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TIF1在四膜虫的二倍体微核和无丝分裂多倍体大核中激活S期内检查点反应。

TIF1 activates the intra-S-phase checkpoint response in the diploid micronucleus and amitotic polyploid macronucleus of Tetrahymena.

作者信息

Yakisich J Sebastian, Sandoval Pamela Y, Morrison Tara L, Kapler Geoffrey M

机构信息

Department of Molecular and Cellular Medicine, Texas A&M Health Science Center, College Station, TX 77843-1114, USA.

出版信息

Mol Biol Cell. 2006 Dec;17(12):5185-97. doi: 10.1091/mbc.e06-05-0469. Epub 2006 Sep 27.

Abstract

The ribosomal DNA origin binding protein Tif1p regulates the timing of rDNA replication and is required globally for proper S-phase progression and division of the Tetrahymena thermophila macronucleus. Here, we show that Tif1p safeguards chromosomes from DNA damage in the mitotic micronucleus and amitotic macronucleus. TIF1p localization is dynamically regulated as it moves into the micro- and macronucleus during the respective S phases. TIF1 disruption mutants are hypersensitive to hydroxyurea and methylmethanesulfonate, inducers of DNA damage and intra-S-phase checkpoint arrest in all examined eukaryotes. TIF1 mutants incur double-strand breaks in the absence of exogenous genotoxic stress, destabilizing all five micronuclear chromosomes. Wild-type Tetrahymena elicits an intra-S-phase checkpoint response that is induced by hydroxyurea and suppressed by caffeine, an inhibitor of the apical checkpoint kinase ATR/MEC1. In contrast, hydroxyurea-challenged TIF1 mutants fail to arrest in S phase or exhibit caffeine-sensitive Rad51 overexpression, indicating the involvement of TIF1 in checkpoint activation. Although aberrant micro- and macronuclear division occurs in TIF1 mutants and caffeine-treated wild-type cells, TIF1p bears no similarity to ATR or its substrates. We propose that TIF1 and ATR function in the same epistatic pathway to regulate checkpoint responses in the diploid mitotic micronucleus and polyploid amitotic macronucleus.

摘要

核糖体DNA起始结合蛋白Tif1p调节rDNA复制的时间,并且对于嗜热四膜虫大核正常的S期进程和分裂全局都是必需的。在此,我们表明Tif1p在有丝分裂的小核和无丝分裂的大核中保护染色体免受DNA损伤。TIF1p的定位是动态调节的,因为它在各自的S期进入小核和大核。TIF1破坏突变体对羟基脲和甲磺酸甲酯超敏感,这两种物质是所有被检测真核生物中DNA损伤和S期内检查点停滞的诱导剂。TIF1突变体在没有外源性基因毒性应激的情况下会产生双链断裂,使所有五条小核染色体不稳定。野生型嗜热四膜虫引发一种S期内检查点反应,该反应由羟基脲诱导并被咖啡因抑制,咖啡因是顶端检查点激酶ATR/MEC1的抑制剂。相比之下,受到羟基脲挑战 的TIF1突变体无法在S期停滞或表现出对咖啡因敏感的Rad51过表达,这表明TIF1参与检查点激活。虽然在TIF1突变体和用咖啡因处理的野生型细胞中会发生异常的小核和大核分裂,但TIF1p与ATR或其底物没有相似性。我们提出TIF1和ATR在同一条上位途径中发挥作用,以调节二倍体有丝分裂小核和多倍体无丝分裂大核中的检查点反应。

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