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Combining AFM and Acoustic Probes to Reveal Changes in the Elastic Stiffness Tensor of Living Cells

机译:结合原子力显微镜和声学探针揭示活细胞的弹性刚度张量的变化

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摘要

Knowledge of how the elastic stiffness of a cell affects its communication with its environment is of fundamental importance for the understanding of tissue integrity in health and disease. For stiffness measurements, it has been customary to quote a single parameter quantity, e.g., Young’s modulus, rather than the minimum of two terms of the stiffness tensor required by elasticity theory. In this study, we use two independent methods (acoustic microscopy and atomic force microscopy nanoindentation) to characterize the elastic properties of a cell and thus determine two independent elastic constants. This allows us to explore in detail how the mechanical properties of cells change in response to signaling pathways that are known to regulate the cell’s cytoskeleton. In particular, we demonstrate that altering the tensioning of actin filaments in NIH3T3 cells has a strong influence on the cell's shear modulus but leaves its bulk modulus unchanged. In contrast, altering the polymerization state of actin filaments influences bulk and shear modulus in a similar manner. In addition, we can use the data to directly determine the Poisson ratio of a cell and show that in all cases studied, it is less than, but very close to, 0.5 in value.
机译:了解细胞的弹性刚度如何影响其与环境的通讯对于了解健康和疾病中的组织完整性至关重要。对于刚度测量,习惯上引用单个参数量(例如,杨氏模量),而不是引用弹性理论要求的刚度张量的最小两项。在这项研究中,我们使用两种独立的方法(声学显微镜和原子力显微镜纳米压痕)来表征细胞的弹性,从而确定两个独立的弹性常数。这使我们能够详细探讨细胞的机械特性如何响应已知调节细胞骨架的信号传导途径而变化。特别是,我们证明了改变NIH3T3细胞中肌动蛋白丝的张力对细胞的剪切模量有很大影响,但其体积模量保持不变。相反,改变肌动蛋白丝的聚合状态以类似的方式影响体积和剪切模量。此外,我们可以使用数据直接确定单元的泊松比,并显示在所有研究的情况下,该值均小于但非常接近0.5。

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