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角质形成细胞迁移过程中的极性、突出-回缩动力学及其相互作用。

Polarity, protrusion-retraction dynamics and their interplay during keratinocyte cell migration.

作者信息

Libotte T, Kaiser H W, Alt W, Bretschneider T

机构信息

Department of Theoretical Biology, Botanical Institute, University of Bonn, Kirschallee 1, Bonn, D-53115, Germany.

出版信息

Exp Cell Res. 2001 Nov 1;270(2):129-37. doi: 10.1006/excr.2001.5339.

DOI:10.1006/excr.2001.5339
PMID:11640877
Abstract

Keratinocyte migration on a two-dimensional substrate can be split into four distinct phases: cell extension, attachment, contraction, and detachment. It is preceded by polarization of the cell which leads to a functional asymmetry observable by the formation of a leading lamella. In this work variation of fibronectin coating concentrations and competitive inhibition with RGD peptides are used to investigate the dependency of polarization, migration, lamella dynamics, and ruffling on substrate adhesiveness. Looking at migrating human epidermal keratinocytes with a well-defined polarity we find that a fibronectin-coating concentration of 10 microg/cm(2) stimulates migration and ruffling speed twofold, whereas protrusion speed increases only by 20% (compared to 2.5 microg/cm(2) fibronectin). Nonpolar cells show a constant migration and ruffling speed independent of the amount of fibronectin. In contrast protrusion speeds of polar and nonpolar cells are equal. Treatment of cells on 10 microg/cm(2) fibronectin with 1 mg/ml GRGDS reduces the characteristic migration, protrusion, and ruffling speed of polar cells which corresponds to lowering the effective coating concentration to under 5 microg/cm(2). The probability of being polarized (quantified by a polarity index) increases with increasing fibronectin concentration. However, addition of soluble RGD on 10 microg/cm(2) fibronectin does not simply reduce the polarity index like one would expect from the corresponding changes in the other motility parameters, but it remains unchanged.

摘要

角质形成细胞在二维基质上的迁移可分为四个不同阶段

细胞伸展、附着、收缩和脱离。在此之前细胞会发生极化,这会导致通过前缘薄板的形成观察到功能不对称。在这项工作中,使用纤连蛋白包被浓度的变化以及与RGD肽的竞争性抑制来研究极化、迁移、薄板动力学和波动对底物粘附性的依赖性。观察具有明确极性的迁移人表皮角质形成细胞时,我们发现纤连蛋白包被浓度为10微克/平方厘米会使迁移和波动速度提高两倍,而突出速度仅增加20%(与2.5微克/平方厘米的纤连蛋白相比)。非极性细胞的迁移和波动速度恒定,与纤连蛋白的量无关。相比之下,极性和非极性细胞的突出速度相等。用1毫克/毫升GRGDS处理在10微克/平方厘米纤连蛋白上的细胞,会降低极性细胞的特征性迁移、突出和波动速度,这相当于将有效包被浓度降低到5微克/平方厘米以下。极化的概率(通过极性指数量化)随纤连蛋白浓度的增加而增加。然而,在10微克/平方厘米纤连蛋白上添加可溶性RGD并不会像人们从其他运动参数的相应变化所预期的那样简单地降低极性指数,而是保持不变。

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