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利用荧光光学成像技术观察脂多糖诱导的炎症性肺损伤过程中Fra-1/AP-1的激活情况。

Visualization of Fra-1/AP-1 activation during LPS-induced inflammatory lung injury using fluorescence optical imaging.

作者信息

Rajasekaran Subbiah, Tamatam Chandramohan R, Potteti Haranatha R, Raman Venu, Lee Jae-Woo, Matthay Michael A, Mehta Dolly, Reddy Narsa M, Reddy Sekhar P

机构信息

Division of Developmental Biology and Basic Research, Department of Pediatrics, University of Illinois at Chicago, Chicago, Illinois;

Division of Cancer Imaging Research, Department of Radiology and Radiological Sciences, The Johns Hopkins University, Baltimore, Maryland;

出版信息

Am J Physiol Lung Cell Mol Physiol. 2015 Aug 15;309(4):L414-24. doi: 10.1152/ajplung.00315.2014. Epub 2015 Jun 12.

Abstract

Inappropriate lung inflammatory response following oxidant and toxicant exposure can lead to abnormal repair and disease pathogenesis, including fibrosis. Thus early detection of molecular and cellular processes and mediators promoting lung inflammation is necessary to develop better strategies for therapeutic intervention and disease management. Previously, we have shown that transcription factor Fra-1/AP-1 plays key roles in lung inflammatory response, as Fra-1-null mice are less susceptible than wild-type mice to LPS-induced lung injury and mortality. Herein, we developed a transgenic reporter mouse model expressing tdTomato under the control of FRA-1 (human) promoter (referred to as FRA-1(TdTg) mice) to monitor its activation during inflammatory lung injury using fluorescence protein-based optical imaging and molecular analysis in vivo and ex vivo. A higher red fluorescent signal was observed in the lungs of LPS-treated FRA-1(TdTg) mice compared with vehicle controls, and Western blot and qRT-PCR analyses revealed a significant correlation with the FRA-1-tdTomato reporter expression. Immunocolocalization demonstrated expression of FRA-1-tdTomato largely in lung alveolar macrophages and to some extent in epithelial cells. Moreover, we validated these results with a second reporter mouse model that expressed green fluorescent protein upon activation of endogenous Fra-1 promoter. Additionally, we demonstrated increased expression of FRA-1 in alveolar macrophages in human lung instilled with Escherichia coli ex vivo. Collectively, our data obtained from two independent reporter mouse models and from human samples underscore the significance of Fra-1 activation in alveolar macrophages during inflammatory lung injury and may aid in developing strategies to target this transcription factor in lung injury and repair.

摘要

氧化剂和毒物暴露后不适当的肺部炎症反应可导致异常修复和疾病发病机制,包括纤维化。因此,早期检测促进肺部炎症的分子和细胞过程及介质对于制定更好的治疗干预和疾病管理策略是必要的。此前,我们已经表明转录因子Fra-1/AP-1在肺部炎症反应中起关键作用,因为Fra-1基因敲除小鼠比野生型小鼠对脂多糖诱导的肺损伤和死亡率更不易感。在此,我们构建了一种转基因报告小鼠模型,该模型在FRA-1(人)启动子的控制下表达tdTomato(称为FRA-1(TdTg)小鼠),以利用基于荧光蛋白的光学成像以及体内和体外分子分析监测其在炎症性肺损伤期间的激活情况。与载体对照相比,在经脂多糖处理的FRA-1(TdTg)小鼠的肺中观察到更高的红色荧光信号,蛋白质免疫印迹和定量逆转录-聚合酶链反应分析显示与FRA-1-tdTomato报告基因表达存在显著相关性。免疫共定位表明FRA-1-tdTomato主要在肺泡巨噬细胞中表达,在一定程度上也在上皮细胞中表达。此外,我们用另一种报告小鼠模型验证了这些结果,该模型在激活内源性Fra-1启动子时表达绿色荧光蛋白。此外,我们还证明了在体外用人源肺灌注大肠杆菌后,肺泡巨噬细胞中FRA-1的表达增加。我们从两个独立的报告小鼠模型和人源样本中获得的数据共同强调了Fra-1激活在炎症性肺损伤期间肺泡巨噬细胞中的重要性,并可能有助于制定针对该转录因子进行肺损伤和修复治疗的策略。

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