Zsak L, Lu Z, Kutish G F, Neilan J G, Rock D L
Plum Island Animal Disease Center, Agricultural Research Service, U.S. Department of Agriculture, Greenport, New York 11944-0848, USA.
J Virol. 1996 Dec;70(12):8865-71. doi: 10.1128/JVI.70.12.8865-8871.1996.
We described previously an African swine fever virus (ASFV) open reading frame, 23-NL, in the African isolate Malawi Lil 20/1 whose product shared significant similarity in a carboxyl-terminal domain with those of a mouse myeloid differentiation primary response gene, MyD116, and the herpes simplex virus neurovirulence-associated gene, ICP34.5 (M. D. Sussman, Z. Lu, G. Kutish, C. L. Afonso, P. Roberts, and D. L. Rock, J. Virol. 66:5586-5589, 1992). The similarity of 23-NL to these genes suggested that this gene may function in some aspect of ASFV virulence and/or host range. Sequence analysis of additional pathogenic viral isolates demonstrates that this gene is highly conserved among diverse ASFV isolates and that the gene product exists in either a long (184 amino acids as in 23-NL) or a short form (70 to 72 amino acids in other examined ASFV isolates). The short form of the gene, NL-S, encodes the complete highly conserved, hydrophilic, carboxyl-terminal domain of 56 amino acids common to 23-NL, MyD116, and ICP34.5. Recombinant NL-S gene deletion mutants and their revertants were constructed from the pathogenic ASFV isolate E70 and an E70 monkey cell culture-adapted virus, MS44, to study gene function. Although deletion of NL-S did not affect viral growth in primary swine macrophages or Vero cell cultures in vitro, the null mutant, E70/43, exhibited a marked reduction in pig virulence. In contrast to revertant or parental E70 where mortality was 100%, all E70/43-infected animals survived infection. With the exception of a transient fever response, E70/43-infected animals remained clinically normal and exhibited a 1,000-fold reduction in both mean and maximum viremia titers. All convalescent E70/43-infected animals survived infection when challenged with parental E70 at 30 days postinfection. These data indicate that the highly conserved NL-S gene of ASFV, while nonessential for growth in swine macrophages in vitro, is a significant viral virulence factor and may function as a host range gene.
我们之前描述过非洲猪瘟病毒(ASFV)的一个开放阅读框23-NL,它存在于非洲分离株马拉维Lil 20/1中,其产物在羧基末端结构域与小鼠髓样分化初级反应基因MyD116以及单纯疱疹病毒神经毒力相关基因ICP34.5的产物具有显著相似性(M. D. 苏斯曼、Z. 卢、G. 库蒂什、C. L. 阿方索、P. 罗伯茨和D. L. 罗克,《病毒学杂志》66:5586 - 5589,1992年)。23-NL与这些基因的相似性表明该基因可能在ASFV毒力和/或宿主范围的某些方面发挥作用。对其他致病性病毒分离株的序列分析表明,该基因在不同的ASFV分离株中高度保守,并且基因产物存在长形式(如23-NL中的184个氨基酸)或短形式(在其他检测的ASFV分离株中为70至72个氨基酸)。该基因的短形式NL-S编码23-NL、MyD116和ICP34.5共有的56个氨基酸的完全保守的亲水性羧基末端结构域。从致病性ASFV分离株E70和适应猴细胞培养的E70病毒MS44构建了重组NL-S基因缺失突变体及其回复体,以研究基因功能。虽然缺失NL-S不影响病毒在原代猪巨噬细胞或体外Vero细胞培养物中的生长,但缺失突变体E70/43在猪的毒力上显著降低。与回复体或亲本E70(死亡率为100%)相比,所有感染E70/43的动物都存活了下来。除了短暂的发热反应外,感染E70/43的动物临床症状正常,平均和最大病毒血症滴度降低了1000倍。所有感染E70/43并康复的动物在感染后30天用亲本E70攻击时都存活了下来。这些数据表明,ASFV高度保守的NL-S基因虽然在体外猪巨噬细胞生长中不是必需的,但却是一个重要的病毒毒力因子,可能作为宿主范围基因发挥作用。
