首页> 外文OA文献 >Characterization of the human activator protein-2gamma (AP-2gamma) gene: control of expression by Sp1/Sp3 in breast tumour cells.
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Characterization of the human activator protein-2gamma (AP-2gamma) gene: control of expression by Sp1/Sp3 in breast tumour cells.

机译:人类激活蛋白2gamma(AP-2gamma)基因的特征:通过Sp1 / Sp3在乳腺肿瘤细胞中的表达控制。

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摘要

The activator protein-2 (AP-2) family of DNA-binding transcription factors are developmentally regulated and also play a role in human neoplasia. In particular, the AP-2gamma protein has been shown to be overexpressed in a high percentage of breast tumours. In the present study, we report the complete sequence determination of the human TFAP2C gene encoding the AP-2gamma transcription factor plus the mapping of the transcription start site used in breast tumour-derived cells. The 5'-end of the gene lies within a CpG island and transcription is initiated at a single site within a classical initiator motif. We have gone on to investigate why some breast tumour-derived cell lines readily express AP-2gamma, whereas others do not, and show that the proximal promoter (+191 to -312) is differentially active in the two cell phenotypes. DNase footprinting led to the identification of three Sp1/Sp3-binding sites within this region, two of which are absolutely required both for promoter function and cell-type-specific activity. By Western blotting a panel of expressing and non-expressing breast tumour lines we show that the latter have higher levels of Sp3. Furthermore, increasing Sp3 levels in AP-2gamma-expressing cells led to the repression of AP-2gamma promoter activity, particularly when Sp3 inhibitory function was maximized through sumoylation. We propose that differences in the level and activity of Sp3 between breast tumour lines can determine the expression level of their AP-2gamma gene.
机译:DNA结合转录因子的激活蛋白2(AP-2)家族受到发育调节,并在人类肿瘤形成中发挥作用。特别是,AP-2γ蛋白已被证明在高百分比的乳腺肿瘤中过表达。在本研究中,我们报告了编码AP-2gamma转录因子的人TFAP2C基因的完整序列测定,以及在乳腺肿瘤衍生细胞中使用的转录起始位点的定位。基因的5'端位于CpG岛内,转录在经典启动子基序内的单个位点启动。我们继续研究了为什么一些乳腺肿瘤衍生的细胞系很容易表达AP-2γ,而另一些则不表达,并且表明近端启动子(+191至-312)在两种细胞表型中具有差异性活性。 DNase足迹导致鉴定出该区域内的三个Sp1 / Sp3结合位点,其中两个绝对是启动子功能和细胞类型特异性活性所必需的。通过蛋白质印迹,一组表达和未表达的乳腺肿瘤系我们显示出后者具有较高水平的Sp3。此外,在表达AP-2γ的细胞中Sp3水平的升高导致AP-2γ启动子活性的抑制,特别是当通过sumoylation最大化Sp3抑制功能时。我们提出,乳腺肿瘤细胞系之间Sp3水平和活性的差异可以决定其AP-2gamma基因的表达水平。

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