The relative contribution of adduct blockage and DNA repair on template utilization during replication of 1,N2-propanodeoxyguanosine and pyrimido[1,2-α]purin-10(3H)-one-adducted M13MB102 genomes

Mutation Research/DNA Repair Pub Date : 2001-04-04 DOI:10.1016/S0921-8777(01)00064-7

Stephen P. Fink , Lawrence J. Marnett

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引用次数: 3

Abstract

The role of replication blockage by the exocyclic DNA adducts propanodeoxyguanosine (PdG) and pyrimido[1,2-α]purin-10(3H)-one (M₁G) was determined through the use of site-specifically adducted M13MB102 genomes containing a C:C-mismatch ∼3000 base-pairs from the site of adduct incorporation. Genomes containing either dG, PdG, or M₁G positioned at site 6256 of the (−)-strand were transformed into repair-proficient and repair-deficient Escherichia coli strains and the percent template utilization was determined by hybridization analysis. Unmodified genomes containing a C:C-mismatch resulted in a percent template utilization of approximately 60 and 40% for the (−)- and (+)-strands, respectively. Transformation of PdG- or M₁G-adducted genomes resulted in approximately a 60–40% and 50–50% (−)-strand to (+)-strand ratio, respectively, indicating that PdG and M₁G are negligible blocks to replication in repair-proficient E. coli. This is in contrast to previous studies using (PdG:T)- and (M₁G:T)-mismatched M13MB102 genomes, which resulted in a majority of the replication events using the unadducted (+)-strand and suggested that both adducts were significant blocks to replication [J. Biol. Chem. 272 (1997) 11434; Proc. Natl. Acad. Sci. U.S.A. 94 (1997) 8652]. The C:C-mismatch results, though, indicate that the large strand bias detected in the earlier studies is due to repair of the adducts and resynthesis of the (−)-strand using the (+)-strand as a template for repair synthesis. Transformation of adducted C:C-mismatched genomes into E. coli strains deficient in nucleotide excision repair did result in an increased strand bias with only approximately 20 and 34% of the replication events using the (−)-strand for PdG- and M₁G-adducted genomes, respectively. The increased strand bias indicates the importance of nucleotide excision repair in the removal of PdG and M₁G.

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加合物阻断和DNA修复对1，N2丙脱氧鸟苷和嘧啶并[1，2-α]嘌呤-10（3H）-酮加合物M13MB102基因组复制过程中模板利用的相对贡献

外环DNA加合物丙脱氧鸟苷（PdG）和嘧啶并[1，2-α]嘌呤-10（3H）-酮（M1G）阻断复制的作用是通过使用位点特异性加合的M13MB102基因组来确定的，该基因组包含与加合物结合位点的C:C错配～3000个碱基对。将位于（−）链6256位点的含有dG、PdG或M1G的基因组转化为修复熟练和修复缺陷的大肠杆菌菌株，并通过杂交分析确定模板利用率。含有C:C错配的未修饰基因组导致（−）-和（+）-链的模板利用率分别约为60%和40%。PdG或M1G加合基因组的转化分别导致约60-40%和50-50%的（−）链与（+）链之比，这表明PdG和M1G在精通修复的大肠杆菌中是可忽略的复制块。这与先前使用（PdG:T）-和（M1G:T的）-错配的M13MB102基因组的研究形成对比，这些研究导致了大多数使用未转导的（+）链的复制事件，并表明两种加合物都是复制的重要阻断[J.Biol.Chem.272（1997）11434；Proc.Natl.Acad.Sci.U.SU.S.a.94（1997）8652]。然而，C:C错配结果表明，早期研究中检测到的大链偏置是由于使用（+）链作为修复合成模板修复加合物和（−）链的再合成。将加合的C:C错配基因组转化为核苷酸切除修复缺陷的大肠杆菌菌株确实导致了链偏倚的增加，对于PdG-和M1G-加合基因组，分别只有大约20%和34%的复制事件使用（−）链。增加的链偏倚表明核苷酸切除修复在去除PdG和M1G中的重要性。

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Mutation Research/DNA Repair

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