The Action of Ribonuclease on Fixed Tissues

To study the optimal conditions for histochemical use of ribonuclease on fixed tissues, the factors of (1) type of fixation, (2) temperature, pH, type of buffer and length of incubation, (3) concentration of enzyme, and (4) staining and dehydration of sections were observed on rabbit pancreas.

The fixing fluids studied were sublimate-alcohol, Bouin's, Zenker-acetic, Zenker-formol, Petrunkevich's cupric-paranitrophenol, 10% neutral formalin, SUSA, Carnoy, Bensley's chrom-sublimate, absolute ethyl alcohol and acetone. Formaldehyde was a satisfactory fixative, although others might be preferred for special purposes. Of the five buffers tested, McIlvaine's citric-acid-disodium-phosphate mixture was the most satisfactory, whereas veronal-acetate extracted considerable stainable cytoplasmic material. The optimum concentration of ribonuclease and length of incubation varied greatly after the 11 different types of fixation. For example, with ribonuclease buffered by Mcllvaine's fluid, the intense cytoplasmic staining of formaldehyde-fixed tissues was removed by concentrations as low as 0.001 mg./ml., whereas, with sections fixed in Zenkers fluid some cytoplasmic staining persisted even after 3 hours in 0.2 mg./ml. Under the conditions employed the temperature and hydrogen-ion concentration during incubation were less important. Examples of nonspecific action of ribonuclease were noted. Until the degree and optimum conditions of specific action have been more precisely established by further experiments, it is suggested that this histo-chemical reaction only be interpreted as a confirmatory test which is, under the best conditions, only relatively specific for ribonucleic acid and not highly quantitative.