孕酮依赖的RUSH/SMARCA3与Egr-1之间的脱氧核糖核酸环化介导c-Rel的抑制作用。
Progesterone-dependent deoxyribonucleic acid looping between RUSH/SMARCA3 and Egr-1 mediates repression by c-Rel.
作者信息
Hewetson Aveline, Chilton Beverly S
机构信息
Department of Cell Biology and Biochemistry, Texas Tech University Health Sciences Center, Texas 79430, USA.
出版信息
Mol Endocrinol. 2008 Apr;22(4):813-22. doi: 10.1210/me.2007-0432. Epub 2008 Jan 3.
Steroids regulate alternative splicing of RUSH/SMARCA3. The full-length, progesterone-dependent alpha-isoform and the 3'-truncated, estrogen-dependent beta-isoform have identical DNA-binding domains, nuclear localization signals, and RING fingers. Transcription of RUSH/SMARCA3 is mediated by a bipartite progesterone receptor half-site/overlapping Y-box combination (-38/-26), where progesterone activation is attenuated by nuclear factor Y binding. Regulation also involves two GC-rich sequences in the proximal promoter (-162/+90) and a RUSH/SMARCA3 site (-616/-611) in the 5'-untranslated region. Isoform-specific binding to the RUSH/SMARCA3 site is dictated by the hormonal milieu, as is the availability of factors that bind to the distal GC-rich site (-131/-126), a composite binding site for Egr-1/specific protein-1/3/Myc-associated zinc finger protein/myeloid zinc finger-1/c-Rel, and the proximal GC-rich site (-62/-53), which binds only Sp1/3. TransSignal TF-TF interaction arrays, supershift assays, and chromatin immunoprecipitation analyses confirmed strong physical interactions between RUSH/Egr-1 and RUSH/c-Rel that were visualized with fluorescent microscopy. Higher-order, long-range interactions between RUSH and Egr-1/c-Rel derivative of the anisotropic flexibility of the intervening DNA sequence were shown by Chromosome Conformation Capture assay. Glutathione S-transferase pull-downs confirmed that the RING finger is the protein-binding domain, suggesting that the RUSH isoforms have equivalent potential for protein interactions. Transient transfection assays showed that the cooperative interaction between RUSH and Egr-1 mediates repression by c-Rel. Thus, progesterone-induced transcription is fine-tuned by isoform-specific autoregulation, in which newly synthesized RUSH-1alpha binds DNA and interacts physically with liganded Egr-1 in the proximal promoter via a DNA-looping mechanism to mediate repression by c-Rel. In the absence of progesterone induction, RUSH-1beta replaces RUSH-1alpha binding, Egr-1 and c-Rel are unavailable as molecular ties, and DNA looping is disfavored.
类固醇调节RUSH/SMARCA3的可变剪接。全长的、孕酮依赖性的α异构体和3'-截短的、雌激素依赖性的β异构体具有相同的DNA结合结构域、核定位信号和RING结构域。RUSH/SMARCA3的转录由一个二分的孕酮受体半位点/重叠的Y盒组合(-38/-26)介导,其中孕酮激活因核因子Y结合而减弱。调节还涉及近端启动子(-162/+90)中的两个富含GC的序列和5'-非翻译区中的一个RUSH/SMARCA3位点(-616/-611)。对RUSH/SMARCA3位点的异构体特异性结合由激素环境决定,与结合到远端富含GC的位点(-131/-126)的因子的可用性一样,该位点是Egr-1/特异性蛋白-1/3/Myc相关锌指蛋白/髓系锌指-1/c-Rel的复合结合位点,以及近端富含GC的位点(-62/-53),其仅结合Sp1/3。转信号TF-TF相互作用阵列、超迁移分析和染色质免疫沉淀分析证实了RUSH/Egr-1和RUSH/c-Rel之间强烈的物理相互作用,这通过荧光显微镜观察到。染色体构象捕获分析显示了RUSH与Egr-1/c-Rel衍生物之间的高阶、远距离相互作用,这是由中间DNA序列的各向异性灵活性引起的。谷胱甘肽S-转移酶下拉实验证实RING结构域是蛋白质结合结构域,表明RUSH异构体具有等效的蛋白质相互作用潜力。瞬时转染实验表明RUSH与Egr-1之间的协同相互作用介导了c-Rel的抑制作用。因此,孕酮诱导的转录通过异构体特异性的自动调节进行微调,其中新合成的RUSH-1α结合DNA,并通过DNA环化机制在近端启动子中与配体化的Egr-1进行物理相互作用,以介导c-Rel的抑制作用。在没有孕酮诱导的情况下,RUSH-1β取代RUSH-1α的结合,Egr-1和c-Rel作为分子纽带不可用,并且DNA环化不受青睐。
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