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使用凝胶电泳或中性滤膜洗脱法测量辐射诱导的DNA损伤,结果显示暴露于pH 9.6后DNA链断裂的频率增加。

Measurement of radiation-induced DNA damage using gel electrophoresis or neutral filter elution shows an increased frequency of DNA strand breaks after exposure to pH 9.6.

作者信息

Flick M B, Warters R L, Yasui L S, Krisch R E

机构信息

Department of Radiation Oncology, University of Pennsylvania School of Medicine, Philadelphia 19104.

出版信息

Radiat Res. 1989 Sep;119(3):452-65.

PMID:2549560
Abstract

The filter elution technique using nondenaturing conditions is widely used to assay DNA double-strand break (DSB) induction and repair. It has been reported that in the measurement of strand breaks higher rates of elution and of initial rejoining are obtained at pH 9.6 compared to pH 7.2. In the present experiments neutral elution at pH 7.2 and 9.6 were compared in the assay of damage to DNA induced by X rays, 125I decay, and restriction enzyme digestion, in an effort to explain this discrepancy and to determine whether the higher rate of elution observed at pH 9.6 corresponds to a greater number of DSBs. X-ray damage to cellular DNA resulted in significantly different elution profiles at the two pH values. In contrast the elution profiles of the DSB induced by intragenomic 125I decays or restriction endonuclease were independent of the pH of the elution buffer. When gamma-irradiated SV40 DNA was exposed to pH 7.2 or 9.6 elution buffer prior to analysis by gel electrophoresis, a significantly greater number of DNA DSBs were detected in the DNA exposed to pH 9.6. We conclude that X and gamma radiation produce lesions (pH 9.6-labile lesions), in proportion to dose, that have the potential of becoming measurable DSBs following incubation under the mildly alkaline condition of pH 9.6. The data suggest that these lesions may result from single-hit events.

摘要

使用非变性条件的滤膜洗脱技术被广泛用于检测DNA双链断裂(DSB)的诱导和修复。据报道,在测量链断裂时,与pH 7.2相比,在pH 9.6时洗脱率和初始重连率更高。在本实验中,比较了在pH 7.2和9.6下的中性洗脱,以检测X射线、125I衰变和限制性内切酶消化对DNA造成的损伤,旨在解释这种差异,并确定在pH 9.6时观察到的较高洗脱率是否对应于更多数量的DSB。X射线对细胞DNA的损伤在两个pH值下产生了显著不同的洗脱图谱。相比之下,基因组内125I衰变或限制性内切酶诱导的DSB的洗脱图谱与洗脱缓冲液的pH值无关。当γ射线照射的SV40 DNA在通过凝胶电泳分析之前暴露于pH 7.2或9.6的洗脱缓冲液中时,在暴露于pH 9.6的DNA中检测到显著更多数量的DNA DSB。我们得出结论,X射线和γ射线按剂量比例产生损伤(pH 9.6敏感损伤),在pH 9.6的轻度碱性条件下孵育后有可能成为可测量的DSB。数据表明这些损伤可能由单次打击事件导致。

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