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Signal and Noise Modeling in Confocal Laser Scanning Fluorescence Microscopy

机译:共焦激光扫描荧光显微镜中的信号和噪声建模

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Fluorescence confocal laser scanning microscopy (CLSM) has revolutionized imaging of subcellular structures in biomedical research by enabling the acquisition of 3D time-series of fluorescently-tagged proteins in living cells, hence forming the basis for an automated quantification of their morphological and dynamic characteristics. Due to the inherently weak fluorescence, CLSM images exhibit a low SNR. We present a novel model for the transfer of signal and noise in CLSM that is both theoretically sound as well as corroborated by a rigorous analysis of the pixel intensity statistics via measurement of the 3D noise power spectra, signal-dependence and distribution. Our model provides a better fit to the data than previously proposed models. Further, it forms the basis for (i) the simulation of the CLSM imaging process indispensable for the quantitative evaluation of CLSM image analysis algorithms, (ii) the application of Poisson denoising algorithms and (iii) the reconstruction of the fluorescence signal.
机译:荧光共聚焦激光扫描显微镜(CLSM)通过实现活细胞中荧光标记蛋白的3D时间序列的采集,彻底改变了生物医学研究中亚细胞结构的成像方法,从而为自动定量其形态和动态特征奠定了基础。由于固有的弱荧光,CLSM图像显示出低SNR。我们提出了一种在CLSM中传输信号和噪声的新颖模型,该模型在理论上是合理的,并且通过对3D噪声功率谱,信号相关性和分布的测量对像素强度统计数据进行了严格的分析,从而得到了证实。与先前提出的模型相比,我们的模型对数据的拟合更好。此外,它为(i)定量评估CLSM图像分析算法必不可少的CLSM成像过程,(ii)泊松去噪算法的应用以及(iii)荧光信号的重建奠定了基础。

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