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Functional expression of the human transferrin receptor cDNA in Chinese hamster ovary cells deficient in endogenous transferrin receptor

机译:人转铁蛋白受体cDNA在缺乏内源性转铁蛋白受体的中国仓鼠卵巢细胞中的功能表达

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摘要

Transferrin (Tf) receptor-variant Chinese hamster ovary cells have been isolated by selection for resistance to two Tf-toxin conjugates. The hybrid toxins contain Tf covalently linked to ricin A chain or a genetically engineered diphtheria toxin fragment. The Tf-receptor- variant (TRV) cells do not have detectable cell-surface Tf receptor; they do not bind fluorescein-Tf or 125I-Tf. TRV cells are at least 100- fold more resistant to the Tf-diphtheria toxin conjugate than are the parent cells. The TRV cells have retained sensitivity to native diphtheria toxin, indicating that the increased resistance to the conjugate is correlated with the loss of Tf binding. The endocytosis of fluorescein-labeled alpha 2-macroglobulin is normal in TRV cells, demonstrating that the defect does not pleiotropically affect endocytosis. Since these cells lack endogenous Tf receptor activity, they are ideally suited for studies of the functional expression of normal or altered Tf receptors introduced into the cells by cDNA transfection. One advantage of this system is that Tf binding and uptake can be used to monitor the behavior of the transfected receptor. A cDNA clone of the human Tf receptor has been transfected into TRV cells. In the stably expressing transfectants, the behavior of the human receptor is very similar to that of the endogenous Chinese hamster ovary cell Tf receptor. Tf binds to cell surface receptors, and is internalized into the para-Golgi region of the cell. Iron is released from Tf, and the apo-Tf and its receptor are recycled back to the cell surface. Thus, the TRV cells can be used to study the behavior of genetically altered Tf receptors in the absence of interfering effects from endogenous receptors.
机译:通过选择对两种Tf-毒素结合物的抗性,已分离出转铁蛋白(Tf)受体变异的中国仓鼠卵巢细胞。杂合毒素包含与蓖麻蛋白A链或基因工程白喉毒素片段共价连接的Tf。 Tf受体变异(TRV)细胞没有可检测的细胞表面Tf受体;它们不结合荧光素-Tf或125I-Tf。 TRV细胞对Tf-白喉毒素缀合物的抗性比亲代细胞高至少100倍。 TRV细胞保留了对天然白喉毒素的敏感性,表明对结合物的抗性增强与Tf结合力的丧失有关。荧光素标记的α2-巨球蛋白的内吞作用在TRV细胞中是正常的,这表明该缺陷不会多效性地影响内吞作用。由于这些细胞缺乏内源性Tf受体活性,因此非常适合研究通过cDNA转染引入细胞的正常或改变的Tf受体的功能性表达。该系统的一个优势是Tf结合和摄取可用于监测转染受体的行为。人Tf受体的cDNA克隆已被转染到TRV细胞中。在稳定表达的转染子中,人类受体的行为与内源中国仓鼠卵巢细胞Tf受体的行为非常相似。 Tf与细胞表面受体结合,并被内化到细胞的对高尔基体区域。铁从Tf中释放出来,而apo-Tf及其受体被循环回到细胞表面。因此,在没有来自内源性受体的干扰作用的情况下,TRV细胞可用于研究遗传改变的Tf受体的行为。

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