G和F基因转移至启动子近端位置的重组呼吸道合胞病毒。
Recombinant respiratory syncytial virus with the G and F genes shifted to the promoter-proximal positions.
作者信息
Krempl Christine, Murphy Brian R, Collins Peter L
机构信息
Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, Bethesda, Maryland 20892-8007, USA.
出版信息
J Virol. 2002 Dec;76(23):11931-42. doi: 10.1128/jvi.76.23.11931-11942.2002.
The genome of human respiratory syncytial virus (RSV) encodes 10 mRNAs and 11 proteins in the order 3'-NS1-NS2-N-P-M-SH-G-F-M2-1/M2-2-L-5'. The G and F glycoproteins are the major RSV neutralization and protective antigens. It seems likely that a high level of expression of G and F would be desirable for a live RSV vaccine. For mononegaviruses, the gene order is a major factor controlling the level of mRNA and protein expression due to the polar gradient of sequential transcription. In order to increase the expression of G and F, recombinant RSVs based on strain A2 were constructed in which the G or F gene was shifted from the sixth or seventh position (in a genome lacking the SH gene), respectively, to the first position (rRSV-G1/DeltaSH and rRSV-F1/DeltaSH, respectively). Another virus was made in which G and F were shifted together to the first and second positions, respectively (rRSV-G1F2/DeltaSH). Shifting one or two genes to the promoter-proximal position resulted in increased mRNA and protein expression of the shifted genes, with G and F expression increased up to 2.4-and 7.8-fold, respectively, at the mRNA level and approximately 2.5-fold at the protein level, compared to the parental virus. Interestingly, the transcription of downstream genes was not greatly affected even though shifting G or F, or G and F together, had the consequence of moving the block of genes NS1-NS2-N-P-M-(G) one or two positions further from the promoter. The efficiency of replication of the gene shift viruses in vitro was increased up to 10-fold. However, their efficiency of replication in the lower respiratory tracts of mice was statistically indistinguishable from that of the parental virus. In the upper respiratory tract, replication was slightly reduced on some days for viruses in which G was in the first position. The magnitude of the G-specific antibody response to the gene shift viruses was similar to that to the parental virus, whereas the F-specific response was increased up to fourfold, although this was not reflected in an increase of the neutralizing activity. Thus, shifting the G and F genes to the promoter-proximal position increased virus replication in vitro, had little effect on replication in the mouse, and increased the antigen-specific immunogenicity of the virus beyond that of parental RSV.
人类呼吸道合胞病毒(RSV)的基因组按3'-NS1-NS2-N-P-M-SH-G-F-M2-1/M2-2-L-5'的顺序编码10种mRNA和11种蛋白质。G糖蛋白和F糖蛋白是RSV主要的中和及保护性抗原。对于减毒活RSV疫苗而言,似乎高水平表达G和F是很有必要的。对于单股负链RNA病毒,由于顺序转录的极性梯度,基因顺序是控制mRNA和蛋白质表达水平的主要因素。为了提高G和F的表达,构建了基于A2株的重组RSV,其中G基因或F基因分别从第六或第七位(在缺失SH基因的基因组中)移至第一位(分别为rRSV-G1/DeltaSH和rRSV-F1/DeltaSH)。还构建了另一种病毒,其中G和F分别一起移至第一位和第二位(rRSV-G1F2/DeltaSH)。将一个或两个基因移至启动子近端位置导致移位基因的mRNA和蛋白质表达增加,与亲本病毒相比,G和F的表达在mRNA水平分别增加高达2.4倍和7.8倍,在蛋白质水平约增加2.5倍。有趣的是,尽管将G或F,或G和F一起移位会导致基因块NS1-NS2-N-P-M-(G) 距离启动子再远一或两个位置,但下游基因的转录并未受到很大影响。基因移位病毒在体外的复制效率提高了10倍。然而,它们在小鼠下呼吸道中的复制效率与亲本病毒在统计学上没有差异。在上呼吸道中,对于G位于第一位的病毒,某些日子的复制略有减少。对基因移位病毒的G特异性抗体反应强度与对亲本病毒的相似,而F特异性反应增加了四倍,尽管这并未反映在中和活性的增加上。因此,将G和F基因移至启动子近端位置可增加病毒在体外的复制,对在小鼠体内的复制影响很小,并增加了病毒的抗原特异性免疫原性,超过了亲本RSV。
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