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Department of Surgery, Section of Urology (H.F.S.H., M.T.L., R.J.I.), Department of Pharmacology, Physiology, and Toxicology (S.V.H.), and Preventive Medicine and Community Health Biostatistics Division (S.V.H.), University of Medicine and Dentistry of New Jersey Medical School, Newark, New Jersey 07103; and the Veterans Affair Medical Center (H.F.S.H.), East Orange, New Jersey 07019
Address all correspondence and requests for reprints to: Dr. Hosea F. S. Huang, Department of Surgery Section of Urology, University of Medicine and Dentistry of New Jersey Medical School, 185 South Orange Avenue, Newark, New Jersey 07103.
Previously, we reported that the steady state level of messenger RNA
(mRNA) transcripts of retinoic acid receptors (RAR)
and
in the
testes of 20-day-old rats can be modulated by exogenous testosterone.
These results suggest that androgen regulation of Sertoli cell
functions may involve biochemical events mediated by RAR genes. In this
study, we examined the effects of castration and testosterone
replacement on the steady state level of mRNA transcripts for RAR
and
in the prostate, seminal vesicles, and kidney of the rat.
Northern blot analysis revealed that in intact adult rats, the relative
steady state levels of the 3.4- and 2.7-kilobase (kb) mRNA transcripts
for RAR
and the 3.4-kb transcript for RAR
in the prostate were at
least 20-fold higher than those in the seminal vesicles and kidney. The
relatively high abundance of RAR mRNA transcripts in the prostate
suggests the physiological importance of RAR-mediated processes in this
organ. Castration resulted in an increase in the level of RAR mRNA
transcripts in the prostate and seminal vesicles, reaching a maximum of
2- to 4-fold in the prostate and 15- to 23-fold in the seminal vesicles
within 6 days. On the other hand, the levels of mRNA transcripts of
RAR
and -
in the kidney were reduced by 4050% 1 day after
castration. The effects of castration on RAR mRNA levels in all three
organs were prevented by implantation of 3-cm testosterone capsules at
the time of castration, a regimen that provides physiological levels of
serum testosterone.
In a subsequent experiment, adult male rats were given a single sc
injection of 2 mg testosterone 3 days after castration. This treatment
resulted in an acute suppression of the level of RAR mRNA transcripts
in all three organs within 30 min. Thereafter, the levels of RAR
and
-
mRNA transcripts in the prostate continued to decrease, whereas
those in the seminal vesicles returned to the castrated levels within
6 h. On the other hand, RAR mRNA levels in the kidney rebounded by
1 h and remained at the level found in the untreated castrated
rats.
These results demonstrate that the steady state level of mRNA
transcripts for RAR
and -
in the prostate, seminal vesicles, and
kidney can be modulated by testosterone in organ-specific manners, thus
suggesting that the RAR-mediated processes may be involved in the
effects of androgen in these organs. Furthermore, the relatively low
increment in prostatic RAR mRNA levels after castration compared to
that in the seminal vesicles demonstrates a difference in androgen
responses between these two organs. This difference could dictate the
efficacy of the effects of androgen on cellular function and may
contribute to the disparate vulnerabilities to androgen-related
uncontrolled cell proliferation and/or malignancy in the prostate and
seminal vesicles.
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