兔滑膜成纤维细胞的细胞骨架动力学:II。胶原酶诱导剂处理后圆形细胞中应力纤维的改造。

J Aggeler
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引用次数: 18

摘要

兔滑膜成纤维细胞调控细胞外基质蛋白和基质降解金属蛋白酶的合成和分泌是研究组织特异性基因表达调控的重要模型系统。胶原酶表达的诱导与细胞形状和肌动蛋白丝分布的变化有关,但细胞骨架在金属蛋白酶的持续合成和分泌中的作用尚未得到仔细研究。当细胞被胰蛋白酶或细胞松弛素(两种已知的金属蛋白酶诱导剂)包围后再增殖时,在血清存在的情况下,2小时内观察到应力纤维的重组。在没有血清的情况下,胰蛋白酶处理的细胞即使在培养24小时后也没有明显的复制。相比之下,细胞松弛素处理的细胞在没有血清的情况下恢复的速度几乎与有血清的情况一样快,在药物去除后30分钟内,形成良好的微丝束重建,尤其是在扩散的细胞边缘。洗涤剂提取的细胞骨架的高分辨率电子显微镜视图证实了外周微丝的快速重新捆绑。丙烯酰胺处理的细胞介于这两个极端之间,在没有血清的情况下扩散缓慢,但在有血清的情况下几乎与细胞松弛素处理的细胞一样快。在所有处理中,正常中间丝分布的重建通常略落后于肌动蛋白,中间丝总是在重组的周围微丝束的范围内扩散回细胞质中。在任何处理后,这两种细胞骨架元件之间没有明显的相互作用,这些结果也没有表明中间丝在这些细胞中调节基因表达的特定作用。胰蛋白酶或丙烯酰胺处理后表现出的血清依赖性可能是由于在这些细胞中观察到的纤维连接蛋白合成紊乱,这与基质降解金属蛋白酶的诱导和持续表达可能涉及通过质膜基质受体(整合素)转导的信号的证据一致。
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Cytoskeletal dynamics in rabbit synovial fibroblasts: II. Reformation of stress fibers in cells rounded by treatment with collagenase-inducing agents.

Modulation of the synthesis and secretion of extracellular matrix proteins and matrix-degrading metalloproteases by rabbit synovial fibroblasts is an important model system for studying the control of tissue-specific gene expression. Induction of collagenase expression is correlated with changes in cell shape and actin filament distribution, but the role of the cellular cytoskeleton in the sustained synthesis and secretion of metalloproteases has not been closely examined. When cells were allowed to respread after rounding by trypsin or cytochalasin, two known metalloprotease inducers, reformation of stress fibers was observed within 2 h in the presence of serum. In the absence of serum, trypsin-treated cells did not respread substantially, even after 24 h in culture. In contrast, cytochalasin-treated cells recovered almost as rapidly in the absence as in the presence of serum, showing reformation of well-formed microfilament bundles within 30 min of drug removal, especially at the spreading cell edges. High resolution electron-microscopic views of detergent-extracted cytoskeletons confirmed the rapid rebundling of peripheral microfilaments. Acrylamide-treated cells fell between these two extremes, spreading slowly in the absence of serum, but almost as rapidly as cytochalasin-treated cells in its presence. Reestablishment of normal intermediate filament distribution generally lagged slightly behind actin for all treatments, and intermediate filaments always appeared to spread back into the cellular cytoplasm within the confines of the reforming peripheral microfilament bundles. No obvious interaction between these two cytoskeletal elements was observed after any treatment, and no specific role for intermediate filaments in modulating gene expression in these cells is suggested by these results. The serum dependence displayed after trypsin or acrylamide treatment may be due to the disturbances in fibronectin synthesis observed in these cells and is consistent with evidence that both induction and sustained expression of matrix-degrading metalloprotease may involve signals transduced through plasma membrane matrix receptors (integrins).

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