胆碱酯酶在鸡肢发育中的作用[j]。体外软骨细胞的酶活性和运动行为[j]。

Ulrich Drews, Ute Drews
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引用次数: 1

摘要

从我们以前的工作中,我们提出了胚胎细胞胆碱酯酶活性与形态发生运动有关的假设。因此,我们在体外分析了间充质细胞通过胆碱酯酶活性阶段向软骨分化的运动行为。鸡肢芽第23/24期的间充质核部分分解并在塑料组织培养皿中培养(图1)。在31/2至5天内,间充质细胞聚集分化成软骨结节,周围环绕成肌细胞(图2、3和5)。通过电镜证实了结节的软骨性质(图6和7)。在培养期间拍摄了一系列照片(24×24 mm)(表1-3)。福尔马林固定后,在培养皿内进行组织化学胆碱酯酶反应。在活体序列照片中识别阳性和阴性细胞,并分析其运动行为。最初,这些细胞表现得像成纤维细胞。运动受接触抑制调节,导致间充质聚集体径向向外迁移。在发育的第一阶段,没有胆碱酯酶活性。然而,在培养12至48小时后,可以检测到che阳性细胞。阳性细胞出现在单层中,从培养皿底部分离并爬到邻近的细胞上(图8a和b)。在聚集体的外围,径向向外迁移的速度明显减慢。中心可见阳性细胞短时间无方向性运动,经常导致细胞体重叠。在发育的第三阶段,che阳性细胞停止运动并转化为软骨细胞(图9a和b)。最后,分化的软骨细胞中che活性消失。从阴性和阳性细胞运动行为的差异可以得出结论,胆碱酯酶的出现伴随着细胞粘附特性的变化。细胞粘附性的增加使che阳性细胞能够从培养皿底部分离,并在细胞聚集体内部建立新的接触抑制平衡。这似乎是细胞外基质分泌和坚固细胞接触发育的先决条件。体内软骨分化可能也开始于软骨细胞黏附性的增加。这引起假足重排,导致软骨胶原的凝结和分化。黏附性的变化伴随着胆碱酯酶活性的变化。
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[Cholinesterase in the development of the chick limb : II. Enzyme activity and locomotory behavior of the presumptive cartilage cellsin vitro].

From our previous work we have put forward the hypothesis that cholinesterase activity in embryonic cells is related to morphogenetic movements. Therefore, the locomotory behavior of mesenchymal cells differentiating into cartilage by passing through a phase of Cholinesterase activity was analysedin vitro.Mesenchymal cores of chick limb buds stage 23/24 were partially disaggregated and cultured in plastic tissue culture dishes (Fig. 1). Within 31/2 to 5 days aggregates of mesenchymal cells differentiated into cartilage nodules surrounded by myoblasts (Figs. 2, 3 and 5). The cartilaginous nature of the nodules was confirmed by electron microscopy (Figs. 6 and 7). During the culture period serial photographs (24×24 mm) were taken (Tables 1-3). After formalin fixation the histochemical Cholinesterase reaction was carried out inside the culture dishes. Positive and negative cells were identified in the live serial photographs and their locomotory behavior was analysed.Initially the cells behaved like fibroblasts. Movements were regulated by contact inhibition, resulting in radial outward migration within the mesenchymal aggregates. In this first phase of development there was no cholinesterase activity. After 12 to 48 hours in culture however ChE-positive cells could be detected. Positive cells, appearing within a monolayer, detached from the bottom of the culture dish and crawled onto neighboring cells (Figs. 8a and b). In the periphery of the aggregates radial outward migration slowed down considerably. In the center short non-directional movements of positive cells could be observed, frequently leading to overlayering of cell bodies.In the third stage of development the ChE-positive cells stopped moving and transformed into cartilage cells (Fig. 9a and b). Finally, ChE-activity disappeared from the differentiated cartilage cells.From the difference in locomotory behaviour of negative and positive cells it is concluded that the appearance of Cholinesterase is accompanied by a change in the adhesive properties of the cells. An increase in cell adhesiveness enables the ChE-positive cells to detach from the bottom of the culture dish and to establish a new equilibrium of contact inhibition inside the cellular aggregates. This seems to be a prerequisite for the secretion of extracellular matrix and development of firm cell contacts. In vivo cartilage differentiation presumably also starts with an increase in cell adhesiveness in the presumptive cartilage cells. This provokes pseudopodial rearrangements leading to the condensation and demarkation of the cartilage anlagen. The change in adhesiveness is accompanied by Cholinesterase activity.

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