LncRNA‐WAKMAR2 regulates expression of CLDN1 to affect skin barrier through recruiting c‐Fos

转录组 核糖核酸 染色质 体内 角质形成细胞 紧密连接 生物 染色质免疫沉淀 细胞生物学 长非编码RNA 基因表达 分子生物学 化学 体外 基因 发起人 遗传学
作者
Yunhua Tu,Li Wang,Xiaoli Wang,Wenjuan Wu,Ying Tu,Dandan Zou,Yuanyuan Deng,Jue Qi,Can Cao,Dan Xu,Yanjie Chai,Yun Zhu,Juan Zhang,Jun Sun,Fan Lai,Li He
出处
期刊:Contact Dermatitis [Wiley]
卷期号:88 (3): 188-200 被引量:7
标识
DOI:10.1111/cod.14256
摘要

Chronic actinic dermatitis (CAD) is an immune-mediated photo-allergic skin disease. In the clinic, the treatment of this disease is hampered by the lack of proper understanding of the skin barrier dysfunction mechanism.To illuminate the mechanism of skin barrier dysfunction in CAD.Transcriptome sequencing and protein profiling were used to detect skin barrier injury-related genes. RNA pull down, a promoter-reporter gene assay, and chromatin isolation by RNA purification-sequencing were used to elucidate the effect of WAKMAR2 in skin barrier functionality.Transcriptome sequencing from patient's tissues showed a significantly decreased expression of WAKMAR2. Down-regulation of WAKMAR2 destroyed the keratinocyte barrier. Moreover, WAKMAR2 can directly bind to the c-Fos protein. This novel long non-coding RNA (LncRNA)-protein complexes were targeted to the CLDN1 promotor. Overexpression of WAKMAR2 enhanced the promoter activity of CLDN1, while the addition of AP-1 inhibitor could reverse this phenomenon. Furthermore, our in vivo results suggested that expression of WAKMAR2 was required for the repair of skin damage in mice induced by ultraviolet irradiation.We identified a crucial LncRNA (WAKMAR2) for the protection of the skin barrier in vitro and in vivo. Mechanically, it can specifically interact with c-Fos protein for the regulation of CLDN1, a finding which could be applied for CAD treatment.
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