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Quantitative measurement of cell migration using time-lapse videomicroscopy and non-linear system analysis

机译:使用延时视频显微镜和非线性系统分析对细胞迁移进行定量测量

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Epithelial cells of the mammary gland possess the inherent capacity to form epithelial monolayers in vitro. This requires coordination of cell migration, cell-cell contact formation, and cell proliferation. Using time-lapse phase contrast videomicroscopy we have observed mammary gland epithelial cells over different time scales. We show the generation of a complete polarized epithelial monolayer in real-time, starting from a few cells. We subsequently concentrated on the early stages of this process by tracking epithelial cells during phases of polarized migration. We performed migration analysis using fractal measures. With this technology the structure of seemingly random processes not accessible to the usual methods of linear analysis can be measured. As a control and proof of principle approach we applied infection of cells with an adenoviral vector, which is used as a gene targeting vector for many applications. Infection markedly influenced the patterns of migratory behavior. We, therefore, believe that time-lapse videomicroscopy in combination with fractal analysis can contribute to differential characterization of distinct cellular migration patterns. This will be useful in situations of long-term alterations in cell culture systems.
机译:乳腺的上皮细胞具有在体外形成上皮单层的固有能力。这需要协调细胞迁移,细胞间接触形成和细胞增殖。使用延时相衬视频显微镜,我们观察了不同时间尺度的乳腺上皮细胞。我们显示了从几个细胞开始实时完整极化的上皮单层的生成。随后,我们通过在极化迁移阶段追踪上皮细胞,集中研究了该过程的早期阶段。我们使用分形测量进行了迁移分析。使用这种技术,可以测量看似随机过程的结构,而线性分析的常规方法无法访问这些过程。作为控制和原理证明的方法,我们应用了腺病毒载体对细胞的感染,该载体被用作许多应用中的基因靶向载体。感染明显影响了迁徙行为的方式。因此,我们认为,延时视频显微镜与分形分析相结合可以促进不同细胞迁移模式的差异表征。这在细胞培养系统中长期变化的情况下将很有用。

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