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VP23R of Infectious Spleen and Kidney Necrosis Virus Mediates Formation of Virus-Mock Basement Membrane To Provide Attaching Sites for Lymphatic Endothelial Cells ▿

机译:感染性脾肾肾坏死病毒VP23R介导病毒模拟基底膜的形成,为淋巴管内皮细胞提供附着位点▿

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摘要

Putative open reading frames (ORFs) encoding laminin-like proteins are found in all members of the genus Megalocytivirus, family Iridoviridae. This is the first study that identified the VP23R protein encoded by ORF23R of the infectious spleen and kidney necrosis virus (ISKNV), a member of these genes of megalocytiviruses. The VP23R mRNA covering the ISKNV genomic coordinates 19547 to 22273 was transcribed ahead of the major capsid protein. Immunofluorescence analysis demonstrated that VP23R was expressed on the plasma membrane of the ISKNV-infected cells and could not be a viral envelope protein. Residues 292 to 576 of VP23R are homologous to the laminin γ1III2-6 fragment, which covers the nidogen-binding site. An immunoprecipitation assay showed that VP23R could interact with nidogen-1, and immunohistochemistry showed that nidogen-1 was localized on the outer membrane of the infected cells. Electron microscopy showed that a virus-mock basement membrane (VMBM) was formed on the surface of the infected cells and a layer of endothelial cells (ECs) was attached to the VMBM. The VMBM contained VP23R and nidogen-1 but not collagen IV. The attached ECs were identified as lymphatic endothelial cells (LECs), which have unique feature of overlapping intercellular junctions and can be stained by immunohistochemistry using an antibody against a specific lymphatic marker, Prox-1. Such infection signs have never been described in viruses. Elucidating the functions of LECs attached to the surface of the infected cells may be useful for studies on the pathogenic mechanisms of megalocytiviruses and may also be important for studies on lymphangiogenesis and basement membrane functions.
机译:在巨轮病毒科Iridoviridae家族的所有成员中都发现了编码层粘连蛋白样蛋白的推定开放阅读框(ORF)。这是第一个鉴定由感染性脾肾坏死病毒(ISKNV)ORF23R编码的VP23R蛋白的研究,ISKNV是巨轮病毒的这些基因的成员。覆盖ISKNV基因座标19547至22273的VP23R mRNA在主要衣壳蛋白之前转录。免疫荧光分析表明,VP23R在感染ISKNV的细胞的质膜上表达,并且可能不是病毒包膜蛋白。 VP23R的残基292至576与层粘连蛋白γ1III2-6片段同源,该片段覆盖了多肽的结合位点。免疫沉淀分析表明VP23R可以与nidogen-1相互作用,免疫组织化学表明nidogen-1位于受感染细胞的外膜上。电子显微镜显示,病毒模拟基底膜(VMBM)形成在被感染细胞的表面,并且内皮细胞(EC)层附着在VMBM上。 VMBM包含VP23R和nidogen-1,但不含胶原IV。附着的EC被鉴定为淋巴管内皮细胞(LEC),具有重叠的细胞间连接的独特特征,可以使用抗特定淋巴标记物Prox-1的抗体通过免疫组织化学进行染色。从未在病毒中描述过这种感染迹象。阐明附着于感染细胞表面的LEC的功能可能对研究巨轮病毒的致病机制有用,对淋巴管生成和基底膜功能的研究也可能很重要。

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