Perinatal Research Facility, 13243 E. 23rd Ave., Mail Stop F441, Aurora, CO 80045.
Am J Physiol Lung Cell Mol Physiol. 2014 Feb 15;306(4):L361-71. doi: 10.1152/ajplung.00277.2013. Epub 2013 Dec 13.
Increased endothelin-1 (ET-1) disrupts angiogenesis in persistent pulmonary hypertension of the newborn (PPHN), but pathogenic mechanisms are unclear. Peroxisome proliferator activated receptor γ (PPARγ) is decreased in adult pulmonary hypertension, but whether ET-1-PPARγ interactions impair endothelial cell function and angiogenesis in PPHN remains unknown. We hypothesized that increased PPHN pulmonary artery endothelial cell (PAEC) ET-1 production decreases PPARγ signaling and impairs tube formation in vitro. Proximal PAECs were harvested from fetal sheep after partial ligation of the ductus arteriosus in utero (PPHN) and controls. PPARγ and phospho-PPARγ protein were compared between normal and PPHN PAECs ± ET-1 and bosentan (ETA/ETB receptor blocker). Tube formation was assessed in response to PPARγ agonists ± ET-1, N-nitro-l-arginine (LNA) (NOS inhibitor), and PPARγ siRNA. Endothelial NO synthase (eNOS), phospho-eNOS, and NO production were measured after exposure to PPARγ agonists and PPARγ siRNA. At baseline, PPHN PAECs demonstrate decreased tube formation and PPARγ protein expression and activity. PPARγ agonists restored PPHN tube formation to normal. ET-1 decreased normal and PPHN PAEC tube formation, which was rescued by PPARγ agonists. ET-1 decreased PPARγ protein and activity, which was prevented by bosentan. PPARγ agonists increased eNOS protein and activity and NO production in normal and PPHN PAECs. LNA inhibited the effect of PPARγ agonists on tube formation. PPARγ siRNA decreased eNOS protein and tube formation in normal PAECs. We conclude that ET-1 decreases PPARγ signaling and contributes to PAEC dysfunction and impaired angiogenesis in PPHN. We speculate that therapies aimed at decreasing ET-1 production will restore PPARγ signaling, preserve endothelial function, and improve angiogenesis in PPHN.
内皮素-1(ET-1)的增加会破坏新生儿持续性肺动脉高压(PPHN)中的血管生成,但发病机制尚不清楚。过氧化物酶体增殖物激活受体γ(PPARγ)在成人肺动脉高压中减少,但 ET-1-PPARγ 相互作用是否会损害 PPHN 中的内皮细胞功能和血管生成仍不清楚。我们假设,增加的 PPHN 肺动脉内皮细胞(PAEC)ET-1 产生会降低 PPARγ 信号转导,并损害体外管形成。在宫内部分结扎动脉导管后(PPHN)和对照组从胎儿羊的近端 PAEC 中采集 PPARγ 和磷酸化 PPARγ 蛋白,并在正常和 PPHN PAEC 中进行比较 ± ET-1 和 bosentan(ETA/ETB 受体阻滞剂)。管形成在 PPARγ 激动剂 ± ET-1、N-硝基-l-精氨酸(LNA)(NOS 抑制剂)和 PPARγ siRNA 的反应中进行评估。暴露于 PPARγ 激动剂和 PPARγ siRNA 后测量内皮型一氧化氮合酶(eNOS)、磷酸化 eNOS 和 NO 产生。在基线时,PPHN PAEC 表现出管形成和 PPARγ 蛋白表达和活性降低。PPARγ 激动剂将 PPHN 管形成恢复正常。ET-1 降低了正常和 PPHN PAEC 的管形成,这被 PPARγ 激动剂挽救。ET-1 降低了 PPARγ 蛋白和活性,这被 bosentan 阻止。PPARγ 激动剂增加了正常和 PPHN PAEC 中的 eNOS 蛋白和活性以及 NO 产生。LNA 抑制了 PPARγ 激动剂对管形成的作用。PPARγ siRNA 降低了正常 PAEC 中的 eNOS 蛋白和管形成。我们得出结论,ET-1 降低了 PPARγ 信号转导,并导致 PPHN 中的 PAEC 功能障碍和血管生成受损。我们推测,旨在降低 ET-1 产生的治疗方法将恢复 PPARγ 信号转导,维持内皮功能,并改善 PPHN 中的血管生成。