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Imaging quantification and visualization of spatio-temporal patterning in mESC colonies under different culture conditions

机译:不同培养条件下mESC菌落的时空格局的成像定量和可视化

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摘要

>Motivation: Mouse embryonic stem cells (mESCs) have developed into a prime system to study the regulation of pluripotency in stable cell lines. It is well recognized that different, established protocols for the maintenance of mESC pluripotency support morphologically and functionally different cell cultures. However, it is unclear how characteristic properties of cell colonies develop over time and how they are re-established after cell passage depending on the culture conditions. Furthermore, it appears that cell colonies have an internal structure with respect to cell size, marker expression or biomechanical properties, which is not sufficiently understood. The analysis of these phenotypic properties is essential for a comprehensive understanding of mESC development and ultimately requires a bioinformatics approach to guarantee reproducibility and high-throughput data analysis.>Results: We developed an automated image analysis and colony tracking framework to obtain an objective and reproducible quantification of structural properties of cell colonies as they evolve in space and time. In particular, we established a method that quantifies changes in colony shape and (internal) motion using fluid image registration and image segmentation. The methodology also allows to robustly track motion, splitting and merging of colonies over a sequence of images. Our results provide a first quantitative assessment of temporal mESC colony formation and estimates of structural differences between colony growth under different culture conditions. Furthermore, we provide a stream-based visualization of structural features of individual colonies over time for the whole experiment, facilitating visual comprehension of differences between experimental conditions. Thus, the presented method establishes the basis for the model-based analysis of mESC colony development. It can be easily extended to integrate further functional information using fluorescence signals and differentiation markers.>Availability: The analysis tool is implemented C++ and Mathematica 8.0 (Wolfram Research Inc., Champaign, IL, USA). The tool is freely available from the authors. We will also provide the source code upon request.>Contact:
机译:>动机:小鼠胚胎干细胞(mESCs)已发展成为研究稳定细胞系中多能性调控的主要系统。众所周知,维持mESC多能性的不同既定方案在形态和功能上支持不同的细胞培养。但是,尚不清楚细胞集落的特性如何随时间发展,以及如何根据培养条件在细胞传代后重新建立。此外,似乎细胞集落具有关于细胞大小,标志物表达或生物力学性质的内部结构,这还没有被充分理解。这些表型特性的分析对于全面了解mESC的发展至关重要,最终需要一种生物信息学方法来保证可重复性和高通量数据分析。>结果:我们开发了自动图像分析和菌落跟踪框架在细胞集落的时空演化过程中获得客观,可重复的结构性量化。特别是,我们建立了一种使用流体图像配准和图像分割来量化菌落形状和(内部)运动变化的方法。该方法还允许在一系列图像上稳健地跟踪运动,菌落的分裂和合并。我们的结果提供了对第一时间mESC集落形成的首次定量评估,并估计了不同培养条件下集落生长之间的结构差异。此外,我们在整个实验过程中提供了基于流的单个菌落结构特征随时间变化的可视化,有助于直观理解实验条件之间的差异。因此,本文提出的方法为基于模型的mESC菌落发育分析奠定了基础。它可以很容易地扩展以使用荧光信号和分化标记物整合更多的功能信息。>可用性:分析工具使用C ++和Mathematica 8.0(Wolfram Research Inc.,美国,伊利诺伊州,香槟)实施。该工具可从作者处免费获得。我们还将根据要求提供源代码。>联系方式:

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