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Loss of H2A.Z Is Not Sufficient to Determine Transcriptional Activity of Snf2-Related CBP Activator Protein or p400 Complexes

机译:H2A.Z的丢失不足以确定Snf2相关的CBP激活蛋白或p400复合物的转录活性。

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摘要

The p400 and SRCAP (Snf2-related CBP activator protein) complexes remodel chromatin by catalyzing deposition of histone H2A.Z into nucleosomes. This remodeling activity has been proposed as a basis for regulation of transcription by these complexes. Transcript levels of p21 or Sp1 mRNAs after knockdown of p400 or SRCAP reveals that each regulates transcription of these promoters differently. In this study, we asked whether deposition of H2A.Z within specific nucleosomes by p400 or SRCAP dictates transcriptional activity. Our data indicates that nucleosome density at specific p21 or Sp1 promoter positions is not altered by the loss of either remodeling complex. However, knockdown of SRCAP or p400 reduces deposition of H2A.Z∼50% into all p21 and Sp1 promoter nucleosomes. Thus, H2A.Z deposition is not targeted to specific nucleosomes. These results indicate that the deposition of H2A.Z by the p400 or SRCAP complexes is not sufficient to determine how each regulates transcription. This conclusion is further supported by studies that demonstrate a SRCAPΔATP mutant unable to deposit H2A.Z has similar transcriptional activity as wild-type SRCAP.
机译:p400和SRCAP(与Snf2相关的CBP激活蛋白)复合物通过催化组蛋白H2A.Z沉积入核小体来重塑染色质。已经提出这种重塑活性作为这些复合物调节转录的基础。敲除p400或SRCAP后,p21或Sp1 mRNA的转录水平显示,每个调节这些启动子的转录方式不同。在这项研究中,我们询问是否通过p400或SRCAP在特定核小体中沉积H2A.Z决定了转录活性。我们的数据表明在特定的p21或Sp1启动子位置的核小体密度不会因任何一种重塑复合物的丢失而改变。但是,敲除SRCAP或p400可以减少H2A.Z〜50%沉积到所有p21和Sp1启动子核小体中。因此,H2A.Z沉积不针对特定的核小体。这些结果表明,p400或SRCAP复合物对H2A.Z的沉积不足以决定它们各自如何调控转录。该研究进一步证明了这一结论,该研究表明SRCAPΔATP突变体无法沉积H2A。Z具有与野生型SRCAP相似的转录活性。

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