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细胞黏附、力生成和细胞外蛋白水解在基质重塑中的相互依赖性。

Interdependency of cell adhesion, force generation and extracellular proteolysis in matrix remodeling.

机构信息

German Cancer Research Center Heidelberg (DKFZ), Im Neuenheimer Feld 280, 69120 Heidelberg, Germany.

出版信息

J Cell Sci. 2011 Jun 1;124(Pt 11):1857-66. doi: 10.1242/jcs.079343. Epub 2011 May 10.

DOI:10.1242/jcs.079343
PMID:21558415
Abstract

It is becoming increasingly evident that the micromechanics of cells and their environment determine cell fate and function as much as soluble molecular factors do. We hypothesized that extracellular matrix proteolysis by membrane type 1 matrix metalloproteinase (MT1-MMP) depends on adhesion, force generation and rigidity sensing of the cell. Melanoma cells (MV3 clone) stably transfected with MT1-MMP, or the empty vector as a control, served as the model system. α2β1 integrins (cell adhesion), actin and myosin II (force generation and rigidity sensing) were blocked by their corresponding inhibitors (α2β1 integrin antibodies, Cytochalasin D, blebbistatin). A novel, anisotropic matrix array of parallel, fluorescently labeled collagen-I fibrils was used. Cleavage and bundling of the collagen-I fibrils, and spreading and durotaxis of the cells on this matrix array could be readily discerned and quantified by a combined set-up for fluorescence and atomic force microscopy. In short, expression of the protease resulted in the generation of structural matrix defects, clearly indicated by gaps in the collagen lattice and loose fiber bundles. This key feature of matrix remodeling depended essentially on the functionality of α2β1 integrin, the actin filament network and myosin II motor activity. Interference with any of these negatively impacted matrix cleavage and three-dimensional matrix entanglement of cells.

摘要

越来越明显的是,细胞及其环境的微力学在很大程度上决定了细胞的命运和功能,就像可溶性分子因素一样。我们假设,膜型 1 基质金属蛋白酶(MT1-MMP)对细胞外基质的蛋白水解作用取决于细胞的黏附、力的产生和刚性感知。以黑色素瘤细胞(MV3 克隆)为模型系统,这些细胞稳定转染了 MT1-MMP,或作为对照的空载体。α2β1 整合素(细胞黏附)、肌动蛋白和肌球蛋白 II(力的产生和刚性感知)被其相应的抑制剂(α2β1 整合素抗体、细胞松弛素 D、blebbistatin)阻断。使用了一种新颖的各向异性平行荧光标记胶原 I 原纤维的基质阵列。通过荧光和原子力显微镜的组合设置,很容易识别和量化胶原 I 原纤维的切割和束集,以及细胞在该基质阵列上的扩展和抗刚性迁移。简而言之,蛋白酶的表达导致结构基质缺陷的产生,这在胶原晶格的间隙和松散的纤维束中得到了明显的体现。这种基质重塑的关键特征主要取决于α2β1 整合素、肌动蛋白丝网络和肌球蛋白 II 运动活性的功能。这些因素中的任何一个受到干扰都会对基质切割和细胞的三维基质缠结产生负面影响。

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