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禽呼肠孤病毒主要的μ类外 capsid 蛋白以病毒株特异性方式影响有生产力的巨噬细胞感染效率。

Avian reovirus major mu-class outer capsid protein influences efficiency of productive macrophage infection in a virus strain-specific manner.

作者信息

O'Hara D, Patrick M, Cepica D, Coombs K M, Duncan R

机构信息

Department of Microbiology and Immunology, Dalhousie University, Halifax, Nova Scotia, Canada B3H 4H7.

出版信息

J Virol. 2001 Jun;75(11):5027-35. doi: 10.1128/JVI.75.11.5027-5035.2001.

Abstract

We determined that the highly pathogenic avian reovirus strain 176 (ARV-176) possesses an enhanced ability to establish productive infections in HD-11 avian macrophages compared to avian fibroblasts. Conversely, the weakly pathogenic strain ARV-138 shows no such macrophagotropic tendency. The macrophage infection capability of the two viruses did not reflect differences in the ability to either induce or inhibit nitric oxide production. Moderate increases in the ARV-138 multiplicity of infection resulted in a concomitant increase in macrophage infection, and under such conditions the kinetics and extent of the ARV-138 replication cycle were equivalent to those of the highly infectious ARV-176 strain. These results indicated that both viruses are apparently equally capable of replicating in an infected macrophage, but they differ in the ability to establish productive infections in these cells. Using a genetic reassortant approach, we determined that the macrophagotropic property of ARV-176 reflects a post-receptor-binding step in the virus replication cycle and that the ARV-176 M2 genome segment is required for efficient infection of HD-11 cells. The M2 genome segment encodes the major mu-class outer capsid protein (muB) of the virus, which is involved in virus entry and transcriptase activation, suggesting that a host-specific influence on ARV entry and/or uncoating may affect the likelihood of the virus establishing a productive infection in a macrophage cell.

摘要

我们确定,与禽成纤维细胞相比,高致病性禽呼肠孤病毒176株(ARV-176)在HD-11禽巨噬细胞中建立有效感染的能力增强。相反,弱致病性毒株ARV-138没有这种嗜巨噬细胞倾向。两种病毒的巨噬细胞感染能力并未反映出诱导或抑制一氧化氮产生能力的差异。ARV-138感染复数的适度增加导致巨噬细胞感染随之增加,在这种情况下,ARV-138复制周期的动力学和程度与高感染性的ARV-176株相当。这些结果表明,两种病毒显然同样有能力在受感染的巨噬细胞中复制,但它们在这些细胞中建立有效感染的能力有所不同。通过基因重配方法,我们确定ARV-176的嗜巨噬细胞特性反映了病毒复制周期中受体结合后的一个步骤,并且ARV-176的M2基因组片段是高效感染HD-11细胞所必需的。M2基因组片段编码病毒的主要μ类外衣壳蛋白(μB),它参与病毒进入和转录酶激活,这表明宿主对ARV进入和/或脱壳的特异性影响可能会影响病毒在巨噬细胞中建立有效感染的可能性。

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