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Quantitative 3D structured illumination microscopy of nuclear structures

机译:核结构的定量3D结构照明显微镜

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3D structured illumination microscopy (3D-SIM) is the super-resolution technique of choice for multicolor volumetric imaging. Here we provide a validated sample preparation protocol for labeling nuclei of cultured mammalian cells, image acquisition and registration practices, and downstream image analysis of nuclear structures and epigenetic marks. Using immunostaining and replication labeling combined with image segmentation, centroid mapping and nearest-neighbor analyses in open-source environments, 3D maps of nuclear structures are analyzed in individual cells and normalized to fluorescence standards on the nanometer scale. This protocol fills an unmet need for the application of 3D-SIM to the technically challenging nuclear environment, and subsequent quantitative analysis of 3D nuclear structures and epigenetic modifications. In addition, it establishes practical guidelines and open-source solutions using ImageJ/Fiji and the TANGO plugin for high-quality and routinely comparable data generation in immunostaining experiments that apply across model systems. From sample preparation through image analysis, the protocol can be executed within one week.
机译:3D结构化照明显微镜(3D-SIM)是多色体积成像的超分辨率技术。在这里,我们提供了验证的样品制备方案,用于标记培养的哺乳动物细胞,图像采集和登记措施以及核结构的下游图像分析和表观遗传标记。使用免疫染色和复制标记与图像分割,在开源环境中的质心映射和最近邻分析,在单个细胞中分析核结构的3D地图,并在纳米级上标准化为荧光标准。该协议填补了将3D-SIM应用于技术挑战的核环境的未满足,以及随后对3D核结构和表观遗传修饰的定量分析。此外,它还使用imagej / fiji和探戈插件来建立实用的准则和开源解决方案,用于在免疫统计实验中应用跨模型系统的高质量和常规可比较的数据生成。从样品制备通过图像分析,协议可以在一周内执行。

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