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鉴定 NFAT5 为集合管中 EDN1 基因的转录调节因子。

Identification of NFAT5 as a transcriptional regulator of the EDN1 gene in collecting duct.

机构信息

Division of Nephrology, University of Utah Health Sciences Center , Salt Lake City, Utah.

Metabolic Phenotyping Core, University of Utah Health Sciences Center , Salt Lake City, Utah.

出版信息

Am J Physiol Renal Physiol. 2019 Mar 1;316(3):F481-F487. doi: 10.1152/ajprenal.00509.2018. Epub 2019 Jan 9.

Abstract

The inner medullary collecting duct (IMCD) produces very high levels of endothelin-1 (ET-1) that acts as an autocrine inhibitor of IMCD Na and water reabsorption. Recent studies suggest that IMCD ET-1 production is enhanced by extracellular hypertonicity as can occur during high salt intake. Although NFAT5 has been implicated in the IMCD ET-1 hypertonicity response, no studies in any cell type have identified NFAT5 as a transcriptional regulator of the EDN1 gene; the current study examined this using a mouse IMCD cell line (IMCD3). Media hypertonicity increased IMCD3 ET-1 mRNA in a dose- and time-dependent manner associated with increased NFAT5 nuclear localization. Knockdown of NFAT5 using small-interfering RNA or by CRISPR/Cas9-mediated targeting of exon 4 of the NFAT5 gene reduced the ET-1 hypertonicity response. Chromatin immunoprecipitation using an NFAT5 antibody pulled down ET-1 promoter regions containing NFAT5 consensus binding sequences. Transfected ET-1 promoter reporter constructs revealed maximal hypertonicity-induced reporter activity in the proximal 1-kb region; mutation of the two NFAT5 consensus-binding sites in this region abolished hypertonicity-induced reporter activity. The 1-kb ET-1 promoter-reporter construct lost hypertonicity responsiveness when transfected in CRISPR/Cas9-induced NFAT5-deficient cells. In summary, these findings represent the first description that NFAT5 is a direct transcriptional regulator of the EDN1 gene in IMCD cells and point to a potentially important mechanism by which body Na homeostasis is maintained.

摘要

内髓集合管(IMCD)产生非常高水平的内皮素-1(ET-1),作为 IMCD Na 和水重吸收的自分泌抑制剂。最近的研究表明,当高盐摄入时会发生细胞外高渗,这会增强 IMCD ET-1 的产生。尽管 NFAT5 已被牵连到 IMCD ET-1 的高渗反应中,但在任何细胞类型中都没有研究表明 NFAT5 是 EDN1 基因的转录调节剂;本研究使用小鼠 IMCD 细胞系(IMCD3)对此进行了检查。高渗培养基以剂量和时间依赖的方式增加 IMCD3 ET-1 mRNA,与 NFAT5 核定位增加相关。使用小干扰 RNA 或通过 CRISPR/Cas9 介导的 NFAT5 基因外显子 4靶向敲低 NFAT5 ,减少了 ET-1 的高渗反应。使用 NFAT5 抗体进行的染色质免疫沉淀法拉下了包含 NFAT5 共有结合序列的 ET-1 启动子区域。转染的 ET-1 启动子报告基因构建体显示,在近端 1-kb 区域中最大程度地诱导了高渗性诱导的报告基因活性;该区域中的两个 NFAT5 共有结合位点的突变消除了高渗性诱导的报告基因活性。在转染 CRISPR/Cas9 诱导的 NFAT5 缺陷细胞时,1-kb ET-1 启动子-报告基因构建体失去了高渗性反应性。总之,这些发现代表了第一个描述 NFAT5 是 IMCD 细胞中 EDN1 基因的直接转录调节剂的描述,并指出了维持体内 Na 平衡的一个潜在重要机制。

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