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Begin with brains from transgenic Drosophila flies, containing different glial cell types harboring a cell-specific recombinase system.
It drives the expression of a cell surface protein fused to different antigenic epitopes on the same type of cells.
Treat the tissue with a fixative to cross-link proteins and preserve the tissue architecture.
Wash to remove excess fixative.
Add blocking proteins to mask non-specific binding sites to reduce background staining.
Incubate the tissue with a primary antibody cocktail that binds to the different epitopes expressed on glial cells.
Wash to remove unbound primary antibodies.
Incubate with fluorophore-conjugated secondary antibodies that bind to the primary antibodies.
Wash to remove unbound secondary antibodies.
Mount the brain inside an imaging spacer and place a coverslip. The spacer creates a chamber for the tissue, preserving its three-dimensional structure.
Different cells of the same glial type labeled with different fluorophore-conjugated antibodies allow an understanding of cell-cell interactions.
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