Micromethods for Analyzing Axon-Target Interactions in Vitro

Abstract In vitro methods for studying interactions between axons and their target cells are presented. The methods maximize the number of cultures that can be produced by limiting the volume and area of the cultures. Small cultures promote cell-cell Interactions and permit rapid conditioning of medium. In addition, valuable reagents added to these microcultures are conserved. The methods include: (a) the manufacture of 40-μl well-volume, coverslip-bottomed culture dishes with plating area of less than 24 mm 2 the dishes allow the small working distances of high-resolution light microscopy; (b) a micromethod to test for the Involvement of secreted factors in cell-cell interactions; cells on different surfaces are cocultured in shared medium; (c) a method to plate explant sources of neurites at a controlled distance from target cells to facilitate neurite identification and to control the timing of growth cone-target cell contacts; and (d) nonisotopic in situ hybridization for chamber-slide cultures combined with immunolabeling of cells in the hybridized culture. These methods can be used in culture assays to identify cell types or molecules involved in a variety of neuronal or, more generally, cell-cell interactions.