Abstract

) It is increasingly apparent that both the normal, differentiated state, and the manifestation of the malignant phenotype in the epithelia, are dependent on the nature and the integrity of the surrounding stroma and the extracellu- lar matrix (ECM). While these phenomena are relatively well studied in animal models, the definition and the role of the """"""""microenvironment"""""""" in the human tissues has lagged behind. My coworkers and I have established culture systems for the cultivation of functional epithelial cells from the rodent mammary gland in which they are able to recreate """"""""lactating"""""""" alveoli in the culture dish. As such, we have unraveled some unexpected aspects of microenvironmental control. Together with the Co-Principal Investigators, we have applied these methods to establish a rapid and versatile assay for distinguishing normal and malignant human breast epithelial cells in a 3- dimensional organotypic assay. Our main collaborator (OWP) and his coworkers have isolated and characterized one of a very few """"""""diploid"""""""" human cell lines (HMT3522) that in our 3-D assay behaves like normal cells from reduction mammoplasties. During passage in culture, these cells become aneuploid and after 205 passages become tumorigenic in the nude mice, and at this stage behave like the carcinomas in our assay. Passages of this line, as well as primary luminal cells from reduction mammoplasty, will be used for functional studies outlined here. We will choose 5 passages between early, intermediate and late stages of HMT3522, with the first being """"""""normal"""""""" by the criteria of our assay, and the last, malignant by the criteria of tumor formation in the nude mice.
The aims are to understand, in a well defined culture model which mimics the behavior or the cells in vivo, the influence of stromal cells (primary or secondary) on the function of the epithelial cells and vice versa. We have recently developed techniques for isolation of the major cell types from the human breast stroma. We will further characterize these cells and use them together with cells from primary tumors in 3-D cultures to explore the origin and the nature of the """"""""stromal reaction"""""""". We have defined a number of markers to distinguish normal (reduction mammoplasty as well as HMT 3522) and malignant epithelial cells as a result of cell-ECM interactions. These include the loss of ability to form TDLU (terminal duct lobular units), loss of polarity (as measured by the localization of sialomucin and expression of E and P cadherins), changes in integrins, and components of the basement membrane, and importantly, the inability to growth arrest in 3-D. We will supplement the list with additional markers including known oncogenes and tumor suppressor genes reported to change in breast cancer, as well as assays for active TGFbeta and TGFalpha to generate an informative panel of markers. These will be used to measure gene expression and to monitor the progression to tumorigenicity after different combinations of """"""""homotypic and heterotypic"""""""" interactions between the stromal and the epithelial cells. The long range goals are a) to define, in a physiological microenvironment, accurate and early markers for changes to the malignant phenotype as a result of stromal- epithelial interactions and b) to pave the way to understanding the detailed mechanism by which the microenvironment regulates function in normal and malignant breast.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA064786-03
Application #
2429821
Study Section
Special Emphasis Panel (SRC (88))
Program Officer
Mohla, Suresh
Project Start
1995-06-01
Project End
1999-05-31
Budget Start
1997-06-01
Budget End
1999-05-31
Support Year
3
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
Lawrence Berkeley National Laboratory
Department
Anatomy/Cell Biology
Type
Organized Research Units
DUNS #
078576738
City
Berkeley
State
CA
Country
United States
Zip Code
94720

  Publications

Furuta, Saori; Ren, Gang; Mao, Jian-Hua et al. (2018) Laminin signals initiate the reciprocal loop that informs breast-specific gene expression and homeostasis by activating NO, p53 and microRNAs. Elife 7:
Ricca, Benjamin L; Venugopalan, Gautham; Furuta, Saori et al. (2018) Transient external force induces phenotypic reversion of malignant epithelial structures via nitric oxide signaling. Elife 7:
Fiore, Ana Paula Zen Petisco; Spencer, Virginia A; Mori, Hidetoshi et al. (2017) Laminin-111 and the Level of Nuclear Actin Regulate Epithelial Quiescence via Exportin-6. Cell Rep 19:2102-2115
Simian, Marina; Bissell, Mina J (2017) Organoids: A historical perspective of thinking in three dimensions. J Cell Biol 216:31-40
Bahrami, S B; Tolg, C; Peart, T et al. (2017) Receptor for hyaluronan mediated motility (RHAMM/HMMR) is a novel target for promoting subcutaneous adipogenesis. Integr Biol (Camb) 9:223-237
Bissell, Mina J (2017) Goodbye flat biology - time for the 3rd and the 4th dimensions. J Cell Sci 130:3-5
Jorgens, Danielle M; Inman, Jamie L; Wojcik, Michal et al. (2017) Deep nuclear invaginations are linked to cytoskeletal filaments - integrated bioimaging of epithelial cells in 3D culture. J Cell Sci 130:177-189
Bhat, Ramray; Belardi, Brian; Mori, Hidetoshi et al. (2016) Nuclear repartitioning of galectin-1 by an extracellular glycan switch regulates mammary morphogenesis. Proc Natl Acad Sci U S A 113:E4820-7
Ghajar, Cyrus M; Bissell, Mina J (2016) Metastasis: Pathways of parallel progression. Nature :
Bissell, Mina J (2016) Thinking in three dimensions: discovering reciprocal signaling between the extracellular matrix and nucleus and the wisdom of microenvironment and tissue architecture. Mol Biol Cell 27:3205-3209

Showing the most recent 10 out of 125 publications