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首页> 外文期刊>Korean Journal of Biological Sciences >Identification of Ku70/Ku80 as ADD1/SREBP1c Interacting Proteins
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Identification of Ku70/Ku80 as ADD1/SREBP1c Interacting Proteins

机译:Ku70 / Ku80作为ADD1 / SREBP1c相互作用蛋白的鉴定

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摘要

In vertebrates, multisubunit cofactors regulate gene expression through interacting with cell-type- and gene-specific DNA-binding proteins in a chromatin-selective manner. ADD1/SREBP1c regulates fatty acid metabolism and insulin-dependent gene expression through binding to SRE and E-box motif with dual DNA binding specificity. Although its transcriptional and post-translational regulation has been extensively studied, its regulation by interacting proteins is not well understood. To identify cellularproteins that associate with nuclear form of ADD1/SREBP1C, we employed the GST pull-down system with Hela cell nuclei extract. In this study, we demonstrated that Ku proteins interact specifically with ADD1/SREBP1 c protein. GST pull-down combined withpeptide sequencing analysis revealed that Ku80 binds to ADD1/SREBP1C in vitro. Additionally, western blot analysis showed that Ku70, a heterodimerizing partner of Ku80, also associates with ADD1/SREBP1c. Furthermore, co-transfection of Ku70/Ku80 with ADD1/SREBP1c enhanced the transcriptional activity of ADD1/SREBP1C. Taken together, these results suggest that the Ku proteins might be involved in the lipogenic and/or adipogenic gene expression through interacting with ADD1/SREBP1c.
机译:在脊椎动物中,多亚基辅因子通过与细胞类型和基因特异性DNA结合蛋白以染色质选择性方式相互作用来调节基因表达。 ADD1 / SREBP1c通过与SRE和E-box基序结合并具有双重DNA结合特异性来调节脂肪酸代谢和胰岛素依赖性基因的表达。尽管已对其转录和翻译后调控进行了广泛研究,但对与蛋白质相互作用的调控尚不清楚。为了鉴定与ADD1 / SREBP1C核形式相关的细胞蛋白,我们将GST下拉系统与Hela细胞核提取物一起使用。在这项研究中,我们证明了Ku蛋白与ADD1 / SREBP1 c蛋白特异性相互作用。 GST下拉结合肽测序分析表明,Ku80在体外与ADD1 / SREBP1C结合。此外,蛋白质印迹分析表明,Ku80的异二聚体伴侣Ku70也与ADD1 / SREBP1c缔合。此外,Ku70 / Ku80与ADD1 / SREBP1c的共转染增强了ADD1 / SREBP1C的转录活性。两者合计,这些结果表明,Ku蛋白可能通过与ADD1 / SREBP1c相互作用而参与脂肪形成和/或脂肪形成基因的表达。

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