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首页> 外文期刊>Archives of virology >Improved detection of Beet necrotic yellow vein virus in a DAS ELISA by means of antibody single chain fragments (scFv) which were selected to protease-stable epitopes from phage display libraries.
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Improved detection of Beet necrotic yellow vein virus in a DAS ELISA by means of antibody single chain fragments (scFv) which were selected to protease-stable epitopes from phage display libraries.

机译:通过抗体单链片段(scFv)改进了DAS ELISA中甜菜坏死黄静脉病毒的检测,该抗体从噬菌体展示库中选择为蛋白酶稳定的表位。

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摘要

The detection of Beet necrotic yellow vein virus (BNYVV) in stored sugar beets by means of monoclonal antibodies or antibody single chain fragments (scFv) often poses problems, because the immunodominant C-terminal epitope of the viral coat protein is readily lost due to proteolysis. Clones which produce scFv specific for protease-stable BNYVV epitopes were selected from two naive phage display libraries.Fusion proteins of the scFv with a human IgG kappa chain (expressed from the newly designed vector pCL) or with alkaline phosphatase,respectively, allow the ELISA detection of BNYVV even in stored sugar beets with a sensitivity which was comparable or often higher than that achieved with polyclonal antibodies.
机译:通过单克隆抗体或抗体单链片段(scFv)检测存储的甜菜中的甜菜坏死黄脉病毒(BNYVV)通常会带来问题,因为病毒外壳蛋白的免疫优势C端表位容易由于蛋白水解而丢失。从两个幼稚的噬菌体展示文库中选择产生对蛋白酶稳定的BNYVV表位特异的scFv的克隆。分别具有人IgG kappa链(从新设计的载体pCL表达)或碱性磷酸酶的scFv融合蛋白可以通过ELISA即使在储存的甜菜中也能检测到BNYVV,其灵敏度与多克隆抗体相当或更高。

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