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ChEC-seq kinetics discriminates transcription factor binding sites by DNA sequence and shape in vivo

机译:ChEC-seq动力学通过DNA序列和体内形状区分转录因子结合位点

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Chromatin endogenous cleavage (ChEC) uses fusion of a protein of interest to micrococcal nuclease (MNase) to target calcium-dependent cleavage to specific genomic loci in vivo. Here we report the combination of ChEC with high-throughput sequencing (ChEC-seq) to map budding yeast transcription factor (TF) binding. Temporal analysis of ChEC-seq data reveals two classes of sites for TFs, one displaying rapid cleavage at sites with robust consensus motifs and the second showing slow cleavage at largely unique sites with low-scoring motifs. Sites with high-scoring motifs also display asymmetric cleavage, indicating that ChEC-seq provides information on the directionality of TF-DNA interactions. Strikingly, similar DNA shape patterns are observed regardless of motif strength, indicating that the kinetics of ChEC-seq discriminates DNA recognition through sequence and/or shape. We propose that time-resolved ChEC-seq detects both high-affinity interactions of TFs with consensus motifs and sites preferentially sampled by TFs during diffusion and sliding.
机译:染色质内源性切割(ChEC)使用目标蛋白与微球菌核酸酶(MNase)融合,将钙依赖性切割靶向体内的特定基因组位点。在这里,我们报道了ChEC与高通量测序(ChEC-seq)的组合,以绘制出芽酵母转录因子(TF)的结合图。 ChEC-seq数据的时间分析揭示了TF的两类位点,一类在具有稳固共有基序的位点上显示出快速切割,而第二类在具有低得分基序的很大程度上独特的位点上显示出缓慢的切割。具有高得分基序的位点也显示不对称切割,表明ChEC-seq提供了有关TF-DNA相互作用方向的信息。引人注目的是,无论基序强度如何,都观察到相似的DNA形状模式,这表明ChEC-seq的动力学通过序列和/或形状来区分DNA识别。我们提出时间分辨的ChEC-seq检测具有共有基序的TF的高亲和力相互作用以及在扩散和滑动过程中TF优先采样的位点。

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