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亚砷酸钠在彗星试验中对DNA断裂和细胞凋亡的时间依赖性影响。

Time-dependent effects of sodium arsenite on DNA breakage and apoptosis observed in the comet assay.

作者信息

Brink Andreas, Schulz Berta, Kobras Kristin, Lutz Werner K, Stopper Helga

机构信息

Department of Toxicology, University of Würzburg, Versbacher Str. 9, D-97078 Würzburg, Germany.

出版信息

Mutat Res. 2006 Feb 28;603(2):121-8. doi: 10.1016/j.mrgentox.2005.10.015. Epub 2005 Dec 27.

Abstract

To assess genotoxic effects of sodium arsenite (NaAsO2) the single-cell gel electrophoresis (comet assay) had been conducted in various studies indicating genotoxicity. However, DNA fragmentation due to NaAsO2-induced apoptosis may constitute a bias in the interpretation of the results. Apoptotic cells can show typically large and diffuse comets, which are usually excluded during genotoxicity analysis. It is controversial whether there is a time-window in which the apoptotic process generates comets that would falsely be interpreted to be the result of genotoxic DNA damage. Therefore, we evaluated frequency histograms for single-cell measures of tail DNA (% DNA in comet tail) in 30-min intervals after incubation of mouse lymphoma L5178Y cells with sodium arsenite (NaAsO2). In parallel, we evaluated apoptosis by measuring annexin V-positive cells with flow cytometry, and visualized apoptotic cells on slides by Hoechst bisbenzimide 33258 staining. The first observed effect at 30 min after treatment was an increase in annexin V-positive cells. At about 60 min the number of cells with moderate DNA migration increased in the comet-assay analysis. After 90 min, an increase in the number of cells with high levels of DNA migration was observed, which resulted in a bimodal distribution of cells with moderate and high levels of DNA migration. Hoechst-stained apoptotic cells could only be observed at later times (> or = 120 min). This means that the treatment would have been considered to be genotoxic if analysed at 120 min even if the cells with high levels of DNA migration would have been excluded. The occurrence of annexin V-positive cells preceded the appearance of cells with moderate levels of DNA migration. We hypothesize that these cells were early apoptotic cells and not indicative of genotoxic damage. We conclude that DNA-damaging effects of NaAsO2 cannot adequately be interpreted if the comet assay is not accompanied by separate analysis of early endpoints for induction of apoptosis.

摘要

为评估亚砷酸钠(NaAsO₂)的遗传毒性,在各项研究中进行了单细胞凝胶电泳(彗星试验),结果表明其具有遗传毒性。然而,NaAsO₂诱导的凋亡所导致的DNA片段化可能会在结果解释中造成偏差。凋亡细胞通常会显示出典型的大而弥散的彗星状条带,在遗传毒性分析中这些通常会被排除。凋亡过程是否存在一个时间窗口,在此期间凋亡产生的彗星状条带会被错误地解释为遗传毒性DNA损伤的结果,这存在争议。因此,在用亚砷酸钠(NaAsO₂)孵育小鼠淋巴瘤L5178Y细胞后,我们以30分钟为间隔评估了尾DNA(彗星尾中的DNA百分比)单细胞测量的频率直方图。同时,我们通过流式细胞术测量膜联蛋白V阳性细胞来评估凋亡情况,并通过Hoechst双苯并咪唑33258染色在载玻片上观察凋亡细胞。处理后30分钟首次观察到的效应是膜联蛋白V阳性细胞增加。在大约60分钟时,彗星试验分析中出现中等程度DNA迁移的细胞数量增加。90分钟后,观察到高水平DNA迁移的细胞数量增加,这导致了中等水平和高水平DNA迁移细胞的双峰分布。仅在较晚时间(≥ 120分钟)才能观察到经Hoechst染色的凋亡细胞。这意味着如果在120分钟时进行分析,即使排除了高水平DNA迁移的细胞,该处理也会被认为具有遗传毒性。膜联蛋白V阳性细胞的出现先于中等水平DNA迁移细胞的出现。我们推测这些细胞是早期凋亡细胞,并不表明存在遗传毒性损伤。我们得出结论,如果彗星试验没有同时对凋亡诱导的早期终点进行单独分析,就无法充分解释NaAsO₂的DNA损伤效应。

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