Male Sprague Dawley rats weighing between 200 and 250 g were housed in a temperature-controlled (20—22°C) environment with a 12-hour light-darkness cycle. All animals were housed in groups of 2 for 2 weeks before adrenalectomy. The rats were given a normal rat chow diet (Gold Coin, Malaysia) and normal saline ad libitum. Prior ethical approval was obtained from the Animal Ethics Committee of Universiti Kebangsaan Malaysia (UKMAEC No: PP/ANAT/2008/FARIHAH/21-AUGUST/240-0CT-2008-JUNE-2009).

Bilateral adrenalectomy was performed through a midline dorsal incision followed by a small incision through the muscle layer under 1:1 Xylazil (Ilium, Australia) and Ketapex (Troy, Australia) anesthesia at 0.1 ml/100 g of body weight. After removal of the adrenal glands, the incision was sutured, and a topical antiseptic, Poviderm (Hoe, Malaysia), was applied over the wound. For the sham-operated rats, the adrenals were left in place.

A total of 20 male Sprague Dawley rats were divided into 3 groups: a baseline control group (n = 6), a sham-operated group (n = 7) and an adrenalectomized group (n = 7). The adrenalectomized group was given intramuscular dexamethasone (Sigma, USA) (ADR+Dexa) at a dose of 120 μg/kg 2 weeks post adrenalectomy.12 The dexamethasone was started 2 weeks after adrenalectomy to reduce the risk of infection and to allow full recovery of the rats. The rats from the sham-operated group were given intramuscular vehicle (olive oil). The intramuscular treatment and vehicle were given to the rats for 8 weeks before sacrifice. All of the rats in the baseline group were sacrificed after 2 weeks of acclimatization in the Animal Unit. The animals were weighed regularly to allow accurate dosing and to monitor the weight gain.

The rats were given diethyl ether (BDH, England) before being sacrificed by cervical dislocation. Pictures of visceral adipose tissue were taken, and perirenal adipose tissues were dissected bilaterally. Some of the adipose tissues were kept at -70°C, and others were fixed in 10 % formalin.

Samples of perirenal adipose tissue were immediately fixed in 10 % formalin, and after 24 hours, the samples were processed using an automatic tissue-processing machine (Microm, Germany). The samples were then embedded in paraffin, and 5 μm sections were obtained. Approximately 25 sections were obtained, and every fifth section was taken for staining. Sections were stained with hematoxylin (Sigma Chemical, USA) and eosin (BDH, England) (H&E) using an automatic staining machine (Leica, Germany). Finally, sections were mounted on dibutyl phthalate in xylene (DPX). Photomicrographs of adipocytes were taken using a camera (CTRMIC from Leica, Germany) and were analyzed with Video T-Test Morphology 5.1 software from Russia. The diameter and the total number of adipocytes were determined.

After samples were fixed in 10 % formalin and processed, 5 μm sections were cut and placed on polysine slides (Thermo Scientific, Germany) for immunohistochemistry. Slides were dewaxed in xylene and dehydrated in a series of alcohol to water. For antigen retrieval, the slides were treated with citrate-buffered solution (200 ml; 0.01 M; pH 6) and rinsed with phosphate-buffered solution (PBS). The slides were then treated with hydrogen peroxide before being incubated with normal goat serum at a dilution of 1:50. Next, the slides were rinsed with PBS and incubated with primary antibody (Cayman Chemical, USA) at a dilution of 1:1000 for 1 hour. Negative-control sections were incubated in PBS without primary antibody. After rinsing with PBS, the tissue-bound primary antibody was detected using biotinylated secondary antibody and the avidin-biotin-peroxidase complex method (Vectastain Elite ABC kit, USA) with diaminobenzidine tetrahydrochloride (DAB) (Vector Laboratories, USA) as the chromogen. Finally, the slides were counterstained with Meyer's Hematoxylin (Richard-Allan Scientific, USA) for 45 seconds and mounted with DPX. Two blinded observers analyzed the slides, and the slides were graded according to the intensity of the immunoreactive stained area. The intensity grading was as follows: no staining was ‘0’; weak staining was ‘1’; mild staining was ‘2’; and strong staining was ‘3’.

The level of 11β-HSD1 dehydrogenase activity in adipose tissue homogenates was determined by measuring the rate of conversion of corticosterone to 11-dehydrocorticosterone, as described by Moison et al., with some modifications.13 Perirenal adipose tissue was homogenized in Krebs-Ringer bicarbonate buffer, and the total protein content was estimated calorimetrically using aliquots of each homogenate. Tissue homogenates containing 0.5 mg of protein were added to a solution of 200 μM NADP (Sigma, Germany), 12 nM [1,2,6,7-3H] corticosterone (American Radioactive Chemicals, USA) and Krebs-Ringer bicarbonate buffer (containing 0.2 % glucose and 0.2 % BSA); the total reaction volume was 250 μl. After incubation in a shaking water bath at 37°C for 1 hour, the reaction was arrested by the addition of 1 ml of ethyl acetate, and the steroids were extracted by centrifugation at 4°C and 3000 rpm for 10 minute. The top layer was then transferred and evaporated to dryness at 55°C before being dissolved in ethanol containing corticosterone and 11-dehydrocorticosterone. The steroid residue was separated using thin-layer chromatography (Whatman, Germany) in chloroform and 95 % ethanol at a ratio of 92:8. The bands containing the labeled corticosterone and 11-dehydrocorticosterone were identified by UV light at 240 nm, scraped and transferred into scintillation vials containing scintillation fluid before being counted with a β-counter (Wallac 1409, Finland). The percentage conversion of corticosterone to 11-dehydrocorticosterone was calculated.

The results are expressed as mean ± standard error mean (SEM). The means were compared using one-way analysis-of-variance (ANOVA) followed by Tukey's post hoc test and a t-test. All of the statistical analyses were performed using the Statistical Package for Social Sciences (SPSS) software.

Adrenalectomized rats treated with dexamethasone (ADR+Dexa) showed less weight gain compared with rats from the sham-operated group following 8 weeks of treatment (Fig. 2(a)).

Figure 2.

(a) Average body weight of the adrenalectomized rats treated with dexamethasone (ADR+Dexa) revealed that these rats gained less weight than the sham-operated rats after 8 weeks. a p<0.05 indicates a significant difference between the ADR+Dexa group and the sham-operated group. # p<0.05 indicates a significant difference between week 1 and week 8 for the sham-operated rats. (b) The diameter of adipocytes of the adrenalectomized rats treated with dexamethasone (ADR+Dexa) was smaller than that of adipocytes from baseline control and sham-operated rats. (c) The number of adipocytes per slide was greater for adrenalectomized rats treated with dexamethasone (ADR+Dexa) than for baseline control and sham-operated rats. (d) The expression level of 11β-HSD1 in adrenalectomized rats treated with dexamethasone (ADR+Dexa) was significant higher than that in baseline control and sham-operated rats. (e) The dehydrogenase activity of 11β-HSD1 of the adrenalectomized rats treated with dexamethasone (ADR+Dexa) was significantly greater than that of the baseline control and sham-operated rats.a p<0.05 indicates a significant difference between the ADR+Dexa group and the baseline control and sham-operated groups.

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Adrenalectomized rats treated with dexamethasone (ADR+Dexa) and rats from sham-operated groups showed more visceral fat deposition compared with the baseline control group (Fig. 1(a)).

Figure 1.

(a) An adrenalectomized rat treated with dexamethasone (ADR+Dexa) and a rat from the sham-operated group had more visceral fat deposition (perirenal fat—red arrows; mesenteric fat—blue arrows) compared with the rat from the baseline control group. (b) The number of adipocytes per slide (H&E staining) was greater in the adrenalectomized rats treated with dexamethasone (ADR+Dexa), but the diameters of these cells were smaller than those seen in rats from the sham-operated and baseline control groups. The circles show hyperplasia of adipocytes, and the arrows show blood vessels. Magnification X 20. (c) Immunoreactive staining of 11β-HSD1 in adrenalectomized rats treated with dexamethasone (ADR+Dexa) showed stronger immunoreactive staining compared with that of the baseline control and sham-operated rats. Magnification X 20.

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Individual adipocytes in adrenalectomized rats treated with dexamethasone (ADR+Dexa) had significantly smaller diameters than the sham-operated and baseline control groups (Figs. 1(b) and 2(b)). The average number of adipocytes on one slide for adrenalectomized rats treated with dexamethasone was significantly greater than that of sham-operated and baseline control rats (Figs. 1(b) and 2(c)).

Expression of 11β-HSD1 was greater in adrenalectomized rats treated with dexamethasone (ADR+Dexa) than in sham-operated and baseline control groups (Figs. 1(c) and 2(d)).

The dehydrogenase activity of 11β-HSD1 in adrenalectomized rats treated with dexamethasone (ADR+Dexa) was significantly higher than that in the sham-operated and baseline control rats (Fig. 2(e)).