Estrogen Opposes the Apoptotic Effects of Bone Morphogenetic Protein 7 on Tissue Remodeling

doi:10.1128/MCB.20.13.4626-4634.2000

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Molecular and Cellular Biology, July 2000, p. 4626-4634, Vol. 20, No. 13
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Estrogen Opposes the Apoptotic Effects of Bone Morphogenetic Protein 7 on Tissue Remodeling

David G. Monroe,¹ Donald F. Jin,² and Michel M. Sanders¹^,^*

Department of Biochemistry, Molecular Biology, and Biophysics, University of Minnesota, Minneapolis, Minnesota 55455,¹ and Creative BioMolecules, Hopkinton, Massachusetts 01748²

Received 30 November 1999/Returned for modification 17 January 2000/Accepted 20 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Interactions between estrogen and growth factor signaling pathways at the level of gene expression play important roles inthe function of reproductive tissues. For example, estrogen regulatestransforming growth factor beta (TGF $beta$ ) in the uterus during theproliferative phase of the mammalian reproductive cycle. Bonemorphogenetic protein 7 (BMP-7), a member of the TGF $beta$ superfamily,is also involved in the development and function of reproductivetissues. However, relatively few studies have addressed the expressionof BMP-7 in reproductive tissues, and the role of BMP-7 remainsunclear. As part of an ongoing effort to understand how estrogenrepresses gene expression and to study its interactions with othersignaling pathways, chick BMP-7 (cBMP-7) was cloned. cBMP-7 mRNAlevels are repressed threefold within 8 h following estrogen treatmentin the chick oviduct, an extremely estrogen-responsive reproductivetissue. This regulation occurs at the transcriptional level. Estrogenhas a protective role in many tissues, and withdrawal from estrogenoften leads to tissue regression; however, the mechanisms mediatingregression of the oviduct remain unknown. Terminal transferase-mediatedend-labeling and DNA laddering assays demonstrated that regressionof the oviduct during estrogen withdrawal involves apoptosis,which is a novel observation. cBMP-7 mRNA levels during estrogenwithdrawal increase concurrently with the apoptotic index of theoviduct. Furthermore, addition of purified BMP-7 induces apoptosisin primary oviduct cells. This report demonstrates that the functionof BMP-7 in the oviduct involves the induction of apoptosis andthat estrogen plays an important role in opposing thisfunction.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Reproductive tissues exist in a delicate balance between the processes of proliferation, differentiation, cell cycle inhibition,and apoptosis (41). These processes are largely mediated bythe actions and interactions of growth factors and steroid hormones(26, 67). Estrogen is a potent mitogenic steroid hormone involvedin many aspects of the development and maintenance of numeroustarget tissues (65). The mammalian female reproductive tract,for example, is extremely sensitive to plasma estrogen levelsduring normal estrus cycles, as proliferation and regression ofthe endometrium depend largely on the estrogen concentration (6).These modulatory actions of estrogen are mediated by the estrogenreceptor (ER), which affects gene expression by binding to estrogenresponse elements (EREs) in the regulatory regions of target genes(39). The interplay between estrogen and growth factor signalingat the level of gene expression is clearly important, since estrogeninduces the genes that encode such growth factors as epidermalgrowth factor, transforming growth factor alpha (TGF- $alpha$ ), and insulin-likegrowth factor-1, which are involved in various aspects of reproductivehomeostasis (25, 44, 45). In contrast, the transforminggrowth factor beta (TGF- $beta$ ) superfamily of growth factors inhibitepithelial cell proliferation in reproductive tissue and oftenact to antagonize the proliferative estrogenic signals (15,55). Although both growth hormone and steroid hormone pathwaysplay important roles in reproductive physiology, little is knownabout the mechanisms of interaction between these pathways atthe level of gene expression and the potential consequences ofthe interaction to reproductivetissues.

The bone morphogenetic proteins (BMPs) are a large subset of the TGF- $beta$ superfamily of extracellular signaling proteins thathave been implicated in differentiation, development, and tissueremodeling (22). BMPs were initially identified by the abilityof bone extracts to induce bone formation at extraskeletal sites(60, 73). BMP-7 (also called osteogenic protein-1 and OP-1)was originally cloned from a human genomic library in a screendesigned to isolate genes involved in bone formation (50) andhas since been cloned from a mouse (51), Xenopus laevis (76),and partially cloned from a chick (23). BMP-7 is synthesizedas an inactive preprohormone and is proteolytically cleaved toproduce a mature protein of 139 amino acids (50). The matureform of BMP-7 binds the type II serine/threonine kinase receptor,ActRII or ActRIIB, subsequently recruiting and phosphorylatingthe type I receptor, ALK-2 (38). The active form of ALK-2 signalsthrough Smad1, -5, and -8, culminating in the regulation of BMP-7target genes such as the genes for type X collagen (17, 74)and Tlx2 (70). Although some downstream events in the BMP-7pathway are known, the regulation of the BMP-7 gene remains amystery since neither the transcriptional start site nor the promoterof the BMP-7 gene has been characterized in anysystem.

BMP-7 has been implicated in such diverse processes as murine hind brain development (2), tooth development (19), nephrogenesis,eye development, and skeletal patterning (36). A BMP-7 nullmutation in mice results in severe developmental defects in theskeleton, eye, and kidney (28). BMP-7-deficient mice also exhibitpolydactyly in their hind limbs, indicating a role for BMP-7 indigit formation (28). These data suggest that BMP-7 may alsohave important roles in tissue remodeling. In addition to therole of BMP-7 in development, a virtually unexplored role in reproductivetissue is emerging. Because estrogen injection into nonpregnantmice decreases BMP-7 mRNA levels in the uterus (49) and becausewithdrawal of estrogen induces apoptosis of the uterine epithelium(75), we speculated that estrogen withdrawal leads to an increasein BMP-7, which triggers apoptosis in estrogen-responsive organssuch as the uterus and oviduct. However, no direct evidence existsto suggest that BMP-7 has a role in induction of apoptosis inthe uterine epithelium, and no biochemical data exist as to theexact function of BMP-7 in theuterus.

To further define the relationship between estrogen and BMP-7 and to determine the physiological significance of BMP-7 expressionin reproductive organs, BMP-7 mRNA levels were examined in thechick oviduct. The oviduct is the functional equivalent of thehuman Fallopian tube and is extremely estrogen responsive (6),making it an ideal system for studying estrogen regulation oftranscription. Additionally, the development of the oviduct canbe precisely controlled in immature chicks, allowing detailedexamination of specific developmental processes. This study providesadditional characterization of the inverse relationship betweenestrogen and BMP-7 mRNA expression by demonstrating that estrogenrepresses chick BMP-7 (cBMP-7) gene expression at the transcriptionallevel. We also report that estrogen deficiency leads to increasedcBMP-7 mRNA production and stimulates apoptosis of the oviduct.Finally, addition of purified BMP-7 to primary oviduct cells directlyinduces apoptosis, demonstrating that BMP-7 has an important rolein tissue remodeling by driving apoptoticevents.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Animals and estrogen treatments. Two-week-old, sexually immature White Leghorn chicks were implanted with 2 diethylstilbestrol (DES) pellets (Hormone PelletPress, Leawood, Kans.) for at least 2 weeks to induce developmentof the oviduct. Withdrawn oviducts were produced by withdrawalof the DES pellets. DES was withdrawn for 5 days, unless otherwisenoted. Secondary stimulation of 5-day estrogen-withdrawn chickswas performed for the indicated times by wing vein injection of17- $beta$ -estradiol (25 mg/kg of body weight). After all treatments,the magnum portion of the oviduct was frozen in liquid nitrogenprior to storage at $-$ 70°C.

Cloning of cBMP-7. In order to clone the complete cBMP-7 coding sequence, a 5-day estrogen-withdrawn chick oviduct cDNA library was screenedwith a PCR-generated probe designed to a chick partial cDNA sequence(23). The probe was constructed using a 5' primer located at+367 to +382 and a 3' primer located at +1306 to +1328 relativeto the translational start codon (Fig. 1). The previously clonedcBMP-7 sequence included nucleotides +367 to +1364. Our effortsresulted in a more complete sequence ranging from +111 to +1728(GenBank accession number AF205877). A 3'-RACE (rapid amplificationof cDNA ends) reaction using a 5-day estrogen-withdrawn libraryconstructed using the Marathon cDNA amplification kit (Stratagene,La Jolla, Calif.) and the 5' primer described above generateda clone extending to +1974 that included a polyadenylation signaland a polyadenylated [poly(A)⁺] tail. Sequence comparison with human and mouse BMP-7 suggestedthat the extreme 5' end of the coding sequence was absent. Furtherscreening of the 5-day W/D oviduct cDNA library and the 5-dayestrogen-withdrawn oviduct RACE library yielded no additional5' sequence. Therefore, a chicken genomic library (courtesy ofKathleen Conklin, University of Minnesota) was screened usinga probe located from +121 to +324, which is contained entirelyon exon 1 in the mouse and is located on the same exon in thechicken (data not shown). A clone located from $-$ 1808 to +374 (GenBankaccession number AF223970) relative to the start site of translationwas isolated that included an in-frame translational start codon.The translated sequence was aligned with both human (GenBank accessionnumber X51801) and mouse (GenBank accession number X56906)sequences (Fig. 2) using the GCG computer package (Genetics ComputerGroup, Madison, Wis.).

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FIG. 1. Full-length cBMP-7 cDNA clone obtained as described in Materials and Methods. The complete cBMP-7 sequence (GenBank accession numbers AF205877 and AF223970) was translated, and the consensus ATG translational start codon is in bold. The nucleotides are numbered on the left using ATG as nucleotide +1 because the promoter and 5'-UTR have not been mapped. The predicted form of cBMP-7 following processing at the RSIR cleavage site is underlined. An asterisk denotes the translational stop codon, and the polyadenylation recognition sequence is boxed. The previously cloned cBMP-7 sequence included nucleotides +367 to +1364 (23).

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FIG. 2. cBMP-7 amino acid sequence is highly homologous to human and mouse BMP-7. The cBMP-7 amino acid sequence was aligned with the human (X51801) and mouse (X56906) BMP-7 sequences using the GCG computer package and found to be 86% identical throughout the entire protein. The dashes represent identical amino acid matches, and the dots represent gaps in the sequence. The amino acid sequence is numbered on the left.

Tissue preparation and Northern blot analysis. Total RNA was isolated using the phenol-guanidinium isothiocyanate-based RNAzol B reagent (Tel-Test, Friendsville, Tex.),and poly(A)⁺-selected RNA was isolated using the Poly(A)⁺ Tract isolation kit (Promega, Madison, Wis.). Northern blot analysiswas conducted by electrophoresing 2 µg of poly(A)⁺ RNA on an 0.8% formaldehyde gel. The separated RNA was transferredto nitrocellulose (Schleicher & Schuell, Keene, N.H.) using anelectrotransfer apparatus (Bio-Rad, Hercules, Calif.) and cross-linkedby UV irradiation (Stratagene). The Northern blots were hybridizedovernight at 42°C with the indicated random primer-labeled cDNAprobes (random primer labeling kit from Stratagene) in hybridizationsolution. The blots were washed in a final wash of 0.2× SSC (1×SSC is 0.15 M NaCl plus 0.015 M sodium citrate)-0.1% sodium dodecylsulfate for 15 min and exposed to Hyperfilm with an intensifyingscreen at $-$ 70°C for 3 days. The housekeeping gene glyceraldehyde-3-phosphatedehydrogenase (GAPDH) was used as a non-estrogen-regulated control(40) to demonstrate equal loading of the lanes. Densitometricanalysis of RNA bands was conducted using a Bio-Rad densitometerand the Molecular Analyst software package (Bio-Rad). Statisticswere generated using Scheffe's analysis of variance test for statisticalsignificance. Differences were considered significant at P < 0.05.

Nuclear run-on transcription assays. Nuclear run-on assays were performed as previously described with a few modifications (47). Briefly, nuclei were obtainedfrom 5-day estrogen-withdrawn and estrogen-stimulated oviductsby Dounce homogenization followed by ultracentrifugation. Thenuclei were placed in a transcription reaction that included 125µCi each of ³²P-labeled UTP and CTP (700 Ci/mmol; New England Nuclear) for 40min and subsequently treated with proteinase K and DNase. Thelabeled RNA was extracted using RNAzol, and approximately 2 ×10⁷ cpm were hybridized for 36 h at 65°C to 4 µg of cDNA immobilizedon a filter. The cBMP-7 cDNA consisted of a fragment spanningthe 3' end of the coding region and the 3' untranslated region(UTR) (nucleotides 360 to 1328). Full-length hepatocyte nuclearfactor 3 $beta$ (HNF-3 $beta$ ) cDNA (3) was used as a non-estrogen-regulatedcontrol. The blots were washed, and unhybridized RNA was removedby treatment with RNase A and RNase T₁ at 37°C for 1 h. Filterswere exposed to a phosphorimager screen overnight, and quantitationwas performed using the Molecular Analyst software (Bio-Rad).

Detection of apoptosis. The induction of apoptosis was determined by using a terminal transferase-mediated end-labeling procedure (TUNEL) on serialsections of paraffin-embedded oviduct tissue (Surgical PathologyLab, University of Minnesota), using the ApopTag assay kit (Intergen,Purchase, N.Y.). TUNEL-positive cells were scored by examinationof four consecutive fields (×200 magnification) and totaled asa percentage of 4,000 cells each. Negative controls for each tissueconsisted of adjacent sections where terminal transferase wasomitted. No significant background staining was observed in anyof the control sections (data not shown). Detection of apoptosisin primary oviduct cell culture was accomplished by measuringinternucleosomal DNA laddering using the TACS apoptotic DNA ladderingkit-isotopic (Sigma, St. Louis, Mo.) per the manufacturer's protocol.Briefly, DNA was extracted from primary oviduct cells and Klenow-labeledusing 0.5 µCi of dCTP (3,000 Ci/mmol; New England Nuclear). Theentire reaction was separated on a 1.5% agarose gel, dried, andexposed to film for 8 h. Quantitation was performed by densitometryof the three smallest oligonucleosomalfragments.

Primary oviduct cell culture. Preparation of the primary oviduct cells was performed as previously described (61). Briefly, 2-day estrogen-withdrawn chickoviducts were dissociated using a mixture of collagenase, protease,DNase, and trypsin. Dissociated cells were washed three timeswith culture medium, and cells from 100 mg of tissue were platedinto each dish containing serum-free Dulbecco's modified Eagle'smedium-F12 medium (1:1) and the indicated concentrations of mouseBMP-7 (Creative BioMolecules, Hopkinton, Mass.). Cells were harvested20 h later, resuspended in Tris buffer, and frozen until the intranucleosomalDNA laddering assay wasperformed.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Cloning of the cBMP-7 coding region indicates that it is highly homologous to human and mouse BMP-7. Characterization of the promoter and enhancer sequences involved in regulation of the BMP-7 gene would facilitate the understandingof BMP-7 function and responsiveness to cellular signals. However,these cis-acting sequences have not been identified in any system.As a first step in studying the regulation of the BMP-7 gene inthe chick oviduct, and since a previously cloned chick cDNA lacksthe 5' end of the open reading frame (23), an effort to clonethe complete open reading frame of cBMP-7 and the 5'-flankingregion was initiated. Cloning of the coding region of cBMP-7 wasaccomplished by screening an estrogen withdrawn chick oviductcDNA library, a 3'-RACE estrogen-withdrawn chick oviduct cDNAlibrary, and a chicken genomic library (see Materials and Methodsfor specifics). The deduced amino acid sequence reveals that thecBMP-7 gene encodes a 435-amino-acid protein (Fig. 1), whereasthe human and mouse BMP-7 genes encode proteins of 431 and 430amino acids, respectively (50, 51). The similarity of thepredicted size of cBMP-7 to human and mouse BMP-7 suggests thatthe entire coding region has been cloned. Alignment of the codingregion of cBMP-7 with human and mouse BMP-7 sequences (Fig. 2)reveals 86% identity. A predicted dibasic protease cleavage sequence(RSIR) exists (amino acids 293 to 296), as observed in human andmouse BMP-7 sequences. Cleavage at this site would produce a matureprotein of 139 amino acids that is 96% identical to human andmouse BMP-7. This predicted protein contains the conserved 7-cysteinedomain observed in many members of the TGF- $beta$ superfamily. The3'-UTR of cBMP-7 contains a polyadenylation signal sequence (11),indicating that the entire 3' coding sequence is cloned. Cloningof the extreme 5' open reading frame was accomplished by screeninga chicken genomic library and is characterized by an extremelyGC-rich sequence. Thus, the cloning of the cBMP-7 coding regionincluding a previously undescribed 3'-UTR has been accomplished.However, S1 analysis of ~500 bp upstream of the start site oftranslation (data not shown) did not reveal an obvious promoteror start site for transcription, so the location and nature ofthe cBMP-7 regulatory sequences remainundetermined.

cBMP-7 mRNAs are repressed by estrogen at the transcriptional level in the oviduct. Regulation of reproductive processes often includes the modulatory actions of estrogen on gene expression, including genesinvolved in growth hormone signaling (15, 25, 44, 45,55). In order to determine whether this generalization can beextended to BMP-7 signaling in the oviduct, Northern blot analysisof poly(A)⁺ RNA from estrogen withdrawn and estrogen-stimulated oviductswas performed using a probe specific for cBMP-7 (data not shown).cBMP-7 mRNA levels are decreased threefold in estrogen-stimulatedoviducts compared to estrogen-withdrawn oviducts (Fig. 3A). Asimilar fourfold repression in the amount of cBMP-7 mRNA was observedin untreated laying hens, indicating that repression by estrogendoes indeed occur in a physiologically relevant state (data notshown). Three major BMP-7 mRNA species are observed, consistentwith a previously published report for mouse BMP-7 (51). Densitometryindicates that all mRNA species are repressed to roughly the sameextent. The exact nature of the multiple transcripts is currentlyunknown in any system. The estrogen-inducible transcription factordelta-EF1 (7) is shown to illustrate that a concomitant inductiveresponse occurs in estrogen-stimulated oviducts, confirming thatestrogen does not have a generalized negative effect on transcriptionin the oviduct. To the contrary, the genes for ovalbumin (62),connexin 43 (20), glycoprotein (27), cystic fibrosis transmembraneregulator (56), leukemia inhibitory factor (54), H-ras (9),and myosin light-chain kinase (57) are induced by estrogen inthe oviducts of various species. Additionally, the genes for epidermalgrowth factor and TGF- $alpha$ are induced in the oviduct (63), demonstratingthat some members of the TGF- $beta$ superfamily can respond positivelyto estrogen in this tissue and that there is some specificityin the repression of the cBMP-7 gene by estrogen.

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FIG. 3. cBMP-7 gene expression is repressed by chronic estrogen treatment. (A) Poly(A)⁺ RNA (2 µg) was isolated from 5-day estrogen-withdrawn (5-day W/D) and estrogen-stimulated (Stim) oviducts and subjected to Northern blot analysis. The blot was probed with a cBMP-7 cDNA fragment spanning nucleotides 360 to 1328 (Fig. 1). This probe was determined to be specific to cBMP-7, since a probe designed exclusively to the 3'-UTR yielded identical results upon Northern blot analysis (data not shown). Arrows point to the main mRNA species (labeled in kilobases). The blot was probed a second time with GAPDH, a gene not regulated by estrogen (40), to normalize for loading of the lanes. The estrogen-inducible gene delta-EF1 (7) is shown to demonstrate that estrogen does not have a generalized repressive effect on the oviduct. (B) The experiment was repeated five times and the 4.4-kb band was subjected to densitometric analysis. The BMP-7-GAPDH ratio was plotted relative to stimulation. The error bars represent the standard deviation, and the repression was determined to be statistically significant (P < 0.0001).

In order to determine the kinetics of repression of cBMP-7 gene expression by estrogen, estrogen-withdrawn chicks were injectedwith 17 $beta$ -estradiol for the indicated times, and Northern blotanalysis was conducted (Fig. 4). cBMP-7 mRNA levels are decreasedto estrogen-stimulated levels within 8 h of treatment. Surprisingly,a 1.5-fold induction of cBMP-7 mRNAs was observed 2 h followingestrogen treatment. The reason for this rapid but transient increasein cBMP-7 mRNA remains unknown. In order to determine whetherthe decrease in cBMP-7 mRNA is due to transcriptional or posttranscriptionalevents, a nuclear run-on experiment was conducted (Fig. 5). Thetranscriptional activity of the cBMP-7 gene is repressed 3.5-foldin the estrogen-treated oviduct compared with the estrogen-withdrawnoviduct. The extent of repression agrees well with the Northernblot data (Fig. 3 and 4), indicating that the regulation of cBMP-7by estrogen occurs at the transcriptional level. These data indicatethat estrogen represses cBMP-7 gene expression and that an inverserelationship between estrogen concentration and cBMP-7 mRNA levelsexists in the oviduct. This is the first information garneredin any system that indicates how the expression of the BMP-7 geneis regulated.

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FIG. 4. 17 $beta$ -Estradiol represses cBMP-7 mRNAs within 8 h. Poly(A)⁺ RNA (2 µg) was isolated from oviducts after injection of 5-day estrogen-withdrawn animals with 17 $beta$ -estradiol, and Northern blot analysis was performed as in Fig. 3. This experiment was performed twice in duplicate. The asterisks signify samples that are statistically different from the 5-day estrogen-withdrawn or zero time point samples (P < 0.0001).

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FIG. 5. Repression of cBMP-7 gene expression by estrogen occurs at the transcriptional level. Nuclei were isolated from 5-day estrogen-withdrawn (W/D) and estrogen-stimulated (Stim) oviducts and placed in a nuclear run-on transcription reaction. RNA was isolated and hybridized to a filter containing either cBMP-7 or HNF-3 $beta$ cDNAs. HNF-3 $beta$ , a gene not transcriptionally regulated by estrogen (3), was used as a control.

Estrogen withdrawal induces apoptosis of the oviduct. Steroid hormones are essential for maintaining reproductive vitality. However, during the female reproductive cycle and duringaging, steroid levels fluctuate or diminish, respectively (6).Few studies have examined the resultant effects on reproductivetissues. In periods of low plasma estrogen levels, the oviductregresses in size due to unknown mechanisms (8, 64). TUNEL(13) and internucleosomal DNA laddering (1) analyses wereperformed on estrogen-stimulated and estrogen-withdrawn oviductsin order to determine whether estrogen withdrawal induces apoptosis.TUNEL analysis indicated that in estrogen-stimulated oviduct,0.44% ± 0.38% (standard deviation) of the total number of cellsare apoptotic, whereas in estrogen-withdrawn oviduct, 7.92% ±2.2% of the cells are apoptotic (Fig. 6A and B, respectively).This demonstrates that estrogen withdrawal triggers an 18-foldincrease in apoptosis. To further verify that estrogen withdrawalinduces apoptosis of the chick oviduct, an internucleosomal DNAladdering assay was performed (Fig. 6C). DNA fragmentation ofchromatin into oligonucleosome-length fragments is a hallmarkof the apoptotic response (34, 35). The internucleosomal DNAladdering assay indicated that estrogen withdrawal induces a sixfoldincrease in DNA laddering compared to the estrogen-stimulatedoviduct (Fig. 6C). The discrepancy between the fold inductionof apoptosis between the TUNEL and DNA laddering assays can beattributed to the different sensitivities of each individual assay(16). Nonetheless, the data indicate that estrogen withdrawalspecifically induces apoptosis. This observation is the firstdirect evidence that the regression of the oviduct due to estrogenwithdrawal is the result of apoptosis.

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FIG. 6. Withdrawal of estrogen induces apoptosis in the oviduct. Oviducts from (A) estrogen-stimulated and (B) 5-day estrogen-withdrawn chicks were sectioned and subjected to TUNEL analysis. The dark spots represent TUNEL-positive cells, which were scored by examination of four consecutive fields and totaled as a percentage of ~4,000 cells. An 18-fold induction of apoptosis was observed in the 5-day estrogen-withdrawn oviduct. The experiment was repeated twice with similar results. (C) Apoptosis was also determined using an internucleosomal DNA fragmentation laddering assay. DNA (1 µg) was Klenow-labeled and separated by gel electrophoresis. The brackets denote the areas subjected to densitometric analysis, and the numbers indicate the sizes of the oligonucleosomal DNA fragments. The values of the three areas were totaled to quantitate the amount of DNA laddering per lane. A sixfold increase in DNA laddering was observed in the 5-day estrogen-withdrawn oviduct. The experiment was repeated twice with similar results.

Regression of the oviduct correlates with increased cBMP-7 mRNA levels. cBMP-7 gene expression is repressed by estrogen (Fig. 3 to 5), suggesting an inverse relationship between estrogen concentrationand both the production of cBMP-7 mRNA and the induction of apoptosis(Fig. 6). Since both events occur following estrogen withdrawal,it seems probable that cBMP-7 is involved in the apoptotic response.To determine whether these events follow a similar time courseduring shorter withdrawal periods, estrogen was withdrawn for1, 2, or 3 days. TUNEL and Northern blot analyses were done todetermine whether apoptosis and an increase in cBMP-7 mRNA levelsoccur concomitantly. As shown in Fig. 7, little apoptosis is observedin the estrogen-stimulated oviduct (Fig. 7A). However, a sixfoldincrease in apoptosis is observed in the 1-day estrogen-withdrawnoviduct (Fig. 7B), with a 10- and 16-fold induction of apoptosisin 2-day and 3-day estrogen-withdrawn oviducts, respectively (Fig.7C and D). Northern blot analysis indicated cBMP-7 mRNA levelsfollow the same temporal pattern as apoptosis, with a 2-fold increasein the 1-day estrogen-withdrawn oviduct, a 2.8-fold increase in2-day withdrawn oviduct, and a 3.5-fold increase in 3-day withdrawnoviduct (Fig. 7E). The increase in cBMP-7 mRNA mirrors the onsetof apoptosis induced by estrogen withdrawal (Fig. 7F). These datademonstrate that the induction of apoptosis and the increase incBMP-7 mRNA levels are concomitant.

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FIG. 7. Increasing apoptosis in oviduct withdrawn from estrogen for various times is correlated with an increase in BMP-7 mRNA. Chicks stimulated with estrogen for 21 days were withdrawn from estrogen for 1, 2, or 3 days. Part of the oviduct was paraffin embedded, sectioned, and subjected to TUNEL analysis. The rest of the oviduct was used to isolate poly(A)⁺ RNA for Northern blot analysis. (A) Results of the TUNEL assay on estrogen-stimulated chicks. The other panels are the results of the TUNEL assay on chicks withdrawn from estrogen for (B) 1, (C) 2, or (D) 3 days, indicating an increase in apoptotic cells throughout the withdrawal time course. (E) Northern blot analysis indicates that the increase in BMP-7 mRNA correlates with the increase in apoptosis. Only the 4.4-kb mRNA of BMP-7 is shown. GAPDH mRNA was measured as the loading control. (F) The induction of cBMP-7 mRNA and an increase in apoptosis over time are graphically represented as the top and bottom line, respectively. This experiment was repeated with comparable results. Data points and error bars represent the mean and the range, respectively.

BMP-7 induces apoptosis in primary oviduct cell culture. To directly test the possibility that BMP-7 induces apoptosis in the oviduct, primary oviduct cells were cultured with increasingconcentrations of mouse BMP-7 and harvested 20 h later. Inductionof apoptosis in primary oviduct cells was dose dependent, witha twofold increase at 10 and 50 ng/ml and a threefold increaseat 100 and 200 ng/ml (Fig. 8). The primary oviduct cell culturemodel system that has been developed (61) utilizes 2-day estrogen-withdrawnoviduct as a source of cells. Since apoptosis is already occurringin this tissue (Fig. 7C), the fold induction of apoptosis reportedin Fig. 8 represents an increase in the apoptotic index over a2-day estrogen-withdrawn oviduct. Thus, the level of apoptosisinduced in primary oviduct cell cultures by treatment with BMP-7for 20 h is comparable to that induced by estrogen withdrawalin vivo. These data demonstrate that BMP-7 induces molecular eventsleading to apoptosis.

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FIG. 8. Addition of mouse BMP-7 to primary oviduct cell culture induces apoptosis. Oviducts withdrawn from estrogen for 2 days were dissociated and placed into tissue culture as previously described (61). Cultures were treated with the indicated BMP-7 concentrations for 20 h and harvested. Internucleosomal DNA laddering was performed as in Fig. 6. Treatment of primary oviduct cells with 10 and 50 ng of BMP-7 per ml resulted in a twofold induction of apoptosis, whereas the highest concentrations induced a threefold response. Each BMP-7 treatment was done in duplicate, and the experiment was conducted twice with similar results. Data points and error bars represent means and ranges, respectively.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This study demonstrates that estrogen represses cBMP-7 gene expression in the oviduct (Fig. 3), agreeing well with a previousobservation that estrogen treatment leads to decreased BMP-7 mRNAsin the mouse uterus (49). Repression of cBMP-7 mRNA levels wasobserved within 8 h following 17 $beta$ -estradiol injection (Fig. 4)and occurs at the transcriptional level (Fig. 5). In an attemptto identify an ER binding site or an estrogen-dependent repressorelement to explain the repression of cBMP-7 by estrogen, a 3.8-kbgenomic DNA fragment upstream of the translational start codonof cBMP-7 was isolated. Sequence analysis did not reveal any estrogenresponse elements or any known estrogen-responsive repressor elements(data not shown). The genomic sequence contained no obvious promoterelements (TATA box, CCAAT box, etc.); however, an extensive GC-richregion containing numerous SP-1 binding sites upstream of thecoding region is reminiscent of TATA-less promoters (66). Sincethe transcriptional start site and promoter for the BMP-7 genehave not yet been characterized in any species, the mechanismsof estrogen-mediated repression of cBMP-7 gene expression remainunknown.

Estrogen-specific repression of gene expression has been observed for the interleukin-6 (53), follicle-stimulating hormone- $beta$ (43), glycoprotein hormone- $alpha$ subunit (30), and gonadotropinreleasing hormone (29) genes. In all cases, repression of geneexpression by estrogen occurs in the absence of a high-affinityDNA-binding site for ER, although mutation or deletion of theDNA-binding domain of ER abolishes repression (43, 53). Itis thought that the DNA-binding domain may participate in protein-proteininteractions or may be required for the proper function of theER. Indeed, the repression of the interleukin-6 gene is mediatedby a protein interaction between ER and the necessary activator,NF- $kappa$ B, preventing it from activating transcription (12, 31,53). Interestingly, there is a potential NF- $kappa$ B site upstreamof the start site of translation of cBMP-7 (data not shown), raisingthe possibility that ER may repress the BMP-7 gene by squelchingthe effects of NF- $kappa$ B. However, functional characterization ofthe cBMP-7 promoter is needed to determine the mechanism ofrepression.

Regulation of the BMP-7 gene by estrogen appears to be a complex process, since a statistically significant 1.5-fold inductionoccurs within 2 h following estrogen treatment. The function ofthis transient increase in mRNA levels is not clear, althoughit is interesting to speculate that the initial increase in BMP-7may play a role in its repression at later times. Similarly, TGF- $beta$ 1-3mRNA levels are also induced quickly (<2 h) following estrogentreatment in the uterus but decrease to below control levels by6 h (68), suggesting that this type of regulation may representa general theme for estrogen-regulated TGF- $beta$ family members. Regulationof BMP-7 mRNA levels also appears to be multihormonal, since androgentreatment of castrated mice results in a fourfold increase inBMP-7 mRNA levels in the prostate within 72 h (71), lendingsupport to the contention that steroid hormones regulate expressionof the BMP-7 gene. Regulation of the BMP-7 signaling pathway inthe oviduct also occurs at the level of the receptor, as estrogenwithdrawal increases the sensitivity of the oviduct to cBMP-7by upregulating its receptor, ALK-2 (38), approximately 2.5-fold(data not shown). Similarly, estrogen withdrawal also inducesan increase in TGF- $beta$ type II receptor mRNA in the uterine endometrium,leading to an increased sensitivity of the tissue to TGF- $beta$ ligands(75). It appears clear that the convergence of the estrogenand BMP-7 pathways occurs at multiple points, generating a greaterresponse of the oviduct to BMP-7signaling.

We report the novel observation that estrogen withdrawal initiates cellular events leading to apoptosis in the oviduct (Fig.6 and 7). Induction of apoptosis following estrogen withdrawalhas been observed in other tissues, such as the uterine epithelium(75), vagina (4), osteocytes (72), and MCF-7 xenograftsin nude mice (10). These observations are not confined to estrogenwithdrawal, since androgen withdrawal also induces apoptosis ofthe ventral prostate gland (5, 32). This is consistent withthe concept that steroid hormones are involved in the maintenanceof their target tissues, and withdrawal from hormone results incellular events that often culminate in apoptosis. However, themolecular mediators directly driving apoptosis in these tissuesare unknown. Our observation that BMP-7 drives apoptosis in theoviduct raises the possibility that BMP-7 mediates apoptosis inthese other reproductive tissues as well. Additionally, whilesome members of the BMP family have been implicated in apoptoticprocesses (14, 37), BMP-7 is the first family member implicatedin apoptosis of a reproductive tissue, which may represent a previouslyunrecognized function for BMPmolecules.

Cellular events leading to apoptosis are mediated by modulation of the expression of specific genes or alteration of existinggene products (48). However, the specific intracellular mechanismsinvolved in the activation of apoptotic pathways by BMP-7 signalingare unknown. We expect that the caspase (42, 48, 52) andBcl (24, 46) gene families are of importance in regulatingapoptotic events in the oviduct due to their nearly universalinvolvement in known apoptotic pathways (33). Delineation ofthe molecular target(s) of BMP-7 signaling in the apoptotic pathwaymay provide a general model of the molecular mechanisms behindtissue remodeling in both normal and pathological reproductivefunction.

The observation that BMP-7 induces apoptosis in a reproductive tissue implies that BMP-7 may be involved in tissues remodelingduring periods of low estrogen in normal reproductive cycles.One report demonstrated that in molting laying hens, which arecharacterized by total regression of the oviduct, a significantincrease in apoptosis is observed (21). However, the estrogenstatus was undetermined, although an earlier study suggested thatestrogen levels are decreased in molting laying hens (69). AlthoughcBMP-7 mRNA levels in the oviduct of a molting hen are unknown,our data suggest that cBMP-7 mRNA levels are induced in the oviductof a molting hen, triggered by declining estrogen concentrations.Similarly, the onset of menstruation in mammalian reproductivecycles is also characterized by a decrease in plasma estrogenlevels followed by extensive endometrial cell death (6). Weprovide the first direct evidence implicating a specific protein,BMP-7, in inducing apoptotic reproductive tissueremodeling.

Previous studies have demonstrated that purified bovine osteogenic protein exists as a BMP-7/BMP-2A heterodimer (58). However,recombinant human BMP-7 existing as a homodimer induces similarlevels of osteogenic activity (59), suggesting that both theheterodimer and homodimer forms are functional in vivo. Anotherreport demonstrated that the heterodimeric form exhibits greateractivity than the homodimeric form (18). Thus, the biologicallyrelevant signaling forms remain controversial. However, sincethe BMP-7 used in this report (Fig. 8) exists as a homodimer,our data suggest that the homodimeric form of BMP-7 is sufficientto induce apoptosis of the oviduct. Whether a heterodimeric formalso exists in chickens must await the cloning of other potentialpartners. For the same reason, these studies also do not addressthe issue of whether other BMP family members elicit apoptosisin theoviduct.

In conclusion, our data indicate that BMP-7 is a molecular mediator of apoptosis, linking the processes of decreased plasmaestrogen levels with the initiation of tissue remodeling. Furthermore,estrogen suppresses these effects by evoking events leading tothe transcriptional repression of the BMP-7 gene. Thus, the reproductivehealth of the oviduct is critically dependent upon the relativelevels of estrogen and BMP-7. Identification of the BMP-7 promoterand sequence elements involved in the response to estrogen willprovide further information regarding the mechanisms by whichestrogen represses BMP-7 gene expression and thus opposesapoptosis.

	ACKNOWLEDGMENTS

We thank Donald F. Jin (Creative BioMolecules) for providing the purified mouse BMP-7 protein and Kathleen Conklin (Universityof Minnesota) for the chick genomiclibrary.

This research was supported by NIH grant R01 DK40082 to M.M.S.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry, Molecular Biology, and Biophysics, University of Minnesota,6-155 Jackson Hall, 321 Church St. SE, Minneapolis, MN 55455.Phone: (612) 624-9637. Fax: (612) 625-2163. E-mail: sande001{at}tc.umn.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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	Articles by Sanders, M. M.

1.	Arends, M. J., R. G. Morris, and A. H. Wyllie. 1990. Apoptosis: the role of the endonuclease. Am. J. Pathol. 136:593-608[Abstract].
2.	Arkell, R., and R. S. P. Beddington. 1997. BMP-7 influences pattern and growth of the developing hindbrain of mouse embryos. Development 124:1-12[Abstract].
3.	Berger, R. R., and M. M. Sanders. 2000. Estrogen modulates HNF-3 $beta$ mRNA levels in the developing oviduct. DNA Cell Biol. 19:103-112[CrossRef][Medline].
4.	Berman, J. R., M. M. McCarthy, and N. Kyprianou. 1998. Effect of estrogen withdrawal on nitric oxide synthase expression and apoptosis in the rat vagina. Urology 51:650-655[CrossRef][Medline].
5.	Brodin, G., P. ten Dijke, K. Funa, C.-H. Heldin, and M. Landstrom. 1999. Increased Smad expression and activation are associated with apoptosis in normal and malignant prostate after castration. Cancer Res. 59:2731-2738[Abstract/Free Full Text].
6.	Carr, B. R. 1992. Disorders of the ovary and female reproductive tract, 8th ed. W. B. Saunders Company, Philadelphia, Pa.
7.	Chamberlain, E. M., and M. M. Sanders. 1999. Identification of the novel player $delta$ EF1 in estrogen transcriptional cascades. Mol. Cell. Biol. 19:3600-3606[Abstract/Free Full Text].
8.	Cohrs, R., B. B. Goswami, and O. K. Sharma. 1988. Occurrence of 2-5A and RNA degradation in the chick oviduct during rapid estrogen withdrawal. Biochemistry 27:3246-3252[CrossRef][Medline].
9.	Cohrs, R. J., B. B. Goswami, and O. K. Sharma. 1988. Down regulation of c-myc, c-fos and erb-B during estrogen induced proliferation of the chick oviduct. Biochem. Biophys. Res. Commun. 150:82-88[CrossRef][Medline].
10.	Detre, S., J. Salter, D. M. Barnes, S. Riddler, M. Hills, S. R. D. Johnston, C. Gillett, R. A'Hern, and M. Dowsett. 1999. Time-related effects of estrogen withdrawal on proliferation and cell death-related events in MCF-7 xenografts. Int. J. Cancer 81:309-313[CrossRef][Medline].
11.	Fitzgerald, M., and T. Schenk. 1981. The sequence 5'-AAUAAA-3' forms part of the recognition sequence for polyadenylation of late SV40 mRNAs. Cell 24:251-260[CrossRef][Medline].
12.	Galien, R., and T. Garcia. 1997. Estrogen receptor impairs interleukin-6 expression by preventing protein binding on the NF- $kappa$ B site. Nucleic Acids Res. 25:2424-2429[Abstract/Free Full Text].
13.	Gavrieli, Y., Y. Sherman, and S. A. Ben-Sasson. 1992. Identification of programmed cell death in situ via specific labeling of nuclear DNA fragmentation. J. Cell Biol. 119:493-501[Abstract/Free Full Text].
14.	Glozak, M. A., and M. B. Rogers. 1996. Specific induction of apoptosis in P19 embryonal carcinoma cells by retinoic acid and BMP2 or BMP4. Dev. Biol. (Orlando) 179:458-470[CrossRef][Medline].
15.	Gold, L. I., and T. V. Parekh. 1999. Loss of growth regulation by transforming growth factor- $beta$ (TGF- $beta$ ) in human cancers: studies on endometrial carcinoma. Semin. Reprod. Endocrinol. 17:73-92[Medline].
16.	Gong, J., F. Traganos, and Z. Darzynkiewicz. 1994. A selective procedure for DNA extraction from apoptotic cells applicable for gel electrophoresis and flow cytometry. Anal. Biochem. 218:314-319[CrossRef][Medline].
17.	Harada, S., T. K. Sampath, J. E. Aubin, and G. A. Rodan. 1997. Osteogenic protein-1 up-regulation of the collagen X promoter activity is mediated by a MEF-2-like sequence and requires an adjacent AP-1 sequence. Mol. Endocrinol. 11:1832-1845[Abstract/Free Full Text].
18.	Hazama, M., A. Aono, N. Ueno, and Y. Fujisawa. 1995. Efficient expression of a heterodimer of bone morphogenetic protein subunits using a baculovirus expression system. Biochem. Biophys. Res. Commun. 209:859-866[CrossRef][Medline].
19.	Helder, M. N., A. Karg, T. J. M. Bervoets, S. Vukicevic, E. H. Burger, R. N. D'Souza, J. H. M. Woltgens, G. Karsenty, and A. L. J. J. Bronckers. 1998. Bone morphogenetic protein-7 (osteogenic protein-1, OP-1) and tooth development. J. Dent. Res. 77:545-554[Abstract/Free Full Text].
20.	Hermoso, M., J. C. Saez, and M. Villalon. 1997. Identification of gap junctions in the oviduct and regulation of connexins during development and by sexual hormones. Eur. J. Cell Biol. 74:1-9[Medline].
21.	Heryanto, B., Y. Yoshimura, T. Tamura, and T. Okamoto. 1997. Involvement of apoptosis and lysosomal hydrolase activity in the oviducal regression during induced molting in chickens: a cytochemical study for end labeling of fragmented DNA and acid phosphatase. Poultry Sci. 76:67-72[Abstract/Free Full Text].
22.	Hogan, B. L. M. 1996. Bone morphogenetic proteins: multifunctional regulators of vertebrate development. Genes Dev. 10:1580-1594[Free Full Text].
23.	Houston, B., B. H. Thorpe, and D. W. Burt. 1994. Molecular cloning and expression of bone morphogenetic protein-7 in the chick epiphyseal growth plate. J. Mol. Endocrinol. 13:289-301[Abstract/Free Full Text].
24.	Huang, D. C., S. Cory, and A. Strasser. 1997. Bcl-2, Bcl-x_L and adenovirus protein E1B19kD are functionally equivalent in their ability to inhibit cell death. Oncogene 14:405-414[CrossRef][Medline].
25.	Huet-Hudson, Y. M., C. Chakraborty, S. K. De, Y. Suzuki, G. K. Andrews, and S. K. Dey. 1990. Estrogen regulates the synthesis of epidermal growth factor in mouse uterine epithelial cells. Mol. Endocrinol. 4:510-523[Abstract/Free Full Text].
26.	Ignar-Trowbridge, D. M., M. Pimentel, C. T. Teng, K. S. Korach, and J. A. McLachlan. 1995. Cross talk between peptide growth factor and estrogen receptor signaling systems. Environ. Health Perspect. 103:35-38.
27.	Jaffe, R. C., E. B. Arias, M. B. O'Day-Bowman, K. M. Donnelly, P. A. Mavrogianis, and H. G. Verhage. 1996. Regional distribution and hormone control of estrogen-dependent oviduct-specific glycoprotein messenger ribonucleic acid in the baboon (Papio anubis). Biol. Reprod. 55:421-426[Abstract].
28.	Jena, N., C. Martin-Seisdedos, P. McCue, and C. M. Croce. 1997. BMP7 null mutation in mice: developmental defects in skeleton, kidney, and eye. Exp. Cell Res. 230:28-37[CrossRef][Medline].
29.	Kepa, J. K., C. I. Neely, B. M. Jacobsen, J. M. Bruder, D. P. McDonnell, K. K. Leslie, and M. E. Wierman. 1994. Estrogen receptor mediated repression of rat gonadotropin releasing hormone (GnRH) promoter activity in hypothalamic cells. Endocr. Rev. 2:1-10[Abstract/Free Full Text].
30.	Keri, R. A., B. Andesen, G. C. Kennedy, D. L. Hamernik, C. M. Clay, A. D. Brace, T. M. Nett, A. C. Notides, and J. H. Nilson. 1991. Estradiol inhibits transcription of the human glycoprotein hormone $alpha$ -subunit despite the absence of a high affinity binding site for estrogen receptor. Mol. Endocrinol. 5:725-733[Abstract/Free Full Text].
31.	Kurebayashi, S., Y. Miyashita, T. Hirose, S. Kasayama, S. Akira, and T. Kishimoto. 1997. Characterization of mechanisms of interleukin-6 repression by estrogen receptor. J. Steroid Biochem. Mol. Biol. 60:11-17[CrossRef][Medline].
32.	Kyprianou, N., and J. T. Isaacs. 1988. Activation of programmed cell death in the rat ventral prostate after castration. Endocrinology 122:552-562[Abstract/Free Full Text].
33.	Lincz, L. F. 1998. Deciphering the apoptotic pathway: all roads lead to death. Immunol. Cell Biol. 76:1-19[CrossRef][Medline].
34.	Llen, R. T., W. J. Hunter, 3rd, and D. K. Agrawal. 1997. Morphological and biochemical characterization and analysis of apoptosis. J. Pharmacol. Toxicol. Methods 37:215-228[CrossRef][Medline].
35.	Loo, D. T., and J. R. Rillema. 1998. Measurement of cell death. Methods Cell Biol. 57:251-264[Medline].
36.	Luo, G., C. Hofmann, A. L. J. J. Bronckers, M. Sohocki, A. Bradley, and G. Karsenty. 1995. BMP-7 in an inducer of nephrogenesis, and is also required for eye development and skeletal patterning. Genes Dev. 9:2808-2820[Abstract/Free Full Text].
37.	Macias, D., Y. Ganan, T. K. Sampath, M. E. Piedra, M. A. Ros, and J. M. Hurle. 1997. Role of BMP2 and OP-1 (BMP-7) in programmed cell death and skeletogenesis during chick limb development. Development 124:1109-1117[Abstract].
38.	Macias-Silva, M., P. A. Hoodless, S. J. Tang, M. Buchwald, and J. L. Wrana. 1998. Specific activation of Smad1 signaling pathways by the BMP7 type I receptor, ALK2. J. Biol. Chem. 273:25628-25636[Abstract/Free Full Text].
39.	Malayer, J. R., and J. Gorski. 1993. An integrated model of estrogen receptor action. Domest. Anim. Endocrinol. 10:159-177[CrossRef][Medline].
40.	Malayer, J. R., and V. M. Woods. 1998. Expression of estrogen receptor and maintenance of hormone-responsive phenotype in bovine fetal uterine cells. Domest. Anim. Endocrinol. 15:141-154[CrossRef][Medline].
41.	McLachlan, J. A., K. G. Nelson, T. Takahashi, N. L. Bossert, R. R. Newbold, and K. S. Korach. 1991. Estrogens and growth factors in the development, growth, and function of the female reproductive tract. Springer-Verlag, New York, N.Y.
42.	Medema, J. P., C. Scaffidi, F. C. Kischkel, A. Shevchenko, M. Mann, P. H. Krammer, and M. E. Peter. 1997. FLICE is activated by association with the CD95 death-inducing signaling complex (DISC). EMBO J. 16:2794-2804[CrossRef][Medline].
43.	Miller, C. D., and W. L. Miller. 1996. Transcriptional repression of the ovine follicle-stimulating hormone- $beta$ gene by 17 $beta$ -estradiol. Endocrinology 137:3437-3446[Abstract].
44.	Murphy, L. J., L. C. Murphy, and H. G. Friesen. 1987. Estrogen induces insulin-like growth factor-I expression in the rat uterus. Mol. Endocrinol. 1:445-450[Abstract/Free Full Text].
45.	Nelson, K. G., T. Takahashi, D. C. Lee, N. C. Luetteke, N. L. Bossert, K. Ross, B. E. Eitzman, and J. A. McLachlan. 1992. Transforming growth factor- $alpha$ is a potential mediator of estrogen action in the mouse uterus. Endocrinology 131:1657-1664[Abstract/Free Full Text].
46.	Newmeyer, D. D., D. M. Farschon, and J. C. Reed. 1994. Cell-free apoptosis in Xenopus egg extracts: inhibition by Bcl-2 and requirement for an organelle fraction enriched in mitochondria. Cell 79:353-364[CrossRef][Medline].
47.	Nordstrom, L. A., D. M. Dean, and M. M. Sanders. 1993. A complex array of double-stranded and single-stranded DNA-binding proteins mediates induction of the ovalbumin gene by steroid hormones. J. Biol. Chem. 268:13193-13202[Abstract/Free Full Text].
48.	Nunez, G., M. A. Benedict, Y. Hu, and N. Inohara. 1998. Caspases: the proteases of the apoptotic pathway. Oncogene 17:3237-3245[CrossRef][Medline].
49.	Ozkaynak, E., D. F. Jin, M. Jelic, S. Vukicevic, and H. Oppermann. 1997. Osteogenic protein-1 mRNA in the uterine endometrium. Biochem. Biophys. Res. Commun. 234:242-246[CrossRef][Medline].
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53.	Ray, P., S. K. Ghosh, D.-H. Zhang, and A. Ray. 1997. Repression of interleukin-6 gene expression by 17 $beta$ -estradiol: inhibition of the DNA-binding activity of the transcription factors NF-IL6 and NF- $kappa$ B by the estrogen receptor. FEBS Lett. 409:79-85[CrossRef][Medline].
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