A new rapid silver impregnation for neuronal bodies.

Frozen sections of avian and rat brains routinely fixed in 6% glutaraldehyde/2% paraformaldehyde and left in phosphate buffer for 1 month are cut at 15-20 microns and collected in distilled water. Sections are placed in ammoniacal silver solution for 30 s, rinsed in 100% acetone and developed in a reducing solution at 75 degrees C. Sections are toned in 1% gold chloride solution and fixed in 50% sodium thiosulfate. After washing, the sections are dehydrated, cleared and mounted in the usual way for light microscopy.