Introduction
Analysis of the brain tissue depends on the experimental setup and question, and needs to be decided by each investigator. However, one should bear in mind that the health of animals as well as the diet they eat will inevitably affect the results obtained. Even though it is commonly thought to be so, the experiment does not start from the day the brains are dissected out and subjected to analysis but from the way animals are handled, fed, and cared for.
Fixation of brain tissue
Fixation is needed to stop degradation of the tissue and to preserve both structure and tissue antigens for analysis. Chemicals used for fixation are compounds that form cross-linking bonds between the components of the tissue and thereby literally fix/preserve them in the state they existed during life. The more cross-linking in the fixative, the more it can preserve the structural morphology of the tissue. The most commonly used fixatives in the order of their cross-linking properties are: glutaraldehyde, formaldehyde, paraformaldehyde, and p-benzoquinone. In addition, different alcohols (acetone, methanol) can be used as fixatives, but they dissolve lipids and therefore do not preserve structure as well.
For electron microscopic analysis of the brain, 1–2% glutaraldehyde is the preferred fixative. For immunocytochemical demonstration of tissue antigens at light microscopic level, 2–4% paraformaldehyde or 0.4% p-benzoquinone are the best alternatives.