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Identification of two initiator elements in the bidirectional promoter of the human dihydrofolate reductase and mismatch repair protein 1 genes

机译:人二氢叶酸还原酶和错配修复蛋白1基因双向启动子中的两个启动子元素的鉴定。

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The human dihydrofolate reductase (DHFR) gene and mismatch repair protein 1 (MRP1) genes are organized in a head-to-head configuration separated by an 90 base pair sequence. We have previously shown that as small as a 114 bp promoter sequences is sufficient for accurate and efficient initiation of divergent transcription. In this study, the mechanism of accurate transcription initiation in vivo from this short bidirectional promoter was analyzed by a newly developed highly sensitive primer extension assay. The GC boxes in the middle of this sequence were essential for bidirectional promoter activity, but not sufficient for accurate initiation. The sequences overlapping the transcription initiation sites of the DHFR and MRP1 genes were shown to function as the initiator, which directs transcription from an internal site. These initiators were strictly position dependent and were active only when located from 40 to 50 base pairs downstream from the GC box. Although there is no apparent sequence homology between two initiators, a common nuclear factor bound to these elements. Existence of two initiators located on both sides of the middle GC box seems to be the molecular basis of bidirectional activity of this short DNA sequence.
机译:人二氢叶酸还原酶(DHFR)基因和错配修复蛋白1(MRP1)基因以头对头的结构排列,并由90个碱基对的序列隔开。先前我们已经表明,小至114 bp的启动子序列足以准确而有效地启动差异转录。在这项研究中,通过新开发的高度灵敏的引物延伸测定法分析了从这种短的双向启动子体内准确转录起始的机制。该序列中间的GC盒对于双向启动子活性是必不可少的,但不足以精确启动。与DHFR和MRP1基因的转录起始位点重叠的序列显示出起起始子的作用,该引物指导内部位点的转录。这些引发剂严格地取决于位置,并且仅当位于GC盒下游40至50个碱基对时才起作用。尽管两个引发剂之间没有明显的序列同源性,但共有一个核因子与这些元素结合。位于中间GC盒两侧的两个引发剂的存在似乎是该短DNA序列双向活性的分子基础。

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