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利用可逆抑制剂剖析膜蛋白降解机制。

Dissection of membrane protein degradation mechanisms by reversible inhibitors.

作者信息

Hare J F

机构信息

Department of Biochemistry, School of Medicine, Oregon Health Sciences University, Portland 97201.

出版信息

J Biol Chem. 1988 Jun 25;263(18):8759-64.

PMID:3379045
Abstract

The degradation of slowly turning over 125I-lactoperoxidase-labeled plasma membrane polypeptides in response to reversible temperature and lysosomotropic inhibitors was studied in rat hepatoma cultures. Cells were radiolabeled and left for 24 h to allow the removal of rapidly degraded proteins. Remaining trichloroacetic acid-precipitable protein was degraded (t 1/2 = 40-68 h) by an apparent first order process 60-86% sensitive to 10 mM NH4Cl or 5 mM methylamine and greater than 95% inhibited by temperature reduction to 18 degrees C. Thus, membrane proteins are selected for degradation in a time-dependent manner by a system which is sensitive to both 18 degrees C and to lysosomotropic amines. When inhibitory conditions were removed after 40-48 h, degradation of 125I-labeled protein resumed at the same rate as that seen in their absence. Since membrane proteins do not exhibit accelerated degradation after removal of inhibitory conditions, there can be no marking or sorting of those proteins destined for degradation during the 40-h exposure to inhibitory conditions. Exposure to amines or 18 degrees C did not affect the position of two-dimensionally resolved labeled polypeptides. Fractionation of labeled cells on Percoll gradients after 40 h of exposure to low temperature or amines showed that labeled protein remained in the plasma membrane fractions of the gradient although shifted to a slightly lower buoyant density in the presence of amines. These results support the notion that selection of plasma membrane proteins for degradation requires their internalization into acidic vesicles. Lysosomotropic amines and reduced temperature interfere with the selection process by preventing membrane fusion events.

摘要

在大鼠肝癌细胞培养物中,研究了可逆温度和溶酶体促渗剂抑制剂对缓慢周转的125I-乳过氧化物酶标记的质膜多肽降解的影响。细胞进行放射性标记并放置24小时,以去除快速降解的蛋白质。剩余的三氯乙酸可沉淀蛋白通过一个明显的一级过程降解(t1/2 = 40 - 68小时),该过程60 - 86%对10 mM氯化铵或5 mM甲胺敏感,并且温度降至18℃时超过95%受到抑制。因此,膜蛋白通过一个对18℃和溶酶体促渗胺都敏感的系统,以时间依赖的方式被选择进行降解。当在40 - 48小时后去除抑制条件时,125I标记蛋白的降解以与不存在抑制条件时相同的速率恢复。由于去除抑制条件后膜蛋白没有表现出加速降解,所以在40小时的抑制条件暴露期间,不可能对那些注定要降解的蛋白进行标记或分选。暴露于胺或18℃并不影响二维分辨的标记多肽的位置。在暴露于低温或胺40小时后,通过Percoll梯度对标记细胞进行分级分离表明,标记蛋白仍保留在梯度的质膜部分,尽管在存在胺的情况下其浮力密度略有降低。这些结果支持这样的观点,即选择质膜蛋白进行降解需要它们内化到酸性小泡中。溶酶体促渗胺和降低的温度通过阻止膜融合事件干扰选择过程。

相似文献

1
Dissection of membrane protein degradation mechanisms by reversible inhibitors.利用可逆抑制剂剖析膜蛋白降解机制。
J Biol Chem. 1988 Jun 25;263(18):8759-64.
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Degradation of proteins in rat liver mitochondrial outer membrane transplanted into different cell types. Evidence for alternative processing.移植到不同细胞类型中的大鼠肝脏线粒体外膜中蛋白质的降解。替代加工的证据。
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Relations between plasma membrane and lysosomal membrane. 1. Fate of covalently labelled plasma membrane protein.质膜与溶酶体膜之间的关系。1. 共价标记质膜蛋白的命运。
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引用本文的文献

1
The kinetic aspects of intracellular fluorescence labeling with TMA-DPH support the maturation model for endocytosis in L929 cells.用TMA-DPH进行细胞内荧光标记的动力学方面支持L929细胞内吞作用的成熟模型。
J Cell Biol. 1994 May;125(4):783-94. doi: 10.1083/jcb.125.4.783.
2
Mechanisms of plasma membrane protein degradation: recycling proteins are degraded more rapidly than those confined to the cell surface.质膜蛋白降解的机制:循环利用的蛋白比那些局限于细胞表面的蛋白降解得更快。
Proc Natl Acad Sci U S A. 1991 Jul 1;88(13):5902-6. doi: 10.1073/pnas.88.13.5902.