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彗星 - FISH 与 rDNA 探针用于分析植物细胞中诱变剂诱导的 DNA 损伤。

Comet-FISH with rDNA probes for the analysis of mutagen-induced DNA damage in plant cells.

机构信息

Department of Plant Anatomy and Cytology, University of Silesia, Jagiellonska 28, 40-032 Katowice, Poland.

出版信息

Environ Mol Mutagen. 2012 Jun;53(5):369-75. doi: 10.1002/em.21699. Epub 2012 May 4.

Abstract

We used comet-fluorescence in situ hybridization (FISH) in the model plant species Crepis capillaris following exposure of seedlings to maleic hydrazide (MH). FISH with 5S and 25S rDNA probes was applied to comets obtained under alkaline conditions to establish whether these DNA regions were preferentially involved in comet tail formation. MH treatment induced significant fragmentation of nuclear DNA and of rDNA loci. A 24-h post-treatment recovery period allowed a partial reversibility of MH-induced damage on nuclear and rDNA regions. Analyses of FISH signals demonstrated that rDNA sequences were always involved in tail formation and that 5S rDNA was more frequently present in the tail than 25S rDNA, regardless of treatment. The involvement of 25S rDNA in nucleolus formation and differences in chromatin structure between the two loci may explain the different susceptibility of the 25S and 5S rDNA regions to migrate into the tail. This work is the first report on the application of FISH to comet preparations from plants to analyze the distribution and repair of DNA damage within specific genomic regions after mutagenic treatment. Moreover, our work suggests that comet-FISH in plants may be a useful tool for environmental monitoring assessment.

摘要

我们在模式植物山瞿麦幼苗中使用彗星荧光原位杂交(FISH),在暴露于马来酰肼(MH)后进行实验。我们使用 5S 和 25S rDNA 探针进行碱性条件下彗星的 FISH,以确定这些 DNA 区域是否优先参与彗星尾形成。MH 处理诱导核 DNA 和 rDNA 位点的显著片段化。24 小时的处理后恢复期允许 MH 诱导的核和 rDNA 区域的损伤部分可逆。FISH 信号分析表明,rDNA 序列始终参与尾形成,并且 5S rDNA 比 25S rDNA 更频繁地存在于尾部,而不管处理如何。25S rDNA 参与核仁形成以及两个位点之间染色质结构的差异可能解释了 25S 和 5S rDNA 区域对进入尾部的迁移的不同敏感性。这项工作是首次报道将 FISH 应用于彗星植物制剂,以分析诱变处理后特定基因组区域内 DNA 损伤的分布和修复。此外,我们的工作表明,植物彗星 FISH 可能是环境监测评估的有用工具。

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