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包膜糖蛋白加工在小鼠白血病病毒感染中的作用。

The role of envelope glycoprotein processing in murine leukemia virus infection.

作者信息

Freed E O, Risser R

出版信息

J Virol. 1987 Sep;61(9):2852-6. doi: 10.1128/JVI.61.9.2852-2856.1987.

Abstract

The murine leukemia virus envelope protein is synthesized as a precursor molecule, Pr85env, which is proteolytically cleaved at an arginine residue to produce two mature envelope proteins, gp70 and p15(E). The results presented here indicate that mutation to lysine of the arginine found at the envelope precursor cleavage site results in a precursor which is cleaved with an efficiency at least 10-fold lower than the efficiency with which the wild-type protein is cleaved. This mutation has been used to investigate the requirement for envelope protein processing in various aspects of retroviral infection. Viruses produced by cells transfected with mutant proviral clones are approximately 10-fold less infectious than wild-type viruses. Mutant viruses are incapable of inducing XC cell syncytium formation and are 100-fold less efficient than wild-type viruses at rendering cells resistant to superinfection. Envelope glycoproteins bearing the lysine mutation are found in reduced amounts on the surface of infected cells, and as a result mutant virions contain significantly less envelope protein than do wild-type virions. The phenotypic effects of the processing mutation described here are most likely the result of this paucity of envelope glycoproteins in virions carrying the mutation.

摘要

鼠白血病病毒包膜蛋白以前体分子Pr85env的形式合成,该前体分子在一个精氨酸残基处被蛋白水解切割,产生两种成熟的包膜蛋白gp70和p15(E)。此处给出的结果表明,包膜前体切割位点处的精氨酸突变为赖氨酸会导致一种前体,其切割效率比野生型蛋白的切割效率至少低10倍。这种突变已被用于研究逆转录病毒感染各个方面对包膜蛋白加工的需求。用突变型原病毒克隆转染的细胞产生的病毒的感染性比野生型病毒低约10倍。突变病毒不能诱导XC细胞形成多核体,并且在使细胞对超感染产生抗性方面比野生型病毒效率低100倍。携带赖氨酸突变的包膜糖蛋白在受感染细胞表面的含量减少,因此突变病毒颗粒所含的包膜蛋白比野生型病毒颗粒明显少。此处描述的加工突变的表型效应很可能是携带该突变的病毒颗粒中包膜糖蛋白缺乏的结果。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/557a/255803/1a94c096b64c/jvirol00100-0207-a.jpg

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