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Single-molecule localization software applied to photon counting imaging

机译:单分子定位软件应用于光子计数成像

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摘要

Centroiding in photon counting imaging has traditionally been accomplished by a single-step, noniterative algorithm, often implemented in hardware. Single-molecule localization techniques in superresolution fluorescence microscopy are conceptually similar, but use more sophisticated iterative software-based fitting algorithms to localize the fluorophore. Here, we discuss common features and differences between single-molecule localization and photon counting imaging and investigate the suitability of single-molecule localization software for photon event localization. We find that single-molecule localization software packages designed for superresolution microscopy-QuickPALM, rapidSTORM, and ThunderSTORM-can work well when applied to photon counting imaging with amicrochannel-plate-based intensified camera system: photon event recognition can be excellent, fixed pattern noise can be low, and the microchannel plate pores can easily be resolved. (C) 2015 Optical Society of America
机译:传统上,光子计数成像中的质心化是通过通常在硬件中实现的单步非迭代算法来完成的。超分辨率荧光显微镜中的单分子定位技术在概念上相似,但是使用更复杂的基于迭代软件的拟合算法来定位荧光团。在这里,我们讨论单分子定位和光子计数成像之间的共同特征和区别,并研究单分子定位软件对光子事件定位的适用性。我们发现,专为超分辨率显微镜而设计的单分子定位软件包QuickPALM,rapidSTORM和ThunderSTORM,在基于微通道板的增强相机系统应用于光子计数成像时,可以很好地发挥作用:光子事件识别可以提供出色的固定模式噪声含量低,并且微通道板的孔很容易解决。 (C)2015年美国眼镜学会

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