The Aromatase Knock-Out Mouse Provides New Evidence That Estradiol Is Required during Development in the Female for the Expression of Sociosexual Behaviors in Adulthood

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The Journal of Neuroscience, October 15, 2002, 22(20):9104-9112

The Aromatase Knock-Out Mouse Provides New Evidence That Estradiol Is Required during Development in the Female for the Expression of Sociosexual Behaviors in Adulthood
Julie Bakker¹, Shin-Ichiro Honda², Nobuhiro Harada², and Jacques Balthazart¹
¹ Center for Cellular and Molecular Neurobiology, Research Group in Behavioral Neuroendocrinology, University of Liège, B-4020 Liège, Belgium, and ² Division of Molecular Genetics, Fujita Health University, Toyoake, 470-11 Aichi, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We used estrogen-deficient aromatase knock-out (ArKO) mice to determine whether estrogens contribute to the development ofthe brain and behavior in females. Female mice of three differentgenotypes [i.e., wild type (WT), heterozygous (HET), and homozygous(ArKO)] were ovariectomized in adulthood and subsequently testedfor odor preferences (choice: intact male vs estrous female) ina Y-maze. When treated with testosterone, ArKO females spent significantlyless time sniffing odors (both volatile and nonvolatile) fromeither male or female stimuli compared with WT and HET females.When given direct access to anesthetized stimulus animals or whengiven a choice between odor and visual cues from both stimulusanimals, ArKO females continued to spend less time investigatingthe stimuli compared with WT and HET females. These defects inolfactory investigation of ArKO females were partially correctedwith estradiol treatment in adulthood. Estradiol-treated ArKOfemales no longer differed from WT and HET females in the timespent investigating either nonvolatile odors or the anogenitalregion of anesthetized animals. However, ArKO females still investigatedvolatile odors and/or visual cues less than WT and HET females.Sexual receptivity was severely impaired in ArKO females aftertreatments with estradiol and progesterone that successfully inducedreceptivity in WT and HET females. Furthermore, ArKO females showeddiminished levels of male sexual behaviors, whereas WT and HETfemales readily mounted an estrous female. Together, these findingsdemonstrate that estrogen is required for normal female development.The concept that the female brain develops in the absence of anyhormonal stimulation should therefore bereconsidered.

Key words: aromatase; olfaction; sex; behavior; preference; development

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The early anatomical and physiological work of Jost (for review, see Jost, 1985) showed that fetal gonadectomy of male andfemale rabbit fetuses results in both sexes developing femaleinternal and external genitalia. It was concluded that the femalephenotype develops in the absence of any hormonal secretion fromthe ovaries, whereas the male phenotype results from the secretionof testosterone and antimüllerian hormone, both secreted by thefetal testes. Additional experiments (Phoenix et al., 1959) demonstratedthat the sexual differentiation of the brain follows a similarpattern; i.e., testosterone secreted by the testes causes masculinization(enhancement of male-typical sexual responses) and defeminization(suppression of female-typical sexual responses) of the neuralsubstrates mediating sexual behavior. For instance, female guineapigs treated with testosterone propionate in utero showed elevatedlevels of male sexual responses (i.e., mounting behavior) andreduced levels of female sexual responses (i.e., lordosis) inadulthood (Phoenix et al., 1959). The absence of testosteroneproduced opposite effects (i.e., demasculinization and feminizationof the brain): females and neonatally castrated male rats (Federand Whalen, 1965; Grady et al., 1965) show diminished levels ofmale sexual behaviors after adult testosterone treatment and highlevels of lordosis behavior after adult treatment with estradioland progesterone. Thus, the female brain seems to develop in theabsence of any hormonal secretion. In contrast to the sexual differentiationof the genitalia, many of the masculinizing and defeminizing effectsof perinatal testosterone on the brain are mediated by estradiolderived from local aromatization of testosterone (Naftolin etal., 1975; McEwen et al., 1977; Baum, 1979; MacLusky and Naftolin,1981).

The concept of female differentiation proceeding in the absence of any hormonal secretion, however, is challenged by severalobservations. First, Toran-Allerand (1976) demonstrated that hypothalamicneurons of newborn mice of both sexes develop neurite processesin vitro only when estradiol is added to the culture medium. Second,Döhler et al. (1984) found that postnatal treatment of femalerats with tamoxifen, an estrogen receptor antagonist, defeminizedboth gonadotropin regulation and female sexual behavior, whereasconcurrent administration of low doses of estradiol preventedthese effects of tamoxifen. Finally, Mack et al. (1993) foundthat estrogen action is required in females for a normal, female-likedevelopment of the corpus callosum, a cortical structure thatis larger in male than in female rats. Ovariectomy of female ratsas late as day 16 after birth increased the cross-sectional areaof the adult corpus callosum (i.e., made it more male-like), whereastreatment with estradiol in a low dose starting at day 25 afterbirth inhibited this effect (Fitch and Denenberg, 1998). Together,these findings suggest that estrogens are required during developmentto feminize the brain. In the present study, we tested this conceptby determining whether sociosexual behaviors are disrupted infemale mice that have been depleted of estrogens during the criticalperiod of development by targeted disruption of the aromatase(Cyp19) gene [aromatase knock-out (ArKO) mice] (Honda et al.,1998).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects and general procedures
ArKO mice were generated by targeted disruption of exons 1 and 2 of the Cyp19 gene (Honda et al., 1998). Heterozygous (HET)males and females of the C57BL/6 strain were bred to generatewild-type (WT), HET, and homozygous-null (ArKO) offspring. Micewere genotyped by PCR analysis of tail DNA (Bakker et al., 2002).All breeding and genotyping were performed at the School of VeterinaryMedicine of the University of Liège. During behavioral testing,all experimental mice were housed alone under reversed light/darkcycle (12 light/dark, lights off at 9:00 A.M.). Food and waterwere always available ad libitum. All experiments were conductedin accordance with the guidelines set forth by the National Institutesof Health Guiding Principles for the Care and Use of ResearchAnimals and were approved by the Ethical Committee for AnimalUse of the University of Liège.
At the age of ~20 weeks, 24 females (eight of each genotype: WT, HET, and ArKO) were ovariectomized under general anesthesiawith a mixture of ketamine (173 µg/gm per mouse) and xylazine(6 µg/gm per mouse). At the time of ovariectomy, a 5-mm-long Silasticcapsule (inner diameter, 1.57 mm; outer diameter, 2.41 mm) filledwith crystalline testosterone was implanted subcutaneously inthe neck. Stimulus animals (males and females) were derived froma different breeding colony of the Naval Medical Research Institutestrain at the University of Liège. Stimulus males were left gonadallyintact. All stimulus females were ovariectomized and injectedsubcutaneously 48 and 24 hr before testing with estradiol benzoate(1.25 mg/kg mouse; dissolved in sesame oil) followed by progesterone(1 mg per mouse; dissolved in sesame oil) 3 hr beforetesting.
All behavioral tests were conducted between 1:00 and 6:00 P.M. during the dark phase of the light/dark cycle. Furthermore,no behavioral testing was conducted during the 24 hr after thesubjects' cages werecleaned.

Odor-preference tests
Description Y-maze. All preference tests were conducted in an enclosed, Plexiglas Y-maze (adapted for mice according to Petrulisand Johnston, 1999). The Y-maze consisted of the stem of the Y(55 cm long) and two arms (65 cm long) that diverged at a 60°angle from the stem. All parts of the maze were 9 cm high and9 cm wide. A removable perforated Plexiglas door at the distalend of the each arm separated the goal box from the rest of themaze. We used either an opaque (to prevent visual cues) or a clear(to allow visual cues) Plexiglas door. A perforated Plexiglasdoor was placed at the other side of the goal box. The start boxwith a removable perforated Plexiglas door was located at thebase of the stem. An electric fan was placed behind the startbox, from which it was separated by a wire screen. The perforateddoors and the fan made it possible to pull air over odor stimuliplaced in the distal goal boxes through the entire maze into thestartbox.
Test procedure. All subjects were housed alone starting at the time of ovariectomy. Their cages were placed at random in aclimate-controlled (light, temperature, and ventilation) animalhousing unit (Iffa-Credo, Arbresle, France). Stimulus males andfemales were always housed in a different animal housing unit,so subjects were never exposed to any male- or estrous female-derivedodors except when they were tested. For each test, cages weretaken randomly out of the housing unit to avoid the possibilitythat the same animals would always be tested first or last. Atthe beginning of each test, the subject was placed in the startbox with the door closed to adapt for 1 min. The test began whenthe door was removed and the subject could move around freelyin the Y-maze. All female subjects were tested three times (5min each) in the Y-maze without any stimulus animals in the goalboxes to adapt to the testing apparatus and to determine whetherthey would develop any sidepreferences.

Experimental procedures

Experiment 1: contribution of the aromatase gene to the development of odor preferences
Approximately 5 weeks after ovariectomy and implantation of a Silastic capsule containing testosterone, female mice of eachgenotype (WT, HET, and ArKO) were subjected to a series of odor-preferencetests using different stimuli (see description below). Subsequently,after 4 weeks of testing, the testosterone capsule was replacedby a 5-mm-long SILASTIC capsule (inner diameter, 1.57 mm; outerdiameter, 2.41 mm) containing crystalline 17 $beta$ -estradiol (diluted1:1 with cholesterol) under ketamine/xylazine anesthesia. Thecapsules were approximately the same size as those used by Wersingeret al. (1999), which resulted in levels of estradiol slightlylower (80 pg/ml) than the levels observed during estrus (150 pg/ml).The inner and outer diameters of our capsules, however, were slightlylarger than those used by Wersinger et al. (inner diameter, 1.02mm; outer diameter, 2.16 mm), resulting in a decreased thickness(outside minus inside diameter = 0.78 mm here vs 1.14 mm) andincreased surface ( $pi$ × outside diameter × length = 37.85 mm² here vs 33.92 mm²). Because the amount of steroid released from a Silastic implantis directly proportional to the surface of the capsule and inverselyrelated to its thickness (Smith et al., 1977), it can be roughlyestimated that our capsules produced circulating levels of estradiolof ~130 pg/ml [i.e., 1.63 times higher, (1.14/0.78) × (37.85/33.92),than in Wersinger et al. (1999)]. These levels are in the rangeof values observed during estrus in mice (Wersinger et al., 1999).After 3 weeks of estradiol treatment, behavioral testing was resumed,and female mice were subjected to the same series of odor-preferencetests (which lasted ~3 weeks) in the same order as had been usedwhile they were on testosterone. To facilitate comparisons, thedata obtained while subjects were treated with testosterone arepresented in Results side by side with those obtained while thesubjects were treated withestradiol.
Volatile olfactory cues. First, female mice were subjected to two consecutive tests (5 min each) in which they were offereda choice between volatile odors of an estrous female versus thoseof a gonad-intact male. The Plexiglas doors separating the goalboxes from the rest of the maze were opaque to prevent the subjectsfrom seeing the stimulus animals. In addition, stimulus animalswere anesthetized with ketamine/xylazine to prevent them fromproducing sounds that could be detected by the test animal. Thelevel of anesthesia was checked and adjusted between each trial.Stimulus animals were regularly placed on a heating pad to preventhypothermia. The position of the stimulus animals was switchedbetween tests. The time the subject spent sniffing the male andfemale odors (poking its nose through the holes of the door andactively sniffing the door of the goal box) was recorded witha stopwatch. In addition, the number of entries into each armwas scored. The maze was cleaned with 70% alcohol betweentrials.
Soiled bedding. Second, female mice were subjected to one 5 min test in which they were given a choice between soiled beddingfrom gonad-intact males versus soiled bedding from estrous females.Stimulus females (n = 3) injected twice with estradiol benzoatesubcutaneously (48 and 24 hr before bedding was collected) andsubsequently with progesterone were placed in a cage containingfresh sawdust. Bedding was collected 10 hr after the progesteroneinjection. Likewise, gonad-intact males (n = 3) were placed ina cage containing fresh sawdust. Bedding was collected 10 hr later.All bedding was stored in plastic freezer bags at $-$ 70°C untilused in the experiment. Bowls containing soiled bedding were placedat the end of each arm of the Y-maze. The doors separating thegoal boxes from the rest of the maze were removed. The time themice spent sniffing the bedding was recorded for each subject.The maze was cleaned with 70% alcohol betweentrials.
Direct access to stimulus animals. Third, female mice were given one 5 min test in which they had direct access to a gonad-intactmale and an estrous female. Stimulus animals were anesthetizedto eliminate any interference of the behavioral interaction betweenthe subjects and the stimulus animals. The doors separating thegoal boxes from the rest of the maze were removed. The time eachsubject spent sniffing the stimulus animal, including its anogenitalregion and flank, was recorded with a stopwatch. The maze wascleaned with 70% alcohol between each trial. As in Experiment1, the level of anesthesia was checked regularly and adjustedbetween each trial if necessary. Furthermore, stimulus animalswere regularly placed on a heating pad to preventhypothermia.
Odor and visual cues. Finally, female subjects were given one 5 min test in which they could choose between an awake gonad-intactmale and an awake estrous female. Stimulus animals were placedbehind a clear Plexiglas door. Subjects could thus see, smell,and hear but not physically interact with the stimulus animals.The time the subject spent sniffing the male and female odors(poking its nose through the holes of the door and actively sniffingthe door of the goal box) was recorded with a stopwatch. The mazewas cleaned with 70% alcohol between eachtrial.

Experiment 2: contribution of the aromatase gene to the development of lordosis behavior
At the end of preference testing, female subjects were tested once a week during 5 weeks for lordosis behavior with a sexuallyactive male. Females were ~35 weeks of age and had received estradioltreatment for >6 weeks. All female subjects continued to receiveestradiol treatment and in addition were injected subcutaneouslywith 1 mg of progesterone 3 hr before each lordosis test. Alllordosis tests were conducted in a Plexiglas aquarium (35 cm long× 25 cm high × 19 cm wide) whose floor was covered with freshsawdust. At the beginning of each test, a sexually active malewas placed alone in the aquarium and allowed to adapt for 15 min.Subsequently, an experimental female was placed in the aquarium,and the lordosis responses of the female to the mounts of thestimulus male were recorded. The receptivity of each female tothe males' mounts was also scored on an ordinal 4 point scaleas follows: 1, female ran away and/or responded aggressively;2, female did not run away but rejected the mount; 3, female acceptedthe mount but did not respond by showing lordosis; and 4, femaleresponded by showing lordosis. The test lasted until the femalehad received 10 mounts or 10 min hadelapsed.

Experiment 3: olfaction test
Two "hidden cookie" tests were conducted to check for gross malfunction of the main olfactory system in female ArKO mice.All female mice were food-deprived overnight (~24 hr). A smallpiece of a chocolate chip cookie was buried (~1 cm deep) at arandom location in a clean Plexiglas aquarium (35 cm long × 25cm high × 19 cm wide) containing fresh sawdust. The time it tookeach mouse to find the cookie was recorded. The test lasted untilthe mouse had located the cookie or 15 min if the cookie was notfound. Mice were tested twice 4 d apart. At the time of thesetests, which were performed 1 week after completion of the lordosistests, mice still had their Silastic capsules containingestradiol.

Experiment 4: open-field test
All female subjects were tested for general locomotor activity in an open field (clean Plexiglas cage; 51 cm long × 18 cmhigh × 30 cm wide). The cage was divided into nine rectangles(17 × 10 cm). At the beginning of the test, the subject was placedin the middle of the cage. The number of crossings (from one rectangleto another) was recorded. We considered the line crossed whenall four legs were over the line. The time spent in each squarewas also recorded. Females were tested once for 5 min. At thetime of this test (1 week after completion of the olfaction tests),mice still had their Silastic capsules containingestradiol.

Experiment 5: contribution of the aromatase gene to the development of male sexual behavior
Previous work on another strain of ArKO mice has indicated that these mice are exposed to increased plasma levels of testosteroneduring adulthood (Fisher et al., 1998). These increased levelsof androgens could result from the interruption of the steroidfeedback on gonadotropin secretion, which is known to be mediatedin part by estrogens, as suggested by the increased levels ofcirculating luteinizing hormone and follicle-stimulating hormonein these mice. Alternatively, the increase in plasma testosteronecould be caused, at least in part, by the accumulation of theandrogenic substrate, which can no longer be transformed intoan estrogen by the ovaries because of the disruption of the aromatasegene. Because the fetal and neonatal ovaries are not (very) active(Weniger, 1993; Weniger et al., 1993), it is unlikely that thisincrease in androgen levels actually takes place before puberty,but no data are available to evaluate this question, and it couldtherefore be speculated that increased levels of androgens contributeto the development of the behavioral phenotype in ArKO mice. Todetermine whether the absence of lordosis behavior in ArKO femalesdid not result from masculinization and defeminization of theirbrains by excessive androgen action during development, a differentset of female ArKO mice was tested for male-typical sexual behaviorwith an estrous female. At the age of ~12 weeks, female mice ofthree different genotypes (10 WT, 7 HET, and 9 ArKO) were ovariectomizedin adulthood under general anesthesia. At the same time, a 5-mm-longSilastic capsule (inner diameter, 1.57 mm; outer diameter, 2.41mm) filled with crystalline testosterone was implanted subcutaneouslyin the neck. After 7 weeks of testosterone treatment, femaleswere tested once for male-typical sexual behavior. To determinewhether the absence of male sexual behavior in ArKO females wasa result of a lack of circulating estradiol, females were testedonce more for male-typical sexual behavior after receiving dailyinjections of estradiol benzoate (5 µg per mouse) for 2 weekswhile remaining on testosterone. All coital behavior tests wereconducted in a Plexiglas aquarium (35 cm long × 25 cm high × 19cm wide) whose floor was covered with fresh sawdust. At the beginningof each test, the female subject was placed alone in the aquariumto adapt for 15 min. Subsequently, an estrous female was introduced,and the number of mounts and intromission-like behaviors displayedby the female subject were scored for 30 min. In addition, latenciesto mounts and intromission-like behaviors were recorded. The femalesubject was never mounted by the stimulus female. Furthermore,ejaculation-like behavior of the female subjects was neverobserved.

Statistical analysis

For experiments 1-4, three WT females that did not survive the second round of anesthesia when the testosterone capsule wasreplaced by one capsule containing estradiol and two ArKO females(one died and one ceased to explore the Y-maze in the course ofbehavioral testing) were excluded from statistical analysis. Alldata were analyzed using repeated-measures ANOVA with variousindependent and repeated factors. First, all data obtained whilesubjects were treated with testosterone were directly comparedwith those obtained while subjects were treated with estradiolin one large multifactor ANOVA. Subsequently, the data were analyzedseparately for each hormone treatment to simplify the presentationof the results. Therefore, in each section of Results, the dataobtained while subjects were treated with testosterone are presentedfirst, followed by those obtained while subjects were treatedwith estradiol, and finally, the two different hormone treatmentsare compared. All male coital data (experiment 5) were analyzedin one ANOVA. When appropriate, all ANOVAs were followed by Tukeyhighly significant difference post hoc comparisons adapted forrepeated-measures ANOVA. Only significant (p < 0.05) effects detectedby the ANOVA are mentioned in detail inResults.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1: contribution of the aromatase gene to the development of odor preferences

Clean Y-maze
No side preferences were detected when subjects were tested without any stimulus animals placed in the goal boxes of the Y-maze.A three-way ANOVA of the time spent in each arm of the maze withgenotypes as the independent factor and tests and side of theY-maze (left vs right) as repeated factors showed a significanteffect only of repeated testing (F_(2,32) = 7.29; p = 0.0025),but neither an effect of genotype (F_(2,16) = 0.96; p = 0.40) noran effect of side of the Y-maze (F_(1,16) = 1.89; p = 0.19) norany significant interactions. Post hoc analysis of the test effectshowed that all subjects spent more time in the arms of the Y-mazein the second than the first test (mean ± SEM for all three genotypes;55.5 ± 3.6 vs 69.2 ± 4.3 sec for test 1 vs test 2, respectively).The number of arm entries did not differ significantly betweengenotypes, although there was a trend toward a decrease in ArKOfemales (mean ± SEM: WT, 4.7 ± 0.4; HET, 4.9 ± 0.3; ArKO, 3.2± 0.2; F_(2,16) = 2.77; p = 0.09).

Volatile olfactory cues
Testosterone treatment. WT females clearly preferred to sniff volatile odors from an estrous female over those from a sexuallyactive male. This preference for female odors was less evidentin HET and ArKO females (Fig. 1A). A three-way ANOVA of the timespent sniffing volatile odors with genotype as the independentfactor and tests and odor stimulus (male vs female) as repeatedfactors revealed a significant effect of genotype (F_(2,16) = 22.70;p = 0.0001), a significant effect of odor stimulus (F_(1,16) =12.99; p = 0.0024), a significant odor stimulus by genotype interaction(F_(2,16) = 6.41; p = 0.009), and a significant test by odor stimulusinteraction (F_(1,16) = 19.80; p = 0.0004). Because we found neithera significant effect of repeated testing (F_(1,16) = 0.73; p =0.41) nor a significant test by genotype interaction (F_(2,16)= 0.05; p = 0.95), data of two preference tests were combined(Fig. 1A,B). Post hoc analysis of the genotype effect showed thatfemale ArKO mice spent less time sniffing volatile odors (eithermale or female) than WT and HET mice (Fig. 1B). Furthermore, posthoc analysis of the odor stimulus by genotype interaction showedthat WT and ArKO females spent significantly more time sniffingfemale odors than male odors, whereas HET females spent equaltime sniffing both odors. Finally, post hoc analysis of the significanttest by odor stimulus interaction showed that all female groupsspent less time sniffing male odors and more time sniffing femaleodors in the second than the first test.

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Figure 1. A, C, Mean amount of time that female WT, HET, and ArKO mice spent investigating volatile olfactory cues when given a choice between intact male odors and estrous female odors in a Y-maze. B, D, Total amount of time spent sniffing volatile odors. A, B, Results when subjects were treated with testosterone. C, D, Results when the same subjects were treated with estradiol. Means with different letters above them are significantly different from each other by post hoc comparisons. Data shown are the mean ± SEM of two successive behavior tests.

Three-way ANOVA on the number of entries into each arm of the Y-maze with genotype as the independent factor and tests andodor stimuli (male vs female) as repeated factors showed a significanteffect only of genotype (F_(2,16) = 8.56; p = 0.003). ArKO femalesmade fewer arm entries than WT and HET females (mean ± SEM: 5.4± 0.3 for ArKO females vs 10.7 ± 1.3 for WT females and 11.6 ±1.2 for HETfemales).
Estradiol treatment. WT females continued to show a preference for sniffing volatile odors from an estrous female. This preferenceto investigate female odors was less pronounced in HET females,whereas ArKO females showed no significant preference (Fig. 1C).Three-way ANOVA of time spent sniffing volatile odors with genotypeas the independent factor and tests and odor stimulus (male vsfemale) as repeated factors showed a significant effect of genotype(F_(2,16) = 20.85; p = 0.0001), a significant effect of odor stimulus(F_(1,16) = 33.46; p = 0.0001), a significant odor stimulus bygenotype interaction (F_(2,16) = 5.64; p = 0.014), a significanttest by stimulus interaction (F_(1,16) = 9.00; p = 0.009), anda significant test by stimulus by genotype interaction (F_(2,16)= 3.81; p = 0.04). Because we found neither an effect of repeatedtesting (F_(1,16) = 0.01; p = 0.91) nor a significant test by genotypeinteraction (F_(2,16) = 0.02; p = 0.98), we combined data for twotests (Fig. 1C,D). Post hoc analysis of the genotype effect showedthat the total time spent sniffing volatile odors (either maleor female) was again reduced in ArKO females compared with WTand HET females (Fig. 1D). Furthermore, post hoc analysis of theodor stimulus by genotype interaction revealed that WT femalesspent more time sniffing female odors compared with HET females,which, in turn, spent more time sniffing female odors comparedwith ArKO females. In addition, WT and HET females spent moretime sniffing male odors compared with ArKO females (Fig. 1C).Finally, post hoc analysis of the test by stimulus and the testby stimulus by genotype interactions revealed that HET females(but not WT and ArKO females) spent more time sniffing male odorsand less time sniffing female odors in the second than the firstpreference test (data notshown).
Three-way ANOVA on the number of arm entries with genotype as the independent factor and tests and odor stimulus as repeatedfactors showed a significant effect of genotype (F_(2,16) = 5.80;p = 0.013), a significant effect of repeated testing (F_(1,16)= 21.82; p = 0.0003), a significant effect of odor stimulus (F_(1,16)= 9.64; p = 0.007), an almost significant stimulus by genotypeinteraction (F_(2,16) = 3.12; p = 0.07), and an almost significanttest by stimulus interaction (F_(2,16) = 4.25; p = 0.06). Again,ArKO females made fewer arm entries than WT and HET females (mean± SEM: 5.6 ± 1.0 for ArKO females vs 12.2 ± 1.3 for WT femalesand 12.2 ± 1.6 for HET females). Furthermore, all female groupsmade fewer arm entries in the second than the first test (no significanttest by genotype interaction: F_(2,16) = 0.21; p = 0.82).
Testosterone versus estradiol treatment. In comparing the effects of hormone treatment on time spent sniffing volatile odors,four-way ANOVA with genotype as the independent factor and hormonetreatment, odor stimulus, and tests as repeated factors showeda significant effect of hormone treatment (F_(1,16) = 5.74; p =0.029). Post hoc analysis of the hormone effect showed that allfemales, but particularly HET females (almost significant hormoneby genotype interaction: F_(2,16) = 2.91; p = 0.08), spent lesstime sniffing volatile odors when treated withestradiol.

Soiled bedding
Testosterone treatment. All female subjects preferred to investigate soiled bedding from estrous females over bedding fromintact males (Fig. 2A). Two-way ANOVA with genotype as the independentfactor and odor stimulus (male vs female bedding) as the repeatedfactor showed a significant effect of genotype (F_(2,16) = 8.29;p = 0.0034) and a significant effect of odor stimulus (F_(1,16)= 14.93; p = 0.0014). Post hoc analysis of the genotype effectshowed that ArKO females spent less time sniffing soiled bedding,either male or female, than WT females (Fig. 2B). Furthermore,all three genotypes spent more time sniffing female bedding thanmale bedding (because there was no significant odor stimulus bygenotype interaction: F_(2,16) = 0.96; p = 0.40).

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Figure 2. A, C, Mean amount of time that female WT, HET, and ArKO mice spent sniffing nonvolatile olfactory cues when given a choice between soiled bedding from intact males and that from estrous females in a Y-maze. B, D, Total amount of time spent sniffing nonvolatile odors. A, B, Results when subjects were treated with testosterone. C, D, Results when the same subjects were treated with estradiol. Means with different letters above them are significantly different from each other by post hoc comparisons.

Estradiol treatment. The preference to investigate female bedding over male bedding disappeared when female subjects weretreated with estradiol (Fig. 2, C vs A). In addition, all femalegroups, particularly ArKO, spent more time sniffing soiled beddingwhen treated with estradiol than when treated with testosterone(Fig. 2, D vs B). As a result, ArKO females no longer differedfrom WT and HET females in total time spent sniffing soiled bedding.This was confirmed by two-way ANOVA with genotype as the independentfactor and odor stimulus as the repeated factor, showing neitheran effect of genotype (F_(2,16) = 0.79; p = 0.47) nor an effectof odor stimulus (F_(1,16) = 0.165; p = 0.69).
Testosterone versus estradiol treatment. In comparing the effects of the two hormone treatments, three-way ANOVA with genotypeas the independent factor and hormone treatment (testosteronevs estradiol) and odor stimulus as repeated factors revealed asignificant effect of hormone treatment (F_(1,16) = 35.41; p =0.0001). Post hoc analysis showed that WT and HET females increasedtheir time sniffing male bedding while on estradiol, whereas ArKOfemales spent more time investigating both types of bedding aftertreatment with estradiol (Fig. 2, B vs D).

Direct access to stimulus animals
Testosterone treatment. No clear preference could be discerned when female subjects were given direct access to an intactmale and an estrous female, with both stimulus animals being anesthetized(Fig. 3A). Two-way ANOVA with genotype as the independent factorand odor stimulus as the repeated factor showed a significanteffect only of genotype (F_(2,16) = 4.91; p = 0.02). Post hoc analysisrevealed that ArKO females spent less time investigating the anogenitalregions and flanks of the stimulus animals compared with WT andHET females (Fig. 3B).

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Figure 3. A, C, Mean amount of time that female WT, HET, and ArKO mice spent sniffing the anogenital region and flanks when given a choice between an anesthetized intact male and an anesthetized estrous female in a Y-maze. B, D, Total amount of time spent sniffing the anogenital region and flanks. A, B, Results when subjects were treated with testosterone. C, D, Results when the same subjects were treated with estradiol. Means with different letters above them are significantly different from each other by post hoc comparisons.

Estradiol treatment. Again, females of all three genotypes showed no clear preference for either stimulus animal (Fig. 3C).As was observed with the soiled bedding in experiment 1, ArKOfemales no longer differed from WT and HET females in total timespent investigating the stimulus animals (Fig. 3D). Accordingly,two-way ANOVA with genotype as the independent factor and odorstimulus as the repeated factor no longer showed a significanteffect of genotype (F_(2,16) = 0.537; p = 0.59).
Testosterone versus estradiol treatment. In comparing the effects of hormone treatment on time spent sniffing the stimulusanimals, three-way ANOVA with genotype as the independent factorand hormone treatment and odor stimulus as repeated factors revealeda significant effect of hormone treatment (F_(1,16) = 4.66; p =0.05). Post hoc analysis showed that all females, but particularlyWT and HET females, decreased their time spent sniffing the stimulusanimals when treated with estradiol. Thus, in contrast to thefindings with the soiled bedding in experiment 1, in which ArKOfemales increased their time spent sniffing soiled bedding aftertreatment with estradiol, WT and HET females decreased their timesniffing the anesthetized stimulus animals after treatment withestradiol, and consequently genotype differencesdisappeared.

Odor and visual cues
Testosterone treatment. All female groups showed a weak preference for the estrous female when given a choice between an awakeintact male and an awake estrous female placed behind a clearPlexiglas door (Fig. 4A). Two-way ANOVA with genotype as the independentfactor and odor stimulus as the repeated factor revealed a significanteffect of genotype (F_(2,16) = 8.72; p = 0.0027) and an almostsignificant effect of odor stimulus (F_(1,16) = 3.36; p = 0.085).Post hoc analysis of the genotype effect showed that ArKO femalesspent less time investigating odor and visual cues of either malesor females compared with WT females (Fig. 4B). Post hoc analysisof the effect of odor stimulus showed that subjects of all threegenotypes showed a preference, albeit small, to investigate theestrous female instead of the intact male.

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Figure 4. A, C, Mean amount of time that female WT, HET, and ArKO mice spent investigating odor and visual cues when given a choice between an awake intact male and an awake estrous female in a Y-maze. B, D, Total amount of time investigating odor and visual cues. A, B, Results when subjects were treated with testosterone. C, D, Results when the same subjects were treated with estradiol. Means with different letters above them are significantly different from each other by post hoc comparisons.

Estradiol treatment. HET females preferred to investigate odor and visual cues from an intact male over those from an estrousfemale, whereas WT and ArKO females showed no preference (Fig.4C). Two-way ANOVA with genotype as the independent factor andodor stimulus as the repeated factor showed a significant effectof genotype (F_(2,16) = 13.46; p = 0.0004), an almost significanteffect of odor stimulus (F_(1,16) = 3.25; p = 0.09), and an almostsignificant stimulus by genotype interaction (F_(1,16) = 2.86;p = 0.087). Post hoc analysis of the genotype effect showed thatArKO females spent less time investigating odor and visual cuesthan WT and HET females (Fig. 4D). Furthermore, HET females spentmore time investigating the intact male than the estrous female,whereas WT and ArKO females spent similar amounts of time investigatingboth stimulusanimals.
Testosterone versus estradiol treatment. In comparing the effects of hormone treatment on time spent investigating odor andvisual cues, three-way ANOVA with genotype as the independentfactor and hormone treatment and odor stimulus as repeated factorsshowed a significant effect of hormone treatment (F_(1,16) = 15.59;p = 0.0012) and a significant hormone treatment by stimulus interaction(F_(1,16) = 8.34; p = 0.011). Post hoc analysis of the hormoneeffect and the interaction showed that all females spent lesstime investigating odor and visual cues from the estrous femaleafter estradiol treatment (Fig. 4, A vs C).

Experiment 2: contribution of the aromatase gene to the development of lordosis behavior

The display of lordosis in response to the mounting of a stud male was clearly impaired in ArKO females that were treatedwith estradiol and progesterone (Fig. 5A). The same hormone treatmentwas effective, however, in inducing lordosis behavior in WT andHET females. Two-way ANOVA with genotype as the independent factorand tests as the repeated factor revealed a significant effectof genotype (F_(2,15) = 19.45; p = 0.0001) and a significant effectof repeated testing (F_(4,60) = 4.57; p = 0.0027). Post hoc analysisshowed that lordosis quotients were lower in ArKO females thanWT and HET females. Furthermore, lordosis quotients increasedin the same way in all female groups over tests, because therewas no significant test by genotype interaction (F_(8,60) = 0.74;p = 0.65). The number of mounts received from the stud male didnot differ between groups (mean ± SEM: WT, 9.9 ± 0.4; HET, 9.8± 0.2; ArKO, 9.7 ± 0.2; F_(2,15) = 0.36; p = 0.70).

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Figure 5. Female sexual behavior with a stud male of female WT, HET, and ArKO mice. A, Lordosis quotients; B, receptivity index. *p < 0.05 compared with WT and HET females.

In addition, ArKO females rejected the stud male more frequently, as indicated by their lower receptivity scores, than WTand HET females (Fig. 5B). Two-way ANOVA with genotype as theindependent factor and tests as the repeated factor indicateda significant effect of genotype (F_(2,15) = 36.0; p = 0.0001)and a significant effect of testing (F_(4,60) = 6.59; p = 0.0002).Post hoc analysis showed that receptivity scores were significantlylower in ArKO females than WT and HET females and increased similarlyin all female groups over the course of testing, because therewas no significant test by genotype interaction (F_(8,60) = 1.35;p = 0.23) (Fig. 5B).

Experiment 3: olfaction test

Overall, there was no significant difference between females of each genotype in the time it took to find the hidden cookie(mean ± SEM: WT, 89 ± 5 sec; HET, 189 ± 15 sec; ArKO, 181 ± 21sec). Two-way ANOVA with genotype as the independent factor andtests as the repeated factor revealed a significant effect oftests (F_(1,15) = 6.24; p = 0.02) but no significant effect ofgenotype (F_(2,15) = 1.70; p = 0.22) nor a significant test bygenotype interaction (F_(2,15) = 2.44; p = 0.12). The longer averagetime to find the cookie in the HET and ArKO groups reflects thepoor performance of two ArKO females and one HET female but didnot appear to be a characteristic of the genotype. Overall, allfemales found the cookie faster in the second test (mean ± SEM:WT, 137 ± 28 vs 42 ± 5 sec; HET, 325 ± 75 vs 53 ± 19 sec; ArKO,189 ± 48 vs 174 ± 101 sec for test 1 vs 2, respectively). Thiseffect of repeated testing appears to be less pronounced in ArKOfemales, but there was no significant test by genotype interaction(F_(2,15) = 2.44; p = 0.12).

Experiment 4: open-field test

Overall, no differences could be detected in general locomotor activity among female groups when subjects were tested in anopen field. One-way ANOVA on the number of crossings did not showany genotype differences (mean ± SEM: WT, 66.6 ± 9.5; HET, 55.2± 8.0; ArKO, 56.2 ± 9.7; F_(2,14) = 0.47; p = 0.64). Furthermore,one-way ANOVA on the maximum amount of time spent immobile alsodid not show any genotype differences (mean ± SEM: WT, 38 ± 7sec; HET, 62 ± 14 sec; ArKO, 62 ± 14 sec; F_(2,14) = 1.04; p =0.38).

Experiment 5: contribution of the aromatase gene to the development of male sexual behaviors

When treated with testosterone alone, female ArKO mice showed no male-typical sexual behaviors with an estrous female, whereasWT and, to a lesser extent, HET females readily displayed mountingand intromission-like behaviors. The addition of estradiol tothe testosterone treatment stimulated a little mounting and intromission-likebehavior in ArKO females, but not up to the levels shown by WTand HET females (Fig. 6). A two-way ANOVA on the number of mountsrevealed a significant effect of genotype (F_(2,23) = 7.06; p =0.0041) and a significant hormone by genotype interaction (F_(2,23)= 6.14; p = 0.0073). Post hoc analysis on the genotype effectshowed that ArKO females displayed fewer mounts than WT and HETfemales. Furthermore, post hoc analysis on the hormone by genotypeinteraction revealed that ArKO females mounted the estrous femalemore frequently when treated with testosterone and estradiol,whereas the total number of mounts remained the same in WT andHET females. Two-way ANOVA on the number of intromission-likebehaviors revealed a significant effect of genotype (F_(2,23) =23.84; p = 0.0001), a significant effect of hormone treatment(F_(1,23) = 5.36; p = 0.03), and a significant hormone by genotypeinteraction (F_(2,23) = 5.90; p = 0.0085). Post hoc analysis ofthe genotype effect showed that ArKO females displayed fewer intromission-likebehaviors compared with WT and HET females, with the latter displayingfewer intromissions than WT females. Post hoc analysis of thehormone by genotype effect showed that ArKO females displayedmore intromission-like behaviors when treated with testosteroneand estradiol, whereas the number of intromissions decreased insimilarly treated WT and HET females.

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Figure 6. A, C, Mean number of mounts and intromission-like behaviors displayed by female WT, HET, and ArKO mice when paired with an estrous female. B, D, Total number of mounts and intromissions together. A, B, Results when subjects were treated with testosterone. C, D, Results when the same subjects also received daily injections with estradiol while remaining on testosterone. Means with different letters above them are significantly different from each other by post hoc comparisons.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study indicates that estradiol is required both during development and in adulthood for a normal expression ofsociosexual behaviors in the female mouse. Female ArKO mice thatare depleted of estradiol because of a targeted mutation of thearomatase gene showed aberrant sociosexual behaviors in adulthood.When treated with testosterone, ArKO females showed little motivationto investigate olfactory (both volatile and nonvolatile) and visualcues from either an estrous female or an intact male. Even whenphysical contact was allowed, ArKO females investigated the stimulusanimals significantly less than WT subjects. These behavioraldifferences could have reflected differences in activation ofolfactory investigation by estradiol, because testosterone treatmentpresumably generated higher levels of estradiol in WT than inArKO females. To distinguish between activational and organizationaleffects of estradiol on olfactory investigation, the same femalesubjects were tested again for odor preferences after they hadreceived estradiol treatment for several weeks in adulthood. Thedefects in olfactory investigation could, in part, be correctedwith adult estradiol treatment. The motivation to investigatesoiled bedding was restored in estradiol-treated ArKO females.In contrast, adult estradiol treatment did not restore the motivationof ArKO females to investigate volatile odors from either stimulusanimal. Furthermore, ArKO females showed little or no lordosisbehavior when treated with doses of estradiol and progesteronethat were behaviorally effective in WT females. These resultssuggest that estradiol has both organizational and activationaleffects on the display of olfactory investigation and sexual receptivityin femalemice.

Organizational effects of estrogens in female mice

Sexual receptivity and olfactory investigations were severely impaired in female ArKO mice even after prolonged (>6 weeks)treatment with estradiol in adulthood. Many rodent species, includingmice, rely on olfactory cues to distinguish the sex and reproductivestatus of conspecifics (Brown, 1979). It is possible that ArKOfemales simply did not recognize the stud male as being male onthe basis of his odors and as a result did not become sexuallyreceptive. Interestingly, the lordosis impairment decreased towardthe end of the tests, possibly as a result of repeated mountingand stimulation of the flanks and back of the female. The deficitsin sexual receptivity might thus be caused by an impairment inolfactoryrecognition.

The deficit in lordosis behavior was unexpected, because male rats neonatally deprived of estradiol showed female-typicallevels of sexual receptivity after treatment with estradiol andprogesterone in adulthood (McEwen et al., 1977; Vreeburg et al.,1979; Fadem and Barfield, 1981; Bakker et al., 1993). These dataled to the concept that the female brain develops in the absenceof ovarian hormones, whereas the development of the male brainrequires the presence of both testosterone and estradiol. Severalstudies have challenged this concept and suggested an active rolefor estradiol in the development of the brain in females (Toran-Allerand,1976; Döhler et al., 1984; Mack et al., 1993). The present workprovides new evidence that estradiol may be required for a normalfemale development and thus a normal expression of sociosexualbehaviors inadulthood.

It seems unlikely that the deficit in lordosis behavior can be attributed to excessive androgen action during developmentleading to a masculinization and defeminization of the brain.Fisher et al. (1998) reported that testosterone levels are elevatedin adult ArKO females. This elevation is probably a result ofthe absence of a negative feedback by estradiol on the hypothalamus,as evidenced by increased levels of luteinizing hormone. However,whether testosterone levels are also elevated during developmentremains questionable. Basal estrogen secretion (and presumablytestosterone production) by the ovaries has been shown to be undetectableduring fetal stages and before day 5 after birth (Weniger, 1993;Weniger et al., 1993). However, even if testosterone levels areelevated perinatally in ArKO females, the strongest evidence againstthis hypothesis is that ArKO females displayed very little mountingbehavior after treatment with testosterone and estradiol in adulthood,whereas similarly treated WT and HET females vigorously mountedstimulus females. Likewise, it seems unlikely that the brainsof ArKO females were defeminized by excessive androgen actionduring development, because many studies (Naftolin et al., 1975;McEwen et al., 1977; Baum, 1979; Vreeburg et al., 1979; Fademand Barfield, 1981; MacLusky and Naftolin, 1981; Bakker et al.,1993) have shown that estradiol and not testosterone is the hormoneimplicated in defeminizing the brain. For instance, male ratstreated neonatally with an aromatase inhibitor but left gonadallyintact (and thus exposed to testosterone) showed levels of lordosisbehavior similar to those of normal females (Bakker et al., 1993).Likewise, male mice and rats carrying a mutation in the androgenreceptor (tfm) did not show any lordosis behavior after treatmentwith estradiol and progesterone in adulthood, suggesting thattheir lordotic potential was lost as a result of estrogen actionduring development (for review, see Olsen, 1992).

Alternatively, the impairment of lordosis behavior in ArKO females could result from their hypersensitivity to small amountsof estrogens coming from their HET mother leading to a defeminizationof their adult lordotic potential. However, concentrations offree maternal estradiol in the fetuses should be very low becauseof the presence of high levels of estradiol-binding $alpha$ -fetoproteinsin the blood. These $alpha$ -fetoproteins are thought to protect thedeveloping female brain from being masculinized and defeminizedby estradiol, and there is no reason why $alpha$ -fetoproteins wouldplay this role differentially in WT and in ArKOsubjects.

Finally, phytoestrogens potentially present in the food could freely enter the fetal brain, because they presumably do notbind to $alpha$ -fetoproteins and thus could be a significant sourceof estrogen action in ArKO females. Limited developmental effectsof phytoestrogens on sexual behavior and neuroendocrine functionhave been reported in rats, although most significant effectswere seen in males (Whitten et al., 1995). However, our mice werefed a mouse chow (UAR, Epinay sur Orge, France) that does notappear to contain biologically active estrogens, as revealed byits lack of effect on uterine growth and on the growth of estrogen-dependentcell lines (M. Huard, UAR, personal communication). Exposure ofour ArKO mice to phytoestrogens was thus negligible. In conclusion,the present results are best explained by assigning an activerole for estradiol in females in the development of the neuralsubstrates that are involved, in later life, in olfactory recognitionand sexualreceptivity.

Sexual differentiation of odor preferences in mice

In contrast to rats (Bakker et al., 1996), odor preferences do not seem to be sexually differentiated in mice. Like male WTmice (Bakker et al., 2002), female WT mice, especially when treatedwith estradiol in adulthood, showed a clear preference to sniffvolatile odors from an estrous female over those from an intactmale. Furthermore, WT females showed high levels of male sexualbehavior when paired with an estrous female, suggesting that femalemice are normally masculinized. HET females displayed male sexualbehaviors and odor preferences at levels that were intermediatebetween WT and ArKO subjects. Correspondingly, brain aromataseactivity was found to be intermediate in HET females, whereasit was undetectable in ArKO females (Baillien et al., 2002). Theseresults suggest that a female-directed odor preference and theexpression of male sexual behavior are organized by aromatizedmetabolites of testosterone in a dose-dependentmanner.

Main versus accessory olfactory system

In most mammalian species, a main olfactory system and an accessory olfactory system can be distinguished neuroanatomically.In rodents, pheromones that are generally composed of nonvolatilemolecules are presumably processed by the accessory olfactorysystem (Meredith and O'Connell, 1979), whereas nonreproductivelyrelevant olfactory cues composed mostly of volatile moleculesare processed primarily through the main olfactory system (O'Connelland Meredith, 1984). The present study shows that estradiol differentiallyaffected the functioning of these two systems. Estradiol appearsto be required for the development of the main olfactory system,because the deficiencies in olfactory investigation of volatileodors by ArKO females could not be corrected by prolonged estradioltreatment in adulthood. ArKO females were not anosmic, however,and could find a hidden food item by its smell as rapidly as WTand HET subjects. In contrast, estradiol is apparently not requiredfor the development of the accessory olfactory system but is neededfor its normal functioning in adulthood: treatment with estradiolof ArKO females corrected the previously observed defects in olfactoryinvestigation of soiled bedding. Thus, estradiol has organizationaleffects on the main olfactory system and activational effectson the accessory olfactorysystem.

In conclusion, the present study using estradiol-deficient ArKO mice indicates that estradiol is required during developmentfor the expression of sociosexual behaviors in adult female mice.The old concept that female differentiation proceeds in the absenceof any hormonal influence therefore requires re-examination. Thepresent data do not identify the developmental stage(s) (i.e.,embryonic, early postnatal, and/or prepubertal and postpubertal)at which exposure to estradiol is required for a normal developmentof the female brain, but this question can be answered using theArKO mouse model, because its genetic deficiency can be bypassedby administration of exogenous estradiol at specific stages ofthe lifecycle.

  FOOTNOTES

Received Feb. 20, 2002; revised June 3, 2002; accepted July 3, 2002.

This work was supported by French Community of Belgium Grant ARC 99/04-241 and National Institutes of Health Grant MH-50388.

Correspondence should be addressed to Dr. Julie Bakker, Center for Cellular and Molecular Neurobiology, Research Group inBehavioral Neuroendocrinology, University of Liège, 17 PlaceDelcour (Bat L1), B-4020 Liège, Belgium. E-mail: jbakker{at}ulg.ac.be.

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RESULTS
DISCUSSION
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