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与支持细胞或支持细胞条件培养基共培养对睾丸间质细胞功能的调节:胰岛素、生长调节素-C和促卵泡激素的作用

Modulation of Leydig cell functions by culture with Sertoli cells or with Sertoli cell-conditioned medium: effect of insulin, somatomedin-C and FSH.

作者信息

Perrard-Sapori M H, Chatelain P C, Rogemond N, Saez J M

出版信息

Mol Cell Endocrinol. 1987 Apr;50(3):193-201. doi: 10.1016/0303-7207(87)90017-7.

Abstract

The potential regulatory action of Sertoli cells on Leydig cell functions has been investigated by using a coculture system of Leydig and Sertoli cells obtained from immature pig or by culturing Leydig cells with Sertoli cell-conditioned medium (SCCM). Coculture of Leydig and Sertoli cells for 48 h in the absence of insulin or somatomedin-C (Sm-C), produced a small but significant increase in both hCG receptors and hCG-induced testosterone production. Addition to the medium of pFSH (100 ng/ml), insulin (5 micrograms/ml) or somatomedin-C (50 ng/ml) produced a marked increase in these two parameters of Leydig cell function. A further significant increase was observed when pFSH was associated with insulin or Sm-C. In contrast, coculture of Leydig cells with aortic endothelial cells decreased both the hCG receptor number and the hCG responsiveness. SCCM stimulated Leydig cell testosterone production following a 4 h incubation. The stimulation depended upon the amount of SCCM used and the conditions in which Sertoli cells were cultured. The most active was the medium from cells cultured in the presence of pFSH and insulin at high concentrations. Since pig Sertoli cells have specific somatomedin-C receptors, but not insulin receptors, it is likely that the effect of micromolar concentrations of insulin are exerted through Sm-C receptors. In addition, SCCM produced a long-term effect after 48 h incubation. SCCM from cells cultured in the absence of insulin and pFSH inhibited both the hCG receptor number and hCG responsiveness. A similar inhibition was observed with SCCM medium from cells cultured without insulin but with pFSH.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过使用从未成熟猪获取的睾丸间质细胞和支持细胞共培养系统,或用支持细胞条件培养基(SCCM)培养睾丸间质细胞,研究了支持细胞对睾丸间质细胞功能的潜在调节作用。在无胰岛素或生长调节素C(Sm - C)的情况下,睾丸间质细胞与支持细胞共培养48小时,人绒毛膜促性腺激素(hCG)受体和hCG诱导的睾酮产生均有小幅但显著增加。向培养基中添加垂体促卵泡素(pFSH,100 ng/ml)、胰岛素(5微克/ml)或生长调节素C(50 ng/ml),睾丸间质细胞功能的这两个参数显著增加。当pFSH与胰岛素或Sm - C联合使用时,观察到进一步显著增加。相反,睾丸间质细胞与主动脉内皮细胞共培养会降低hCG受体数量和hCG反应性。SCCM孵育4小时后刺激睾丸间质细胞睾酮产生。刺激程度取决于所用SCCM的量以及支持细胞的培养条件。最具活性的是在高浓度pFSH和胰岛素存在下培养的细胞的培养基。由于猪支持细胞有特异性生长调节素C受体,但无胰岛素受体,微摩尔浓度胰岛素的作用可能是通过Sm - C受体发挥的。此外,SCCM孵育48小时后产生长期效应。无胰岛素和pFSH培养的细胞的SCCM会抑制hCG受体数量和hCG反应性。在无胰岛素但有pFSH培养的细胞的SCCM培养基中也观察到类似抑制作用。(摘要截断于250字)

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