Your search keyword '"Wicha M"' showing total 5 results

1. Posttranscriptional regulation of alpha-casein mRNA accumulation by laminin.

Author

Zeigler ME and Wicha MS

Subjects

Animals, Blotting, Northern, Cells, Cultured, Dactinomycin pharmacology, Epithelium physiology, Gene Expression Regulation drug effects, In Vitro Techniques, Prolactin pharmacology, RNA, Messenger genetics, RNA, Messenger metabolism, Rats, Transcription, Genetic drug effects, Caseins genetics, Laminin pharmacology, Mammary Glands, Animal physiology

Abstract

We have utilized primary cultures of rat mammary epithelial cells to study mechanisms by which laminin regulates the prolactin-dependent accumulation of alpha-casein mRNA. Mammary cells accumulate approximately fivefold more alpha-casein mRNA when cultured on laminin than when cultured on tissue plastic and the accumulation of alpha-casein mRNA is prolactin dependent. On the basis of transcription assays there is approximately a twofold increase in the alpha-casein mRNA transcription rate in cells cultured on laminin over that of tissue culture plastic. Measurements on the turnover of alpha-casein mRNA show that this mRNA is stabilized fourfold more on laminin than on tissue culture plastic, while there was no significant difference in the turnover of poly(A) RNA on either substratum. These data indicate that laminin regulates the cytoplasmic levels of alpha-casein mRNA accumulation primarily at the post-transcriptional level by increasing the stabilization of this mRNA.

Published

1992

2. Regulation of rat mammary gene expression by extracellular matrix components.

Author

Blum JL, Zeigler ME, and Wicha MS

Subjects

Animals, Caseins biosynthesis, Cell Differentiation, Epithelial Cells, Extracellular Matrix cytology, Extracellular Matrix metabolism, Female, Kinetics, Mammary Glands, Animal metabolism, Mammary Glands, Animal physiology, Milk Proteins genetics, Milk Proteins metabolism, RNA, Messenger metabolism, Rats, Rats, Inbred Strains, Transferrin biosynthesis, Extracellular Matrix physiology, Gene Expression Regulation, Mammary Glands, Animal cytology

Abstract

In the mammary gland the induction and maintenance of differentiation are dependent on both lactogenic hormones and the extracellular matrix (ECM). Since mammary epithelial cells differentiate on a basement membrane in vivo we have examined the effects of basement membrane components on the expression of milk protein genes in primary rat mammary cultures. We examined the effects of a basement membrane gel derived from the Englebreth-Holm-Swarm tumor as well as its major component, laminin, on the expression of a group of milk protein genes. We demonstrate that the basement membrane gel induces alpha-casein and alpha-lactalbumin (alpha-LA) accumulation up to 160- and 70-fold, respectively, of that on tissue culture plastic. Laminin, a major component of the basement membrane, also caused significant induction of these same proteins. In order to determine whether these ECM effects occurred at a translational or post-translational level, pulse-chase experiments were performed. These experiments demonstrated that a laminin substratum selectively effects milk protein turnover and secretion. In order to demonstrate whether ECM effects occurred at the level of steady state accumulation of mRNA we performed dot blot and Northern analyses using cloned cDNA probes for alpha-, beta-, and gamma-caseins and alpha-LA. These studies demonstrated that ECM components induced alpha- and beta-caseins up to 10-fold, and alpha-LA up to 3-fold, with no significant effect on gamma-casein. These results demonstrate that milk protein genes are not coordinately regulated by ECM components. Furthermore, since the amount of induction of milk proteins exceeds the amount of induction of mRNAs for these proteins, we conclude that in our system a major effect of ECM components is at the translational and/or post-translational levels. Based on these findings we propose a model in which basement membrane components effect mammary gene expression at multiple levels.

Published

1987

3. Macrophages express cell surface laminin.

Author

Wicha MS and Huard TK

Subjects

Animals, Ascitic Fluid cytology, Cell Membrane analysis, Female, Fibronectins analysis, Fluorescent Antibody Technique, Laminin, Mice, Mice, Inbred C57BL, Receptors, Mitogen analysis, Glycoproteins analysis, Macrophages analysis

Abstract

Laminin, a non-collagenous extracellular connective tissue glycoprotein, was detected on the surface of mouse peritoneal macrophages. As determined by indirect immunofluorescence, as many as 60% of peritoneal macrophages elicited with thioglycollate expressed cell surface laminin. Only 14% of resident cells displayed detectable laminin. The expression of laminin increased with time post-injection. Concomitant with laminin expression, macrophages also displayed a receptor for the IB4 isolectin from Griffonia simplicifolia. This lectin, which binds methyl-alpha-D-galactopyranoside, may also react with the carbohydrate moeity of laminin. A small population of macrophages displayed both laminin and surface fibronectin. Unlike the difference in laminin expression between resident and thioglycollate-stimulated cells, there was no difference in cell surface fibronectin between these cell populations. Since laminin has been found to mediate cell attachment in other systems, expression of this molecule on the surface of stimulated macrophages may be important in cell-cell and cell-matrix adhesive properties of these cells.

Published

1983

4. Basement membrane collagen requirements for attachment and growth of mammary epithelium.

Author

Wicha MS, Liotta LA, Garbisa S, and Kidwell WR

Subjects

Animals, Cell Division, Cells, Cultured, Collagen biosynthesis, Epithelial Cells, Female, Mammary Glands, Animal growth & development, Rats, Basement Membrane physiology, Cell Adhesion, Collagen metabolism, Mammary Glands, Animal cytology

Published

1979

5. Clustering of cell surface laminin enhances its association with the cytoskeleton.

Author

Cody RL and Wicha MS

Subjects

Animals, Cell Line, Cell Membrane metabolism, Fibrosarcoma metabolism, Fluorescent Antibody Technique, Mice, Cytoskeleton metabolism, Laminin metabolism

Abstract

In order to provide evidence for an association of cell surface laminin with the cytoskeleton, we have examined the detergent extractability of cell surface laminin on murine fibrosarcoma cells. We utilized indirect immunofluorescence with affinity-purified anti-laminin antibodies to determine the distribution, mobility and detergent extractability of laminin bound to the cell surface. We demonstrate that antibody induces clustering of cell surface laminin rendering it resistant to detergent extraction. At low receptor occupancy, approx. 80% of cell surface laminin is detergent-extractable. If cell surface laminin is induced to cluster with anti-laminin antibody, IB4 isolectin from Bandeiraea simplicifolia or by high receptor occupancy, then it is rendered resistant to detergent extraction. This process is temperature-sensitive and inhibited by cytochalasin D (CD). On the basis of these findings, we propose a model in which laminin anchored in the basement membrane in vivo affects the cellular cytoskeleton by facilitating the clustering of cell surface transmembrane laminin receptors which are able to interact with cellular actin.

Published

1986