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从成年大鼠睾丸分离的纯化睾丸间质细胞的原代培养。

Primary culture of purified Leydig cells isolated from adult rat testes.

作者信息

Browning J Y, Heindel J J, Grotjan H E

出版信息

Endocrinology. 1983 Feb;112(2):543-9. doi: 10.1210/endo-112-2-543.

DOI:10.1210/endo-112-2-543
PMID:6848362
Abstract

Methods for isolating highly purified Leydig cells permit the study of acute responses and biochemical properties of Leydig cells independent of other testicular cell types. The present study describes the development of a primary culture system for purified Leydig cells from adult rats in which the cells retain their ability to secrete testosterone for at least 72 h in culture. When Leydig cells were cultured in tissue culture medium 199--0.1% BSA (M199-BSA), basal testosterone secretion declined by 72 h, whereas hCGB-stimulated testosterone secretion was reduced by 48 h. Changing the culture medium twice daily or adding 0.5% fetal calf serum (fcs) enhanced basal and gonadotropin-stimulated testosterone secretion at 72 h in culture, although responsiveness to hCG was reduced to 57% of that in freshly isolated cells. Incubation of Leydig cells in the defined culture medium Dulbecco's Modified Eagles-Ham's F-12 (1:1, vol/vol) supplemented with 15 mM Hepes buffer, transferrin, insulin, and epidermal growth factor (DHG:F12 + Hepes + TIE) in either the presence or absence of 0.5% fcs yielded functional Leydig cells for longer intervals in culture. Furthermore, testosterone secretion was greater in DHG:F12 + Hepes + TIE than in M199-BSA at all time intervals tested. In DHG:F12 + Hepes + TIE, basal and gonadotropin-stimulated testosterone production by Leydig cells were maintained for 72 h in culture. Degenerative changes in morphology were apparent in some cells at 72 h, but not at earlier times in culture. This primary culture system for isolated Leydig cells provides a valuable tool to examine the temporally regulated events in Leydig cell function.

摘要

分离高纯度睾丸间质细胞的方法使得对睾丸间质细胞急性反应和生化特性的研究能够独立于其他睾丸细胞类型进行。本研究描述了一种用于从成年大鼠中分离纯化睾丸间质细胞的原代培养系统的建立,在该系统中,细胞在培养过程中至少72小时保持分泌睾酮的能力。当睾丸间质细胞在含有0.1%牛血清白蛋白的组织培养基199(M199 - BSA)中培养时,基础睾酮分泌在72小时时下降,而人绒毛膜促性腺激素(hCGB)刺激的睾酮分泌在48小时时减少。每天更换两次培养基或添加0.5%胎牛血清(fcs)可增强培养72小时时基础和促性腺激素刺激的睾酮分泌,尽管对hCG的反应性降至新鲜分离细胞的57%。在含有15 mM Hepes缓冲液、转铁蛋白、胰岛素和表皮生长因子(DHG:F12 + Hepes + TIE)的限定培养基Dulbecco改良Eagle培养基 - Ham's F - 12(1:1,体积/体积)中培养睾丸间质细胞,无论是否存在0.5% fcs,都能在更长的培养时间内产生功能性睾丸间质细胞。此外,在所有测试的时间间隔内,DHG:F12 + Hepes + TIE中的睾酮分泌均高于M199 - BSA中的分泌。在DHG:F12 + Hepes + TIE中,睾丸间质细胞基础和促性腺激素刺激的睾酮产生在培养72小时时得以维持。在72小时时,一些细胞出现明显的形态退化变化,但在培养早期未出现。这种分离睾丸间质细胞的原代培养系统为研究睾丸间质细胞功能中受时间调控的事件提供了一个有价值的工具。

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