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亨德拉病毒包膜糖蛋白的功能表达及膜融合嗜性

Functional expression and membrane fusion tropism of the envelope glycoproteins of Hendra virus.

作者信息

Bossart K N, Wang L F, Eaton B T, Broder C C

机构信息

Department of Microbiology, Uniformed Services University, Bethesda, Maryland 20814, USA.

出版信息

Virology. 2001 Nov 10;290(1):121-35. doi: 10.1006/viro.2001.1158.

Abstract

Hendra virus (HeV) is an emerging paramyxovirus first isolated from cases of severe respiratory disease that fatally affected both horses and humans. Understanding the mechanisms of host cell infection and cross-species transmission is an important step in addressing the risk posed by such emerging pathogens. We have initiated studies to characterize the biological properties of the HeV envelope glycoproteins. Recombinant vaccinia viruses encoding the HeV F and G open reading frames were generated and glycoprotein expression was verified by metabolic labeling and detection using specific antisera. Glycoprotein function and cellular tropism were examined with a quantitative assay for HeV-mediated membrane fusion. Fusion specificity was verified through specific inhibition by anti-HeV antiserum and a peptide corresponding to one of the alpha-helical heptad repeats of F. HeV requires both F and G to mediate fusion. Permissive target cells have been identified, including cell lines derived from cat, bat, horse, human, monkey, mouse, and rabbit. Fusion negative cell types have also been identified. Protease treatments of the target cells abolished fusion activity, suggesting that the virus is employing a cell-surface protein as its receptor.

摘要

亨德拉病毒(HeV)是一种新出现的副粘病毒,最初从严重呼吸道疾病病例中分离出来,这些病例对马和人类均造成致命影响。了解宿主细胞感染和跨物种传播的机制是应对此类新出现病原体所带来风险的重要一步。我们已启动研究,以表征HeV包膜糖蛋白的生物学特性。构建了编码HeV F和G开放阅读框的重组痘苗病毒,并通过代谢标记和使用特异性抗血清进行检测来验证糖蛋白的表达。通过对HeV介导的膜融合进行定量测定来检查糖蛋白功能和细胞嗜性。通过抗HeV抗血清和对应于F的α-螺旋七肽重复序列之一的肽的特异性抑制来验证融合特异性。HeV需要F和G两者来介导融合。已鉴定出允许性靶细胞,包括源自猫、蝙蝠、马、人、猴、小鼠和兔的细胞系。也已鉴定出融合阴性细胞类型。对靶细胞进行蛋白酶处理消除了融合活性,这表明该病毒利用一种细胞表面蛋白作为其受体。

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