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Mapping of the nuclear matrix-bound chromatin hubs by a new M3C experimental procedure.

机译:通过新的M3C实验程序绘制核基质结合的染色质集线器的图谱。

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We have developed an experimental procedure to analyze the spatial proximity of nuclear matrix-bound DNA fragments. This protocol, referred to as Matrix 3C (M3C), includes a high salt extraction of nuclei, the removal of distal parts of unfolded DNA loops using restriction enzyme treatment, ligation of the nuclear matrix-bound DNA fragments and a subsequent analysis of ligation frequencies. Using the M3C procedure, we have demonstrated that CpG islands of at least three housekeeping genes that surround the chicken -globin gene domain are assembled into a complex (presumably, a transcription factory) that is stabilized by the nuclear matrix in both erythroid and non-erythroid cells. In erythroid cells, the regulatory elements of the -globin genes are attracted to this complex to form a new assembly: an active chromatin hub that is linked to the pre-existing transcription factory. The erythroid-specific part of the assembly is removed by high salt extraction. Based on these observations, we propose that mixed transcription factories that mediate the transcription of both housekeeping and tissue-specific genes are composed of a permanent compartment containing integrated into the nuclear matrix promoters of housekeeping genes and a 'guest' compartment where promoters and regulatory elements of tissue-specific genes can be temporarily recruited.
机译:我们已经开发了一种实验程序来分析核基质结合的DNA片段的空间接近性。该协议称为Matrix 3C(M3C),包括高盐提取核,使用限制性内切酶处理去除未折叠的DNA环的远端部分,连接核基质结合的DNA片段并随后分析连接频率。使用M3C程序,我们已经证明,围绕鸡-珠蛋白基因域的至少三个管家基因的CpG岛被组装成复合物(大概是转录工厂),该复合物被红系和非红系中的核基质所稳定。红系细胞。在红系细胞中,-珠蛋白基因的调控元件被这种复合物吸引而形成一个新的装配体:一个活跃的染色质集线器,该染色质集线器与已有的转录工厂相连。组件的类红细胞特定部分通过高盐萃取去除。基于这些观察结果,我们建议介导管家基因和组织特异性基因转录的混合转录工厂由包含整合到管家基因核基质启动子中的永久区室和其中启动子和调控元件的“来宾”区室组成组织特异性基因可以暂时募集。

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