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Spatial Localization of Genes Determined by Intranuclear DNA Fragmentation with the Fusion Proteins Lamin KRED and Histone KRED und Visible Light

机译:通过融合蛋白Lamin KRED和Histone KRED和可见光融合核内DNA片段确定的基因的空间定位

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摘要

The highly organized DNA architecture inside of the nuclei of cells is accepted in the scientific world. In the human genome about 3 billion nucleotides are organized as chromatin in the cell nucleus. In general, they are involved in gene regulation and transcription by histone modification. Small chromosomes are localized in a central nuclear position whereas the large chromosomes are peripherally positioned. In our experiments we inserted fusion proteins consisting of a component of the nuclear lamina (lamin B1) and also histone H2A, both combined with the light inducible fluorescence protein KillerRed (KRED). After activation, KRED generates reactive oxygen species (ROS) producing toxic effects and may cause cell death. We analyzed the spatial damage distribution in the chromatin after illumination of the cells with visible light. The extent of DNA damage was strongly dependent on its localization inside of nuclei.The ROS activity allowed to gain information about the location of genes and their functions via sequencing and data base analysis of the double strand breaks of the isolated DNA. A connection between the damaged gene sequences and some diseases was found.
机译:细胞核内部高度组织化的DNA结构已为科学界所接受。在人类基因组中,约30亿个核苷酸以染色质的形式组织在细胞核中。通常,它们通过组蛋白修饰参与基因调控和转录。小染色体位于中央核位置,而大染色体位于外围。在我们的实验中,我们插入了由核纤层蛋白(lamin B1)和组蛋白H2A组成的融合蛋白,两者均与光诱导荧光蛋白KillerRed(KRED)结合。激活后,KRED产生活性氧(ROS),产生毒性作用,并可能导致细胞死亡。我们用可见光照射细胞后分析了染色质中的空间损伤分布。 DNA损伤的程度在很大程度上取决于其在核内的定位.ROS活性可以通过对分离的DNA的双链断裂进行测序和数据库分析来获得有关基因位置及其功能的信息。发现受损的基因序列与某些疾病之间存在联系。

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