Faculty of Biology, M.V. Lomonosov Moscow State University, Moscow, Russia.
Centre de recherche, Centre hospitalier de l'Université de Montréal (CRCHUM) - Technopôle Angus, Montreal, PQ, Canada.
Cell Calcium. 2015 Sep;58(3):317-24. doi: 10.1016/j.ceca.2015.06.009. Epub 2015 Jun 30.
Previously, we reported that Ca(2+) depletion increased permeability of the plasma membrane for Na(+). This study examined the relative impact of [Na(+)]i/[K(+)]i-mediated signaling on transcriptomic changes in cultured vascular smooth muscle cells from rat aorta (VSMC) subjected to Ca(2+)-depletion by extra-(EGTA) and intracellular (BAPTA-AM) Ca(2+) chelators. Na(+),K(+)-ATPase inhibition in K(+)-free medium during 3 h led to elevation of [Na(+)]i and attenuation of [K(+)]i by ∼7- and 10-fold, whereas Ca(2+)-depletion resulted in alteration of these parameters by ∼3- and 2-fold, respectively. Augmented VSMC permeability for Na(+) and elevation of the [Na(+)]i/[K(+)]i ratio was triggered by addition to Ca(2+)-free medium 50 μM EGTA and was not affected by 10 μM BAPTA-AM. Na(+),K(+)-ATPase inhibition and Ca(2+)-depletion changed expression of 3677 and 4610 mRNA transcripts, respectively. We found highly significant (p<10(-12)) positive (R(2)>0.51) correlation between levels of expression of 2071 transcripts whose expression was affected by both stimuli. Among genes whose expression in Ca(2+)-depleted cells was augmented by more than 7-fold we noted cyclic AMP-dependent transcription factor Atf3, early growth response protein Egr1 and nuclear receptor subfamily 4, group A member Nr4a1. Dissipation of transmembrane gradients of monovalent cations in high-K(+), low-Na(+)-medium abolished the increments of the [Na(+)]i/[K(+)]i ratio as well as the augmented expression of these genes triggered by incubation of VSMC in EGTA containing medium. Thus, our results demonstrate, for the first time, that robust transcriptomic changes triggered by Ca(2+)-depletion in the presence of extracellular Ca(2+)-chelators are at least partially mediated by elevation of the [Na(+)]i/[K(+)]i ratio and activation of Ca(2+)i-independent, [Na(+)]i/[K(+)]i-mediated mechanism of excitation-transcription coupling. These results shad a new light on analysis of data obtained in cells subjected to long-term exposure to Ca(2+) chelators.
先前,我们曾报道过钙耗竭会增加质膜对钠离子的通透性。本研究通过使用细胞外(EGTA)和细胞内(BAPTA-AM)钙螯合剂来耗竭钙,观察了在大鼠主动脉血管平滑肌细胞(VSMC)中,[Na+]i/[K+]i 介导的信号对转录组变化的相对影响。在无钾介质中,通过抑制钠钾 ATP 酶 3 小时,可使 [Na+]i 升高 7 倍,[K+]i 降低 10 倍,而钙耗竭使这些参数分别改变 3 倍和 2 倍。在无钙介质中加入 50μM EGTA 可引发 VSMC 对钠离子的通透性增加,[Na+]i/[K+]i 比值升高,而 10μM BAPTA-AM 则不影响这一过程。钠钾 ATP 酶抑制和钙耗竭分别改变了 3677 和 4610 个 mRNA 转录本的表达。我们发现,在两种刺激因素的影响下,有 2071 个转录本的表达水平具有高度显著的正相关(p<10(-12))(R(2)>0.51)。在钙耗竭细胞中表达增加超过 7 倍的基因中,我们注意到了环腺苷酸依赖性转录因子 Atf3、早期生长反应蛋白 Egr1 和核受体亚家族 4、A 型成员 Nr4a1。在高钾低钠介质中,一价阳离子跨膜梯度的耗散消除了[Na+]i/[K+]i 比值的增加,以及 EGTA 孵育介质中 VSMC 引发的这些基因表达的增加。因此,我们的研究结果首次表明,在存在细胞外钙螯合剂的情况下,钙耗竭引起的强大转录组变化至少部分是通过升高[Na+]i/[K+]i 比值和激活 Ca(2+)i 独立的、[Na+]i/[K+]i 介导的兴奋-转录偶联机制来介导的。这些结果为分析长期暴露于钙螯合剂的细胞所获得的数据提供了新的视角。
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