direct immunofluorescence (dif)

How is tissue prepared for DIF?

Preparation of tissue for DIF typically involves fixation, sectioning, and mounting on slides. The tissue is often fixed in a solution that preserves antigenicity, such as formalin or acetone. It is then sectioned using a microtome and mounted on glass slides. The sections are incubated with the fluorescently labeled antibody, washed to remove unbound antibody, and then examined under the fluorescence microscope.

Frequently asked queries:

What is Direct Immunofluorescence (DIF)?
How does DIF work?
What are the applications of DIF in Histology?
What are the advantages of DIF?
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How is DIF different from Indirect Immunofluorescence (IIF)?
What are the common fluorescent dyes used in DIF?
How is tissue prepared for DIF?
What are the controls used in DIF?
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