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首页> 外文期刊>Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses >De novo telomere formation is suppressed by the Mec1-dependent inhibition of Cdc13 accumulation at DNA breaks.

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De novo telomere formation is suppressed by the Mec1-dependent inhibition of Cdc13 accumulation at DNA breaks.

机译：从头端粒的形成受到DNA断裂处Cdc13积累的Mec1依赖性抑制的抑制。

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DNA double-strand breaks (DSBs) are a threat to cell survival and genome integrity. In addition to canonical DNA repair systems, DSBs can be converted to telomeres by telomerase. This process, herein termed telomere healing, endangers genome stability, since it usually results in chromosome arm loss. Therefore, cells possess mechanisms that prevent the untimely action of telomerase on DSBs. Here we report that Mec1, the ATR ortholog, couples the detection of DNA ends with the inhibition of telomerase. Mec1 inhibits telomere healing by phosphorylating Cdc13 on its S306 residue, a phosphorylation event that suppresses Cdc13 accumulation at DSBs. Conversely, telomere addition at accidental breaks is promoted by Pph3, the yeast protein phosphatase 4 (PP4). Pph3 is itself modulated by Rrd1, an activator of PP2A family phosphatases. Rrd1 and Pph3 oppose Cdc13 S306 phosphorylation and are necessary for the efficient accumulation of Cdc13 at DNA breaks. These studies therefore identify a mechanism by which the ATR family of kinases enforces genome integrity, and a process that underscores the contribution of Cdc13 to the fate of DNA ends.

机译：DNA双链断裂（DSB）对细胞存活和基因组完整性构成威胁。除经典的DNA修复系统外，DSB还可通过端粒酶转化为端粒。该过程在本文中被称为端粒修复，危及基因组稳定性，因为它通常会导致染色体臂丢失。因此，细胞具有阻止端粒酶对DSB的不合时宜的作用的机制。在这里，我们报告说Mec1，ATR直系同源物，结合了DNA末端的检测与端粒酶的抑制作用。 Mec1通过在其S306残基上磷酸化Cdc13抑制端粒愈合，磷酸化事件抑制了Cdc13在DSB处的积累。相反，意外断裂时端粒的添加由酵母蛋白磷酸酶4（PP4）Pph3促进。 Pph3本身受PP2A家族磷酸酶的激活剂Rrd1调控。 Rrd1和Pph3反对Cdc13 S306磷酸化，并且是在DNA断裂处有效积累Cdc13所必需的。因此，这些研究确定了ATR激酶家族增强基因组完整性的机制，以及强调Cdc13对DNA命运的贡献的过程。

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《Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses》 |2010年第5期|共14页
作者
Zhang W; Durocher D;
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正文语种 eng
中图分类医学遗传学;
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1. De novo telomere formation is suppressed by the Mec1-dependent inhibition of Cdc13 accumulation at DNA breaks. [J] . Zhang W, Durocher D Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses . 2010,第5期

机译：从头端粒的形成受到DNA断裂处Cdc13积累的Mec1依赖性抑制的抑制。
2. Alkylation DNA damage in combination with PARP inhibition results in formation of S-phase-dependent double-strand breaks. [J] . Heacock ML, Stefanick DF, Horton JK, DNA repair . 2010,第8期

机译：烷基化DNA损伤与PARP抑制作用相结合会导致形成S相依赖的双链断裂。
3. Defective Resection at DNA Double-Strand Breaks Leads to De Novo Telomere Formation and Enhances Gene Targeting [J] . Woo-Hyun Chung, Zhu Zhu, Alma Papusha, PLoS Genetics . 2010,第5期

机译：DNA双链断裂处的缺陷切除会导致 De Novo 端粒形成并增强基因靶向
4. Formation of seqence-specific telomeric DNA loops via a direct effects of psoralen-photosensitization on telomeres [C] . Cao En-Hua, Chen Ai, Sun, Conference on Biomedical Photonics and Optoelectronic Imaging 8-10 November 2000 Beijing, China . 2000

机译：通过补骨脂素光敏作用对端粒的直接影响形成序列特异性端粒DNA环
5. Limiting the DNA damage checkpoint response at telomeres and DNA double-strand breaks. [D] . Downey, Michael Sean. 2008

机译：限制端粒和DNA双链断裂处的DNA损伤检查点反应。
6. De novo telomere formation is suppressed by the Mec1-dependent inhibition of Cdc13 accumulation at DNA breaks [O] . Wei Zhang, Daniel Durocher 2010

机译：从头端粒形成受到DNA断裂时Mec1依赖性Cdc13积累抑制的抑制
7. De novo telomere formation is suppressed by the Mec1-dependent inhibition of Cdc13 accumulation at DNA breaks [O] . Zhang, Wei, Durocher, Daniel 2010

机译：从头端粒形成受到DNA断裂时Mec1依赖性Cdc13积累抑制的抑制

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