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1 James Buchanan Brady
Urological Institute, The Johns Hopkins
Hospital, Baltimore, Maryland
Characterization of cytosol and 0.6 M KCl-nuclear androgen and estrogen receptors in
the canine prostate is described, including
methods for assay of these molecules in tissue
samples from intact, adult dogs. Androgen receptors were quantitated by exchange incubations (20 hours for cytosol and 26 hours for nuclear extract at 0 C; incubations at higher temperatures (15 or 30 C) resulted in substantial
reduction of saturable binding activity. Apparently, virtually all the estrogen receptor sites in
cytosol and nuclear extract are unoccupied,
since these were equally filled with H3-estradiol
at 0 C (nonexchange incubation) and 30 C (exchange conditions) during 20-hour incubatlons.
Androgen receptors were assayed using the
synthetic androgen methyltrienolone (R1881),
and estradiol-17
was selected for estrogen
receptor determinations. Using the assay conditions described, neither of these ligands
bound to the sex steroid-binding protein of
canine blood. Steroid competition experiments
indicated that the androgen and estrogen receptors are distinct molecules. Scatchard plot
analyses were linear, suggesting a single class
of high affinity sites for each receptor (Kd's in
the 10-9 to 10-10 mol/l range). Saturable estradiol binding was additionally detected by sucrose gradient analysis of cytosol and nuclear
extract. The 4S sedimentation of the cytosol receptor is typical of prostate cytoplasmic estrogen receptors; the nuclear form sedimented at
5S. The estrogen and androgen binding proteins satisfy criteria that distinguish them from
blood steroid binding proteins and classify
them as intracellular steroid hormone receptors.
Key words: androgen receptor, estrogen receptor, canine prostate, benign prostatic hypertrophy, prostate
Submitted on March 24, 1980
Revised on May 19, 1980
Accepted on May 20, 1980
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