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Actin and microtubule networks contribute differently to cell response for small and large strains

机译:肌动蛋白和微管网络对大小菌株的细胞反应的贡献不同

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摘要

Cytoskeletal filaments provide cells with mechanical stability and organization. The main key players are actin filaments and microtubules governing a cell's response to mechanical stimuli. We investigated the specific influences of these crucial components by deforming MCF-7 epithelial cells at small (≤5% deformation) and large strains (>5% deformation). To understand specific contributions of actin filaments and microtubules, we systematically studied cellular responses after treatment with cytoskeleton influencing drugs. Quantification with the microfluidic optical stretcher allowed capturing the relative deformation and relaxation of cells under different conditions. We separated distinctive deformational and relaxational contributions to cell mechanics for actin and microtubule networks for two orders of magnitude of drug dosages. Disrupting actin filaments via latrunculin A, for instance, revealed a strain-independent softening. Stabilizing these filaments by treatment with jasplakinolide yielded cell softening for small strains but showed no significant change at large strains. In contrast, cells treated with nocodazole to disrupt microtubules displayed a softening at large strains but remained unchanged at small strains. Stabilizing microtubules within the cells via paclitaxel revealed no significant changes for deformations at small strains, but concentration-dependent impact at large strains. This suggests that for suspended cells, the actin cortex is probed at small strains, while at larger strains; the whole cell is probed with a significant contribution from the microtubules.
机译:细胞骨架细丝为细胞提供机械稳定性和组织性。主要的关键参与者是肌动蛋白丝和微管,它们控制细胞对机械刺激的反应。我们通过使MCF-7上皮细胞变形小(≤5%变形)和大应变(> 5%变形)来研究这些关键成分的特定影响。为了了解肌动蛋白丝和微管的特定作用,我们系统地研究了受细胞骨架影响药物治疗后的细胞反应。用微流态光学担架定量可以捕获不同条件下细胞的相对变形和松弛。我们将肌动蛋白和微管网络对细胞力学的独特的变形和松弛贡献分为两个数量级的药物剂量。例如,通过latrunculin A破坏肌动蛋白丝可显示出与应变无关的软化作用。通过用jasplakinolide处理来稳定这些细丝,可以使小菌株的细胞软化,但在大菌株中却没有显示出明显的变化。相反,用诺考达唑处理以破坏微管的细胞在大菌株下显示出软化,而在小菌株下保持不变。通过紫杉醇稳定细胞内的微管显示,小菌株的变形没有明显变化,但大菌株的浓度依赖性影响。这表明对于悬浮细胞,肌动蛋白皮层是在小应变时探测的,而在大应变时探测的。整个细胞被微管显着贡献。

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