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A tapered channel microfluidic device for comprehensive cell adhesion analysis, using measurements of detachment kinetics and shear stress-dependent motion

机译:用于分离细胞动力学和剪切应力相关运动的测量的锥形通道微流体装置,用于全面的细胞粘附分析

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摘要

We have developed a method for studying cellular adhesion by using a custom-designed microfluidic device with parallel non-connected tapered channels. The design enables investigation of cellular responses to a large range of shear stress (ratio of 25) with a single input flow-rate. For each shear stress, a large number of cells are analyzed (500–1500 cells), providing statistically relevant data within a single experiment. Besides adhesion strength measurements, the microsystem presented in this paper enables in-depth analysis of cell detachment kinetics by real-time videomicroscopy. It offers the possibility to analyze adhesion-associated processes, such as migration or cell shape change, within the same experiment. To show the versatility of our device, we examined quantitatively cell adhesion by analyzing kinetics, adhesive strength and migration behaviour or cell shape modifications of the unicellular model cell organism Dictyostelium discoideum at 21 °C and of the human breast cancer cell line MDA-MB-231 at 37 °C. For both cell types, we found that the threshold stresses, which are necessary to detach the cells, follow lognormal distributions, and that the detachment process follows first order kinetics. In addition, for particular conditions’ cells are found to exhibit similar adhesion threshold stresses, but very different detachment kinetics, revealing the importance of dynamics analysis to fully describe cell adhesion. With its rapid implementation and potential for parallel sample processing, such microsystem offers a highly controllable platform for exploring cell adhesion characteristics in a large set of environmental conditions and cell types, and could have wide applications across cell biology, tissue engineering, and cell screening.
机译:我们已经开发出一种通过使用具有平行非连接锥形通道的定制设计的微流体装置来研究细胞粘附的方法。该设计能够以单个输入流速研究细胞对大范围剪切应力(比率为25)的响应。对于每个剪切应力,将分析大量单元(500–1500个单元),从而在单个实验中提供统计上相关的数据。除了粘附强度测量外,本文介绍的微系统还可以通过实时视频显微镜对细胞分离动力学进行深入分析。它提供了在同一实验中分析与粘附相关的过程(例如迁移或细胞形状变化)的可能性。为了展示我们设备的多功能性,我们通过分析21°C下单细胞模型细胞生物盘基网柄菌和人类乳腺癌细胞系MDA-MB-的动力学,粘附强度和迁移行为或细胞形状修饰,定量检查了细胞粘附性在37°C时为231。对于这两种细胞类型,我们发现分离细胞所必需的阈值应力遵循对数正态分布,并且分离过程遵循一阶动力学。此外,发现在特定条件下,细胞表现出相似的粘附阈值应力,但分离动力学却大不相同,这揭示了进行动力学分析以充分描述细胞粘附的重要性。凭借其快速实施和并行样品处理的潜力,这种微系统提供了一个高度可控的平台,用于在大量环境条件和细胞类型中探索细胞粘附特性,并且可能在细胞生物学,组织工程和细胞筛选中得到广泛应用。

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