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人类细胞中的修复复制。利用羟基脲的简化测定法。

Repair replication in human cells. Simplified determination utilizing hydroxyurea.

作者信息

Smith C A, Hanawalt P C

出版信息

Biochim Biophys Acta. 1976 May 19;432(3):336-47. doi: 10.1016/0005-2787(76)90143-x.

Abstract

A simplified and shortened procedure has been developed for the determination of repair replication of DNA in cultured mammalian cells. The procedure, using the bromodeoxyuridine density label and a radio-isotopic label has been applied to normal diploid human cells (WI38) and to their SV40 transformants (VA13). After incubation with the repair label the cells are lysed and digested for two hours at 50 degrees C with proteinase K. This digest can then be immediately subjected to alkaline cesium chloride density gradient centrifugation with no need for DNA extraction. Hydroxyurea is used to reduce the level of semi-conservative synthesis that a quantitative determination of repair replication can be accomplished by a single centrifugation. The method is not affected by variation in the effectiveness of the inhibitor although a small amount of semi-conservative synthesis normally occurs in the presence of the drug. The time course of repair replication in WI38 cells is unaffected by the drug. The apparent amount of repair synthesis in ultraviolet irradiated cells is increased 25 to 40% in the presence of hydroxyurea when thymidine is used as tracer. Under certain conditions in which the level of semiconservative synthesis is low (e.g., contact inhibited cells, high ultraviolet doses) the use of hydroxyurea is unnecessary.

摘要

已开发出一种简化且缩短的程序,用于测定培养的哺乳动物细胞中DNA的修复复制。该程序使用溴脱氧尿苷密度标记和放射性同位素标记,已应用于正常二倍体人类细胞(WI38)及其SV40转化体(VA13)。用修复标记物孵育细胞后,将细胞裂解并用蛋白酶K在50℃消化两小时。然后,该消化物可立即进行碱性氯化铯密度梯度离心,无需提取DNA。使用羟基脲来降低半保留合成的水平,从而通过单次离心即可完成对修复复制的定量测定。尽管在药物存在下通常会发生少量的半保留合成,但该方法不受抑制剂有效性变化的影响。WI38细胞中修复复制的时间进程不受该药物影响。当使用胸苷作为示踪剂时,在羟基脲存在下,紫外线照射细胞中修复合成的表观量增加25%至40%。在某些半保留合成水平较低的条件下(例如,接触抑制的细胞、高紫外线剂量),无需使用羟基脲。

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