressing the even greater rates of resorption that accompany this event in vivo.


FOOTNOTES

*   This work was supported by National Institutes of Health Grants DK47421 (to T. L. M.) and DK37449 (to P. R.) and by NASA Grant NAGW-4550 (to T. L. M.).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 and reprint requests should be addressed: Section of Plastic Surgery, 333 Cedar St., P. O. Box 208041, New Haven, CT 06520-8041. Tel.: 203-785-4927; Fax: 203-785-5714; E-mail: McCarthyTL{at}maspo3.mas.yale.edu.
1   The abbreviations used are: OVX, ovariectomized; IL, interleukin; IGF-I, insulin-like growth factor-I; IGF-I P1, promoter 1 of the rat IGF-I gene; PTH, parathyroid hormone; PKA, cAMP-activated protein kinase; DMEM, Dulbecco's modified Eagle's medium; ER, estrogen receptor; ERE, estrogen response element; DTT, dithiothreitol; bp, base pair(s); CRE, cAMP response element.
2   T. L. McCarthy and M. Centrella, unpublished data.
3   T. L. McCarthy, Y. Umayahara, M. Centrella, C. Ji, and P. Rotwein, manuscript in preparation.

REFERENCES

  1. Kalu, D. N. (1991) Bone Miner. 15, 175-192 [Medline] [Order article via Infotrieve]
  2. Heaney, R. P., Recher, R. R., and Saville, P. D. (1978) J. Lab. Clin. Med. 92, 964-970 [Medline] [Order article via Infotrieve]
  3. Stepann, J. J., Pospichal, J., Presl, J., and Pacovsky, V. (1987) Bone (N. Y.) 8, 279-284 [Medline] [Order article via Infotrieve]
  4. Turner, R. T., Riggs, B. L., and Spelsberg, T. C. (1994) Endocr. Rev. 15, 129-154
  5. Cantatore, F. P., Loverro, G., Ingrosso, A. M., Lacanna, R., Sassanelli, E., Selvaggi, L., and Carrozzo, M. (1995) Clin. Rheumat. 14, 157-160 [Medline] [Order article via Infotrieve]
  6. Baron, R. (1996) in Primer on the Metabolic Bone Diseases and Disorders of Mineral Metabolism (Favus, M. J., ed), 3rd Ed., pp. 3-10, Lippincott-Raven Publishers, New York
  7. Kalu, D. N., Liu, C. C., Salerno, E., Hollis, B., Echon, R., and Ray, M. (1991) Bone Miner. 14, 175-187 [Medline] [Order article via Infotrieve]
  8. Turner, R. T., Evans, G. L., and Wakley, G. K. (1993) J. Bone Miner. Res. 8, 359-366 [Medline] [Order article via Infotrieve]
  9. Dempster, D. W., Birchman, R., Xu, R., Lindsay, R., and Shen, V. (1995) Bone (N. Y.) 16, 157-161 [CrossRef][Medline] [Order article via Infotrieve]
  10. Gowen, M., Wood, D. D., Ihrie, E. J., McGuire, M. K. B., and Russell, G. G. (1983) Nature 306, 378-380 [Medline] [Order article via Infotrieve]
  11. Girasole, G., Jilka, R. L., Passeri, G., Boswell, S., Boder, G., Williams, D. C., and Manolagas, S. C. (1992) J. Clin. Invest. 89, 883-891 [Medline] [Order article via Infotrieve]
  12. Ray, A., Prefontaine, K. E., and Ray, P. (1994) J. Biol. Chem. 269, 12940-12946 [Abstract/Free Full Text]
  13. Stein, B., and Yang, M. X. (1995) Mol. Cell. Biol. 15, 4971-4979 [Abstract]
  14. Poli, V., Balena, R., Fattori, E., Markatos, A., Yamamoto, M., Tanaka, H., Ciliberto, G., Rodan, G. A., and Costantini, F. (1994) EMBO J. 13, 1189-1196 [Abstract]
  15. Sato, F., Ouchi, Y., Masuyama, A., Nakamura, T., Hosoi, T., Okamoto, Y., Sasaki, N., Shiraki, M., and Orimo, H. (1993) Calcif. Tissue Int. 53, 111-116 [Medline] [Order article via Infotrieve]
  16. Kalu, D. N., Arjmandi, B. H., Liu, C.-C., Salih, M. A., and Birnbaum, R. S. (1994) Bone Miner. 25, 135-148 [Medline] [Order article via Infotrieve]
  17. Shewmon, D. A., Stock, J. L., Rosen, C. J., Heiniluoma, K. M., Hogue, M. M., Morrison, A., Doyle, E. M., Ukena, T., Weale, V., and Baker, S. (1994) Arterioscler. Thromb. 14, 1586-1593 [Abstract]
  18. Russell, S. M., and Spencer, E. M. (1985) Endocrinology 116, 2563-2567 [Abstract]
  19. Skottner, A., Clark, R. G., Robinson, I. C. A. F., and Fryklund, L. (1987) J. Endocrinol. 112, 123-132 [Abstract]
  20. Bagi, C. M., Brommage, R., Deleon, L., Adams, S., Rosen, D., and Sommer, A. (1994) J. Bone Miner. Res. 9, 1301-1312 [Medline] [Order article via Infotrieve]
  21. Bagi, C. M., van der Meulem, M., Brommage, R., Rosen, D., and Sommer, A. (1995) Bone (N. Y.) 16, 559-565 [CrossRef][Medline] [Order article via Infotrieve]
  22. McCarthy, T. L., Centrella, M., and Canalis, E. (1989) Endocrinology 124, 1247-1253 [Abstract]
  23. Canalis, E., Centrella, M., and McCarthy, T. L. (1989) J. Clin. Invest. 83, 60-65 [Medline] [Order article via Infotrieve]
  24. Hock, J. M., Centrella, M., and Canalis, E. (1988) Endocrinology 122, 254-260 [Abstract]
  25. Schmid, C., Guler, H.-P., Rowe, D., and Froesh, E. R. (1989) Endocrinology 125, 1575-1580 [Abstract]
  26. McCarthy, T. L., Centrella, M., and Canalis, E. (1989) Endocrinology 124, 301-309 [Abstract]
  27. McCarthy, T. L., Centrella, M., and Canalis, E. (1990) J. Biol. Chem. 265, 15353-15356 [Abstract/Free Full Text]
  28. Howard, G. A., Bottemiller, B. L., Turner, R. T., Rader, J. I., and Baylink, D. J. (1981) Proc. Natl. Acad. Sci. U. S. A. 78, 3204-3208 [Abstract]
  29. Tam, C. S., Heersche, J. N. M., Murray, T. M., and Parsons, J. A. (1982) Endocrinology 110, 506-512 [Abstract]
  30. Slovik, D. M., Rosenthal, D. I., Doppelt, S. H., Potts, J. T., Jr., Daly, M. A., Campbell, J. A., and Neer, R. M. (1986) J. Bone Miner. Res. 1, 377-381 [Medline] [Order article via Infotrieve]
  31. Shen, V., Dempster, D. W., Mellish, R. M., Birchman, R., Horbert, W., and Lindsay, R. (1992) Calcif. Tissue Int. 50, 214-220 [Medline] [Order article via Infotrieve]
  32. Wronski, T. J., Yen, C.-F., Qi, H., and Dann, L. M. (1993) Endocrinology 132, 823-831 [Abstract]
  33. Ernst, M., Heath, J. K., and Rodan, G. A. (1989) Endocrinology 125, 825-833 [Abstract]
  34. Ernst, M., and Rodan, G. A. (1991) Mol. Endocrinol. 5, 1081-1089 [Abstract]
  35. Turner, R. T., Backup, P., Kline, B. C., Colvard, D. S., and Spelsberg, T. C. (1991) in Molecular Concepts of Insulin-like Growth Factors (Spencer, E. M., ed), pp. 143-153, Elsevier Science Publishing Co., Inc., New York
  36. Turner, R. T., Bachup, P., Shermanm, P. J., Hill, E., Evans, G. L., and Spelsberg, T. C. (1992) Endocrinology 131, 883-889 [Abstract]
  37. McCarthy, T. L., Centrella, M., Raisz, L. G., and Canalis, E. (1991) Endocrinology 128, 2895-2900 [Abstract]
  38. Bichell, D. P., Rotwein, P., and McCarthy, T. L. (1993) Endocrinology 133, 1020-1028 [Abstract]
  39. McCarthy, T. L., Thomas, M. J., Centrella, M., and Rotwein, P. (1995) Endocrinology 136, 3901-3908 [Abstract]
  40. Thomas, M. J., Umayahara, Y., Shu, H., Centrella, M., Rotwein, P., and McCarthy, T. L. (1996) J. Biol. Chem. 271, 21835-21841 [Abstract/Free Full Text]
  41. McCarthy, T. L., Centrella, M., and Canalis, E. (1988) J. Bone Miner. Res. 3, 401-408 [Medline] [Order article via Infotrieve]
  42. Centrella, M., Canalis, E., McCarthy, T. L., Orloff, J. J., Stewart, A. F., and Insogna, K. L. (1989) Endocrinology 125, 199-208 [Abstract]
  43. Centrella, M., Kim, J., Pham, T., Casinghino, S., Rosen, V., Wozney, J., and McCarthy, T. L. (1995) Mol. Cell. Biol. 15, 3273-3281 [Abstract]
  44. Centrella, M., Casinghino, S., Gundberg, C., McCarthy, T. L., Wozney, J., and Rosen, V. (1996) Ann. N. Y. Acad. Sci. 785, 224-226 [Medline] [Order article via Infotrieve]
  45. Hall, L. J., Kajimoto, Y., Bichell, D., Kim, S.-W., James, P. L., Counts, D., Nixon, L. J., Tobin, G., and Rotwein, P. (1992) DNA Cell Biol. 11, 301-313 [Medline] [Order article via Infotrieve]
  46. Bradford, M. M. (1976) Anal. Biochem. 72, 248-254 [CrossRef][Medline] [Order article via Infotrieve]
  47. Lee, K. A., Bindereif, A., and Green, M. R. (1988) Gene. Anal. Tech. 5, 22-31 [CrossRef][Medline] [Order article via Infotrieve]
  48. Revzin, A. (1989) BioTechniques 7, 346-355 [Medline] [Order article via Infotrieve]
  49. Carey, J. (1991) Methods Enzymol. 208, 103-117 [Medline] [Order article via Infotrieve]
  50. Oldham, S. B., Gruber, H. E., and Rude, R. K. (1992) Osteoporosis Int. 2, 174-179 [Medline] [Order article via Infotrieve]
  51. Kimble, R. B., Vannice, J. L., Bloedow, D. C., Thompson, R. C., Hopfer, W., Kung, V. T., Brownfield, C., and Pacifici, R. (1994) J. Clin. Invest. 93, 1959-1967 [Medline] [Order article via Infotrieve]
  52. Murphy, L. J., and Friesen, H. G. (1988) Endocrinology 122, 325-332 [Abstract]
  53. Borski, R. J., Tsai, W., Demottfriberg, R., and Barkan, A. L. (1996) Endocrinology 137, 3253-3259 [Abstract]
  54. Turner, R. T., Riggs, B. L., and Spelsberg, T. C. (1994) Endocr. Rev. 15, 129-154
  55. Salih, M. A., Liu, C. C., Arjmandi, B. H., and Kalu, D. N. (1993) Bone Miner. 23, 285-299 [Medline] [Order article via Infotrieve]
  56. Zofkova, I., and Kancheva, R. L. (1996) Bone (N. Y.) 19, 227-232 [CrossRef][Medline] [Order article via Infotrieve]
  57. Jee, W. S., Mori, S., Li, X. J., and Chan, S. (1990) Bone 11, 253-266 [Medline] [Order article via Infotrieve]
  58. Jee, W. S., Akamine, T., Ke, H. Z., Li, X. J., Tang, L. Y., and Zeng, Q. Q. (1992) Bone (N. Y.) 13, 153-159 [Medline] [Order article via Infotrieve]
  59. Kawaguchi, H., Pilbeam, C. C., Harrison, J. R., and Raisz, L. G. (1995) Clin. Orthop. 313, 36-46 [Medline] [Order article via Infotrieve]
  60. Hsueh, A. J. W. (1989) in Endocrinology (DeGroot, L. J., ed), 2nd Ed., pp. 1929-1939, W. B. Saunders Co., Philadelphia
  61. Umayahara, Y., Kawamori, R., Watada, H., Imano, E., Iwama, N., Morishima, T., Yamasaki, Y., Kajimoto, Y., and Kamada, T. (1994) J. Biol. Chem. 269, 16433-16442 [Abstract/Free Full Text]
  62. Aronica, S. M., and Katzenellenbogen, B. S. (1993) Mol. Endocrinol. 7, 743-752 [Abstract]
  63. Kato, S., Endoh, H., Masuhiro, Y., Kitamoto, T., Uchiyama, S., Sasaki, H., Masushige, S., Gotoh, Y., Nishida, E., Kawashima, H., Metzger, D., and Chambon, P. (1995) Science 270, 1491-1494 [Abstract]
  64. Rodan, G. A., and Martin, T. J. (1981) Calcif. Tissue Int. 33, 349-351 [Medline] [Order article via Infotrieve]
  65. Hill, P. A., Reynolds, J. J., and Meikle, M. C. (1995) Endocrinology 136, 124-131 [Abstract]
  66. Slootweg, M. C., Most, W. W., van Beek, E., Schot, L. P., Papapoulos, S. E., and Lowik, C. W. (1992) J. Endocrinol. 132, 433-438 [Abstract]
  67. Kaji, H., Sugimoto, T., Kanatani, M., Nasu, M., and Chihara, K. (1996) Endocrinology 137, 2217-2224 [Abstract]
  68. Diamond, T., Ng, A. T. M., Levy, S., Magarey, C., and Smart, R. (1996) Osteoporosis Int. 6, 329-333 [Medline] [Order article via Infotrieve]
  69. Smith, E. P., Boyd, J., Frank, G. R., Takahashi, H., Cohen, R. M., Specker, B., Williams, T. C., Lubahn, D. B., and Korach, K. S. (1994) N. Engl. J. Med. 331, 1056-1061 [Abstract/Free Full Text]
  70. Lubahn, D. B., Moyer, J. S., Golding, T. S., Couse, J. F., Korach, K. S., and Smithies, O. (1993) Proc. Natl. Acad. Sci. U. S. A. 90, 11162-11166 [Abstract]

©1997 by The American Society for Biochemistry and Molecular Biology, Inc.