Your search keyword '"M. Dunand"' showing total 3 results

1. Purification of PRL receptors from toad kidney: comparisons with rabbit mammary PRL receptors

Author

M. Dunand, M. L. Aubert, B. C. Rossier, and J. P. Kraehenbuhl

Subjects

endocrine system, medicine.medical_specialty, Receptors, Prolactin, Physiology, Toad, Peptide hormone, Kidney, Mammary Glands, Animal, Affinity chromatography, biology.animal, Internal medicine, medicine, Animals, Receptor, Gel electrophoresis, Affinity labeling, biology, Immune Sera, Affinity Labels, Cell Biology, Molecular biology, Prolactin, Endocrinology, Solubility, Polyclonal antibodies, Chromatography, Gel, biology.protein, Bufo marinus, Rabbits, hormones, hormone substitutes, and hormone antagonists

Abstract

The binding characteristics of the prolactin (PRL) receptors present in toad (Bufo marinus) kidneys were investigated and compared to those of PRL receptors present in rabbit mammary glands. The molecular characteristics of the Triton X-100 solubilized renal and mammary PRL receptors were assessed by gel filtration and by migration analysis on sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) after affinity labeling of the binding sites with 125I-human growth hormone. Similar results were obtained for both receptors. Partial purification of the toad PRL receptor could be achieved by affinity chromatography. The molecular weight of this purified receptor could be determined by analysis on SDS-PAGE. With the use of a polyclonal antiserum raised against a purified preparation of rabbit mammary PRL receptor, one or several antigenic epitope(s) could be identified on the core of the toad renal PRL receptor. In conclusion, although the structure and the biological role(s) of PRL have substantially changed during evolution, the receptor for this hormone has retained many of its structural features as could be assessed between an amphibian and a mammalian species on functionally different target tissues.

Published

1988

2. Establishment of two rabbit mammary epithelial cell lines with distinct oncogenic potential and differentiated phenotype after microinjection of transforming genes

Author

H Diggelmann, J P Kraehenbuhl, M Dunand, Irène Garcia, Bernard Sordat, and E Rauccio-Farinon

Subjects

Cell, Caseins/genetics, Simian virus 40, Biology, ddc:616.07, Cell Line, Mammary Glands, Animal, medicine, Doubling time, Animals, Primary cell, Receptor, Gene, Molecular Biology, DNA, Neoplasm/genetics, Contact inhibition, Caseins, Cell Differentiation, Epithelial Cells, Cell Biology, DNA, Neoplasm, Neoplasms, Experimental, Oncogenes, DNA, Viral/genetics, Cell Transformation, Viral, Molecular biology, Microscopy, Electron, medicine.anatomical_structure, Gene Expression Regulation, Cell culture, Neoplasms, Experimental/genetics, Mammary Glands, Animal/cytology, DNA, Viral, Rabbits, Immortalised cell line, Research Article

Abstract

The goal of this work was to establish an assay for transformation of epithelial cells. Two epithelial cell lines were obtained after microinjecting transforming genes into primary rabbit mammary secretory cells. The cell lines were analyzed for their oncogenic potential and for the maintenance of a differentiated phenotype. A fully transformed cell line, which retained epithelial cell organization, was obtained by coinjecting simian virus 40 DNA and the activated human c-Ha-ras gene. The proliferation rate of these cells was high, with a doubling time of 16 h. Their growth was anchorage independent, and they had lost contact inhibition. The cells were tumorigenic in nude mice, but had no metastatic potential. Both microinjected DNAs were efficiently transcribed and translated, in contrast to the casein genes, which were expressed in primary cells but not in the transformed cell line. An immortalized cell line established after injection with simian virus 40 DNA alone was characterized by a moderate rate of proliferation with a doubling time of approximately 30 h. The growth of these cells was contact inhibited and anchorage dependent. The cells were not tumorigenic in nude mice. The viral DNA was expressed during early passages, as shown by the presence of the large T antigen in cell nuclei, but not at later passages. A high number of lactogenic hormone receptors were found associated with the cell surface. Despite the presence of these receptors, no induction of genes coding for milk proteins was observed after addition of prolactin. These data demonstrate that this assay system can be used to assess the immortalizing and transforming potential of candidate oncogenes in epithelial cells.

Published

1986

3. Specific binding sites for ovine prolactin in three amphibian cell lines

Author

M. Dunand, J. P. Kraehenbuhl, M. L. Aubert, and B. C. Rossier

Subjects

endocrine system, medicine.medical_specialty, Physiology, Receptors, Prolactin, Xenopus, Urinary Bladder, Receptors, Cell Surface, Toad, Biology, Cell Line, Cell surface receptor, Internal medicine, biology.animal, medicine, Animals, Bovine somatotropin, Binding site, Sheep, urogenital system, Tissue Extracts, Cell Biology, Prolactin, Kinetics, Endocrinology, Cell culture, Pituitary Gland, Bufo marinus, Luteinizing hormone, hormones, hormone substitutes, and hormone antagonists, Hormone

Abstract

Established cell lines (TB-6c and TB-M) obtained by continuous culture of epithelial cells from toad Bufo marinus urinary bladder, which, in culture, maintained a high degree of functional differentiation, exhibited a significant number of high-affinity (KA = 1-2 X 10(10) M-1) binding sites detected both with radioiodinated (125I) ovine prolactin (oPRL) and human growth hormone (hGH). Binding capacity was higher in the case of TB-6c cells (7,573 +/- 581 sites/cell) than with the TB-M cells (1,160 +/- 87). Similarly, binding sites for oPRL were characterized on Xenopus laevis kidney-derived cell line A6. With oPRL used both as tracer and standard, significant cross-reaction was observed with hGH, less with human or rat prolactin (PRL), and none with human chorionic somatomammotropin, bovine growth hormone, and rat luteinizing hormone or follicle-stimulating hormones. B. marinus pituitary extracts completely displaced the binding of 125I-oPRL to toad bladder binding sites. This finding of specific sites for PRL on amphibian bladder and kidney cells confirms that PRL exerts specific biological actions for the control of electrolyte and water metabolism in the amphibians.

Published

1985