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Spatiotemporal Analysis of Cell Response to a Rigidity Gradient: A Quantitative Study Using Multiple Optical Tweezers

机译:时空分析细胞对刚性梯度的响应:使用多个光学镊子的定量研究。

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摘要

We investigate the dynamic response of single cells to weak and local rigidities, applied at controlled adhesion sites. Using multiple latex beads functionalized with fibronectin, and each trapped in its own optical trap, we study the reaction in real time of single 3T3 fibroblast cells to asymmetrical tensions in the tens of pN · μm−1 range. We show that the cell feels a rigidity gradient even at this low range of tension, and over time develops an adapted change in the force exerted on each adhesion site. The rate at which force increases is proportional to trap stiffness. Actomyosin recruitment is regulated in space and time along the rigidity gradient, resulting in a linear relationship between the amount of recruited actin and the force developed independently in trap stiffness. This time-regulated actomyosin behavior sustains a constant and rigidity-independent velocity of beads inside the traps. Our results show that the strengthening of extracellular matrix-cytoskeleton linkages along a rigidity gradient is regulated by controlling adhesion area and actomyosin recruitment, to maintain a constant deformation of the extracellular matrix.
机译:我们研究了单细胞对弱和局部刚性的动态响应,在受控的粘附位点应用。我们使用被纤连蛋白功能化的多个乳胶珠,每个珠都被困在自己的光阱中,我们实时研究了单个3T3成纤维细胞对数十pN·μm -1 范围内的不对称张力的反应。我们表明,即使在这种低张力范围内,电池也能感觉到刚度梯度,并且随着时间的流逝,在每个粘附部位上施加的力都会发生适应性变化。力增加的速度与捕集阱的刚度成正比。肌动球蛋白的募集在空间和时间上沿着刚度梯度进行调节,从而导致募集的肌动蛋白的量与捕集阱刚度中独立产生的力之间呈线性关系。这种时间调节的肌动球蛋白行为维持了捕集器内珠子的恒定且不依赖于刚度的速度。我们的结果表明,通过控制粘附面积和肌动球蛋白募集,维持细胞外基质的恒定变形,可以调节沿刚性梯度增强的细胞外基质与细胞骨架之间的联系。

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