Lee E, Stocks C E, Amberg S M, Rice C M, Lobigs M
Division of Immunology and Cell Biology, John Curtin School of Medical Research, The Australian National University, Canberra, Australian Capital Territory 2601, Australia.
J Virol. 2000 Jan;74(1):24-32. doi: 10.1128/jvi.74.1.24-32.2000.
Proteolytic processing at the C-prM junction in the flavivirus polyprotein involves coordinated cleavages at the cytoplasmic and luminal sides of an internal signal sequence. We have introduced at the COOH terminus of the yellow fever virus (YFV) prM signal sequence amino acid substitutions (VPQAQA mutation) which uncoupled efficient signal peptidase cleavage of the prM protein from its dependence on prior cleavage in the cytoplasm of the C protein mediated by the viral NS2B-3 protease. Infectivity assays with full-length YFV RNA transcripts showed that the VPQAQA mutation, which enhanced signal peptidase cleavage in vitro, was lethal for infectious virus production. Revertants or second-site mutants were recovered from cells transfected with VPQAQA RNA. Analysis of these viruses revealed that single amino acid substitutions in different domains of the prM signal sequence could restore viability. These variants had growth properties in vertebrate cells which differed only slightly from those of the parent virus, despite efficient signal peptidase cleavage of prM in cell-free expression assays. However, the neurovirulence in mice of the VPQAQA variants was significantly attenuated. This study demonstrates that substitutions in the prM signal sequence which disrupt coordinated cleavages at the C-prM junction can impinge on the biological properties of the mutant viruses. Factors other than the rate of production of prM are vitally controlled by regulated cleavages at this site.
黄病毒多聚蛋白中C-prM连接处的蛋白水解加工涉及内部信号序列细胞质侧和腔侧的协同切割。我们在黄热病毒(YFV)prM信号序列的COOH末端引入了氨基酸取代(VPQAQA突变),该突变使prM蛋白的有效信号肽酶切割与其对病毒NS2B-3蛋白酶介导的C蛋白在细胞质中先前切割的依赖性脱钩。对全长YFV RNA转录本的感染性测定表明,在体外增强信号肽酶切割的VPQAQA突变对感染性病毒的产生是致命的。从用VPQAQA RNA转染的细胞中回收了回复突变体或第二位点突变体。对这些病毒的分析表明,prM信号序列不同结构域中的单个氨基酸取代可以恢复活力。尽管在无细胞表达试验中prM有有效的信号肽酶切割,但这些变体在脊椎动物细胞中的生长特性与亲本病毒的生长特性仅略有不同。然而,VPQAQA变体在小鼠中的神经毒力明显减弱。这项研究表明,prM信号序列中的取代破坏了C-prM连接处的协同切割,可能会影响突变病毒的生物学特性。除了prM的产生速率外,其他因素在该位点的调控切割中也至关重要。