Background Knowledge of the subcellular localization of a protein can provide useful insights about its function. While the subcellular localization of many alphaherpesvirus UL51 proteins has been well characterized, little is known about where duck enteritis virus (DEV) UL51 protein (pUL51) is targeted to. Thus, in this study, we investigated the subcellular localization and distribution of DEV pUL51 by computer aided analysis, as well as indirect immunofluorescence (IIF) and transmission immunoelectron microscopy (TIEM) approaches in DEV-infected cells. Results The DEV UL51 gene product was identified as an approximate 34 kDa protein in DEV-infected cells analyzed by western blotting. Computer aided analysis suggested that DEV pUL51 is not targeted to the mitochondrial, extra-cellular or nucleus, but be targeted to the cytoplasmic in host cells, more specifically, palmitoylation of the pUL51 through the N-terminal cysteine at position 9 makes membrane association and Golgi localization possible. Using IIF analysis, we found that DEV pUL51 was first detected in a juxtanuclear region of DEV-infected cells at 9 h postinfection (p.i.), and then was detected widely distributed in the cytoplasm and especially was stronger in the juxtanuclear region from 12 to 60 h p.i. TIEM analysis revealed that DEV pUL51 was mainly associated with cytoplasmic virions and also with some membranous structure near the pUL51-specific immuno-labeling intracellular virion in the cytoplasmic vesicles; moreover, the pUL51 efficiently accumulated in the Golgi apparatus at first, and then was sent to the plasma membrane from the Golgi by some unknown mechanism. Conclusion In this work, we described the basic characteristics of pUL51 subcellular localization and distribution for the first time. From these results, we concluded that palmitoylation at the N-terminal cysteine, which is conserved in all alphaherpesvirus UL51 homologs, is required for its membrane association and Golgi localization, and the pUL51 mainly localized to the juxtanuclear region of DEV-infected cells, as well seemed to be incorporated into mature virions as a component of the tegument. The research will provide useful clues for DEV pUL51 functional analysis, and will be usefull for further understanding the localization properties of alphaherpesvirus UL51 homologs.
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机译:背景技术关于蛋白质亚细胞定位的知识可以提供有关其功能的有用见解。尽管已经很好地表征了许多α疱疹病毒UL51蛋白的亚细胞定位,但是对于鸭肠炎病毒(DEV)UL51蛋白(pUL51)的目标却鲜为人知。因此,在这项研究中,我们通过计算机辅助分析以及DEV感染细胞中的间接免疫荧光(IIF)和透射免疫电子显微镜(TIEM)方法研究了DEV pUL51的亚细胞定位和分布。结果通过蛋白质印迹分析,在DEV感染的细胞中,DEV UL51基因产物被鉴定为大约34 kDa的蛋白质。计算机辅助分析表明,DEV pUL51并非针对线粒体,细胞外或细胞核,而是针对宿主细胞中的细胞质,更具体地说,pUL51的棕榈酰化是通过位置9的N端半胱氨酸使膜结合并高尔基语本地化是可能的。使用IIF分析,我们发现DEV pUL51首先在感染后9小时(pi)在DEV感染细胞的近核区域中检测到,然后被发现广泛分布在细胞质中,尤其是在12到60的近核区域中更强^ h PI TIEM分析显示,DEV pUL51主要与胞质病毒颗粒有关,并且在胞质小泡中靠近pUL51特异性免疫标记细胞内病毒颗粒的地方还具有一些膜结构。而且,pUL51首先有效地积聚在高尔基体中,然后通过某种未知的机制从高尔基体中传递到质膜。结论在这项工作中,我们首次描述了pUL51亚细胞定位和分布的基本特征。从这些结果,我们得出结论,其膜结合和高尔基体定位需要在所有α疱疹病毒UL51同源物中保守的N端半胱氨酸的棕榈酰化,并且pUL51主要定位于DEV感染细胞的近核区域,如似乎已被整合到成熟的病毒体中,成为外皮的一部分。该研究将为DEV pUL51功能分析提供有用的线索,对于进一步了解α疱疹病毒UL51同系物的定位特性将是有用的。
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