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如彗星试验所示,外源性DNA连接酶对经限制性内切酶MspI或博来霉素处理的G0期人淋巴细胞的保护作用。

Protection provided by exogenous DNA ligase in G0 human lymphocytes treated with restriction enzyme MspI or bleomycin as shown by the comet assay.

作者信息

Flores M J, Ortiz T, Piñero J, Cortés F

机构信息

Department of Cell Biology, University of Seville, Spain.

出版信息

Environ Mol Mutagen. 1998;32(4):336-43.

PMID:9882008
Abstract

DNA double-strand breaks (DSB) may arise either spontaneously during cellular processes or as a result of exposure to DNA-damaging agents such as ionizing radiation, or radiomimetic agents such as restriction endonucleases or bleomycin. It is widely accepted that nonrepaired or misrepaired DSB are the main lesions leading to the production of chromosomal aberrations, mutagenesis, oncogenic transformation, and cell killing. Studies focusing on this relationship, as well as the possible modulation of DNA repair mechanisms, are currently of major interest. A wide variety of test systems are available to study DNA damage. In the last few years, single-cell gel electrophoresis, commonly known as "comet assay," has been considered a rapid, sensitive, and visual method for quantifying DNA strand breaks and alkali-labile damage in individual cells. In this study, making use of the comet assay, we tried to find out if under conditions that maintain chromatin structure the DNA ligase from T4 phage is able to facilitate the rejoining of strand breaks with different end structures, induced by the restriction endonuclease MspI or bleomycin in living human lymphocytes in a nonproliferating state. T4 DNA ligase, as well as the restriction endonuclease or bleomycin, were introduced together by electroporation into human lymphocytes. Our results support the idea that it is possible to modulate the DSB-rejoining of different DNA strand-breaking agents by exogenous T4 DNA ligase.

摘要

DNA双链断裂(DSB)可能在细胞过程中自发产生,也可能是由于暴露于DNA损伤剂(如电离辐射)或放射模拟剂(如限制性内切核酸酶或博来霉素)而导致的。人们普遍认为,未修复或错配的DSB是导致染色体畸变、诱变、致癌转化和细胞死亡的主要损伤。目前,专注于这种关系以及DNA修复机制可能的调节的研究备受关注。有各种各样的测试系统可用于研究DNA损伤。在过去几年中,单细胞凝胶电泳,通常称为“彗星试验”,已被认为是一种快速、灵敏且直观的方法,用于定量单个细胞中的DNA链断裂和碱不稳定损伤。在本研究中,利用彗星试验,我们试图弄清楚在维持染色质结构的条件下,来自T4噬菌体的DNA连接酶是否能够促进在非增殖状态的活人类淋巴细胞中由限制性内切核酸酶MspI或博来霉素诱导的具有不同末端结构的链断裂的重新连接。通过电穿孔将T4 DNA连接酶以及限制性内切核酸酶或博来霉素一起导入人类淋巴细胞。我们的结果支持这样一种观点,即外源性T4 DNA连接酶有可能调节不同DNA链断裂剂的DSB重新连接。

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