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猪水疱病病毒2A蛋白酶的精氨酸20对活性和毒力的重要性。

Importance of arginine 20 of the swine vesicular disease virus 2A protease for activity and virulence.

作者信息

Inoue Toru, Alexandersen Soren, Clark Angela T, Murphy Ciara, Quan Melvyn, Reid Scott M, Sakoda Yoshihiro, Johns Helen L, Belsham Graham J

机构信息

Department of Exotic Disease, National Institute of Animal Health, Kodaira, Tokyo, Japan.

出版信息

J Virol. 2005 Jan;79(1):428-40. doi: 10.1128/JVI.79.1.428-440.2005.

Abstract

A major virulence determinant of swine vesicular disease virus (SVDV), an Enterovirus that causes an acute vesicular disease, has been mapped to residue 20 of the 2A protease. The SVDV 2A protease cleaves the 1D-2A junction in the viral polyprotein, induces cleavage of translation initiation factor eIF4GI, and stimulates the activity of enterovirus internal ribosome entry sites (IRESs). The 2A protease from an attenuated strain of SVDV (Ile at residue 20) is significantly defective at inducing cleavage of eIF4GI and the activation of IRES-dependent translation compared to the 2A protease from a pathogenic strain (J1/73, Arg at residue 20), but the two proteases have similar 1D-2A cleavage activities (Y. Sakoda, N. Ross-Smith, T. Inoue, and G. J. Belsham, J. Virol. 75:10643-10650, 2001). Residue 20 has now been modified to every possible amino acid, and the activities of each mutant 2A protease has been analyzed. Selected mutants were reconstructed into full-length SVDV cDNA, and viruses were rescued. The rate of virus growth in cultured swine kidney cells reflected the efficiency of 2A protease activity. In experimentally infected pigs, all four of the mutant viruses tested displayed much-reduced virulence compared to the J1/73 virus but a significant, albeit reduced, level of viral replication and excretion was detected. Direct sequencing of cDNA derived from samples taken early and late in infection indicated that a gradual selection-reversion to a more efficient protease occurred. The data indicated that extensive sequence change and selection may introduce a severe bottleneck in virus replication, leading to a decreased viral load and reduced or no clinical disease.

摘要

猪水疱病病毒(SVDV)是一种引起急性水疱病的肠道病毒,其主要毒力决定因素已定位到2A蛋白酶的第20位氨基酸残基。SVDV 2A蛋白酶切割病毒多聚蛋白中的1D-2A连接点,诱导翻译起始因子eIF4GI的切割,并刺激肠道病毒内部核糖体进入位点(IRES)的活性。与致病株(J1/73,第20位氨基酸残基为精氨酸)的2A蛋白酶相比,减毒株SVDV(第20位氨基酸残基为异亮氨酸)的2A蛋白酶在诱导eIF4GI切割和IRES依赖性翻译激活方面存在显著缺陷,但这两种蛋白酶具有相似的1D-2A切割活性(Y. Sakoda、N. Ross-Smith、T. Inoue和G. J. Belsham,《病毒学杂志》75:10643-10650,2001年)。现已将第20位氨基酸残基修饰为每一种可能的氨基酸,并分析了每个突变型2A蛋白酶的活性。将选定的突变体重建成全长SVDV cDNA,并拯救出病毒。病毒在培养的猪肾细胞中的生长速率反映了2A蛋白酶活性的效率。在实验感染的猪中,与J1/73病毒相比,所测试的四种突变病毒的毒力均大幅降低,但仍检测到显著水平(尽管有所降低)的病毒复制和排泄。对感染早期和晚期采集的样本进行cDNA直接测序表明,发生了向更高效蛋白酶的逐渐选择-回复突变。数据表明,广泛的序列变化和选择可能会在病毒复制过程中引入严重瓶颈,导致病毒载量降低以及临床疾病减轻或无临床疾病。

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