Figure 1.

Measurement of endogenous levels of 4HNE and MDA in a panel of neuroblastoma cells (panel A; p < 0.001). Expression of RLIP76 in neuroblastoma cells as assessed by Western-blot analyses using anti-RLIP76 IgG as a primary-antibodies. The bands were quantified by scanning densitometry using Innotech Alpha Imager HP. β-actin was used as a loading control (panel B). Protective effect of control-liposome and RLIP76-proteoliposomes (50 μg/mL) on radiation-toxicity by colony-forming assay (panel C; p < 0.01). In panels A and C, results are average and standard deviation from three separate experiments, each in triplicates (n = 9).