Developmental Action of Estrogen Receptor-alpha  Feminizes the Growth Hormone-Stat5b Pathway and Expression of Cyp2a4 and Cyp2d9 Genes in Mouse Liver

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Vol. 56, Issue 3, 473-477, September 1999

Developmental Action of Estrogen Receptor- $alpha$ Feminizes the Growth Hormone-Stat5b Pathway and Expression of Cyp2a4 and Cyp2d9 Genes in Mouse Liver

Tatsuya Sueyoshi, Norihiko Yokomori, Kenneth S. Korach, and Masahiko Negishi

Pharmacogenetics (T.S., N.Y., M.N.) and Receptor Biology (K.S.K.) Sections, Laboratory of Reproductive and Developmental Toxicology, National Institute of Environmental Health Sciences, National Institutes of Health, Research Triangle Park, North Carolina

	Summary

Top Summary Introduction Experimental Procedures Results Discussion References

We have studied the roles of estrogen receptor- $alpha$ (ER $alpha$ ) and the Stat5b form of STAT (signal transducers and activators of transcription)in sex-specific expression of Cyp2a4 (steroid 15 $alpha$ -hydroxylase)and Cyp2d9 (steroid 16 $alpha$ -hydroxylase) genes using ER $alpha$ -deficientmice. ER $alpha$ deficiency resulted in the repression of the female-specificCyp2a4 and expression of the male-specific Cyp2d9 genes, respectivelyin females. In ER $alpha$ -deficient males, the Cyp2d9 gene continuedto be expressed. Nuclear localization of Stat5b occurs in bothsexes of ER $alpha$ -deficient mice, although it is normally observedin only wild-type males. Nuclear localization of Stat5b correlateswith the repression of Cyp2a4 and expression of Cyp2d9, respectively.Because Stat5b was not detectable in liver nuclear extracts preparedfrom hypophysectomized ER $alpha$ -deficient females, the regulation byER $alpha$ appeared to be mediated through a pituitary hormone (i.e.,growth hormone). Thus, ER $alpha$ appears to play a key role in the mechanismthat inhibits nuclear localization of Stat5b in female mice, leadingto feminization of a ER $alpha$ -GH-Stat5b pathway and Cyp expression.Defaulting to this ER $alpha$ -dependent mechanism results in localizationof Stat5b to nuclei, which masculinizes the expression of Cypgenes in malemice.

	Introduction

Top Summary Introduction Experimental Procedures Results Discussion References

Hepatic metabolism of steroids and xenochemicals is sexually dimorphic in rodents and other animals (Negishi et al., 1993).Sex-specific metabolism is catalyzed by cytochrome P-450s (CYPs)that are expressed either in male or female animals. Certain metabolismby sex-specific CYPs may lead to sex-dependent susceptibilityfor chemical toxicity and carcinogenicity (Waxman and Chang, 1995aand references therein). Various molecular and/or cellular mechanismsthat may regulate transcription of sex-specific CYP genes havebeen proposed: DNA methylation (Yokomori et al., 1995), hepatocytenuclear factor 6 (Lahuna et al., 1997) and the Stat5b form ofSTAT (signal transducers and activators of transcription) (Subramanianet al., 1995; Udy et al., 1997; Teglund et al., 1998). However,defining the regulatory mechanism of sex-specific CYP expressionremains to be a major interest in continuousinvestigations.

Hormonally, growth hormone (GH) is known to play a central role in regulating sex-specific CYP genes. Gustafsson and Stenberg(1976) first suggested the existence of a pituitary factor thatfeminizes steroid metabolism by rat liver microsomes and calledit "a feminization factor". Later, this pituitary factor was foundto be GH (Kramer and Colby, 1976). In rats, pulsatile GH secretion(in males) is required for activation of the male-specific CYP2C11gene, whereas continuous GH secretion (in females) is essentialfor activating the female-specific CYP2C12 gene (Mode et al.,1981). CYP2A4 and CYP2D9 are the well-characterized sex-specificmouse steroid hydroxylases; the former is the female-specificsteroid 15 $alpha$ -hydroxylase, whereas the latter is the male-specificsteroid 16 $alpha$ -hydroxylase (Harada and Negishi, 1984a,b, 1988). UsingGH-deficient Little mice, we previously showed that GH activatesand represses the male-specific Cyp2d9 and female-specific Cyp2a4gene expression, respectively, dictating the male phenotype ofthe Cyp genes (Noshiro and Negishi, 1986; Aida and Negishi, 1993).On the other hand, the female phenotype (i.e., expression andrepression of the Cyp2a4 and Cyp2d9 genes, respectively) is notregulated by GH (Noshiro and Negishi, 1986). In mice, the sex-specificexpression is hormonally regulated by GH in males, whereas itis constitutive in females. GH, thus, is permissive for female-specificCyp expression in mice. Recently, the cellular mechanism mediatingthe GH-regulated sex-specific Cyp expression has begun to unfold(Udy et al., 1997; Teglund et al., 1998).

STAT represents a group of cellular proteins that can be activated by extracellular peptide signals including GH (Darnell,1997). In response to GH, for example, tyrosine protein kinasescalled Janus kinases (JAKs) phosphorylate Stat proteins that undergonuclear translocation to activate target genes. Waxman and hisassociates demonstrated that pulsatile GH secretion (i.e., malepattern) elicits a Stat5b nuclear translocation, suggesting Stat5bas a direct transcription factor regulating the sex-specific CYP2C11and CYP2C12 genes in rats (Waxman et al., 1995b; Gebert et al.,1997). Stat5b-deficient mice have recently provided unequivocalevidence that Stat5b regulates the sex-specific Cyp2a4 and Cyp2d9genes in male mice, whereas the deficiency does not affect theseCyp genes in female mice (Udy et al., 1997; Teglund et al., 1998).In conjunction with our previous findings (Noshiro and Negishi,1986), a GH-Stat5b pathway may be a regulatory mechanism thatmasculinizes transcription of the Cyp genes in murineliver.

Neonatal action of androgen is thought to regulate sex-specific expression of CYP genes in adult rats (Waxman and Chang, 1995aand references therein). Neonatal castration alters the sex-specificexpression of Cyp genes in mice (Wong et al., 1987). To understandthe developmental role of estrogen and/or estrogen receptor inthe GH-Stat5b regulation of sex-specific Cyp genes, we have nowexamined expression of Cyp2a4 and Cyp2d9 genes and nuclear localizationof Stat5b in estrogen receptor- $alpha$ (ER $alpha$ )-deficient mice. Disruptionof the ER $alpha$ gene has dramatically altered sex-specific Cyp expressionand Stat5b nuclear localization. These findings implicate a developmentalrole of ER $alpha$ in feminizing Cyp expression in mouse liver via aGH-Stat5b-CYPpathway.

	Experimental Procedures

Top Summary Introduction Experimental Procedures Results Discussion References

Animals. ER $alpha$ -deficient homozygous ERKO mice were produced through gene targeting as previously reported (Lubahn et al., 1993). Hypophysectomyof both male and female mice and ovariectomy were performed bythe Comparative Medicine Branch at the National Institute of EnvironmentalHealth Sciences according to an approved National Institute ofEnvironmental Health Sciences animal study protocol. Mice werehoused following surgery for at least 2 weeks before removal ofliver tissues or estradiol treatment. Estradiol was administratedi.p. in saline at a dose of 25 µg/kg b.wt./day for 7 consecutivedays.

Reverse Transcription-Polymerase Chain Reaction (RT-PCR). Liver RNA was prepared using Trizol reagent (Life Technologies, Gaithersburg, MD). RT was performed with 2 µg of RNA and 50ng of random hexamer using the Superscript Preamplification System(Life Technologies). cDNAs were then purified using QIAquick spincolumns (Qiagen Inc., Chatsworth, CA) and eluted with 40 µl H₂O.Two micoliters of cDNA solution was used as template for a 50-µlPCR reaction that contained: 1× PCR reaction buffer (BoehringerMannheim, Indianapolis, IN), 0.4 U Taq polymerase and Taq antibody(Clontech Inc., Palo Alto, CA), 0.1 µg each of forward and reverseprimers, and 200 µM dNTP. Thermal cyclizations were performedat 94°C for 30 s, 55°C for 30 s, and 72°C for 40 s with the GeneAmp System 9600 (Perkin Elmer, Norwalk, CT). RT-PCR amplificationsfor CYP2A4, CYP2D9, and Stat5 were 28, 28, and 33 cycles, respectively.These amplification reactions were shown to be within linear range.Primers used were as follows: CYP2A4 (Lindberg et al., 1989),5'-CTACCTTCGACTGGCTTTTC-3' and 5'-GCATTCGGATGAGGAAGGAG-3'; CYP2D9(Wong et al., 1989), 5'-CTTTGGGGACATTGTTCCAG-3' and 5'-AAGAATACCATAGACTCCAG-3';and Stat5 (Liu et al., 1995), 5'-CAGGTGAAGGCGACCATCAT-3', and5'-TGCTGTTGTAGTCCTCGAGG-3'. Amplified cDNAs for CYP2A4 and Stat5were purified with QIAquick spin columns and subsequently digestedwith HindIII and NcoI, respectively. Following digestion, CYPs2A4 and 2A5 or Stat5a and Stat5b DNA fragments were separatedon an agarose gel. Fragments derived from CYP2A4 were 503 bp;from CYP2A5 were 299 bp and 204 bp; from Stat5a were 310 bp and240 bp; and from Stat5b were 550 bp. Fragment size of the amplifiedCYP2D9 DNA was 347bp.

Western Blotting of Nuclear Stat5b. Nuclear extracts were prepared from mouse livers as previously reported (Sueyoshi et al., 1995). Thirty micograms of nuclearextract was incubated with 1 µg of anti-Stat5b (SC-835; SantaCruz Biotechnology, Santa Cruz, CA) for 2 h at 4°C. The antibody-antigencomplex was precipitated using protein A Sepharose (Pharmacia,Piscataway, NJ) by incubation for 1 h at 4°C. The complex-boundSepharose was washed four times with 50 mM Tris-HCl, pH 8.0, 150mM NaCl, 1.0% Nonidet P-40, 0.5% sodium deoxycholate, 0.1% SDS,100 µM sodium vanadate, and 1 µg/ml leupeptin. One third of theprecipitated protein was applied on a 8% SDS-polyacrylamide gel,transferred to a polyvinylidene difluoride membrane and visualizedwith anti-Stat5b antibody and enhanced chemiluminescence Westernblotting detection reagents (Amersham, Arlington Heights, IL).For Western blots of nuclear extracts for Stat5b or retinoid Xreceptor $alpha$ (RXR $alpha$ ), 10 µg of liver nuclear extracts were separatedon a 8% SDS-polyacrylamide gel, transferred and detected usinganti-Stat5b or anti-RXR $alpha$ antibody (SC-553; Santa CruzBiotechnology).

	Results

Top Summary Introduction Experimental Procedures Results Discussion References

Expression of Sex-Specific CYPs in ER $alpha$ -Deficient Mice. As expected from our previous work (Squires and Negishi, 1988), CYP2A4 mRNA was expressed only in wild-type females (Fig.1A). This female-specific mRNA was completely repressed in ER $alpha$ -deficientfemales, whereas mRNA levels varied significantly in ER $alpha$ -deficientmales, ranging from levels nearly as high as those observed inwild-type females to undetectable (Fig. 1A). The other subfamily-memberCYP2A5 mRNA (Squires and Negishi, 1988; Lindberg et al., 1989)was measured simultaneously using a specific digestion method(Negishi et al., 1991). CYP2A5 mRNA was consistently expressedin all male and female mice examined (Fig. 1A), thereby indicatingthat ER $alpha$ does not regulate non-sex-specific expression of theCyp2a5 gene. These results indicate that the presence of the functionalER $alpha$ gene is an essential factor required for expression of theCyp2a4 gene in female mice. The regulatory mechanism that repressesthis gene in males however, appears to be more complex, and afactor other than ER $alpha$ may be involved.

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Fig. 1. Hepatic levels of the sex-specific CYP mRNAs in ER $alpha$ -deficient mice. Amplified cDNAs for CYP2A4 (A) and CYP2D9 (B) from liver RNAs (lanes 1-5) of individual wild-type (+/+) and ER $alpha$ -deficient ( $-$ / $-$ ) mice were separated on a 1.5% agarose gel. DNA bands were visualized by ethidium bromide in the gel as well as in the electrode buffer. Wild-type females were ovariectomized and treated with estradiol as described in Experimental Procedures, and liver RNAs prepared from pools of the ovariectomized females (Ovex) and ovariectomized/estradiol-treated (Ovex + E₂) were subjected to RT-PCR.

Consistent with our previous findings (Wong et al., 1989

), male-specific CYP2D9 mRNA was expressed at high levels only inwild-type males (Fig. 1B). In contrast, both males as well asfemales of ER $alpha$ -deficient mice showed high expression of CYP2D9mRNA (Fig. 1B). CYP2D9, thus, becomes sexually nonspecific inER $alpha$ -deficient mice, indicating that the presence of a functionalER $alpha$ gene is an essential factor required for repression of theCyp2d9 gene in female mice. ER $alpha$ , on the other hand, does not seemto play a role in expression of the Cyp2d9 gene in malemice.

Neither ovariectomy nor ovariectomy combined with estrogen treatment of wild-type females affected expression of Cyp2a4 gene(Fig. 1A, last two lanes). Ovariectomy further decreased CYP2D9mRNA, whereas estrogen treatment slightly increased CYP2D9 mRNAto the levels as observed in wild-type females (Fig. 1B, lasttwo lanes). ER $alpha$ does not regulate expression of Cyp2a4 gene inadult females, whereas it may play only a minor role in repressingCyp2d9 gene. Thus, the role of ER $alpha$ in regulation of the expressionof the sex-specific Cyp genes appears to bedevelopmental.

Nuclear Localization of Stat5b in ER $alpha$ -Deficient Mice. First, the liver nuclear extracts from two animals from each experimental group were separated on a SDS-polyacrylamide gel,transferred, and immunostained using anti-Stat5b antibody (Fig.2). Nuclear Stat5b was not detectable in nuclear extracts fromboth wild-type female mice, whereas it was present in one of twoindividuals of wild-type male mice and in both males and femalesof ER $alpha$ -deficient mice. For further investigation, then we precipitatedStat5b using anti-Stat5b antibody from various liver nuclear extractsand subjected these immunoprecipitates to Western blot analysis(Fig. 3A). Again, Stat5b was present in the extracts from wild-typemales but not from wild-type females, suggesting that nuclearlocalization of Stat5b occurred in only wild-type male livers.In contrast, Stat5b localized to liver nuclei in both males andfemales of ER $alpha$ -deficient mice (Fig. 3A). Intriguingly, of thefive wild-type males examined, only three males showed nuclearlocalization of Stat5b and only two of the five ER $alpha$ -deficientmales and three of ER $alpha$ -deficient females, respectively. Individualdifferences in nuclear Stat5b levels implied that nuclear localizationof Stat5b is episodic in its nature. In contrast, RXR $alpha$ was alwayslocalized in nuclei and was neither sex-specific nor affectedby disruption of the ER $alpha$ gene (Fig. 3B). Stat5b mRNA was expressedin all mice and remained at the same levels regardless of sexdifference and ER $alpha$ deficiency (Fig. 3C). Thus, ER $alpha$ appears toimprint the mechanism that prevents nuclear localization of Stat5bin female mice.

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Fig. 2. Western blot for Stat5b in liver nuclear extracts. Hepatic nuclear extracts were prepared from individual wild-type (+/+) and ER $alpha$ -deficient ( $-$ / $-$ ) mice. Nuclear extracts were separated and Western blots performed as described in Experimental Procedures.

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Fig. 3. Expression and localization of Stat5b in ER $alpha$ -deficient mice. Liver nuclear extracts were prepared from the individual mice that was used to isolate total RNA in Fig. 1. A, nuclear Stat5b was measured using Western blot analysis: Stat5b was immunoprecipitated, transferred to a polyvinylidene difluoride membrane, and stained with anti-Stat5. Molecular size makers (Broad range prestained marker; New England Biolabs, Beverly, MA) are indicated by arrows with molecular weights. B, Western blot analysis of RXR $alpha$ . Nuclear extracts from individual mice used in Fig. 1 were separated on a SDS polyacrylamide gel, transferred, and immunostained using anti-RXR $alpha$ antibody. C, RT-PCR of Stat5a and Stat5b mRNAs was performed as described in Experimental Procedures, and amplified products were analyzed by electrophoresis on a 1.5% agarose gel.

Effect of Hypophysectomy on CYPs and Stat5b in ER $alpha$ -Deficient Females. To further examine the role of ER $alpha$ in the nuclear localization of Stat5b, we measured Stat5b in liver nuclear extracts fromhypophysectomized ER $alpha$ -deficient females. Consistent with the findingwith wild-type males and ER $alpha$ -deficient females (Fig. 3A), nuclearStat5b was readily detected from three of four sham-operated ER $alpha$ -deficientfemales (Fig. 4A). Hypophysectomy of ER $alpha$ -deficient females decreasednuclear Stat5b to practically undetectable levels (Fig. 4A), whichwas reminiscent of nuclear Stat5b in wild-type female mice (Fig.3A). Episodic nuclear localization of Stat5b appeared to be underpituitary control and moreover, correlated with pulsatile (male)GH secretion pattern. In accordance with the decreased Stat5bin nuclei, CYP2A4 mRNA was induced in hypophysectomized femalesand CYP2D9 mRNA was reduced (Fig. 4B). The period for episodicnuclear localization of Stat5b must be much shorter than the half-lifeof CYP2D9 mRNA. Thus, ER $alpha$ appears to regulate Stat5b nuclear localizationthrough the pituitary gland, presumably by the secretion patternof GH.

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Fig. 4. Hepatic nuclear Stat5b and sex-specific CYP mRNAs in ER $alpha$ -deficient hypophysectomized females. A, hepatic nuclear extracts were prepared from individual hypophysectomized female mice and subjected to Western analysis as described in Experimental Procedures. B, CYP mRNAs were amplified and analyzed using the methods as described in Experimental Procedures and also in the legend of Fig. 1. RNAs were pooled from at least three female mice for each experiment. Symbols used are same as those in Fig. 1, except that Hypox denotes hypophysectomy.

	Discussion

Top Summary Introduction Experimental Procedures Results Discussion References

A regulatory role of ER $alpha$ in sex-specific Cyp expression is proposed in Fig. 5. The sex-specific Cyp2a4 and Cyp2d9 genes areeither constitutively expressed or repressed in female mice becausehypophysectomy does not affect their expressions (Yoshioka etal., 1990). Our present studies with ER $alpha$ -deficient female micehave clearly indicated that this constitutive expression and repressionis developmentally imprinted by an action of ER $alpha$ . To the contrary,GH is an essential factor for masculinizing Cyp expression inmale mice, as suggested by our previous finding that the male-specificCyp2d9 and female-specific Cyp2a4 genes are repressed and expressed,respectively in GH-deficient Little male mice (Noshiro and Negishi,1986; Yoshioka et al., 1990). It is paradoxical to see that GHand ER $alpha$ act as if they were independent and unrelated factors,although both are involved in the regulation of the sex-specificCyp genes. This paradox may be explained by hypothesis that adevelopmental action of ER $alpha$ is to imprint GH secretion patternin female mice, whereas the lack of ER $alpha$ defaults GH to the malesecretion in both ER $alpha$ -deficient males and females. The GH secretionpatterns in ER $alpha$ -deficient mice remains to be established in thefuture.

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Fig. 5. Proposed mechanism for the feminization of the sex-specific CYPs. GH secretion patterns are depicted from MacLeod et al. (1991)

. GH in male mice, via GH receptor (open box with arrow), translocates Stat5b into nuclei. Nuclear Stat5b, then activates transcription of Cyp2d9 gene and represses that of Cyp2a4 genes. Under the female secretion pattern of GH, however, hepatic nuclear translocation of Stat5b does not occur. The absence of nuclear Stat5b in female mice results in the constitutive activation and repression of Cyp2a4 and Cyp2d9 genes, respectively. It should be emphasized that the female pattern of GH secretion is permissive for the female phenotype of Cyp expression in mice, meaning that GH plays no regulatory role in females. ER $alpha$ may imprint the mechanism regulating the GH secretion pattern in female mice, so that Stat5b is not translocated into hepatic nuclei.

A role of GH in the sex-specific CYP expression is to regulate nuclear translocation of Stat5b in liver. Waxman and his associates(Waxman et al., 1995b; Gebert et al., 1997) have previously shownthat nuclear translocation of Stat5b is male-specific in rat liver.The nuclear hepatic Stat5b content of individual male rats variedsignificantly, implying that Stat5 shuttles between the cytoplasmand nucleus. Moreover, the hepatic nuclear Stat5b contents ofindividual male rats correlated positively with plasma GH levels.Our present study reveals that the individual variability in anuclear Stat5b level appears to be pronounced in male mice. Theregular periodicity of the GH pulse is shorter in male mice (2.5h) than male rats (4 h) (Jansson et al., 1985; MacLeod et al.,1991). The shorter periodicity may make the time of nucleocytoplasmicshuttle of Stat5b faster in male mice, reflecting the strong individualdifferences in nuclear Stat5b level. Despite the variable Stat5blevels, the male-specific Cyp2d9 gene is expressed in every individualof wild-type males and ER $alpha$ -deficient males and females examined.This suggests that the half-life of Stat5b in nucleus must bemuch shorter than that of CYP2D9 mRNA in mouse liver. NuclearStat5b represses the female-specific Cyp2a4 gene, whereas it activatesthe male-specific Cyp2d9 gene. Because Stat5b can be translocatedonly under the male secretion pattern of GH, either a physiologicalcondition of the female GH secretion or the pathological conditionof no GH results in no nuclear translocation of Stat5b in liver.The Cyp expression thus becomes the male phenotype in both ER $alpha$ -deficientmale and female mice as well as in wild-typemales.

In general, neonatal imprinting is considered to occur during sexual differentiation (i.e., feminization versus masculinization)of brain function (MacLusky and Naftolin, 1981; Bardine and Catterall,1981), including sexual differentiation of GH secretion patternand sex-specific expression of CYP genes (Gustafsson et al., 1983;Jansson et al., 1985). The majority of these studies were performedin rats, concluding that a neonatal action of androgen is a keyfactor for imprinting. Androgen can be aromatized to estrogen,which imprints masculinization in male rats, and the lack of androgen(i.e., estrogen) results in feminization in female rats. Studiesusing ER $alpha$ -deficient mice have provided some evidence that ER $alpha$ -mediatedestrogen may, infact, act as a masculinization factor for sexualdifferentiation. ER $alpha$ -deficient females exhibit similar dopaminergicneurons to those observed in males, whereas the female-type dopaminergicneurons are largely retained in ER $alpha$ -deficient females (Simerlyet al., 1997). Given the fact that ER $alpha$ feminizes the Cyp expressionin mice, sexual differentiation may be diverse processes thatare centered around ER $alpha$ and/or estrogens. It is increasingly evidentthat any given biological signal can be transduced in positiveas well as negative manners. It may not be so surprising, evenif the apparent regulation of GH-Stat5b-CYP pathway observed inER $alpha$ -deficient mice is contrary to a general imprinting mechanismpreviously established in rats. Is ER $alpha$ -mediated feminization ofthe GH-Stat5b-CYP pathway regulated by estrogen? It is difficultto speculate this at the present time. There may or may not besufficient levels of estrogen to activate ER $alpha$ in neonatal mousebrain. Because steroid receptors including ER $alpha$ can be activatedin the absence of cognate ligands (Cenni and Picard, 1999), evenif there is absolutely no estrogen in brain, ER $alpha$ may be activatedby a ligand-independent mechanism, thereby feminizing the GH-Stat5b-CYPpathway. The regulation mechanism of sex-specific CYP genes israther complex and diverse. The complexity and diversity appearto arise from the fact that ER $alpha$ does not directly regulate theCYP genes. There are multiple regulatory steps leading ER $alpha$ actionto CYP genes. Whether ER $alpha$ also acts a factor that feminizes CYPexpression in other species remains a subject for further investigation.Nevertheless, our present study using ER $alpha$ -deficient mice unequivocallyshows that ER $alpha$ plays a central role in feminizing Cyp expressioninmice.

	Acknowledgments

Our deep appreciation is due to Rick Moore, Kim and Todd Washburn, and Chizuko Sueyoshi for excellent technical assistance.We also thank Dr. Joyce Goldstein for critical reading of thismanuscript.

	Footnotes

Received February 2, 1999; Accepted May 13, 1999

Send reprint requests to: Dr. Masahiko Negishi, Pharmacogenetics Section, Laboratory of Reproductive and Developmental Toxicology, National Institute of Environmental Health Sciences, National Institutes of Health, P.O. Box 12233, Research Triangle Park, NC 27709. E-mail: negishi{at}niehs.nih.gov

	Abbreviations

CYP, cytochrome P-450; ER $alpha$ , estrogen receptor- $alpha$ ; STATs, signal transducers and activators of transcription; Stat5a and Stat5b, 5a and 5b forms of STATs; GH, growth hormone; PCR, polymerase chain reaction; RT, reverse transcription.

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				M. Skavdahl, C. Steenbergen, J. Clark, P. Myers, T. Demianenko, L. Mao, H. A. Rockman, K. S. Korach, and E. Murphy Estrogen receptor-{beta} mediates male-female differences in the development of pressure overload hypertrophy Am J Physiol Heart Circ Physiol, February 1, 2005; 288(2): H469 - H476. [Abstract] [Full Text] [PDF]

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				C. A. Wiwi, M. Gupte, and D. J. Waxman Sexually Dimorphic P450 Gene Expression in Liver-Specific Hepatocyte Nuclear Factor 4{alpha}-Deficient Mice Mol. Endocrinol., August 1, 2004; 18(8): 1975 - 1987. [Abstract] [Full Text] [PDF]

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				E. R. Levin Genome and Hormones: Gender Differences in Physiology: Invited Review: Cell localization, physiology, and nongenomic actions of estrogen receptors J Appl Physiol, October 1, 2001; 91(4): 1860 - 1867. [Abstract] [Full Text] [PDF]