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条件性沉默:HMRE交配型沉默子对酵母HSP82热休克基因施加快速可逆的位置效应。

Conditional silencing: the HMRE mating-type silencer exerts a rapidly reversible position effect on the yeast HSP82 heat shock gene.

作者信息

Lee S, Gross D S

机构信息

Department of Biochemistry and Molecular Biology, Louisiana State University Medical Center, Shreveport 71130.

出版信息

Mol Cell Biol. 1993 Feb;13(2):727-38. doi: 10.1128/mcb.13.2.727-738.1993.

Abstract

The HMRE silencer of Saccharomyces cerevisiae has been previously shown to transcriptionally repress class II and class III genes integrated within the HMR silent mating-type locus up to 2.6 kb away. Here we study the ability of this element to repress at an ectopic position, independent of sequences normally associated with it. When integrated 750 bp upstream of the HSP82 heat shock gene, the silencer represses basal-level transcription approximately 5-fold but has no effect on chemical- or heat-shock-induced expression. Such conditional silencing is also seen when the HMRE/HSP82 allele is carried on a centromeric episome or when the entire HMRa domain is transplaced 2.7 kb upstream of HSP82. Notably, the a1 promoter within the immigrant HMRa locus remains fully repressed at the same time HSP82 is derepressed. The position effect mediated by the E silencer is absolutely dependent on the presence of a functional SIR4 gene product, is lost within 1 min following stress induction, and is fully reestablished within 15 min following a return to nonstressful conditions. Similar kinetics of reestablishment are seen in HMRE/HSP82 and HMRa/HSP82 strains, indicating that complete repression can be mediated over thousands of base pairs within minutes. DNase I chromatin mapping reveals that the ABF1, RAP1, and autonomously replicating sequence factor binding sites within the silencer are constitutively occupied in chromatin, unaltered by heat shock or the presence of SIR4. Similarly, the heat shock factor binding site upstream of HSP82 remains occupied under such conditions, suggesting concurrent occupancy of silencer and activator binding sites. Our results are consistent with a model in which silencing at the HMRE/HSP82 allele is mediated by direct or indirect contacts between the silencer protein complex and heat shock factor.

摘要

酿酒酵母的HMRE沉默子先前已被证明可转录抑制整合在HMR沉默交配型基因座内、距离达2.6 kb远的II类和III类基因。在此,我们研究该元件在异位位置进行抑制的能力,这与通常与之相关的序列无关。当整合到HSP82热休克基因上游750 bp处时,该沉默子可将基础水平转录抑制约5倍,但对化学或热休克诱导的表达无影响。当HMRE/HSP82等位基因携带在着丝粒附加体上或整个HMRa结构域被转移到HSP82上游2.7 kb处时,也能观察到这种条件性沉默。值得注意的是,在HSP82去抑制的同时,移入的HMRa基因座内的a1启动子仍被完全抑制。由E沉默子介导的位置效应绝对依赖于功能性SIR4基因产物的存在,在应激诱导后1分钟内消失,并在恢复到非应激条件后15分钟内完全重新建立。在HMRE/HSP82和HMRa/HSP82菌株中观察到类似的重新建立动力学,表明在几分钟内可介导数千个碱基对的完全抑制。DNase I染色质图谱显示,沉默子内的ABF1、RAP1和自主复制序列因子结合位点在染色质中持续被占据,不受热休克或SIR4存在的影响。同样,在这种条件下,HSP82上游的热休克因子结合位点仍被占据,表明沉默子和激活剂结合位点同时被占据。我们的结果与一个模型一致,即HMRE/HSP82等位基因处的沉默是由沉默子蛋白复合物与热休克因子之间的直接或间接接触介导的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f4f7/358955/625b64c24e6a/molcellb00014-0013-a.jpg

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