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Dif1通过介导R2亚基的核输入来控制核糖核苷酸还原酶的亚细胞定位。

Dif1 controls subcellular localization of ribonucleotide reductase by mediating nuclear import of the R2 subunit.

作者信息

Wu Xiaorong, Huang Mingxia

机构信息

Department of Biochemistry and Molecular Genetics, University of Colorado School of Medicine, Aurora, Colorado 80045, USA.

出版信息

Mol Cell Biol. 2008 Dec;28(23):7156-67. doi: 10.1128/MCB.01388-08. Epub 2008 Oct 6.

Abstract

Fidelity in DNA replication and repair requires adequate and balanced deoxyribonucleotide pools that are maintained primarily by regulation of ribonucleotide reductase (RNR). RNR is controlled via transcription, protein inhibitor association, and subcellular localization of its two subunits, R1 and R2. Saccharomyces cerevisiae Sml1 binds R1 and inhibits its activity, while Schizosaccharomyces pombe Spd1 impedes RNR holoenzyme formation by sequestering R2 in the nucleus away from the cytoplasmic R1. Here we report the identification and characterization of S. cerevisiae Dif1, a regulator of R2 nuclear localization and member of a new family of proteins sharing separate homologous domains with Spd1 and Sml1. Dif1 is localized in the cytoplasm and acts in a pathway different from the nuclear R2-anchoring protein Wtm1. Like Sml1 and Spd1, Dif1 is phosphorylated and degraded in cells encountering DNA damage, thereby relieving inhibition of RNR. A shared domain between Sml1 and Dif1 controls checkpoint kinase-mediated phosphorylation and degradation of the two proteins. Abolishing Dif1 phosphorylation stabilizes the protein and delays damage-induced nucleus-to-cytoplasm redistribution of R2. This study suggests that Dif1 is required for nuclear import of the R2 subunit and plays an essential role in regulating the dynamic RNR subcellular localization.

摘要

DNA复制和修复的保真度需要足够且平衡的脱氧核糖核苷酸库,这主要通过调节核糖核苷酸还原酶(RNR)来维持。RNR通过转录、蛋白质抑制剂结合及其两个亚基R1和R2的亚细胞定位来控制。酿酒酵母Sml1结合R1并抑制其活性,而裂殖酵母Spd1通过将R2隔离在细胞核中使其远离细胞质中的R1来阻碍RNR全酶的形成。在这里,我们报告了酿酒酵母Dif1的鉴定和特征,它是R2核定位的调节剂,也是一个新的蛋白质家族的成员,该家族与Spd1和Sml1共享不同的同源结构域。Dif1定位于细胞质中,其作用途径不同于核R2锚定蛋白Wtm1。与Sml1和Spd1一样,Dif1在遭遇DNA损伤的细胞中被磷酸化并降解,从而解除对RNR的抑制。Sml1和Dif1之间的一个共享结构域控制着检查点激酶介导的这两种蛋白质的磷酸化和降解。消除Dif1磷酸化会使该蛋白稳定,并延迟损伤诱导 的R2从细胞核到细胞质的重新分布。这项研究表明,Dif1是R2亚基核输入所必需的,并且在调节RNR亚细胞定位动态中起重要作用。

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本文引用的文献

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Mol Cell. 2008 Oct 10;32(1):70-80. doi: 10.1016/j.molcel.2008.08.018.
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