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Temporal Filtering to Improve Single Molecule Identification in High Background Samples

机译:时间滤波可改善高背景样品中的单分子鉴定

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摘要

Single molecule localization microscopy is currently revolutionizing the life sciences as it offers, for the first time, insights into the organization of biological samples below the classical diffraction limit of light microscopy. While there have been numerous examples of new biological findings reported in the last decade, the technique could not reach its full potential due to a set of limitations immanent to the samples themselves. Particularly, high background signals impede the proper performance of most single-molecule identification and localization algorithms. One option is to exploit the characteristic blinking of single molecule signals, which differs substantially from the residual brightness fluctuations of the fluorescence background. To pronounce single molecule signals, we used a temporal high-pass filtering in Fourier space on a pixel-by-pixel basis. We evaluated the performance of temporal filtering by assessing statistical parameters such as true positive rate and false discovery rate. For this, ground truth signals were generated by simulations and overlaid onto experimentally derived movies of samples with high background signals. Compared to the nonfiltered case, we found an improvement of the sensitivity by up to a factor 3.5 while no significant change in the localization accuracy was observable.
机译:单分子定位显微镜技术目前正在彻底改变生命科学,因为它首次提供了对低于光学显微镜经典衍射极限的生物样品组织的见解。尽管在过去十年中报道了许多新的生物学发现的例子,但由于样品本身固有的一系列限制,该技术无法发挥其全部潜力。特别是,高背景信号会阻碍大多数单分子识别和定位算法的正常运行。一种选择是利用单分子信号的特征闪烁,这与荧光背景的残留亮度波动大不相同。为了发出单分子信号,我们在傅里叶空间中逐像素使用了时间高通滤波。我们通过评估统计参数(例如真实阳性率和错误发现率)来评估时间过滤的性能。为此,通过仿真生成了地面真实信号,并将其叠加到具有高背景信号的样本的实验得出的影片上。与未过滤的情况相比,我们发现灵敏度提高了3.5倍,而定位精度没有明显变化。

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