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. 2016 Nov 18;16(1):59–72. doi: 10.1080/15384101.2016.1252881

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Figure 4. — PPARβ/δ (A) and β-catenin (B) immunolocalization in SH-SY5Y during differentiation. Undifferentiated (CTR) and differentianted (N2) cells at 4h from N2 treatment. Bar = 10 μm. C: WB and relative densitometric analyses for PPARβ/δ and β-catenin in undifferentiated (CTR) and differentiating (N2) cells at the indicated time-points. D: WB and relative densitometric analyses for 4-HNE in undifferentiated (CTR) and differentiating (N2) cells at the indicated time-points. The relative densities of the immunoreactive bands were determined and normalized with respect to GAPDH using a semiquantitative densitometric analysis. Data are mean ± SE of 4 different experiments. *P ≤ 0.05; **P ≤ 0.005. E: PPARα IF in SH-SY5Y during differentiation. Undifferentiated (CTR) and differentianted (N2) cells at 4h and 24h from N2 treatment Bar = 10 μm. F: WB and relative densitometric analysis for PPARα in undifferentiated (CTR) and differentiating (N2) cells at the indicated time-points. The relative densities of the immunoreactive bands were determined and normalized with respect to GAPDH, using a semiquantitative densitometric analysis. Data are mean ± SE of 4 different experiments. *P ≤ 0.05.