Functional Interactions between Estrogen and Insulin-Like Growth Factor-I in the Regulation of alpha 1B-Adrenoceptors and Female Reproductive Function

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The Journal of Neuroscience, March 15, 2002, 22(6):2401-2408

Functional Interactions between Estrogen and Insulin-Like Growth Factor-I in the Regulation of $alpha$ _1B-Adrenoceptors and Female Reproductive Function
Arnulfo Quesada and Anne M. Etgen
Department of Neuroscience, Albert Einstein College of Medicine, Bronx, New York 10461

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The ovarian hormone estradiol (E₂) and insulin-like growth factor-I (IGF-I) interact in the CNS to regulate neuroendocrinefunction and synaptic remodeling. Previously, our laboratory showedthat 2 d E₂ treatment induces $alpha$ _1B-adrenoceptor expression andpromotes IGF-I enhancement of $alpha$ ₁-adrenoceptor potentiation ofcAMP accumulation in the preoptic area (POA) and hypothalamus(HYP). This study examined the hypothesis that E₂-dependent aspectsof female reproductive function, including $alpha$ _1B-adrenoceptor expressionand function in the POA and HYP, are mediated by brain IGF-I receptors(IGF-IRs) in female rats. Ovariohysterectomized rats were implantedwith a guide cannula aimed at the third ventricle and treatedin vivo with vehicle or E₂ daily for 2 d before experimentation.Intracerebroventricular infusions of JB-1, a selective IGF-IRantagonist, were administered every 12 hr beginning 1 hr beforethe first E₂ injection. Administration of JB-1 during E₂ primingcompletely blocks hormone-induced luteinizing hormone releaseand partially inhibits hormone-dependent reproductive behavior.Reproductive behavior is restored by intracerebroventricular infusionof 8-bromo-cGMP, the second messenger implicated in $alpha$ ₁-adrenergicfacilitation of lordosis. In addition, blockade of IGF-IRs duringE₂ priming prevents E₂-induced increases in $alpha$ _1B-adenoceptor bindingdensity and abolishes acute IGF-I enhancement of NE-stimulatedcAMP accumulation in HYP and POA slices. These data document theexistence of a novel mechanism by which IGF-I participates inthe remodeling of noradrenergic receptor signaling in the HYPand POA after E₂ treatment. These events may help coordinate thetiming of ovulation with the expression of sexualreceptivity.

Key words: estradiol; IGF-I; adrenoceptor; hypothalamus; preoptic area; reproduction

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Estradiol (E₂), the main estrogenic hormone produced and secreted by the ovaries, acts on the hypothalamus (HYP) and preopticarea (POA), brain regions responsible for female reproductivefunction (Barfield and Chen, 1977; Chappel, 1985). E₂ actionsin these brain regions enhance reproductive success by ensuringthat female sexual receptivity (lordosis) coincides with the releaseof pituitary luteinizing hormone (LH), which triggers ovulation(Pfaff, 1980; Etgen et al., 1992; Freeman, 1994).

E₂ action in the HYP and POA modifies several cellular and molecular components of the noradrenergic system. Norepinephrine(NE) has been implicated as a major neurochemical mediator ofboth sexual receptivity and the preovulatory LH surge (Kalra andKalra, 1983; Crowley, 1986; Etgen et al., 1992; Freeman, 1994;Herbison, 1997). NE actions in the HYP-POA can either facilitateor inhibit lordosis behavior and LH release, depending on thehormonal status of the animal (Etgen et al., 1992). NE activationof $alpha$ ₁-adrenoceptors facilitates lordosis behavior and LH releaseonly if animals have been exposed to E₂ (Crowley, 1986; Kow etal., 1992; Weesner et al., 1993; Herbison, 1997). E₂ increases $alpha$ _1B-adrenoceptor binding and mRNA levels in both HYP and POA (Petittiet al., 1992; Karkanias et al., 1996). These NE receptors arebelieved to mediate NE facilitation of sexual receptivity andpreovulatory LH release (Kow et al., 1992; Hosny and Jennes, 1998).Despite evidence that E₂ remodels the biochemical responses ofthe HYP and POA to NE, the mechanism or mechanisms by which E₂modulates the noradrenergic system are stillunclear.

Cross-talk or interactions between E₂ and insulin-like growth factor-I (IGF-I) have been demonstrated in the CNS, in variousreproductive tissues and in cell cultures. For example, E₂ canregulate the expression of IGF-I, IGF-I binding proteins, andIGF-I receptors (IGF-IRs) (Dickson et al., 1986; Pons and Torres-Aleman,1993; Wimalasena et al., 1993; Sahlin et al., 1994). Likewise,IGF-I can regulate the expression and function of E₂ receptors(Aronica and Katzenellenbogen, 1993; Stoica et al., 2000). Inaddition, IGF-I has been implicated in certain effects of E₂ onsynaptic structure and on neuroprotection (Duenas et al., 1996;Garcia-Segura et al., 1996; Patrone et al., 1996; Azcoitia etal., 1999; Fernandez-Galaz et al., 1999). Recently, we showedthat IGF-I enhances $alpha$ ₁-adrenoceptor function in the HYP and POA,but only in E₂-primed rats (Quesada and Etgen, 2001). Becausethese observations suggest that E₂ effects on NE receptor functionmay involve IGF-I, we hypothesized that E₂-dependent sexual receptivity,LH release and remodeling of the biochemical responses of HYPand POA slices to NE may be mediated via IGF-IR activity. Presentdata show that in vivo blockade of brain IGF-IRs during E₂ primingprevents increased expression of $alpha$ _1B-adrenoceptor in the HYP-POAand completely blocks E₂-dependent LH release. In vivo blockadeof IGF-IRs during E₂ priming also blocks IGF-I enhancement of $alpha$ ₁-adrenoceptor signaling in POA and HYP slices and partiallyinhibits E₂-dependent sexual receptivity. These novel findingsdemonstrate that brain IGF-IRs are involved in the cellular andmolecular actions underlying E₂ regulation of female reproductivefunction.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animal treatments. Female Sprague Dawley rats (Taconic Farms, Germantown, NY) weighing 175-200 gm were anesthetized with ketamine(80 mg/kg body weight) and xylazine (4 mg/kg body weight), placedinto a stereotaxic apparatus, and secured with ear bars and anosepiece set at +5.0 mm. A 26 gauge guide cannula (Plastics One,Roanoke, VA) was implanted into the third ventricle using coordinatesfrom the atlas of Pellegrino et al. (1979). Animals were bilaterallyovariohysterectomized (OVX) to remove the primary source of estrogenand progesterone immediately after stereotaxic surgery. Four toseven days after stereotaxic surgery and OVX, all rats were injectedsubcutaneously with either peanut oil (control) or with 2 µg ofE₂ benzoate (EB) (Steraloids Inc., Wilton, NH) in peanut oil 24and 48 hr before killing. In most cases, multiple infusions of1 µl of saline or 4 µg of JB-1 (Bachem, San Carlos, CA), a selectiveantagonist for IGF-IR, in 1 µl of saline were given intracerebroventricularly1 hr before and 12 hr after both EB injections. Experimental useof animals was in accordance with the National Institutes of HealthGuidelines for the Care and Use of Laboratory Animals. The InstitutionalAnimal Care and Use Committee of the Albert Einstein College ofMedicine approved all animalprotocols.

NE-stimulated cAMP accumulation. The animals were rapidly killed, and the brains were placed in artificial CSF (aCSF) (Yamamoto,1972). In all experiments, brain slices were prepared between1000 and 1100 hr to eliminate potential diurnal variation in cAMP(Kant et al., 1981) and adrenoceptor (Krauchi et al., 1984; Jhanwar-Uniyalet al., 1986) content. HYP and POA were dissected, and 350 µmslices were made on a McIlwain tissue chopper beginning ~2 mmanterior to the optic chiasm and ending 1 mm anterior to the mammillarybodies. The first four slices containing the medial and lateralPOA, suprachiasmatic nucleus, and supraoptic nucleus were takenand designated POA. The next slice was discarded, and the followingfour slices containing the anterior, lateral, ventromedial, paraventricular,arcuate, and dorsomedial nuclei of the HYP were kept and designatedHYP. Individual slices were incubated at 35°C in 300 µl of oxygenatedaCSF, which included a phosphodiesterase (PDE) inhibitor, 1 mM3-isobutyl-1-methylxanthine (IBMX). IBMX was dissolved in absoluteethanol and added to slices such that the final concentrationof ethanol was 1%. After a 75 min equilibration period sliceswere exposed for 15 min to 10 nM IGF-I (National Institutes ofHealth, National Hormone and Pituitary Program) dissolved in distilledwater. Slices were then stimulated with either vehicle or 100µM NE (Research Biochemicals, Natick, MA) dissolved in 0.01 NHCl. Each experiment included POA and HYP slices from EB-treatedanimals infused with either saline or JB-1, and each experimentwas repeated four times. cAMP determination was done as previouslydescribed (Quesada and Etgen, 2001) using a modified Gilman cAMPassay (Brostrom and Kon, 1974).

Immunoblotting for phosphorylated extracellular receptor-activated kinase 1/2. HYP slices from E₂-primed rats that were alsoinfused with JB-1 or saline were incubated at 35°C in 300 µl ofoxygenated aCSF for 75 min, then exposed for 15 min to vehicleor 10 nM IGF-I dissolved in distilled water. After vehicle orIGF-I treatments, two slices were pooled and prepared by Teflonhomogenization in ice-cold 1% Triton X-100, 1 mM sodium vanadate,1 mM phenylmethylsulfonyl fluoride, and 10 mM Tris-HCl, pH 7.4.After homogenization, samples were spun for 15 min at 14,000 ×g to remove insoluble material. Protein concentrations were determinedby a modified Lowry assay. Fifty micrograms of protein were appliedto 12.5% SDS-polyacrylamide minigels and resolved at 150 V for1.5 hr. Proteins were transferred electrophoretically onto polyvinylidenediflouridemembranes (Renaissance; New England Nuclear, Boston, MA) at 150amps for 1 hr. Membranes were then blocked for 1 hr in 5% bovinealbumin serum (BSA) and 0.1% Tween 20 in Tris-buffered saline(TBS) at 37°C. Membranes were incubated for 1 hr at 37°C withan antibody for phosphorylated extracellular receptor-activatedkinase 1/2 (ERK1/2) (Tyr 204; 1:1000; Santa Cruz Biotechnology,Santa Cruz, CA). Blots were stripped by incubating the membranesfor 30 min at 50°C in stripping solution (0.0625 M Tris-HCl, pH6.8; 0.2% SDS, 0.1 M $beta$ -mercaptoethanol), washed three or fourtimes in TBS for 10 min, and reprobed with rabbit anti-ERK2 (1:1000;Santa Cruz Biotechnology) for total ERK2 protein assessment. Bindingof the primary antibody was detected by anti-rabbit secondaryantibodies conjugated to horseradish peroxidase (1:10,000) in5% BSA. Peroxidase activity was visualized by means of chemiluminescence.Blots were exposed to FUJI medical x-ray film (Fisher Scientific,Pittsburgh, PA). Band intensity was obtained by scanning autoradiogramson a DC-120 digital camera (Eastman Kodak, Rochester, NY) witha +3 diopter lens and analyzing the image using the Kodak 1D gelanalysis program. Immunoblots were quantitatively analyzed bytaking the ratio of the optical density (OD) of the phospho-ERK2band to the OD of the total ERK2 band. That ratio was used tocalculate the percentage of change in ERK2 activation of IGF-Iversus vehicle-treated HYP slices run on the samegel.

Radioligand binding assays. To provide sufficient material for Scatchard analysis, tissue from two rats given identical hormoneinjections and drug treatments was combined. POA and HYP sampleswere homogenized separately in 5 ml of ice-cold Tris-MgCl₂ buffer(50 mM Tris HCl and 10 mM MgCl₂, pH 7.4) using a Polytron at speed5-6 for 20 sec. The homogenates were centrifuged for 10 min at20,000 × g, the supernatant was discarded, and the pellet containingthe membrane fraction was frozen at $-$ 70°C until assay. Freezingof the crude membrane fraction does not result in a measurableloss of any NE receptor subtype (Etgen and Karkanias, 1990).

The radioligand ³H-prazosin (87 Ci/mmol; New England Nuclear) was used to measure total $alpha$ ₁-adrenoceptor binding in brain membranes.To distinguish $alpha$ _1A and $alpha$ _1B-adrenoceptor subtypes, chlorethylclonidine(CEC; Research Biochemicals), a selective, irreversible inactivatorof the $alpha$ _1B-adrenoceptor, was used. Frozen membranes were resuspendedin 6 ml of Na-HEPES buffer and split into two equal fractions.Each fraction was preincubated for 10 min at 37°C with vehicleor with 10 µM CEC. Reactions were stopped by addition of 6 mlof ice-cold Na-HEPES buffer and centrifugation for 10 min at 20,000× g. The supernatant was discarded, and the pellet was resuspendedin 6 ml of Tris-MgCl₂ buffer. For Scatchard analysis, duplicate200 µl aliquots were incubated for 20 min at 37°C with 0.05-5nM ³H-prazosin with and without a 2000-fold excess of phentolamineto assess nonspecific binding. Specific ³H-prazosin binding after CEC inactivation reflects the $alpha$ _1A-adrenergicreceptor population. The $alpha$ _1B-adrenoceptor population was determinedby subtracting the binding of ³H-prazosin after CEC inactivation from total specific ³H-prazosin binding. Bound and free ³H-prazosin were separated by rapid filtration through glass fiberfilters (FPB-148 Whatman GF/B) on a Brandel (Gaithersburg, MD)cell harvester as described previously (Petitti et al., 1992).Ligand affinities (K_d), apparent receptor numbers (B_max), andHill coefficients were calculated using the EBDA ligand program(Elsevier-Biosoft, Cambridge, UK). Experiments used tissue fromOVX control and EB-primed female rats infused chronically witheither saline or JB-1 and were repeated fourtimes.

LH radioimmunoassay. Concentration of LH in serum was determined using primary antibody for rat LH (1:30,000; National Hormoneand Pituitary Program) and ¹²⁵I-LH (3000-5000 cpm/100 µl; Covance Laboratories, Inc., Vienna,VA). Secondary antibody, goat anti-rabbit IgG, was obtained fromSigma (St. Louis, MO). Concentration of rat LH was expressed asng RP-3 per ml, provided by the National Hormone and PituitaryProgram. Animals were maintained on a reverse 14:10 light/darkcycle with the lights off at 11:00 A.M. Trunk blood samples werecollected when the animals were decapitated at 8:00 P.M., allowedto clot overnight at 4°C, then centrifuged at 2000 × g for 30min. Serum was decanted into polypropylene tubes and frozen at $-$ 20°C until analysis. Concentrations of LH in 100 µl aliquotsof serum were determined in triplicate. Incubation periods betweenadditions of primary antibody, radioiodinated hormone, and secondantibody were 24 hr at room temperature. The sensitivity of theassay was 0.05 ng/tube, and samples were run in two separate assays.The intra-assay and inter-assay variances were 6 and 18%,respectively.

Reproductive behavior testing. Animals were maintained on a reverse 14:10 light/dark cycle with the lights off at 11:00 A.M.OVX female rats were primed with EB for 48 hr as described previouslyfollowed by 500 µg of progesterone 4 hr before behavior testing.Animals were tested once a week for 3 weeks after receiving oneof three treatments in random order: (1) multiple infusions ofJB-1 (4 µg/1 µl) dissolved in saline, (2) multiple infusions of1 µl of saline, or (3) multiple infusions of JB-1 (4 µg/1 µl)followed by a single infusion of 8-bromo-cGMP (1 µg/2 µl) (Calbiochem,La Jolla, CA) administered 4 hr before behavior testing. Separategroups of rats received a single acute infusion of JB-1 (4 µg/1µl) given either at 12 or 4 hr before testing (12 hr, n = 6; 4hr, n = 4). Experienced stimulus male rats were placed in 20 gallonglass arenas and allowed to adapt for 10 min. Females were thenplaced in the arenas with a male until they received 10 mountswith pelvic thrusting. A lordosis quotient (LQ = number of lordosisresponses/number of mounts × 100) was used as a measure of behavioralreceptivity. The quality of lordosis was also scored on a scaleof 0-3 (0, no lordosis; 1, shallow lordosis; 2, definitive dorsiflexionof the spine; 3, exaggerated lordosis). Anatomical verificationof the cannula placement was made according to the atlas of Pellegrinoet al. (1979).

Statistics. cAMP levels were analyzed with one-way ANOVA using the Statview statistical program with drug treatment as theonly factor. Significant differences between means were determinedfor main effects by Fisher's PLSD. Radioligand binding and LHdata were analyzed using two-way ANOVA with drug treatment andhormone as the two factors. Significant differences between meanswere determined for main effects by Fisher's PLSD. Behavioraldata were analyzed using repeated measures one-way ANOVA withdrug as the repeated factor, followed by Fisher's PLSD. Differenceswere considered significant if p < 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

E₂ induction of $alpha$ _1B-adrenoceptor in the POA and HYP requires IGF-IR activity

Receptor tyrosine kinases such as IGF-I and insulin can increase $alpha$ _1D-adrenoceptor gene expression and function in vascularsmooth muscle cells (Hu et al., 1996), and general tyrosine kinaseinhibitors can block NE upregulation of $alpha$ _1B-adrenoceptors in clonalH cells (Bird et al., 1997). We examined the possibility thatthe E₂-dependent increase in $alpha$ _1B-adrenoceptor density in the POAand HYP in female rats may require IGF-I activity. E₂-treatedfemale rats received multiple intracerebroventricular infusionsof JB-1 or saline, and receptor density for total $alpha$ ₁-adrenoceptor, $alpha$ _1A- and $alpha$ _1B-adrenoceptor was examined in HYP and POA membranes.JB-1 is a peptide analog of IGF-I based on the amino acid sequenceof the C-terminal, D domain of IGF-I, which is involved in bindingto the IGF-IR. It is a potent, highly selective, competitive antagonistof IGF-I-dependent receptor autophosphorylation and cellular proliferation(Pietrzkowski et al., 1992).

As reported previously, E₂ modestly increases the density of ³H-prazosin binding sites (total $alpha$ ₁-adrenoceptor) in POA and HYPmembranes from saline-infused animals (p < 0.05). Multiple intracerebroventricularinfusions of JB-1 block E₂-induced increases in total $alpha$ ₁-adrenoceptorbinding in POA and HYP (Fig. 1A). When the $alpha$ _1A- and $alpha$ _1B-adrenoceptorsubtypes were pharmacologically distinguished, POA and HYP membranesfrom saline-infused, E₂-treated females demonstrate a fourfoldto fivefold fold increase in $alpha$ _1B-adrenoceptor density when comparedwith OVX control animals (p < 0.05). The density of $alpha$ _1A-adrenoceptorsis not affected by E₂ treatment (Fig. 1B). Multiple intracerebroventricularinfusions of JB-1 prevent E₂ induction of $alpha$ _1B-adrenoceptor expressionin POA and HYP (Fig. 1C). Neither E₂ treatment nor infusions ofJB-1 affect the binding affinity of ³H-prazosin in POA and HYP membranes (Table 1).

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Figure 1. Effect of JB-1 infused into the third ventricle on E₂-induced $alpha$ _1B-adrenoceptor (AR) density in the POA and HYP. Membranes from POA and HYP were prepared from OVX control and E₂-treated (EB) female rats infused with saline or JB-1 as described in Materials and Methods. A, Total ³H-prazosin binding corrected for nonspecific binding reflects both $alpha$ ₁-AR subtypes. B, The $alpha$ _1A-AR population is measured after CEC inactivation. C, The $alpha$ _1B-AR population is determined by subtracting the binding of ³H-prazosin after CEC inactivation from total ³H-prazosin binding. B_max values were obtained by Scatchard analysis. The data presented are the means ± SEM from four independent replications. *p < 0.05.


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Table 1. Effects of JB-1 on ³H-prazosin binding affinity

E₂-induced LH surge is dependent on IGF-IR activity

Administration of E₂ to OVX female rats causes a daily LH surge (Caligaris et al., 1971). IGF-I can also affect LH releaseby altering gonadotropin-releasing hormone (GnRH) release fromthe HYP (Hiney et al., 1991; Soldani et al., 1994; Wilson, 1995;Hiney et al., 1996). We tested the hypothesis that steroid-inducedLH release requires IGF-IR activation. OVX rats were given oneof three hormone treatments (Oil, EB, or EB + progesterone; N= 4-8) and were infused every 12 hr with either JB-1 or saline.The estrogen priming consisted of two injections of EB (2 µg)24 and 48 hr before killing. Progesterone (500 µg) was injected44 hr after the first EB injection and 4 hr before killing. LHlevels in OVX rats are chronically elevated because of the lossof steroid negative feedback (Ortmann et al., 1988). Multipleintracerebroventricular infusions of JB-1 have no effect on theseelevated LH levels in OVX rats given no hormone replacement (Fig.2). Treatment of OVX, saline-infused rats with E₂ alone tendsto lower LH levels, but this effect is not statistically significant.However, LH levels in E₂-treated rats given multiple intracerebroventricularinfusions of JB-1 are significantly lower than in OVX controls(p < 0.05). Because this result does not conclusively indicateif blockade of IGF-IR activity enhances E₂ negative feedback orinhibits E₂ positive feedback on LH secretion, we treated OVXrats with both E₂ and progesterone. LH release is further enhancedwhen E₂-treated, OVX female rats are subsequently given progesterone(Caligaris et al., 1971). The administration of E₂ plus progesteronesignificantly increases LH levels when compared with OVX controls(p < 0.05). Intracerebroventricular infusions of JB-1 during estrogenpriming abolish the LH surge produced by administration of EBplus progesterone to OVX female rats (p < 0.05) (Fig. 2).

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Figure 2. Effect of JB-1 infused into the third ventricle on hormone-induced LH secretion. Serum for LH radioimmunoassay was prepared as described in Materials and Methods. OVX rats were given one of the following treatments: OIL, EB, or EB + progesterone (P). Multiple intracerebroventricular infusions of vehicle saline (SAL) or JB-1 were given 1 hr before the first EB injection and every 12 hr thereafter. The data presented are the means ± SEM from four to eight independent replications. *OIL + SAL, OIL + JB-1, EB + SAL, and EB + P + SAL (p < 0.05); **all other groups (p < 0.05), #OIL + SAL, OIL + JB-1, and EB + P + SAL (p < 0.05).

E₂-dependent sexual behavior is partially dependent on IGF-IR activity

To examine the possibility that E₂-dependent sexual behavior requires IGF-IR activity, E₂ plus progesterone-treated, OVX femalerats received multiple intracerebroventricular infusions of JB-1during estrogen priming. The E₂ priming dosages used in our experimentalparadigm are subthreshold for lordosis behavior; administrationof progesterone is required to facilitate sexual receptivity inthese animals (Pfaff et al., 1994). JB-1 modestly but significantly(p < 0.05) decreases lordosis behavior (Fig. 3A,B). Recently,acute intracerebroventricular infusion of IGF-I was shown to facilitatefemale sexual behavior independent of E₂ priming (Apostolakiset al., 2000). Therefore, we assessed whether acute JB-1 infusionto block IGF-IRs near the time of lordosis testing would inhibitthe behavior. Acute intracerebroventricular infusion of JB-1 ateither 12 hr (Fig. 3C) or 4 hr (LQ: saline = 70 ± 4.0; JB-1 =75 ± 2.9) before testing has no effect on lordosis behavior.

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Figure 3. Effect of JB-1 infused into the third ventricle on lordosis behavior of E₂- and progesterone-primed female rats. A, Lordosis quotient (LQ) after chronic infusions of saline (SAL) or JB-1 alone or JB-1 followed by intracerebroventricular infusion of 1 µg of 8-bromo-cGMP 4 hr before behavior testing. B, Quality of lordosis (QL) in same animals shown in A. Values presented are the means ± SEM (n = 9). *p < 0.05. C, LQ after acute infusion of 4 µg of JB-1 or SAL 12 hr before behavior testing. Values presented are the means ± SEM (n = 6).

A likely mechanism by which $alpha$ ₁-adrenoceptors facilitate female sexual behavior is by stimulating cGMP synthesis, which inturn activates protein kinase G (Chu and Etgen, 1999). For example,intracerebroventricular infusion of 8-bromo-cGMP 4 hr before lordosisbehavior testing reversed $alpha$ ₁-adrenoceptor antagonist inhibitionof lordosis behavior (Chu and Etgen, 1999). Thus, we examinedwhether the inhibitory effects of multiple intracerebroventricularinfusions of JB-1 on sexual behavior can be rescued by intracerebroventricularinfusion of 8-bromo-cGMP. During one of their three weekly tests,E₂-primed animals receiving multiple intracerebroventricular infusionsof JB-1 were infused with 1 µg of 8-bromo-cGMP at the time ofprogesterone injection. Intracerebroventricular infusion of 8-bromo-cGMPreverses the inhibitory effects of multiple intracerebroventricularinfusions of JB-1 on sexual behavior (p < 0.05) (Fig. 3A,B).

Blockade of IGF-IR during E₂ priming prevents E₂-dependent, IGF-I enhancement of NE-stimulated cAMP accumulation

We previously demonstrated that acute application of IGF-I enhanced NE-stimulated cAMP accumulation in POA and HYP slices,via modulation of $alpha$ ₁-adrenoceptor function, only if the animalis E₂-primed (Quesada and Etgen, 2001). The present study showedthat blockade of IGF-IR during estrogen priming prevents E₂-dependentincreases in $alpha$ _1B-adrenoceptor binding in the HYP and POA. We thereforeexamined the hypothesis that E₂-dependent, IGF-I modulation ofNE signaling in the POA and HYP of female rats requires IGF-IRactivation during E₂priming.

E₂-treated, OVX female rats received multiple intracerebroventricular infusions of JB-1 or saline every 12 hr during the 2d E₂ priming period. IGF-I enhances NE-stimulated cAMP accumulationin POA and HYP slices of E₂-treated female rats infused with saline.Multiple intracerebroventricular infusions of JB-1 abolish IGF-Ienhancement of NE-stimulated cAMP accumulation in POA and HYPslices of E₂-primed animals (Fig. 4). It is possible that residualJB-1 from the multiple intracerebroventricular infusions was presentin the slices and blocked IGF-I potentiation of NE-stimulatedcAMP accumulation. To determine if IGF-IRs could be activatedby application of IGF-I onto brain slices, phosphorylation ofERK1/2 in response to acute application of IGF-I onto slices fromJB-1 infused rats was monitored. The mitogen-activated proteinkinase cascade, including ERK1 and ERK2, are known downstreamsubstrates of IGF-IR activation (Zumkeller and Schwab, 1999).Figure 5 shows that multiple infusions of JB-1 do not interferewith the ability of acute IGF-I application to activate IGF-IRs,as measured by IGF-I-induced phosphorylation of ERK1/2 in HYPslices from E₂-treated rats.

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Figure 4. Effect of JB-1 infused into the third ventricle on E₂-dependent, IGF-I enhancement of NE-stimulated cAMP. POA and HYP slices from E₂-treated female rats were prepared from animals infused chronically with JB-1 or saline (SAL) as described in Materials and Methods. Slices were incubated for 15 min with 10 nM IGF-I followed by a 20 min incubation with 0.01 N HCl vehicle (VEH) or 100 µM NE. The PDE inhibitor 1 mM IBMX was included. The data presented are the means ± SEM from four independent replications. *VEH; **all other groups (p < 0.05).

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Figure 5. Effect of JB-1 infused into the third ventricle on acute IGF-I activation of extracellular receptor activated kinase 2 (ERK2). HYP slices from E₂-treated female rats were prepared from animals infused chronically with JB-1 or saline (Sal) as described in Materials and Methods and incubated for 15 min with 10 nM IGF-I or vehicle (Veh). Immunoblots were done using a monoclonal antibody for phosphorylated ERK1/2 (P-ERK1/2) and for total ERK2. Phosphotyrosine immunoblots were quantitatively analyzed by taking the ratio of the OD of the P-ERK2 band to the OD of the total ERK2 band. The immunoblot shown is representative of two independent experiments.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The data presented herein demonstrate that the positive feedback effects of E₂ on LH release require IGF-IR activity in thebrain and that E₂ priming of sexual receptivity also involvesIGF-I action. Present results also show that E₂-induced increasesin $alpha$ ₁-adrenoceptor binding and function in the HYP and POA requireIGF-IR activity. Thus, our findings provide the first evidencethat IGF-IRs in the brain are physiological mediators of multipleaspects of estrogen action on the hypothalamic-pituitary-gonadalaxis and sexualbehavior.

E₂ and IGF-I regulation of gene transcription

E₂ actions in the POA and HYP facilitate reproductive success by ensuring that the period of female sexual receptivity coincideswith the release of LH, which triggers ovulation (Pfaff, 1980;Etgen et al., 1992; Freeman, 1994). These effects of E₂ requiregene transcription and protein synthesis in target HYP-POA neuronsthat control reproductive function (Pfaff et al., 1994). We haveshown that E₂ increases $alpha$ _1B-adrenoceptor mRNA levels and bindingdensity in the HYP-POA (Petitti et al., 1992; Karkanias et al.,1996). We now demonstrate that chronic blockade of brain IGF-IRswith the competitive antagonist JB-1 prevents the E₂-induced increasein the density of $alpha$ _1B-adrenoceptor binding sites in the HYP andPOA. JB-1 treatment does not have nonspecific effects on brainNE receptors, because neither basal $alpha$ _1B-adrenoceptor nor $alpha$ _1A-adrenoceptordensities are affected by the drug. It is also unlikely that theactions of JB-1 are attributable to interference with other growthfactor signaling pathways (e.g., epidermal growth factor, platelet-derivedgrowth factor), because this peptide analog of IGF-1 does notblock the actions of other growth factors (Pietrzkowski et al.,1992).

The mechanism or mechanisms by which IGF-IR and E₂ interact to regulate $alpha$ _1B-adrenoceptor expression in the HYP-POA remainunknown, although there are several possibilities. Downstreammitogenic signals activated by IGF-IR may increase the expressionor transcription activating function of E₂ receptors (Aronicaand Katzenellenbogen, 1993; Stoica et al., 2000). Therefore, blockadeof IGF-IRs could result in downregulation of either the expressionand/or transcription activation function of E₂ receptors. Thispossibility is consistent with the observation that IGF-IRs arecolocalized with both E₂ receptor- $alpha$ and - $beta$ in neurons and gliain various brain regions, including HYP and POA (Cardona-Gomezet al., 2000). Alternatively, IGF-I may promote secretion of othertrophic factors or signaling molecules from HYP-POA glial cellsin an E₂-dependent manner, resulting in increased expression of $alpha$ _1B-adrenoceptor in the HYP-POA.

The increased expression of $alpha$ _1B-adrenoceptor in the HYP-POA, observed in response to E₂ treatment, is believed to mediatethe facilitatory component of NE action on sexual receptivityand LH secretion (Kow et al., 1992; Hosny and Jennes, 1998). Both $alpha$ _1B-adrenoceptor mRNA and protein are expressed in the POA andHYP (Blendy et al., 1990; Pieribone et al., 1994; Acosta-Martinezet al., 1999). In the POA, GnRH cell bodies show the highest densityof $alpha$ _1B-adrenoceptor-immunostaining, whereas GnRH nerve terminalsin the median eminence show moderate immunostaining (Hosny andJennes, 1998). Many cells and fibers in the arcuate nucleus-medianeminence, the site of GnRH release, demonstrate robust $alpha$ _1B-adrenoceptorimmunostaining (Acosta-Martinez et al., 1999). This is also theprimary neural site at which IGF-I and E₂ interact to regulatesynaptic plasticity (Fernandez-Galaz et al., 1999). The ventromedialHYP, the major site of E₂ facilitation of sexual receptivity,also contains both mRNA and protein for $alpha$ _1B-adrenoceptor (Pieriboneet al., 1994; Acosta-Martinez et al., 1999). Thus, E₂ regulationof the hypothalamic-pituitary-gonadal axis and sexual behaviormay involve IGF-IR-dependent increases in the expression of $alpha$ _1B-adrenoceptorsin target regions of the HYP-POA.

E₂ and IGF-I regulation of LH release

The ability of chronic JB-1 treatment to reduce E₂ and progesterone-dependent increases in plasma LH suggests that IGF-IRblockade suppresses estrogen positive feedback regulation of LHrelease. JB-1 treatment did not interfere with LH synthesis orrelease, because JB-1 infusion into OVX rats given no hormonereplacement does not reduce the elevated plasma LH levels observedin OVX rats. If JB-1 acts on pituitary gonadotropes to block LHsynthesis or secretion, LH levels in the OVX control rats infusedwith JB-1 should have been reduced. This was clearly not the case.Nonetheless, it is possible that treatment with the IGF-IR antagonistinfluenced pituitary sensitivity to GnRH. Future experiments couldevaluate this issue by measuring the LH response to exogenouslyadministered GnRH in JB-1-infusedanimals.

Although we cannot rule out the possibility that the IGF-IR antagonist interferes with progesterone action as well, it ismore likely that JB-1 acted primarily to interfere with estrogen-positivefeedback. First, progesterone facilitation of LH release requiresE₂ priming; in the absence of previous exposure to estrogen, progesteroneinhibits LH secretion (Freeman, 1994). Second, at the time bloodsamples were taken from E₂-treated rats infused with saline, plasmaLH levels were not significantly lower than in OVX control animals(Fig. 2). Blood was collected 48 hr after the first estrogen injection,~9 hr into the dark phase of the reverse light/dark cycle. Thus,it is likely that the LH values observed in E₂-treated, saline-infusedrats reflect positive feedback caused by estrogen alone. PlasmaLH levels in E₂-treated rats were significantly reduced by JB-1,suggesting that antagonism of IGF-IR activity influences estrogen-positivefeedback.

E₂-induced synaptic remodeling in the arcuate nucleus, which is also dependent on IGF-IR activity (Fernandez-Galaz et al.,1999), is believed to be critical for the preovulatory releaseof GnRH (Perez et al., 1993; Garcia-Segura et al., 1994). Thus,JB-1 treatment in our experimental paradigm may also inhibit E₂-inducedsynaptic remodeling in the arcuate nucleus, resulting in inhibitionof E₂-induced positive feedback on GnRH release, and ultimatelyinhibition of LH release. Our results add to an increasing bodyof evidence suggesting that IGF-I and E₂ work together to modulateLH secretion. Furthermore, they implicate the $alpha$ _1B-adrenoceptoras a mediator of E₂/IGF-I enhancement of gonadotropinrelease.

Interaction between IGF-I and E₂ may also be involved in changes in estrogen-negative feedback believed to be essential forthe initiation of female puberty. Peripheral administration ofIGF-I to OVX, adolescent female monkeys attenuates E₂ negativefeedback on LH release (Wilson, 1995). Likewise, intracerebroventricularadministration of IGF-I enhances LH release in both juvenile andperipubertal female rats, accelerating the initiation of puberty(Hiney et al., 1996).

E₂ and IGF-I regulation of reproductive behavior

IGF-IR blockade during E₂ priming partially attenuates E₂-dependent sexual behavior. The effects of JB-1 on lordosis are causedby blockade of IGF-IRs during E₂ priming rather than by residualJB-1 remaining in the brain after multiple infusions. This conclusionis supported by the observation that acute intracerebroventricularinfusion of JB-1 between 4 and 12 hr before behavior testing hasno effect on lordosis. We also showed that infusion of 8-bromo-cGMP,a cell-permeable analog of cGMP, reverses the partial inhibitionof sexual behavior induced by multiple intracerebroventricularinfusions of JB-1. This observation is in accordance with previousresults from our laboratory demonstrating that inhibition of sexualbehavior by systemic administration of an $alpha$ ₁-adrenoceptor antagonistis reversed by intracerebroventricular administration of 8-bromo-cGMP(Chu and Etgen, 1999). Moreover, administration of progesteroneto E₂-primed rat switches $alpha$ ₁-adrenoceptor signaling from phospholipaseC activation and potentiation of adenylyl cyclase activity tostimulation of nitric oxide-dependent activation of cGMP synthesis(Chu and Etgen, 1999; Chu et al., 1999). Hence, the ability of8-bromo-cGMP to rescue the partial inhibition of E₂-dependentsexual behavior by JB-1 indirectly suggests that interferencewith $alpha$ ₁-adrenoceptor signaling pathways may be responsible forthe observed lordosisinhibition.

There are several reasons why JB-1 may produce only partial attenuation of sexual behavior. First, It is possible that multipleintracerebroventricular infusions of JB-1 did not completely blockbrain IGF-IRs. Therefore, future experiments using higher dosesor constant intracerebroventricular delivery of JB-1 might producea more complete inhibition of lordosis. Second, JB-1 treatmentblocks the E₂-dependent increase of $alpha$ _1B-adrenoceptor binding withoutaffecting basal $alpha$ _1B-adrenoceptor in the HYP-POA. Hence, the remaining $alpha$ _1B-adrenoceptor present might be sufficient to support partialexpression of sexual behavior. Third, E₂ is thought to producemaximal sexual receptivity in part by induction of progesteronereceptor expression in the HYP (Mac-Lusky and McEwen, 1978; Blaustein,1982). Thus, JB-1 administration may have incompletely blockedE₂ induction of progesterone receptors in the HYP. Fourth, becausethe survival of species is dependent on successful reproduction,there are likely to be redundant neural elements (neurotransmitters,neurohormones and neuropeptides) on which E₂ and progesteroneact to coordinate reproductive physiology. Therefore, IGF-IRsmay mediate the actions of E₂ on only a subset of these neuraltargets of hormoneaction.

E₂ and IGF-I modulation of $alpha$ ₁-adrenoceptor signaling

Previously, we demonstrated that acute application of IGF-I onto HYP and POA slices in vitro enhances NE-stimulated cAMP accumulation,via $alpha$ ₁-adrenoceptor potentiation of adenylyl cyclase activation,only in E₂-primed female rats (Quesada and Etgen, 2001). We nowshow that blockade of IGF-IR activation during E₂ priming preventsboth the increased expression of $alpha$ _1B-adrenoceptors and IGF-I enhancementof NE-stimulated cAMP accumulation in the HYP and POA. Thus, theE₂-dependent effect of acute application of IGF-I on $alpha$ ₁-adrenoceptorsignaling, like E₂ induction of $alpha$ _1B-adrenoceptors and LH release,relies on brain IGF-IR activity during E₂ priming. The E₂ dependenceof IGF-I potentiation of NE-stimulated cAMP synthesis might beattributable to the induction of $alpha$ _1B-adrenoceptor expression inHYP and POA cells that also express IGF-IRs. Because in vitroapplication of IGF-I onto HYP slices from JB-1-infused rats inducesERK1/2 phosphorylation, the effects of JB-1 on NE signaling mustbe caused by blockade of IGF-IR during E₂ priming rather thanresidual JB-1 remaining in the brain after the multiple intracerebroventricularinfusions. In addition, E₂ can increase ¹²⁵I-IGF-I binding density (Quesada and Etgen, 2001) and IGF-IR contentin the HYP (Michels et al., 1993; Pons and Torres-Aleman, 1993;Wimalasena et al., 1993). Therefore, E₂ dependence of the interactionbetween IGF-I and NE may involve upregulation of IGF-IR, the $alpha$ _1B-adrenoceptororboth.

In summary, these data indicate that brain IGF-IR activity is necessary for long-term effects of E₂ on $alpha$ _1B-adrenoceptor expressionand function in the HYP and POA as well as for hormone-dependentsexual receptivity and positive feedback regulation of LH release.These results demonstrate a novel mechanism by which changes innoradrenergic signal transduction resulting from E₂ and IGF-Iaction in the brain control GnRH release and the expression ofreproductivebehavior.

  FOOTNOTES

Received Aug. 17, 2001; revised Dec. 21, 2001; accepted Jan. 8, 2002.

This work was supported by National Institutes of Health Grants R37 MH 41414, RO1 HD 29856, and T32 DK 07513 and by the Departmentof Neuroscience, Albert Einstein College of Medicine. We thankChioma Oyeamalu for technical assistance and Dr. Jorge Laroccafor critical review of this manuscript. The human IGF-I and antibodyfor rat LH were obtained through National Hormone and PituitaryProgram, National Institute of Diabetes and Digestive and KidneyDiseases, and Dr. A. F. Parlow (Harbor-UCLA Research and EducationInstitute).

Correspondence should be addressed to Anne M. Etgen, Department of Neuroscience, Albert Einstein College of Medicine, 1300Morris Park Avenue, Bronx, NY 10461. E-mail: Etgen{at}aecom.yu.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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