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Bi-functional cross-linking reagents efficiently capture protein-DNA complexes in Drosophila embryos

机译:双功能交联剂可有效捕获果蝇胚胎中的蛋白质-DNA复合物

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摘要

Chromatin immunoprecipitation (ChIP) is widely used for mapping DNA-protein interactions across eukaryotic genomes in cells, tissues or even whole organisms. Critical to this procedure is the efficient cross-linking of chromatin-associated proteins to DNA sequences that are in close proximity. Since the mid-nineties formaldehyde fixation has been the method of choice. However, some protein-DNA complexes cannot be successfully captured for ChIP using formaldehyde. One such formaldehyde refractory complex is the developmentally regulated insulator factor, Elba. Here we describe a new embryo fixation procedure using the bi-functional cross-linking reagents DSG (disuccinimidyl glutarate) and DSP (dithiobis[succinimidyl propionate). We show that unlike standard formaldehyde fixation protocols, it is possible to capture Elba association with insulator elements in 2–5 h embryos using this new cross-linking procedure. We show that this new cross-linking procedure can also be applied to localize nuclear proteins that are amenable to ChIP using standard formaldehyde cross-linking protocols, and that in the cases tested the enrichment was generally superior to that achieved using formaldehyde cross-linking.
机译:染色质免疫沉淀(ChIP)被广泛用于绘制细胞,组织甚至整个生物体中真核基因组之间DNA-蛋白质相互作用的图谱。该过程的关键是染色质相关蛋白与紧密相邻的DNA序列的有效交联。自九十年代中期以来,甲醛固定一直是选择的方法。但是,某些蛋白-DNA复合物无法使用甲醛成功地捕获ChIP。一种这样的甲醛耐火复合物是受发育调节的绝缘子因子Elba。在这里,我们描述了一种新的胚胎固定程序,该程序使用了双功能交联试剂DSG(谷氨酸二琥珀酰亚胺基)和DSP(二硫代双琥珀酰亚胺丙酸酯)。我们证明,与标准甲醛固定方案不同,使用这种新的交联程序可以捕获2-5小时胚胎中Elba与绝缘子元素的缔合。我们表明,这种新的交联程序还可用于使用标准甲醛交联方案来定位适合ChIP的核蛋白,并且在测试的情况下,其富集通常优于使用甲醛交联所实现的。

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