Dissociation of Actin Microfilament Organization from Acquisition and Maintenance of Elongated Shape of Human Dermal Fibroblasts in Three-Dimensional Collagen Gel

Matrix (Stuttgart, Germany) Pub Date : 1993-11-01 DOI:10.1016/S0934-8832(11)80111-3

Toshio Nishiyama , Makoto Tsunenaga , Nobuko Akutsu , Izumi Horii , Yasuhisa Nakayama , Eijiro Adachi , Masayuki Yamato , Toshihiko Hayashi

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引用次数: 24

Abstract

Actin micro filaments of the fibroblasts cultured in a collagen gel were distributed along the inner surface of the entire cell membrane, in either spherical shape at an initial stage of culture or elongated shape at a later stage. The distribution was quite different from that of the fibroblast cultured on a two-dimensional surface, where actin microfilaments were found to be aligned essentially along the inner membrane which is in contact with a flat surface. Timing of morphological change from spherical shape to spread shape or elongated shape was also greatly affected by contact with substrates whether in two-dimension or in three-dimension: distinct morphological change was observed within 6 h on glass or on the collagen gel, and at 30 h or later within the collagen gel. The retardation of cell elongation in the gel was antagonized by a low dose (0.2 µM) of cytochalasin D, although the drug kept the cells in round shape at a concentration of 2 µM. Since a low concentration of cytochalasin was reported to induce actin polymerization in vitro, the organization of actin micro filaments was examined by rhodamine-phalloidin staining. It was found that actin filaments in elongated cells by low cytochalasin D were disrupted. These results suggest that accelerated acquisition of elongated shape by the treatment of a low dose of cytochalasin D might be initiated by destabilization of the actin microfilaments that may scaffold the spherical shape of the cell in the collagen gel. The elongated shape thus formed returned to spherical upon washing of the added free cytochalasin D. This is not the case with the elongated cells which had been established by a prolonged culture such as 40 h after starting the culture in the gel. That is, addition of cytochalasin D at a highest dose of 2.0 µM did not change the elongated shape in spite of the complete disruption of actin micro filaments of the fibroblasts. These findings suggest that actin microfilament organization is not actively involved in, or dissociated from, acquisition and maintenance of elongated shape of fibroblasts in the collagen gel.

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三维胶原凝胶中肌动蛋白微丝组织与人皮肤成纤维细胞获得和维持细长形状的分离

胶原凝胶培养成纤维细胞的肌动蛋白微丝沿整个细胞膜内表面分布，培养初期呈球形，培养后期呈细长状。这种分布与在二维表面培养的成纤维细胞的分布完全不同，在二维表面培养的成纤维细胞中，肌动蛋白微丝基本上沿着与平面接触的内膜排列。无论是在二维还是三维中，与底物的接触也对从球形到铺展形状或细长形状的形态变化时间有很大影响:在玻璃或胶原凝胶上，在6小时内观察到明显的形态变化，在胶原凝胶内，在30小时或更晚的时间内观察到明显的形态变化。低剂量(0.2µM)的细胞松弛素D可拮抗凝胶中细胞伸长的阻滞，但浓度为2µM的细胞松弛素D可使细胞保持圆形。由于低浓度的细胞松弛素在体外诱导肌动蛋白聚合，因此采用罗丹明-phalloidin染色法检测肌动蛋白微丝的组织。发现低细胞松弛素D使细长细胞中的肌动蛋白丝被破坏。这些结果表明，低剂量的细胞松弛素D处理可能是由肌动蛋白微丝的不稳定引起的，而肌动蛋白微丝可能在胶原凝胶中支撑细胞的球形。在添加的游离细胞松弛素d洗涤后，这样形成的细长形状恢复为球形。这与在凝胶中开始培养40小时后通过长时间培养建立的细长细胞不同。也就是说，尽管成纤维细胞的肌动蛋白微丝被完全破坏，但以最高剂量2.0µM添加细胞松弛素D并没有改变其拉长的形状。这些发现表明，肌动蛋白微丝组织不积极参与或游离于胶原凝胶中成纤维细胞细长形状的获得和维持。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Matrix (Stuttgart, Germany)

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