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酵母核糖体RNA基因位点的转录:活性基因拷贝的分布及其侧翼调控序列的染色质结构

Transcription in the yeast rRNA gene locus: distribution of the active gene copies and chromatin structure of their flanking regulatory sequences.

作者信息

Dammann R, Lucchini R, Koller T, Sogo J M

机构信息

Institute of Cell Biology, Eidgenössiche Technische Hochschule-Hönggerberg, Zürich, Switzerland.

出版信息

Mol Cell Biol. 1995 Oct;15(10):5294-303. doi: 10.1128/MCB.15.10.5294.

DOI:10.1128/MCB.15.10.5294
PMID:7565678
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC230777/
Abstract

In growing yeast cells, about half of the 150 tandemly repeated rRNA genes are transcriptionally active and devoid of nucleosomes. By using the intercalating drug psoralen as a tool to mark accessible sites along chromatin DNA in vivo, we found that the active rRNA gene copies are rather randomly distributed along the ribosomal rRNA gene locus. Moreover, results from the analysis of a single, tagged transcription unit in the tandem array are not consistent with the presence of a specific subset of active genes that is stably maintained throughout cell divisions. In the rRNA intergenic spacers of yeast cells, an enhancer is located at the 3' end of each transcription unit, 2 kb upstream of the next promoter. Analysis of the chromatin structure along the tandem array revealed a structural link between transcription units and adjacent, 3' flanking enhancer sequences: each transcriptionally active gene is flanked by a nonnucleosomal enhancer, whereas inactive, nucleosome-packed gene copies are followed by enhancers regularly packaged in nucleosomes. From the fact that nucleosome-free enhancers were also detected in an RNA polymerase I mutant strain, we interpret these open chromatin structures as being the result of specific protein-DNA interactions that can occur before the onset of transcription. In contrast, in this mutant strain, all of the rRNA coding sequences are packaged in nucleosomal arrays. This finding indicates that the establishment of the open chromatin conformation on the activated gene copies requires elongating RNA polymerase I molecules advancing through the template.

摘要

在生长的酵母细胞中,150个串联重复的rRNA基因约有一半具有转录活性且不含核小体。通过使用嵌入药物补骨脂素作为标记体内染色质DNA上可及位点的工具,我们发现活性rRNA基因拷贝沿着核糖体rRNA基因位点相当随机地分布。此外,对串联阵列中单个标记转录单元的分析结果与在整个细胞分裂过程中稳定维持的特定活性基因子集的存在不一致。在酵母细胞的rRNA基因间隔区,一个增强子位于每个转录单元的3'端,即下一个启动子上游2 kb处。对串联阵列的染色质结构分析揭示了转录单元与相邻的3'侧翼增强子序列之间的结构联系:每个转录活性基因两侧都有一个无核小体的增强子,而无活性的、被核小体包裹的基因拷贝后面跟着规则地被核小体包裹的增强子。从在RNA聚合酶I突变株中也检测到无核小体增强子这一事实,我们将这些开放染色质结构解释为转录开始前可能发生的特定蛋白质-DNA相互作用的结果。相比之下,在该突变株中,所有rRNA编码序列都被包装在核小体阵列中。这一发现表明,在活化的基因拷贝上建立开放染色质构象需要延伸的RNA聚合酶I分子穿过模板。

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本文引用的文献

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