A possible role for a low molecular weight peptide in regulation of testosterone production by rat Leydig cells.

Sodium dodecyl sulphate-polyacrylamide gel electrophoresis of Percoll purified Leydig cell proteins from 20- and 120-day-old rats revealed a significant decrease in a low molecular weight peptide in the adult rats. Administration of human chorionic gonadotropin to immature rats resulted in a decrease in the low molecular weight peptide along with increase in testosterone production. Modulation of the peptide by human chorionic gonadotropin could be confirmed by Western blotting. The presence of a similar peptide could be detected by Western blotting in testes of immature mouse, hamster, guinea pig but not in adrenal, placenta and corpus luteum. Administration of testosterone propionate which is known to inhibit the pituitary luteinizing hormone levels in adult rats resulted in an increase in the low molecular weight peptide, as checked by Western blotting. It is suggested that this peptide may have a role in regulation of acquisition of responsiveness to luteinizing hormone by immature rat Leydig cells.     

Effect of estradiol on the metabolism of testosterone by rat prostate

Prostatic tissue from normal, estradiol-treated, and castrated rats was incubated with testosterone, and the metabolites formed were studied. Pretreatment with estradiol-17β did not affect the total amount of testosterone metabolized per unit weight of tissue. In contrast, the total amount of testosterone metabolized was significantly reduced following castration. The formation of dihydrotestosterone (17β-hydroxy-5α-androstan-3-one; DHT) was not affected by treatment with estradiol, but was significantly reduced by previous castration. Estradiol treatment enhanced the formation of 17-keto metabolites of testosterone by the prostate, giving lower 17-hydroxy to 17-keto ratios than incubations with prostates from control or castrated rats. These results are consistent with the theory that the mechanisms leading to the involution of prostate after estradiol treatment and after castration are different.     

Some effects of testosterone on the rat ventral prostate

1. Labelled testosterone, injected directly into the ventral prostate of castrated rats became associated, in part, with a cytoplasmic high-molecular-weight fraction, fraction ;A'. 2. The label present in fraction ;A' was found to be mainly associated with dihydrotestosterone. 3. Unlike fraction ;A' from testosterone-pelleted castrated rats, fraction ;A' obtained from untreated castrated rats, 48h or more after castration, was strongly inhibitory towards Escherichia coli RNA polymerase in vitro. 4. The inhibition of RNA polymerase by fraction ;A' from castrated rats was not changed by the addition of testosterone or dihydrotestosterone in vitro, but pre-heating it to 80 degrees C resulted in a loss of its inhibitory capacity. 5. Fraction ;A' from castrated rats contained ribonuclease activity. The elution profile of ribonuclease activity from Sephadex columns indicated that this activity was responsible for the inhibitory effect on the RNA polymerase assays. 6. It is concluded that, unlike the inhibitor present in the uterus of ovariectomized rats (Talwar, Segal, Evans & Davidson, 1964), no direct connexion exists between the steroid-binding capacity of prostatic fraction ;A' and its effect on E. coli RNA polymerase activity in vitro.     

Propranolol stimulates histone phosphorylation by a putative PK-C in partially purified homogenate of rat testicular interstitial cells. A possible mechanism for increased testosterone secretion by propranolol.

The beta-adrenoceptor blocker propranolol stimulated testosterone secretion by rat testicular interstitial cells (Leydig cell-enriched preparation) in vitro at concentrations ranging from 10(-5) M to 10(-4) M. Treatment of these cells with H7 (20 microM), an inhibitor of protein kinase C, reduced the stimulatory effect of L-propranolol on testosterone secretion by about 5-fold. At concentrations ranging from 31.25 microM to 1000 microM, L-propranolol reduced [3H]phorbol 12,13-dibutyrate binding (IC50 = 75 microM) to rat testicular interstitial cells. At similar concentrations, L-propranolol displaced the binding of [3H]phorbol 12,13-dibutyrate to the homogenate of these cells by only 5%. These findings suggest that the effect of L-propranolol on [3H]phorbol 12,13-dibutyrate binding could be indirect, possibly by increasing the concentration of a chemical mediator interacting with the regulatory domain of protein kinase C. At even lower concentrations (10(-9) M to 10(-7) M), propranolol added directly to the reaction mixture with protein kinase C partially purified from rat testicular interstitial cells increases the phosphorylation of histone. This phosphorylation was comparable to that obtained with (25 microg/ml) phosphatidylserine. The D- and L-stereoisomers of propranolol were equally active. A complete reversal of this propranolol effect on histone phosphorylation was achieved with (20 microM) H-7. In the absence of Ca2+, propranolol was not able to phosphorylate the histone. Taken together, these results suggest that protein kinase C could be the putative kinase involved in this reaction and that its activation by propranolol may be due to interaction of the drug with the regulatory domain of the enzyme at a site differing from the site of interaction with phorbol 12,13-dibutyrate. The ability of propranolol to activate the putative protein kinase C could be related to its stimulatory effect on testosterone secretion by Leydig cells.     

The hypertriglyceridaemia of the cobalt chloride-treated rat: A possible mechanism

The cobalt chloride-treated rat is an animal model of induced hypertriglyceridaemia. Associated with the hyperlipaemia is an increase in hepatic triglyceride and decrease in total body lipid content. Lipoprotein lipase (EC.3.1.1.3), the enzyme responsible for regulation of the rate of uptake of triglyceride by adipose tissue was investigated and its activity shown to be reduced by cobalt treatment. Plasma post-heparin lipoprotein lipase activity was also reduced in the cobalt chloride-treated rat and plasma clearance of exogenous triglyceride was halved. The heavy metal ions, Zn⁺⁺, Cu⁺⁺ and Fe⁺⁺, reduced post-heparin lipoprotein lipase activity. These findings suggest a possible mechanism for production of the hypertriglyceridaemia by cobalt chloride involving a decrease in plasma triglyceride clearance coupled with a possible increase in hepatic triglyceride production.     

A possible physiological function of pancreatic pro-colipase activation peptide in appetite regulation

Pancreatic pro-colipase activation peptide, a pentapeptide with the sequence VPDPR was found to significantly suppress food intake of 20 h fasted Sprague-Dawley rats in a dose-dependent way. A rat treated with pro-colipase-enriched pellets for 26 days showed decreased daily food intake and retarded growth, which were restored during a following period of regular feeding. Genetically obese Zucker rats (fa/fa) were found to contain a reduced content of pancreatic pro-colipase (60% reduction), whereas the pancreatic lipase content was normal. A physiological function of pancreatic pro-colipase activation peptide as an endogenous satiety signal is suggested.     

The regulation by growth hormone of microsomal testosterone 6 beta-hydroxylase in male rat livers

The relationship between growth hormone and testosterone (T) 6 beta-hydroxylase was investigated in normal and hypophysectomized (hypox) male rats. The administration of human growth hormone (hGH) by either intermittent injections or continuous infusion to normal and hypox rats decreased the activity of T 6 beta-hydroxylase in hepatic microsomes. Hypophysectomy did not reduce, but rather increased the 6 beta-hydroxylase activity, while the 16 alpha-hydroxylase activity decreased. These results, together with the data from a Western blot, indicate that growth hormone acts as a repressive factor for the expression of T 6 beta-hydroxylase in a manner different from the regulation of T 16 alpha-hydroxylase.     

睾丸酮对大鼠前列腺上皮细胞有丝分裂方向的影响

目的探讨丙酸睾丸酮（T）对大鼠前列腺上皮细胞染色体有丝分裂方向的影响及其差异基因表达。方法 SPF级SD雄性大鼠（110~130 g）20只,随机分为2组。深麻醉下对所有大鼠进行去势手术,恢复一周后,给药组大鼠皮下注射T,每只0.5 mg,每日1次,连续30d;对照组大鼠皮下注射橄榄油0.1 mL。取前列腺。通过免疫组化、HE染色观察结果。并做基因芯片检查差异基因表达谱。结果给药组大鼠前列腺发生形态学增生。前列腺腺腔扩张,腺上皮高度明显增高,前列腺增生。且前列腺上皮细胞染色体有丝分裂的方向与基底膜平行,而对照组前列腺上皮细胞有丝分裂的方向与基底膜垂直。AR免疫组化染色后发现给药组的前列腺上皮中,均可见到AR标记的阳性细胞,而对照组均为阴性。基因芯片和RT-PCR结果：促进细胞增殖的基因如雄激素受体相关蛋白（RAN）、TGM4和Wnt通道的WNT2等基因均上调,而抑制细胞增殖的基因如负调控Wnt通道的DKK3和促进细胞凋亡的Fas等基因下调。结论 T注射后改变了前列腺上皮细胞有丝分裂的方向,Wnt和AR信号转导通路参与了细胞增殖和有丝分裂方向改变。     

Metabolism of testosterone by tes epididymis and ventral prostate of rat and its inhibition by cyproterone acetate

The metabolism of ³H-testosterone by the epididymis and accessory organs of adult male rats exposed continuously to microdoses of cyproterone acetate from subcutaneous capsules were studied. The major metabolite of ³M-testosterone in the epididymis, vas deferens and ventral prostate of control rat was dihydrotestosterone while the formation of androstanediol by these tissues was low. The highest percentage of DHT was formed by the ventral prostate and cauda epididymis. In rats exposed to cyproterone acetate for four months, the conversion of testosterone to DHT was inhibited in all the tissues but maximally in the ventral prostate and cauda epididymis. In these rats, the secretory function of the ventral prostate was normal while that of the epididymis was markedly decreased. These data are discussed based on the differential thresholds of androgens required to regulate the functions of the accessory organs.