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秀丽隐杆线虫的HIM-17将染色质修饰与减数分裂重组起始能力联系起来。

C. elegans HIM-17 links chromatin modification and competence for initiation of meiotic recombination.

作者信息

Reddy Kirthi C, Villeneuve Anne M

机构信息

Department of Developmental Biology, Stanford University School of Medicine, Stanford, CA 94305, USA.

出版信息

Cell. 2004 Aug 20;118(4):439-52. doi: 10.1016/j.cell.2004.07.026.

Abstract

Initiation of meiotic recombination by double-strand breaks (DSBs) must occur in a controlled fashion to avoid jeopardizing genome integrity. Here, we identify chromatin-associated protein HIM-17 as a link between chromatin state and DSB formation during C. elegans meiosis. Dependencies of several meiotic prophase events on HIM-17 parallel those seen for DSB-generating enzyme SPO-11: HIM-17 is essential for DSB formation but dispensable for homolog synapsis. Crossovers and chiasmata are eliminated in him-17 null mutants but are restored by artificially induced DSBs, indicating that all components required to convert DSBs into chiasmata are present. Unlike SPO-11, HIM-17 is also required for proper accumulation of histone H3 methylation at lysine 9 on meiotic prophase chromosomes. HIM-17 shares structural features with three proteins that interact genetically with LIN-35/Rb, a known component of chromatin-modifying complexes. Furthermore, DSB levels and incidence of chiasmata can be modulated by loss of LIN-35/Rb. These and other data suggest that chromatin state governs the timing of DSB competence.

摘要

双链断裂(DSB)引发的减数分裂重组必须以可控方式发生,以避免危及基因组完整性。在此,我们鉴定出与染色质相关的蛋白HIM-17是秀丽隐杆线虫减数分裂过程中染色质状态与DSB形成之间的联系。减数分裂前期的几个事件对HIM-17的依赖性与产生DSB的酶SPO-11的情况相似:HIM-17对DSB形成至关重要,但对同源染色体联会则可有可无。在him-17基因敲除突变体中交叉和交叉点被消除,但通过人工诱导的DSB可恢复,这表明将DSB转化为交叉点所需的所有成分都存在。与SPO-11不同,HIM-17对于减数分裂前期染色体赖氨酸9处组蛋白H3甲基化的正确积累也是必需的。HIM-17与三种与LIN-35/Rb(染色质修饰复合物的已知成分)发生遗传相互作用的蛋白具有结构特征。此外,LIN-35/Rb的缺失可调节DSB水平和交叉点发生率。这些以及其他数据表明染色质状态控制着DSB能力的时机。

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