Glutaraldehyde-Ammoniacal Silver Carbonate-Formaldehyde Staining of Histones of Mitotic Chromosomes

Abstract

Cells from monolayer culture of Chinese hamster line Don were treated by Colcemid (0.1 μg/ml) for 2 hr, trypsinized and spun; resuspended in 0.5% sodium citrate solution for 10 min, respun, and then resuspended in a small volume of the supernatant. Slide preparations were made by smearing, followed by air drying for 1 min at room temperature. They were fixed and stained by the following sequence: 2.5% glutaraldehyde in Millonig's buffer, 30 min; distilled water, 6 min, 5 changes; ammoniacal silver at 18-26 C, 10 sec; distilled water, 30 min, 5 changes; 2.5% formalin, 2 min; and distilled water, 3 changes during 15 min. Staining solution: add 225 ml of 5% Na₂CO₃ to 75 ml of 10% AgNO₃, then add concentrated NH₄OH slowly, drop by drop, until the solution is transparent. Finally add 300 ml of dstilled water. Cells treated with cold 0.25 N HCl before fixation were not stained. Sequence modifications show that chromatin does not reduce silver by itself. This method stains the sites of high histone concentrations in mitotic chromosomes of cytogenetic preparations.