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Analysis of transcription factor interactions in osteoblasts using competitive chromatin immunoprecipitation

机译:竞争性染色质免疫沉淀法分析成骨细胞中的转录因子相互作用

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摘要

Chromatin immunoprecipitation (ChIP) is a widely used technique for quantifying proteinDNA interactions in living cells. This method commonly uses fixed (crosslinked) chromatin that is fragmented by sonication (X-ChIP). We developed a simple new ChIP procedure for the immunoprecipitation of sonicated chromatin isolated from osteoblasts in the absence of crosslinking (N-ChIP). The use of noncrosslinked chromatin allowed development of a new modification of the ChIP assay: the combination of N-ChIP and competition with double-stranded oligonucleotides containing specific binding sites for individual transcription factors (Competitive N-ChIP). Using this approach, we were able to discriminate between individual binding sites for the Runx2 transcription factor in the osteocalcin and bone sialoprotein genes that cannot be resolved by traditional X-ChIP. N-ChIP assays were also able to detect several other types of chromatin interactions including those with Dlx homeodomain factors and nuclear proteins such as Sin3a that lack an intrinsic DNA-binding motif and, therefore, bind to chromatin via interactions with other proteins.
机译:染色质免疫沉淀(ChIP)是一种广泛用于定量活细胞中蛋白质DNA相互作用的技术。此方法通常使用固定的(交联的)染色质,该染色质通过超声(X-ChIP)进行片段化。我们开发了一种简单的新ChIP程序,用于在不存在交联(N-ChIP)的情况下对从成骨细胞中分离的超声染色质进行免疫沉淀。非交联的染色质的使用允许开发一种新的ChIP检测方法:N-ChIP结合并与含有特定转录因子结合位点的双链寡核苷酸竞争(竞争性N-ChIP)。使用这种方法,我们能够区分骨钙蛋白中Runx2转录因子的单个结合位点和传统X-ChIP无法解决的骨唾液蛋白基因。 N-ChIP分析还能够检测几种其他类型的染色质相互作用,包括与Dlx同源域因子和核蛋白(例如Sin3a)的相互作用,这些蛋白缺乏固有的DNA结合基序,因此通过与其他蛋白的相互作用与染色质结合。

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