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首页> 外文期刊>Journal of proteomics >A rapid screening method for cell lines producing singly-tagged recombinant proteins using the 'TARGET tag' system.
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A rapid screening method for cell lines producing singly-tagged recombinant proteins using the 'TARGET tag' system.

机译:使用“ TARGET标签”系统快速筛选产生单标签重组蛋白的细胞系。

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摘要

Recombinant production of extracellular glycoproteins in stable mammalian cell lines is an ideal technique for obtaining a large quantity of high-quality proteins. In most cases, however, current methodologies do not allow for sufficiently rapid cell line development and protein purification. Here, we describe a 21-residue peptide tag (designated as TARGET tag) and its use for rapid stable cell line development and purification. The ability of the anti-tag antibody P20.1 to withstand repetitive regeneration cycles has enabled the development of a sensitive surface plasmon resonance-based screening format that requires only 20 microl of cell culture supernatants. Direct and semi-quantitative screening at the 96-well culture scale eliminated the need for a second screening, re-cloning, or sorting, thereby minimizing culture pre-production time. Using this system, "high producer" cell lines were established in less than a month, and milligram quantities of target proteins could be purified with a standardized protocol.
机译:在稳定的哺乳动物细胞系中重组生产胞外糖蛋白是获得大量高质量蛋白的理想技术。但是,在大多数情况下,当前的方法无法实现足够快速的细胞系开发和蛋白质纯化。在这里,我们描述了21个残基的肽标签(称为TARGET标签)及其在快速稳定的细胞系开发和纯化中的用途。抗标签抗体P20.1承受重复再生循环的能力使得能够开发基于敏感表面等离子体共振的筛选形式,该形式仅需要20微升细胞培养上清液。在96孔培养规模上进行直接和半定量筛选,无需进行第二次筛选,重新克隆或分选,从而最大限度地缩短了培养前生产时间。使用该系统,可以在不到一个月的时间内建立“高产”细胞系,并且可以用标准化方案纯化毫克量的靶蛋白。

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