单纯疱疹病毒1型开放阅读框O和P对于在小鼠中建立潜伏感染并非必需。
Herpes simplex virus 1 open reading frames O and P are not necessary for establishment of latent infection in mice.
作者信息
Randall G, Lagunoff M, Roizman B
机构信息
The Marjorie B. Kovler Viral Oncology Laboratories, The University of Chicago, Chicago, Illinois 60637, USA.
出版信息
J Virol. 2000 Oct;74(19):9019-27. doi: 10.1128/jvi.74.19.9019-9027.2000.
Open reading frame (ORF) O and ORF P partially overlap and are located antisense to the gamma(1)34.5 gene within the domain transcribed during latency. In wild-type virus-infected cells, ORF O and ORF P are completely repressed during productive infection by ICP4, the major viral transcriptional activator/repressor. In cells infected with a mutant in which ORF P was derepressed there was a significant delay in the appearance of the viral alpha-regulatory proteins ICP0 and ICP22. The ORF O protein binds to and inhibits ICP4 binding to its cognate DNA site in vitro. These characteristics suggested a role for ORF O and ORF P in the establishment of latency. To test this hypothesis, two recombinant viruses were constructed. In the first, R7538(P-/O-), the ORF P initiator methionine codon, which also serves as the initiator methionine codon for ORF O, was replaced and a diagnostic restriction endonuclease was introduced upstream. In the second, R7543(P-/O-)R, the mutations were repaired to restore the wild-type virus sequences. We report the following. (i) The R7538(P-/O-) mutant failed to express ORF O and ORF P proteins but expressed a wild-type gamma(1)34.5 protein. (ii) R7538(P-/O-) yields were similar to that of the wild type following infection of cell culture or following infection of mice by intracerebral or ocular routes. (iii) R7538(P-/O-) virus reactivated from latency following explanation and cocultivation of murine trigeminal ganglia with Vero cells at a frequency similar to that of the wild type, herpes simplex virus 1(F). (iv) The amount of latent R7538(P-/O-) virus as assayed by quantitative PCR is eightfold less than that of the repair virus. The repaired virus could not be differentiated from the wild-type parent in any of the assays done in this study. We conclude that ORF O and ORF P are not essential for the establishment of latency in mice but may play a role in determining the quantity of latent virus maintained in sensory neurons.
开放阅读框(ORF)O和ORF P部分重叠,且位于潜伏期转录区域内与γ(1)34.5基因反义的位置。在野生型病毒感染的细胞中,在生产性感染期间,主要的病毒转录激活因子/抑制因子ICP4会完全抑制ORF O和ORF P。在感染了ORF P被解除抑制的突变体的细胞中,病毒α调节蛋白ICP0和ICP22的出现有显著延迟。ORF O蛋白在体外能结合并抑制ICP4与其同源DNA位点的结合。这些特性表明ORF O和ORF P在潜伏期的建立中起作用。为了验证这一假设,构建了两种重组病毒。第一种是R7538(P-/O-),其中作为ORF O起始甲硫氨酸密码子的ORF P起始甲硫氨酸密码子被替换,并在其上游引入了一种诊断性限制性内切酶。第二种是R7543(P-/O-)R,修复了突变以恢复野生型病毒序列。我们报告如下:(i)R7538(P-/O-)突变体未能表达ORF O和ORF P蛋白,但表达野生型γ(1)34.5蛋白。(ii)在细胞培养感染后或通过脑内或眼内途径感染小鼠后,R7538(P-/O-)的产量与野生型相似。(iii)在对小鼠三叉神经节进行解释并与Vero细胞共培养后,R7538(P-/O-)病毒从潜伏期重新激活,频率与野生型单纯疱疹病毒1(F)相似。(iv)通过定量PCR检测,潜伏的R7538(P-/O-)病毒量比修复病毒少八倍。在本研究进行的任何检测中,修复病毒与野生型亲本无法区分。我们得出结论,ORF O和ORF P对于小鼠潜伏期的建立不是必需的,但可能在决定感觉神经元中潜伏病毒的数量方面起作用。
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