Androgen and prostatic stroma.
- Author:
Yuan-Jie NIU
1
;
Teng-Xiang MA
;
Ju ZHANG
;
Yong XU
;
Rui-Fa HAN
;
Guang SUN
Author Information
- Publication Type:Journal Article
- MeSH: Animals; Biomarkers; Cell Differentiation; drug effects; physiology; Cell Division; drug effects; physiology; Cells, Cultured; Dihydrotestosterone; pharmacology; Dogs; Estradiol; blood; Fibroblast Growth Factor 2; genetics; pharmacology; Gene Expression; Humans; Male; Muscle, Smooth; cytology; physiology; Orchiectomy; Prostate; cytology; physiology; Prostatic Hyperplasia; physiopathology; RNA, Messenger; analysis; Receptors, Androgen; genetics; Receptors, Estrogen; genetics; Stromal Cells; cytology; physiology; Testosterone; blood; Transforming Growth Factor beta; genetics; pharmacology
- From: Asian Journal of Andrology 2003;5(1):19-26
- CountryChina
- Language:English
-
Abstract:
AIMTo investigate the effect of androgen on the proliferation, differentiation and regression of canine prostatic stromal cells in vivo and human stromal cells in vitro.
METHODSTwenty-two dogs, including 15 normal prostate dogs and 7 prostatic hyperplasia dogs, had their serum concentration of testosterone and estrodiol determined by radioimmunoassay before and after castration. The expression of androgen receptor (AR) and estrogen receptor (ER) in the prostate were analysed by immunohistochemistry and semi-quantitative RT-PCR before and after castration. Light microscopy, transmission electron microscopy and TUNEL assay were carried out successively before and after castration to evaluate the prostatic histomorphology. In vitro serum-free cell cultures from human prostatic stroma were established and exposed to dihydrotestosterone (DHT). The proliferation of the cell culture was detected by MTT assay. The expression of TGFbgr, bFGF, AR, and smooth muscle cell (SMC) specific proteins (myosin and/or smoothelin) were detected using immunohistochemistry and RT-PCR. The differentiation from fibroblasts to smooth muscle cells was deduced by measuring the expression of SMC specific proteins.
RESULTSBefore castration, the serum concentrations of testosterone and estrodiol were not statistically different between normal and hyperplasia groups. Following castration, the serum concentration of testosterone decreased rapidly in 2 days, and the concentration of estrodiol had no significant change compared with the pre-castration data. In the prostate, AR was presented in both the epithelial and stromal cells and the AR mRNA level was higher in hyperplasia than in normal prostate tissues (P<0.05). While ER predominantly existed in the prostate stromal cells and the ER mRNA had no difference between the hyperplasia and the normal group. Within the early phase of castration (
CONCLUSIONThe whole prostate gland is an androgen-sensitive organ with both the epithelium and stroma under the control of androgen. Androgen may direct the proliferation, differentiation and regression of stromal cells by regulating the expression of TGFbgr, bFGF, AR and smooth muscle cell specific proteins.
