通过胞外域的点突变恢复羧基末端截短的伪狂犬病病毒糖蛋白B的功能。
Restoration of function of carboxy-terminally truncated pseudorabies virus glycoprotein B by point mutations in the ectodomain.
作者信息
Nixdorf R, Klupp B G, Mettenleiter T C
机构信息
Institute of Molecular Biology, Friedrich-Loeffler-Institutes, Federal Research Centre for Virus Diseases of Animals, D-17498 Insel Riems, Germany.
出版信息
J Virol. 2001 Dec;75(23):11526-33. doi: 10.1128/JVI.75.23.11526-11533.2001.
Glycoprotein B (gB) of pseudorabies virus (PrV) is essential for virus entry into target cells and direct viral cell-to-cell spread. Recently, we described a carboxy-terminally truncated derivative of PrV gB, gB-007, which was inefficiently incorporated into virions, was unable to complement infectivity, but was fully capable of restoring direct viral cell-to-cell spread of gB-negative PrV (R. Nixdorf, B. G. Klupp, and T. C. Mettenleiter, J. Virol. 74:7137-7145, 2000). Since recombinant PrV-007, which expresses gB-007 instead of wild-type gB, was able to spread directly from cell to cell, we attempted to obtain compensatory mutations leading to restoration of the entry defect by performing serial passages in cell culture. This procedure has previously been used to successfully restore entry defects in gD- or gL-deficient PrV mutants. From an initial titer of 100 PFU per ml in the supernatant, titers increased, reaching wild-type levels of up to 10(7) PFU after ca. 20 passages. One single-plaque isolate of the passaged mutant, designated PrV-007Pass, was further characterized. PrV-007Pass gB was efficiently incorporated into the viral envelope and restored infectivity to a gB-negative PrV mutant, PrV-gB(-). Interestingly, localization of PrV-007Pass gB in the plasma membrane was similar to that of PrV-007. In contrast, wild-type gB is mainly found in intracellular vesicles. Marker rescue experiments and trans-complementation assays demonstrated the presence of compensatory mutations within the gB gene of PrV-007Pass. DNA sequencing revealed two point mutations in the gB open reading frame of PrV-007Pass, resulting in amino acid substitutions at positions 305 and 744 of gB, both of which are required for compensation of the defect in PrV-007. Our data again demonstrate the power of reversion analysis of herpesviruses and suggest that cytosolic and ectodomains play a role in incorporation of gB into virions.
伪狂犬病病毒(PrV)的糖蛋白B(gB)对于病毒进入靶细胞以及病毒在细胞间的直接传播至关重要。最近,我们描述了一种PrV gB的羧基末端截短衍生物gB - 007,它低效地掺入病毒粒子中,无法补充感染性,但完全能够恢复gB阴性PrV的病毒细胞间直接传播(R. Nixdorf,B. G. Klupp,和T. C. Mettenleiter,《病毒学杂志》74:7137 - 7145,2000)。由于表达gB - 007而非野生型gB的重组PrV - 007能够在细胞间直接传播,我们试图通过在细胞培养中进行连续传代来获得导致恢复进入缺陷的补偿性突变。该方法先前已成功用于恢复gD或gL缺陷的PrV突变体中的进入缺陷。上清液中初始滴度为每毫升100个空斑形成单位(PFU),滴度增加,约20代后达到高达10⁷ PFU的野生型水平。对传代突变体的一个单斑分离株,命名为PrV - 007Pass,进行了进一步表征。PrV - 007Pass gB有效地掺入病毒包膜中,并恢复了gB阴性PrV突变体PrV - gB(-)的感染性。有趣的是,PrV - 007Pass gB在质膜中的定位与PrV - 007相似。相比之下,野生型gB主要存在于细胞内囊泡中。标记拯救实验和反式互补分析证明了PrV - 007Pass的gB基因内存在补偿性突变。DNA测序揭示了PrV - 007Pass的gB开放阅读框中的两个点突变,导致gB第305和744位氨基酸替换,这两个替换都是补偿PrV - 007缺陷所必需的。我们的数据再次证明了疱疹病毒回复分析的作用,并表明胞质和胞外结构域在gB掺入病毒粒子中起作用。
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