Ovariectomy of Adult Rats Leads to Increased Expression of Astrocytic Basic Fibroblast Growth Factor in the Ventral Tegmental Area and in Dopaminergic Projection Regions of the Entorhinal and Prefrontal Cortex

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The Journal of Neuroscience, October 1, 1999, 19(19):8665-8673

Ovariectomy of Adult Rats Leads to Increased Expression of Astrocytic Basic Fibroblast Growth Factor in the Ventral Tegmental Area and in Dopaminergic Projection Regions of the Entorhinal and Prefrontal Cortex
Cecilia Flores, Natalina Salmaso, Sean Cain, Demetra Rodaros, and Jane Stewart
Center for Studies in Behavioral Neurobiology, Department of Psychology, Concordia University, Montréal, Québec, Canada H3G 1M8

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Changes in astrocytic function may underlie the neurochemical and morphological alterations in limbic and cortical areas afterestrogen loss in adult females. We assessed whether increasedexpression of basic fibroblast growth factor (bFGF), an astrocyticresponse involved in injury-induced neuronal plasticity, occursafter ovariectomy. We examined bFGF immunoreactivity (IR) in ovariectomizedrats with oil or estradiol benzoate (5 µg every 4 d; Experiment1) and in ovariectomized and intact animals (Experiment 2). Inthe ventral tegmental area (VTA), bFGF-IR and glial fibrillaryacidic protein (GFAP)-IR were greater in ovariectomized animalsthan in animals with estrogen replacement. bFGF-IR in the VTAwas greater in ovariectomized than in intact females. In the dorsalraphe, no differences between groups were found in GFAP-IR orbFGF-IR. In mesolimbic dopaminergic target areas within entorhinalcortex (Ent), prefrontal cortex, and nucleus accumbens, bFGF-IRwas higher in Ent of ovariectomized animals 4 weeks after surgeryin both experiments, but no differences were seen in nucleus accumbensor in an occipital cortical, control, area in either study. InExperiment 2, small increases in bFGF-IR were seen in the prefrontalcortex after ovariectomy. In the VTA and Ent, changes in bFGF-IRdeveloped gradually, peaking at 4 weeks and waning at 40 weeks.Furthermore, increased dendritic arbor of Ent layer II/III pyramidalcells was found in ovariectomized females with the use of a modifiedGolgi-Cox staining procedure. These findings suggest that, withinspecific regions, ovariectomy induces astrocytic responses similarto those observed after injury that may affect neuronal chemistryandmorphology.

Key words: estrogen; astrocytes; bFGF; ventral tegmental area; entorhinal cortex; prefrontal cortex; dendritic arbor; Golgi; GFAP

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Estrogens have widespread influence on affective and cognitive functioning in adult females. Estrogens and their loss havebeen implicated in mood changes (Fink et al., 1996) and memory(Sherwin, 1997) as well as in mental disorders (Gregoire et al.,1996; Henderson, 1997; Lindamer et al., 1999). Ovariectomy hasbeen associated with morphological and neurochemical changes incortex and hippocampus. In rats, ovariectomy leads to rapid decreasesin dendritic spine density of hippocampal CA1 pyramidal cellsthat are prevented by estradiol (E2) (Gould et al., 1990). Theseeffects appear to be mediated indirectly via changes in glutamatergictone (Woolley and McEwen, 1994) through E2 actions on brain-derivedneurotrophic factor and GABAergic activity (Murphy et al., 1998a,b).In contrast, increased dendritic branching and spine density ofparietal cortex pyramidal cells are observed in long-term ovariectomizedrats (Stewart and Kolb, 1994), effects similar to those seen afterearly injury to adjacent cortical regions and to noradrenergicinputs (Kolb et al., 1997). These findings suggest that changesin cell morphology induced by ovariectomy could result from theloss of estrogenic actions on cells that innervate the affectedcells, causing compensatory reactions in the target cells to changesin previous patterns of input. In fact, estrogen loss resultsin reduced cholinergic activity in cortex and hippocampus (Luine,1985; Singh et al., 1994), and such effects probably are mediatedby alterations in the effects of neurotrophins on cholinergiccells of the basal forebrain (Toran-Allerand et al., 1992; Sohrabjiet al., 1995; McMillan et al., 1996; Gibbs, 1998).

Ovariectomy induces changes in other systems that have widespread influence on the cortex, such as the midbrain dopaminergicand serotonergic systems. In adult monkeys, long-term ovariectomydecreases dorsal raphe tryptophan hydroxylase but increases 5-HT1Areceptor and transporter mRNA expression (Pecins-Thompson et al.,1996, 1998; Pecins-Thompson and Bethea, 1999) and substantiallyreduces tyrosine hydroxylase-immunoreactive fiber density in thecortex (Kritzer and Kohama, 1998). In rats, ovariectomy decreases5-HT2A receptor mRNA expression and binding (Fink and Sumner,1996; Fink et al., 1996) and dopamine receptor binding (Bosséand Di Paolo, 1996). Furthermore, the behavioral and neurochemicaleffects of drugs that act directly on dopaminergic neurons aredecreased after ovariectomy (Camp et al., 1986; Robinson, 1988;Becker, 1990; Castner et al., 1993; Forgie and Stewart, 1993,1994; Stewart and Rodaros, 1999).

Recent evidence shows that estrogens are neuroprotective (Dluzen et al., 1996; Dluzen, 1997; Green et al., 1997), suggestingthat their loss might induce responses seen after minor injury.Estrogen loss and replacement affect astrocytic activity (Luquinet al., 1993), and the effects of estrogens on neuronal functionmight be mediated in part via their actions on astrocytes (García-Seguraet al., 1994, 1996). Interestingly, astrocytic expression of basicfibroblast growth factor (bFGF) is increased in midbrain dopaminecell body regions after injury to dopaminergic cells (Chadi etal., 1994) and after repeated injections of psychostimulant drugs(Flores et al., 1998). Thus, because of the sensitivity of themonoamine systems to estrogen loss and replacement, we hypothesizedthat, after ovariectomy, astrocytes in cell body and/or targetregions of these systems might show changes in bFGF expressionsimilar to those seen in response to stress, drugs, or minor injury.In addition, we speculate that these changes may be related tothe morphological changes in cortical regions that are seen afterestrogenloss.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects
Female Wistar rats (Charles River, St. Constant, Québec) 80-90 d of age at the time of surgery served as subjects in Experiments1, 2, and 3. All animals were maintained in a temperature- andhumidity-controlled environment under a 12 hr light/dark cyclewith free access to food andwater.

Hormones and antibodies
Estradiol benzoate (EB; Sigma, St. Louis, MO), was dissolved in peanut oil and injected subcutaneously at a dose of 5 µg/0.1ml per animal or, as in Experiment 4, 10 µg/0.1 ml per animal.bFGF immunoreactivity was detected by using a mouse monoclonalantibody (Upstate Technology, Lake Placid, NY) that recognizesthe biologically active isoform of bFGF (Matsuzaki et al., 1989).The antibody was used at a concentration of 1:500. A mouse monoclonalantibody (Sigma), at a concentration of 1:500, was used to identifyglial fibrillary acidic protein (GFAP) immunoreactivity; a rabbitpolyclonal antibody (Eugene Tech, Ramsay, NJ), at a concentrationof 1:2000, was used for tyrosine hydroxylase (TH)immunolabeling.

Immunohistochemistry
Animals were anesthetized deeply with sodium pentobarbital (120 mg/kg) and perfused transcardially with 200 ml of cold PBS,followed by 100 ml of a cold solution of 4% paraformaldehyde (w/v)and 15% picric acid (v/v) in phosphate buffer (PB; pH 6.9). Brainswere removed and stored overnight in the fixative solution at4°C. Coronal 50 µm sections were cut by vibratome and stored overnightin PB at 4°C. In Experiment 1, adjacent brains sections were processedfor GFAP or bFGF immunohistochemistry (in Experiment 2, only forbFGF) by using the ABC method (Hsu et al., 1981). Free-floatingsections were incubated for 24 hr at 4°C with the anti-bFGF oranti-GFAP antibody diluted 1:500 with 0.3% Triton X-100 (Sigma)in PB and 1% normal horse serum (Vector, Burlingame, CA). Thenthe sections were rinsed (three times for 5 min) in cold PB andincubated for 1 hr at room temperature in a solution of rat adsorbedbiotinylated anti-mouse antibody (Vector) diluted 1:200 with PBand 1% normal horse serum. After washings (three times for 5 min)in cold PB, the sections were incubated in an avidin-horseradishperoxidase complex (Vectastain Elite ABC Kit, Vector) for 30 minat room temperature and rinsed again (three times for 5 min) incold PB. Next the sections were incubated for 10 min at room temperature,and, under constant agitation, in a solution of 0.05% 3,3'-diaminobenzidine(Sigma) in PB. Then, without washing, the sections were transferredto a 3,3'-diaminobenzidine/PB solution, pH 7.8, with 0.01% H₂O₂to catalyze the reaction and with 8% NiCl₂ to darken the reactionproduct. This incubation was terminated 8 min (bFGF-treated sections)or 3 min (GFAP-treated sections) later by washing the sections(three times for 10 min) with coldPB.
Double labeling for bFGF-GFAP and for bFGF-TH was obtained by processing the sections, first, for bFGF immunoreactivity andthen for either GFAP or TH immunoreactivity, using the ABC method.For TH immunoreactivity the sections were preincubated in 0.3%Triton X-100 PB and 1% normal goat serum for 1 hr at room temperature.For both GFAP and TH immunoreactivity no NiCl₂ was added to the3,3'-diaminobenzidine-PB-H₂O₂ solution to obtain a lighter reactionproduct.
Sections were mounted on gelatin-coated slides, dried for at least 1 d, hydrated in distilled water (1 min), and graduallydehydrated in 70, 90, and 100% ethanol. Slides then were clearedin Hemo-De and coverslipped with Permount. To reveal anatomicallandmarks, we lightly counterstained midbrain sections for Nisslsubstance by using 0.1% cresyl violet. This latter step was notdone in double-labeledtissue.

Image analysis
Immunostained sections were observed under a Leica microscope (Leitz DMRB, Wetzlar, Germany). Quantitative analysis was performedvia an image analysis system (National Institutes of Health Image1.6) on digitized images of sampling areas of the dorsal raphenucleus (DR), ventral tegmental area (VTA), nucleus accumbens(NAcc) shell and core, entorhinal cortex (Ent) layer II, medialprefrontal cortex (PFC) layer II of the supragenual cingulatecortex area 2, and occipital cortex area 2 mediolateral (Oc2)layers V and VI. Boundaries of cortical and subcortical structureswere defined by using as a guide Zilles (1985) and Paxinos andWatson (1997), respectively. Sampling areas of the DR were takenfrom sections corresponding to plates 47, 49, and 51; of the VTA,Ent, and Oc2 from sections corresponding to plates 38 and 39;of the NAcc from sections corresponding to plates 11, 12, and13; and of the PFC from sections corresponding to plates 14 and15 (Paxinos and Watson, 1997). Images for each structure (labeledwith either bFGF or GFAP) were taken from three sections fromeach brain; they were digitized and assigned codenames.
GFAP-immunoreactive surface density analysis. We performed a quantitative evaluation of the surface density of GFAP-immunoreactivecell bodies and cell processes according to the point-countingmethod of Weibel (1979), using a stereological grid. This methodprovides an estimate of the morphological changes in astrocytes(Luquin et al., 1993). For each image the number of points atwhich GFAP-immunoreactive cell bodies and cell processes crossedthe test grid lines was assessed by an individual that was blindto the code designation. GFAP-immunoreactive surface density thenwas calculated by using the following formula: Surface Density= 2I/L, where I is the number of points at which the immunoreactiveprofiles cross the test grid lines and L is the total length ofthe test grid line (length of each test grid line × number oflines) in the tissue. The mean GFAP-immunoreactive surface densityfrom the three sections for each structure in each animal wascalculated. These values then were used to calculate group means± SEM per each brain region that was analyzed. The number of GFAP-positivecells in each of the digitized images also was counted to checkfor changes in the number of astrocytes expressing GFAP. Fromthe work of others, however, it was not expected that hormonemanipulations would result in changes in astrocytic number (Luquinet al., 1993).
bFGF immunoreactivity analysis. The number of bFGF-positive cells in each of the digitized images was counted by an individualthat was blind to the code assignment. The mean cell counts fromthe three sections of each structure for each animal were calculated.Then these values were used to calculate group means ± SEM pereach area that wasanalyzed.

Golgi
For the study of dendritic branching the animals were given an overdose of pentobarbital and perfused transcardially with0.9% saline at 4 weeks after ovariectomy. The brains were removedand immersed whole in 20 ml of a Golgi-Cox solution and left inthe dark for 14 d. Then the brains were placed in a 30% sucrosesolution for 2 d, cut on a vibratome at 200 µm (Gibb and Kolb,1998), and developed by using a procedure described previously(Kolb and McLimans, 1986). Layer II/III pyramidal cells in theEnt were traced by using a camera lucida drawing tube magnifiedat 250×. To be included in the data analysis, the dendritic treesof pyramidal cells had to fulfill the following criteria: (1)a cell had to be well impregnated and not obscured by blood vessels,astrocytes, or heavy clusters of dendrites from other cells; and(2) the apical and basilar arborization had to appear to be mainlyintact and visible in the place of section. The branch segmentsand branch order were determined from the camera lucida drawingsby using the procedure of Coleman and Riesen (1968). Branch orderwas determined for the apical dendrites such that branches originatingfrom the primary apical dendrite were first order, after one bifurcationsecond order, and so on. For basilar dendrites, those originatingat the cell body were first order, and so on. Ten cells were drawnper animal per area. Dendritic length was analyzed by using theconcentric ring method of Sholl (1956). The number of intersectionsof dendrites with a series of concentric spheres at 20 µm intervalsfrom the center of the cell body was counted for eachcell.
For each cell, spine density was measured from one apical dendritic branch in the terminal tuft, from an oblique branch runningoff the main apical dendritic shaft approximately half-way upthe shaft, and from a secondary branch proximal to the cell bodyfor one basilar branch, after the procedure of Woolley et al.(1990).
Brains from experimental and control subjects were always processed in parallel from perfusion to image analysis. In addition,special caution was taken to treat brains from each experimentalcondition in exactly the same manner: same fixative, time of post-fixation,washes, exposure to antibodies and chromogen, temperature, anddehydration.

Design and procedures
Experiment 1A: Expression of GFAP immunoreactivity. This experiment was conducted to determine the effect of ovariectomy andestrogen replacement on astrocytic morphology as reflected bychanges in GFAP-immunoreactive surface density in serotonergicand dopaminergic somatodendritic regions. To this end, adult femalerats were ovariectomized under methoxyflurane (Metofane) anesthesiaby bilateral dorsal incisions. Animals then were assigned randomlyto receive 5 µg of EB (EB group) or 0.1 ml of peanut oil (OILgroup) every 4 d for 4 weeks. This replacement regimen is similarto that used by Forgie and Stewart (1993) and has been found topotentiate the locomotor-stimulating effects of amphetamine inovariectomized animals. The animals were housed individually instandard stainless steel hanging cages throughout the entire study.At 24 hr after the last EB or oil injection the animals were killed,and their brains were processed for GFAP immunoreactivity. Levelsof GFAP-immunoreactive surface density and the number of immunoreactivecells were assessed in the DR andVTA.
Experiment 1B: Expression of bFGF immunoreactivity. bFGF immunoreactivity in the DR and VTA was studied in alternate sectionsfrom the brains of animals described in Experiment 1A. In addition,we measured bFGF immunoreactivity in projection regions of mesolimbicDA neurons: the NAcc shell, NAcc core, and layer II of the Entand of the PFC (Fallon and Moore, 1978; Fallon and Loughlin, 1987;Akil and Lewis, 1993, 1994). For comparison, we measured bFGFimmunoreactivity in layers V and VI ofOc2.
Experiment 2: Time course of changes in the expression of bFGF immunoreactivity. This experiment was done to compare bFGFimmunoreactivity in intact females and ovariectomized femalesat a number of time points after surgery. Although the analysisof GFAP-immunoreactive surface density in Experiment 1 providedclear evidence of changes in astrocytic activity in the VTA, thefindings paralleled the changes seen in bFGF expression. It wasdecided, therefore, for practical reasons to measure only bFGFimmunoreactivity in this study because of the large number ofbrain sections needed to complete such a time course experiment.For this experiment, adult female rats were either ovariectomized(Ovx group) or sham-operated (Intact group) under Metofane anesthesiaby bilateral dorsal incisions. Animals were killed 1, 2, 4, 8,and 40 weeks after surgery. With the exception of the animalskilled at 40 weeks in which cycles were difficult to detect, allanimals were killed on the afternoon of the estrus phase of theestrous cycle of the animals in the Intact group (defined by thepresence of cornified cells in the vaginal smear), and their brainswere processed for bFGF immunoreactivity. To induce synchronyof the estrous cycle within each Intact group and to prevent anypossible effects of long-term isolation within the 40 week groups,we housed together the animals that had undergone the same hormonalmanipulation (ovariectomy or sham surgery) and that were goingto be killed at the same time point after surgery (1, 2, 4, 8,and 40 weeks) during the time between surgery and killing. Dailyvaginal smears were taken from all animals. Within each Intactgroup (1, 2, 4, 8, and 40 weeks) the animals from which the afternoonof estrus could not be identified clearly at the time of perfusionwere not used in thestudy.
First, we analyzed bFGF immunoreactivity within the same brain regions assessed in Experiment 1B (DR, NAcc shell, NAcc core,layer II of the Ent and of the PFC, and layers V and VI of theOc2) in brains of animals killed 4 weeks after ovariectomy. Onthe basis of the findings from 4 weeks after ovariectomy, we subsequentlyinvestigated levels of bFGF immunoreactivity within the VTA andEnt 1, 2, 8, and 40 weeks after surgery. Levels of bFGF immunoreactivitywithin the PFC also were examined at these time intervals, withthe exception of 8 weeks for which sections were notavailable.
Experiment 3: Double-labeling study. To examine the nature of the cells expressing bFGF in the regions that were analyzed,we killed two ovariectomized rats given either EB or oil replacementunder the same conditions as animals in Experiment 1 at 24 hrafter the last EB or oil injection; we processed their brainsfor bFGF-GFAP and bFGF-TH double-labelingimmunohistochemistry.
Experiment 4: Dendritic branching of layer II/III pyramidal cells of the Ent. In a previous study we found increases in thedendritic arbor of pyramidal neurons in parietal cortex severalmonths after ovariectomy of adult females (Stewart and Kolb, 1994).We had argued at that time that these changes might arise in responseto mild injury or a reduction of neural input brought about bythe sudden and complete loss of estrogens. To examine whethersimilar changes might be seen after ovariectomy in cortical areasfound to increase the expression of bFGF in the present experimentand to determine whether these changes could be prevented by estrogenreplacement, we studied cells in the Ent of rats ovariectomizedat 80-90 d of age and treated immediately with EB (n = 6) or OIL(n = 5) (10 µg every other day for 4 weeks or 0.1 ml peanut oilonly). These female Wistar rats were part of another ongoing studyand were born and raised in the laboratory at Concordia University;with the exception of the dose of EB given, they were treatedsimilarly to those in the otherexperiments.

Statistical analysis
For GFAP and bFGF, all analyses were done on the raw data, using estimates of GFAP-immunoreactive surface density and thenumber of GFAP- and bFGF-immunoreactive cells per square millimeter.For Experiment 1, comparisons were made between the EB-treatedgroup and oil-treated group within a single region. Likewise,in Experiment 2, because the number of bFGF-immunoreactive cellsdiffered considerably as a function of time after surgery, differencesbetween Intact and Ovx groups were tested within a region in animalsthat were killed at the same time after surgery. The data wereanalyzed by using Student's t tests for independent samples. Alldata in the figures are presented as a percentage of the meanof the EB group in a particular region in Experiment 1 and asa percentage of the mean of the Intact group killed at the sametime in a particular region in Experiment 2. For the Golgi studythe data for dendritic branches were analyzed by ANOVA for group× branch order for apical and basilar dendrites separately; thedata for dendritic length also were analyzed by ANOVA. Similarly,the data of numbers of spines were analyzed by ANOVA for groupby spinelocation.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1A: GFAP-immunoreactive surface density in VTA and DR of ovariectomized animals with EB or oil replacement

Changes in astrocytic morphology were assessed by using GFAP-immunoreactive surface density in the VTA and DR of adult femalerats 4 weeks after ovariectomy with or without estrogen replacement(5 µg every 4 d). As shown in Figure 1, within the VTA the surfacedensity of GFAP-immunoreactive cell bodies and processes was significantlyhigher (68 ± 11%) in the brains of ovariectomized animals withoutestrogen replacement. No difference in GFAP-immunoreactive surfacedensity was found in the DR. In agreement with previous findings,no effects of hormonal manipulations on the number of GFAP-immunoreactiveastrocytes were observed in either region (Luquin et al., 1993).

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Figure 1. Glial fibrillary acidic protein (GFAP)-immunoreactive cells and surface density in dorsal raphe (DR) and ventral tegmental area (VTA). Values are expressed as the mean ± SEM percentage of the levels in estradiol benzoate (EB)-treated animals. All animals were ovariectomized and treated with either EB (5 µg every 4 d for 4 weeks; VTA, n = 4; DR, n = 4) or oil (0.1 ml of peanut oil every 4 d for 4 weeks; VTA, n = 3; DR, n = 4). *Student's t test conducted on the actual counts of the VTA showed a significant difference between EB and oil treatment [t (5) = 5.77; p = 0.002].

Experiment 1B: bFGF immunoreactivity in ovariectomized animals with EB or oil replacement

Figure 2 shows the mean number of bFGF-immunoreactive cells within several areas of the brain of the ovariectomized animalstreated with EB or oil every 4 d for 4 weeks. It can be seen thatthe number of bFGF-immunoreactive cells within the VTA (86 ± 23%)and Ent (203 ± 67%) was significantly higher in ovariectomizedfemales without estrogen replacement. No differences were foundwithin the DR, NAcc shell, NAcc core, PFC, or Oc2.

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Figure 2. bFGF immunoreactivity in the dorsal raphe (DR), ventral tegmental area (VTA), nucleus accumbens shell (Shell), nucleus accumbens core (Core), entorhinal cortex (Ent), prefrontal cortex (PFC), and occipital cortex area 2 (Oc2). Values are expressed as the mean ± SEM percentage of the levels in estradiol benzoate (EB)-treated animals. All animals were ovariectomized and treated with either EB (5 µg every 4 d for 4 weeks; midbrain regions, n = 4; forebrain regions, n = 3) or oil (0.1 ml every 4 d for 4 weeks; midbrain regions, n = 4; forebrain regions, n = 3). *Student's t test conducted on the actual counts of the VTA and Ent showed a significant difference between EB and oil treatment [VTA, t (6) = 3.06, p = 0.02; Ent, t (6) = 2.78, p = 0.03].

The photomicrographs in Figure 3 provide examples of bFGF immunoreactivity in the Ent of two ovariectomized animals treatedwith either EB or oil every 4 d for 4 weeks. A greater numberof darkly labeled bFGF-immunoreactive cells can be seen in layerII of the Ent of ovariectomized animals without estrogen replacement.

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Figure 3. Digitized images showing darkly labeled bFGF-immunoreactive cells (black dots) in tissue lightly counterstained with cresyl violet (lightly stained cells in the background). Images were taken from the entorhinal cortex of representative animals that were ovariectomized and treated with either 5 µg of estradiol (EB) or 0.1 ml of peanut oil (OIL) every 4 d for 4 weeks. The area delimited by the white arrows corresponds to layer II, the region from which the number of bFGF-immunoreactive cells was assessed. Scale bar, 100 µm.

Experiment 2: bFGF immunoreactivity in intact versus ovariectomized rats 4 weeks after surgery

In this experiment, bFGF immunoreactivity was first assessed within the DR, NAcc shell, NAcc core, Ent, PFC, and Oc2 in ovariectomizedand intact animals 4 weeks after surgery. As depicted in Figure4, ovariectomy produced significant increases in the number ofbFGF-labeled cells within the VTA (31 ± 10%) and within the Ent(60 ± 8%). Although there was a noticeable increase in bFGF immunoreactivitywithin the PFC (22 ± 7%) in the Ovx group, this difference didnot reach statistical significance.

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Figure 4. bFGF immunoreactivity in the dorsal raphe (DR), ventral tegmental area (VTA), nucleus accumbens shell (Shell), nucleus accumbens core (Core), entorhinal cortex (Ent), prefrontal cortex (PFC), and occipital cortex area 2 (Oc2). Values are expressed as the mean ± SEM percentage of the levels in intact animals. Intact animals were killed in the afternoon of the estrus phase of their estrous cycle, 4 weeks after sham surgery (all regions, n = 4, except Oc2, n = 3). Ovariectomized animals were killed 4 weeks after surgery (all regions, n = 4, except PFC, n = 3). *Student's t test conducted on the actual counts [VTA, t (6) = 2.42, p = 0.05; Ent, t (6) = 2.48, p = 0.04; PFC, t (5) = 2.16; p = 0.08].

It should be noted that the percentage of difference in bFGF immunoreactivity between ovariectomized oil-treated rats andEB-treated rats in Experiment 1 was greater than that betweenovariectomized and intact animals killed 4 weeks after surgeryin Experiment 2. Several factors may have accounted for this difference,including the dose of estradiol used in Experiment 1 and/or theabsence of progesterone. Future studies will be needed to examinetheseissues.

Time course of the changes in bFGF immunoreactivity

We next assessed the time course of the changes in the number of bFGF-immunoreactive cells within those areas showing increases4 weeks after ovariectomy: the VTA, Ent, and PFC. As shown inFigure 5, although not all of the changes that were observed werestatistically significant, there was a gradual increase in bFGFimmunoreactivity within the VTA of ovariectomized rats. Thesechanges appeared to peak between 4 and 8 weeks and to return tolevels similar to those observed in intact animals by 40 weeks.Similarly, within the Ent the number of cells expressing bFGFimmunoreactivity showed a small increase 2 weeks after ovariectomy.At 4 weeks the increase was statistically significant and thendecreased at 8 weeks and returned to levels similar to those inintact animals after 40 weeks. The changes in expression of bFGFimmunoreactivity within the PFC were minimal, as shown in Figure5. No differences were observed until 4 weeks after ovariectomy(.10 > p < 0.05). At 40 weeks after ovariectomy the number ofbFGF-immunoreactive cells returned to levels seen in intact animals.It is interesting, however, that just as was seen in other areasat 40 weeks, there was a small but nonsignificant decrease (18± 4%) in bFGF immunoreactivity in Ovx groups.

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Figure 5. bFGF immunoreactivity in the ventral tegmental area (VTA), entorhinal cortex (Ent), and prefrontal cortex (PFC). Values are expressed as the mean ± SEM percentage of the levels in intact animals. Intact animals were killed 1, 2, 4, 8, and 40 weeks after sham surgery on the afternoon of the estrus phase of their estrous cycle (n = 4, except at 1 week, n = 3). Ovariectomized animals were killed 1, 2, 4, 8, and 40 weeks after surgery (VTA and Ent, n = 4, except at 1 week, n = 3; PFC, n = 3, except at 2 weeks, n = 4). *Student's t tests conducted on the actual counts showed a significant difference between groups 4 weeks after ovariectomy [VTA, 4 weeks, t (6) = 2.42, p = 0.05; Ent, 4 weeks, t (6) = 2.48, p = 0.04; PFC, 4 weeks, t (5) = 2.16, p = 0.08]. The sampling areas from which the number of bFGF-immunoreactive cells was assessed are indicated in black on the adjacent tracing of the coronal plate taken from the Swanson atlas (1992).

Localization of the expression of bFGF immunoreactivity

Brain sections from two ovariectomized animals that received either oil or EB (5 µg) replacement every 4 d for 4 weeks weredouble-labeled with bFGF-GFAP and bFGF-TH. In agreement with ourprevious study (Flores et al., 1998), these studies revealed thatin all areas that were examined bFGF-positive cells were alsoGFAP-positive and that in the VTA the dopaminergic neurons didnot express bFGF. The photomicrographs shown in Figure 6 weretaken from the VTA region of the ovariectomized animal withoutEB treatment. Figure 6A shows bFGF-GFAP double labeling and Figure6B shows bFGF-TH double labeling. bFGF immunoreactivity was seenonly in astrocytes, never in TH-positive cells. As can be seen,however, not all GFAP-positive astrocytes expressed bFGF. Similarfindings were observed in the brain of the EB-treated rat (datanot shown).

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Figure 6. Digitized images from the ventral tegmental area of an ovariectomized animal given estradiol benzoate (EB) replacement (5 µg every 4 d) and killed 4 weeks after surgery. A, Section labeled with both GFAP and bFGF. The black arrow points to an astrocyte labeled with both bFGF and GFAP. The white arrow points to an astrocyte that was not bFGF-immunoreactive. B, Section labeled with both tyrosine hydroxylase (TH) and bFGF. bFGF immunoreactivity (indicated by the white arrow) was not found within TH-positive cells (indicated by the black arrow). Oil immersion. Scale bar, 20 µm.

Morphology of cells in entorhinal cortex

Figure 7 shows the number of branches on the apical dendrites of layer II/III pyramidal cells in the entorhinal cortex 4 weeksafter ovariectomy. It can be seen that, in general, there weremore branches on the cells from ovariectomized animals treatedwith oil than there were on the cells from those treated withestrogen. This effect was statistically significant only for thefirst and second order branches (p values < 0.05). In the caseof the basilar branches, although the mean numbers were consistentlyhigher in cells from oil-treated animals, there were no significantdifferences between OIL- and EB-treated animals. The Sholl analysisrevealed no significant differences between groups in dendriticlength. No significant differences were found in the numbers ofspines in any of the regions that were counted.

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Figure 7. Mean ± SEM number of apical dendritic branches as a function of order in layer II/III entorhinal cortex in adult ovariectomized females given EB replacement (10 µg every 2 d for 4 weeks) or OIL (0.1 ml every 2 d for 4 weeks). *Significantly different from EB (p < 0.05).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effects in cell body regions

We explored the effects of ovariectomy on astrocytic activity, as reflected by the expression of GFAP and bFGF, in cell bodyregions of dopaminergic neurons in the VTA and serotonergic neuronsin the DR at 4 weeks after surgery. In Experiment 1 it was foundthat in the VTA the surface density of GFAP-positive astrocyteswas greater in ovariectomized animals than in animals given estrogenreplacement (5 µg of EB every 4 d for 4 weeks). In both Experiments1 and 2 bFGF expression in the VTA was greater in ovariectomizedfemales than in estrogen-replaced or intact groups. There wereno differences between groups in either study in theDR.

Changes in astrocytic bFGF and/or GFAP expression similar to those seen here have been observed in the VTA after toxic insultsto dopaminergic neurons and after drug-induced increases in dopaminergicactivity (Stromberg et al., 1986; Beitner-Johnson et al., 1993;Chadi et al., 1994; Flores et al., 1998). These changes may bepart of a cascade of neuroprotective events initiated by insult.bFGF promotes growth and survival of dopaminergic cells (see Chadiet al., 1993; Bouvier and Mytilineou, 1995) and upregulates GFAPsurface density (Gómez-Pinilla et al., 1995); furthermore, theeffects of bFGF on dopaminergic function appear to be mediatedby astrocytes (Engele and Bohn, 1991; Hou et al., 1997).

How estrogen loss induces injury-like reactions in particular brain regions is unknown. Estrogens have anti-oxidative effectsthat are independent of the activation of estrogen receptors (Behlet al., 1997; Green et al., 1998; Sawada et al., 1998). Interestingly,oxidative events are associated with lesions of the dopaminergicsystem (Cohen and Heikkila, 1974), and the protective actionsof bFGF on dopaminergic cells are mediated, at least in part,via anti-oxidative effects (Hou et al., 1997). Thus, one interpretationof the present findings is that a sudden loss of estrogen servesas a minor insult to dopaminergic neurons in the VTA, leadingto the recruitment of a series of neuroprotective events. In supportof this idea is the evidence that, in the absence of estrogens,neurons are more vulnerable to the toxic effects of a varietyof insults (Bishop and Simpkins, 1994; Green et al., 1997), includingthose to the midbrain dopaminergic system (Dluzen et al., 1996;Dluzen, 1997).

Alternatively, the observed changes might well be mediated via effects at estrogen receptors. The VTA contains, however, onlya few cells that express the classic nuclear estrogen receptor- $alpha$ .These cells are found within VTA subregions that were examinedin the present study but are nondopaminergic. In fact, the morphologyof some of the estrogen receptor- $alpha$ -immunoreactive cells withinthe VTA suggests that they are glia (Kritzer, 1997), and astrocytesare known to express estrogen receptors- $alpha$ (Jung-Testas et al.,1991; Santagati et al., 1994). Another possibility is that theeffects are mediated by the estrogen receptor- $beta$ , the mRNA forwhich is densely expressed in the VTA (Shughrue et al., 1997),or by effects at estrogen membrane sites (Ramirez and Zheng, 1996).

It contrast to the VTA, no effects were found in the DR in either experiment. This lack of effects was somewhat surprisingconsidering the known influence of estrogens on serotonergic function(Fink and Sumner, 1996; Fink et al., 1996; Pecins-Thompson etal., 1996, 1998; Pecins-Thompson and Bethea, 1999) and the presenceof estrogen receptor- $alpha$ protein in this area (Alves et al., 1998).The disparity between the observations in the VTA and DR supportsthe idea that the effects of ovarian hormones on astrocytic functionare restricted to specific brain regions (Luquin et al., 1993).

Effects in cortical regions

A major finding of the present study is that 4 weeks after surgery bFGF expression was higher in the entorhinal cortex ofovariectomized animals without estrogen. bFGF immunoreactivitywas assessed in layer II of the rostral entorhinal cortex, a regionthat receives substantial innervation from dopaminergic cellsof the VTA (Fallon and Loughlin, 1987; Akil and Lewis, 1993, 1994).Cells within these layers of the entorhinal cortex also receivea major input from cholinergic cells of the basal forebrain (Luitenet al., 1987) that also are known to be sensitive to changes inestrogen levels (Luine, 1985; Toran-Allerand et al., 1992; McMillanet al., 1996; Gibbs and Aggarwal, 1998). Interestingly, cellsof layer II are among the first to undergo neurofibrillary changesin Alzheimer's disease (Braak and Braak, 1992).

Recently, it has been found that bFGF protects entorhinal cortex layer II neurons from injury induced by lesions of the perforantpath carrying fibers to and from the hippocampus (Cummings etal., 1992; Peterson et al., 1996). In addition, bFGF mRNA expressionis upregulated in entorhinal cortex after electroconvulsive shock(Follesa et al., 1994) and seizures (Riva et al., 1992). Thus,the increased expression of bFGF in entorhinal cortex found inthe present study is suggestive of an injury-like response toovariectomy that may or may not be related to the effects observedwithin the VTA. Estrogen receptor binding is seen in the entorhinalcortex (Pfaff and Keiner, 1973; Loy et al., 1988), as are mRNAsfor both estrogen receptor- $alpha$ and - $beta$ (see Pelletier et al., 1988;Simerly et al., 1990; Shughrue et al., 1997). In light of thesefindings it will be important to determine whether lesions ofthe dopaminergic neurons of the VTA alter the expression of bFGFin the entorhinalcortex.

We also found, 4 weeks after ovariectomy, a small but nonsignificant increase in bFGF expression in supragenual layer II ofthe medial PFC, a region innervated by midbrain dopaminergic cells(Fallon and Loughlin, 1987). There was, however, no differencebetween ovariectomized animals and animals given the 4 week estrogentreatment within this region. This lack of effect of estrogenon bFGF expression in this region might have resulted from thefact that estrogen, but not progesterone, was replaced (see, forexample, Kritzer and Kohama, 1998). Again, these effects of ovariectomymay be mediated directly, possibly via estrogen receptor- $beta$ (Shughrueet al., 1997). However, the facts that PFC receives VTA dopaminergicprojections (Fallon and Loughlin, 1987) and that ovariectomy reducesthe density of TH-immunoreactive fibers in PFC (Kritzer and Kohama,1998) suggest that changes in bFGF expression could be relatedto changes in dopaminergic function, although the noradrenergicsystem cannot be ruled out. In addition, as discussed in relationto the entorhinal cortex, projections from the basal forebrainalso could be involved. No effects of ovariectomy or estrogenreplacement were seen in the occipital cortex, suggesting thatthe changes in bFGF that were seen in the present study are specificto particular corticalareas.

Finally, no differences in bFGF expression were found in the nucleus accumbens in either study at 4 weeks after surgery. Thelack of effect of ovariectomy on bFGF expression in this dopaminergicterminal region parallels what is seen after repeated injectionsof amphetamine (Flores et al., 1998) or after 6-hydroxydopaminelesions (Chadi et al., 1994) when there is sustained upregulationof bFGF in cell body regions, but not in nucleus accumbens. Thefact that changes were seen in terminal regions in cortex andnot in the nucleus accumbens may reflect differences in characteristicsof the midbrain dopamine cells that project to each region (Bunneyand Chiodo, 1984; Domesick, 1988); alternatively, it may reflectlocally mediated effects in particular cortical areas or effectsbrought about by interactions between systems projecting to theseareas.

Time course of changes in bFGF immunoreactivity

In the VTA and entorhinal cortex the changes in bFGF expression induced by ovariectomy developed gradually, increasing at2 weeks and peaking by 4 weeks. In the medial PFC changes didnot appear before 4 weeks. These findings suggest that the reactionto ovariectomy is delayed and prolonged. The fact that the effectsof ovariectomy were not evident after 40 weeks may indicate thatadjustment to the changes in circulating hormones is complete,bFGF is self-regulating, or the astrocytic response isspent.

Pyramidal cell morphology in entorhinal cortex

The increase in numbers of apical dendrites of layer II/III pyramidal cells in entorhinal cortex found 4 weeks after ovariectomyin animals without estrogen replacement in the present study,although considerably smaller, parallels the finding of Stewartand Kolb (1994) in parietal cortex when animals were studied 4months after ovariectomy and compared with intact animals. Atthe time of the latter study, we suggested that it was likelythat the increase in dendritic arbor was mediated indirectly,possibly in response to impaired functioning of cells projectingto the area or locally via effects on astrocytes. Thus, althoughcorrelational, the present findings provide additional supportfor this idea. The effects seen in the entorhinal cortex in thesestudies are particularly provocative in view of the well documentedvulnerability of cells of the entorhinal cortex after injury andin aging. It will now be important to determine whether thereis an interaction among the age of the animal at ovariectomy,the length of the period without estrogenic hormones, and themagnitude of the observed changes in this region of thebrain.

  FOOTNOTES

Received June 3, 1999; revised July 16, 1999; accepted July 20, 1999.

This work was supported by grants to J.S. from the Natural Science and Engineering Research Council of Canada and Fonds pourla Formation de Chercheurs et l'Aide à la Recherche (FCAR, Québec).C.F. was supported by a graduate fellowship from ConcordiaUniversity.
Correspondence should be addressed to Dr. Jane Stewart, Center for Studies in Behavioral Neurobiology, Department of Psychology,Concordia University, 1455 de Maisonneuve Boulevard, Montréal,Québec, Canada H3G1M8.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Akil M, Lewis DA (1993) The dopaminergic innervation of monkey entorhinal cortex. Cereb Cortex 3:533-550[Abstract/Free Full Text].
Akil M, Lewis DA (1994) The distribution of tyrosine hydroxylase-immunoreactive fibers in the human entorhinal cortex. Neuroscience 60:857-874[Web of Science][Medline].
Alves S, Weiland N, Hayashi S, McEwen B (1998) Immunocytochemical localization of nuclear estrogen receptors and progestin receptors within the rat dorsal raphe nucleus. J Comp Neurol 391:322-334[Web of Science][Medline].
Becker JB (1990) Estrogen rapidly potentiates amphetamine-induced striatal dopamine release and rotational behavior during microdialysis. Neurosci Lett 118:169-171[Web of Science][Medline].
Behl C, Skutella T, LezoualXh F, Post A, Widmann M, Newton C, Holsboer F (1997) Neuroprotection against oxidative stress by estrogens: structure-activity relationship. Mol Pharmacol 51:535-541[Abstract/Free Full Text].
Beitner-Johnson D, Guitart X, Nestler EJ (1993) Glial fibrillary acidic protein and the mesolimbic dopamine system: regulation by chronic morphine and Lewis-Fischer strain differences in the rat ventral tegmental area. J Neurochem 61:1766-1773[Web of Science][Medline].
Bishop J, Simpkins J (1994) Estradiol treatment increases viability of glioma and neuroblastoma cells in vitro. Mol Cell Neurosci 5:303-308[Web of Science][Medline].
Bossé R, Di Paolo T (1996) The modulation of brain dopamine and GABA_A receptors by estradiol: a clue for CNS changes occurring at menopause. Cell Mol Neurobiol 16:199-212[Web of Science][Medline].
Bouvier M, Mytilineou C (1995) Basic fibroblast growth factor increases division and delays differentiation of dopamine precursors in vitro. J Neurosci 15:7141-7149[Abstract].
Braak H, Braak E (1992) The human entorhinal cortex: normal morphology and lamina-specific pathology in various diseases. Neurosci Res 15:6-31[Web of Science][Medline].
Bunney BS, Chiodo LA (1984) Mesocortical dopamine systems: further electrophysiological and pharmacological characteristics. In: Monoamine innervation of cerebral cortex (Descarries L, Reader T, Jasper H, eds), pp 263-277. New York: Liss.
Camp DM, Becker JB, Robinson TE (1986) Sex differences in the effects of gonadectomy on amphetamine-induced rotational behavior in rats. Behav Neural Biol 46:491-495[Web of Science][Medline].
Castner SA, Xiao L, Becker JB (1993) Sex differences in striatal dopamine: in vivo microdialysis and behavioral studies. Brain Res 610:127-134[Web of Science][Medline].
Chadi G, Møller A, Rosén L, Janson A, Agnati L, Goldstein M, Ögren S-O, Pettersson R, Fuxe K (1993) Protective actions of human recombinant basic fibroblast growth factor on MPTP-lesioned nigrostriatal dopamine neurons after intraventricular infusion. Exp Brain Res 97:145-158[Web of Science][Medline].
Chadi G, Cao Y, Pettersson RF, Fuxe K (1994) Temporal and spatial increase of astroglial basic fibroblast growth factor synthesis after 6-hydroxydopamine-induced degeneration of the nigrostriatal dopamine neurons. Neuroscience 61:891-910[Web of Science][Medline].
Cohen G, Heikkila R (1974) The generation of hydrogen peroxide, superoxide radical, and hydroxyl radical by 6-hydroxydopamine, dialuric acid, and related cytotoxic agents. J Biol Chem 249:2447-2452[Abstract/Free Full Text].
Coleman P, Riesen A (1968) Environmental effects on cortical dendritic fields. I. Rearing in the dark. J Anat 102:363-374[Web of Science][Medline].
Cummings B, Yee G, Cotman C (1992) bFGF promotes the survival of entorhinal layer II neurons after perforant path axotomy. Brain Res 591:271-276[Web of Science][Medline].
Dluzen D (1997) Estrogen decreases corpus striatal neurotoxicity in response to 6-hydroxydopamine. Brain Res 767:340-344[Web of Science][Medline].
Dluzen D, McDermott J, Liu B (1996) Estrogen alters MPTP-induced neurotoxicity in female mice: effects on striatal dopamine concentrations and release. J Neurochem 66:658-666[Web of Science][Medline].
Domesick V (1988) Neuroanatomical organization of dopamine neurons in the ventral tegmental area. Ann NY Acad Sci 537:10-26[Web of Science][Medline].
Engele J, Bohn MC (1991) The neurotrophic effects of fibroblast growth factors on dopaminergic neurons in vitro are mediated by mesencephalic glia. J Neurosci 11:3070-3078[Abstract].
Fallon J, Loughlin S (1987) Monoamine innervation of cerebral cortex and a theory of the role of monoamines in cerebral cortex and basal ganglia. In: Cerebral cortex (Jones E, Peters A, eds), pp 41-127. New York: Plenum.
Fallon JH, Moore RY (1978) Catecholamine innervation of the basal forebrain. IV. Topography of the dopamine projection to the basal forebrain and neostriatum. J Comp Neurol 180:545-580[Web of Science][Medline].
Fink G, Sumner B (1996) Oestrogen and mental state. Nature 383:306[Medline].
Fink G, Sumner B, Rosie R, Grace O, Quinn J (1996) Estrogen control of central neurotransmission: effect on mood, mental state, and memory. Cell Mol Neurobiol 16:325-343[Web of Science][Medline].
Flores C, Rodaros D, Stewart J (1998) Long-lasting induction of astrocytic basic fibroblast growth factor by repeated injections of amphetamine: blockade by concurrent treatment with a glutamate antagonist. J Neurosci 18:9547-9555[Abstract/Free Full Text].
Follesa P, Gale K, Mocchetti I (1994) Regional and temporal pattern of expression of nerve growth factor and basic fibroblast growth factor mRNA in rat brain following electroconvulsive shock. Exp Neurol 127:37-44[Medline].
Forgie ML, Stewart J (1993) Sex differences in amphetamine-induced locomotor activity in adult rats: role of testosterone exposure in the neonatal period. Pharmacol Biochem Behav 46:637-645[Web of Science][Medline].
Forgie ML, Stewart J (1994) Effect of prepubertal ovariectomy on amphetamine-induced locomotor activity in adult female rats. Horm Behav 28:241-260[Medline].
García-Segura LM, Chowen JA, Párducz A, Naftolin F (1994) Gonadal hormones as promoters of structural synaptic plasticity: cellular mechanism. Prog Neurobiol 44:279-307[Web of Science][Medline].
García-Segura ML, Chowen JA, Naftolin F (1996) Endocrine glia: roles of glial cells in the brain actions of steroid and thyroid hormones and in the regulation of hormone secretion. Front Neuroendocrinol 17:180-211[Web of Science][Medline].
Gibb R, Kolb B (1998) A method for vibratome sectioning of Golgi-Cox stained whole rat brain. J Neurosci Methods 79:1-4[Web of Science][Medline].
Gibbs RB (1998) Levels of trkA and BDNF mRNA, but not NGF mRNA, fluctuate across the estrous cycle and increase in response to acute hormone replacement. Brain Res 787:259-268[Web of Science][Medline].
Gibbs RB, Aggarwal P (1998) Estrogen and basal forebrain cholinergic neurons: implications for brain aging and Alzheimer's disease-related cognitive decline. Horm Behav 34:98-111[Medline].
Gómez-Pinilla F, Vu L, Cotman C (1995) Regulation of astrocyte proliferation by FGF-2 and heparan sulfate in vivo. J Neurosci 15:2021-2029[Abstract].
Gould E, Woolley CS, Frankfurt M, McEwen BS (1990) Gonadal steroids regulate dendritic spine density in hippocampal pyramidal cells in adulthood. J Neurosci 10:1286-1291[Abstract].
Green PS, Bishop J, Simpkins JW (1997) 17 $alpha$ -Estradiol exerts neuroprotective effects on SK-N-SH cells. J Neurosci 17:511-515[Abstract/Free Full Text].
Green PS, Gridley KE, Simpkins JW (1998) Nuclear estrogen receptor-independent neuroprotection by estratrienes: a novel interaction with glutathione. Neuroscience 84:7-10[Web of Science][Medline].
Gregoire A, Kumar R, Everitt B, Henderson A, Studd J (1996) Transdermal oestrogen for treatment of severe postnatal depression. Lancet 347:930-933[Web of Science][Medline].
Henderson V (1997) The epidemiology of estrogen replacement therapy and Alzheimer's disease. Neurology 48:S27-S35[Abstract].
Hou J-GG, Cohen G, Mytilineou C (1997) Basic fibroblast growth factor stimulation of glial cells protects dopamine neurons from 6-hydroxydopamine toxicity: involvement of the glutathione system. J Neurochem 69:76-83[Web of Science][Medline].
Hsu S, Raine L, Fanger H (1981) The use of anti-avidin antibody and avidin-biotin-peroxidase complex in immunoperoxidase techniques. Am J Clin Pathol 75:816-821[Web of Science][Medline].
Jung-Testas I, Renoir J, Gasc J, Baulieu E (1991) Estrogen-inducible progesterone receptor in primary cultures of rat glial cells. Exp Cell Res 193:12-19[Web of Science][Medline].
Kolb B, McLimans J (1986) A process for cryostat sectioning of Golgi-Cox tissue. Stain Technol 61:379-380[Medline].
Kolb B, Stewart J, Sutherland RJ (1997) Recovery of function is associated with increased spine density in cortical pyramidal cells after frontal lesions and/or noradrenaline depletion in neonatal rats. Behav Brain Res 89:61-70[Web of Science][Medline].
Kritzer M (1997) Selective colocalization of immunoreactivity for intracellular gonadal hormone receptors and tyrosine hydroxylase in the ventral tegmental area, substantia nigra, and retrorubral fields in the rat. J Comp Neurol 379:247-260[Web of Science][Medline].
Kritzer M, Kohama S (1998) Ovarian hormones influence the morphology, distribution, and density of tyrosine hydroxylase-immunoreactive axons in the dorsolateral prefrontal cortex of adult rhesus monkeys. J Comp Neurol 395:1-17[Web of Science][Medline].
Lindamer L, Lohr J, Harris M, McAdams L, Jeste D (1999) Gender-related clinical differences in older patients with schizophrenia. J Clin Psychiatry 60:61-67[Web of Science][Medline].
Loy R, Gerlach J, McEwen B (1988) Autoradiographic localization of estradiol-binding neurons in the rat hippocampal formation and entorhinal cortex. Dev Brain Res 39:245-251.
Luine V (1985) Estradiol increases choline acetyltransferase activity in specific basal forebrain nuclei and projection areas of female rats. Exp Neurol 89:484-490[Web of Science][Medline].
Luiten PGM, Gaykema RPA, Traber J, Spencer Jr DG (1987) Cortical projection patterns of magnocellular basal nucleus subdivisions as revealed by anterogradely transported phaseolus vulgaris leucoagglutinin. Brain Res 413:229-250[Web of Science][Medline].
Luquin S, Naftolin F, García-Segura LM (1993) Natural fluctuation and gonadal hormone regulation of astrocyte immunoreactivity in dentate gyrus. J Neurobiol 24:913-924[Medline].
Matsuzaki K, Yoshitake Y, Matuo Y, Sasaki H, Nishikawa K (1989) Monoclonal antibodies against heparin-binding growth factor II/basic fibroblast growth factor that block its biological activity: invalidity of the antibodies for tumor angiogenesis. Proc Natl Acad Sci USA 86:9911-9915[Abstract/Free Full Text].
McMillan P, Singer C, Dorsa D (1996) The effects of ovariectomy and estrogen replacement on trkA and choline acetyltransferase mRNA expression in the basal forebrain of the adult female Sprague Dawley rat. J Neurosci 16:1860-1865[Abstract/Free Full Text].
Murphy D, Cole N, Greenberger V, Segal M (1998a) Estradiol increases dendritic spine density by reducing GABA neurotransmission in hippocampal neurons. J Neurosci 18:2550-2559[Abstract/Free Full Text].
Murphy D, Cole N, Segal M (1998b) Brain-derived neurotrophic factor mediates estradiol-induced dendritic spine formation in hippocampal neurons. Proc Natl Acad Sci USA 95:11412-11417[Abstract/Free Full Text].
Paxinos G, Watson C (1997) In: The rat brain in stereotaxic coordinates, Ed 3. New York: Academic.
Pecins-Thompson M, Bethea C (1999) Ovarian steroid regulation of serotonin-1A autoreceptor messenger RNA expression in the dorsal raphe of rhesus macaques. Neuroscience 89:267-277[Web of Science][Medline].
Pecins-Thompson M, Brown N, Kohama S, Bethea C (1996) Ovarian steroid regulation of tryptophan hydroxylase mRNA expression in rhesus macaques. J Neurosci 16:7021-7029[Abstract/Free Full Text].
Pecins-Thompson M, Brown N, Bethea C (1998) Regulation of serotonin reuptake transporter mRNA expression by ovarian steroids in rhesus macaques. Mol Brain Res 53:120-129[Medline].
Pelletier G, Liao N, Follea N, Govindan M (1988) Mapping of estrogen receptor-producing cells in the rat brain by in situ hybridization. Neurosci Lett 94:23-28[Web of Science][Medline].
Peterson D, Lucidi-Phillipi C, Murphy D, Ray J, Gage F (1996) Fibroblast growth factor-2 protects entorhinal layer II glutamatergic neurons from axotomy-induced death. J Neurosci 16:886-898[Abstract/Free Full Text].
Pfaff D, Keiner M (1973) Atlas of estradiol-concentrating cells in the central nervous system of the female rat. J Comp Neurol 151:121-158[Web of Science][Medline].
Ramirez V, Zheng J (1996) Membrane sex-steroid receptors in the brain. Front Neuroendocrinol 17:402-439[Web of Science][Medline].
Riva M, Gale K, Mocchetti I (1992) Basic fibroblast growth factor mRNA increases in specific brain regions following convulsive seizures. Mol Brain Res 15:311-318[Medline].
Robinson TE (1988) Stimulant drugs and stress: factors influencing individual differences in the susceptibility to sensitization. In: Sensitization in the nervous system (Kalivas PW, Barnes CD, eds), pp 145-173. Caldwell, NJ: Telford.
Santagati S, Melcangi R, Celotti F, Martini L, Maggi A (1994) Estrogen receptor is expressed in different types of glial cells in culture. J Neurochem 63:2058-2064[Web of Science][Medline].
Sawada H, Ibi M, Kihira T, Urushitani M, Akaike A, Shimohana S (1998) Estradiol protects mesencephalic dopaminergic neurons from oxidative stress-induced neural death. J Neurosci Res 54:707-719[Web of Science][Medline].
Sherwin B (1997) Estrogen effects on cognition in menopausal women. Neurology 48:S21-S26[Abstract].
Sholl D (1956) In: The organization of the cerebral cortex. London: Methuen.
Shughrue P, Lane M, Merchenthaler I (1997) Comparative distribution of estrogen receptor- $alpha$ and - $beta$ mRNA in the rat central nervous system. J Comp Neurol 388:507-525[Web of Science][Medline].
Simerly R, Chang C, Muramatsu M, Swanson L (1990) Distribution of androgen and estrogen receptor mRNA-containing cells in the rat brain: an in situ hybridization study. J Comp Neurol 294:76-95[Web of Science][Medline].
Singh M, Meyer EM, Millard WJ, Simpkins JW (1994) Ovarian steroid deprivation results in a reversible learning impairment and compromised cholinergic function in female Sprague Dawley rats. Brain Res 644:305-312[Web of Science][Medline].
Sohrabji F, Miranda RC, Toran-Allerand CD (1995) Identification of a putative estrogen response element in the gene encoding brain-derived neurotrophic factor. Proc Natl Acad Sci USA 92:11110-11114[Abstract/Free Full Text].
Stewart J, Kolb B (1994) Dendritic branching in cortical pyramidal cells in response to ovariectomy in adult female rats: suppression by neonatal exposure to testosterone. Brain Res 654:149-154[Web of Science][Medline].
Stewart J, Rodaros D (1999) The effects of gonadal hormones on the development and expression of the stimulant effects of morphine in male and female rats. Behav Brain Res 102:89-98[Web of Science][Medline].
Stromberg I, Bjorklund H, Dahl D, Jonsson G, Sundstrom E, Olson L (1986) Astrocyte responses to dopaminergic denervations by 6-hydroxydopamine and 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine as evidenced by glial fibrillary acidic protein immunohistochemistry. Brain Res Bull 17:225-236[Medline].
Swanson L (1992) In: Brain maps: structure of the rat brain. Amsterdam: Elsevier.
Toran-Allerand CD, Miranda RC, Bentham WDL, Sohrabji F, Brown TJ, Hochberg RB, MacLusky NJ (1992) Estrogen receptors colocalize with low-affinity nerve growth factor receptors in cholinergic neurons of the basal forebrain. Proc Natl Acad Sci USA 89:4668-4672[Abstract/Free Full Text].
Weibel E (1979) In: Stereological methods, Vol 1, Practical methods for biological morphometry. London: Academic.
Woolley CS, McEwen BS (1994) Estradiol regulates hippocampal dendritic spine density via an N-methyl-D-aspartate receptor-dependent mechanism. J Neurosci 14:7680-7687[Abstract].
Woolley CS, Gould E, Frankfurt M, McEwen BS (1990) Naturally occurring fluctuations in dendritic spine density on adult hippocampal pyramidal neurons. J Neurosci 10:4035-4039[Abstract].
Zilles K (1985) In: The cortex of the rat: a stereotaxic atlas. New York: Springer.

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