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Eliminating helper phage from phage display

机译:从噬菌体展示中消除辅助噬菌体

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摘要

Phage display technology involves the display of proteins or peptides, as coat protein fusions, on the surface of a phage or phagemid particles. Using standard technology, helper phage are essential for the replication and assembly of phagemid particles, during library production and biopanning. We have eliminated the need to add helper phage by using 'bacterial packaging cell lines' that provide the same functions. These cell lines contain M13-based helper plasmids that express phage packaging proteins which assemble phagemid particles as efficiently as helper phage, but without helper phage contamination. This results in genetically pure phagemid particle preparations. Furthermore, by using constructs differing in the form of gene 3 that they contain, we have shown that the display, from a single library, can be modulated between monovalent (phagemid-like) and multivalent display (phage-like) without any further engineering. These packaging cells eliminate the use of helper phage from phagemid-based selection protocols; reducing the amount of technical preparation, facilitating automation, optimizing selections by matching display levels to diversity, and effectively using the packaged phagemid particles as means to transfer genetic information at an efficiency approaching 100%.
机译:噬菌体展示技术涉及作为外壳蛋白融合蛋白的蛋白质或肽在噬菌体或噬菌粒颗粒表面的展示。使用标准技术,在噬菌体生产和生物淘选过程中,辅助噬菌体对于噬菌粒颗粒的复制和组装至关重要。我们已经不再需要通过使用具有相同功能的“细菌包装细胞系”来添加辅助噬菌体。这些细胞系包含基于M13的辅助质粒,该质粒表达噬菌体包装蛋白,该蛋白可像辅助噬菌体一样高效组装噬菌粒颗粒,但不会污染辅助噬菌体。这产生了遗传上纯的噬菌粒颗粒制剂。此外,通过使用它们所包含的基因3形式不同的构建体,我们已经表明,单个库中的展示可以在单价(噬菌粒样)和多价展示(噬菌体样)之间进行调节。这些包装细胞从基于噬菌粒的选择方案中消除了辅助噬菌体的使用。减少技术准备的数量,促进自动化,通过使展示水平与多样性匹配来优化选择,并有效地利用包装的噬菌粒颗粒作为转移遗传信息的手段,其效率接近100%。

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