塞姆利基森林病毒膜融合蛋白的寡聚化依赖性折叠
Oligomerization-dependent folding of the membrane fusion protein of Semliki Forest virus.
作者信息
Andersson H, Barth B U, Ekström M, Garoff H
机构信息
Department of Biosciences at Novum, Huddinge, Sweden.
出版信息
J Virol. 1997 Dec;71(12):9654-63. doi: 10.1128/JVI.71.12.9654-9663.1997.
The spikes of alphaviruses are composed of three copies of an E2-E1 heterodimer. The E1 protein possesses membrane fusion activity, and the E2 protein, or its precursor form, p62 (sometimes called PE2), controls this function. Both proteins are, together with the viral capsid protein, translated from a common C-p62-E1 coding unit. In an earlier study, we showed that the p62 protein of Semliki Forest virus (SFV) dimerizes rapidly and efficiently in the endoplasmic reticulum (ER) with the E1 protein originating from the same translation product (so-called heterodimerization in cis) (B.-U. Barth, J. M. Wahlberg, and H. Garoff, J. Cell Biol. 128:283-291, 1995). In the present work, we analyzed the ER translocation and folding efficiencies of the p62 and E1 proteins of SFV expressed from separate coding units versus a common one. We found that the separately expressed p62 protein translocated and folded almost as efficiently as when it was expressed from a common coding unit, whereas the independently expressed E1 protein was inefficient in both processes. In particular, we found that the majority of the translocated E1 chains were engaged in disulfide-linked aggregates. This result suggests that the E1 protein needs to form a complex with p62 to avoid aggregation. Further analyses of the E1 aggregation showed that it occurred very rapidly after E1 synthesis and could not be avoided significantly by the coexpression of an excess of p62 from a separate coding unit. These latter results suggest that the p62-E1 heterodimerization has to occur very soon after E1 synthesis and that this is possible only in a cis-directed reaction which follows the synthesis of p62 and E1 from a common coding unit. We propose that the p62 protein, whose synthesis precedes that of the E1 protein, remains in the translocon of the ER and awaits the completion of E1. This strategy enables the p62 protein to complex with the E1 protein immediately after the latter has been made and thereby to control (suppress) its fusion activity.
甲病毒的刺突由三个E2-E1异二聚体拷贝组成。E1蛋白具有膜融合活性,而E2蛋白或其前体形式p62(有时称为PE2)控制此功能。这两种蛋白与病毒衣壳蛋白一起,从一个共同的C-p62-E1编码单元翻译而来。在早期研究中,我们发现塞姆利基森林病毒(SFV)的p62蛋白在内质网(ER)中与源自同一翻译产物的E1蛋白迅速且高效地二聚化(即所谓的顺式异二聚化)(B.-U. 巴特、J.M. 瓦尔贝里和H. 加罗夫,《细胞生物学杂志》128:283-291,1995年)。在本研究中,我们分析了从单独编码单元与共同编码单元表达的SFV的p62和E1蛋白的内质网转位和折叠效率。我们发现,单独表达的p62蛋白的转位和折叠效率几乎与从共同编码单元表达时一样高,而独立表达的E1蛋白在这两个过程中效率都很低。特别是,我们发现大多数转位的E1链参与了二硫键连接的聚集体。这一结果表明,E1蛋白需要与p62形成复合物以避免聚集。对E1聚集的进一步分析表明,它在E1合成后很快就会发生,并且通过从单独编码单元共表达过量的p62并不能显著避免。后一个结果表明,p62-E1异二聚化必须在E1合成后很快发生,并且这只有在从共同编码单元合成p62和E1后进行的顺式定向反应中才有可能。我们提出,合成先于E1蛋白的p62蛋白保留在内质网的转位子中,并等待E1完成合成。这种策略使p62蛋白能够在E1蛋白合成后立即与其形成复合物,从而控制(抑制)其融合活性。
Zotero 插件