动态荧光显微镜中粒子的自动跟踪

Daniel Sage, F. Hediger, Susan M. Gasser, M. Unser
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引用次数: 13

摘要

我们提出了一个新的,鲁棒算法跟踪荧光粒子在动态图像序列获得的明场或共聚焦显微镜。具体地说,我们考虑的问题提取染色体端粒的运动在一个芽殖酵母细胞的细胞核内。我们的方法有三个组成部分。第一个是校准模块,补偿在调查的生物结构的运动。在我们的应用中,图像与核的重心对齐,核的重心通过阈值检测并与椭圆拟合。第二步是墨西哥帽滤波,我们证明它最适合于检测分形噪声中的高斯点。最后一个组件是跟踪算法,该算法使用动态规划来提取粒子的最优(x,y,t)轨迹。我们已经将该方法作为公共领域ImageJ软件的Java插件实现。我们将其应用于实际数据,并获得了与手动跟踪一样好的结果。我们的新算法将300幅图像序列的分析时间从手动完成的10分钟减少到几秒钟,并提供了可重复性的好处。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Automatic tracking of particles in dynamic fluorescence microscopy
We present a new, robust algorithm for tracking fluorescent particles in dynamic image sequences obtained by brightfield or confocal microscopy. Specifically, we consider the problem of extracting the movement of chromosomal telomeres within the nucleus of a budding yeast cell. Our method has three components. The first is an alignment module that compensates for the movement of the biological structure under investigation. In our application, the images are aligned to the center of gravity of the nucleus which is detected by thresholding and fitted with an ellipse. The second step is a Mexican-hat filtering which we show to be optimally tailored to the detection of a Gaussian-like spot in fractal noise. The final component is a tracking algorithm that uses dynamic programming to extract the optimal (x,y,t) trajectory of a particle. We have implemented the method as a Java Plugin for the public-domain ImageJ software. We have applied it to real data and have obtained results that are as good - if not better as manual tracings. Our new algorithm reduces the analysis time of a 300 image sequence from 10 minutes, when it is done manually, to just a few seconds and offers the benefit of reproducibility.
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