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N-terminus of the rat adenine glycosylase MYH affects excision rates and processing of MYH-generated abasic sites

机译:大鼠腺嘌呤糖基化酶MYH的N端影响切除率和MYH产生的脱碱基位点的加工

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摘要

Repair of most modified and mispaired bases in the genome is initiated by DNA glycosylases, which bind to their respective targets and cleave the N-glycosyl bond to initiate base excision repair (BER). The mammalian homolog of the Escherichia coli MutY DNA glycosylase (MYH) cleaves adenine residues paired with either oxidized or non-modified guanines. MYH is crucial for the avoidance of mutations resulting from oxidative DNA damage. Multiple N-terminal splice variants of MYH exist in mammalian cells and it is likely that different variants result in the production of enzymes with altered properties. To investigate whether modifications in the N-terminus are consequential to MYH function, we overexpressed intact and N-terminal-deletion rat MYH proteins and examined their activities. We found that deletion of 75 amino acids, which perturbs the catalytic core that is conserved with E.coli MutY, abolished excision activity. In contrast, deletions limited to the extended mammalian N-terminal domain, differentially influenced steady-state excision rates. Notably, deletion of 50 amino acids resulted in an enzyme with a significantly lower K-m favoring formation of excision products with 3'-OH termini. Our findings suggest that MYH isoforms divergent in the N-terminus influence excision rates and processing of abasic sites.
机译:DNA糖基化酶可启动基因组中大多数修饰和错配碱基的修复,DNA糖基化酶与各自的靶标结合并切割N-糖基键以启动碱基切除修复(BER)。大肠杆菌MutY DNA糖基化酶(MYH)的哺乳动物同源物可裂解腺嘌呤残基与氧化或未修饰的鸟嘌呤配对。 MYH对于避免DNA氧化损伤引起的突变至关重要。哺乳动物细胞中存在MYH的多个N末端剪接变体,并且不同的变体可能导致产生具有改变的性质的酶。若要调查是否在N末端的修饰是MYH功能的结果,我们过表达完整和N末端缺失的大鼠MYH蛋白,并检查了它们的活性。我们发现删除75个氨基酸,扰乱了与大肠杆菌MutY保守的催化核心,消除了切除活性。相比之下,仅限于扩展的哺乳动物N末端域的删除差异地影响稳态切除率。值得注意的是,缺失50个氨基酸会导致酶的K-m值大大降低,有利于形成带有3'-OH末端的切除产物。我们的发现表明,MYH亚型在N末端发散,影响切除率和无碱基位点的加工。

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