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The Journal of Neuroscience, March 15, 1999, 19(6):2356-2361
Effect of Chronic High-Dose Exogenous Cortisol on Hippocampal Neuronal Number in Aged Nonhuman Primates
James B. Leverenz1, 3, 4, Charles W. Wilkinson2, 4, Molly Wamble1, Shannon Corbin1, Jo Ellen Grabber5, Murray A. Raskind1, 4, and Elaine R. Peskind1, 4 Veterans Affairs Puget Sound Health Care System, 1 Mental Illness Research,
Education, and Clinical Center and 2 Geriatric Research, Education, and Clinical Center, Seattle, Washington 98108, and Departments of 3 Neurology and 4 Psychiatry and Behavioral Sciences, University of Washington School of Medicine, Seattle, Washington 98195, and 5 Washington Regional Primate Research Center, Seattle, Washington 98195
ABSTRACT
Top
Abstract
Introduction
Chronic exposure to increased glucocorticoid concentrations appears to lower the threshold for hippocampal neuronal degeneration in the old rat. It has been proposed that increased brain exposure to glucocorticoids may lower the threshold for hippocampal neuronal degeneration in human aging and Alzheimer's disease. Here, we asked whether chronic administration of high-dose cortisol to older nonhuman primates decreases hippocampal neuronal number as assessed by unbiased stereological counting methodology. Sixteen Macaca nemestrina (pigtailed macaques) from 18 to 29 years of age were age-, sex-, and weight-matched into pairs and randomized to receive either high-dose oral hydrocortisone (cortisol) acetate (4-6 mg/kg/d) or placebo in twice daily palatable treats for 12 months. Hypothalamic-pituitary-adrenal activity was monitored by measuring plasma adrenocorticotropin and cortisol, 24 hr urinary cortisol, and CSF cortisol. Urinary, plasma, and CSF cortisol were elevated, and plasma adrenocorticotropin was reduced in the active treatment group. Total hippocampal volume, subfield volumes, subfield neuronal density, and subfield total neuronal number did not differ between the experimental groups. These findings suggest that chronically elevated cortisol concentrations, in the absence of stress, do not produce hippocampal neuronal loss in nonhuman primates.
Key words: cortisol; aging; nonhuman primate; hippocampus; stereology; CSF cortisol
INTRODUCTION
Rodent studies suggest that prolonged exposure to elevated glucocorticoid (GC) concentrations lowers the threshold for hippocampal neuronal degeneration and loss (Sapolsky et al., 1985
). A few studies suggest GC neurotoxic effects in primates (Uno et al., 1989
Most in vivo studies addressing GC effects on hippocampal neuronal integrity have used either chronic stress or adrenalectomy versus intact animal paradigms and have attributed effects on the hippocampus to changes in endogenous GC levels produced by these paradigms (Uno et al., 1989
Studies in nonhuman primates are more likely to be relevant than rodent studies for evaluating the potential hippocampal neurotoxicity of high-dose GC therapy in older humans or the potential role of chronically elevated endogenous GC in the hippocampal neuronal loss of Alzheimer's disease (Raskind et al., 1982
MATERIALS AND METHODS Animals. Sixteen retired breeder pigtailed macaques (Macaca nemestrina) in middle to late life [mean age, 23.1 ± 1.0 years (mean ± SEM) at termination of experiment; ranged from 18 to 29 years] were selected from the Washington Regional Primate Research Center. There were five males and 11 females. They had been housed in a reproduction colony before the experimental protocol. For the protocol, all were individually housed in the same room. Housing temperature and humidity conditions conformed to the Animal Welfare Act and Guide for the Care and Use of Laboratory Animals. All animals were in good general health. Purina monkey chow was provided during the protocol on a twice daily basis, with fruit supplements. The Washington Regional Primate Research Center is fully accredited by American Association for the Assessment and Accreditation of Laboratory Animal Care International, and all procedures were reviewed and approved by the University of Washington Animal Care and Use Committee.
Treatment protocol. The monkeys were divided into eight pairs matched as closely as possible for age, gender, and weight. Each pair was randomized to receive either high-dose hydrocortisone (cortisol) acetate or placebo for 12 months. The groups did not differ in age (cortisol-treated, 23.1 ± 1.3 years at time of death; placebo, 23.1 ± 1.5 years at time of death) or pretreatment weight (cortisol-treated, 11.1 ± 1.7 kg; placebo, 9.8 ± 1.9 kg; p = 0.63). Because there were 11 females and five males, the groups could not be matched evenly for gender (cortisol-treated, five females and three males; placebo, six females and two males). The initial dose of cortisol was 3.85 mg/kg/d (hydrocortisone acetate; Upjohn, Kalamazoo, MI). This cortisol dose is approximately equivalent to an adult human receiving the commonly prescribed synthetic GC, prednisone, at a dose of 60 mg/d, a very high therapeutic dose (Schimmer and Parker, 1996
Neuroendocrine measures. Plasma cortisol, plasma ACTH, and 24 hr urinary cortisol were measured during the week before the beginning of drug treatment (baseline), after 2 weeks, and after 3, 6, 9, and 12 months of treatment. After a 24 hr adaptation period, total 24 hr urine for cortisol measurement was collected in a metabolic cage designed for that purpose. Containers placed on solid CO2 were positioned under a collection spout and replaced at frequent intervals. Urine containers remained frozen until thawed for volume determinations. All containers from a given monkey for the 24 hr sampling interval were mixed thoroughly after thawing. After volume measurement, 3 ml aliquots of urine for each monkey from each sampling period were stored frozen at
70°C. Urine samples (500 µl) were extracted by mixing thoroughly with 1 ml of chilled methylene chloride, removing an aliquot of the organic phase, and drying. Dried samples were reconstituted with buffer and assayed as described previously for plasma cortisol (Wilkinson et al., 1997
Blood samples for plasma cortisol and ACTH measurements were collected from sedated monkeys (ketamine hydrochloride, 10 mg/kg) using a "squeeze cage" technique by which monkeys were briefly immobilized to allow venipuncture. Blood samples for cortisol and ACTH measurements were drawn within 10 min of sedation of animals. All sampling was done between 9:00 and 10:15 A.M. Blood was stored on ice in chilled polystyrene tubes and cold centrifuged within 1 hr of sample collection; plasma was then separated and stored at
Monkeys were killed during an 8 hr period on 3 consecutive days, with animals from cortisol and placebo groups alternating in sequence. CSF was obtained after prekilling sedation by either lumbar or cisternal puncture. Cortisol concentration was measured in 100 µl aliquots of unextracted CSF with a 125I-radioimmunoassay kit (Pantex, Santa Monica, CA). All samples were measured in the same assay. Interassay and intra-assay coefficients of variation for this method in our laboratory are 7.1 and 3.7%, respectively. To evaluate possible effects of elapsed time from A.M. cortisol dose on cortisol concentrations achieved in the central compartment, we performed Pearson product-moment correlations within treatment groups between
time from A.M. cortisol dose to CSF sampling. Correlations were nonsignificant (r = 0.199 and 0.273 for cortisol and placebo groups, respectively). Therefore, there is no indication that a marked fluctuation in CSF cortisol levels occurred during the 12 hr between successive cortisol doses during the course of the study.
Tissue preparation. After 12 months of treatment, the animals were killed by valium-phenobarbitol injection. Brains were then rapidly removed and sectioned into 0.5-cm-thick coronal blocks of the cerebral hemispheres and 0.5-cm-thick horizontal blocks of the brainstem. The right hemispheric blocks were fixed flat (to maintain gross morphology) between 4% paraformaldehyde-soaked sponges for 36 hr and then stored in PBS, pH 7.4, with 20% sucrose and 0.02% sodium azide. Fixed blocks of temporal lobe from the right hemisphere were serially sectioned on a cryostat at 50 µm. Every twelfth section (600 µm interval) was taken for thionin staining. The left hemisphere and brainstem were rapidly frozen between cooled aluminum plates in a
Stereological counting techniques. All counting was performed blind to treatment condition. Principles of stereology were used to select and count neurons within the subfields of the hippocampus (West and Gundersen, 1990
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Figure 1. Representative coronal sections from rostral to caudal hippocampus (A, C, E, G) and outlines of dentate granule cell layer, hilus, CA2/3, CA1, and subiculum as used in stereological cell counting (B, D, F, H). CA1' (Rosene and Van Hoesen, 1987
Neurohistology. Light microscopic examination for neuropathology was performed (by J. B. Leverenz) on all thionin-stained slides. Slides were examined blind to treatment condition.
Statistical analyses. Values are expressed as mean ± SEM. Differences in neuroendocrine measures over time within each treatment group were evaluated by repeated measures ANOVA. A significant difference over time prompted paired t test comparisons between each treatment time point value and the baseline value in that group. Differences in neuroendocrine measures between treatment groups at each time point were evaluated by unpaired t tests. Differences in hippocampal subfield neuronal counts and volumes between groups also were evaluated by unpaired t tests. To minimize the likelihood of type II error, no correction was made for multiple comparisons.
RESULTS Animals' general condition during study
All monkeys survived the 12 month treatment period in good general health, except for one of the cortisol-treated monkeys. This monkey died of Klebsiella sepsis 2 weeks after the 9 month evaluation point. Although this monkey's brain was removed within 60 min of death, the brain was not used for the analysis of neuronal number in the hippocampal formation. The 12 month weight and weight gain of the placebo-treated monkeys (9.8 ± 1.9 and 0.4 ± 0.3 kg) did not differ from the 12 month weight and weight gain of the cortisol-treated monkeys (11.1 ± 1.7 and 1.0 ± 0.4 kg) (t = 0.87; p = 0.40; and t = 0.82; p = 0.43, respectively, for end weights and weight gain). Brain weights did not differ between cortisol-treated monkeys (93.0 ± 2.6 gm) and placebo-treated monkeys (99.5 ± 4.0 gm) (t = 1.32; p = 0.21).
Endocrine effects of cortisol treatment
Cortisol-treated monkeys tended toward greater, but not statistically significant, weight gain (see previous section) versus the placebo group. Many of the cortisol-treated monkeys, but not those in the placebo group, developed cushingoid features (facial puffiness, buffalo hump). Two of the cortisol-treated animals developed mild glucose intolerance, but none required insulin treatment.
Twenty-four hour urinary cortisol excretion (expressed as nanomoles of cortisol per millimoles of creatinine) at baseline, after 2 weeks, and after 3, 6, 9, and 12 months of treatment are presented in Figure 2. Baseline pretreatment 24 hr urinary cortisol did not differ between cortisol and placebo groups. Within the cortisol-treated group, 24 hr urinary cortisol was significantly increased from baseline at all time points (p < 0.05). Twenty-four hour urinary cortisol was significantly higher in the cortisol-treated group compared with the placebo group at 2 weeks and 3, 6, 9, and 12 months of treatment (p < 0.01). Plasma cortisol concentrations in the cortisol treatment group were significantly higher than baseline values during exogenous cortisol administration at all time points (p < 0.01) and significantly higher than in the placebo treatment group at 3, 6, 9, and 12 months of treatment (p <0.05) (data not shown).
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Figure 2. Twenty-four hour urinary cortisol concentrations (expressed as nanomoles per millimoles creatinine) in placebo- and cortisol-treated groups at baseline (BL), after 2 weeks (wk), and after 3, 6, 9, and 12 months (m) of treatment. *p < 0.05, higher than baseline; p < 0.01, higher than placebo group.
Plasma ACTH concentrations at the same time points are presented in Figure 3. Plasma ACTH did not differ between groups at baseline (p = 0.12). Exogenous cortisol administration appropriately suppressed plasma ACTH concentrations, which were significantly lower than baseline at all treatment time points in the cortisol-treated group (p < 0.01). Plasma ACTH in the cortisol-treated group was significantly lower than in the placebo group at 6, 9, and 12 months of treatment (p < 0.05). Plasma ACTH did not differ over time in the placebo group.
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Figure 3. Plasma ACTH concentrations (expressed as picomoles per liter) in placebo- and cortisol-treated groups at baseline (BL), after 2 weeks (wk), and after 3, 6, 9, and 12 months (m) of treatment. *p < 0.01, lower than baseline;
CSF cortisol concentrations before death are presented in Figure 4. CSF cortisol levels were significantly higher in the cortisol-treated group than in the placebo group (p < 0.01).
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Figure 4. CSF cortisol concentrations (expressed as nanomoles per liter) in placebo- and cortisol-treated groups after 12 months of treatment obtained by lumbar or cisternal puncture in sedated animals before death. *p < 0.01, higher in placebo group.
Hippocampal subfield neuronal numbers and volumes
Hippocampal subfield neuronal numbers, volumes, and density are presented in Table 1. There were no significant differences in neuronal number between groups in any hippocampal subfield (p > 0.20) nor were there significant differences in subfield volumes or densities between treatment groups (p > 0.10). Total hippocampal volumes between groups did not significantly differ (p = 0.64) (data not shown).
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Table 1. Neuronal volume, density, and cell number in five hippocampal regions Neurohistology
There were no apparent differences in perikaryal size, nuclear size, or nuclear density between treatment groups in any hippocampal subfield. The regularity of pyramidal cell layers was indistinguishable between groups.
DISCUSSION These results do not confirm the hypothesis that high-dose chronic exogenous GC administration produces loss of hippocampal neurons in older nonhuman primates. The threefold increase in CSF cortisol found in the treated monkeys indicates that substantial elevations in cortisol concentration were achieved in the CNS. There were no effects of cortisol treatment on neuronal number, density, or volume of any hippocampal subfield. In particular, there was no suggestion that cortisol treatment reduced neuronal number in CA2/3, the area considered most vulnerable to GC neurotoxic effects (Landfield et al., 1981
The current study is not alone in failing to demonstrate that chronic GC administration produces hippocampal neuronal loss. Bodnoff et al. (1995)
Several studies have inferred GC-induced hippocampal neuronal loss in chronically stressed older rats (Kerr et al., 1991
Application of unbiased stereological counting techniques to nonhuman primate studies has failed to demonstrate hippocampal neuronal loss after exogenous cortisol administration in macaques in the current study or after chronic stress associated with increased cortisol secretion in tree shrews (Vollmann-Honsdorf et al., 1997
FOOTNOTES Received July 10, 1998; revised Dec. 1, 1998; accepted Jan. 5, 1999.
This work was supported by National Institutes of Health Grant 2P51RR00166, National Institute on Aging Grant AGO6136, the Alzheimer's Association, and the Department of Veterans Affairs. We gratefully acknowledge the assistance of Bradley T. Hyman and T. Gomez-Isla with the stereological methods, the assistance of William R. Morton as Director of the Washington Regional Primate Research Center, and the tireless technical assistance of Lynne Greenup, Elizabeth Colasurdo, Richard Vertz, Judy Johnson, and Mark Murchison.
Correspondence should be addressed to Dr. Elaine R. Peskind, Veterans Affairs Puget Sound Health Care System, Mental Illness Research, Education and Clinical Center (116 MIRECC), 1660 South Columbian Way, Seattle, WA 98108.
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Copyright © 1999 Society for Neuroscience 0270-6474/99/1962356-06$05.00/0
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