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细胞与纤连蛋白和腱生蛋白的黏附:初始结合及后续强化反应的定量测定

Cell adhesion to fibronectin and tenascin: quantitative measurements of initial binding and subsequent strengthening response.

作者信息

Lotz M M, Burdsal C A, Erickson H P, McClay D R

机构信息

Department of Zoology, Duke University, Durham, North Carolina 27706.

出版信息

J Cell Biol. 1989 Oct;109(4 Pt 1):1795-805. doi: 10.1083/jcb.109.4.1795.

Abstract

Cell-substratum adhesion strengths have been quantified using fibroblasts and glioma cells binding to two extracellular matrix proteins, fibronectin and tenascin. A centrifugal force-based adhesion assay was used for the adhesive strength measurements, and the corresponding morphology of the adhesions was visualized by interference reflection microscopy. The initial adhesions as measured at 4 degrees C were on the order of 10(-5)dynes/cell and did not involve the cytoskeleton. Adhesion to fibronectin after 15 min at 37 degrees C were more than an order of magnitude stronger; the strengthening response required cytoskeletal involvement. By contrast to the marked strengthening of adhesion to FN, adhesion to TN was unchanged or weakened after 15 min at 37 degrees C. The absolute strength of adhesion achieved varied according to protein and cell type. When a mixed substratum of fibronectin and tenascin was tested, the presence of tenascin was found to reduce the level of the strengthening of cell adhesion normally observed at 37 degrees C on a substratum of fibronectin alone. Parallel analysis of corresponding interference reflection micrographs showed that differences in the area of cell surface within 10-15 nm of the substratum correlated closely with each of the changes in adhesion observed: after incubation for 15 min on fibronectin at 37 degrees C, glioma cells increased their surface area within close contact to the substrate by integral to 125-fold. Cells on tenascin did not increase their surface area of contact. The increased surface area of contact and the inhibitory activity of cytochalasin b suggest that the adhesive "strengthening" in the 15 min after initial binding brings additional adhesion molecules into the adhesive site and couples the actin cytoskeleton to the adhesion complex.

摘要

利用成纤维细胞和胶质瘤细胞与两种细胞外基质蛋白(纤连蛋白和腱生蛋白)的结合,对细胞与基质的黏附强度进行了量化。采用基于离心力的黏附试验来测量黏附强度,并通过干涉反射显微镜观察黏附的相应形态。在4℃下测量的初始黏附力约为10^(-5)达因/细胞,且不涉及细胞骨架。在37℃下孵育15分钟后,与纤连蛋白的黏附力增强了一个多数量级;这种增强反应需要细胞骨架的参与。与对纤连蛋白黏附力的显著增强形成对比的是,在37℃下孵育15分钟后,与腱生蛋白的黏附力未发生变化或减弱。所达到的黏附绝对强度因蛋白质和细胞类型而异。当测试纤连蛋白和腱生蛋白的混合基质时,发现腱生蛋白的存在会降低通常在37℃下在仅含纤连蛋白的基质上观察到的细胞黏附增强水平。对相应干涉反射显微照片的平行分析表明,基质表面10 - 15纳米内细胞表面面积的差异与观察到的每种黏附变化密切相关:在37℃下于纤连蛋白上孵育15分钟后,胶质瘤细胞与底物紧密接触的表面积整体增加了125倍。在腱生蛋白上的细胞未增加其接触表面积。接触表面积的增加以及细胞松弛素b的抑制活性表明,初始结合后15分钟内黏附的“增强”将额外的黏附分子带入黏附位点,并将肌动蛋白细胞骨架与黏附复合物相连。

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