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叠氮溴乙锭光亲和损伤后碱敏感性及切除修复的快速启动

Alkali lability and rapid initiation of excision repair following photoaffinity damage by ethidium azide.

作者信息

Kulkarni M S, Yielding K L

出版信息

Chem Biol Interact. 1985 Dec 17;56(1):89-99. doi: 10.1016/0009-2797(85)90041-9.

Abstract

DNA damage and repair provoked by ethidium azide (EA) photoaffinity labeling in mouse leukemia cells was studied by measuring sedimentation properties of nucleoids in neutral sucrose gradients, and it was found that the strand opening step was faster than that which followed damage of cells by ultraviolet (UV) light. The two insults were compared at levels of damage which gave the same overall rates of repair synthesis in intact cells and which required the same length of time to complete repair, as judged by the restoration of supercoiling of the isolated nucleoids. In the case of UV, single-strand breaks in DNA were detectable at 30 min, maximum at 2 h, and the superhelical properties restored at 21 h. With photoaffinity labeling, single-strand breaks were prominent immediately, even when photolabeling of cells was done on ice, but restoration of DNA supercoiling still required 21 h. Photolabeling of isolated nucleoids or isolated viral DNA with EA failed to introduce DNA strand breaks. However, it was discovered that photoaffinity labeling of DNA with EA resulted in alkali labile sites shown by single strand breaks produced on alkaline sucrose sedimentation or by alkali exposure followed by sedimentation on neutral formamide gradients. These results suggest that the drug attachment sites should be identifiable by the location of such single strand breaks.

摘要

通过测量中性蔗糖梯度中核小体的沉降特性,研究了叠氮溴乙锭(EA)光亲和标记对小鼠白血病细胞造成的DNA损伤及修复情况。结果发现,与紫外线(UV)照射损伤细胞相比,EA光亲和标记引发的链断裂步骤更快。在完整细胞中,两种损伤在修复合成总体速率相同且完成修复所需时间相同的损伤水平下进行比较,这是通过分离核小体超螺旋的恢复来判断的。对于UV损伤,DNA单链断裂在30分钟时可检测到,2小时时达到最大值,21小时时超螺旋特性恢复。而对于光亲和标记,即使在冰上对细胞进行光标记,单链断裂也立即很明显,但DNA超螺旋的恢复仍需21小时。用EA对分离的核小体或分离的病毒DNA进行光标记未能引入DNA链断裂。然而,发现用EA对DNA进行光亲和标记会导致碱不稳定位点,这可通过碱性蔗糖沉降产生的单链断裂或碱处理后在中性甲酰胺梯度上沉降来显示。这些结果表明,药物附着位点应可通过此类单链断裂的位置来识别。

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