Denaturation and condensation of DNA in situ induced by acridine orange in relation to chromatin changes during growth and differentiation of friend erythroleukemia cells

Abstract
DNA in situ is progressively denatured when the cells or nuclei are treated with increasing concentration of acridine orange (AO). This transition can be monitored by flow cytometry as a decrease in green fluorescence. The complexes of denatured DNA and AO undergo immediate condensation and aggregation; this step is manifested by appearance of red luminescence and formation of precipitates that can be detected by electron microscopy. The precipitates form preferentially in heterochromatin as well as in ribosomes and polysomes. Their formation and further aggregation affects cellular light scatter properties in both the forward and right-angle direction. The AO-induced DNA denaturation and condensation was studied in nuclei of Friend erythroleukemia cells from exponentially growing, differentiated or quiescent cells. The DNA in nuclei of quiescent cells, from plateau-phase cultures, was the most sensitive to denaturation; it denatured (measured by changes in luminescence) at an AO concentration between 50 and 80 μM with the midpoint of the transition (Cd) at 70 μM. DNA in nuclei of differentiated cells (dimethyl-sulfoxide-induced erythroid differentiation) was more resistant (Cd = 77–83 μM), whereas DNA in exponentially growing cells was the most resistant (Cd = 86 μM). Extraction of proteins with 0.1 M HCl at 0°CC abolished the differences between the cells and shifted the transition to a lower AO concentration (Cd = 46 μM). For comparison, the midpoint transitions representing condensation of free, nucleic acids measured as light scatter changes occurred at 13, 22, 31 and 53 μM of AO, for rRNA, tRNA, and denatured and native-calf thymus DNA, respectively. Denaturation and condensation of DNA, which can be induced by AO either in isolated nuclei or viable permealized or fixed cells provides a new approach to discriminate cell sub-populations with different chromatin structure by flow cytometry. The molecular mechanisms of this phenomenon are discussed.