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A quantitative description of the extension and retraction of surface protrusions in spreading 3T3 mouse fibroblasts

机译:扩散3T3小鼠成纤维细胞中表面突起的伸缩的定量描述

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摘要

We suggest a method of quantitating the motile actions of surface protrusions in spreading animal cells in culture. Its basis is the determination of the percentage of freshly plated cells which produce particle-free areas around them on a gold particle-coated glass cover slip within 50 min. Studying 3T3 cells with this assay, we found that the presence of Na+, K+, Cl-, and Mg++ or Ca++ in a neutral or slightly alkaline phosphate or bicarbonate buffered solution is sufficient to support the optimal particle removal by the cells for at least 50 min. Two metabolic inhibitors, 2,4-dinitrophenol and Na-azide, inhibit the particle removal. If D-glucose is added along with the inhibitors, particle removal can be restored, whereas the addition of three glucose analogues which are generally believed to be nonmetabolizable cannot restore the activity. Serum is not required for the mechanism(s) of the motile actions of surface protrusions in spreading 3T3 cells. However, it contains components which can neutralize the inhibitory actions of bovine serum albumin and several amino acids, particularly L-cystine or L-cystein and L-methionine. Furthermore, serum codetermines which of the major surface extension, filopodia, lamellipodia, or lobopodia, is predominantly active. We found three distinct classes of extracellular conditions under which the active surface projections are predominantly either lamellipodia, (sheetlike projections), lobopodia (blebs), or filopodia (microspikes). The quantitated dependencies on temperature, pH and the inhibition by cytochalasin B or the particle removal are very similar in all three cases. Preventing the cells from anchoring themselves for 15-20 min before plating in serum-free medium seems to stimulate particle removal threefold.
机译:我们提出了一种在培养中的传播动物细胞中定量表面突起运动功能的方法。它的基础是确定在50分钟内在镀有金颗粒的玻璃盖玻片上在其周围产生无颗粒区域的新鲜电镀细胞的百分比。用此测定法研究3T3细胞,我们发现在中性或弱碱性磷酸盐或碳酸氢盐缓冲溶液中存在Na +,K +,Cl-和Mg ++或Ca ++足以支持细胞至少50最佳去除颗粒分钟两种代谢抑制剂2,4-二硝基苯酚和叠氮化钠可抑制颗粒去除。如果将D-葡萄糖与抑制剂一起加入,则可以恢复去除颗粒的作用,而通常认为不可代谢的三种葡萄糖类似物的加入不能恢复活性。在扩散的3T3细胞中,表面突起的运动作用机制不需要血清。然而,它含有可以中和牛血清白蛋白和几种氨基酸,特别是L-胱氨酸或L-半胱氨酸和L-蛋氨酸的抑制作用的成分。此外,主要代际活动的血清密码子主要有丝状伪足,片状脂质体或叶状伪足。我们发现三种不同类型的细胞外条件,在这些条件下,活性表面投射主要是lamellipodia(片状投射),lopopodia(小泡)或filopodia(微穗)。在所有三种情况下,对温度,pH值和细胞松弛素B抑制作用或颗粒去除的定量依赖性非常相似。在无血清培养基中铺板之前,防止细胞锚定自身15-20分钟,似乎可以将颗粒去除刺激三倍。

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