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大鼠食管上皮细胞的克隆生长与连续传代培养

Clonal growth and serial propagation of rat esophageal epithelial cells.

作者信息

Babcock M S, Marino M R, Gunning W T, Stoner G D

出版信息

In Vitro. 1983 May;19(5):403-15. doi: 10.1007/BF02619557.

Abstract

The clonal growth and serial propagation of rat esophageal epithelial cells in low serum-containing medium has been achieved without feeder layers or conditioned medium. To date, a total of four lines have been developed and maintained for as many as 40 passages in culture. Growth of the cells was possible only after modifying the culture medium (PFMR-4) by reducing the calcium concentration from 1 to 0.1 mM, and by adding low levels of dialyzed fetal bovine serum and seven growth factors; i.e. epidermal growth factor, hydrocortisone, ethanolamine, phosphoethanolamine, insulin, transferrin, and cholera toxin. Cell lines have been developed from both explant outgrowths and enzyme dissociated esophagi. The epithelial nature of the cells was confirmed by electron microscopy and immunological methods. Clonal growth studies revealed that optimal cell growth occurred in medium containing 2.4% dialyzed fetal bovine serum and 0.1 mM calcium. Calcium levels of 0.3 mM or higher caused the cells to stratify and undergo terminal differentiation. Coating the culture dishes with collagen, or a combination of collagen, fibronectin, and bovine serum albumin, increased both the cell growth rate and the colony forming efficiency. The successful long term culture of rat esophageal epithelial cells permits their use as models in studies concerned with esophageal differentiation and carcinogenesis.

摘要

已在不含饲养层或条件培养基的低血清培养基中实现了大鼠食管上皮细胞的克隆生长和连续传代。迄今为止,共建立了四条细胞系,并在培养中传代多达40次。只有在对培养基(PFMR - 4)进行改良后,细胞才能生长,改良方法是将钙浓度从1 mM降至0.1 mM,并添加低水平的透析胎牛血清和七种生长因子,即表皮生长因子、氢化可的松、乙醇胺、磷酸乙醇胺、胰岛素、转铁蛋白和霍乱毒素。细胞系既从外植体生长物中建立,也从酶解离的食管中建立。通过电子显微镜和免疫方法证实了细胞的上皮性质。克隆生长研究表明,在含有2.4%透析胎牛血清和0.1 mM钙的培养基中细胞生长最佳。钙水平为0.3 mM或更高会导致细胞分层并发生终末分化。用胶原蛋白或胶原蛋白、纤连蛋白和牛血清白蛋白的组合包被培养皿,可提高细胞生长速率和集落形成效率。大鼠食管上皮细胞的成功长期培养使其能够作为模型用于食管分化和致癌作用的研究。

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