Dipartimento di Scienze Biomolecolari e Biotecnologie, Università degli Studi di Milano, Milano, Italy.
PLoS Genet. 2010 Aug 5;6(8):e1001047. doi: 10.1371/journal.pgen.1001047.
Saccharomyces cerevisiae Rad9 is required for an effective DNA damage response throughout the cell cycle. Assembly of Rad9 on chromatin after DNA damage is promoted by histone modifications that create docking sites for Rad9 recruitment, allowing checkpoint activation. Rad53 phosphorylation is also dependent upon BRCT-directed Rad9 oligomerization; however, the crosstalk between these molecular determinants and their functional significance are poorly understood. Here we report that, in the G1 and M phases of the cell cycle, both constitutive and DNA damage-dependent Rad9 chromatin association require its BRCT domains. In G1 cells, GST or FKBP dimerization motifs can substitute to the BRCT domains for Rad9 chromatin binding and checkpoint function. Conversely, forced Rad9 dimerization in M phase fails to promote its recruitment onto DNA, although it supports Rad9 checkpoint function. In fact, a parallel pathway, independent on histone modifications and governed by CDK1 activity, allows checkpoint activation in the absence of Rad9 chromatin binding. CDK1-dependent phosphorylation of Rad9 on Ser11 leads to specific interaction with Dpb11, allowing Rad53 activation and bypassing the requirement for the histone branch.
酿酒酵母 Rad9 在整个细胞周期中都需要有效的 DNA 损伤反应。DNA 损伤后,Rad9 在染色质上的组装是由组蛋白修饰促进的,这些修饰为 Rad9 的募集创造了对接位点,从而激活检查点。Rad53 的磷酸化也依赖于 BRCT 介导的 Rad9 寡聚化;然而,这些分子决定因素之间的串扰及其功能意义还知之甚少。在这里,我们报告在细胞周期的 G1 和 M 期,组成型和 DNA 损伤依赖性 Rad9 染色质关联都需要其 BRCT 结构域。在 G1 期细胞中,GST 或 FKBP 二聚化结构域可以替代 BRCT 结构域用于 Rad9 染色质结合和检查点功能。相反,在 M 期强制 Rad9 二聚化不能促进其在 DNA 上的募集,尽管它支持 Rad9 检查点功能。事实上,一个平行的途径,不依赖于组蛋白修饰,由 CDK1 活性控制,允许在没有 Rad9 染色质结合的情况下激活检查点。CDK1 依赖性 Rad9 Ser11 磷酸化导致与 Dpb11 的特异性相互作用,从而激活 Rad53 并绕过对组蛋白分支的需求。
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