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Production of monoclonal antibodies against hepatitis E virus capsid protein and evaluation of their neutralizing activity in a cell culture system.

机译:抗戊型肝炎病毒衣壳蛋白的单克隆抗体的生产及其在细胞培养系统中的中和活性评估。

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摘要

Nine murine monoclonal antibodies (mAbs) generated against a recombinant ORF2 protein (amino acids 111-660) of a genotype 4 hepatitis E virus (HEV) strain recognized four sets of epitopes by pairwise competitive ELISA. One mAb (H6225) was able to capture HEV efficiently regardless of genotype and was tested for its ability to neutralize a genotype 3 HEV strain (JE03-1760F) in a recently developed cell culture system for HEV in a hepatocarcinoma cell line (PLC/PRF/5). When PLC/PRF/5 cells were inoculated with HEV (4.0 x 10(5) or 4.0 x 10(6) copies/ml) incubated with 100 mug/ml of a negative control mAb, HEV RNA in the culture medium continued to be detectable after day 14 or 12 post-inoculation (dpi), respectively. However, when cells were inoculated with the two distinct concentrations of HEV that had been mixed with 100 mug/ml of H6225, the harvested culture supernatants were negative for HEV RNA throughout the 60-day observation period. Upon prior mixing of the virus with 10 mug/ml of H6225, HEV RNA in culture supernatant continued to be undetectable until 46 or 28 dpi, respectively. In conclusion, one mAb (H6225) against HEV capsid protein that can efficiently neutralize HEV in vitro was obtained in the present study.
机译:针对成对的4型戊型肝炎病毒(HEV)株的重组ORF2蛋白(氨基酸111-660)生成的九种鼠类单克隆抗体(mAb)通过成对竞争ELISA识别了四组表位。一种mAb(H6225)能够有效捕获HEV,而与基因型无关,并已在最近开发的肝癌细胞系(PLC / PRF)的HEV细胞培养系统中测试了其中和基因型3 HEV株(JE03-1760F)的能力。 / 5)。当PLC / PRF / 5细胞接种HEV(4.0 x 10(5)或4.0 x 10(6)拷贝/ ml)与100杯/ ml阴性对照mAb孵育时,培养基中的HEV RNA继续分别在接种后第14天或第12天可检测到。但是,当用两种不同浓度的HEV接种细胞后,混合了100杯/ ml的H6225,在整个60天的观察期内,收获的培养上清液对HEV RNA均为阴性。事先将病毒与10杯/毫升的H6225混合后,培养上清液中的HEV RNA分别持续检测到46或28 dpi。综上所述,本研究获得了一种抗HEV衣壳蛋白的单抗(H6225),可以在体外有效中和HEV。

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