Granule Cells in Aging Rats Are Sexually Dimorphic in Their Response to Estradiol

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The Journal of Neuroscience, May 1, 1999, 19(9):3316-3325

Granule Cells in Aging Rats Are Sexually Dimorphic in Their Response to Estradiol
Phillippa Miranda¹^,², Christina L. Williams³, and Gillian Einstein¹^,²
¹ Department of Neurobiology and ² Joseph and Kathleen Bryan Alzheimer's Disease Research Center, Duke University Medical Center, Durham, North Carolina, 27710 and ³ Department of Psychology: Experimental, Duke University, Durham, North Carolina 27708

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Normal aging comprises cognitive decline, including deterioration of memory. It has been suggested that this decline in memoryis sexually dimorphic because of the cessation in gonadal steroidsecretion that occurs during reproductive aging in female, butnot male, mammals. We wondered whether neurons in brain regionsassociated with learning and memory underwent morphological changesthat were dimorphic as well and whether cessation of the secretionof gonadal steroids influenced these morphological changes. Toexplore these questions, we deprived and restored estrogens toyoung and old gonadectomized females and males and studied themorphology of dentate granule cells by intracellular dye fillingin a lightly fixed slice preparation. We found the following:(1) Aged female dentate granule cells deprived of gonadal steroidslong-term have a paucity of dendritic spines compared with youngfemales deprived short-term; however, aged male dentate granulecells deprived of gonadal steroids long-term have no decreasein dendritic spines compared with young males deprived short-term.(2) Aged female dentate granule cells with long-term estrogenreplacement at either high or low levels still had a decline inspine density. (3) Aged female dentate granule cells with short-termestradiol replacement had spine density increased to levels normallyobserved in young adults, whereas aged males with short-term estradiolreplacement had decreased spine density. These data suggest thatthe response of rat dentate granule cells to aging and estradiolis sexually dimorphic and that, in females, the responsivenessof granule cells depends on the temporal pattern of estradiolreplacement.

Key words: estrogens; aging; Alzheimer's disease; memory; dentate granule cells; hormone replacement therapy; dendritic spines; hippocampus; neuronal morphology

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Memory decline is associated with normal aging in both rodents and humans (Rissenberg and Glanzer, 1986; Chiarello and Hoyer,1988; Kadar et al., 1990; Youngjohn and Crook, 1993; Frick etal., 1995). In normal aging, female and male rat brains also undergostructural and functional changes, including loss and retractionof dendrites, spines, and myelin, as well as decreases in thedensity of receptor proteins and levels of neurotransmitters (Nunziet al., 1987; Moroi-Fetters et al., 1989; Garcia-Segura et al.,1991). It has been suggested that, in females, memory loss isexacerbated by the decline in gonadal estrogens, marking reproductivesenescence (rats) and menopause (humans) (Sulkava et al., 1985;Alliot and Giry, 1991). Conversely, replacement of estrogens protectsagainst decline in memory in normal aging, as well as in Alzheimer'sdisease (Paganini-Hill and Henderson, 1994; Kimura, 1995; Hendersonet al., 1996; O'Neal et al., 1996; Tang et al., 1996; Henderson,1997; Kawas et al., 1997; Sherwin, 1997). These data suggest thatthe decrease in gonadal steroids that accompanies normal agingin females may accelerate age-related cognitive decline by increasingthe structural and functional changes to neurons in brain regionsassociated with learning andmemory.

It is well established that estrogens can lead to an increase in neurite outgrowth, spine density, and synaptic input bothin vitro (Toran-Allerand, 1976) and in vivo (Woolley and McEwen,1992, 1993). Thus, we speculate that changes in estrogen availabilityand utilization by the brain of aging females enhances connectivitychanges in aging female brains. To explore this possibility, weasked the following. (1) What is the morphology of neurons inestrogen-deprived aging females and males? (2) Does estrogen replacementin gonadectomized animals change this morphology? (3) Do morphologicalchanges depend on the temporal pattern of estrogen replacement?We know already that, in the cycling female, CA1 pyramidal neuronsundergo synaptic remodeling over the course of the estrous cyclebut that under the same conditions dentate granule cells are unresponsive(Woolley and McEwen, 1992). However, because dentate granule cellslose spines quickly under other conditions, such as denervationcaused by aging and disease (Nadler et al., 1973, 1977; Whiteet al., 1979; Flood and Coleman, 1986; Flood et al., 1987; Einsteinet al., 1994; Shetty and Turner, 1995), we wondered whether theywould be responsive to estrogen deprivation and replacement inthe aginganimal.

In females, we mimicked different conditions of naturally occurring estrogen exposure during aging in humans and rats: "humanmenopause" by ovariectomizing female rats and providing no steroidreplacement; "constant estrus" (as in aging rats) by providinga constant high-dose estradiol replacement to ovariectomized rats;and "persistent diestrus" (as in very old rats) by providing aconstant low-dose estradiol replacement. Cyclical exposure toestrogens of young females was mimicked by injecting a short-termpulse of estradiol. In males, as comparison groups, we gonadectomizedand either left them in an androgen/estrogen-deprived state orgave short-term estradiol replacement. Dendritic morphology wasstudied by making intracellular dye injections in fixed brainslices (Einstein, 1988).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Twenty-five ovariectomized female and 14 gonadectomized male Charles River Sprague Dawley CD strain rats were used for thisstudy. Rats were housed in same-sex pairs in clear plastic cagesand were given food and water ad libitum. They were kept on a12 hr light/dark cycle with lights on at 7:30 A.M. All rats killedat 16-20 months of age were gonadectomized at 2 months of age,implanted with SILASTIC capsules filled with estradiol benzoate(EB) or oil, and behaviorally trained in an appetitively motivatedlearning paradigm at 3 months and again at 14 months of age (Williams,1996).

Animal surgery. Ovariectomies were performed on all the female, and castrations were performed on all the male rats. Theywere anesthetized with a mixture of xylazine (5 mg/kg) and ketaminehydrochloride (45 mg/kg). During the same surgery, different groupsof the females were implanted subcutaneously with the followingdoses of EB administered via SILASTIC capsule: (1) no estradiol,one 10 mm empty capsule (n = 8); (2) low estradiol, one 15 mmcapsule filled with a solution of 200 µg of EB/ml of sesame oil(n = 8); and (3) high estradiol, five 10 mm capsules filled witha solution of 200 µg of EB/ml of sesame oil (n = 4). The capsuleswere constructed using SILASTIC medical grade tubing (inner diameterof 0.147 cm, outer diameter of 0.196 cm), SILASTIC adhesive (DowCorning Corporation, Midland, MI), and round toothpicks. The tubingwas cut into 14 and 19 mm sections, and the ends were pluggedwith 2 mm of toothpick and an adhesive seal. None of the malesreceived EB implants. Estradiol levels were checked monthly (bloodwas taken from the tail vein under CO₂ anesthetic), and implantswere replaced every 3-4 months as necessary to maintain serumestradiol levels. Median serum estradiol levels for long-termreplacement were as follows: no estradiol, <20 pg/ml; low estradiol,27.7 pg/ml; and high estradiol, 42.95 pg/ml.

At 16-20 months of age, four of the females with no estradiol replacement, four of the females with low estradiol replacement,and three of the males with no estradiol replacement were injectedwith 10 µg of EB/0.1 ml of sesame oil at 48 and 24 hr before beingkilled. At the same time points, matched groups of female andmale rats were injected with an oil vehicle before beingkilled.

Another group of five female rats was ovariectomized, and eight male rats were gonadectomized at 4.5 months of age and killed3 weeks later. Forty-eight and 24 hr before being killed, threefemales and four males were injected with 10 µg of EB/0.1 ml ofsesame oil, and, at the same time, two females and four maleswere injected with an oilvehicle.

Preparation of tissue. All animals were killed by decapitation. The brains were removed immediately, cut in half along themidsagittal plane, and fixed in 4% paraformaldehyde in 0.1 M PBSfor 3 hr at room temperature. After 3 hr, the left hemispherewas removed from fixative and rinsed in 0.1 M PBS. Using a vibratome,sagittal sections of 300 µm thickness were cut through the entireleft hemisphere, collected in series in 0.1 M PBS, and storedin the refrigerator in preparation for intracellular injectionwith Luciferyellow.

Intracellular injections. Granule cells of the dentate gyrus were injected intracellularly with Lucifer yellow as describedpreviously (Einstein, 1988). Cell filling was performed undervisual control using epifluorescence. In all cases, at least threeslices through the dentate gyrus were injected per animal, with~10-15 granule cells injected per slice. To minimize any difficultiesin interpreting morphological changes, slices from the dorsalhippocampus were used consistently (Buterbaugh and Hudson, 1991).To minimize differences in the dendritic field size and branchingpatterns of the dentate granule cells caused by position withinthe cell layer, as well as the possibility of injecting interneurons,granule cells located in the outer one-third of the granule celllayer were also chosen consistently (Green and Juraska, 1985;Claiborne et al., 1990; Soriano and Frotscher, 1993). Neuronsin both the dorsal and ventral blades of the dentate were filledin approximately equal numbers and were analyzed separately, aswell astogether.

Data analysis. After injection, sections were rinsed in 0.1 M PBS and post-fixed overnight in 10% formalin solution in 0.1M PBS. Using a 4× objective and a drawing tube, the distributionof injected neurons on each slice was plotted, the number of neuronsinjected was counted, and the quality of intracellular fillingwas assessed. The tissue was placed in a solution of 25% sucrosein 0.1 M PBS for cryoprotection and resectioned at 60 µm on afreezing microtome. Sections were collected serially, mountedon gelatin-coated slides, air dried, and coverslipped with Krystalon(Diagnostic Systems, Webster,TX).

To ensure objectivity in our analysis, rats were killed, and brains were numbered by one of the coauthors; cell injections,drawing, and quantification of morphology was done by another.In addition, the drawings and data analysis were performed severalmonths after the intracellular injections. In this way, all quantificationof morphology was performed by experimenters who were blind tohormonecondition.

Approximately 50 granule cells were filled intracellularly per rat. The criteria for choosing neurons to analyze in detailwere as follows: (1) complete filling of dendritic tree out tothe hippocampal fissure; (2) brightness or complete penetrationof Lucifer yellow into dendrites and spines, as assessed at 160×;and (3) soma located in the outer one-third of the granule celllayer. By these criteria, many neurons were well filled; however,only four of the best filled neurons from each blade were drawnand analyzed per rat. If neurons branched into several 60 µm sections,their cell body and processes in each 60 µm section were drawnand reconstructed for analysis. One aged female with no estradiolreplacement and one young female with short-term estradiol replacementhad no filled neurons that met our criteria for analysis; therefore,these animals were excluded. We measured dendritic length andcounted the total number of varicosities and spines. Varicositieswere identified as small oval swellings, integral to the dendrite.Spines were identified as smaller rounded protuberances, eitherextending from the dendrite via a thin shaft or lying close toor just slightly above the plane of focus of the dendrite. Boththe density of varicosities and spines (number per micrometer)were calculated but kept separate so that the final spine countincluded no varicosities. An ANOVA (using the number of animalsin each treatment group as the n value) was used to assess theeffects of aging and estradiol exposure on various features ofneuronal morphology. Dendritic length was not compared acrosstreatment groups because dye injections in fixed slices occasionallyyield truncated dendritic trees because of either sectioning orlack of diffusion of the dye. Therefore, this parameter was beyondthe scope of themethod.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Over 1000 dentate granule cells in females and males were filled intracellularly. Injection of granule cells with Luciferyellow produced cell bodies and dendrites that were bright greenor yellow in color, with crisp edges and spines that were wellfilled (Fig. 1A-D). Because of the extremely small size of thecell bodies of granule cells (8-10 µm in diameter), multiple cellswere occasionally filled at one injection site. However, it wasstill possible under high magnification to identify dendritesas belonging to a single cell body. Lucifer yellow filling wascomplete enough to reveal qualitative differences in spine densityand morphology (Fig. 1B-D). In some animals, the dendrites carriedirregular swellings resembling varicosities (Fig. 1B,C).

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Figure 1. Photomicrographs of dentate granule cells from 16-month-old females filled with Lucifer yellow. A, Low magnification showing completeness of neuronal filling. Note that dendrites are filled to the boundary of the hippocampal fissure. B, C, High-magnification photomicrographs of proximal dendrites showing the level of detail observable by the intracellular filling at approximately the same level of the dendritic tree. Qualitative observation suggests that spine density under EB deprivation (B) or long-term replacement (C) is different from under short-term replacement (D). Arrows point to dendritic spines; asterisks mark varicosities. Scale bar in B also applies to C, D.

Morphology of granule cells in aged rats in reproductive senescence

To determine the morphology of dentate granule cells of female rats under various conditions of reproductive senescence, westudied filled neurons from aging females that had been deprivedof gonadal steroids for >12 months (mimicking human menopause)and those replaced with low and high concentrations of estradiol(mimicking rat persistent diestrous and constant estrous, respectively).Qualitative inspection of neurons from all three conditions revealeddendritic trees with a paucity of spines (Fig. 2A-C). Subsequentquantification of spine density revealed no significant differencein spine density between females that had been estrogen-deprivedand those that had received either form of long-term replacement(Fig. 2D).

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Figure 2. Camera lucida drawings and histogram demonstrating the relatively spine-poor state of 16- to 20-month-old female dentate granule cells and lack of observable difference in spine density between those with long-term estrogen deprivation and long-term estradiol replacement. A, Long-term deprivation. B, Long-term low-dose estradiol replacement. C, Long-term high-dose estradiol replacement. D, Histogram of spine density under each condition. Scale bar in C also applies to A and B. EB, Estradiol benzoate; GCL, granule cell layer; ML, molecular layer; PP, perforant pathway. Note that there is one boundary for the perforant pathway marked for all the drawn neurons, although the molecular layer varies in width across its full extent. This abbreviation for purposes of visual clarity makes some dendritic trees appear to not branch the full extent of the molecular layer. However, all illustrated neurons have branches that filled to the perforant pathway unless they are obviously truncated by the plane of section of the slice. This holds true for all figures that follow, as well. n = 4 for all conditions.

To determine whether there was a sex difference in the effects of aging with long-term steroid deprivation, we also examinedfilled dentate granule cells from aging males deprived of gonadalsteroids for >12 months. In contrast to the females, qualitativeinspection of neurons from aged males revealed dendritic treeswith no paucity of spines (Fig. 3). An ANOVA with sex as the independentvariable revealed a significant sex difference in spine densityof granule cells of long-term gonadectomized rats (F_(1,4) = 11.04;p < 0.05).

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Figure 3. Camera lucida drawings and histogram showing an observable spine density in 16- to 20-month-old female and male dentate granule cells with long-term estrogen deprivation. A, Female dentate granule cell. B, Male dentate granule cell. C, Histogram of spine density for females and males. n = 4 for all conditions.

Morphology of granule cells in aged rats with short-term replacement of estradiol

To determine whether dentate granule cells from aged rats might be responsive to a pulse of estradiol, we compared the morphologyof dentate granule cells from aged, long-term gonadectomized maleand female rats that received short-term estradiol replacementwith rats that received control oil injections. Qualitative inspectionof neurons from aged females revealed that rats with short-termestradiol replacement had granule cells with full spiny dendritictrees compared with those with no replacement (Fig. 4A,B,E). Incontrast, qualitative inspection of granule cells of male ratsrevealed less spiny dendritic trees in the estradiol-replacedmales compared with those with no replacement (Fig. 4C,D). A two-wayANOVA with sex and short-term EB treatment as factors revealedno significant effects of either treatment or sex but did reveala significant interaction between sex and EB treatment (F_(1,9)= 11.333; p < 0.005). Short-term estradiol replacement also increasedthe spine density of neurons from females that had received long-termreplacement of low doses of EB. Qualitative inspection of thesegranule cells revealed fully branching dendritic trees with manyspines (Fig. 5C,D). Quantitative analysis of spine density revealedthat short-term EB replacement increased dendritic spine densityregardless of previous long-term EB exposure (Fig. 5E). A two-wayANOVA with short-term and long-term EB replacement as factorsrevealed no significant effect of long-term treatment alone andno interaction between long-term and short-term EB replacement.It did reveal a significant effect of short-term EB replacement(F_(1,11) = 17.268; p < 0.005).

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Figure 4. Camera lucida drawings and histogram showing dimorphic response of dentate granule cells in 16- to 20-month-old females and males that have been deprived of estrogens long-term and replaced with estrogens short-term. A, Long-term deprivation, females. B, Short-term estradiol replacement, females. C, Long-term deprivation, males. D, Short-term estradiol replacement, males. E, Histogram of spine density under each condition. Scale for A-D is the same. EB, Estradiol benzoate; GCL, granule cell layer; ML, molecular layer; PP, perforant pathway. n = 4 for all conditions, except short-term replacement for the males for which n = 3.

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Figure 5. Camera lucida drawings and histogram showing that after ovariectomy at 2 months of age, dentate granule cells in 16- to 20-month-old females respond to short-term replacement of estrogens whether they have been deprived of estrogens long-term or had low levels of long-term EB replacement. A, Estrogen-deprived state. B, Short-term EB replacement after estrogen deprivation. C, Long-term low-estradiol replacement. D, Short-term estrogen replacement after long-term low-estradiol replacement. Note how spine density increases after short-term replacement regardless of whether the neurons are deprived or have long-term low-dose replacement. E, Histogram of spine density. Scale for A-C is the same. ST, Short-term; LT, long-term; EB, estradiol benzoate. n = 4 for all conditions.

When we examined spine densities of granule cells from the dorsal and ventral blades of the dentate gyrus separately, we foundthat EB replacement appeared to increase spine density in femalesmainly in the neurons of the dorsal blade (Fig. 6). A two-wayANOVA on spine densities of dorsal blade cells only also revealedno significant effect of treatment or sex but did reveal a significantsex by EB treatment interaction (F_(1,9) = 7.515; p < 0.05). Thesame analysis run on ventral blade neurons revealed no significantmain effects or interactions.

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Figure 6. Histograms of spine density of dentate granule cells of 16-month-old females and males in dorsal and ventral blades with long-term estrogen deprivation and short-term replacement. A, Spine density of granule cells in the dorsal blade. B, Spine density of granule cells in the ventral blade. Note that whereas the effect in the females is carried primarily by the dorsal blade, the effect in the males is carried by both the dorsal and ventral blades. n = 4 for all conditions, except short-term replacement for the males for which n = 3.

Varicosities were counted separately from spines; age nor treatment nor sex influenced the number or density of varicositiessignificantly. There were also no significant correlations betweenvaricosities and spine density acrossconditions.

Interaction of aging and short-term replacement of estradiol

To determine whether there was an interaction between aging and short-term estrogen replacement, we compared the spine densityof dentate granule cells in young female and male rats gonadectomized3 weeks before being killed with granule cells from aged femalesand males gonadectomized 14-28 months before being killed. Wefound that dentate granule cells from young females deprived ofgonadal steroids for only a few weeks were noticeably spinierthan then those from aged females that had suffered long-termdeprivation (Fig. 7A,C). In fact, short-term EB replacement appearedto return dendritic spine density in aged ovariectomized femalesto that of the younger ovariectomized females (Fig. 7A,D). Incontrast to the aged females, the spine density of dentate granulecells in young females was not altered by ovariectomy or EB replacement(Fig. 7A-D). Quantification supported these qualitative observations;a two-way ANOVA with age and EB replacement as factors revealedno significant effect of age or short-term EB replacement on granulecell spine density. However, there was a significant interactionbetween age and short-term EB replacement (F_(1,8) = 7.109; p <0.05) (Fig. 7E).

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Figure 7. Camera lucida drawings and histogram showing that dentate granule cells in females ovariectomized at 4.5 months do not respond to short-term EB replacement at 5 months of age, whereas 16- to 20-month-old females ovariectomized at 2.5 months do respond to short-term EB replacement. A, Estrogen-deprived young adult. Note the full spiny dendritic tree. B, Young adult with short-term estradiol replacement. Note that there is relatively little change in spine density compared with A. C, Aged adult, estrogen-deprived. Note the paucity of dendritic spines. D, Aged adult, short-term EB replacement. Note the dramatic increase in spine density compared with C. E, Histogram of spine densities. Scale bar in D also applies to A-C. ST, Short term; LT, long-term; EB, estradiol benzoate. n = 4 for all conditions, except short-term replacement for the females for which n = 3.

In contrast, in males, dentate granule cells from young rats deprived of androgens for only a few weeks were not noticeablydifferent from granule cells of aged rats that had suffered long-termandrogen deprivation (Fig. 8). Visual inspection revealed thatshort-term EB replacement tended to decrease spine density slightlyin both young and aged rats, but the effect of EB replacementwas significant only in the aged male rats (F_(1,4) = 14.06; p< 0.05).

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Figure 8. Histogram showing that dentate granule cells in males gonadectomized at 2.5 months show a decrease in spine density at both 5 months and 16-20 months after short-term EB replacement. EB, Estradiol benzoate. n = 4 for all conditions, except short-term replacement in the older males for which n = 3.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We investigated the effects of estrogen deprivation and replacement on dentate granule cells in aged long-term gonadectomizedfemale and male rats. This work emerges from the important observationof Woolley and McEwen (1992) that the spine density of apicaldendrites of CA1 pyramidal neurons changes over the 4 d periodof the rat estrous cycle. Our new approach was to focus on theeffects of estrogen deprivation and replacement on the aging brain,to examine a different neuronal population, and to compare responsesof females and males. We found the following. (1) Aged femalesdeprived of gonadal steroids long-term have a paucity of dendriticspines on hippocampal granule cells compared with young femalesdeprived for the short-term; however, aged males deprived of gonadalsteroids long-term show no decrease in dendritic spines comparedwith young males deprived for the short-term. (2) No differencein spine density exists between females that suffered long-termdeprivation and those exposed to long-term replacement of bothhigh and low doses of EB. (3) Short-term estradiol replacementto aged female rats increases spine density of hippocampal granulecells to levels observed in young adults and decreases spine densityin agedmales.

We used intracellular dye injections that revealed dendritic morphology in as much detail as Golgi methods (Gould et al.,1990a,b; Woolley et al., 1990; Woolley and McEwen, 1992). Othershave also found dye filling to be a method that allows completedocumentation of changes in spine density in response to estradioladministration (Woolley et al., 1997). Although our spine densitiesare in the range of those reported in other studies (Hama et al.,1989; Trommald et al., 1995), absolute numbers of dendritic spineswill always remain in question because sex and treatment of theanimals differ between studies. For technical reasons alone, spinenumbers vary from study to study depending on whether or not correctionvalues are used (Feldman and Peters, 1979) and which morphologicalmethod is used. In this study, all the drawing and spine countswere performed by one person (P.M.), ensuring consistent intrastudyvalues and allowing us to demonstrate changes in relativedensities.

We demonstrate that, in aged females that have been ovariectomized for many months, acute estradiol administration quickly(in <48 hr) increases granule cell spine density. This is surprisingbecause, in young females, dentate granule cells (in contrastto CA1 pyramidal neurons) do not respond rapidly to estradioladministration or to the natural fluctuation of hormones duringthe estrous cycle (Gould et al., 1990b; Woolley and McEwen, 1992,1993, 1994; present report). These results demonstrate that theaged hippocampus is still rapidly responsive to acute changesin the hormonal milieu. Whether it is aging and/or estrogen deprivationthat increases estradiol responsivity in this neuronal populationremains to be determined. However, we have found that after ovariectomyof 5-month-old rats, spine density of granule cells declines veryslowly over months, not days, suggesting that in young femalesgranule cell spine density is not maintained by circulating estradiol(C. Cullen, C. Williams, and G. Einstein, unpublishedobservations).

Our finding that chronic long-term estradiol replacement in females results in the same decrease in dendritic spine densityas complete estrogen deprivation suggests that responsivity ofneurons to estrogen requires a cyclical or pulsatile exposure.This is an intriguing finding because it suggests that the commonfeature of hormonal aging in rats and humans is that the agingfemale is no longer exposed to cyclical changes in ovarian secretions.Human females experience many years of estrogen deprivation aftermenopause, whereas rats undergo a stage of constant estrus whenestrogen levels are constant but high and then persistent diestruswhen estrogen levels are constant and low (Lefevre and McClintock,1988). Given our results, it is possible that if aging femalerats were to continue to cycle regularly or to receive cyclicalestradiol replacement, spine density of the granule cells wouldbe maintained into old age. In fact, our finding that short-termestradiol replacement increases spine density in dentate granulecells of long-term ovariectomized aged female rats demonstratesthat these neurons are still responsive to estrogen, but theirresponsiveness depends on the pattern of estrogen exposure. Whetherdentate granule cells of aged females would undergo remodelingunder conditions that mimic ovarian hormone cycling remains tobedetermined.

The pattern of response of dentate granule cell spines to gonadectomy and estrogen replacement is quite different in agedmale rats. Aged males do not show an age-related decline in granulecell spines after long-term gondectomy, and in response to short-termestradiol replacement spines are lost, suggesting that femalesand males age differently on the neuronal level. This sexuallydimorphic response may be programmed by developmental history.Neurons in the ventromedial hypothalamus also show this same typeof dimorphism; replacing estradiol in gonadectomized females increasesspine density, whereas it decreases spine density in males (Lewiset al., 1995). Thus, depending on sex, neurons in different brainregions may have similar responses to estradiol replacement, reflectingthe difference in developmental plan between female andmale.

What is the mechanism by which a previously unresponsive neuronal type becomes responsive? Although estrogens can act to altergene transcription (McEwen et al., 1978), it is unlikely thatthis is the case in the present study because in the hippocampus,both $alpha$ - and $beta$ -estrogen receptors have been identified on interneuronsand glial cells and not on dentate granule cells (Rainbow et al.,1982; Loy et al., 1988; Pelletier et al., 1988; Weiland et al.,1996; Kuiper et al., 1997; Li et al., 1997). Estradiol might actdirectly on membranes, altering their properties to induce glutamaterelease, thus increasing intraneuronal calcium, stimulating NMDAreceptors, leading to the addition of dendritic spines (Parpuraet al., 1994; Woolley and McEwen, 1994; Klintsova et al., 1995).Estradiol might also affect dentate granule cells via astrocytes(Klintsova et al., 1995). The explanation we favor, however, isthat estrogen may be acting indirectly on neurons projecting todentate granule cells, such as entorhinal cortical or basal forebrainneurons that are known to have estrogen receptors (Pfaff and Keiner,1973; Loy et al., 1988; Weiland et al., 1996). Such sensitivityto denervation and reinnervation would not be unusual for dentategranule cells and is reminiscent of their quick loss of spinesbecause of loss of inputs during aging or disease (Nadler et al.,1973, 1977; White et al., 1979; Flood and Coleman, 1986; Flood,1987; Einstein et al., 1994; Shetty and Turner, 1995). Our findingthat the brunt of the effect is carried by neurons of the dorsalblade further supports the hypothesis that responsivity to estrogensis caused by denervation-innervation effects because granule cellsin the dorsal and ventral blades have been shown to differ inboth morphology (Claiborne et al., 1990) and inputs (Amaral andWitter, 1995).

The functional ramification of increased or decreased spine density is still an open question. It has been shown in male rodentsthat spine density and number of excitatory synapses correlatewith the efficiency of learning spatial tasks (Moser et al., 1994).Direct correlation of changes in spine density with changes insynaptic density suggests that, at the very least, changes inspine density reflect changes in excitatory input (Westrum andBlackstad, 1962; Calverley and Jones, 1990; Jaslove, 1992; Woolleyand McEwen, 1992); by the same token, decreases in spine densityprobably reflect a loss of excitatory inputs and thus a decreasein neuronal excitability. Exacerbation of spine loss by estrogendeprivation in normal aging suggests that the estrogen-deficientstate after human menopause is one of decreased excitatory synapticinput, which may contribute to cognitive decline in aging andAlzheimer's disease-affectedwomen.

It also suggests that recently reported positive effects of hormone replacement therapy, such as the reversal of normal memorydecline in elderly women (Henderson, 1994), the delay in the ageof onset of Alzheimer's disease (Paganini-Hill and Henderson etal., 1994; Kawas et al., 1997), and the amelioration of cognitivedecline in Alzheimer's disease (Fillit et al., 1986; Ohkura etal., 1994a,b; Birge, 1997), may be mediated through structuralchanges of hippocampal neurons. Our data suggest that administeringestrogens in a cyclic manner in humans might strengthen neuronalconnectivity, which might lead to cognitive enhancement. Thisnewly discovered rapid plasticity in the female brain may haveimplications for the protection of neurons in Alzheimer's disease,as well as for our conception of the relative effects of agingon the female and malebrain.

  FOOTNOTES

Received Nov. 12, 1998; revised Jan. 25, 1999; accepted Feb. 10, 1999.

This work was supported by American Foundation for Aging Research (to P.M.), National Institutes of Health (NIH) Grant AG09525(to C.L.W.), NIH Grant P50AG05128 (Project 2), and Alzheimer'sAssociation Grant IIRG-95136 (to G.E.). We thank Laurie Kenningtonfor her technical assistance and Dr. Anthony LaMantia for helpfulcomments on thismanuscript.
Correspondence should be addressed to Gillian Einstein, Box 3209, Duke University Medical Center, Durham, NC27710.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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