Growth and differentation of rat mammary epithelial cells cultured in serum-free medium

被引:0
作者
Dong Yeum Kim
Byung-Hak Jhun
Kyung Hee Lee
Seung Chul Hong
Kelly H. Clifton
Nam Deuk Kim
机构
[1] Pusan National University,College of Pharmacy
[2] Pusan National University,Research Institute of Drug Development
[3] University of Wisconsin Comprehensive Cancer Center,Department of Human Oncology, K4/330 CSC
[4] Pusan National University,Dept. of Pharmacy
来源
Archives of Pharmacal Research | 1997年 / 20卷
关键词
Mammary epithelial cell; Differentiation; Flow cytometry; Cell-cell communication;
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摘要
A new serum-free defined medium was developed that supports the growth of normal rat mammary epithelial cells. Mammary organoids from the glands of female F344 rats were cultured in a serum-free medium. Monolayer culture colonies developed within a week and remained viable for months in culture. Upon subculture of one-week-old primary colonies, almost the same morphology of colonies was developed. The scrape loading/dye transfer technique showed that most of colonies that developed in a serum-free medium containing EGF, human transferrin, insulin, and hydrocortisone (basal serum-free medium, BSFM) failed to show cell-cell communication. However, colonies cultured in BSFM supplemented with prolactin, E2, and progesterone (complete hormone serum-free medium, CHSFM) showed cell-cell communication at 14 days of primary culture or of subculture. By flow cytometry with FITC-PNA and PE-anti-Thy-1.1 monoclonal antibody, we distinguished four RMEC subpopulations in cultures in both media: Thy-1.1+ cells, PNA+ cells, cells negative to both reagents and cells positive to both reagents. It is likely that combined prolactin, cortisol, and insulin in CHSFM stimulate terminal differentiation of clonogenic cells.
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页码:297 / 305
页数:8
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