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两种不同的人类DNA二酯酶,可从氧化的DNA中水解3'-封闭的脱氧核糖片段。

Two distinct human DNA diesterases that hydrolyze 3'-blocking deoxyribose fragments from oxidized DNA.

作者信息

Chen D S, Herman T, Demple B

机构信息

Department of Molecular and Cellular Toxicology, Harvard School of Public Health, Boston, MA 02115.

出版信息

Nucleic Acids Res. 1991 Nov 11;19(21):5907-14. doi: 10.1093/nar/19.21.5907.

DOI:10.1093/nar/19.21.5907
PMID:1719484
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC329046/
Abstract

Mammalian cells were investigated for enzymes that help correct oxidative damages in DNA. We focused on 3'-repair diesterases, which process DNA ends at oxidative strand breaks by removing 3'-blocking fragments of deoxyribose that prevent DNA repair synthesis. Two enzymes were found in a variety of mouse, bovine and human tissues and cultured cells. The two activities were purified to differing degrees from HeLa cells. One enzyme had the properties of the known HeLa AP endonuclease (Mr approximately 38,000, with identical substrate specificity and reaction requirements, and cross-reactivity with anti-HeLa AP endonuclease antiserum) and is presumed identical to that protein. The second activity did not interact with anti-HeLa AP endonuclease antibodies and had relatively less AP endonuclease activity. This second enzyme may have been detected in other studies but never characterized. In addition to the 3'-repair diesterase and AP endonuclease, this partially purified preparation also harbored DNA 3'-phosphatase and 3'-deoxyribose diesterase activities. It is unknown whether all activities detected in the second preparation are due to a single protein, although activity against undamaged DNA was not detected. The in vivo roles of these two widely distributed 3'-repair diesterase/AP endonucleases have not been determined, but with the characterizations presented here such questions may now be focused.

摘要

对哺乳动物细胞中有助于纠正DNA氧化损伤的酶进行了研究。我们重点关注3'-修复二酯酶,该酶通过去除阻止DNA修复合成的脱氧核糖3'-阻断片段来处理氧化链断裂处的DNA末端。在多种小鼠、牛和人类组织及培养细胞中发现了两种酶。从HeLa细胞中对这两种活性进行了不同程度的纯化。一种酶具有已知的HeLa AP内切核酸酶的特性(分子量约为38,000,具有相同的底物特异性和反应要求,且与抗HeLa AP内切核酸酶抗血清有交叉反应),推测与该蛋白相同。第二种活性不与抗HeLa AP内切核酸酶抗体相互作用,且AP内切核酸酶活性相对较低。这种第二种酶可能在其他研究中已被检测到,但从未被鉴定过。除了3'-修复二酯酶和AP内切核酸酶外,这种部分纯化的制剂还具有DNA 3'-磷酸酶和3'-脱氧核糖二酯酶活性。虽然未检测到针对未受损DNA的活性,但尚不清楚在第二种制剂中检测到的所有活性是否都归因于单一蛋白质。这两种广泛分布的3'-修复二酯酶/AP内切核酸酶在体内的作用尚未确定,但基于本文所提供的特性描述,现在可以聚焦此类问题。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6293/329046/c507e1611d90/nar00101-0109-b.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6293/329046/cc97c3dfc6ba/nar00101-0109-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6293/329046/c507e1611d90/nar00101-0109-b.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6293/329046/cc97c3dfc6ba/nar00101-0109-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6293/329046/c507e1611d90/nar00101-0109-b.jpg

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