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分析重组杆状病毒中禽偏肺病毒附着糖蛋白的表达和糖基化。

Analysis of expression and glycosylation of avian metapneumovirus attachment glycoprotein from recombinant baculoviruses.

机构信息

National Centre for Foreign Animal Disease, Canadian Food Inspection Agency, 1015 Arlington Street, Winnipeg, Manitoba, Canada R3E 3M4.

出版信息

Virus Res. 2010 Nov;153(2):244-9. doi: 10.1016/j.virusres.2010.08.008. Epub 2010 Aug 14.

DOI:10.1016/j.virusres.2010.08.008
PMID:20713098
Abstract

Recently, we reported the expression and glycosylation of avian metapneumovirus attachment glycoprotein (AMPV/C G protein) in eukaryotic cell lines by a transient-expression method. In the present study, we investigated the biosynthesis and O-linked glycosylation of the AMPV/C G protein in a baculovirus expression system. The results showed that the insect cell-produced G protein migrated more rapidly in SDS-PAGE as compared to LLC-MK2 cell-derived G proteins owing to glycosylation differences. The fully processed, mature form of G protein migrated between 78 and 86 kDa, which is smaller than the 110 kDa mature form of G expressed in LLC-MK2 cells. In addition, several immature G gene products migrating at 40-48 and 60-70 kDa were also detected by SDS-PAGE and represented glycosylated intermediates. The addition of the antibiotic tunicamycin, which blocks early steps of glycosylation, to insect cell culture resulted in the disappearance of two glycosylated forms of the G protein and identified a 38 kDa unglycosylated precursor. The maturation of the G protein was completely blocked by monensin, suggesting that the O-linked glycosylation of G initiated in the trans-Golgi compartment. The presence of O-linked sugars on the mature protein was further confirmed by lectin Arachis hypogaea binding assay. Furthermore, antigenic features of the G protein expressed in insect cells were evaluated by ELISA.

摘要

最近,我们通过瞬时表达法报道了禽类嵌合型副黏病毒(avian metapneumovirus, AMPV)的黏附糖蛋白(AMPV/C G 蛋白)在真核细胞系中的表达和糖基化。在本研究中,我们在杆状病毒表达系统中研究了 AMPV/C G 蛋白的生物合成和 O-连接糖基化。结果表明,与 LLC-MK2 细胞来源的 G 蛋白相比,昆虫细胞产生的 G 蛋白由于糖基化差异,在 SDS-PAGE 中迁移更快。完全加工的成熟形式的 G 蛋白在 SDS-PAGE 中迁移的位置在 78 和 86 kDa 之间,小于在 LLC-MK2 细胞中表达的 110 kDa 成熟形式的 G 蛋白。此外,还通过 SDS-PAGE 检测到几种迁移率在 40-48 和 60-70 kDa 的不成熟 G 基因产物,它们代表糖基化中间体。向昆虫细胞培养物中添加阻断早期糖基化步骤的抗生素衣霉素,导致两种糖基化形式的 G 蛋白消失,并鉴定出 38 kDa 的未糖基化前体。莫能菌素完全阻断了 G 蛋白的成熟,表明 G 的 O-连接糖基化始于反式高尔基体隔室。成熟蛋白上存在 O-连接糖的事实进一步通过花生凝集素 Arachis hypogaea 结合试验得到证实。此外,还通过 ELISA 评估了昆虫细胞中表达的 G 蛋白的抗原特征。

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