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The Journal of Neuroscience, July 9, 2003, 23(14):6013-6022
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c-fos Reduces Corticosterone-Mediated Effects on Neurotrophic Factor Expression in the Rat Hippocampal CA1 Region
A. C. Hansson,1,2 W. Sommer,2 R. Rimondini,2 B. Andbjer,2 I. Strömberg,1 andK. Fuxe1 Departments of 1Neuroscience and 2NEUROTEC, Karolinska Institutet, 171 77 Stockholm, Sweden
Abstract
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Abstract
Introduction
The transcription of neurotrophic factors, i.e., basic fibroblast growth factor (bFGF) and brain-derived neurotrophic factor (BDNF) is regulated by glucocorticoid receptor (GR) and mineralocorticoid receptor (MR) activation despite the lack of a classical glucocorticoid response element in their promoter region.A time course for corticosterone (10 mg/kg, s.c.) in adrenalectomized rats revealed a peak hormone effect at the 4 hr time interval for bFGF (110–204% increase), BDNF (53–67% decrease), GR (53–64% decrease), and MR (34–56% decrease) mRNA levels in all hippocampal subregions using in situ hybridization. c-fos mRNA levels were affected exclusively in the dentate gyrus after 50 min to 2 hr (38–46% decrease).
Furthermore, it was evaluated whether corticosterone regulation of these genes depends on interactions with the transcription factor complex activator protein-1. c-fos antisense oligodeoxynucleotides were injected into the dorsal hippocampus of adrenalectomized rats. Corticosterone was given 2 hr later, and the effects on gene expression were measured 4 hr later. In CA1, antisense treatment significantly and selectively enhanced the hormone action on the expression of bFGF (44% enhanced increase) and BDNF (38% enhanced decrease) versus control oligodeoxynucleotide treatment. In addition, an upregulation of c-fos expression (89% increase) was found. There were no effects of c-fos antisense on hippocampal GR and MR expression. Thus it seems that a tonic c-fos mechanism exists within CA1, which reduces GR- and MR-mediated effects on expression of bFGF and BDNF.
Key words: adrenalectomy; basic fibroblast growth factor; brain-derived growth factor; glucocorticoid receptor; mineralocorticoid receptor; immediate early gene; antisense oligodeoxynucleotides; in situ hybridization; rat brain
Introduction
The adrenal steroid hormone corticosterone (CORT) regulates transcription via activation of two types of corticosteroid receptors, namely the mineralocorticoid receptor [MR (or type I)] and the glucocorticoid receptor [GR (or type II)], which can act directly as transcription factors by binding to their common glucocorticoid response element (GRE) (Beato et al., 1995). However, although there are clearly documented CORT effects on transcription of a number of genes, among them GR and MR as well as basic fibroblast growth factor (bFGF) and brain-derived neurotrophic factor (BDNF) (Barbany and Persson, 1992
The GR and the transcription factor activator protein-1 (AP-1) complex appear to interact with each other via mechanisms both dependent on and independent from DNA binding (Diamond et al., 1990
With use of the adrenalectomized (ADX) animal model, it has been shown recently by means of in situ hybridization that CORT affects neurotrophic factor gene mRNA levels in the dorsal hippocampus that are unique for each particular gene in a cellular and region-specific manner and therefore seem to be strongly context dependent (Hansson et al., 2000
Materials and Methods
Animals and treatment. Male Sprague Dawley rats (Alab, Stockholm, Sweden), weighing 200–250 gm, were kept under a standard light/dark cycle (lights on at 6 A.M. and off at 6 P.M.) and constant room temperature (23°C) and had ad libitum access to tap water and food pellets.Rats were bilaterally adrenalectomized under halothane anesthesia. The ADX model used has been characterized recently by Hansson et al. (2000
Using the same ADX animal model, a 15-mer partially phosphorothioated antisense ODN to c-fos (5'-GAA CAT CAT GGT CGT -3', 1 nmol in 1 µl of Ringer's solution, as c-fos oligo group; n = 6) or a corresponding control random ODN (5'-GTA CCA ATC GGG ATT -3', as control oligo group; n = 6) was injected in a second experiment via a previously unilaterally implanted cannula guide into the dorsal hippocampus [1 µl over 2 min; bregma anterior (A) -3.3 mm, lateral (L) +2.7 mm, ventral (V) -4.3 mm, according to the atlas of Paxinos and Watson (1982)]. Two hours later a single dose of CORT was given (10 mg/kg in propylene glycol, s.c.). After four hours the animals were anesthetized with sodium pentobarbital and intracardially perfused with 100 ml ice-cold saline after blood samples for serum CORT had been collected by cardiac puncture. After the rats were killed, brains were rapidly removed, frozen in liquid isopentane (-40°C), and stored at -70°C. Coronal sections (10 µm) were taken at bregma levels close to the cannula guide and at bregma level -4 to -4.5 mm and mounted on slides (ProbeOn slides, Fischer/Biotech, Hampton, NH).
In a third experiment animals were unilaterally intrahippocampally injected with end-labeled [S 35]
ATP antisense c-fos ODN (1 µl over 1 min; bregma A -3.3 mm, L +2.7 mm, V -4.3 mm), and rats were killed by decapitation after 1 hr (n = 4)and 6 hr (n = 4). Transversal sections (10 µm) were taken through the injection site, exposed for 2 and 7 d to
-Max Hyperfilm (Amersham Biosciences, Arlington Heights, IL), and counterstained with cresyl violet.
The animal experiments were approved by the local ethical committee (Stockholm Norra Försöksdjurs Etiska Kommittee).
Radioimmunoassay for corticosterone. Cardiac blood samples were collected in EDTA-containing tubes and centrifuged at 4 x g for 20 min at 4°C. Serum CORT levels were determined by radioimmunoassay (RIA) (Coat-a-count, Diagnostic Products Corporation, Los Angeles, CA). The RIA was performed with rat [125I]CORT. The CORT assay had a detection limit of
5.7 ng/ml.
RNA probe synthesis. The bFGF riboprobes, both antisense and sense, were synthesized from a SmaI–XhoI fragment from rat cDNA (position: 525–1004 bp corresponding to the coding region for the mature protein) in Bluescript/SK + (Stratagene, San Diego, CA). The BDNF riboprobes (antisense and sense) were generated from a 350 bp PvuII–PstI fragment from rat cDNA, coding for a corresponding protein, and subcloned into the Bluescript/SK + plasmid. A 513 bp EcoRI fragment from the 5' end of the rat MR cDNA was subcloned into the vector pGEM4 (Promega, Madison, WI) and used for antisense and sense riboprobe generation. For the generation of the GR riboprobes (antisense and sense), we used a 673 bp EcoRI–PstI rat GR cDNA fragment (position: 1691–2364 bp, corresponding to the 3'portion of the coding region), subcloned into the vector pSP64 (Promega). The c-fos riboprobe was a 557 bp BglII–StuI fragment from rat cDNA in Bluescript KS II + (Stratagene).
Antisense and sense RNA probes were synthesized from a 1 µg linearized DNA template, incubated with transcription buffer (40 mM Tris-HCl, pH 7.5, 6 mM MgCl2,2 mM spermidine) in the presence of 12.5 nmol ATP, CTP, GTP, 500 pmol UTP, and 125 pmol [
-35S]UTP (1350 Ci/mmol; NEN/DuPont, Boston, MA), 1 U RNase inhibitor, and 1 U RNA polymerase (Roche Molecular Biochemicals, Bromma, Sweden) at 37°C for 1 hr. The DNA was removed by digestion with RNase-free DNase at 37°C for 15 min. The transcripts were purified using spin columns (Amersham Biosciences), and the quality of the riboprobes was analyzed on a 8 M urea/5% polyacrylamide gel (PAGE).
End-labeling of oligodeoxynucleotides. Radioactive labeling of phosphorothioate-modified antisense c-fos ODN was made by end-labeling with [S 35]ATP
In situ hybridization. The sections mounted on slides were brought to room temperature and fixed for 15 min in 4% paraformaldehyde in PBS, pH 7.0. After fixation the slides were washed in PBS, pH 7.4, for 10 min and rinsed two times in sterilized water for 5 min, each followed by a deproteination of the tissue with 0.1 M HCl for 10 min. The slides were rinsed twice in PBS, pH 7.4, for 5 min and were acetylated in 0.1 M triethanolamine, pH 8.0/0.25% acetic anhydride for 20 min, washed again twice in PBS, pH 7.4, for 5 min, dehydrated in graded ethanol, and air dried. The slides were prehybridized in a humidified chamber with prehybridization buffer [50% deionized formamide, 50 mM Tris-HCl, pH 7.6, 25 mM EDTA, pH 8.0, 20 mM NaCl, 0.25 mg/ml yeast tRNA, 2.5x Denhardt's solution (0.05% Ficoll, 0.05% polyvinylpyrrolidone, 0.05% bovine serum albumin)] at 37°C for 2–3 hr. After the prehybridization buffer was drained off the slides, the sections were hybridized with 80 µl hybridization buffer (50% deionized formamide, 20 mM Tris-HCl, pH 7.6, 1 mM EDTA, pH 8.0, 0.3 M NaCl, 0.2 M DTT, 0.5 mg/ml yeast tRNA, 0.1 mg/ml poly-A-RNA, 1x Denhardt's solution, 10% dextransulfate) containing 0.5–1x 10 6 cpm of either the labeled antisense RNA or sense RNA. The sections were covered with siliconized coverslips and incubated at 44°C for 18 hr in a humidified chamber. After hybridization, the coverslips were removed by washing with 1x standard saline citrate (SSC) at 48°C for 30 min, followed by washing twice in 0.5x SSC/50% formamide at 48°C for 30 min. After two additional washings in 1x SSC for 15 min at 48°C, the sections were treated with 1 µg/ml RNAaseA in 0.5 M NaCl, 10 mM Tris-HCl, 5 mM EDTA, pH 8.0, for 45 min at 37°C. After two washing steps in 1x SSC for 20 min at 55°C followed by a washing in 1x SSC for 15 min at room temperature, the slides were dehydrated in graded ethanol and air dried. The hybridized sections were exposed for 1–4 weeks to
Double labeling of c-fos transcripts and glial fibrillary acidic protein immunoreactivity. After in situ hybridization with S 35-labeled c-fos riboprobes, sections were rinsed in 0.1 M phosphate buffer, pH 7.4, and incubated with the primary antibody [glial fibrillary acidic protein (GFAP), monoclonal mouse anti-GFAP, 1:200; Chemicon International, Harrow, UK] for 48 hr at 4°C. The antibodies were diluted in 0.1 M phosphate buffer with 0.3% Triton X-100 (Sigma, St. Louis, MO), and all incubations were performed in humidified chambers. The sections were rinsed in 0.1 M phosphate buffer, and the secondary antibody (biotinylated horse anti-mouse, 1:100; Vector Laboratories, Burlingame, CA) was applied and incubated for 2 hr at room temperature. After rinsing the sections were incubated with solutions A and B in 0.1 M phosphate buffer (1:100; Vectastain ABC Reagent, Vector Laboratories) for 1 hr at room temperature. The sections were then exposed to 0.05 M Trizma buffer, pH 7.1, and reacted with 3,3' diaminobenzidine tetrahydrochloride as a chromogen. The reaction was stopped by a pH shift in 0.05 M Trizma, pH 8.5. Sections were dehydrated in graded ethanol, coated with film emulsion (Ilford, Cheshire, UK), and stored in desiccated light-tight boxes at 4°C for 4 weeks. After development the sections were counterstained with cresyl violet and coverslipped with Mountex (Göteborgs Termometerfabrik). Sections were digitized and evaluated using a Leica microscope connected with a high-resolution digital CCD video camera.
Double immunofluorescence staining. Sections were brought to room temperature, rehydrated, rinsed in 0.01 M phosphate buffer, and incubated with a mixture of two primary antibodies [polyclonal rabbit anti-c-fos antibody (Ab-5; Oncogene Research Products, San Diego, CA; 1:300) and either monoclonal mouse anti-GR antibody, a generous gift from Dr. A.-C. Wikström, Karolinska Institutet (Okret et al., 1984
Data analysis. Semiquantitative values of the mRNA levels were obtained by measuring the gray values of the film autoradiograms as illustrated in Figures 3 and 4 using an SAS Biovision image analyzing system (Avanzati, Milan, Italy). Radioactivity artifacts on autoradiograms close to tissue damage were carefully excluded in all measurements. Three measurements were performed for each region: (1) the total value, i.e., measurements of the region in the sections hybridized with [
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Figure 3. a, Schematic representation to show the position of the cannula guide and of the sampled areas for densitometric evaluation in a coronal section through the dorsal hippocampus (bregma level -3.3 mm). CA1–CA3, Cornus Ammon areas; DG, dentate gyrus. b, Distribution of 35S-end-labeled antisense c-fos ODN 1 hr after intrahippocampal injection as shown in a cresyl violet-counterstained coronal section (bregma level = -3 to -4 mm). c, Dark-field microphotographs from in situ hybridization of autoradiograms of bFGF and BDNF mRNA levels in response to CORT (10 mg/kg, s.c.) after randomized (left panel) and antisense c-fos ODN (right panel) treatment. Arrowheads show mRNA signals in the CA1 region (bregma levels = -3 to -4.5 mm). Scale bar, 1 mm. d, Densitometric evaluation of in situ hybridization autoradiograms. Values are given as percentage of random oligo-treated group (mean ± SEM; n = 6). Statistical analysis was performed by one-way ANOVA (treatment) followed by Bonferroni's correction. *p < 0.05, **p < 0.01 versus random oligo group. CA1, Cornus Ammon area. For details on treatment, see Materials and Methods.
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Figure 4. Bright-field photomicrographs showing a strongly labeled nerve cell enriched in silver grains, representing c-fos transcripts, and a GFAP-ir (brown color) astroglial cell lacking silver grains in the same cresyl violet counterstained section in the CA1 region of corticosterone-treated (10 mg/kg, s.c.; 4 hr) ADX rat. CA1, Cornus Ammon area. For details on treatment, see Materials and Methods. Scale bar, 15 µm. Bregma level = -3 to -4.5 mm.
Results
Radioimmunoassay for corticosterone serum levels
After a single subcutaneous injection of CORT (10 mg/kg) to ADX rats, the serum levels of CORT were determined at the time of killing. Serum CORT levels were high after 50 min (2545 ± 321 ng CORT/ml blood serum; mean ± SEM; n = 5) and then gradually declined over the 2 hr (805 ± 143 ng CORT/ml; n = 5), 4 hr (147 ± 27 ng CORT/ml; n = 5), and 8 hr time interval (29 ± 4 ng CORT/ml; n = 5) down to undetectable serum CORT levels 24 hr after the injection. In all vehicle-injected ADX rats, serum levels of CORT were undetectable in each time interval analyzed.In the second experiment, CORT (10 mg/kg, s.c.) was injected 2 hr after antisense c-fos or control ODN treatment in 24 hr ADX rats. Four hours later, serum CORT levels did not differ between the c-fos oligo group (275 ± 80 ng CORT/ml serum) and the control oligo animal group (372 ± 65 ng CORT/ml serum; one-way ANOVA: F(1,10) = 0.89; not significant).
Effects of corticosterone treatment on gene expression in the dorsal hippocampus
In situ hybridization analysis was performed for bFGF, BDNF, GR, MR, and c-fos mRNAs. Optical density values from the dorsal hippocampus were obtained from autoradiograms, and the data were analyzed either by two-way ANOVA in the CORT time course experiment or by one-way ANOVA in the as c-fos experiment, followed by Bonferroni's correction. The optical density data and the results of the post hoc analysis are summarized in Tables 1, 2, 3. To better demonstrate the most important actions of CORT on gene expression levels, the optical density values were transformed into relative changes (%) in relation to the ADX + vehicle-treated group in Figure 1. Figure 3d shows the effects of CORT on gene expression levels after c-fos blockade as relative changes (percentage) in relation to control ODN-injected ADX rats. The distribution patterns for bFGF, BDNF, GR, and MR mRNA levels in the dorsal hippocampus are shown in Figure 2 and are similar to those described in Hansson et al. (2000
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Table 1. Effects of corticosterone (10 mg/kg, s.c.) on gene expression levels in the dorsal hippocampus of ADX rats
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Table 2. Effects of injection stress on c-fos mRNA levels in the dorsal hippocampus of ADX rats
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Table 3. Effects of c-fos antisense oligonucleotides on gene expression in response to corticosterone (10 mg/kg, s.c.) in the dorsal hippocampus of ADX rats
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Figure 1. Densitometric evaluation of in situ hybridization from autoradiograms. Values are given in percentage of the ADX group (mean ± SEM; n = 5) versus vehicle-treated control ADX rats. Statistical analysis was performed by two-way ANOVA (treatment x time) followed by Fisher's PLSD test and Bonferroni's correction. *p < 0.05, **p < 0.01, ***p < 0.001 versus ADX group. CA1, CA3, Cornus Ammon areas; DG, dentate gyrus. For details on treatment, see Materials and Methods.
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Figure 2. Dark-field microphotographs from autoradiograms of in situ hybridization of bFGF, BDNF, GR, and MR mRNA levels 4 hr after injection and of c-fos mRNA levels 50 min after subcutaneous injection in ADX + vehicle-treated (left panel) and ADX + CORT-treated (10 mg/kg, right panel) rats. Arrowheads show mRNA signals in the dentate gyrus. Bregma levels were -3 to -4 mm. Scale bar, 1 mm.
Time course of gene expression after corticosterone treatment
bFGF
bFGF mRNA levels were significantly and time-dependently increased after acute CORT treatment in all hippocampal subregions as shown by two-way ANOVA for treatment (CA1: F(1,40) = 132.3, p < 0.0001; CA2: F(1,40) = 70.1, p < 0.0001; CA3: F(1,40) = 148.9, p < 0.0001; DG: F(1,40) = 123.6, p < 0.0001) and interaction of treatment and time (CA1: F(1,40) = 18.7, p < 0.0001; CA2: F(1,40) = 7.7, p = 0.0001; CA3: F(1,40) = 28.6, p < 0.0001; DG: F(1,40) = 46, p < 0.0001). Bonferroni's corrected post hoc analysis revealed that CORT induced strong and significant increases of bFGF mRNA levels in all hippocampal subfields between 2 and 8 hr after treatment (CA1: 90 to 119%, CA2: 110 to 146%, CA3: 85 to 157%, DG: 84 to 204%) (Table 1, Figs. 1, 2). Only in CA2 did CORT induce long-lasting changes of bFGF mRNA levels observed even after 24 hr (105% increase) (Table 1). Levels of bFGF mRNAs were not changed in vehicle-treated ADX rats over the time course of the experiment in all analyzed subregions.BDNF
CORT induced time-dependent significant changes of BDNF mRNA levels as revealed by two-way ANOVA for treatment (CA1: F(1,39) = 38, p < 0.0001; CA3: F(1,39) = 12.1, p = 0.0013; DG: F(1,39) = 108, p < 0.0001) and interaction of treatment and time (CA1: F(1,39) = 2.9, p = 0.03; CA3: F(1,39) = 0.8, not significant; DG: F(1,39) = 14.7, p < 0.0001). The corrected post hoc test suggested a CORT-induced decrease of BDNF mRNA levels after 2–8 hr treatment in CA1 (30 to 53%) and DG (44 to 67%) (Table 1, Figs. 1, 2). In CA3, levels of BDNF mRNA were only significantly decreased after 2 hr (26%) (Table 1, Fig. 1). BDNF mRNA levels were not changed in vehicle-treated ADX rats during the time course in all subregions analyzed.GR
A significant time-dependent decrease of GR mRNA levels by CORT was found in all hippocampal subregions using two-way ANOVA for treatment (CA1: F(1,39) = 149.2, p < 0.0001; CA2: F(1,39) = 116.2, p < 0.0001; CA3: F(1,39) = 62.7, p < 0.0001; DG: F(1,39) = 130.6, p < 0.0001) and interaction of treatment and time (CA1: F(1,39) = 6.2, p = 0.0006; CA2: F(1,39) = 3.3, p = 0.0194; CA3: F(1,39) = 4.0, p = 0.0085; DG: F(1,39) = 8.8, p < 0.0001). Corrected post hoc analysis revealed strong and significant long-lasting decreases of GR mRNA levels from 2 to 24 hr (CA1: 35 to 64%; CA2: 32 to 64%; CA3: 40 to 63%; DG: 23 to 62%) (Table 1, Figs. 1, 2). GR mRNA levels were not changed in vehicle-treated rats at any time point analyzed.MR
The expression of MR was significantly and time-dependently decreased by CORT in all hippocampal subregions as demonstrated by two-way ANOVA for treatment (CA1: F(1,40) = 21.8, p < 0.0001; CA2: F(1,40) = 10.8, p = 0.0021; CA3: F(1,38) = 47.3, p < 0.0001; DG: F(1,38) = 42.9, p < 0.0001) and interaction of treatment and time (CA1: F(1,40) = 3.2, p = 0.023; CA3: F(1,38) = 12.8, p < 0.0001; DG: F(1,38) = 12.2, p < 0.0001). Bonferroni's corrected Fisher's post hoc analysis revealed a significant decrease in MR mRNA levels after 2 and 4 hr in CA1 (27 to 39%) (Table 1, Figs. 1, 2), after 4 hr in CA3 (34 to 43%) (Table 1, Figs. 1, 2), and between 4 and 8 hr in DG (31 to 56%) (Table 1, Figs. 1, 2). Interestingly, there was a small and significant increase in MR mRNA levels by 21% in CA3 after 50 min (Table 1, Fig. 1). In CA2, the corrected post hoc test did not show significant differences between CORT- and vehicle-treated rats (Table 1, Figs. 1, 2). Furthermore, MR mRNA levels were not changed in vehicle-treated rats at any time point analyzed.c-fos
The expression of c-fos was time-dependently and significantly decreased after CORT treatment only in the DG as suggested by two-way ANOVA for treatment (F(1,38) = 21.8, p < 0.0001) and interaction of treatment and time (F(1,38) = 3.3, p = 0.021). The corrected post hoc test showed significant decreases of c-fos mRNA levels in the DG between 50 min and 2 hr (38 to 46%) (Table 1, Figs. 1, 2). There was no treatment or interaction effect in other hippocampal regions.Furthermore, the two-way ANOVA demonstrated a strong time effect in all subregions (CA1: F(1,38) = 33, p < 0.0001; CA3: F(1,40) = 16.6, p < 0.0001; DG: F(1,38) = 16.1, p < 0.0001). Corrected post hoc analysis revealed strong and significant increases in c-fos mRNA levels at 50 min in both vehicle- and CORT-treated rats compared with the other time points in CA1 (2–24 hr: 123 to 245% increase), CA3 (4–24 hr: 63 to 116% increase), and DG (2–24 hr: 64 to 130% increase) (Table 1).
There was a decrease in c-fos mRNA levels by 27% in vehicle injected versus non-injected ADX rats at 50 min in DG (two-way ANOVA for treatment and time: F(2,14) = 6.0, p < 0.0133) (Table 2). There were no significant differences in c-fos mRNA levels between injected and non-injected ADX rats in CA1 and CA3 at any time interval (Table 2).
Effects of intrahippocampal c-fos antisense ODN injection on corticosterone-induced gene expression
bFGF
In CA1, c-fos antisense ODN increased bFGF mRNA levels (44%) 4 hr after CORT treatment compared with control ODN-treated rats as revealed by one-way ANOVA followed by Bonferroni's correction (F(1,11) = 22.4, corrected p = 0.0024) (Table 3, Fig. 3c,d). bFGF mRNA levels were not affected by antisense treatment in other subregions. The antisense effect was observed only at bregma levels close to the injection site.BDNF
Blockade of c-fos expression enhanced the 4 hr CORT response on BDNF in CA1 by decreasing mRNA levels to 38% versus control oligo-treated rats (one-way ANOVA: F(1,7) = 32.7, corrected p = 0.0021) (Table 3, Fig. 3c,d). Other hippocampal subregions were not affected by antisense treatment. The antisense effect was observed only at bregma levels close to the injection site.GR and MR
Intrahippocampal c-fos blockade did not affect the CORT response on GR and MR mRNA levels in any subregion (Table 3).c-fos
Antisense c-fos treatment induced a strong increase of c-fos mRNA levels in CA1 (89%) as shown by one-way ANOVA followed by Bonferroni's correction (F(1,10) = 10.8, corrected p = 0.0246) (Table 3, Fig. 3d). The increase of c-fos mRNA levels was observed only at bregma levels close to the injection site.Distribution of end-labeled antisense c-fos oligodeoxynucleotides
The distribution of [S35]Cellular distribution of c-fos mRNA in the hippocampus
Double labeling of c-fos mRNA and GFAP immunoreactivity (-ir) demonstrates that c-fos is mainly located outside of GFAP-immunoreactive profiles in large and weakly cresyl violet-stained cell nuclei within the pyramidal cell layer of CA and the granular cell layer of DG, probably representing nerve cells. The distribution of the c-fos signal appears in a "speckled" pattern, i.e., a few large neurons here and there are strongly labeled above the average c-fos signal (Fig. 4).Colocalization of c-fos and GR, c-fos and NeuN, and c-fos and GFAP-ir in the hippocampus
The colocalization of c-fos-ir and GR-ir and markers for neurons (NeuN-ir) and astrocytes (GFAP-ir) were studied in CA1, CA3, and DG of ADX rats 1.5 hr after corticosterone treatment. Double immunofluorescence analysis of nuclear c-fos-ir (red color) and nuclear GR-ir or nuclear NeuN-ir (both with green color) showed a predominant colocalization (yellow color) of the relatively low number of c-fos-ir nuclei, with GR-ir and NeuN-ir nuclei found in large numbers in all analyzed regions of the hippocampus (Fig. 5). There was no colocalization of c-fos-ir and GFAP-ir in the hippocampus. Thus, c-fos-ir is found mainly in GR-ir neurons of the hippocampus; however, only a small population of the GR-ir neurons is c-fos-ir.
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Figure 5. Fluorescence photomicrographs involving double immunolabeling procedures showing the colocalization (yellow color) of c-fos-ir (Texas Red) with NeuN-ir (FITC, green, left) or with GR-ir (FITC, green, right), but not with GFAP-ir (FITC, middle) in the CA1 region of corticosterone-treated (10 mg/kg, s.c.; 1.5 hr) ADX rats. CA1, Cornus Ammon area. For details on treatment, see Materials and Methods. Scale bar, 40 µm. Bregma level = -3 to -4.5 mm.
Discussion
The data presented here support the view that hippocampal neurotrophic factors and corticosteroid receptors are target genes for glucocorticoid regulation (Chao et al., 1989Effects of corticosterone on hippocampal c-fos gene expression
In the present paper, c-fos mRNA levels are significantly downregulated by CORT in the DG. Previous communications on CORT effects on c-fos expression reported conflicting results. In tissue cultures, glucocorticoids increased c-fos mRNA levels, as shown for AtT-20 pituitary tumor cells (Lin et al., 1992Normally, basal c-fos levels in naive animals are low (Herdegen and Leah, 1998
As stated above, CORT seems to counteract the initial increase of c-fos expression in the DG. The mechanism involved may be that activated GR/MR can suppress c-fos transcription via binding to a putative GRE in the promoter region (Wang and Howells, 1994
Effects of antisense blockade of c-fos on gene expression
Inducible transcription factors may not only interact directly with DNA but may also indirectly modify transcription processes by complexing with other transcriptionally operating proteins. Therefore the second experiment tested whether AP-1, i.e. c-fos, is involved in the CORT regulation of genes by use of intrahippocampal antisense "knockdown" of c-fos expression. Antisense treatment increased bFGF and decreased BDNF mRNA levels after CORT administration, and hence an enhancement of the CORT-induced transcriptional regulation of these genes was found. The CA1 area contains fewer bFGF and BDNF mRNA signals than the CA3 or the DG, and the magnitude of changes induced by the antisense treatment was modest using semiquantitative measurements. Nevertheless, such a change in a modest signal may have consequences for the relatively low signaling at the receptors for these neurotrophic factors in CA1, because the corresponding changes in the proteins may be at least as large. An inhibitory effect of c-fos on gene regulation by glucocorticoids has earlier been described in tissue culture studies by Diamond et al. (1990The injection of ODNs into various regions of the brain has been used in a large number of studies to investigate the role of c-fos in the regulation of downstream genes or in behavioral or physiological responses associated with the activation of c-fos (for review, see Szklarczyk and Kaczmarek, 1999
Along with these and other studies, the c-fos antisense approach has been validated by various control experiments to demonstrate specificity and to establish the pharmacokinetics (Szklarczyk and Kaczmarek, 1999
In addition to the antisense effects on bFGF and BDNF expression in the CA1 region, a strong upregulation was also found of the c-fos transcript itself in this region. Interestingly, in previous studies increased levels of c-fos mRNA was observed after intrastriatal c-fos antisense treatment (Sommer et al., 1996
Both the regulation of c-fos target genes (i.e., bFGF, BDNF) and the c-fos autoregulation appear to be region specific, because in the present study it is observed only in the CA1 region but not in the adjacent DG, although the ODN can be found in both regions (Fig. 3b). The absence of an antisense effect in the DG may be explained by the fact that CORT is already suppressing c-fos expression in this region in contrast to CA1.
To demonstrate anatomic specificity of the intrahippocampally injected ODNs, we used radiolabeled partially phosphorothioated ODNs that have been found to remain intact in brain tissue up to 24 hr after injection (Sommer et al., 2000
Despite the demonstrated antagonistic functional interaction between GR and c-fos, only a small subpopulation of neurons within the pyramidal cell layer of the CA1 region is c-fos-ir; the majority of these nerve cells are also GR-ir. No c-fos-ir is found in astroglial cells, demonstrating a major involvement of neuronal cells. Nevertheless, it seems possible that the actions of the antisense c-fos treatment on bFGF and BDNF gene expression found in large numbers of nerve and glial cells all over the CA1 area could be related to an antagonistic interaction between GR and c-fos in this small population of nerve cells. Thus, this antagonistic interaction at the promoter regions of such genes and others in this special group of cells could lead to a marked alteration in their neuronal activity, whether representing glutamate or GABA neurons, which may initiate a cascade of events leading to an altered control of the majority of BDNF nerve cells and bFGF glial cells in this region, involving recurrent collaterals and widespread terminal networks. In this way it becomes possible to understand how a potential interaction of GR and c-fos in a small group of neurons could lead to the demonstrated GR-enhancing actions of antisense c-fos treatment on BDNF and bFGF expression in neuronal and glial networks, respectively, the majority of which exhibit no c-fos-ir but only GR-ir. Thus, the response of these cells to GR activation with regard to BDNF and bFGF expression becomes altered in view of their altered afferent input, triggered by the altered antagonistic interactions of GR and c-fos on the antisense treatment in this small population of nerve cells found mainly in the CA1 pyramidal cell layer. It must be noted, however, that in the damaged area not analyzed for c-fos-ir, c-fos-ir could exist in cells not containing GR-ir. Therefore, actions of antisense c-fos treatment may exist that occur independently of GREs.
In summary, the time course for CORT in the ADX rat revealed a peak hormone effect on neurotrophic factors (bFGF, BDNF) and corticosteroid receptor (GR and MR) mRNA levels at the 4 hr time interval. c-fos mRNA levels were negatively regulated in the dentate gyrus at the 50 min to 2 hr time interval. The major finding was that local antisense c-fos ODN treatment significantly and selectively enhanced the CORT action only in the CA1 region on the expression of bFGF and BDNF mRNA versus randomized control ODN treatment. Thus, it seems as if within the CA1 area a tonic c-fos mechanism exists that reduces GR- or MR-induced effects, or both, on gene expression of bFGF and BDNF.
Footnotes
Received May. 1, 2002; revised Apr. 7, 2003; accepted Apr. 11, 2003.This work was supported by a grant from the Marianne and Marcus Wallenberg Foundation and by a grant from the Swedish Medical Research Council (04X-715). We are grateful to Ulla-Britt Finman for technical assistance.
Correspondence should be addressed to Dr. A. C. Hansson, Department of NEUROTEC, Karolinska Institutet, Huddinge University Hospital, M 57, S-141 86 Stockholm, Sweden. E-mail: anita.hansson{at}neuro.ki.se.
Copyright © 2003 Society for Neuroscience 0270-6474/03/236013-10$15.00/0
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