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与无嘌呤位点绕过相关的DNA合成错误

Infidelity of DNA synthesis associated with bypass of apurinic sites.

作者信息

Schaaper R M, Kunkel T A, Loeb L A

出版信息

Proc Natl Acad Sci U S A. 1983 Jan;80(2):487-91. doi: 10.1073/pnas.80.2.487.

Abstract

The mutagenic potential of apurinic sites in vivo has been studied by transfection of depurinated phi X174 DNA containing amber mutations into SOS-induced Escherichia coli spheroplasts. Mutagenicity is abolished by treatment of the depurinated DNA with an apurinic endonuclease from Hela cells, establishing the apurinic site as the mutagenic lesion. The frequency of copying apurinic sites in vitro was analyzed by measuring the extent of DNA synthesis using E. coli DNA polymerase I and avian myeloblastosis DNA polymerase. The inhibition of DNA synthesis by apurinic sites was less with avian myeloblastosis DNA polymerase, suggesting that this error-prone enzyme copies apurinic sites with greater frequency. Consistent with this conclusion is the observation that, upon transfection into (normal) spheroplasts, the reversion frequency of depurinated phi X174 am3 DNA copied with avian myeloblastosis virus DNA polymerase is much greater than that of the same DNA copied with E. coli DNA polymerase I. Sequence analysis of the DNA of 33 revertant phage produced by depurination indicates a preference for incorporation of deoxyadenosine opposite putative apurinic sites. The combined results indicate that mutagenesis resulting from apurinic sites is associated with bypass of these noncoding lesions during DNA synthesis.

摘要

通过将含有琥珀突变的脱嘌呤φX174 DNA转染到经SOS诱导的大肠杆菌原生质球中,研究了体内脱嘌呤位点的诱变潜力。用来自Hela细胞的脱嘌呤内切酶处理脱嘌呤DNA后,诱变活性消失,这表明脱嘌呤位点是诱变损伤。通过使用大肠杆菌DNA聚合酶I和禽成髓细胞瘤DNA聚合酶测量DNA合成的程度,分析了体外复制脱嘌呤位点的频率。禽成髓细胞瘤DNA聚合酶对脱嘌呤位点引起的DNA合成抑制作用较小,这表明这种易出错的酶更频繁地复制脱嘌呤位点。与此结论一致的是,观察到在转染到(正常)原生质球后,用禽成髓细胞瘤病毒DNA聚合酶复制的脱嘌呤φX174 am3 DNA的回复频率远高于用大肠杆菌DNA聚合酶I复制的相同DNA的回复频率。对由脱嘌呤产生的33个回复噬菌体的DNA进行序列分析表明,在假定的脱嘌呤位点对面优先掺入脱氧腺苷。综合结果表明,脱嘌呤位点引起的诱变与DNA合成过程中这些非编码损伤的绕过有关。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/13e0/393403/18cdd730c9d9/pnas00628-0176-a.jpg

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