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Combination of culture on collagen gels and glucose starvation for cloning human colon cancer cells

机译:结合胶原凝胶和葡萄糖饥饿培养法克隆人结肠癌细胞

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摘要

Glucose starvation has been widely used to select differentiated subpopulations from the heterogenous human colon cancer cell line HT29. We observed that the important cell loss elicited by culturing these cells in glucose-free medium could be limited when type I collagen gel was used as substratum instead of conventional plastic support. We took advantage of this property to develop a new protocol, which combined glucose starvation and culture on collagen gels, for cloning HT29 cells. Using this procedure we have isolated four clones that were characterized on the basis of morphological (optical and transmission electron microscopy), electrophysiological (determination of transepithelial electrical parameters) and biochemical (detection of villin, sucrase-isomaltase and carcinoembryonic antigen) criteria. These four clones expressed different patterns of enterocytic differentiation regarding to these criteria. These results confirmed the heterogeneity of the HT29 cell line. One of these clones, HT29-A7, which displayed numerous intercellular cysts that disappeared at confluency, appears as a complementary model in the study of epithelial biogenesis.
机译:葡萄糖饥饿已广泛用于从异种人结肠癌细胞系HT29中选择分化的亚群。我们观察到,当将I型胶原蛋白凝胶用作基质而不是常规塑料支持物时,在无葡萄糖培养基中培养这些细胞所引起的重要细胞损失可能受到限制。我们利用这一特性开发了一种新的方案,该方案结合了葡萄糖饥饿和胶原蛋白凝胶上的培养,用于克隆HT29细胞。使用该程序,我们分离出了四个克隆,这些克隆的特征是形态学(光学和透射电子显微镜),电生理学(测定上皮电参数)和生化(检测villin,蔗糖酶-异麦芽糖酶和癌胚抗原)标准。关于这些标准,这四个克隆表达了不同的肠细胞分化模式。这些结果证实了HT29细胞系的异质性。这些克隆之一HT29-A7表现出许多在融合时消失的细胞间囊肿,在上皮生物发生研究中作为互补模型出现。

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