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Affinity selection of DNA-binding protein complexes using mRNA display

机译:使用mRNA展示亲和力选择DNA结合蛋白复合物

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Comprehensive analysis of DNA–protein interactions is important for mapping transcriptional regulatory networks on a genome-wide level. Here we present a new application of mRNA display for in vitro selection of DNA-binding protein heterodimeric complexes. Under improved selection conditions using a TPA-responsive element (TRE) as a bait DNA, known interactors c-fos and c-jun were simultaneously enriched about 100-fold from a model library (a 1:1:20 000 mixture of c-fos, c-jun and gst genes) after one round of selection. Furthermore, almost all kinds of the AP-1 family genes including c-jun, c-fos, junD, junB, atf2 and b-atf were successfully selected from an mRNA display library constructed from a mouse brain poly A+ RNA after six rounds of selection. These results indicate that the mRNA display selection system can identify a variety of DNA-binding protein complexes in a single experiment. Since almost all transcription factors form heterooligomeric complexes to bind with their target DNA, thismethod should be most useful to search for DNA-binding transcription factor complexes.
机译:DNA-蛋白质相互作用的全面分析对于在全基因组水平上绘制转录调控网络至关重要。在这里,我们介绍了mRNA展示的新应用,用于体外选择DNA结合蛋白异二聚体复合物。在使用TPA响应元件(TRE)作为诱饵DNA的改良选择条件下,已知的相互作用因子c-fos和c-jun同时从模型库中富集了约100倍(c-fos的1:1:20000混合物) fos,c-jun和gst基因)。此外,经过六轮筛选后,从小鼠大脑poly A + RNA构建的mRNA展示文库中成功选择了几乎所有种类的AP-1家族基因,包括c-jun,c-fos,junD,junB,atf2和b-atf。选择。这些结果表明,mRNA展示选择系统可以在单个实验中鉴定多种DNA结合蛋白复合物。由于几乎所有转录因子均形成杂聚体复合物以与其靶DNA结合,因此该方法对于搜索与DNA结合的转录因子复合物最为有用。

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