Direct effect of ghrelin on leptin production by cultured rat white adipocytes.

OBJECTIVE: Because ghrelin is known to stimulate adipogenesis, we tested whether ghrelin could contribute to the maintenance of homeostasis, directly affecting rat white adipocyte leptin production. RESEARCH METHODS AND PROCEDURES: Isolated retroperitoneal adipocytes were cultured for 0.5 to 48 hours without (baseline) or with (0.001 to 1 nM) ghrelin alone or in combination with insulin (0.01 to 10 nM) or dexamethasone (1 to 100 nM). Adipocytes were also incubated with ghrelin and inhibitors either of RNA (actinomycin D) or protein synthesis (cycloheximide) or with several concentrations (10 to 1000 nM) of a specific ghrelin antagonist. When cultures were terminated, we evaluated adipocyte leptin secretion and ob mRNA expression. RESULTS: Our data indicate that ghrelin directly enhanced adipocyte leptin release and ob mRNA expression, that the leptin-releasing activity of ghrelin was additive to the action of both insulin and dexamethasone and was abrogated by protein synthesis inhibitors, and that effects of ghrelin on adipocyte ob mRNA expression and release were blocked by coincubation with the specific growth hormone secretagogue receptor 1a antagonist. DISCUSSION: Our study supports the ability of ghrelin to enhance white adipose tissue leptin production by a direct receptor-mediated effect. This activity of ghrelin could play a potentially significant role in rapid restoration of homeostasis after food intake.

Modulatory effects of leptin on leydig cell function of normal and hyperleptinemic rats.

Neonatal L-monosodium glutamate (MSG) administration in rats induces several neuroendocrine and metabolic disruptions. Leptin, the adipocyte product, modulates several neuroendocrine systems including the hypothalamic-pituitary-gonadal (HPG) axis in mammals. The aim of the present study was to determine whether MSG-induced chronic hyperleptinemia could play any relevant role in the hypogonadism developed by male rats when examined in adulthood. We found that 120-day-old MSG male rats displayed significant hyperleptinemia, hypogonadism, and undisturbed basic testis structure and spermatogenesis. In vitro studies in purified Leydig cells from normal (CTR) and MSG-damaged rats revealed that basal and human chorionic gonadotropin (hCG)-stimulated 17-hydroxy-progesterone (17-HO-P(4)), Delta(4)-androstenedione (Delta(4)A) and testosterone (T) secretions were significantly lower in MSG than in CTR cells. Exposure to murine leptin (Mleptin, 10(-8)M) significantly inhibited hCG-elicited T secretion by CTR cells after 180 min incubation. While Mleptin significantly inhibited hCG-stimulated Delta(4)A output and the Delta(4)A:17-OH-P(4) ratio of secretion, conversely, it failed to modify the ratio T:Delta(4)A release by CTR Leydig cells. Interestingly, the effects of Mleptin found on CTR Leydig cells were absent in MSG Leydig cells. Finally, endogenous hyperleptinemia was associated with a significant decrease in Leydig cell expression of Ob-Rb mRNA in MSG rats. In summary, this study demonstrates that: (1) Mleptin inhibited testicular steroidogenesis in CTR rats; (2) MSG-treated rats showed lower in vitro 17-OH-P(4), Delta(4)A and T production under basal and post-hCG stimulation conditions; (3) purified Leydig cells from MSG-treated rats displayed resistance to the inhibitory action of Mleptin on T release, and (4) endogenous leptin exerts a modulatory effect on Leydig cell Ob-Rb mRNA expression. The inhibitory effect of leptin on testicular function is thus abrogated in MSG-damaged rats. The testicular leptin-resistance developed by MSG rats seems to be due to early chronic exposure of Leydig cells to high leptin circulating levels, which in turn down-regulate testicular Ob-Rb expression. It remains to be determined whether the testicular dysfunction of MSG rats can be reversed after correction of hyperleptinemia or whether it is an irreversible effect of the hypothalamic lesion.

Involvement of tumor necrosis factor-alpha in the pathogenesis of autoimmune orchitis in rats.

We studied the testicular macrophages of rats with experimental autoimmune orchitis (EAO) and analyzed whether the tumor necrosis factor-alpha (TNFalpha) is involved in germ cell apoptosis and in Leydig cell steroidogenesis. The EAO was induced in adult male Sprague-Dawley rats by active immunization with testicular homogenate and adjuvants. In the experimental group, a severe orchitis was observed 80 days after the first immunization. ED1- and ED2-positive macrophages were quantified by immunohistochemistry. The TNFalpha concentration of conditioned media from testicular macrophages (TMCM) was determined by ELISA. The number of apoptotic TNF receptor 1 (TNFR1)-positive germ cells was identified by combining in situ end labeling of apoptotic DNA and immunohistochemical techniques. The effect of TNFalpha on Leydig cell testosterone production was determined by RIA. In rats with EAO, we observed a significant increase in the number of TNFalpha-positive testicular macrophages, the TNFalpha concentration in TMCM, and the number of TNFR1-positive germ cells. Sixty percent of TNFR1-positive germ cells were apoptotic. These results suggest that TNFalpha could be involved in the pathogenesis of EAO. Acting together with other local factors such as Fas-FasL, TNFalpha could trigger germ cell apoptosis. We also demonstrated that TNFalpha inhibited in vitro testosterone production in basal and hCG-stimulated Leydig cells from rats with orchitis.

Role of type IV collagen in prolactin release from anterior pituitaries of male rats.

We previously demonstrated that laminin, a component of basement membranes, modulates pituitary hormone secretion. In the present study, we evaluated the effect of type IV collagen, another component of this membrane, on the release of prolactin (PRL) by anterior pituitary gland from adult male rats. Hemipituitaries were incubated for 3 h with type IV collagen or antibodies against it and PRL release was studied. Rabbit IgG to type IV collagen at concentrations of 10(-7) - 10(-5) M had a significant stimulatory effect on PRL release, in comparison to normal rabbit serum IgG or medium alone used as controls. Type IV collagen induced a significant inhibitory effect on basal release of PRL at a concentration of 30 microg/mL. A slight decrease in PRL release was detected in thyrotropin-releasing hormone-stimulated hemipituitaries incubated with type IV collagen at all concentrations used. These results suggest that type IV collagen, similar to laminin-1, modulates PRL released from hemipituitaries, in vitro.

Prolactin effects on testicular interstitial cells in primary cultures

En el presente trabajo se determinaron los efectos de la prolactina (PRL) "in vitro" sobre la esteroidogénesis testicular, utilizando un cultivo primario de células intersticiales de rata inmadura. Las células fueron cultivadas en un medio químicamente definido, con el agregado de insulina y transferrina durante 2 días a 34§C. La producción de andrógenos durante el segundo día de cultivo resultó ser significativamente mayor que en el primer día (3 alfa-Androstandiol (3 alfa-Diol) 5.14 ñ 0.46 vs. 3.74 ñ 0.10 ng/microng ADN, p < 0.001); Testosterona (T) + Dihidrotestosterona (DHT) 0.40 ñ 0.04 vs. 0.34 ñ 0.03 ng/microng ADN, p < 0.001). La curva dosis respuesta para distintas dosis de hCG mostró un ED50= 2.5 mUI/ml. El efecto agudo de la PRL (10, 100 y 1000 ng/ml) sobre la producción basal de 3 alfa/Diol se evaluó luego de 45 h de cultivo. Sólo la dosis de PRL de 1000 ng/ml reveló diferencias significativas con respcto al control y dicho efecto pordría ser debido a su contaminación con LH. En otra serie de experimentos se evaluaron los efectos de menores dosis de la hormona a tiempos prolongados. La PRL (10 ng/ml), agregada durante todo el tiempo de cultivo, causó una inhibición significativa en la producción basal de 3 alfa-Diol, mientras que la respuesta a un estímulo máximo con hCG no varió. Cuando se determinó la producción de T+DHT se observó un cambio notorio en la relación T+DHT/Diol, tanto en condiciones basales (Control: 0.09 vs. PRL: 0.38) como ante el estímulo con hCG...

Prolactin effects on testicular interstitial cells in primary cultures

En el presente trabajo se determinaron los efectos de la prolactina (PRL) "in vitro" sobre la esteroidogénesis testicular, utilizando un cultivo primario de células intersticiales de rata inmadura. Las células fueron cultivadas en un medio químicamente definido, con el agregado de insulina y transferrina durante 2 días a 34ºC. La producción de andrógenos durante el segundo día de cultivo resultó ser significativamente mayor que en el primer día (3 alfa-Androstandiol (3 alfa-Diol) 5.14 ñ 0.46 vs. 3.74 ñ 0.10 ng/microng ADN, p < 0.001); Testosterona (T) + Dihidrotestosterona (DHT) 0.40 ñ 0.04 vs. 0.34 ñ 0.03 ng/microng ADN, p < 0.001). La curva dosis respuesta para distintas dosis de hCG mostró un ED50= 2.5 mUI/ml. El efecto agudo de la PRL (10, 100 y 1000 ng/ml) sobre la producción basal de 3 alfa/Diol se evaluó luego de 45 h de cultivo. Sólo la dosis de PRL de 1000 ng/ml reveló diferencias significativas con respcto al control y dicho efecto pordría ser debido a su contaminación con LH. En otra serie de experimentos se evaluaron los efectos de menores dosis de la hormona a tiempos prolongados. La PRL (10 ng/ml), agregada durante todo el tiempo de cultivo, causó una inhibición significativa en la producción basal de 3 alfa-Diol, mientras que la respuesta a un estímulo máximo con hCG no varió. Cuando se determinó la producción de T+DHT se observó un cambio notorio en la relación T+DHT/Diol, tanto en condiciones basales (Control: 0.09 vs. PRL: 0.38) como ante el estímulo con hCG... (AU)