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Basal level transcription of the histone H10 gene is mediated by a 80 bp promoter fragment

机译:组蛋白H10基因的基础水平转录由一个80 bp的启动子片段介导

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The replacement histone H10 of the H1 group, known to interact with general transcription factors, has been found associated with transcriptionally repressed chromatin. Transcription of the gene in F9 stem cells is low but can be stimulated by treating the cells with retinoic acid. Using mutant deletions, we now demonstrate that basal level transcription in F9 cells is mediated by an 80 bp DNA fragment, located 430 bp upstream of the TATA box, which does not include the retinoic acid responsive element (RARE) known to bind retinoic acid receptors and stimulate transcription from an heterologous promoter after retinoic acid treatment. By footprinting, DMS interference, site-directed mutagenesis and UV-cross linking techniques we demonstrate that at least two nuclear factors, with MW of 90,000 and 30,000, bind to the 80 bp fragment and that this binding is necessary for transcription. Furthermore, positioning of this fragment upstream of the HSV-tk gene promoter stimulates transcription 2–3 times over control values, far less than the activity observed for this fragment in the homologous promoter, indicating that full activity of this fragment requires sequences located in the proximal part of the promoter.
机译:已经发现已知与一般转录因子相互作用的H1组的置换组蛋白H1 0 与转录抑制的染色质有关。 F9干细胞中的基因转录很低,但可以通过用视黄酸处理细胞来刺激。使用突变删除,我们现在证明F9细胞中的基础水平转录是由一个80 bp的DNA片段介导的,位于TATA盒上游430 bp,其中不包括已知与视黄酸受体结合的视黄酸响应元件(RARE)视黄酸处理后刺激异源启动子转录。通过足迹,DMS干扰,定点诱变和UV交联技术,我们证明了至少两个核因子与MW分别为90,000和30,000结合到80 bp片段,并且这种结合对于转录是必需的。此外,将该片段置于HSV-tk基因启动子的上游可刺激转录超过对照值2-3倍,远低于同源启动子中该片段的活性,表明该片段的全部活性需要位于启动子的近端部分。

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