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首页> 外文期刊>The Journal of Chemical Physics >A method for single molecule tracking using a conventional single-focus confocal setup
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A method for single molecule tracking using a conventional single-focus confocal setup

机译:一种使用传统的单焦共聚焦设置的单分子跟踪方法

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摘要

One way to achieve spatial resolution using fluorescence imaging-and track single molecules-is to use wide-field illumination and collect measurements over multiple sensors (camera pixels). Here we propose another way that uses confocal measurements and a single sensor. Traditionally, confocal microscopy has been used to achieve high temporal resolution at the expense of spatial resolution. This is because it utilizes very few, and commonly just one, sensors to collect data. Yet confocal data encode spatial information. Here we show that nonuniformities in the shape of the confocal excitation volume can be exploited to achieve spatial resolution. To achieve this, we formulate a specialized hidden Markov model and adapt a forward filtering-backward sampling Markov chain Monte Carlo scheme to efficiently handle molecular motion within a symmetric confocal volume characteristically used in fluorescence correlation spectroscopy. Our method can be used for single confocal volume applications or incorporated into larger computational schemes for specialized, multi-confocal volume, optical setups. Published under license by AIP Publishing.
机译:使用荧光成像实现空间分辨率的一种方法 - 以及跟踪单分子 - 是使用宽场照明并通过多个传感器(相机像素)收集测量。在这里,我们提出了一种使用共聚焦测量和单个传感器的另一种方式。传统上,共聚焦显微镜已经用于以牺牲空间分辨率为代价来实现高的时间分辨率。这是因为它利用很少,通常只是一个传感器来收集数据。然而,共焦数数据编码空间信息。在这里,我们表明可以利用共聚焦励磁体积形状的不均匀性以实现空间分辨率。为此,我们制定了专用隐马尔可夫模型,并适应前向返回后向采样马尔本蒙特卡罗方案,以有效地处理特征在荧光相关光谱中的对称共焦体积内的分子运动。我们的方法可用于单个共焦体积应用,或者包含专门的多个共聚焦体积,光学设置的较大计算方案。通过AIP发布在许可证下发布。

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