利用嵌合病毒研究甲病毒装配所需的PE2、E1和6K之间的相互作用。
Interactions between PE2, E1, and 6K required for assembly of alphaviruses studied with chimeric viruses.
作者信息
Yao J S, Strauss E G, Strauss J H
机构信息
Division of Biology, California Institute of Technology, Pasadena 91125, USA.
出版信息
J Virol. 1996 Nov;70(11):7910-20. doi: 10.1128/JVI.70.11.7910-7920.1996.
During the assembly of alphaviruses, a preassembled nucleocapsid buds through the cell plasma membrane to acquire an envelope containing two virally encoded glycoproteins, E2 and E1. Using two chimeric viruses, we have studied interactions between E1, E2, and a viral peptide called 6K, which are required for budding. A chimeric Sindbis virus (SIN) in which the 6K gene had been replaced with that from Ross River virus (RR) produced wild-type levels of nucleocapsids and abundant PE2/E1 heterodimers that were processed and transported to the cell surface. However, only about 10% as much chimeric virus as wild-type virus was assembled, demonstrating that there is a sequence-specific interaction between 6K and the glycoproteins required for efficient virus assembly. In addition, the conformation of E1 in the E2/E1 heterodimer on the cell surface was different for the chimeric virus from that for the wild type, suggesting that one function of 6K is to promote proper folding of E1 in the heterodimer. A second chimeric SIN, in which both the 6K and E1 genes, as well as the 3' nontranslated region, were replaced with the corresponding regions of RR also resulted in the production of large numbers of intracellular nucleocapsids and of PE2/E1 heterodimers that were cleaved and transported to the cell surface. Budding of this chimera was severely impaired, however, and the yield of the chimera was only approximately 10(-7) of the SIN yield in a parallel infection. The conformation of the SIN E2/RR E1 heterodimer on the cell surface was different from that of the SIN E2/SIN E1 heterodimer, and no interaction between viral glycoproteins and nucleocapsids at the cell plasma membrane could be detected in the electron microscope. We suggest that proper folding of the E2/E1 heterodimer must occur before the E2 tail is positioned properly in the cytoplasm for budding and before heterodimer trimerization can occur to drive virus budding.
在甲病毒组装过程中,预先组装好的核衣壳通过细胞质膜出芽,获得一个包含两种病毒编码糖蛋白E2和E1的包膜。我们利用两种嵌合病毒研究了出芽所需的E1、E2和一种名为6K的病毒肽之间的相互作用。一种嵌合辛德毕斯病毒(SIN),其6K基因已被罗斯河病毒(RR)的6K基因取代,产生了野生型水平的核衣壳和大量经加工并转运至细胞表面的PE2/E1异二聚体。然而,组装的嵌合病毒量仅约为野生型病毒的10%,这表明6K与高效病毒组装所需的糖蛋白之间存在序列特异性相互作用。此外,细胞表面E2/E1异二聚体中E1的构象,对于嵌合病毒而言与野生型不同,这表明6K的一个功能是促进异二聚体中E1的正确折叠。第二种嵌合SIN,其6K和E1基因以及3'非翻译区均被RR的相应区域取代,也导致产生大量细胞内核衣壳和经切割并转运至细胞表面的PE2/E1异二聚体。然而,这种嵌合体的出芽严重受损,在平行感染中其产量仅约为SIN产量的10^(-7)。细胞表面SIN E2/RR E1异二聚体的构象与SIN E2/SIN E1异二聚体不同,并且在电子显微镜下未检测到细胞质膜处病毒糖蛋白与核衣壳之间的相互作用。我们认为,E2/E1异二聚体的正确折叠必须在E2尾部在细胞质中正确定位以进行出芽之前发生,并且在异二聚体三聚化以驱动病毒出芽之前发生。
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