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Visualization of subdiffusive sites in a live single cell

机译:在活单细胞中沉闷的网站的可视化

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We measured anomalous diffusion in human prostate cancer cells which were transfected with the Alexa633 fluorescent RNA probe and co-transfected with enhanced green fluorescent protein-labeled argonaute2 protein by laser scanning microscopy. The image analysis arose from diffusion based on a “two-level system”. A trap was an interaction site where the diffusive motion was slowed down. Anomalous subdiffusive spreading occurred at cellular traps. The cellular traps were not immobile. We showed how the novel analysis method of imaging data resulted in new information about the number of traps in the crowded and heterogeneous environment of a single human prostate cancer cell. The imaging data were consistent with and explained by our modern ideas of anomalous diffusion of mixed origins in live cells. Our original research presented in this study is significant as we obtained a complex diffusion mechanism in live single cells.
机译:我们在人前列腺癌细胞中测量了异常的扩散,其用Alexa633荧光RNA探针转染,并通过激光扫描显微镜用增强的绿色荧光蛋白标记的Argonaute2蛋白转染。 基于“两级系统”,图像分析从扩散产生。 陷阱是互动部位,漫游动作减慢了。 细胞疏水阀发生异常的副屈光度蔓延。 细胞捕集物不是不动的。 我们展示了如何进行成像数据的新型分析方法,导致关于单个人前列腺癌细胞的拥挤和异质环境中的陷阱数量的新信息。 成像数据符合我们的现代化混合起源在活细胞中的现代思想。 我们在本研究中提出的原始研究是显着的,因为我们在活单细胞中获得了复杂的扩散机制。

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