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首页> 外文期刊>The Journal of general virology >Vaccinia virus-free rescue of fluorescent replication-defective vesicular stomatitis virus and pseudotyping with Puumala virus glycoproteins for use in neutralization tests
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Vaccinia virus-free rescue of fluorescent replication-defective vesicular stomatitis virus and pseudotyping with Puumala virus glycoproteins for use in neutralization tests

机译:无痘苗病毒的荧光复制缺陷性水疱性口腔炎病毒的无营救和使用Puumala病毒糖蛋白的假型用于中和测试

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摘要

Puumala virus (PUUV) grows slowly in cell culture. To study antigenic properties of PUUV, an amenable method for their expression would be beneficial. To achieve this, a replication-defective recombinant vesicular stomatitis virus, rVSVΔG*EGFP, was rescued using BSRT7/5 and encephalomyocarditis virus (EMCV) internal ribosomal entry site (IRES)-enabled rescue plasmids. Using these particles, pseudotypes bearing PUUV Sotkamo strain glycoproteins were produced, with titres in the range 105–108, and were used in pseudotype focus reduction neutralization tests (pFRNTs) with neutralizing monoclonal antibodies and patient sera. The results were compared with those from orthodox focus reduction neutralization tests (oFRNTs) using native PUUV with the same samples and showed a strong positive correlation (rs?=?0.82) between the methods. While developing the system we identified three amino acids which were mutated in the Vero E6 cell culture adapted PUUV prototype Sotkamo strain sequence, and changing these residues was critical for expression and neutralizing antibody binding of PUUV glycoproteins.
机译:Puumala病毒(PUUV)在细胞培养中生长缓慢。为了研究PUUV的抗原特性,一种合适的表达方法将是有益的。为此,使用BSRT7 / 5和脑心肌炎病毒(EMCV)启用了核糖体进入位点(IRES)的救援质粒来挽救复制缺陷型重组水泡性口腔炎病毒rVSVΔG* EGFP。使用这些颗粒,可产生带有PUUV Sotkamo菌株糖蛋白的假型,滴度在105-108之间,并用于中和单克隆抗体和患者血清的假型减焦中和试验(pFRNT)。将结果与使用天然PUUV和相同样品的传统减焦中和测试(oFRNT)的结果进行比较,结果表明这两种方法之间存在很强的正相关性(rs?=?0.82)。在开发系统时,我们确定了在适应Vero E6细胞培养的PUUV原型Sotkamo菌株序列中突变的三个氨基酸,改变这些残基对于PUUV糖蛋白的表达和中和抗体结合至关重要。

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