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小鼠白血病病毒包膜糖蛋白前体的结构

Structure of the murine leukemia virus envelope glycoprotein precursor.

作者信息

Witte O N, Wirth D F

出版信息

J Virol. 1979 Feb;29(2):735-43. doi: 10.1128/JVI.29.2.735-743.1979.

Abstract

The glycosylated env gene precurosr (Pr80env) of Moloney murine leukemia virus has been isolated by selective immunoprecipitation. Use of the drug tunicamycin to inhibit nascent glycosylation or specific cleavage with endoglycosidase H demonstrated that the precursor contained an apoprotein with a molecular weight of 60,000. The finished virion glycoprotein (gp70) was largely resistant to the action of endoglycosidase H. Chromatography of the glycopeptides of Pr80env in conjunction with endoglycosidase H digestion studies suggested that the precursor contained two distinct major glycosylation sites. Analysis of partial proteolytic cleavage fragments of Pr80env before and after endoglycosidase H treatment placed the two glycosylation sites within a 30,000-dalton region of the apoprotein sequence. Kinetic experiments showed that carbohydrate processing as well as proteolytic cleavage are late steps in the maturation of Pr80env.

摘要

莫洛尼鼠白血病病毒的糖基化env基因前体(Pr80env)已通过选择性免疫沉淀法分离出来。使用衣霉素抑制新生糖基化或用内切糖苷酶H进行特异性切割表明,该前体含有一种分子量为60,000的脱辅基蛋白。成熟的病毒粒子糖蛋白(gp70)对内切糖苷酶H的作用具有很大抗性。Pr80env糖肽的色谱分析结合内切糖苷酶H消化研究表明,该前体含有两个不同的主要糖基化位点。对Pr80env在内切糖苷酶H处理前后的部分蛋白水解裂解片段进行分析,将这两个糖基化位点定位在脱辅基蛋白序列的一个30,000道尔顿区域内。动力学实验表明,碳水化合物加工以及蛋白水解裂解是Pr80env成熟过程中的后期步骤。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/982e/353205/80dc175a1c78/jvirol00182-0325-a.jpg

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