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首页> 外文期刊>Journal of Biophysical and Biochemical Cytology >Imaging of native transcription factors and histone phosphorylation at high resolution in live cells
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Imaging of native transcription factors and histone phosphorylation at high resolution in live cells

机译:在活细胞高分辨率下对天然转录因子和组蛋白磷酸化的成像

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Fluorescent labeling of endogenous proteins for live-cell imaging without exogenous expression of tagged proteins or genetic manipulations has not been routinely possible. We describe a simple versatile antibody-based imaging approach (VANIMA) for the precise localization and tracking of endogenous nuclear factors. Our protocol can be implemented in every laboratory allowing the efficient and nonharmful delivery of organic dye-conjugated antibodies, or antibody fragments, into different metazoan cell types. Live-cell imaging permits following the labeled probes bound to their endogenous targets. By using conventional and super-resolution imaging we show dynamic changes in the distribution of several nuclear transcription factors (i.e., RNA polymerase II or TAF10), and specific phosphorylated histones (γH2AX), upon distinct biological stimuli at the nanometer scale. Hence, considering the large panel of available antibodies and the simplicity of their implementation, VANIMA can be used to uncover novel biological information based on the dynamic behavior of transcription factors or posttranslational modifications in the nucleus of single live cells.
机译:在没有外源性的标记蛋白或遗传操作的情况下,活细胞成像的内源性蛋白质的荧光标记并未常规。我们描述了一种简单的多功能抗体的成像方法(vanima),用于内源性核因子的精确定位和跟踪。我们的协议可以在每个实验室中实施,允许有机染料缀合的抗体或抗体片段的有效和非加工递送到不同的甲卓酮细胞类型中。在与其内源目标结合的标记探针后允许活细胞成像。通过使用常规和超分辨率的成像,我们显示在纳米级的不同生物刺激之上,若干核转录因子(即RNA聚合酶II或TAF10或TAF10)和特异性磷酸化的组蛋白(γH2AX)的动态变化。因此,考虑到大面板的可用抗体和它们实现的简单性,凡民赛可用于基于单一活细胞核中的转录因子或后期改性的动态行为来揭示新的生物信息。

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