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Method and System for Acquisition of Fluorescence Images of Live-cell Biological Samples

机译:获取活细胞生物样品荧光图像的方法和系统

摘要

A method is disclosed for acquiring a single, in-focus two-dimensional projection image of a live, three-dimensional cell culture sample, with a fluorescence microscope. One or more long-exposure “Z-sweep” images are obtained, i.e. via a single or series of continuous acquisitions, while moving the Z-focal plane of a camera through the sample, to produce one or more two-dimensional images of fluorescence intensity integrated over the Z-dimension. The acquisition method is much faster than a Z-stack method, which enables higher throughput and reduces the risk of exposing the sample to too much fluorescent light. The long-exposure Z-sweep image(s) is then input into a neural network which has been trained to produce a high-quality (in-focus) two-dimensional projection image of the sample. With these high-quality projection images, biologically relevant analysis metrics can be obtained to describe the fluorescence signal using standard image analysis techniques, such as fluorescence object count and other fluorescence intensity metrics (e.g., mean intensity, texture, etc.).
机译:公开了一种用荧光显微镜获取活的三维细胞培养样品的单个,焦细胞培养样品的单个,焦细胞培养样品的单一,焦细胞投影图像。获得一个或多个长曝光“Z-Sweep”图像,即通过单个或一系列连续采集,同时通过样本移动相机的Z焦平面,以产生一个或多个荧光的二维图像强度集成在z维上。采集方法比Z堆栈方法快得多,这使得能够更高的吞吐量并降低将样品暴露于太多荧光的风险。然后将长时间曝光Z-SweeP图像输入到已经训练的神经网络中以产生样本的高质量(焦点)二维投影图像。利用这些高质量投影图像,可以获得生物相关的分析度量来描述使用标准图像分析技术的荧光信号,例如荧光对象计数和其他荧光强度度量(例如,平均强度,质地等)。

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