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β-连环蛋白调控的细胞外基质基质细胞蛋白在炎症性肺损伤后的上皮修复中的作用。

Role of β-catenin-regulated CCN matricellular proteins in epithelial repair after inflammatory lung injury.

机构信息

Division of Pulmonary, Critical Care, and Sleep Medicine, Department of Medicine, National Jewish Health, Denver, CO 80206, USA.

出版信息

Am J Physiol Lung Cell Mol Physiol. 2013 Mar 15;304(6):L415-27. doi: 10.1152/ajplung.00180.2012. Epub 2013 Jan 11.

Abstract

Repair of the lung epithelium after injury is integral to the pathogenesis and outcomes of diverse inflammatory lung diseases. We previously reported that β-catenin signaling promotes epithelial repair after inflammatory injury, but the β-catenin target genes that mediate this effect are unknown. Herein, we examined which β-catenin transcriptional coactivators and target genes promote epithelial repair after inflammatory injury. Transmigration of human neutrophils across cultured monolayers of human lung epithelial cells resulted in a fall in transepithelial resistance and the formation of discrete areas of epithelial denudation ("microinjury"), which repaired via cell spreading by 96 h. In mice treated with intratracheal (i.t.) LPS or keratinocyte chemokine, neutrophil emigration was associated with increased permeability of the lung epithelium, as determined by increased bronchoalveolar lavage (BAL) fluid albumin concentration, which decreased over 3-6 days. Activation of β-catenin/p300-dependent gene expression using the compound ICG-001 accelerated epithelial repair in vitro and in murine models. Neutrophil transmigration induced epithelial expression of the β-catenin/p300 target genes Wnt-induced secreted protein (WISP) 1 and cysteine-rich (Cyr) 61, as determined by real-time PCR (qPCR) and immunostaining. Purified neutrophil elastase induced WISP1 upregulation in lung epithelial cells, as determined by qPCR. WISP1 expression increased in murine lungs after i.t. LPS, as determined by ELISA of the BAL fluid and qPCR of whole lung extracts. Finally, recombinant WISP1 and Cyr61 accelerated repair, and Cyr61-neutralizing antibodies delayed repair of the injured epithelium in vitro. We conclude that β-catenin/p300-dependent expression of WISP1 and Cyr61 is critical for epithelial repair and represents a potential therapeutic target to promote epithelial repair after inflammatory injury.

摘要

肺上皮细胞在损伤后的修复对于多种炎症性肺疾病的发病机制和结果至关重要。我们之前曾报道过β-catenin 信号通路促进炎症损伤后的上皮修复,但介导这种作用的β-catenin 靶基因尚不清楚。在此,我们研究了哪些β-catenin 转录共激活因子和靶基因促进炎症损伤后的上皮修复。人中性粒细胞穿过人肺上皮细胞培养单层的迁移导致跨上皮电阻下降,并形成离散的上皮剥脱区域(“微损伤”),这些区域在 96 小时内通过细胞扩展修复。在接受气管内(i.t.)LPS 或角质形成细胞趋化因子治疗的小鼠中,中性粒细胞的迁移与肺上皮通透性的增加有关,这通过支气管肺泡灌洗液(BAL)中白蛋白浓度的增加来确定,该浓度在 3-6 天内降低。使用化合物 ICG-001 激活β-catenin/p300 依赖性基因表达可加速体外和小鼠模型中的上皮修复。中性粒细胞迁移诱导上皮细胞表达β-catenin/p300 靶基因 Wnt 诱导的分泌蛋白(WISP)1 和富含半胱氨酸(Cyr)61,通过实时 PCR(qPCR)和免疫染色确定。通过 qPCR 确定纯化的中性粒细胞弹性蛋白酶诱导肺上皮细胞中 WISP1 的上调。通过 BAL 液的 ELISA 和全肺提取物的 qPCR 确定 i.t. LPS 后小鼠肺部 WISP1 的表达增加。最后,重组 WISP1 和 Cyr61 加速修复,而 Cyr61 中和抗体延迟体外损伤上皮的修复。我们得出结论,β-catenin/p300 依赖性表达的 WISP1 和 Cyr61 对于上皮修复至关重要,代表了促进炎症损伤后上皮修复的潜在治疗靶点。

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