Flow-cytometric analysis of mouse peritoneal macrophages

Abstract

Flow-cytometric analysis of mouse peritoneal macrophages (MΦ) stained with acridine orange defined three populations with increasing RNA content. Resident MΦ displayed variable bimodal distributions of low and intermediate cellular RNA content with high RNA content only observed after in vitro stimulation with fetal calf serum or/and bacterial lipopolysaccharide (LPS). In contrast, only few resident macrophages from the LPS nonresponder strain C3H/HeJ increased in RNA content upon LPS stimulation. Macrophages with high RNA content developed transiently after in vivo stimulation with either thioglycollate broth or paraffin oil. Proteose peptone-elicited macrophages transformed only after additional in vitro stimulation with fetal calf serum and/or LPS. The magnitude of the in vitro response upon stimulation, assessed as increasing percentage of either intermediate or high RNA macrophages, was dependent on the composition of the MΦ population at the onset of in vitro culture. Effective increase in cellular RNA content was always paralleled by improved adherence of plated macrophages to the culture vessel. In conclusion, flow-cytometric measurement of macrophage populations might become a useful tool to quantify macrophage activation or stimulation.