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DNA Multiphoton Absorption Generates Localized Damage for Studying Repair Dynamics in Live Cells

机译:DNA多光子吸收产生局部损伤用于研究活细胞的修复动力学

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摘要

Investigations into the spatiotemporal dynamics of DNA repair using live-cell imaging are aided by the ability to generate well defined regions of ultravioletlike photolesions in an optical microscope. We demonstrate that multiphoton excitation of DNA in live cells with visible femtosecond pulses produces thymine cyclopyrimidine dimers (CPDs), the primary ultraviolet DNA photoproduct. The CPDs are produced with a cubic to supercubic power dependence using pulses in the wavelength range from at least 400 to 525 nm. We show that the CPDs are confined in all three spatial dimensions, making multiphoton excitation of DNA with visible light an ideal technique for generating localized DNA photolesions in a wide variety of samples, from cultured cells to thicker tissues. We demonstrate the utility of this method by applying it to investigate the spatiotemporal recruitment of GFP-tagged topoisomerase I (TopI) to sites of localized DNA damage in polytene chromosomes within live cells of optically thick Drosophila salivary glands.
机译:利用活细胞成像技术对DNA修复的时空动力学进行研究,是因为能够在光学显微镜中生成清晰定义的类紫外线光致病变区域。我们证明了可见光飞秒脉冲在活细胞中DNA的多光子激发产生胸腺嘧啶环嘧啶二聚体(CPDs),主要的紫外线DNA光产物。使用波长范围从至少400到525 nm的脉冲产生的CPD具有立方到超立方功率依赖性。我们表明,CPD局限在所有三个空间维度上,使可见光对DNA的多光子激发成为在从培养细胞到较厚组织的各种样品中生成局部DNA光损伤的理想技术。我们通过应用它来调查时空募集的GFP标记的拓扑异构酶I(TopI)到光学厚果蝇唾液腺的活细胞内的多烯染色体中的局部DNA损伤的位点,证明了该方法的实用性。

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