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细胞内 S 期检查点蛋白 Tof1 与解旋酶 Rrm3 和 F-box 蛋白 Dia2 合作,以维持酿酒酵母的基因组稳定性。

The intra-S phase checkpoint protein Tof1 collaborates with the helicase Rrm3 and the F-box protein Dia2 to maintain genome stability in Saccharomyces cerevisiae.

机构信息

Department of Biochemistry and Molecular Biology, Medical University of South Carolina, Charleston, South Carolina 29425, USA.

出版信息

J Biol Chem. 2011 Jan 28;286(4):2445-54. doi: 10.1074/jbc.M110.189456. Epub 2010 Nov 18.

Abstract

The intra-S phase checkpoint protein complex Tof1/Csm3 of Saccharomyces cerevisiae antagonizes Rrm3 helicase to modulate replication fork arrest not only at the replication termini of rDNA but also at strong nonhistone protein binding sites throughout the genome. We investigated whether these checkpoint proteins acted either antagonistically or synergistically with Rrm3 in mediating other important functions such as maintenance of genome stability. High retromobility of a normally quiescent retrovirus-like transposable element Ty1 of S. cerevisiae is a form of genome instability, because the transposition events induce mutations. We measured the transposition of Ty1 in various genetic backgrounds and discovered that Tof1 suppressed excessive retromobility in collaboration with either Rrm3 or the F-box protein Dia2. Although both Rrm3 and Dia2 are believed to facilitate fork movement, fork stalling at DNA-protein complexes did not appear to be a major contributor to enhancement of retromobility. Absence of the aforementioned proteins either individually or in pair-wise combinations caused karyotype changes as revealed by the altered migrations of the individual chromosomes in pulsed field gels. The mobility changes were RNase H-resistant and therefore, unlikely to have been caused by extensive R loop formation. These mutations also resulted in alterations of telomere lengths. However, the latter changes could not fully account for the magnitude of the observed karyotypic alterations. We conclude that unlike other checkpoint proteins that are known to be required for elevated retromobility, Tof1 suppressed high frequency retrotransposition and maintained karyotype stability in collaboration with the aforementioned proteins.

摘要

酿酒酵母细胞内 S 期检查点蛋白复合物 Tof1/Csm3 拮抗 Rrm3 解旋酶,不仅在 rDNA 的复制末端,而且在整个基因组中强非组蛋白结合位点调节复制叉停滞。我们研究了这些检查点蛋白是否在介导其他重要功能(如基因组稳定性的维持)中与 Rrm3 拮抗或协同作用。酿酒酵母中正常静止的逆转录病毒样可移动元件 Ty1 的高返座率是基因组不稳定性的一种形式,因为转座事件会引起突变。我们在各种遗传背景下测量 Ty1 的转座,并发现 Tof1 与 Rrm3 或 F-box 蛋白 Dia2 协同抑制过度返座。尽管 Rrm3 和 Dia2 都被认为有助于叉的移动,但叉在 DNA-蛋白质复合物处的停滞似乎不是增强返座率的主要原因。上述蛋白质的缺失无论是单独缺失还是两两缺失,都会导致染色体组型改变,这可以通过脉冲场凝胶中单个染色体的迁移变化来揭示。这些移动变化对 RNase H 具有抗性,因此不太可能是由广泛的 R 环形成引起的。这些突变还导致端粒长度的改变。然而,后者的变化不能完全解释观察到的染色体组型改变的幅度。我们得出的结论是,与已知需要提高返座率的其他检查点蛋白不同,Tof1 与上述蛋白协同抑制高频率的 retrotransposition 并维持染色体组型稳定性。

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