首页> 外文期刊>Journal of Physics, D. Applied Physics: A Europhysics Journal >Super-resolution imaging of densely packed DNA in nuclei of zebrafish embryos using stimulated emission double depletion microscopy
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Super-resolution imaging of densely packed DNA in nuclei of zebrafish embryos using stimulated emission double depletion microscopy

机译:使用刺激的发射双耗尽显微镜显微镜斑马鱼胚胎核细胞中密集包装DNA的超分辨率成像

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摘要

Knowledge about the spatial distribution of DNA in the cell nucleus is an essential aspect of understanding how cells control gene expression. Here, we describe a protocol for the preparation of samples for super-resolution stimulated emission depletion (STED) fluorescence imaging of bulk DNA in nuclei of blastomeres within animal caps of zebrafish embryos. We evaluated different mounting media and DNA stains. With samples stained with the silicon-rhodamine dye JF646 conjugated to Hoechst 33342 as a DNA tag and mounted in glycerol, we compared confocal, STED and stimulated emission double depletion (STEDD), in particular with respect to background fluorescence and image resolution. We show that super-resolved images of lateral planes through the cell nuclei can be collected up to imaging depths of several tens of micrometers with greatly reduced background using STEDD. Acquisition of axial image stacks using both lateral and axial STED confinement was also feasible, though at reduced resolution due to photobleaching. Further optimization steps are discussed to obtain a robust experimental platform for imaging the three-dimensional distribution of DNA inside zebrafish embryo tissue.
机译:关于细胞核中DNA的空间分布的知识是理解细胞控制基因表达的基本方面。在这里,我们描述了一种制备用于在斑马鱼胚胎动物盖中的卵泡细胞核中批量DNA的超分辨率刺激耗尽(STED)荧光成像的样品的方案。我们评估了不同的安装介质和DNA污渍。对于用与Hoechst 33342缀合的硅 - 罗丹明染料JF646染色的样品作为DNA标签并安装在甘油中,我们比较了辅焦,SED和刺激的发射双耗尽(STEDD),特别是关于背景荧光和图像分辨率。我们表明,通过细胞核的超分辨率图像可以收集到几十微米的成像深度,其使用STEDD大大减少了背景。使用横向和轴向型围栏的轴向图像堆叠的采集也是可行的,但由于摄影引起的分辨率降低。讨论了进一步的优化步骤以获得用于对斑马鱼胚组织内的DNA的三维分布进行成像的稳健实验平台。

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