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钠钾ATP酶α1亚基缺乏增强了高渗对椎间盘髓核细胞的抗增殖作用。

Deficiency in the α1 subunit of Na+/K+-ATPase enhances the anti-proliferative effect of high osmolality in nucleus pulposus intervertebral disc cells.

作者信息

Mavrogonatou Eleni, Papadimitriou Konstantinos, Urban Jill P, Papadopoulos Vassilios, Kletsas Dimitris

机构信息

Laboratory of Cell Proliferation and Ageing, Institute of Biosciences and Applications, National Centre for Scientific Research "Demokritos", Athens, Greece.

Department of Food Science and Human Nutrition, Agricultural University of Athens, Iera Odos 75, Athens, Greece.

出版信息

J Cell Physiol. 2015 Dec;230(12):3037-48. doi: 10.1002/jcp.25040.

DOI:10.1002/jcp.25040
PMID:25967398
Abstract

Intervertebral disc cells are constantly exposed to a hyperosmotic environment. Among cellular responses towards this stress is the inhibition of proliferation through the activation of p38 MAPK and p53. In an effort to further elucidate the biochemical pathways triggered by hyperosmotic stress, we assessed the high osmolality-induced transcriptional changes of bovine nucleus pulposus cells using whole-genome arrays. A 5- and a 24-h hyperosmotic treatment led to the differential expression of >100 and >200 genes, respectively, including nine genes encoding transporters (SLC4A11, SLC5A3, ATP1A1, SLC38A2, KCNK17, KCTD20, KCTD11, SLC7A5, and CLCA2). Differences in the transcriptional profile of these selected genes, as indicated by the microarrays experiments, were validated by qRT-PCR in 2D and 3D cell cultures, under hyperosmolar salt and sorbitol conditions, revealing the presence of a common triggering signal for osmotic adaptation. The key signaling molecules p38 MAPK and p53 were demonstrated to differently participate in the regulation of the aforementioned transporters. Finally, siRNA-mediated knocking-down of each one of the three transporters with the highest and sustained over-expression (i.e., SLC4A11, SLC5A3, and ATP1A1) had a distinct outcome on the transcriptional profile of the other transporters, on p38 MAPK and p53 phosphorylation and consequently on cell cycle progression. The inhibition of ATP1A1 had the most prominent effect on the transcription of the rest of the transporters and was found to enhance the anti-proliferative effect of hyperosmotic conditions through an increased G2/M cell cycle block, ascribing to this pump a central role in the osmoregulatory response of nucleus pulposus cells.

摘要

椎间盘细胞持续暴露于高渗环境中。细胞对这种应激的反应之一是通过激活p38丝裂原活化蛋白激酶(p38 MAPK)和p53来抑制增殖。为了进一步阐明高渗应激触发的生化途径,我们使用全基因组芯片评估了高渗诱导的牛髓核细胞转录变化。5小时和24小时的高渗处理分别导致100多个和200多个基因的差异表达,其中包括9个编码转运蛋白的基因(溶质载体家族4成员11(SLC4A11)、溶质载体家族5成员3(SLC5A3)、ATP酶1A1(ATP1A1)、溶质载体家族38成员2(SLC38A2)、钾通道亚家族K成员17(KCNK17)、钾通道四聚体结构域包含蛋白20(KCTD20)、钾通道四聚体结构域包含蛋白11(KCTD11)、溶质载体家族7成员5(SLC7A5)和钙激活氯离子通道蛋白2(CLCA2))。如微阵列实验所示,这些选定基因转录谱的差异在二维和三维细胞培养中,于高渗盐和山梨醇条件下通过定量逆转录聚合酶链反应(qRT-PCR)得到验证,揭示了存在一个共同的渗透适应触发信号。关键信号分子p38 MAPK和p53被证明以不同方式参与上述转运蛋白的调节。最后,小干扰RNA(siRNA)介导的对三个过表达最高且持续时间最长的转运蛋白(即SLC4A11、SLC5A和ATP1A1)中每一个的敲低,对其他转运蛋白的转录谱、p38 MAPK和p53磷酸化以及细胞周期进程产生了不同的影响。对ATP1A1的抑制对其余转运蛋白的转录影响最为显著,并且发现通过增加G2/M期细胞周期阻滞来增强高渗条件的抗增殖作用,这表明该泵在髓核细胞的渗透调节反应中起核心作用。

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