Morancho Beatriz, Minguillón Jordi, Molkentin Jeffery D, López-Rodríguez Cristina, Aramburu Jose
Immunology Unit, Department of Experimental and Health Sciences, Universitat Pompeu Fabra, Barcelona, Spain.
BMC Mol Biol. 2008 Jan 25;9:13. doi: 10.1186/1471-2199-9-13.
The transcription factor NFAT5/TonEBP regulates the response of mammalian cells to hypertonicity. However, little is known about the physiopathologic tonicity thresholds that trigger its transcriptional activity in primary cells. Wilkins et al. recently developed a transgenic mouse carrying a luciferase reporter (9xNFAT-Luc) driven by a cluster of NFAT sites, that was activated by calcineurin-dependent NFATc proteins. Since the NFAT site of this reporter was very similar to an optimal NFAT5 site, we tested whether this reporter could detect the activation of NFAT5 in transgenic cells.
The 9xNFAT-Luc reporter was activated by hypertonicity in an NFAT5-dependent manner in different types of non-transformed transgenic cells: lymphocytes, macrophages and fibroblasts. Activation of this reporter by the phorbol ester PMA plus ionomycin was independent of NFAT5 and mediated by NFATc proteins. Transcriptional activation of NFAT5 in T lymphocytes was detected at hypertonic conditions of 360-380 mOsm/kg (isotonic conditions being 300 mOsm/kg) and strongly induced at 400 mOsm/kg. Such levels have been recorded in plasma in patients with osmoregulatory disorders and in mice deficient in aquaporins and vasopressin receptor. The hypertonicity threshold required to activate NFAT5 was higher in bone marrow-derived macrophages (430 mOsm/kg) and embryonic fibroblasts (480 mOsm/kg). Activation of the 9xNFAT-Luc reporter by hypertonicity in lymphocytes was insensitive to the ERK inhibitor PD98059, partially inhibited by the PI3-kinase inhibitor wortmannin (0.5 microM) and the PKA inhibitor H89, and substantially downregulated by p38 inhibitors (SB203580 and SB202190) and by inhibition of PI3-kinase-related kinases with 25 microM LY294002. Sensitivity of the reporter to FK506 varied among cell types and was greater in primary T cells than in fibroblasts and macrophages.
Our results indicate that NFAT5 is a sensitive responder to pathologic increases in extracellular tonicity in T lymphocytes. Activation of NFAT5 by hypertonicity in lymphocytes was mediated by a combination of signaling pathways that differed from those required in other cell types. We propose that the 9xNFAT-Luc transgenic mouse model might be useful to study the physiopathological regulation of both NFAT5 and NFATc factors in primary cells.
转录因子NFAT5/TonEBP可调节哺乳动物细胞对高渗状态的反应。然而,关于在原代细胞中触发其转录活性的生理病理渗透压阈值却知之甚少。威尔金斯等人最近培育出一种转基因小鼠,其携带一个由一组NFAT位点驱动的荧光素酶报告基因(9xNFAT-Luc),该报告基因可被钙调神经磷酸酶依赖性NFATc蛋白激活。由于该报告基因的NFAT位点与最佳NFAT5位点非常相似,我们测试了该报告基因能否检测转基因细胞中NFAT5的激活情况。
在不同类型的未转化转基因细胞(淋巴细胞、巨噬细胞和成纤维细胞)中,9xNFAT-Luc报告基因以NFAT5依赖的方式被高渗激活。佛波酯PMA加离子霉素对该报告基因的激活不依赖于NFAT5,而是由NFATc蛋白介导。在360 - 380 mOsm/kg的高渗条件下(等渗条件为300 mOsm/kg)检测到T淋巴细胞中NFAT5的转录激活,在400 mOsm/kg时强烈诱导。这种水平已在患有渗透调节障碍的患者血浆以及水通道蛋白和血管升压素受体缺陷的小鼠中记录到。骨髓来源的巨噬细胞(430 mOsm/kg)和胚胎成纤维细胞(480 mOsm/kg)激活NFAT5所需的高渗阈值更高。淋巴细胞中高渗对9xNFAT-Luc报告基因的激活对ERK抑制剂PD98059不敏感,部分受到PI3激酶抑制剂渥曼青霉素(0.5 microM)和PKA抑制剂H89的抑制,并且被p38抑制剂(SB203580和SB202190)以及用25 microM LY294002抑制PI3激酶相关激酶而大幅下调。报告基因对FK506的敏感性因细胞类型而异,在原代T细胞中比在成纤维细胞和巨噬细胞中更高。
我们的结果表明,NFAT5是T淋巴细胞中细胞外渗透压病理性升高的敏感应答者。淋巴细胞中高渗对NFAT5的激活是由多种信号通路共同介导的,这些信号通路与其他细胞类型所需的不同。我们认为9xNFAT-Luc转基因小鼠模型可能有助于研究原代细胞中NFAT5和NFATc因子的生理病理调节。
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