Rhodamine 123 (Rh123) is widely used as a flow cytometric probe for mitochondrial membrane potential (MMP) in metabolic, pharmacologic, and toxicological studies. However, the use of relatively high concentrations of Rh123 (up to 10 pg/ml) and prolonged incubation times (up to 1 h), including washing steps, may be inconvenient for certain applications in which labile cells are used or which demand rapid or repeated analysis. In this paper we describe a rapid kinetic assay of MMP in isolated rat hepatocytes, based upon the quantitation of the initial rate of Rh123 uptake by living cells, selected by their scattering properties. The results indicate that at an appropriate dye-to-cell ratio (in our experiments, 50 ng Rh123/ml for 250,000300,000 cells/ml), the initial rate of Rh123 uptake is a highly reproducible and sensitive parameter for estimation of MMP, as demonstrated by the effects of substrates and inhibitors of the glycolytic pathway and mitochondrial respiration. Because of its simplicity, rapidity (about 5 min) and metabolic implications, this assay would be also suitable for the routine evaluation of metabolic state of cell suspensions, as a complementary test to the standard dualstaining tests of viability. Other possible applications in screening pharmacologic and toxicological analysis are discussed. o 1994 Wiley-Liss, Ine.Key terms: Mitochondria, mitochondrial membrane potential, rhodamine 123, flow cytometry, hepatocyte, glucose metabolism Mitochondrial membrane potential (MMP) is a key parameter to assess cellular energy metabolism under physiological and pathological conditions (5). However, the conventional approach of studying isolated mitochondria in vitro does not allow integration of the mitochondrial function into the whole cell.Flow cytometry provides convenient methods for the analysis of MMP in situ. Recently, most flow cytometric studies on mitochondrial function have been performed with rhodamine 123 (Rh123), a lipophilic cationic fluorochrome which is incorporated by mitochondria according to transmembrane potential (6,9,11,14,20,22). Rh123 has been applied extensively in flow cytometric studies of mitochondrial metabolism (2,30,33) and metabolic heterogeneity (341, cell activation (81, differentiation (71, oncogenic transformation (32), stem cell characterization and purification (37,381, aging (16), and apoptotic death (lo), as well as for assessment of cytotoxicity (20,22,23,24) and drug resistance (15,17). Some of the multiple applications of Rh123 have been reviewed by Ronot et al. (26,271 and Chen (5,6).The most usual techniques to study MMP by flow cytometry in whole cells follow the one described by Johnson et al. (13,14), with slight modifications. Following a 30-60 min equilibration of cells with Rh123
