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温度敏感型中国仓鼠细胞突变体中的脂质 - 糖中间体与糖蛋白生物合成

Lipid-saccharide intermediates and glycoprotein biosynthesis in a temperature-sensitive Chinese hamster cell mutant.

作者信息

Tenner A J, Scheffler I E

出版信息

J Cell Physiol. 1979 Feb;98(2):251-66. doi: 10.1002/jcp.1040980202.

DOI:10.1002/jcp.1040980202
PMID:217883
Abstract

The characterization of a temperature-sensitive Chinese hamster cell mutant has been continued with the aim of localizing the apparent defect in glycoprotein synthesis (Tenner et al., '77). Although the mutation is lethal, a demonstration of the ability of the mutant cells to support proliferation of Mengo virus at the nonpermissive temperature indicates that the general metabolic processes of the cells remain intact at a time when glycoprotein synthesis is severely depressed. A quantitative study of protein synthesis on membrane-associated polysomes suggests that the synthesis of the polypeptide portion of the glycoproteins at 40.8 degrees C may be normal. The investigation of lipid-saccharide molecules which have been implicated in the formation and transfer of the oligosaccharide "core" to polypeptide acceptors shows that mutant cells at the nonpermissive temperature are capable of synthesizing these lipid saccharides normally, and that the pool of the dolichyl oligosaccharides is maintained at a constant level independent of the temperature. The rate of formation of the lipid-oligosaccharide, however, is reduced in intact mutant cells at the nonpermissive temperature. Further investigations show this decreased rate to be the result of an increased half life of the lipid-oligosaccharide at 40.8 degrees C. These data indicate that the temperature-sensitive step in glycoprotein biosynthesis is the transfer of the oligosaccharide core from the lipid-oligosaccharide intermediates to the nascent polypeptide chain. The data presented also provide evidence that the lipid-saccharide intermediates, previously described mainly in in vitro systems, are in fact involved in the glycosylation of a majority, if not all, of the mannose-containing glycoproteins in intact, growing hamster cells.

摘要

为了确定糖蛋白合成中明显的缺陷,对一种温度敏感的中国仓鼠细胞突变体的特性研究仍在继续(Tenner等人,1977年)。尽管该突变是致死性的,但有证据表明,突变细胞在非允许温度下支持Mengo病毒增殖的能力表明,在糖蛋白合成严重受抑时,细胞的一般代谢过程仍保持完整。对膜结合多核糖体上蛋白质合成的定量研究表明,在40.8摄氏度时糖蛋白多肽部分的合成可能是正常的。对参与寡糖“核心”向多肽受体形成和转移的脂糖分子的研究表明,处于非允许温度的突变细胞能够正常合成这些脂糖,并且多萜醇寡糖池保持在与温度无关的恒定水平。然而,在非允许温度下完整的突变细胞中,脂寡糖的形成速率降低。进一步的研究表明,这种降低的速率是由于脂寡糖在40.8摄氏度时半衰期增加的结果。这些数据表明,糖蛋白生物合成中温度敏感的步骤是寡糖核心从脂寡糖中间体转移到新生多肽链上。所提供的数据还证明,以前主要在体外系统中描述的脂糖中间体实际上参与了完整的、正在生长的仓鼠细胞中大多数(如果不是全部)含甘露糖糖蛋白的糖基化过程。

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引用本文的文献

1
Selection of mutant Chinese hamster ovary cells altered glycoproteins by means of tritiated fucose suicide.通过氚化岩藻糖自杀法筛选改变糖蛋白的突变型中国仓鼠卵巢细胞。
Mol Cell Biol. 1981 Oct;1(10):902-9. doi: 10.1128/mcb.1.10.902-909.1981.
2
Membrane mutants of animal cells: rapid identification of those with a primary defect in glycosylation.动物细胞膜突变体:快速鉴定糖基化存在原发性缺陷的突变体。
Mol Cell Biol. 1985 May;5(5):923-9. doi: 10.1128/mcb.5.5.923-929.1985.
3
Rat gene encoding the 78-kDa glucose-regulated protein GRP78: its regulatory sequences and the effect of protein glycosylation on its expression.
编码78 kDa葡萄糖调节蛋白GRP78的大鼠基因:其调控序列以及蛋白质糖基化对其表达的影响。
Proc Natl Acad Sci U S A. 1987 Feb;84(3):680-4. doi: 10.1073/pnas.84.3.680.