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Immunolabeling of Neuronal Membrane Proteins in a Freeze-fractured Specimen of Mouse Brain Tissue
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Transcrição
Take a freeze-fractured specimen of mouse brain tissue in a buffer.
The specimen is coated with platinum to enhance surface details and with carbon for structural stability.
Transfer the specimen to a vial with a digestion buffer containing detergent.
Incubate to facilitate tissue breakdown, leaving intact the membrane and proteins embedded in the coating.
Wash with buffer to remove debris.
Add a blocking solution to prevent non-specific antibody binding.
Introduce primary antibodies specific to target neuronal membrane protein.
Wash with buffer to remove unbound antibodies.
Incubate with gold-conjugated secondary antibodies that bind to primary antibodies.
Wash with buffer to remove excess antibodies.
Rinse with water to prevent artifacts from salt residues during microscopy.
Mount the specimen on a transmission electron microscope or TEM grid.
Under the TEM, visualize the target neuronal membrane protein identified by gold particles, which appear as black dots.
Immunolabeling of Neuronal Membrane Proteins in a Freeze-fractured Specimen of Mouse Brain Tissue
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