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Potential transcriptional regulatory regions exist upstream of the human ezrin gene promoter in esophageal carcinoma cells

机译:食管癌细胞中人ezrin基因启动子上游存在潜在的转录调控区

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摘要

We previously demonstrated that the region −87/+134 of the human ezrin gene (VIL2) exhibited promoter activity in human esophageal carcinoma EC109 cells, and a further upstream region −1324/−890 positively regulated transcription. In this study, to identify the transcriptional regulatory regions upstream of the VIL2 promoter, we cloned VIL2 −1541/−706 segment containing the −1324/−890, and investigated its transcriptional regulatory properties via luciferase assays in transiently transfected cells. In EC109 cells, it was found that VIL2 −1541/−706 possessed promoter and enhancer activities. We also localized transcriptional regulatory regions by fusing 5′- or 3′-deletion segments of VIL2 −1541/−706 to a luciferase reporter. We found that there were three positive and one negative transcriptional regulatory regions within VIL2 −1541/−706 in EC109 cells. When these regions were separately located upstream of the luciferase gene without promoter, or located upstream of the VIL2 promoter or SV40 promoter directing the luciferase gene, only VIL2 −1297/−1186 exhibited considerable promoter and enhancer activities, which were lower than those of −1541/−706. In addition, transient expression of Sp1 increased ezrin expression and the transcriptional activation of VIL2 −1297/−1186. Other three regions, although exhibiting significantly positive or negative transcriptional regulation in deletion experiments, showed a weaker or absent regulation. These data suggested that more than one region upstream of the VIL2 promoter participated in VIL2 transcription, and the VIL2 −1297/−1186, probably as a key transcriptional regulatory region, regulated VIL2 transcription in company with other potential regulatory regions.
机译:我们先前证明,人ezrin基因(VIL2)的−87 / + 134区在人食管癌EC109细胞中表现出启动子活性,而另一个上游区域-1324 / -890则正调控转录。在这项研究中,为了鉴定VIL2启动子上游的转录调控区,我们克隆了包含−1324 / -890的VIL2 −1541 / −706片段,并通过荧光素酶测定法在瞬时转染的细胞中研究了其转录调控特性。在EC109细胞中,发现VIL2 -1541 / -706具有启动子和增强子活性。我们还通过将VIL2 -1541 / -706的5'-或3'-缺失片段融合到荧光素酶报道基因上来定位转录调控区域。我们发现EC109细胞的VIL2 -1541 / -706内有3个正和1个负转录调控区。当这些区域分别位于没有启动子的萤光素酶基因的上游或位于指导萤光素酶基因的VIL2启动子或SV40启动子的上游时,只有VIL2 -1297 / -1186表现出显着的启动子和增强子活性,低于- 1541 / -706。此外,Sp1的瞬时表达增加了ezrin的表达和VIL2-12-1297 / -1186的转录激活。其他三个区域,尽管在缺失实验中表现出明显的正或负转录调控,但显示出较弱或不存在的调控。这些数据表明,VIL2启动子上游的一个以上区域参与了VIL2转录,而VIL2-12-1297 / -1186(可能是一个关键的转录调控区)与其他潜在的调控区共同调控了VIL2转录。

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  • 来源
    《Acta Biochimica et Biophysica Sinica》 |2011年第6期|p.455-464|共10页
  • 作者

    Jie Yu;

  • 作者单位

    , Peking University Shenzhen Hospital, @%@, Peking University, @%@, Shenzhen PKU-HKUST Medical Center, @%@;

    Fax: +@%@;

    E-mail:;

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