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成纤维细胞牵引机制的分子剖析

Molecular dissection of the fibroblast-traction machinery.

作者信息

Sawhney Ravi K, Howard Jonathon

机构信息

Max Planck Institute of Molecular Cell Biology and Genetics, Dresden, Germany.

出版信息

Cell Motil Cytoskeleton. 2004 Jul;58(3):175-85. doi: 10.1002/cm.20004.

Abstract

Motile fibroblasts generate forces that can be expressed as cell migration or as traction, the drawing-in of extracellular matrix. Traction by cultured fibroblasts can induce a rapid concerted reorganization of collagen gel, creating a pattern of collagen alignment similar to that seen in tendons and ligaments. In such fibrous connective tissues, after pattern morphogenesis is complete, ongoing traction may be responsible for the maintenance of proper form and function. The molecules that generate and transmit forces have been catalogued; however, how these nanometer-scale molecules contribute to millimeter-scale patterns has not been directly tested. Here, we placed pairs of explants of human periodontal ligament fibroblasts in collagen gels, where ligament-like straps of anisotropic collagen formed on the axes between them. We scrutinized the traction apparatus using electron microscopy, video microscopy, and computer-based pattern analysis, augmented with pharmacologic inhibitors of cytoskeletal function. Patterning was marked by the co-alignment of collagen, fibroblasts, and their actin cytoskeletons, all parallel to the axis between explants. The pattern was diminished by depolymerizing actin filaments or by blocking myosin activity, but was accentuated by depolymerizing microtubules. The plasma membrane also seems to contribute to the traction force. These molecular components combine to exert a sub-maximal traction force on the matrix, suggesting that the force may be regulated to ensure tissue tensional homeostasis.

摘要

运动性成纤维细胞产生的力可以表现为细胞迁移或牵引,即细胞外基质的内拉。培养的成纤维细胞的牵引可以诱导胶原凝胶快速协同重组,形成与肌腱和韧带中所见相似的胶原排列模式。在这种纤维结缔组织中,模式形态发生完成后,持续的牵引可能负责维持适当的形态和功能。产生和传递力的分子已被分类;然而,这些纳米级分子如何促成毫米级模式尚未得到直接验证。在此,我们将成对的人牙周膜成纤维细胞外植体置于胶原凝胶中,在它们之间的轴上形成了各向异性胶原的韧带样带。我们使用电子显微镜、视频显微镜和基于计算机的模式分析,并辅以细胞骨架功能的药理学抑制剂,仔细研究了牵引装置。模式形成的特征是胶原、成纤维细胞及其肌动蛋白细胞骨架共同排列,均与外植体之间的轴平行。通过使肌动蛋白丝解聚或阻断肌球蛋白活性,模式会减弱,但通过使微管解聚,模式会增强。质膜似乎也有助于牵引力。这些分子成分共同作用,对基质施加次最大牵引力,表明该力可能受到调节以确保组织张力稳态。

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