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Presence of three different estradiol binding proteins in rat prostate cytosol
Affiliation:1. School of Pharmaceutical Sciences, Liaoning University, Shenyang 110036, People''s Republic of China;2. Department of Epidemiology, University of Florida, Gainesville, FL 32608, USA;3. Natural Products Pharmaceutical Engineering Technology Research Center of Liaoning Province, Shenyang 110036, People''s Republic of China;1. School of Life Sciences, Faculty of Medicine, Tianjin University, Tianjin 300072, PR China;2. State Key Laboratory for Chemistry and Molecular Engineering of Medicinal Resources, Guangxi Normal University, Guilin 541004, PR China;3. Key Laboratory of Biotechnology and Bioresources Utilization of Ministry of Education, Dalian Minzu University, Dalian, Liaoning 116024, PR China
Abstract:Depending upon the experimental conditions, three distinct [3H]-17β-estradiol binding entities can be detected in rat prostate cytosol. A protein with characteristics similar to other estrogen receptors is found in prostate cytosol from intact rats. This protein has a sedimentation coefficient of 8S on sucrose gradients. It has a high affinity only for natural and synthetic estrogens. It decreases rapidly after castration (less than 20% of binding activity after 24 hr) and reappears progressively after 8–10 days.A second binding entity with a sedimentation coefficient of 4–5S on sucrose gradients is also observed. It is found both in intact and castrated rats. At low temperatures, the binding of estradiol increases progressively and reaches a maximum after 24–48 hr of incubation as determined by charcoal assay. This binding species is highly specific for natural estrogens but not for diethylstilbestrol and is probably identical with the 4–5S binder.Finally, a third binding entity is found in 24 hr castrated rats with short incubations at 0°C This binding is labile even at low temperatures. Natural and synthetic androgens compete more strongly than estradiol for this binding. This behaviour suggests that the third estradiol binding entity is identical with the androgen receptor.
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