Vlaycheva Leonsia A, Chambers Thomas J
Department of Molecular Microbiology and Immunology, St. Louis University Health Sciences Center, St. Louis, Missouri 63104, USA.
J Virol. 2002 Jun;76(12):6172-84. doi: 10.1128/jvi.76.12.6172-6184.2002.
Serial passage of yellow fever 17D virus (YF5.2iv, derived from an infectious molecular clone) on mouse neuroblastoma (NB41A3) cells established a persistent noncytopathic infection associated with a variant virus. This virus (NB15a) was dramatically reduced in plaque formation and exhibited impaired replication kinetics on all cell lines examined compared to the parental virus. Nucleotide sequence analysis of NB15a revealed a substitution in domain III of the envelope (E) protein at residue 360, where an aspartic acid residue was replaced by glycine. Single mutations were also found within the NS2A and NS3 proteins. Engineering of YF5.2iv virus to contain the E(360) substitution yielded a virus (G360 mutant) whose plaque size and growth efficiency in cell culture resembled those of NB15a. Compared with YF5.2iv, both NB15a and G360 were markedly restricted for spread through Vero cell monolayers and mildly restricted in C6/36 cells. On NB41A3 cells, spread of the viruses was similar, but all three were generally inefficient compared with spread in other cell lines. Compared to YF5.2iv virus, NB15a was uniformly impaired in its ability to penetrate different cell lines, but a difference in cell surface binding was detected only on NB41A3 cells, where NB15a appeared less efficient. Despite its small plaque size, impaired growth, and decreased penetration efficiency, NB15a did not differ from YF5.2iv in mouse neurovirulence testing, based on mortality rates and average survival times after intracerebral inoculation of young adult mice. The data indicate that persistence of yellow fever virus in NB41A3 cells is associated with a mutation in the receptor binding domain of the E protein that impairs the virus entry process in cell culture. However, the phenotypic changes which occur in the virus as a result of the persistent infection in vitro do not correlate with attenuation during pathogenesis in the mouse central nervous system.
黄热病17D病毒(YF5.2iv,源自感染性分子克隆)在小鼠神经母细胞瘤(NB41A3)细胞上连续传代,建立了与一种变异病毒相关的持续性非细胞病变感染。与亲代病毒相比,这种病毒(NB15a)在空斑形成方面显著减少,并且在所有检测的细胞系中复制动力学均受损。对NB15a的核苷酸序列分析显示,包膜(E)蛋白结构域III中第360位残基发生了替换,天冬氨酸残基被甘氨酸取代。在NS2A和NS3蛋白中也发现了单个突变。构建含有E(360)替换的YF5.2iv病毒,产生了一种病毒(G360突变体),其在细胞培养中的空斑大小和生长效率与NB15a相似。与YF5.2iv相比,NB15a和G360在通过Vero细胞单层传播时均受到明显限制,在C6/36细胞中受到轻度限制。在NB41A3细胞上,病毒的传播相似,但与在其他细胞系中的传播相比,这三种病毒总体上效率都较低。与YF5.2iv病毒相比,NB15a穿透不同细胞系的能力普遍受损,但仅在NB41A3细胞上检测到细胞表面结合的差异,在该细胞上NB15a的效率似乎较低。尽管NB15a空斑小、生长受损且穿透效率降低,但基于对年轻成年小鼠脑内接种后的死亡率和平均存活时间,在小鼠神经毒力测试中,NB15a与YF5.2iv并无差异。数据表明,黄热病病毒在NB41A3细胞中的持续性与E蛋白受体结合结构域的突变有关,该突变损害了病毒在细胞培养中的进入过程。然而,由于体外持续性感染而在病毒中发生的表型变化与在小鼠中枢神经系统发病机制中的减毒无关。