Suppression and recovery of estrous behavior in Syrian hamsters after changes in metabolic fuel availability

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Suppression and recovery of estrous behavior in Syrian hamsters after changes in metabolic fuel availability

Juli E. Jones and Laura S. Lubbers

Center for Neuroendocrine Studies, University of Massachusetts, Amherst, Massachusetts 01003-7720

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A reduction in the availability of oxidizable metabolic fuels inhibits reproduction. Forty-eight hours of metabolic fuel deprivationinhibits estrous behavior in ovariectomized, steroid-treated Syrianhamsters, but little is known about the time course of this inhibition.Likewise, refeeding reverses deprivation-induced suppression,but the rate of recovery has not been examined. In two experimentswe determined 1) the rate at which estrous behavior declines inhamsters treated with metabolic inhibitors and 2) how rapidlysexual receptivity is restored when hamsters are refed after a48-h fast. We also measured circulating levels of leptin and insulinin an attempt to determine their relationship to the inhibitionand restoration of estrous behavior. More than 24 h of metabolicinhibitor administration were required to inhibit lordosis, whereasonly 6 h of refeeding were sufficient to restore the display ofsexual receptivity to normal levels. Neither plasma insulin norleptin levels paralleled the changes in estrous behavior. We concludedthat 1) suppression of estrous behavior occurs more slowly thanrecovery after a fast and 2) changes in circulating leptin andinsulin probably do not have a critical role in these behavioralchanges.

methyl palmoxirate; insulin; leptin; food deprivation; 2-deoxy-D-glucose

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

ADEQUATE SUPPLIES OF METABOLIC fuels are necessary to sustain all of life's physiological processes, including reproduction.Because reproduction is exceedingly costly, especially for femalemammals, it is closely regulated by the availability of metabolicfuels. This becomes apparent when food is scarce, when an animal'sability to utilize metabolic fuels is inhibited, or when energyexpenditure exceeds intake. Under these conditions reproductionis interrupted (3, 17, 25, 32).

Syrian hamsters have become a useful model for studying the metabolic requirements for reproduction. Syrian hamster estrouscycles are highly sensitive to food deprivation; just 48 h offood deprivation on days 1 and 2 [estrus and diestrus (I)] ofthe cycle is sufficient to inhibit ovulation and estrous behavior(21). Estrous behavior also is suppressed in steroid-primedovariectomized hamsters that are deprived of food for 48 h (10).Similar to fasting, 48 h of treatment with inhibitors of glucoseand fatty acid oxidation [2-deoxy-D-glucose (2-DG) and methylpalmoxirate (MP), respectively] also suppresses estrous behaviorand ovulatory cycles (20, 27). These and other findings suggestthat suppression of estrous behavior is not related to the abundanceof body fat but rather to the ability to oxidize metabolic fuels(29, 32).

Nutritional infertility is due in part to a suppression of gonadotropin-releasing hormone (GnRH) and luteinizing hormone (LH)secretion. Reduced availability of metabolic fuels inhibits theLH surge and subsequently ovulation. Furthermore, in rats deprivedof food for 48 h (6) or given metabolic inhibitors (2),a decrease in mean plasma LH levels and LH pulse frequency andamplitude occurs. Conversely, pulsatile LH secretion resumes withinas few as 1-2 h after refeeding in previously food-deprived animals(4, 7, 9, 13, 23). Thus it is well established thatadministration of metabolic inhibitors and refeeding produce arapid termination and restoration of pulsatile LH secretion,respectively.

On the other hand, little is known about the time course of changes in estrous behavior following metabolic fuel manipulations.It is important to know this time course to further aid in investigatingthe neuroendocrine changes that are associated with the suppressionand restoration of estrous behavior. Therefore, the purpose ofthe first experiment was to determine how rapidly normal levelsof estrous behavior are attenuated after administration of metabolicinhibitors. We used pharmacological inhibitors (2-DG and MP),because they produce an immediate reduction in metabolic fueloxidation. This is in contrast to the metabolic consequences offood deprivation that develop gradually as the gut empties andother fuel sources diminish. This study focused on the first 24h after inhibition of metabolic fuel availability. The secondstudy examined the time course of recovery of estrous behaviorwhen hamsters are refed after a 48-h fast. One earlier paper fromthis laboratory (10) suggested that it took more than 48 h ofrefeeding to fully restore estrous behavior. In several previousattempts to replicate Dickerman et al. (10), we found that normallevels of lordosis were found in hamsters that were refed for24 or 48 h (data not shown). Hence, a further investigation usingtime points between 0 and 24 h of refeeding wasconducted.

Leptin and insulin appear to be involved in the control of reproduction (1). Circulating levels of leptin and insulin varyin proportion to the amount of adipose tissue, and it has beensuggested that circulating levels of these two metabolic hormonesmay signal the availability of metabolic fuels to the neural circuitscontrolling reproduction (1, 12, 16, but cf. 29). Another aimof these experiments was to determine physiological correlatesof the metabolic inhibitor-induced suppression of lordosis andthe refeeding-induced restoration of lordosis, beginning withcirculating levels of leptin and insulin. If these hormones playa crucial role in the suppression and recovery of estrous behavior,then the changes in their levels should precede the fluctuationsinlordosis.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Animals and housing. One hundred ten female Syrian hamsters (Mesocricetus auratus) weighing 80-100 g were obtained from Charles River BreedingLaboratories (St. Constant, Quebec). Animals were singly housedin wire-bottom, stainless steel cages (17.5 × 17.5 × 17.5 cm)in a room maintained at 22°C with a 14:10-h light-dark cycle (lightson at 0700). Hamsters were fed Purina Laboratory Chow (no. 5001)placed in hoppers mounted on the outside of the cages. Food andwater were available ad libitum except when indicated. All procedureswere approved by the University of Massachusetts InstitutionalAnimal Care and UseCommittee.

Surgery and behavioral testing. After a 1-wk period of adaptation to the laboratory, hamsters were anesthetized using pentobarbital sodium (80 mg/kg), supplementedwhen necessary with Metofane (methoxyflurane; Pitman-Moore, Mundelein,IL), and bilaterally ovariectomized. Two weeks following surgery,hamsters were primed with estradiol benzoate (EB, 2.5 µg sc, dissolvedin 0.1 ml sesame oil) followed 42 h later with progesterone (500µg sc, dissolved in 5% benzyl alcohol and 15% benzyl benzoatein 0.1 ml sesame oil) (8, 10, 20, 24, 31). Two weeksafter this priming regimen, all hamsters were given the same steroidtreatment. Six hours after progesterone injection, the animalswere placed with males and screened for sexualreceptivity.

Behavioral testing was conducted as follows. Each hamster was placed alone in a Plexiglas arena (30 × 36 × 30 cm) for 5 min.After the 5-min habituation to the testing chamber, a sexuallyexperienced male hamster was placed in the test chamber with thefemale for 3 min while the experimenter continually brushed thefemale's flanks with an artist's paintbrush to ensure that shereceived consistent tactile stimulation (24). The male was permittedto investigate and mount the female but not to intromit. Duringthis time, the amount of time that the female spent in lordosiswas recorded. The animals that did not display lordosis were removedfrom the study. The remaining animals were randomly placed intotreatment groups, counterbalanced for bodyweight.

Experiment 1. Two weeks after the screening test, 72 animals were given the same steroid-priming regimen before behavioral testing. Thetreatment groups were given metabolic inhibitors 0, 3, 6, 12,24, and 48 h before the behavioral test (Fig. 1). The inhibitor-treatedanimals were given 2-DG (750 mg/kg ip, in 0.15 M NaCl) and MPvia gavage (25 mg/kg suspended in 0.5% methyl cellulose). At thetime points when animals did not receive metabolic inhibitors,they were given both vehicles (0.15 M NaCl and 0.5% methyl cellulose).All animals were allowed to eat ad libitum. At the time of EBinjection, all animals began to receive both intraperitoneal (vehicleor 2-DG) and gavage (vehicle or MP) treatments every 6 h untilbehavioral testing. Administration of MP began 6 h before theonset of 2-DG administration. Immediately after behavioral testing,animals were killed by decapitation. Trunk blood was collectedand centrifuged, and plasma was frozen ( $-$ 22°C) until time of hormoneassay.

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Fig. 1. Experimental design. Top: lordosis termination. Five groups of ovariectomized hamsters were given metabolic inhibitors for 3, 6, 12, 24, or 48 h before testing for estrous behavior. One group (0 h) was not given metabolic inhibitors. All animals were treated with estradiol benzoate (EB, 2.5 µg) and progesterone (P, 500 µg). 2-DG, 2-deoxy-D-glucose; MP, methyl palmoxirate. Bottom: lordosis recovery. Five groups of ovariectomized hamsters were deprived of food for 48 h. Four groups were then refed for 3, 6, 12, or 24 h before testing for estrous behavior. One group (0 h) was not refed. A sixth group was fed ad libitum throughout the experiment.

Experiment 2. Two weeks after a behavioral screening test, a different set of 60 animals was given the same steroid-priming regimen as inthe first experiment. One group of hamsters was fed ad libitumthroughout the experiment, whereas the other five groups werefasted for 48 h and refed for either 0, 3, 6, 12, or 24 h priorto the behavioral test (Fig. 1). Immediately after behavioraltesting, animals were killed by decapitation and trunk blood wascollected and processed as in the firstexperiment.

Hormone assays. Plasma leptin levels were measured using the Linco Multi-Species Leptin RIA kit, XL-85K (St. Charles, MO). The leptin lower-detectionlimit was 2.0 ng/ml. Plasma insulin levels were measured usingthe Linco Rat Insulin RIA kit, FI-13K. The insulin lower-detectionlimit was 0.1 ng/ml.

Data analysis. All statistical analyses were carried out by one-way ANOVA. Significant differences at $alpha$ = 0.05 were followed with Fisher'sleast significant difference post hocanalysis.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Experiment 1: Suppression of lordosis. Forty-eight hours of metabolic inhibitor administration significantly reduced lordosis duration compared with animals givenmetabolic inhibitors for 0, 3, or 6 h, but not compared with animalsthat received inhibitors for 12 or 24 h [F(5,65) = 2.43, P < 0.05];yet the animals that received metabolic inhibitors for 12 or 24h were not significantly different from those that received inhibitorsfor 0, 3, or 6 h (Fig. 2). Metabolic inhibitor administrationdid not significantly affect either leptin [F(5,26) = 1.28, P> 0.3] or insulin levels [F(5,62) < 1; Fig. 3].

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Fig. 2. Effect of metabolic inhibitor administration on estrous behavior. Forty-eight hours of metabolic inhibitor administration significantly reduced lordosis duration compared with animals given metabolic inhibitors for 0, 3, or 6 h, but not compared with animals that received treatments for 12 and 24 h. Data shown as means ± SE for groups of 10 hamsters/group. Bars with different letters are significantly different from one another.

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Fig. 3. Effect of metabolic inhibitor administration on circulating leptin (top) and insulin (bottom) levels. Forty-eight hours of metabolic inhibitor administration affected neither leptin nor insulin levels significantly. Gray bars, groups showing significant suppression of lordosis. Data are shown as means ± SE for groups of 10 hamsters/group.

Experiment 2: Recovery of lordosis. Lordosis duration was significantly reduced following 48 h of food deprivation in EB- plus progesterone-treated hamsters.Lordosis duration remained suppressed after 3 h of refeeding.However, lordosis duration was not different from ad libitum-fedhamsters following 6, 12, and 24 h of refeeding [F(5,54) = 16.48,P < 0.001; Fig. 4]. Plasma leptin [F(5,54) = 4.14, P < 0.01] andinsulin [F(5,54) = 8.8, P < 0.001] levels were significantly reducedby 48 h fast. Insulin remained significantly reduced at all subsequenttime points. The same was true of leptin except at the 6-h refeedingtime point (Fig. 5).

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Fig. 4. Effect of refeeding on estrous behavior in food-deprived hamsters. Lordosis duration was significantly reduced after 48 h of food deprivation in EB- plus progesterone-treated hamsters (refed 0 h). There was no evidence of any recovery by 3 h of refeeding, but 6 h after food was returned recovery appeared to be complete. Data are shown as means ± SE for groups of 10 hamsters/group. Bars with different letters are significantly different from one another.

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Fig. 5. Effects of refeeding on circulating leptin (top) and insulin (bottom) levels in food-deprived hamsters. Plasma leptin and insulin levels were significantly reduced by a 48-h fast, but there was no evidence of any recovery even after 24 h of refeeding. Gray bars, groups showing significant suppression of lordosis. Data are shown as means ± SE for groups of 10 hamsters/group. Bars with different letters are significantly different from one another.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The results of these experiments indicate that 1) more than 24 h of metabolic inhibitor administration is necessary to suppressestrous behavior, 2) 6 h of refeeding is sufficient to restoreestrous behavior after a 48-h fast, and 3) neither circulatingleptin nor insulin levels are correlated with changes in expressionof estrous behavior under theseconditions.

More than 24 h of metabolic fuel restriction, whether due to food deprivation or metabolic inhibitor administration, was requiredto significantly suppress lordosis. This would suggest that thelong latency for food deprivation-induced suppression of lordosisis not due solely to a slowly developing metabolic cue. In monkeys,rats, and sheep, the metabolic consequences of 2-DG and MP treatmentaffect LH pulsatility very quickly (5, 7, 22), but forhamsters more than 24 h of treatment is still required for thesuppression of estrous behavior (Fig. 2). These results indicatethat the suppression of lordosis develops more slowly than theinhibition of pulsatile LH release. Thus it appears that the neuralmechanisms controlling GnRH (2) respond to metabolic cues muchmore rapidly than those controlling lordosis or else they respondto different cues, which make this process more rapid. Indeed,a number of neuropeptides that affect food intake, including neuropeptideY (8) and corticotropin-releasing hormone (Jones, unpublisheddata) can suppress lordosis within minutes in ad libitum-fed,steroid-primed hamsters. Thus the delay in suppression of estrousbehavior may lie in the very gradual processing of informationsomewhere between detection of the metabolic signals and the releaseof inhibitory neurotransmitters and/orneuropeptides.

In contrast to inhibition of estrous behavior, recovery is more rapid. Our results clearly demonstrate that estrous behaviorrecovers rapidly and abruptly following refeeding after a 48-hfast in female Syrian hamsters. There was no evidence of recoveryby 3 h of refeeding, but by 6 h lordosis duration had returnedto normal levels. This indicates that metabolic cues related torefeeding are detected and processed relatively quickly. This3- to 6-h latency to recovery is still somewhat slower than thelatency reported for resumption of LH pulses in other species(typically 1-2 h) (4, 13, 23). It is not clear whetherthis reflects differences in the neuroendocrine mechanisms controllingestrous behavior vs. pulsatile LH release. Another possibilityis that the longer latency for restoration of estrous behaviorcould be due to the absence of a postfast hyperphagia in Syrianhamsters (30) in contrast to other species, which were usedto study LH pulsatility (4, 23).

The fact that estrous behavior recovers rapidly in refed hamsters suggests that the physiological processes contributing toreinstatement of estrous behavior in food-deprived animals alsorespond rapidly and likely before restoration of body lipid orglycogen stores. Thus rapid recovery of estrous behavior aftera fast gives a relatively narrow temporal window in which to lookfor relevant neuroendocrinechanges.

Circulating levels of leptin and insulin vary in proportion to the amount of adipose tissue in the body, and it has been suggestedthat circulating levels of these two metabolic hormones may signalthe availability of metabolic fuels to the neural circuits controllingreproduction (1, 12, 16, but cf. 29). Receptors for leptin andinsulin are found in the central nervous system and other tissuesand have a role in the regulation of energy balance (16, 18).Animals with mutations of either the leptin or leptin receptorgenes are obese and infertile. Treatment of leptin-deficient animalswith exogenous leptin causes weight loss and restores some indexesof fertility (11, 28). In wild-type animals, leptin treatmentcan prevent some of the suppressive effects of food deprivationon reproduction. For example, in Syrian hamsters, administrationof leptin reverses the effects of food deprivation on estrouscyclicity, but it does not restore reproductive behaviors in food-deprived,ovariectomized animals treated with exogenous steroids (26,31). In fact, treatment with leptin intensified the inhibitionof estrous behavior in food-deprived hamsters, whereas it facilitatedfemale sexual behavior in ad libitum-fed hamsters (31).

Adequate levels of insulin also are required for normal fertility. Streptozotocin-treated diabetic female rats and hamstersare typically anovulatory and exhibit reduced behavioral responsivenessfollowing treatment with ovarian steroids (15, 20). Thesedeficits are corrected by insulin replacement (19, 20). Therefore,the presence of some level of both leptin and insulin is requiredfor normal estrous behavior. However, it is not at all clear whetherfluctuations in circulating levels of these two hormones withinthe normal physiological range play a crucial role in the controlof reproduction by foodavailability.

In the present experiments, circulating levels of leptin and insulin bore no consistent relation to levels of estrous behavior.Neither plasma leptin nor insulin levels decreased significantlywith administration of metabolic inhibitors. Moreover, plasmaleptin and insulin levels were not restored prior to recoveryof estrous behavior. In fact, leptin and insulin levels remainedlow even after 24 h of refeeding, long after estrous behaviorwas restored. Thus while the presence of some insulin and leptinis required for normal fertility in a number of species, maintenanceof fed levels of these two hormones does not appear to be requiredfor the expression of normal levels of estrous behavior in Syrianhamsters. These findings are consistent with previously publishedwork in both rats and hamsters (14, 31). However, these findingsdo not preclude a significant role for leptin and/or insulin signalingin the control of lordosis via changes in leptin and/or insulinneural receptorabundance.

During metabolic fuel deprivation there are myriad changes in neuroendocrine and/or metabolic function, and it is often difficultto determination the existence and direction of causality amongthese events. The gradual suppression of estrous behavior andits more rapid recovery following manipulations of metabolic fuelavailability provide a framework within which to study the neuroendocrinebases of the behavioral aspects of nutritional infertility. Alongwith previous work on the time course of changes in LH secretion,this information will aid in determining which physiological eventsplay a causal role in altering hormone secretion and estrous behavior.This step in that direction does not provide any support for acrucial role for physiological fluctuations in either insulinor leptinlevels.

	ACKNOWLEDGEMENTS

We thank George Wade, Eric Corp, Carrie Marín-Bivens, and Rebecca Pick for the helpful comments on a previous version ofthemanuscript.

	FOOTNOTES

This research was supported by Research Grant NS-10873-29, Senior Scientist Award MH-00321-20, and Institutional TrainingGrant MH-20051-01 from the National Institutes of Health and bypostdoctoral Research Grant 98-35203-6309 from the United StatesDepartment ofAgriculture.

Address for reprint requests and other correspondence: J. E. Jones, Center for Neuroendocrine Studies, Box 37720, Tobin Hall,Univ. of Massachusetts, Amherst, MA 01003-7720 (E-mail: jones{at}cns.umass.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 27 November 2000; accepted in final form 10 January 2001.

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