Expanded bed chromatography of proteins in small-diameter columns. II. Methods development and scale up.

S Ghose, H Chase
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引用次数: 16

Abstract

The scaled down system developed in Part I of this series was further validated by using a 1-cm diameter column for method development studies for the separation of two model proteins, alcohol dehydrogenase and alpha-glucosidase, from unclarified yeast homogenate by hydrophobic interaction expanded bed chromatography based on the STREAMLINE matrix. The efficacy of solids removal and establishment of optimal binding and separation condition by stepwise elution were investigated. Equilibration of the EBA column and loading at high salt strengths affected the subsequent recovery of the two target proteins. Although good resolution between the target proteins could be achieved, peak tailing was found to be a consistent problem. The optimised separation protocol was scaled up 25-fold to a column diameter of 5.0 cm. The results were in good agreement with the run conducted in the 1-cm column, indicating the potential of using the small columns as an viable approach for method scouting and development studies.

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小直径柱中蛋白质的扩展床层析。2方法开发和推广。
本系列第一部分中开发的缩小系统通过使用直径1厘米的柱进行方法开发研究,进一步验证了基于streamlined基质的疏水相互作用扩展床层析,从未澄清的酵母均质液中分离两种模型蛋白,醇脱氢酶和α -葡萄糖苷酶。研究了分步洗脱法去除固体的效果,并建立了最佳结合分离条件。EBA柱的平衡和在高盐强度下的负载影响了两个目标蛋白的随后恢复。虽然目标蛋白之间可以实现很好的分辨,但发现峰尾是一个一致的问题。将优化后的分离方案放大25倍至柱径5.0 cm。结果与在1厘米柱中进行的运行很好地一致,表明使用小柱作为方法寻找和开发研究的可行方法的潜力。
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