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大鼠支持细胞和睾丸间质细胞的蛋白质分泌模式受培养条件影响。

Protein secretory patterns of rat Sertoli and peritubular cells are influenced by culture conditions.

作者信息

Kierszenbaum A L, Crowell J A, Shabanowitz R B, DePhilip R M, Tres L L

出版信息

Biol Reprod. 1986 Aug;35(1):239-51. doi: 10.1095/biolreprod35.1.239.

Abstract

An approach combining two-dimensional gel electrophoresis and autoradiography was used to correlate patterns of secretory proteins in cultures of Sertoli and peritubular cells with those observed in the incubation medium from segments of seminiferous tubules. Sertoli cells in culture and in seminiferous tubules secreted three proteins designated S70 (Mr 72,000-70,000), S45 (Mr 45,000), and S35 (Mr 35,000). Cultured Sertoli and peritubular cells and incubated seminiferous tubules secreted two proteins designated SP1 (Mr 42,000) and SP2 (Mr 50,000). SP1 and S45 have similar Mr but differ from each other in isoelectric point (pI). Cultured peritubular cells secreted a protein designated P40 (Mr 40,000) that was also seen in intact seminiferous tubules but not in seminiferous tubules lacking the peritubular cell wall. However, a large number of high-Mr proteins were observed only in the medium of cultured peritubular cells but not in the incubation medium of intact seminiferous tubules. Culture conditions influence the morphology and patterns of protein secretion of cultured peritubular cells. Peritubular cells that display a flat-stellate shape transition when placed in culture medium free of serum (with or without hormones and growth factors), accumulate various proteins in the medium that are less apparent when these cells are maintained in medium supplemented with serum. Two secretory proteins stimulated by follicle-stimulating hormone (FSH) (designated SCm1 and SCm2) previously found in the medium of cultured Sertoli cells, were also observed in the incubation medium of seminiferous tubular segments stimulated by FSH. Results of this study show that, although cultured Sertoli and peritubular cells synthesize and secrete proteins also observed in segments of incubated seminiferous tubules anther group of proteins lacks seminiferous tubular correlates. Our observations should facilitate efforts to achieve a differentiated functional state of Sertoli and peritubular cells in culture as well as to select secretory proteins for assessing their possible biological role in testicular function.

摘要

采用二维凝胶电泳和放射自显影相结合的方法,将支持细胞和睾丸间质细胞培养物中的分泌蛋白模式与曲细精管片段孵育培养基中观察到的模式进行关联。培养的支持细胞和曲细精管中的支持细胞分泌三种蛋白质,分别命名为S70(分子量72,000 - 70,000)、S45(分子量45,000)和S35(分子量35,000)。培养的支持细胞和睾丸间质细胞以及孵育的曲细精管分泌两种蛋白质,分别命名为SP1(分子量42,000)和SP2(分子量50,000)。SP1和S45分子量相似,但等电点不同。培养的睾丸间质细胞分泌一种名为P40(分子量40,000)的蛋白质,完整曲细精管中也可见到,但缺乏睾丸间质细胞壁的曲细精管中则未见到。然而,大量高分子量蛋白质仅在培养的睾丸间质细胞培养基中观察到,而在完整曲细精管的孵育培养基中未观察到。培养条件影响培养的睾丸间质细胞的形态和蛋白质分泌模式。置于无血清培养基(含或不含激素和生长因子)中的睾丸间质细胞会从扁平星状形态转变,培养基中会积累各种蛋白质,而当这些细胞维持在补充血清的培养基中时,这些蛋白质则不太明显。先前在培养的支持细胞培养基中发现的两种受促卵泡激素(FSH)刺激的分泌蛋白(分别命名为SCm1和SCm2),在受FSH刺激的曲细精管片段孵育培养基中也观察到。本研究结果表明,尽管培养的支持细胞和睾丸间质细胞合成和分泌的蛋白质在孵育的曲细精管片段中也有观察到,但另一组蛋白质在曲细精管中却没有对应物。我们的观察结果应有助于努力使培养的支持细胞和睾丸间质细胞达到分化的功能状态,以及选择分泌蛋白来评估它们在睾丸功能中可能的生物学作用。

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