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导致细胞内钾离子浓度增加的遗传改变不利于酿酒酵母的 DNA 完整性。

Genetic alterations leading to increases in internal potassium concentrations are detrimental for DNA integrity in Saccharomyces cerevisiae.

机构信息

Instituto de Biología Molecular y Celular de Plantas, Universidad Politécnica de Valencia-Consejo Superior de Investigaciones Científicas, Ciudad Politécnica de Innovación, 46022 Valencia, Spain.

出版信息

Genes Cells. 2011 Feb;16(2):152-65. doi: 10.1111/j.1365-2443.2010.01472.x. Epub 2010 Dec 9.

DOI:10.1111/j.1365-2443.2010.01472.x
PMID:21143561
Abstract

We have investigated the effects of alterations in potassium homeostasis on cell cycle progression and genome stability in Saccharomyces cerevisiae. Yeast strains lacking the PPZ1 and PPZ2 phosphatase genes, which aberrantly accumulate potassium, are sensitive to agents causing replicative stress or DNA damage and present a cell cycle delay in the G(1) /S phase. A synthetic slow growth phenotype was identified in a subset of DNA repair mutants upon inhibition of Ppz activity. Moreover, we observe that this slow growth phenotype observed in cdc7(ts) mutants with reduced Ppz activity is reverted by disrupting the TRK1 potassium transporter gene. As over-expression of a mammalian potassium transporter leads to similar phenotypes, we conclude that these defects can be attributed to potassium accumulation. As we reported previously, internal potassium accumulation activates the Slt2 MAP kinase pathway. We show that the removal of SLT2 in ppz1 ppz2 mutants ameliorates sensitivity to agents causing replication stress and DNA damage, whereas over-activation of the pathway leads to similar cell cycle-related defects. Taken together, these results are consistent with inappropriate potassium accumulation reducing DNA replication efficiency, negatively influencing DNA integrity and leading to the requirement of mismatch repair, the MRX complex, or homologous recombination pathways for normal growth.

摘要

我们研究了钾离子稳态的改变对酿酒酵母细胞周期进程和基因组稳定性的影响。缺乏 PPZ1 和 PPZ2 磷酸酶基因的酵母菌株,这些基因异常积累钾离子,对导致复制应激或 DNA 损伤的试剂敏感,并在 G1/S 期出现细胞周期延迟。在抑制 Ppz 活性的情况下,一部分 DNA 修复突变体中出现了合成生长缓慢表型。此外,我们观察到,在 Ppz 活性降低的 cdc7(ts)突变体中,破坏 TRK1 钾转运基因可逆转这种生长缓慢表型。由于过表达哺乳动物钾转运体也会导致类似表型,因此我们得出结论,这些缺陷可归因于钾离子积累。正如我们之前报道的,内部钾离子积累会激活 Slt2 MAP 激酶途径。我们表明,在 ppz1 ppz2 突变体中去除 SLT2 可改善对导致复制应激和 DNA 损伤的试剂的敏感性,而过度激活该途径会导致类似的细胞周期相关缺陷。综上所述,这些结果与钾离子积累不当降低 DNA 复制效率、对 DNA 完整性产生负面影响以及导致需要错配修复、MRX 复合物或同源重组途径来正常生长的观点一致。

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