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madSTORM: a superresolution technique for large-scale multiplexing at single-molecule accuracy

机译:madSTORM:一种超分辨率技术,用于以单分子精度进行大规模多路复用

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摘要

Investigation of heterogeneous cellular structures using single-molecule localization microscopy has been limited by poorly defined localization accuracy and inadequate multiplexing capacity. Using fluorescent nanodiamonds as fiducial markers, we define and achieve localization precision required for single-molecule accuracy in dSTORM images. Coupled with this advance, our new multiplexing strategy, madSTORM, allows accurate targeting of multiple molecules using sequential binding and elution of fluorescent antibodies. madSTORM is used on an activated T-cell to localize 25 epitopes, 14 of which are on components of the same multimolecular T-cell receptor complex. We obtain an average localization precision of 2.6 nm, alignment error of 2.0 nm, and < 0.01% cross-talk. Combining these technical advances affords the ability to move beyond obtaining superresolved structures to defining spatial relationships among constituent molecules within structures. Probing the molecular topology of complex signaling cascades and other heterogeneous networks is feasible with madSTORM.
机译:使用单分子定位显微镜研究异质细胞结构受到局限性的定位精度和多路复用能力不足的限制。使用荧光纳米金刚石作为基准标记,我们定义并实现了dSTORM图像中单分子精度所需的定位精度。结合这一进步,我们新的多路复用策略madSTORM可使用顺序结合和荧光抗体洗脱来精确靶向多个分子。 madSTORM用于激活的T细胞上,以定位25个表位,其中14个位于同一多分子T细胞受体复合物的成分上。我们获得的平均定位精度为2.6 nm,对准误差为2.0 nm,串扰<0.01%。结合这些技术进步,提供了超越获得超分辨结构而定义结构内组成分子之间空间关系的能力。使用madSTORM可以探测复杂的信号级联和其他异构网络的分子拓扑。

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