Hosie Margaret J, Willett Brian J, Klein Dieter, Dunsford Thomas H, Cannon Celia, Shimojima Masayuki, Neil James C, Jarrett Oswald
Department of Veterinary Pathology, University of Glasgow, Glasgow G61 1QH, United Kingdom.
J Virol. 2002 Jun;76(12):6062-72. doi: 10.1128/jvi.76.12.6062-6072.2002.
The development of an effective vaccine against human immunodeficiency virus is considered to be the most practicable means of controlling the advancing global AIDS epidemic. Studies with the domestic cat have demonstrated that vaccinal immunity to infection can be induced against feline immunodeficiency virus (FIV); however, protection is largely restricted to laboratory strains of FIV and does not extend to primary strains of the virus. We compared the pathogenicity of two prototypic vaccine challenge strains of FIV derived from molecular clones; the laboratory strain PET(F14) and the primary strain GL8(414). PET(F14) established a low viral load and had no effect on CD4(+)- or CD8(+)-lymphocyte subsets. In contrast, GL8(414) established a high viral load and induced a significant reduction in the ratio of CD4(+) to CD8(+) lymphocytes by 15 weeks postinfection, suggesting that PET(F14) may be a low-virulence-challenge virus. However, during long-term monitoring of the PET(F14)-infected cats, we observed the emergence of variant viruses in two of three cats. Concomitant with the appearance of the variant viruses, designated 627(W135) and 628(W135,) we observed an expansion of CD8(+)-lymphocyte subpopulations expressing reduced CD8 beta-chain, a phenotype consistent with activation. The variant viruses both carried mutations that reduced the net charge of the V3 loop (K409Q and K409E), giving rise to a reduced ability of the Env proteins to both induce fusion and to establish productive infection in CXCR4-expressing cells. Further, following subsequent challenge of naïve cats with the mutant viruses, the viruses established higher viral loads and induced more marked alterations in CD8(+)-lymphocyte subpopulations than did the parent F14 strain of virus, suggesting that the E409K mutation in the PET(F14) strain contributes to the attenuation of the virus.
开发一种有效的抗人类免疫缺陷病毒疫苗被认为是控制全球艾滋病疫情蔓延的最可行手段。对家猫的研究表明,针对猫免疫缺陷病毒(FIV)可诱导产生抗感染的疫苗免疫;然而,保护作用在很大程度上仅限于FIV的实验室毒株,并不适用于该病毒的原始毒株。我们比较了两种源自分子克隆的FIV原型疫苗攻击毒株的致病性;实验室毒株PET(F14)和原始毒株GL8(414)。PET(F14)建立了低病毒载量,对CD4(+)或CD8(+)淋巴细胞亚群没有影响。相比之下,GL8(414)建立了高病毒载量,并在感染后15周导致CD4(+)与CD8(+)淋巴细胞的比例显著降低,这表明PET(F14)可能是一种低毒力攻击病毒。然而,在对感染PET(F14)的猫进行长期监测期间,我们在三只猫中的两只身上观察到了变异病毒的出现。与命名为627(W135)和628(W135)的变异病毒出现同时,我们观察到表达减少的CD8β链的CD8(+)淋巴细胞亚群扩大,这是一种与激活一致的表型。这两种变异病毒都携带了降低V3环净电荷的突变(K409Q和K409E),导致Env蛋白诱导融合以及在表达CXCR4的细胞中建立有效感染的能力降低。此外,在用突变病毒对未感染的猫进行后续攻击后,这些病毒建立了更高的病毒载量,并比亲本F14病毒株在CD8(+)淋巴细胞亚群中诱导了更明显的变化,这表明PET(F14)毒株中的E409K突变导致了病毒的减毒。