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Cytokeratin provides a specific marker for human arachnoid cells grown in vitro
Authors:Edmund H Frank  Boyce W Burge  Boleslaw H Liwnicz  Linda J Lotspeich  Jocelyn C White  Steven L Wechsler  Frank H Mayfield  Jeffrey T Keller  
Institution:1. Department of Neurosurgery, The Christ Hospital, USA;2. Mayfield Neurosurgical Institute, USA;3. The Christ Hospital Institute of Medical Research, USA;4. Department of Anatomy and Cell Biology, University of Cincinnati College of Medicine Cincinnati, OH 45219, USA;5. Department of Pathology, University of Cincinnati College of Medicine, Cincinnati, OH 45219, USA
Abstract:Cells from cranial and spinal arachnoid membranes of humans were grown in culture. Their growth characteristics, morphology and details of their cytoskeletal composition are described. Arachnoid membranes, obtained at autopsy, were finely minced and incubated in tissue culture medium. Monolayers of cells of homogeneous morphology grew from these tissue fragments. The cells were flat and polygonal. They divided slowly to form non-overlapping monolayers of low cell density. Electron microscopic examination of cultured arachnoid cells revealed numerous desmosome-like tight junctions and abundant intermediate filaments (tonofilaments). Both morphological features are characteristic of arachnoid cells in situ, but not of cells in the fibroblast-rich dura mater. Immunofluorescence microscopy with monoclonal antibodies demonstrated cytokeratin in the cytoplasm of primary cultures of arachnoid cells. Thus we demonstrated that these cultured cells retained certain of the specific differentiated properties of arachnoid cells in situ and that they are not fibroblasts (which lack tight junctions and cytokeratins). To our knowledge, there have been no previous reports of in vitro growth of arachnoid cells. This in vitro model should be useful in studying the response of arachnoid cells to a variety of substances thought to be involved in the chronic inflammatory condition of the meninges known as arachnoiditis.
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