首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >The End2 mutation in CHO cells slows the exit of transferrin receptors from the recycling compartment but bulk membrane recycling is unaffected
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The End2 mutation in CHO cells slows the exit of transferrin receptors from the recycling compartment but bulk membrane recycling is unaffected

机译:CHO细胞中的End2突变会减慢转铁蛋白受体从回收室的排出但是大容量膜回收不会受到影响

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摘要

We have characterized a new CHO cell line (12-4) derived from a parental line, TRVb-1, that expresses the human transferrin receptor. This mutant belongs to the end2 complementation group of endocytosis mutants. Like other end2 mutants, the endosomes in 12-4 cells show a partial acidification defect. These cells internalize LDL and transferrin at 70% of the rate of parental cells and externalize transferrin at 55% of the parental rate (Johnson, L. S., J. F. Presley, J. C. Park, and T. E. McGraw. J. Cell Physiol. 1993). In this report, we have used fluorescence microscopy to determine which step in receptor trafficking is affected in the mutants. Transferrin is sorted from LDL and is delivered to a peri-centriolar recycling compartment at rates similar to parental cells. However, the rate constant for exit of transferrin from the recycling compartment in mutant cells is 0.025 min- 1 vs 0.062 min-1 in the parental line. We also measured the trafficking of a bulk membrane marker, 6-[N-[7-nitrobenzo-2-oxa-1,3-diazol-4-yl]- amino]hexanoyl- sphingosylphosphorylcholine (C6-NBD-SM) that labels the exofacial side of the plasma membrane. C6-NBD-SM enters the same recycling compartment as transferrin, and it exits the recycling compartment at a rate of 0.060-0.065 min-1 in both parental and 12-4 cells. We conclude that bulk membrane flow in the recycling pathway of 12-4 cells is normal, but exit of transferrin from the recycling compartment is slowed due to retention in this compartment. Thus, in the mutant cell line the recycling compartment carries out a sorting function, retaining transferrin over bulk membrane.
机译:我们已经表征了一种新的CHO细胞系(12-4),该细胞系衍生自表达人运铁蛋白受体的亲本系TRVb-1。该突变体属于胞吞作用突变体的end2互补组。像其他end2突变体一样,12-4细胞中的内体显示出部分酸化缺陷。这些细胞以亲代细胞率的70%内在化LDL和运铁蛋白,以亲代率55%的外在化转铁蛋白(Johnson,L.S.,J.F.Presley,J.C.Park,and T.E.McGraw.J.Cell Physiol.1993)。在本报告中,我们使用荧光显微镜来确定突变体中受体运输的哪一步受到影响。转铁蛋白是从LDL中分选出来的,并以与亲代细胞相似的速率输送到重心周围的回收室。然而,突变细胞中运铁蛋白从回收室中退出的速率常数为0.025 min-1,而亲本系为0.062 min-1。我们还测量了标记的大容量膜标记物6- [N- [7-硝基苯并-2-氧杂-1,3-二氮杂-4-基]-氨基]己酰基-鞘氨酰磷酰胆碱(C6-NBD-SM)的贩运质膜的颌面侧。 C6-NBD-SM与运铁蛋白进入同一回收室,在亲代和12-4细胞中,其以0.060-0.065 min-1的速率离开回收室。我们得出的结论是,在12-4个细胞的再循环途径中,大量的膜流动是正常的,但是由于保留在该室中,运铁蛋白从再循环室中的排出变慢了。因此,在突变细胞系中,回收室执行分类功能,将运铁蛋白保留在整个膜上。

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