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呼吸道合胞病毒M2-2蛋白的过表达抑制病毒复制。

Overexpression of the M2-2 protein of respiratory syncytial virus inhibits viral replication.

作者信息

Cheng Xing, Park HyunJung, Zhou Helen, Jin Hong

机构信息

MedImmune Vaccines Inc., 297 N. Bernardo Ave., Mountain View, CA 94043, USA.

出版信息

J Virol. 2005 Nov;79(22):13943-52. doi: 10.1128/JVI.79.22.13943-13952.2005.

Abstract

The M2-2 protein of respiratory syncytial virus (RSV) is involved in regulation of viral RNA transcription and replication. Encoded by the next-to-last gene of RSV, the M2-2 open reading frame (ORF) overlaps with the upstream M2-1 ORF, suggesting that the production of the M2-2 protein might be tightly regulated during virus replication. To evaluate the effect of M2-2 overexpression on RSV replication, the M2-2 gene was separated from M2-1 by leaving it at the position prior to the M2-1 or moving it to the promoter proximal position as an independent transcriptional unit in the RSV A2 genome. Although recombinant viruses bearing the shuffled M2-2 gene were recovered and expressed higher levels of M2-2, most of these viruses grew poorly in HEp-2 cells. Sequence analysis revealed that various mutations (substitution, insertion, and deletion) occurred in the M2-2 gene, resulting in reduced M2-2 activity as measured by the RSV minigenome system. Further examination of the M2-2 sequence and its function showed that either one of the first two AUG codons located at the 5' end of M2-2 could be used to produce a functional M2-2 protein and that deletion of the first six amino acids from its N terminus or four amino acids from its C terminus greatly reduced its function. The effect of M2-2 protein on RSV replication was also studied by examining RSV replication in cells transiently expressing M2-2. The M2-2 protein expressed at a high level completely inhibited RSV replication. These results strongly suggested that the level of the M2-2 protein produced in the infected cells is critical to RSV replication.

摘要

呼吸道合胞病毒(RSV)的M2-2蛋白参与病毒RNA转录和复制的调控。M2-2开放阅读框(ORF)由RSV的倒数第二个基因编码,与上游的M2-1 ORF重叠,这表明在病毒复制过程中,M2-2蛋白的产生可能受到严格调控。为了评估M2-2过表达对RSV复制的影响,在RSV A2基因组中,通过将M2-2基因留在M2-1之前的位置或将其作为独立转录单元移至启动子近端位置,使其与M2-1分离。尽管携带重排M2-2基因的重组病毒得以回收并表达更高水平的M2-2,但这些病毒中的大多数在HEp-2细胞中生长不佳。序列分析显示,M2-2基因发生了各种突变(替换、插入和缺失),通过RSV微型基因组系统检测,这导致M2-2活性降低。对M2-2序列及其功能的进一步研究表明,位于M2-2 5'端的前两个AUG密码子中的任何一个都可用于产生功能性M2-2蛋白,并且从其N端缺失前六个氨基酸或从其C端缺失四个氨基酸会大大降低其功能。通过检测在瞬时表达M2-2的细胞中的RSV复制,也研究了M2-2蛋白对RSV复制的影响。高水平表达的M2-2蛋白完全抑制了RSV复制。这些结果有力地表明,感染细胞中产生的M2-2蛋白水平对RSV复制至关重要。

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