Fixation protocols for neurohistology: neurons to genes

Abstract

Since ancient times, tissue fixation for neurohistology has been an evolving area of research. Alcohol fixation first made possible examination of brain tissue specimens. In the late 1800s formaldehyde was introduced as a cross-linking fixative, which enabled histological advances. Various aldehyde solutions remain the staple for neurohistology in the neuroscience community including formalin, paraformaldehyde, glutaraldehyde, and combinations of these fixatives. A 4% paraformaldehyde solution is commonly used for numerous cytochemical procedures including tract tracing, immunohistochemistry, and in situ hybridization. A glutaraldehyde–paraformaldehyde solution is the fixative of choice for ultrastructural investigations using the electron microscope. With the advent of modern molecular and cellular biological techniques, it is now possible to isolate and study genomic DNA, RNA species, and proteins from microdissected tissue sources. Similar to light and electron microscopy, alcohol and aldehyde tissue fixation are compatible with preserving RNA integrity for regional and single cell gene array experiments using immersion- and perfusion-fixed tissue from a myriad of brain tissue sources including humans and relevant animal and cellular models.