Article Purification of His-tagged proteins using printed monolith adsorption columns

化学 整体 色谱法 亲和层析 吸附 溶解 蛋白质纯化 整体式高效液相色谱柱 亚氨基二乙酸 洗脱 膨胀床吸附 高分子 高效液相色谱法 生物化学 金属 有机化学 催化作用
作者
Sean Feast,James Titterington,Viet-Anh Hoang,Timothy M. Allison,Conan J. Fee,Ali Reza Nazmi
出处
期刊:Journal of Chromatography A [Elsevier BV]
卷期号:1733: 465216-465216 被引量:2
标识
DOI:10.1016/j.chroma.2024.465216
摘要

Bio-separation is a crucial process in biotechnology and biochemical engineering for separating biological macromolecules, and the field has long relied on bead-based and expanded bed chromatography. Printed monolith adsorption (PMA) is a new alternative to which uses a 3D-printed monolithic structure containing self-supporting, ordered flow channels. PMA allows for direct purification of biological molecules from crude cell lysates and cell cultures, and like the other technologies, can functionalized to specifically target a molecule and enable affinity chromatography. Here we have combined PMA technology with an immobilized metal affinity ligand (iminodiacetic acid) to provide selectivity of binding to polyhistidine-tagged proteins during PMA chromatography. Two different PMA structures were created and tested for both static and dynamic protein-binding capacity. At comparative linear flow rates, the dynamic binding capacity of both columns was ≈3 mg/mL, while static capacity was shown to differentiate based on column voidage. We show that a polyhistidine-tagged protein can be directly purified from crude lysate with comparable results to the available commercial providers of IMAC, and with a substantially reduced purification time.

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