Abstract
The use of cell culture models is a principal and fundamental technology used in understanding how mammalian cells work. However, for some cell types such as mammary epithelia, the lines selected for extended culture are often transformed or have chromosomal abnormalities, while primary cultures have such a curtailed lifespan that their use is restricted. For example, mammary luminal epithelial cells (MECs) are used to study mechanisms of breast cancer, but the proliferation of primary cell cultures is highly limited. Here we describe the establishment of a new culture system to allow extended analysis of cultures of primary mouse MECs. In 2D monolayer culture, primary MECs showed a burst of proliferation 2–3 days post isolation, after which cell cycle decreased substantially. Addition of mammary epithelial growth factors, such as Epidermal Growth Factor, Fibroblast Growth Factor-2, Hepatocyte Growth Factor, and Receptor Activator for Nuclear Factor κB Ligand, or extracellular matrix proteins did not maintain their proliferation potential, neither did replating the cells to increase the mitogenic response. However, culturing MECs directly after tissue extraction in a 3D microenvironment consisting of basement membrane proteins, extended the time in culture in which the cells could proliferate. Our data reveal that the cellular microenvironment has profound effects on the proliferative properties of the mammary epithelia and is dominant over growth factors. Moreover, manipulating the cellular environment using this novel method can maintain the proliferative potential of primary MECs, thus enabling cell cycle to be studied as an endpoint after gene transfer or gene deletion experiments.
Highlights
Understanding the mechanisms of cell cycle regulation in normal breast epithelia is essential for deciphering the defects of breast cancer, and for developing new therapies to treat the disease
We initially examined the proportion of mammary luminal epithelial cells (MECs) in S-phase that were isolated from pregnant mouse mammary gland (P16–P18) and cultured on collagen Icoated dishes (Fig. 1a)
40% of the cells were in S-phase 2–3 days following isolation, but this fell to less than 10% cycling cells for the remaining time of analysis. Both luminal and myoepithelial cells are isolated during the preparation of MECs
Summary
Understanding the mechanisms of cell cycle regulation in normal breast epithelia is essential for deciphering the defects of breast cancer, and for developing new therapies to treat the disease. We have discovered, using molecular genetic approaches, that the b1-integrin gene is necessary for the proliferation of normal luminal epithelial cells within the breast [1,2]. Gene deletion studies have shown that b1-integrin is required for breast cancer progression [3,4]. Luminal epithelial cells are the precursors of most breast cancers and it is important to determine the mechanisms linking integrins with proliferative responses in this cell type. This poses logistical issues because of the problems associated with growing luminal cells in tissue culture
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