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Integrin-mediated cell adhesion to fibronectin: initial binding and strengthening responses

机译:整合素介导的细胞与纤连蛋白的粘附:初始结合和加强反应

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Cell adhesion to fibronectin involves integrin receptor-ligand binding and adhesion strengthening, which includes integrin clustering, interactions with cytoskeletal components to form focal adhesions, and spreading. Because of the complex nature of the strengthening process, quantitative analyses of cell adhesion have been limited to initial events. In this study, we applied micropatterning methods to control focal adhesion size and decouple focal adhesion assembly from gross changes in cell morphology, allowing for rigorous analysis of adhesion strength independently of cell spreading and redistribution of adhesive structures. Microcontact printing was used to pattern arrays of circular adhesive islands within a non-adhesive background. Fibroblasts adhered to fibronectin-coated islands and remained nearly spherical. The cell-substrate contact area was constrained to the micropatterned domain and immunofluorescence staining revealed robust assembly of adhesive structures containing components associated with conventional focal adhesions. Cell adhesion strength to fibronectin-coated islands was quantified using a spinning disk device. Adhesion strength exhibited significant time- and adhesive area-dependent increases. Comparison of experiments for similar contact areas at different time points showed a 9-fold increase in adhesion strength over time, independently of cell spreading. This work provides an experimental framework for the functional analysis of focal adhesion components in physiological and pathological conditions.
机译:细胞与纤连蛋白的粘附涉及整联蛋白受体-配体的结合和粘附增强,这包括整联蛋白聚集,与细胞骨架成分的相互作用以形成粘着斑和扩散。由于强化过程的复杂性,对细胞粘附的定量分析仅限于初始事件。在这项研究中,我们应用了微图案化方法来控制粘着斑的大小,并使粘着斑的组装与细胞形态的总体变化脱钩,从而能够对粘附强度进行严格的分析,而与细胞的铺展和粘着结构的重新分布无关。微接触印刷用于在非胶粘剂背景下对圆形胶粘剂岛阵列进行图案化。成纤维细胞粘附在被纤连蛋白包被的岛上,并保持接近球形。细胞-底物的接触区域被限制在微图案域,免疫荧光染色揭示了包含与常规粘着相关的成分的粘合剂结构的牢固组装。使用旋转盘装置定量细胞对纤连蛋白包被的岛的粘附强度。粘合强度表现出明显的时间依赖性和粘合面积依赖性。在不同时间点对相似接触区域进行的实验比较表明,粘附强度随时间增长了9倍,而与细胞扩散无关。这项工作为生理和病理条件下的粘着斑成分的功能分析提供了一个实验框架。

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