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Isolation and culture of adult Sertoli cells and their effects on the function of co-cultured allogeneic islets in vitro

机译:成年支持细胞的分离培养及其对异基因胰岛共培养功能的影响

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Background Globally, 180 million people suffer from diabetes mellitus. Islet transplantation is believed to be an almost ideal therapy for insulin-dependent patients. How to maintain the viability and the function of isolated human islets is a challenge in clinical practice. Sertoli cells are considered ' nurse cells' in the seminiferous tubules and have been used in cell graft protocols for neurodegenerative diseases and diabetes in many studies. Many researchers have used immature murine testes as the primarily source of Sertoli cells in islet transplantation because they are easily purified. Mature human Sertoli cells have been seldom investigated. In the present study, we developed a method for the isolation and culture of Sertoli cells derived from adult human testes, and investigated their effects on the function of allogeneic islets when they were cultured together in vitro. Methods Adult Sertoli cells were prepared successfully by two-step enzyme digestion with trypsin, collagenase and hyaluronidase. They were identified by morphological characteristics and their activity was determined by MTT colorimetry over a 28-day culture time in vitro. A glucose-stimulated insulin secretion test was performed to detect the effects of Sertoli cells on allogeneic islets' function when they were co-cultured for 21 days in vitro. Results In cultured cells, mature human Sertoli cells accounted for more than 90% of total cells. The activity of Sertoli cells reached 95 % and they remained highly cytoactive for a long time in vitro ( P > 0. 05 ). Compared with the islets cultured alone, the co-cultured islets with allogeneic Sertoli cells maintained higher sensitivity to glucose stimulation for the duration of the experiment (P <0. 01). Conclusions A method of isolation and culture of Sertoli cells from adult testes has been established. Sertoli cells could enhance allogeneic islets' function when they were co-cultured in vitro. They could be a helper cell in islet transplantation.
机译:背景技术全球有1.8亿人患有糖尿病。胰岛移植被认为是胰岛素依赖型患者几乎理想的疗法。如何维持离体的人类胰岛的生存力和功能是临床实践中的一个挑战。睾丸支持细胞被认为是曲细精管中的“护士细胞”,在许多研究中已被用于神经变性疾病和糖尿病的细胞移植方案中。许多研究人员已将未成熟的鼠睾丸用作胰岛移植中支持细胞的主要来源,因为它们易于纯化。很少研究成熟的人类支持细胞。在本研究中,我们开发了一种分离和培养源自成人睾丸的支持细胞的方法,并研究了它们在体外一起培养时对同种异体胰岛功能的影响。方法采用胰蛋白酶,胶原酶和透明质酸酶两步酶切法成功制备成年的支持细胞。通过形态特征鉴定它们,并通过MTT比色法在体外28天的培养时间内确定它们的活性。进行葡萄糖刺激的胰岛素分泌试验,以检测Sertoli细胞在体外共培养21天时对同种异体胰岛功能的影响。结果在培养的细胞中,成熟的人支持细胞占总细胞的90%以上。 Sertoli细胞的活性达到95%,并且在体外长时间保持高细胞活性(P> 0. 05)。与单独培养的胰岛相比,在实验期间,同种异体支持细胞共培养的胰岛对葡萄糖刺激的敏感性更高(P <0.01)。结论建立了成年睾丸支持细胞的分离培养方法。 Sertoli细胞在体外共培养时可以增强同种异体胰岛的功能。它们可能是胰岛移植的辅助细胞。

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