Herrold R E, Marchini A, Fruehling S, Longnecker R
Department of Microbiology--Immunology, Northwestern University Medical School, Chicago, Illinois 60611, USA.
J Virol. 1996 Mar;70(3):2049-54. doi: 10.1128/JVI.70.3.2049-2054.1996.
The Epstein-Barr virus (EBV) glycoprotein gp110 has substantial amino acid homology to gB of herpes simplex virus but localizes differently within infected cells and is essentially undetectable in virions. To investigate whether gp110, like gB, is essential for EBV infection, a selectable marker was inserted within the gp110 reading frame, BALF4, and the resulting null mutant EBV stain, B95-110HYG, was recovered in lymphoblastoid cell lines (LCLs). While LCLs infected with the parental virus B95-8 expressed the gp110 protein product following productive cycle induction, neither full-length gp110 nor the predicted gp110 truncation product was detectable in B95-110HYG LCLs. Infectious virus could not be recovered from B95-110HYG LCLs unless gp110 was provided in trans. Rescued B95-110HYG virus latently infected and growth transformed primary B lymphocytes. Thus, gp110 is required for the production of transforming virus but not for the maintenance of transformation of primary B lymphocytes by EBV.
爱泼斯坦-巴尔病毒(EBV)糖蛋白gp110与单纯疱疹病毒的gB具有大量氨基酸同源性,但在受感染细胞内的定位不同,且在病毒粒子中基本检测不到。为了研究gp110是否像gB一样对EBV感染至关重要,在gp110阅读框BALF4内插入了一个选择标记,然后在淋巴母细胞系(LCLs)中获得了产生的无功能突变EBV毒株B95-110HYG。虽然感染亲本病毒B95-8的LCLs在生产性周期诱导后表达gp110蛋白产物,但在B95-110HYG LCLs中既检测不到全长gp110,也检测不到预测的gp110截短产物。除非通过反式提供gp110,否则无法从B95-110HYG LCLs中回收感染性病毒。拯救后的B95-110HYG病毒潜伏感染并生长转化原代B淋巴细胞。因此,gp110是产生转化病毒所必需的,但不是EBV维持原代B淋巴细胞转化所必需的。
