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转化生长因子-β1对培养的猪支持细胞乳酸生成的直接调节作用。

Direct regulating effects of transforming growth factor-beta 1 on lactate production in cultured porcine Sertoli cells.

作者信息

Esposito G, Keramidas M, Mauduit C, Feige J J, Morera A M, Benahmed M

机构信息

CJF INSERM 90-08, Hopital Sainte Eugénie, Centre Hospitalier Lyon-Sud, Pierre Bénite, France.

出版信息

Endocrinology. 1991 Mar;128(3):1441-9. doi: 10.1210/endo-128-3-1441.

Abstract

In the present study we have tested the direct effects of transforming growth factor-beta 1 (TGF beta 1) on lactate production by Sertoli cells isolated from immature porcine testes. In Sertoli cells cultured in a defined medium, TGF beta 1 was shown to stimulate lactate production in a time- and dose-dependent manner. The maximal and half-maximal effects of TGF beta 1 on lactate production were obtained in the picomolar concentration range, respectively 24 and 8 pM TGF beta 1. TGF beta 1 action was found closely related to that of insulin since 1) both TGF beta 1 (40 pM) and insulin (1 microgram/ml) induced the secretion of similar and nonadditive amounts of lactate; and 2) TGF beta 1 and insulin induced comparable increases in lactate production in FSH (1 microgram/ml)-treated Sertoli cells. Because lactate is derived from glucose, 2-deoxy-D-glucose (2-DOG) was used to investigate the hexose transport system of Sertoli cells after insulin, FSH, and TGF beta 1 treatments. Insulin (1 microgram/ml) and FSH (1 microgram/ml) were found to stimulate 2-DOG transport with a similar time course, with an effect detected up to 30 min and maximal at 150 min. In contrast, although TGF beta 1 also enhanced 2-DOG uptake by Sertoli cells, the increase in glucose transport was delayed, since the TGF beta 1 effect was first detected at 150 min and was maximal at 360 min. These effects of TGF beta 1 action on Sertoli cell activity are exerted through specific membrane TGF beta 1 receptors. Scatchard analysis of the binding of TGF beta 1 to cultured Sertoli cells revealed the presence of both a high affinity (Kd, approximately 180 pM) and a low affinity binding site systems for TGF beta 1. Affinity labeling of these receptors by covalent attachment to [125I] TGF beta 1 with disuccinimidyl suberate and subsequent electrophoretic analysis of the labeled complexes revealed the specific binding of [125I] TGF beta 1 to three predominant molecules of 260, 130, and 70 kDa. In conclusion, the present study demonstrates that testicular Sertoli cells are targets for TGF beta 1 action. In view of the importance of lactate as a substrate for germ cells, it is suggested that TGF beta 1 might also be involved in the development of normal germinal epithelium.

摘要

在本研究中,我们测试了转化生长因子β1(TGFβ1)对从未成熟猪睾丸分离的支持细胞乳酸生成的直接影响。在限定培养基中培养的支持细胞中,TGFβ1呈时间和剂量依赖性地刺激乳酸生成。TGFβ1对乳酸生成的最大和半数最大效应分别在皮摩尔浓度范围内获得,即24 pM和8 pM的TGFβ1。发现TGFβ1的作用与胰岛素密切相关:1)TGFβ1(40 pM)和胰岛素(1微克/毫升)诱导分泌相似且无相加作用量的乳酸;2)TGFβ1和胰岛素在FSH(1微克/毫升)处理的支持细胞中诱导乳酸生成有相当程度的增加。由于乳酸源自葡萄糖,因此使用2-脱氧-D-葡萄糖(2-DOG)来研究胰岛素、FSH和TGFβ1处理后支持细胞的己糖转运系统。发现胰岛素(1微克/毫升)和FSH(1微克/毫升)以相似的时间进程刺激2-DOG转运,在30分钟时可检测到效应,150分钟时达到最大。相比之下,尽管TGFβ1也增强了支持细胞对2-DOG的摄取,但葡萄糖转运的增加出现延迟,因为TGFβ1的效应在150分钟时首次检测到,360分钟时达到最大。TGFβ1对支持细胞活性的这些作用是通过特异性膜TGFβ1受体发挥的。对TGFβ1与培养的支持细胞结合进行Scatchard分析显示存在TGFβ1的高亲和力(Kd,约180 pM)和低亲和力结合位点系统。用辛二酸二琥珀酰亚胺酯将[125I]TGFβ1共价连接对这些受体进行亲和标记,随后对标记复合物进行电泳分析,结果显示[125I]TGFβ1与260、130和70 kDa的三个主要分子特异性结合。总之,本研究表明睾丸支持细胞是TGFβ1作用的靶点。鉴于乳酸作为生殖细胞底物的重要性,提示TGFβ1可能也参与正常生精上皮的发育。

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