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Substrate specificity of the Ogg1 protein of Saccharomyces cerevisiae: excision of guanine lesions produced in DNA by ionizing radiation- or hydrogen peroxide/metal ion-generated free radicals.

机译:酿酒酵母Ogg1蛋白的底物特异性:通过电离辐射或过氧化氢/金属离子生成的自由基对DNA中产生的鸟嘌呤损伤的切除。

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摘要

We have investigated the substrate specificity of the Ogg1 protein of Saccharomyces cerevisiae (yOgg1 protein) for excision of modified DNA bases from oxidatively damaged DNA substrates using gas chromatography/isotope dilution mass spectrometry. Four DNA substrates prepared by treatment with H2O2/Fe(III)-EDTA/ascorbic acid, H2O2/Cu(II) and gamma-irradiation under N2O or air were used. The results showed that 8-hydroxyguanine (8-OH-Gua) and 2,6-diamino-4-hydroxy-5-formamidopyrimidine (FapyGua) were efficiently excised from DNA exposed to ionizing radiation in the presence of N2O or air. On the other hand, 8-OH-Gua and FapyGua were not excised from H2O2/Fe(III)-EDTA/ascorbic acid-treated and H2O2/Cu(II)-treated DNA respectively. Fourteen other lesions, including the adenine lesions 8-hydroxyadenine and 4,6-diamino-5-formamidopyrimidine, were not excised from any of the DNA substrates. Kinetics of excision significantly depended on the nature of the damaged DNA substrates. The findings suggest that, in addition to 8-OH-Gua, FapyGua may also be a primary substrate of yOgg1 in cells. The results also show significant differences between the substrate specificities of yOgg1 protein and its functional analog Fpg protein in Escherichia coli.
机译:我们已经研究了酿酒酵母Ogg1蛋白(yOgg1蛋白)的底物特异性,可使用气相色谱/同位素稀释质谱法从氧化损伤的DNA底物中切除修饰的DNA碱基。使用通过H 2 O 2 / Fe(III)-EDTA /抗坏血酸,H 2 O 2 / Cu(II)和在N 2 O或空气下的γ-辐射处理制备的四种DNA底物。结果表明,在存在N2O或空气的情况下,可以从暴露于电离辐射的DNA中有效地切除8-羟基鸟嘌呤(8-OH-Gua)和2,6-二氨基-4-羟基-5-甲酰胺基嘧啶(FapyGua)。另一方面,未分别从H 2 O 2 / Fe(III)-EDTA /抗坏血酸处理的DNA和H 2 O 2 / Cu(II)处理的DNA中切除8-OH-Gua和FapyGua。没有从任何DNA底物中切下14个其他损伤,包括腺嘌呤损伤8-羟基腺嘌呤和4,6-二氨基-5-甲酰胺基嘧啶。切除的动力学很大程度上取决于受损的DNA底物的性质。这些发现表明,除了8-OH-Gua外,FapyGua还可能是细胞中yOgg1的主要底物。结果还显示,yOgg1蛋白的底物特异性与其功能类似物Fpg蛋白在大肠杆菌中有显着差异。

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