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嵌入胶原凝胶中的人乳腺上皮细胞原代培养。

Primary culture of human mammary epithelial cells embedded in collagen gels.

作者信息

Yang J, Guzman R, Richards J, Jentoft V, DeVault M R, Wellings S R, Nandi S

出版信息

J Natl Cancer Inst. 1980 Aug;65(2):337-43.

PMID:6995666
Abstract

Human mammary epithelial cells were dissociatd from mastectomy tissues. The contaminating fibroblasts were removed by the use of Percoll density-gradient centrifugation, which utilizes the difference in buoyant densities between epithelial cells and fibroblasts. A preparation highly enriched for mammary epithelial cells ws then embedded in collagen gel and cultured in Ham's F12 medium containing 12.5% horse serum, 2.5% fetal calf serum, 0.1 microgram cholera toxin/ml, an extract prepared from human male urine (L microgram protein/ml), and a hormone combination of 10 microgram insulin/ml, 10 microgram human placental lactogen/ml, 1 microgram aldosterone/ml, and 0.5 microgram hydrocortisone/ml. Sustained growth leading to an increase of tenfold to thirtyfold in cell number over the initial value was accomplished in primary culture, and this growth was maintained even after passage to secondary culture. Deletion of either the urine extract or the hormone combination resulted in less than optimal growth. Subsequent studies showed that hydrocortisone alone could replace the hormone combination. In addition, urine extract could be replaced by extracts prepared from human kidneys or brains. The collagen gel system provies a reproducible and consistent method for sustained three-dimensional growth of mammary epithelial cells from human breast tissue in primary as well as passaged cultures.

摘要

人乳腺上皮细胞从乳房切除组织中分离出来。通过使用Percoll密度梯度离心法去除污染的成纤维细胞,该方法利用上皮细胞和成纤维细胞之间浮力密度的差异。然后将高度富集乳腺上皮细胞的制剂包埋在胶原凝胶中,并在含有12.5%马血清、2.5%胎牛血清、0.1微克/毫升霍乱毒素、从人男性尿液制备的提取物(1微克蛋白质/毫升)以及10微克胰岛素/毫升、10微克人胎盘催乳素/毫升、1微克醛固酮/毫升和0.5微克氢化可的松/毫升的激素组合的Ham's F12培养基中培养。在原代培养中实现了持续生长,导致细胞数量比初始值增加了10倍至30倍,并且即使传代至二代培养,这种生长仍得以维持。去除尿液提取物或激素组合中的任何一种都会导致生长不理想。随后的研究表明,单独的氢化可的松可以替代激素组合。此外,尿液提取物可以用人肾或脑制备的提取物替代。胶原凝胶系统为来自人乳腺组织的乳腺上皮细胞在原代和传代培养中进行持续的三维生长提供了一种可重复且一致的方法。

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