Figure 1
Figure 1. BAZF regulates EC network formation in culture. (A) Expression pattern of BAZF mRNA after VEGF-A (50 ng/mL) stimulation in HUVECs. Quantitative RT-PCR of BAZF mRNA was performed using a TaqMan-gene expression system. The results represent mean values from 3 independent experiments. Error bars represent ± SD. (B) Analysis of BAZF protein level in HUVECs after VEGF-A stimulation by Western blotting using an anti-BAZF antibody. Relative intensity of each band was measured by Lane Analyzer 3.0 software (ATTO) and normalized relative to β-actin (loading control). (C) Angiogenic sprouting from AdBAZF-infected or AdGFP-infected HUVECs. Arrows show sprouting cells. Left panels represent microscopic images, and right panel shows total number of sprouting cells in 50 beads. Scale bar: 100 μm (***P < .001). (D) Protein level of BAZF in HUVEC transfected with BAZF or control siRNA with or without VEGF-A stimulation. BAZF protein was detected by Western blotting using an anti-BAZF antibody. (E) BAZF knockdown disrupts VEGF-A–induced network formation of HUVECs on the Matrigel. The cells were stained with Calcein-AM and the images were acquired. Scale bar: 500 μm. (F) Quantification of the network formation of HUVEC transfected with BAZF or control siRNA. The total length of the network per field (mm2) was measured by ImagePro Plus software 4.5. (Roper). The results represent mean values from 3 experiments. Error bars represent ± SD (***P < .001). (G) Time-lapse imaging of the network formation in HUVEC treated with BAZF or control siRNA. Scale bar: 10 μm.

BAZF regulates EC network formation in culture. (A) Expression pattern of BAZF mRNA after VEGF-A (50 ng/mL) stimulation in HUVECs. Quantitative RT-PCR of BAZF mRNA was performed using a TaqMan-gene expression system. The results represent mean values from 3 independent experiments. Error bars represent ± SD. (B) Analysis of BAZF protein level in HUVECs after VEGF-A stimulation by Western blotting using an anti-BAZF antibody. Relative intensity of each band was measured by Lane Analyzer 3.0 software (ATTO) and normalized relative to β-actin (loading control). (C) Angiogenic sprouting from AdBAZF-infected or AdGFP-infected HUVECs. Arrows show sprouting cells. Left panels represent microscopic images, and right panel shows total number of sprouting cells in 50 beads. Scale bar: 100 μm (***P < .001). (D) Protein level of BAZF in HUVEC transfected with BAZF or control siRNA with or without VEGF-A stimulation. BAZF protein was detected by Western blotting using an anti-BAZF antibody. (E) BAZF knockdown disrupts VEGF-A–induced network formation of HUVECs on the Matrigel. The cells were stained with Calcein-AM and the images were acquired. Scale bar: 500 μm. (F) Quantification of the network formation of HUVEC transfected with BAZF or control siRNA. The total length of the network per field (mm2) was measured by ImagePro Plus software 4.5. (Roper). The results represent mean values from 3 experiments. Error bars represent ± SD (***P < .001). (G) Time-lapse imaging of the network formation in HUVEC treated with BAZF or control siRNA. Scale bar: 10 μm.

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