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Establishment of a rescue system for porcine parvovirus using a seamless cloning method

机译:使用无缝克隆方法建立猪剖视病毒的救援系统

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In this study, we describe a novel and rapid method for the construction of a full-length infectious clone (pPPV). The constructed clone contained an engineered EcoRv site that served as a genetic marker and was shown to be infectious when transfected into a monolayer of PK-15 cells. The rescued virus (rPPV) of the infectious clone was found to be indistinguishable from wild-type virus BQ in terms of its biological properties. The generation of this PPV infectious clone provides a potentially powerful tool with which to elucidate the molecular pathogenesis of PPV.
机译:在这项研究中,我们描述了一种用于构建全长传染性克隆(PPPV)的新型和快速方法。 构造的克隆含有用于遗传标记的工程化ECORV位点,当转染到PK-15细胞的单层时,显示出感染。 在其生物学特性方面,发现感染性克隆的救出病毒(RPPV)与野生型病毒BQ无法区分。 这种PPV传染性克隆的产生提供了一种潜在的强大工具,可以阐明PPV的分子发病机制。

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