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Interleukin~(-1)0 protects cultured fetal rat type II epithelial cells from injury induced by mechanical stretch

机译:白介素〜(-1)0保护培养的胎鼠II型上皮细胞免受机械牵张所致的伤害

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摘要

First published December 7, 2007; doi:10.1152/ajplung.00370.2007.-Mechanical ventilation plays a central role in the pathogenesis of bronchopulmonary dysplasia. However, the mechanisms by which excessive stretch of fetal or neonatal type II epithelial cells contributes to lung injury are not well defined. In these investigations, isolated embryonic day 19 fetal rat type II epithelial cells were cultured on substrates coated with fibronectin and exposed to 5% or 20% cyclic stretch to simulate mechanical forces during lung development or lung injury, respectively. Twenty percent stretch of fetal type II epithelial cells increased necrosis, apoptosis, and proliferation compared with control, unstretched samples. By ELISA and real-time PCR (qRT-PCR), 20% stretch increased secretion of IL-8 into the media and IL-8 gene expression and inhibited IL~(-1)0 release. Interestingly, administration of recombinant IL~(-1)0 before 20% stretch did not affect cell lysis but significantly reduced apoptosis and IL-8 release compared with stretched samples without IL~(-1)0. Collectively, our studies suggest that IL~(-1)0 may play an important role in protection of fetal type fl epithelial cells from injury secondary to stretch.
机译:首次发布于2007年12月7日; doi:10.1152 / ajplung.00370.2007.-机械通气在支气管肺发育不良的发病机理中起着核心作用。然而,胎儿或新生儿II型上皮细胞过度拉伸导致肺损伤的机制尚不清楚。在这些研究中,将分离的第19天胚胎胚胎的II型胎儿大鼠上皮细胞培养在涂有纤连蛋白的基质上,并暴露于5%或20%的循环拉伸下,以分别模拟肺发育或肺损伤期间的机械力。与未拉伸的对照样品相比,胎儿II型上皮细胞拉伸的百分之二十增加了坏死,凋亡和增殖。通过ELISA和实时PCR(qRT-PCR),拉伸20%可以增加IL-8向培养基的分泌和IL-8基因的表达,并抑制IL〜(-1)0的释放。有趣的是,与没有IL〜(-1)0的拉伸样品相比,在拉伸20%之前施用重组IL〜(-1)0不会影响细胞裂解,但会显着降低细胞凋亡和IL-8释放。总体而言,我们的研究表明IL〜(-1)0可能在保护胎儿型fl上皮细胞免受继发性拉伸损伤中起重要作用。

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