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呼吸道合胞病毒糖蛋白的合成动力学

Kinetics of synthesis of respiratory syncytial virus glycoproteins.

作者信息

Fernie B F, Dapolito G, Cote P J, Gerin J L

出版信息

J Gen Virol. 1985 Sep;66 ( Pt 9):1983-90. doi: 10.1099/0022-1317-66-9-1983.

Abstract

The synthesis of the two respiratory syncytial (RS) virus glycoproteins (VP66 and VP84) was examined under standard conditions and after treatment with tunicamycin and monensin. The protein backbone for VP66, the fusion protein (F1,2) is cotranslationally glycosylated to form F0, which is cleaved to form F1,2 by 20 min of chase. Monensin treatment inhibited the cleavage of F0 over an 80 min chase period, indicating that this occurred late in the transit of F0 through the Golgi apparatus or after exit from the Golgi apparatus. Tunicamycin treatment resulted in the synthesis of a 50K to 55K unglycosylated F0 which is cleaved to a 40K protein. VP84, the large glycoprotein, contains a protein backbone of only 26K to 30K which is modified by N-linked and probable O-linked glycosylation. Tunicamycin treatment results in the synthesis of a 70K protein (p70) which incorporates [3H]glucosamine and [3H]fucose but not [3H]mannose. Glycosylated precursors varying in mol. wt. from 29K to 45K (p45) are found in infected cells at regular 2K to 3K intervals, producing a 'ladder' effect. The step from p45 to VP84 is severely delayed by monensin treatment thereby enhancing the 'ladder' effect of the precursors.

摘要

在标准条件下以及用衣霉素和莫能菌素处理后,对两种呼吸道合胞病毒(RS)糖蛋白(VP66和VP84)的合成进行了检测。VP66即融合蛋白(F1,2)的蛋白质骨架在共翻译过程中进行糖基化形成F0,在追踪20分钟后F0被切割形成F1,2。在80分钟的追踪期内,莫能菌素处理抑制了F0的切割,这表明该切割发生在F0通过高尔基体的后期或从高尔基体出来之后。衣霉素处理导致合成一种50K至55K的未糖基化F0,其被切割为一种40K的蛋白质。VP84即大糖蛋白,含有仅26K至30K的蛋白质骨架,该骨架通过N - 连接和可能的O - 连接糖基化进行修饰。衣霉素处理导致合成一种70K的蛋白质(p70),其掺入[3H]葡糖胺和[3H]岩藻糖,但不掺入[3H]甘露糖。在感染细胞中发现分子量从29K到45K不等的糖基化前体(p45)以2K到3K的固定间隔出现,产生“阶梯”效应。从p45到VP84的步骤被莫能菌素处理严重延迟,从而增强了前体的“阶梯”效应。

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