首页> 外文期刊>Cell Calcium: The International Interdisciplinary Forum for Research on Calcium >Fully-automated image processing software to analyze calcium traces in populations of single cells.
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Fully-automated image processing software to analyze calcium traces in populations of single cells.

机译:全自动图像处理软件,可分析单细胞群体中的钙痕迹。

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摘要

Advances in fluorescence live cell imaging over the last decade have revolutionized cell biology by providing access to single-cell information in space and time. One current limitation of live-cell imaging is the lack of automated procedures to analyze single-cell data in large cell populations. Most commercially available image processing softwares do not have built-in image segmentation tools that can automatically and accurately extract single-cell data in a time series. Consequently, individual cells are usually identified manually, a process which is time consuming and inherently low-throughput. We have developed a MATLAB-based image segmentation algorithm that reliably detects individual cells in dense populations and measures their fluorescence intensity over time. To demonstrate the value of this algorithm, we measured store-operated calcium entry (SOCE) in hundreds of individual cells. Rapid access to single-cell calcium signals in large populations allowed us to precisely determine the relationship between SOCE activity and STIM1 levels, a key component of SOCE. Our image processing tool can in principle be applied to a wide range of live-cell imaging modalities and cell-based drug screening platforms.
机译:过去十年来,荧光活细胞成像技术的进步通过提供对时空单细胞信息的访问,彻底改变了细胞生物学。活细胞成像的当前限制之一是缺乏自动化程序来分析大细胞群体中的单细胞数据。大多数商用图像处理软件没有内置的图像分割工具,该工具可以自动,准确地提取时间序列中的单细胞数据。因此,通常手动识别单个细胞,这是耗时的并且固有地低通量的过程。我们已经开发了一种基于MATLAB的图像分割算法,该算法可以可靠地检测密集群体中的单个细胞并随时间测量其荧光强度。为了证明该算法的价值,我们在数百个单个细胞中测量了存储操作性钙输入(SOCE)。快速访问大量人群中的单细胞钙信号使我们能够精确确定SOCE活性和STIM1水平(SOCE的关键组成部分)之间的关系。我们的图像处理工具原则上可以应用于各种活细胞成像模式和基于细胞的药物筛选平台。

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