Murray Ab scite author profile

Murray Ab

3Publications

37Citation Statements Received

49Citation Statements Given

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Affiliations

Institute of Bioinformatics and Systems Biology, Munich Security Conference

Publications

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c-fos expression precedes osteogenic differentiation of cartilage cells in vitro.

Closs

Schmidt

et al. 1990

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Abstract. We have investigated the temporal pattern of expression of c-fos in cartilage ceils in mouse mandibular condyles. During in vitro cultivation, the progenitor cells in this organ differentiate to osteoblasts, and hypertrophic chondrocytes start to show features indicative of osteogenic differentiation. Prior to these processes we observed two distinct patterns of c-fos expression. High, transient c-fos expression was found in the entire tissue within 30 min of culture. This type of c-fos expression appeared to result from mechanical forces applied during dissection. The second type of c-fos expression appeared in individual cells in the zone of hypertrophic chondrocytes. A varying number of formerly quiescent chondrocytes expressed high levels of c-fos mRNA after between 30 min and 10 d in culture, with a peak in the number of cells between days 1 and 3. c-fos expression in these cartilage cells was followed by DNA replication and expression of genes typifying osteoblastic differentiation. After 7 d in culture, groups of cells with the typical ultrastructural features of osteoblasts, and surrounded by an osteoid-like matrix, were observed in single chondrocyte-type lacunae, suggesting division of chondrocytes and differentiation to osteoblasts. The data suggest that c-fos may play a crucial role in the perturbation of determined pathways of skeletoblast differentiation and in the regulation of endochondral bone formation.

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In Situ Embedding of Cell Monolayers Cultured on Plastic Surfaces for Electron Microscopy

Ab¹,

Schulze²,

Blauw³

1991

Biotechnic & Histochemistry

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Various procedures suitable for routine in situ embedding of cell monolayers were tested including: (1) the use of different Epon substitutes, (2) the use of different types of plasticware obtained from different sources, and (3) different methods of preparing capsules for sectioning. Different resins reacted differently with different plastics and type of preparation. Merck Epon substitute bound to most of the plastics tested. Ladd Epon substitute released cleanly from all plastics tested when a suitable method of preparation was used. The results show that for routine embedding of cell monolayers it is necessary to select an appropriate Epon substitute and method of preparation of capsules for the type of plasticware used. A routine method is described, with various alternative steps which can be applied when particular difficulties are encountered.

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In Situ Hybridization of Cytospin Preparations: A Rapid Nonisotopic Screening Method for Isolated Cells

Mandry

Höfler

1994

Biotechnic & Histochemistry

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A simple and rapid method for light microscopic in situ hybridization on cytospin preparations is described and demonstrated for detection of viral nucleic acid in a virus-infected cell line. Cells were fixed by acetone followed by chloroform, denatured by heat, hybridized at 37 C, and hybridized sites detected with a multiple step procedure (primary anti-biotin antibody, biotinylated second antibody, streptavidin-peroxidase). This method can be used for screening studies at the light microscope level, and offers a useful and simple way to determine optimum hybridization conditions for subsequent electron microscopic investigations.

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Murray Ab

c-fos expression precedes osteogenic differentiation of cartilage cells in vitro.

In Situ Embedding of Cell Monolayers Cultured on Plastic Surfaces for Electron Microscopy

In Situ Hybridization of Cytospin Preparations: A Rapid Nonisotopic Screening Method for Isolated Cells

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