Paraffin-Beeswax-Stearic Acid: An Embedding Mass for thin Sections

Abstract

It is possible to cut 1-3 μ sections of rat tissue after passing it through ethanol and chloroform and infiltrating in a wax mixture consisting of 95% Shell Chemical Co. paraffin (MP 125-130° F) and 5% commercial beeswax (clarified by boiling with water and decanting), to which is finally added 10% of technical stearic acid (melted, and clarified by filtration). A potential disadvantage is the slow expansion of the section on the water flotation bath, due to a surface spreading effect of the contained stearic acid. This expansion can be minimised as follows: by adding 0.5% concentration of a secondary alkyl-aryl sulfonate detergent, such as Shell Chemical Co. Teepol, to the notation water; by keeping the temperature of the water at 45° C; by making sure that no section is left on the water for more than 30 sec; and by drying on chemically cleaned slides for 4-18 hr at 45° C., controlled to ±2°. The spreading effect is advantageous in reticulo-endothelial studies, where overlap of cells needs to be reduced to a minimum, and thinly layered cytoplasm expanded.