I have included the cells in culture, in epoxy resin directly on multiwell plates. To detach, I tried using liquid nitrogen, but the plate was not broken. Do you know a method to separate the inclusions from the plate? Alternatively can you suggest a good method to include adherent cell cultures with epoxy resin without, however, bringing them into suspension so that I can observe them by TEM?
Tanja Višnjar
For adherent cells I suggest to use chambered coverslips (http://ibidi.com/xtproducts/en/ibidi-Labware/Open-Slides-Dishes:-ibidi-Standard-Bottom/m-Slide-8-well) or porous membranes (https://de.vwr.com/app/Header?tmpl=/life_science/hts_transwell.htm).
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Samad Khan
Use the oval pedidish and cell particals by using chamber for counting the cell by coverslips
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