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Quantification of regenerative potential in primary human mammary epithelial cells
Author(s) -
Jelena R. Linnemann,
Haruko Miura,
Lisa K. Meixner,
Martin Irmler,
Uwe J. Kloos,
Benjamin Hirschi,
Harald Bartsch,
Steffen Sass,
Johannes Beckers,
Fabian J. Theis,
Christian J. Gabka,
Karl Sotlar,
Christina Scheel
Publication year - 2015
Publication title -
development
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.15
H-Index - 36
eISSN - 1477-9129
pISSN - 0950-1991
DOI - 10.1242/dev.123554
Subject(s) - biology , organoid , microbiology and biotechnology , stromal cell , morphogenesis , population , regeneration (biology) , mesenchymal stem cell , progenitor cell , contractility , stem cell , biochemistry , endocrinology , cancer research , gene , demography , sociology
We present an organoid regeneration assay in which freshly isolated human mammary epithelial cells are cultured in adherent or floating collagen gels, corresponding to a rigid or compliant matrix environment. In both conditions, luminal progenitors form spheres, whereas basal cells generate branched ductal structures. In compliant but not rigid collagen gels, branching ducts form alveoli at their tips, express basal and luminal markers at correct positions, and display contractility, which is required for alveologenesis. Thereby, branched structures generated in compliant collagen gels resemble terminal ductal-lobular units (TDLUs), the functional units of the mammary gland. Using the membrane metallo-endopeptidase CD10 as a surface marker enriches for TDLU formation and reveals the presence of stromal cells within the CD49f(hi)/EpCAM(-) population. In summary, we describe a defined in vitro assay system to quantify cells with regenerative potential and systematically investigate their interaction with the physical environment at distinct steps of morphogenesis.

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