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An image analysis method for the study of cell adhesion to biomaterials.
Authors:J C Dubois  C Souchier  M L Couble  P Exbrayat  M Lissac
Affiliation:Laboratoire des Surfaces et Interfaces en Odontologie, Faculté d'Odontologie, Université Claude Bernard Lyon I, France. dubois@laennec.univ-lyon1.fr
Abstract:This fluorescence image analysis method for the quantitative determination of cell adhesion on biomaterials allows bone cells labelled with propidium iodide to be counted automatically, directly on their support. The reliability of the estimation by fluorescence image analysis was validated by comparison with visual counting and with results obtained by an electronic particle counter. In this way it was possible to demonstrate that the adhesive properties of bone cells are dependent on the type of substrate--enstatite (MgO, SiO2, CaO-P2O5-Al2O3), Thermanox (modified polyethyleneterephthalate), or glass. In contrast, the spread of the cell cytoplasm, labelled with fluorescein isothiocyanate and measured by image analysis, does not vary significantly according to the substrate. The characterisation by SKIZ tessellation of the spatial cell arrangement shows that the bone cells have a random organisation on Thermanox and glass, whereas they form aggregates on enstatite.
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