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本文引用的文献

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Histone H3K4 methylation regulates deactivation of the spindle assembly checkpoint through direct binding of Mad2.组蛋白H3K4甲基化通过Mad2的直接结合来调节纺锤体组装检查点的失活。
Genes Dev. 2016 May 15;30(10):1187-97. doi: 10.1101/gad.278887.116. Epub 2016 May 19.
2
PAT-seq: a method to study the integration of 3'-UTR dynamics with gene expression in the eukaryotic transcriptome.PAT-seq:一种研究真核转录组中3'-UTR动态与基因表达整合的方法。
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EdU Incorporation for FACS and Microscopy Analysis of DNA Replication in Budding Yeast.用于芽殖酵母DNA复制的流式细胞术和显微镜分析的EdU掺入法
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Histone core modifications regulating nucleosome structure and dynamics.组蛋白核心修饰调节核小体结构和动力学。
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Cell cycle population effects in perturbation studies.扰动研究中的细胞周期群体效应。
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6
Role of histone modifications and early termination in pervasive transcription and antisense-mediated gene silencing in yeast.组蛋白修饰和早期终止在酵母中普遍转录和反义介导的基因沉默中的作用。
Nucleic Acids Res. 2014 Apr;42(7):4348-62. doi: 10.1093/nar/gku100. Epub 2014 Feb 4.
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Control of cell cycle transcription during G1 and S phases.控制 G1 期和 S 期细胞周期转录。
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8
H3K4 methyltransferase Set1 is involved in maintenance of ergosterol homeostasis and resistance to Brefeldin A.H3K4 甲基转移酶 Set1 参与维持麦角固醇稳态和对布雷菲德菌素 A 的抗性。
Proc Natl Acad Sci U S A. 2013 Mar 12;110(11):E1016-25. doi: 10.1073/pnas.1215768110. Epub 2013 Feb 4.
9
Two distinct repressive mechanisms for histone 3 lysine 4 methylation through promoting 3'-end antisense transcription.通过促进 3'-端反义转录,两种截然不同的组蛋白 3 赖氨酸 4 甲基化抑制机制。
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10
Systematic dissection of roles for chromatin regulators in a yeast stress response.系统剖析染色质调控因子在酵母应激反应中的作用。
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细胞周期进程与有丝分裂纺锤体组装的协调涉及Set1/COMPASS介导的组蛋白H3赖氨酸4甲基化。

Coordination of Cell Cycle Progression and Mitotic Spindle Assembly Involves Histone H3 Lysine 4 Methylation by Set1/COMPASS.

作者信息

Beilharz Traude H, Harrison Paul F, Miles Douglas Maya, See Michael Ming, Le Uyen Minh Merry, Kalanon Ming, Curtis Melissa Jane, Hasan Qambar, Saksouk Julie, Margaritis Thanasis, Holstege Frank, Geli Vincent, Dichtl Bernhard

机构信息

Development and Stem Cells Program, Monash Biomedicine Discovery Institute and Department of Biochemistry and Molecular Biology, Monash University, Melbourne, Victoria 3800, Australia.

Monash Bioinformatics Platform, Monash University, Melbourne, Victoria 3800, Australia.

出版信息

Genetics. 2017 Jan;205(1):185-199. doi: 10.1534/genetics.116.194852. Epub 2016 Nov 14.

DOI:10.1534/genetics.116.194852
PMID:28049706
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5223502/
Abstract

Methylation of histone H3 lysine 4 (H3K4) by Set1 complex/COMPASS is a hallmark of eukaryotic chromatin, but it remains poorly understood how this post-translational modification contributes to the regulation of biological processes like the cell cycle. Here, we report a H3K4 methylation-dependent pathway in Saccharomyces cerevisiae that governs toxicity toward benomyl, a microtubule destabilizing drug. Benomyl-sensitive growth of wild-type cells required mono- and dimethylation of H3K4 and Pho23, a PHD-containing subunit of the Rpd3L complex. Δset1 and Δpho23 deletions suppressed defects associated with ipl1-2 aurora kinase mutant, an integral component of the spindle assembly checkpoint during mitosis. Benomyl resistance of Δset1 strains was accompanied by deregulation of all four tubulin genes and the phenotype was suppressed by tub2-423 and Δtub3 mutations, establishing a genetic link between H3K4 methylation and microtubule function. Most interestingly, sine wave fitting and clustering of transcript abundance time series in synchronized cells revealed a requirement for Set1 for proper cell-cycle-dependent gene expression and Δset1 cells displayed delayed entry into S phase. Disruption of G1/S regulation in Δmbp1 and Δswi4 transcription factor mutants duplicated both benomyl resistance and suppression of ipl1-2 as was observed with Δset1 Taken together our results support a role for H3K4 methylation in the coordination of cell-cycle progression and proper assembly of the mitotic spindle during mitosis.

摘要

Set1复合物/COMPASS对组蛋白H3赖氨酸4(H3K4)的甲基化是真核染色质的一个标志,但这种翻译后修饰如何促进细胞周期等生物过程的调控仍知之甚少。在此,我们报道了酿酒酵母中一条依赖H3K4甲基化的途径,该途径控制对苯菌灵(一种微管去稳定药物)的毒性。野生型细胞对苯菌灵敏感的生长需要H3K4以及Rpd3L复合物中含PHD的亚基Pho23的单甲基化和二甲基化。缺失Set1和Pho23可抑制与Ipl1-2极光激酶突变体相关的缺陷,Ipl1-2是有丝分裂期间纺锤体组装检查点的一个重要组成部分。缺失Set1的菌株对苯菌灵的抗性伴随着所有四个微管蛋白基因的失调,并且tub2-423和缺失tub3的突变抑制了该表型,从而在H3K4甲基化与微管功能之间建立了遗传联系。最有趣的是,对同步化细胞中转录本丰度时间序列进行正弦波拟合和聚类分析发现,Set1对细胞周期依赖性基因的正常表达是必需的,缺失Set1的细胞进入S期延迟。在缺失Mbp1和缺失Swi4转录因子突变体中G1/S调控的破坏,使对苯菌灵的抗性以及对Ipl1-2的抑制现象都与缺失Set1时观察到的情况相同。综合我们的结果支持H3K4甲基化在有丝分裂期间协调细胞周期进程和有丝分裂纺锤体的正确组装中发挥作用。