Figure 3.

Western blot and immunocytochemical analysis of UGT1A4 expression in EPI-EC. (A–A1) Pattern of UGT1A4 protein expression as evaluated in primary brain endothelial cells (EPI-EC; n = 4 patients, see Table 1). HBMEC were used as comparison. Blots were quantified and normalized by β-actin. Control HBMEC signal was set as 100% of UGT1A4 expression. We found increased UGT1A4 expression in three of the four EPI-ECs analyzed. (B–B1) Example of UGT1A4 overexpression in EPI-ECs compared to HBMECs.