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哺乳动物复制性DNA聚合酶催化的DNA合成过程中N2-乙基-2'-脱氧鸟苷三磷酸的有效利用。

Effective utilization of N2-ethyl-2'-deoxyguanosine triphosphate during DNA synthesis catalyzed by mammalian replicative DNA polymerases.

作者信息

Matsuda T, Terashima I, Matsumoto Y, Yabushita H, Matsui S, Shibutani S

机构信息

Research Center for Environmental Quality Control, Kyoto University, Shiga, Japan.

出版信息

Biochemistry. 1999 Jan 19;38(3):929-35. doi: 10.1021/bi982134j.

Abstract

Acetaldehyde is produced by metabolic oxidation of ethanol after drinking alcoholic beverages. This agent reacts with nucleosides and nucleotides, resulting in the formation of N2-ethyl-guanine residues. N2-ethyl-2'-deoxyguanosine (N2-ethyl-dG) adduct has been detected in the lymphocyte DNA of alcoholic patients [Fang, J. L., and Vaca, C. E. (1997) Carcinogenesis 18, 627-632]. Thus, the nucleotide pool is also expected to be modified by acetaldehyde. N2-Ethyl-2'-deoxyguanosine triphosphate (N2-ethyl-dGTP) was chemically synthesized. The utilization of N2-ethyl-dGTP during DNA synthesis was determined by steady-state kinetic studies. N2-Ethyl-dGTP was efficiently incorporated opposite template dC in reactions catalyzed by mammalian DNA polymerase alpha and delta. When pol alpha was used, the insertion frequency of N2-ethyl-dGTP was 400 times less than that of dGTP, but 320 times higher than that of 7,8-dihydro-8-oxo-2'-deoxyguanosine triphosphate (8-oxo-dGTP), an oxidative damaged nucleotide. Using pol delta, the insertion frequency of N2-ethyl-dGTP was only 37 times less than that of dGTP. The chain extension from dC:N2-ethyl-dG pair occurred much more rapidly: the extension frequencies for pol alpha and pol delta were only 3.8 times and 6.3 times, respectively, lower than that of dC:dG pair. We also found that N2-ethyl-dG can be detected in urine samples obtained from healthy volunteers who had abstained from drinking alcohol for 1 week before urine collection. This indicates that humans are exposed constantly to acetaldehyde even without drinking alcoholic beverages. Incorporation of N2-ethyl-dG adducts into DNA may cause mutations and may be related to the development of alcohol- and acetaldehyde-induced human cancers.

摘要

饮用含酒精饮料后,乙醇经代谢氧化产生乙醛。该物质与核苷和核苷酸发生反应,导致形成N2 - 乙基鸟嘌呤残基。在酒精性患者的淋巴细胞DNA中已检测到N2 - 乙基 - 2'-脱氧鸟苷(N2 - 乙基 - dG)加合物[Fang, J. L., and Vaca, C. E. (1997) Carcinogenesis 18, 627 - 632]。因此,核苷酸池也有望被乙醛修饰。N2 - 乙基 - 2'-脱氧鸟苷三磷酸(N2 - 乙基 - dGTP)已通过化学合成得到。通过稳态动力学研究确定了DNA合成过程中N2 - 乙基 - dGTP的利用情况。在哺乳动物DNA聚合酶α和δ催化的反应中,N2 - 乙基 - dGTP能有效地掺入与模板dC相对应的位置。当使用聚合酶α时,N2 - 乙基 - dGTP的插入频率比dGTP低400倍,但比氧化损伤核苷酸7,8 - 二氢 - 8 - 氧代 - 2'-脱氧鸟苷三磷酸(8 - 氧代 - dGTP)高320倍。使用聚合酶δ时,N2 - 乙基 - dGTP的插入频率仅比dGTP低37倍。从dC:N2 - 乙基 - dG碱基对开始的链延伸发生得更快:聚合酶α和聚合酶δ的延伸频率分别仅比dC:dG碱基对低3.8倍和6.3倍。我们还发现,在收集尿液前已戒酒1周的健康志愿者的尿液样本中可检测到N2 - 乙基 - dG。这表明即使不饮用含酒精饮料,人类也持续暴露于乙醛中。N2 - 乙基 - dG加合物掺入DNA可能会导致突变,并且可能与酒精和乙醛诱导的人类癌症的发生有关。

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