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

作者信息

Mukherjee Rudra Palash, Fruchtl McKinzie S, Beitle Robert R, Brune Ellen M

机构信息

Ralph E. Martin Department of Chemical Engineering, Bell Engineering Center, University of Arkansas, Fayetteville, AR 72701, USA.

Boston Mountain Biotech, LLC, 700W Research Center Blvd, Fayetteville, AR 72701, USA.

出版信息

Protein Expr Purif. 2018 Feb;142:32-36. doi: 10.1016/j.pep.2017.09.012. Epub 2017 Sep 27.

Abstract

This article reports on the analysis of an engineered Escherichia coli designed 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. An E. coli strain 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.

摘要

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