A protocol for setting-up robust hydrophobic interaction chromatography targeting the analysis of intact proteins and monoclonal antibodies

IF 3 Q2 CHEMISTRY, ANALYTICAL Analytical science advances Pub Date : 2022-12-24 DOI:10.1002/ansa.202200058
Raphael Ewonde Ewonde, Nico Lingg, Daniel Eßer, Sebastiaan Eeltink
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Abstract

Hydrophobic interaction chromatography (HIC) is a chromatographic technique that mainly targets the separation of biomolecules (intact proteins, monoclonal antibodies, etc.) based on the difference in surface hydrophobicity while applying non-denaturing conditions. This protocol paper provides guidelines for setting-up robust HIC analysis and considers the instrument configuration, mobile-phase and sample preparation, as well as chromatographic conditions and settings. The separation of a mixture of intact proteins and monoclonal antibodies is demonstrated by applying conventional HIC conditions, that is, using a mildly hydrophobic (C4) stationary phase in combination with an inverse ammonium sulphate gradient dissolved in aqueous phosphate buffer. The effect of sample-preparation conditions on sample breakthroughs is presented. Finally, good run-to-run repeatability (relative standard deviation < 2%) is demonstrated for five different columns obtained from three different column lots, considering chromatographic retention, peak width, peak area and column pressure.

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建立针对完整蛋白和单克隆抗体分析的稳健疏水相互作用色谱的方案
疏水相互作用色谱(HIC)是在非变性条件下,基于表面疏水性的差异,对生物分子(完整蛋白、单克隆抗体等)进行分离的一种色谱技术。本协议文件提供了建立稳健的HIC分析的指导方针,并考虑了仪器配置,流动相和样品制备,以及色谱条件和设置。完整蛋白和单克隆抗体混合物的分离是通过应用传统的HIC条件来证明的,即使用轻度疏水(C4)固定相结合反硫酸铵梯度溶解在磷酸盐缓冲液中。介绍了样品制备条件对样品突破的影响。最后,良好的运行重复性(相对标准偏差<在考虑色谱保留、峰宽、峰面积和柱压的情况下,对从3个不同色谱批次获得的5个不同色谱进行了2%的验证。
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