8-NH2-Ado promotes cell death and inhibits cell growth but with only minor cell-cycle effects in MCL cell lines. (A) Cell death after 24 hours of continuous incubation was quantified by loss of mitochondrial membrane potential as measured by DiOC6 staining, at various concentrations of 8-NH2-Ado. For each cell line, the dose-response curve was estimated by nonlinear regression using a variable Hill Slope model. The EC50 was defined as the drug concentration required to achieve 50% of the maximum response. The standard errors of the estimated EC50 values for JeKo, Mino, and SP-53 were less than 3%; the EC50 value could not be accurately estimated for Granta 519. (B) Cell death was also evaluated by PARP cleavage. The arrow denotes cleaved PARP. The cells were continuously incubated with 3μM 8-NH2-Ado for 24 hours. (C) The growth inhibition of MCL cells was determined after 24 hours of continuous exposure to multiple concentrations of 8-NH2-Ado. The cell concentrations were quantified using a particle count and size analyzer (Beckman Coulter). The IC50 values were estimated by nonlinear regression using a variable Hill Slope model. The IC50 value was defined as the drug concentration required to achieve 50% of the maximum growth inhibition. The standard errors for the IC50 value estimates were less than 8% for all cell lines. (D) The cell-cycle effects were determined by flow cytometry for JeKo and Granta 519 after continuous treatment with 3μM 8-NH2-Ado at various time points up to 24 hours. Independent experiments were performed in triplicate shown with SD error bars.