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通过一种简单的两步策略纯化毕赤酵母中产生的重组植物过氧化物酶。

Purification of a recombinant plant peroxidase produced in Pichia pastoris by a simple 2-step strategy.

作者信息

Spadiut Oliver, Rossetti Laura, Dietzsch Christian, Herwig Christoph

机构信息

Vienna University of Technology, Institute of Chemical Engineering, Research Area Biochemical Engineering, Vienna, Austria.

出版信息

Protein Expr Purif. 2012 Dec;86(2):89-97. doi: 10.1016/j.pep.2012.09.008. Epub 2012 Sep 28.

Abstract

The enzyme horseradish peroxidase (HRP), which is frequently applied in industry and medicine, is primarily isolated from plant. This purification procedure is costly and the obtainable amount of HRP from the horseradish root is low. However, recombinant HRP (rHRP) produced in yeast is hyperglycosylated rendering the subsequent purification cumbersome and the recombinant production of HRP in yeast not competitive. In this study, we screened different common techniques to develop a fast and efficient purification strategy for hyperglycosylated rHRP expressed in Pichia pastoris. We demonstrated that the extensive glycosylation pattern on the surface of rHRP masked its physico-chemical properties, which is why standard purification strategies were rather unsuccessful. Only switching the strategies to a flowthrough mode gave satisfactory results. After determining the optimal operation conditions in a multivariate Design of Experiments approach, we present a simple 2-step strategy for the purification of hyperglycosylated rHRP. Combining a hydrophobic charge induction chromatography operated in flowthrough mode and a size-exclusion chromatography, we were able to purify rHRP more than 12-fold from a specific activity of 80U/mg to more than 1000U/mg.

摘要

辣根过氧化物酶(HRP)这种酶常用于工业和医学领域,主要从植物中分离得到。这种纯化过程成本高昂,且从辣根中可获得的HRP量很低。然而,酵母中产生的重组HRP(rHRP)高度糖基化,使得后续纯化过程繁琐,并且在酵母中重组生产HRP缺乏竞争力。在本研究中,我们筛选了不同的常用技术,以开发一种针对毕赤酵母中表达的高度糖基化rHRP的快速高效纯化策略。我们证明,rHRP表面广泛的糖基化模式掩盖了其物理化学性质,这就是标准纯化策略相当不成功的原因。只有将策略转换为流通模式才能得到令人满意的结果。在通过多变量实验设计方法确定最佳操作条件后,我们提出了一种简单的两步策略来纯化高度糖基化的rHRP。结合以流通模式运行的疏水电荷诱导色谱法和尺寸排阻色谱法,我们能够将rHRP的比活性从80U/mg纯化至超过1000U/mg,纯化倍数超过12倍。

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