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Development of a novel engineered E.?coli host cell line platform with improved column capacity performance for ion-exchange chromatography

机译:开发新颖的工程化 e.?coli 宿主细胞系平台,具有改进的离子交换色谱柱容量性能

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AbstractThis article reports on the analysis of an engineeredEscherichia colidesigned to reduce the host cell protein (HCP) burden on recombinant protein purification by column chromatography. Since downstream purification accounts for a major portion of production costs when using a recombinant platform, minimization of HCPs that are initially captured or otherwise interfere during chromatography will positively impact the entire purification process. Such a strategy, of course, would also require the cell line to grow, and express recombinant proteins, at levels comparable to, or better than, its parent strain. AnE.?colistrain with a small number of strategic deletions (LTSF06) was transformed to produce three different recombinant biologics to examine growth and expression, and with another model protein to assess growth and the effect of selectively reduced HCPs on target product capture on DEAE ion exchange medium. Cell growth levels were maintained or increased for all constructs, and a significant reduction in HCP adsorption was realized. Indeed, a breakthrough analysis indicated that as a result of reducing adsorption of particular HCPs, a 37% increase in target protein capture was observed. This increase in product capture efficiency was achieved by focusing not on HCPs that co-elute with the recombinant target, but rather on those possessing particular column adsorption and elution characteristics.
机译:<![CDATA [ 抽象 本文有关工程化的分析 echerichia coli 设计通过柱色谱法降低重组蛋白质纯化的宿主细胞蛋白(HCP)负担。由于下游净化占生产成本的主要部分,当使用重组平台时,最小化最初捕获或在色谱期间干扰的HCP将积极影响整个净化过程。当然,这种策略还将需要细胞系来生长,并且表达重组蛋白,其水平与其亲本菌株相当或更好。转化具有少量战略缺失(LTSF06)的斜体>菌株,以产生三种不同的重组生物制剂,以检查生长和表达,以及另一种模型蛋白质评估生长和评估生长选择性降低HCP对DEAE离子交换介质对目标产品捕获的影响。对于所有构建体保持或增加细胞生长水平,并且实现了HCP吸附的显着降低。实际上,突破分析表明,由于减少特定HCP的吸附,观察到目标蛋白质捕获的增加37%。通过专注于与重组目标共同洗脱的HCP来实现产品捕获效率的这种增加,而是实现了具有特定柱吸附和洗脱特性的HCP。

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