七肽重复区的残基调节仙台病毒在小鼠中的毒力。
Residues in the heptad repeat a region of the fusion protein modulate the virulence of Sendai virus in mice.
机构信息
Division of Virology, Department of Infectious Diseases, MS 330, St. Jude Children's Research Hospital, 262 Danny Thomas Place, Memphis, TN 38105-3678, USA.
出版信息
J Virol. 2010 Jan;84(2):810-21. doi: 10.1128/JVI.01990-09. Epub 2009 Nov 11.
While the molecular basis of fusion (F) protein refolding during membrane fusion has been studied extensively in vitro, little is known about the biological significance of membrane fusion activity in parainfluenza virus replication and pathogenesis in vivo. Two recombinant Sendai viruses, F-L179V and F-K180Q, were generated that contain F protein mutations in the heptad repeat A region of the ectodomain, a region of the protein known to regulate F protein activation. In vitro, the F-L179V virus caused increased syncytium formation (cell-cell membrane fusion) yet had a rate of replication and levels of F protein expression and cleavage similar to wild-type virus. The F-K180Q virus had a reduced replication rate along with reduced levels of F protein expression, cleavage, and fusogenicity. In DBA/2 mice, the hyperfusogenic F-L179V virus induced greater morbidity and mortality than wild-type virus, while the attenuated F-K180Q virus was much less pathogenic. During the first week of infection, virus replication and inflammation in the lungs were similar for wild-type and F-L179V viruses. After approximately 1 week of infection, the clearance of F-L179V virus was delayed, and more extensive interstitial inflammation and necrosis were observed in the lungs, affecting entire lobes of the lungs and having significantly greater numbers of syncytial cell masses in alveolar spaces on day 10. On the other hand, the slower-growing F-K180Q virus caused much less extensive inflammation than wild-type virus, presumably due to its reduced replication rate, and did not cause observable syncytium formation in the lungs. Overall, the results show that residues in the heptad repeat A region of the F protein modulate the virulence of Sendai virus in mice by influencing both the spread and clearance of the virus and the extent and severity of inflammation. An understanding of how the F protein contributes to infection and inflammation in vivo may assist in the development of antiviral therapies against respiratory paramyxoviruses.
虽然融合(F)蛋白在膜融合过程中重折叠的分子基础已在体外得到广泛研究,但对于副粘病毒在体内复制和发病机制中膜融合活性的生物学意义知之甚少。生成了两种含有 F 蛋白在其胞外域七肽重复 A 区突变的重组仙台病毒,F-L179V 和 F-K180Q,该蛋白区域已知调节 F 蛋白的激活。在体外,F-L179V 病毒引起了更多的合胞体形成(细胞-细胞膜融合),但其复制率以及 F 蛋白的表达和切割水平与野生型病毒相似。F-K180Q 病毒的复制率降低,同时 F 蛋白的表达、切割和融合能力降低。在 DBA/2 小鼠中,高融合性的 F-L179V 病毒引起的发病率和死亡率高于野生型病毒,而衰减的 F-K180Q 病毒的致病性要低得多。在感染的第一周,野生型和 F-L179V 病毒的肺部病毒复制和炎症相似。大约感染后 1 周,F-L179V 病毒的清除被延迟,并且在肺部观察到更广泛的间质炎症和坏死,影响整个肺叶,在第 10 天肺泡空间中具有显著更多的合胞体细胞块。另一方面,生长缓慢的 F-K180Q 病毒引起的炎症比野生型病毒少得多,这可能是由于其复制率降低,并且在肺部不会引起可观察到的合胞体形成。总体而言,结果表明 F 蛋白七肽重复 A 区的残基通过影响病毒的传播和清除以及炎症的程度和严重程度来调节仙台病毒在小鼠中的毒力。了解 F 蛋白如何有助于体内感染和炎症可能有助于开发针对呼吸道副粘病毒的抗病毒疗法。
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