Abstract

The hypothesis that some types of damage to DNA may be involved in the aging process will be investigated using a model system, adrenocortical cells in culture. Some of the damage to DNA in aging may result from the toxic side-effects of oxygen. Adrenocortical cells form a useful system for investigating the role of this oxidative damage in aging. Both human and bovine adrenocortical cells are well-studied systems for investigating cell culture senescence. Protocols to increase or decrease the amount of oxidative damage occurring in cultured adrenocortical cells will be developed, by changing the oxygen concentration at which the cells are grown; by modifying the glutathione content of the cells; by varying the tocopherol and selenium status of the cells, by depletion and selective readdition; by addition of other biological or synthetic antioxidants; by irradiation; and by addition of peroxides or superoxide-generating systems. The effectiveness of these protocols will be assessed by release of 45Ca; measurement of changes in superoxide dismutase, catalase, and glutathione peroxidase, the principal cellular enzymatic defenses against oxidative damage; assessment of cellular levels of ubiquinone, which is sensitive to oxidative damage; and fluorescence microscopic determination of lipofuscin, a measure of an oxidative damage product in the living cell. Using protocols that yield varying degrees of oxidative damage, the amount of damage to DNA will be measured, by unscheduled DNA synthesis, a measure of DNA repair; by poly(ADP-ribose) synthesis, a response to DNA damage; by sister chromatid exchange rate; and by frequency of chromosome aberrations. These assays measure viable cell responses to damage to DNA and have been shown to respond to oxidative damage. Such protocols will then be tested for effects on replicative potential (life span) and cloning efficiency, to determine if the replicative life span is associated with the level or type of oxidative damage incurred by the cells and with the level or type of DNA damage. Some of these protocols will be used to examine losses of differentiated functions during culture senescence. Functions to be measured are ACTH receptor content; ACTH- and PGE1-stimulated cyclic AMP production; mitogenic response to angiotensin II; restimulated levels of steroidogenic cytochrome P-450 enzymes (11-hydroxylase, cholesterol side-chain cleavage, 21-hydroxylase, and 17-hydroxylase); P-450 enzymes involved in benzo[a]pyrene metabolism; 3beta-hydroxysteroid dehydrogenase; and synthesis of prostaglandins. Differentiated functions may be affected directly by oxidative damage, or secondary to DNA damage.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute on Aging (NIA)
Type
Research Project (R01)
Project #
5R01AG006108-02
Application #
3116901
Study Section
Molecular Cytology Study Section (CTY)
Project Start
1985-08-01
Project End
1987-03-31
Budget Start
1986-04-01
Budget End
1987-03-31
Support Year
2
Fiscal Year
1986
Total Cost
Indirect Cost

  Institution

Name
Medical College of Georgia (MCG)
Department
Type
Schools of Medicine
DUNS #
City
Augusta
State
GA
Country
United States
Zip Code
30912

  Publications

Hornsby, P J; Thomas, M; Northrup, S R et al. (1998) Cell transplantation: a tool to study adrenocortical cell biology, physiology, and senescence. Endocr Res 24:909-18
Endoh, A; Yang, L; Hornsby, P J (1998) CYP21 pseudogene transcripts are much less abundant than those from the active gene in normal human adrenocortical cells under various conditions in culture. Mol Cell Endocrinol 137:13-9
Kristiansen, S B; Endoh, A; Casson, P R et al. (1997) Induction of steroidogenic enzyme genes by insulin and IGF-I in cultured adult human adrenocortical cells. Steroids 62:258-65
Didenko, V V; Hornsby, P J (1996) A quantitative luminescence assay for nonradioactive nucleic acid probes. J Histochem Cytochem 44:657-60
Didenko, V V; Wang, X; Yang, L et al. (1996) Expression of p21(WAF1/CIP1/SDI1) and p53 in apoptotic cells in the adrenal cortex and induction by ischemia/reperfusion injury. J Clin Invest 97:1723-31
Didenko, V V; Hornsby, P J (1996) Presence of double-strand breaks with single-base 3' overhangs in cells undergoing apoptosis but not necrosis. J Cell Biol 135:1369-76
Yang, L; Didenko, V V; Noda, A et al. (1995) Increased expression of p21Sdi1 in adrenocortical cells when they are placed in culture. Exp Cell Res 221:126-31
Maghsoudlou, S S; Hughes, T R; Hornsby, P J (1995) Analysis of the distal 5' region of the human CYP17 gene. Genome 38:845-9
Cheng, C Y; Hornsby, P J (1992) Expression of 11 beta-hydroxylase and 21-hydroxylase in long-term cultures of bovine adrenocortical cells requires extracellular matrix factors. Endocrinology 130:2883-9
Lala, D S; Hornsby, P J (1992) Activity of the CYP17 promoter in bovine adrenocortical cells before and after phenotypic switching. Mol Cell Endocrinol 89:19-24

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