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Quantitative Analysis of Factors Regulating Angiogenesis for Stem Cell Therapy
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(1) Background: The control of angiogenesis is essential in disease treatment. We investigated angiogenesis-promoting or -suppressing factors and their molecular mechanisms. (2) Methods: Angiogenesis from HUVECs was quantitatively analyzed using the Angiogenesis Analysis Kit (Kurabo, Osaka, Japan). Human rAng-1-producing 107-35 CHO cells or mouse DFAT-D1 cells were co-cultured with HUVEC. Antioxidant polyphenols were added to the culture. Gene expression was analyzed by RT-PCR. (3) Results: The addition of rAng-1-producing cells, their culture supernatant, or commercially available rAng-1 showed a promoting effect on angiogenesis. The co-culture of DFAT-D1 cells promoted angiogenesis. Polyphenols showed a dose-dependent inhibitory effect on angiogenesis. Luteolin and quercetin showed remarkable anti-angiogenic effects. The expression of vWF, Flk1, and PECAM-1 was increased by adding rAng-1-producing cell culture supernatant. Polyphenols suppressed these genes. Apigenin and luteolin markedly suppressed α-SMA and Flk1. Resveratrol and quercetin enhanced the expression of PPARγ, and luteolin suppressed the expression of COX-1. The expression of endothelial nitric oxide synthase (eNOS), an oxidative stress-related gene, was slightly increased by luteolin. These results suggest that polyphenols induce ROS reduction. (4) Conclusions: We showed the promoting effect of Ang-1 or DFAT and the suppressing effect of polyphenols on angiogenesis and studied their molecular mechanisms. These results help control angiogenesis in regenerative therapy.
Title: Quantitative Analysis of Factors Regulating Angiogenesis for Stem Cell Therapy
Description:
(1) Background: The control of angiogenesis is essential in disease treatment.
We investigated angiogenesis-promoting or -suppressing factors and their molecular mechanisms.
(2) Methods: Angiogenesis from HUVECs was quantitatively analyzed using the Angiogenesis Analysis Kit (Kurabo, Osaka, Japan).
Human rAng-1-producing 107-35 CHO cells or mouse DFAT-D1 cells were co-cultured with HUVEC.
Antioxidant polyphenols were added to the culture.
Gene expression was analyzed by RT-PCR.
(3) Results: The addition of rAng-1-producing cells, their culture supernatant, or commercially available rAng-1 showed a promoting effect on angiogenesis.
The co-culture of DFAT-D1 cells promoted angiogenesis.
Polyphenols showed a dose-dependent inhibitory effect on angiogenesis.
Luteolin and quercetin showed remarkable anti-angiogenic effects.
The expression of vWF, Flk1, and PECAM-1 was increased by adding rAng-1-producing cell culture supernatant.
Polyphenols suppressed these genes.
Apigenin and luteolin markedly suppressed α-SMA and Flk1.
Resveratrol and quercetin enhanced the expression of PPARγ, and luteolin suppressed the expression of COX-1.
The expression of endothelial nitric oxide synthase (eNOS), an oxidative stress-related gene, was slightly increased by luteolin.
These results suggest that polyphenols induce ROS reduction.
(4) Conclusions: We showed the promoting effect of Ang-1 or DFAT and the suppressing effect of polyphenols on angiogenesis and studied their molecular mechanisms.
These results help control angiogenesis in regenerative therapy.
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