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Brr6 plays a role in gene recruitment and transcriptional regulation at the nuclear envelope

机译:BRR6在核信封的基因招生和转录规则中起着作用

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Correlation between transcriptional regulation and positioning of genes at the nuclear envelope is well established in eukaryotes, but the mechanisms involved are not well understood. We show that brr6-1, a mutant of the essential yeast envelope transmembrane protein Brr6p, impairs normal positioning and expression of the PAB1 and FUR4-GAL1,10,7 loci. Similarly, expression of a dominant negative nucleoplasmic Brr6 fragment in wild-type cells reproduced many of the brr6-1 effects. Histone chromatin immunoprecipitation (ChIP) experiments showed decreased acetylation at the key histone H4K16 residue in the FUR4-GAL1,10,7 region in brr6-1. Importantly, blocking deacetylation significantly suppressed selected brr6-1 phenotypes. ChIPseq with FLAG-tagged Brr6 fragments showed enrichment at FUR4 and several other genes that showed striking changes in brr6-1 RNAseq data. These associations depended on a Brr6 putative zinc finger domain. Importantly, artificially tethering the GAL1 locus to the envelope suppressed the brr6-1 effects on GAL1 and FUR4 expression and increased H4K16 acetylation between GAL1 and FUR4 in the mutant. Together these results argue that Brr6 interacts with chromatin, helping to maintain normal chromatin architecture and transcriptional regulation of certain loci at the nuclear envelope.
机译:在真核生物中确定了核包封中基因的转录调节与基因定位的相关性,但涉及的机制并不熟知。我们表明,BRR6-1,必需酵母包络跨膜蛋白BRR6P的突变体,损害了PAB1和FUR4-GAL1,10,7基因座的正常定位和表达。类似地,在野生型细胞中的显性负硝基骨质BRR6片段的表达再现许多BRR6-1效应。组蛋白染色质免疫沉淀(芯片)实验表明在BRR6-1中Fur4-gall1,10,7区的关键组蛋白H4K16残基下降下降。重要的是,阻断脱乙酰化显着抑制了所选BRR6-1表型。 Chipseq与标志标记的BRR6片段显示呋喃4的富集和几种在BRR6-1 RNASEQ数据中显示出醒目的变化。这些关联取决于BRR6推定的锌指域。重要的是,在突变体中,人工地将Gal1轨迹抑制对盖子和Fur4表达的BRR6-1和Fur4表达的影响,并增加了Gal1和Fur4之间的H4K16乙酰化。这些结果共同认为,BRR6与染色质相互作用,有助于维持核信封在某些基因座的正常染色质架构和转录调节。

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