Gassanov Natig, Er Fikret, Michels Guido, Zagidullin Naufal, Brandt Mathias C, Hoppe Uta C
Department of Internal Medicine III, University of Cologne, Kerpener Str. 62, 50937 Cologne, Germany.
J Physiol. 2009 Mar 15;587(Pt 6):1319-29. doi: 10.1113/jphysiol.2008.168385. Epub 2009 Jan 26.
The cardiac transient outward current I(to) is regulated by thyroid hormone (T3). However, it remains unclear whether T3 directly modulates underlying gene transcription and which thyroid receptor (TR) isoform might be responsible for gene transactivation. To clarify this situation, we analysed the role of T3 and its receptors alpha1 (TRalpha1) and beta1 (TRbeta1) in regulation of KCNA4, KCND2, KCND3 and KCNIP2 transcription in rat cardiomyocytes. Initial results demonstrated a T3-mediated increase of I(to) current density. T3 stimulation enhanced KCND2 and KCND3 expression and decreased KCNA4 transcription, while KCNIP2 remained unaffected. To dissect the role of TRalpha1 and TRbeta1 in T3-dependent I(to) modulation, TRalpha1 and TRbeta1 were overexpressed in cardiomyocytes by adenovirus-mediated gene transfer. TRalpha1 increased I(to), while TRbeta1 significantly reduced I(to) in size, which was associated with TRalpha1-mediated increase and TRbeta1-mediated reduction of KCND2/3 transcription. To further evaluate a possible direct interaction of TRalpha1 and TRbeta1 with the KCND3 promoter, TR expression vectors were cotransfected with a construct containing 2335 bp of the KCND3 5'-flanking sequence linked to a luciferase reporter into ventricular myocytes. While the TRalpha1 aporeceptor enhanced KCND3 transcription, the TRbeta1 aporeceptor suppressed KCND3 expression, with both effects exhibiting ligand-dependent amplification upon T3 stimulation. Deletion of the KCND3 5'-flanking region localized the suppressible promoter sequence for TRbeta1 to within -293 bp and the activating promoter sequence for TRalpha1 to within -2335 to -1654 bp of the transcription start site. Disruption of putative TR binding sites by mutagenesis abolished the TRalpha1- (G-1651T) and TRbeta1- (G-73T) mediated effects, indicating that TRalpha1 and TRbeta1 response elements map to different regions of the KCND3 promoter. Thus, I(to) is modulated by diverse T3-dependent regulation of underlying gene transcription. TRalpha1 and TRbeta1 exhibit distinct effects on KCND3 transactivation with TRalpha1 enhancing and TRbeta1 suppressing KCND3 transcription.
心脏瞬时外向电流I(to)受甲状腺激素(T3)调节。然而,T3是否直接调节潜在的基因转录以及哪种甲状腺受体(TR)亚型可能负责基因反式激活仍不清楚。为了阐明这种情况,我们分析了T3及其受体α1(TRα1)和β1(TRβ1)在大鼠心肌细胞中对KCNA4、KCND2、KCND3和KCNIP2转录调控中的作用。初步结果显示T3介导I(to)电流密度增加。T3刺激增强了KCND2和KCND3的表达并降低了KCNA4的转录,而KCNIP2不受影响。为了剖析TRα1和TRβ1在T3依赖性I(to)调节中的作用,通过腺病毒介导的基因转移在心肌细胞中过表达TRα1和TRβ1。TRα1增加了I(to),而TRβ1显著减小了I(to)的大小,这与TRα1介导的KCND2/3转录增加和TRβ1介导的KCND2/3转录减少有关。为了进一步评估TRα1和TRβ1与KCND3启动子可能的直接相互作用,将TR表达载体与包含与荧光素酶报告基因相连的KCND3 5'侧翼序列2335 bp的构建体共转染到心室肌细胞中。虽然TRα1无配体受体增强了KCND3转录,但TRβ1无配体受体抑制了KCND3表达,在T3刺激下,这两种效应均表现出配体依赖性放大。删除KCND3 5'侧翼区域将TRβ1的可抑制启动子序列定位在转录起始位点的 -293 bp范围内,将TRα1的激活启动子序列定位在 -2335至 -1654 bp范围内。通过诱变破坏假定的TR结合位点消除了TRα1(G - 1651T)和TRβ1(G - 73T)介导的效应,表明TRα1和TRβ1反应元件定位于KCND3启动子的不同区域。因此,I(to)受潜在基因转录的多种T3依赖性调节。TRα1和TRβ1对KCND3反式激活表现出不同的影响,TRα1增强而TRβ1抑制KCND3转录。
Zotero 插件