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LAMMER激酶有助于维持玉米黑粉菌的基因组稳定性。

LAMMER kinase contributes to genome stability in Ustilago maydis.

作者信息

de Sena-Tomás Carmen, Sutherland Jeanette H, Milisavljevic Mira, Nikolic Dragana B, Pérez-Martín José, Kojic Milorad, Holloman William K

机构信息

Department of Microbiology and Immunology, Weill Cornell Medical College, New York, NY 10065, USA.

Laboratory for Plant Molecular Biology, Institute of Molecular Genetics and Genetic Engineering, University of Belgrade, Serbia.

出版信息

DNA Repair (Amst). 2015 Sep;33:70-7. doi: 10.1016/j.dnarep.2015.05.011. Epub 2015 Jun 19.

Abstract

Here we report identification of the lkh1 gene encoding a LAMMER kinase homolog (Lkh1) from a screen for DNA repair-deficient mutants in Ustilago maydis. The mutant allele isolated results from a mutation at glutamine codon 488 to a stop codon that would be predicted to lead to truncation of the carboxy-terminal kinase domain of the protein. This mutant (lkh1(Q488*)) is highly sensitive to ultraviolet light, methyl methanesulfonate, and hydroxyurea. In contrast, a null mutant (lkh1Δ) deleted of the entire lkh1 gene has a less severe phenotype. No epistasis was observed when an lkh1(Q488*)rad51Δ double mutant was tested for genotoxin sensitivity. However, overexpressing the gene for Rad51, its regulator Brh2, or the Brh2 regulator Dss1 partially restored genotoxin resistance of the lkh1Δ and lkh1(Q488*) mutants. Deletion of lkh1 in a chk1Δ mutant enabled these double mutant cells to continue to cycle when challenged with hydroxyurea. lkh1Δ and lkh1(Q488*) mutants were able to complete the meiotic process but exhibited reduced heteroallelic recombination and aberrant chromosome segregation. The observations suggest that Lkh1 serves in some aspect of cell cycle regulation after DNA damage or replication stress and that it also contributes to proper chromosome segregation in meiosis.

摘要

在此,我们报告了从玉米黑粉菌DNA修复缺陷突变体筛选中鉴定出编码LAMMER激酶同源物(Lkh1)的lkh1基因。分离出的突变等位基因源于谷氨酰胺密码子488突变为终止密码子,预计这将导致该蛋白羧基末端激酶结构域的截短。这种突变体(lkh1(Q488*))对紫外线、甲基磺酸甲酯和羟基脲高度敏感。相比之下,缺失整个lkh1基因的无效突变体(lkh1Δ)具有不太严重的表型。当测试lkh1(Q488*)rad51Δ双突变体对基因毒素的敏感性时,未观察到上位性。然而,过表达Rad51、其调节因子Brh2或Brh2调节因子Dss1的基因部分恢复了lkh1Δ和lkh1(Q488*)突变体对基因毒素的抗性。在chk1Δ突变体中缺失lkh1使这些双突变细胞在受到羟基脲挑战时能够继续循环。lkh1Δ和lkh1(Q488*)突变体能够完成减数分裂过程,但表现出异源等位基因重组减少和染色体分离异常。这些观察结果表明,Lkh1在DNA损伤或复制应激后的细胞周期调控的某些方面发挥作用,并且它也有助于减数分裂中正确的染色体分离。

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