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聚乙二醇(PEG)链长影响固相蛋白 PEG 化的产率和离子交换色谱法分离 PEG 化蛋白的效率:机制模型的见解。

PEG chain length impacts yield of solid-phase protein PEGylation and efficiency of PEGylated protein separation by ion-exchange chromatography: insights of mechanistic models.

机构信息

School of Engineering and Graduate School of Medicine, Yamaguchi University, Ube, Japan.

出版信息

Biotechnol J. 2013 Jul;8(7):801-10. doi: 10.1002/biot.201200325. Epub 2013 Jun 21.

DOI:10.1002/biot.201200325
PMID:23788446
Abstract

The mechanisms behind protein PEGylation are complex and dictated by the structure of the protein reactant. Hence, it is difficult to design a reaction process which can produce the desired PEGylated form at high yield. Likewise, efficient purification processes following protein PEGylation must be constructed on an ad hoc basis for each product. The retention and binding mechanisms driving electrostatic interaction-based chromatography (ion-exchange chromatography) of PEGylated proteins (randomly PEGylated lysozyme and mono-PEGylated bovine serum albumin) were investigated, based on our previously developed model Chem. Eng. Technol. 2005, 28, 1387-1393. PEGylation of each protein resulted in a shift to a smaller elution volume compared to the unmodified molecule, but did not affect the number of binding sites appreciably. The shift of the retention volume of PEGylated proteins correlated with the calculated thickness of PEG layer around the protein molecule. Random PEGylation was carried out on a column (solid-phase PEGylation) and the PEGylated proteins were separated on the same column. Solid-phase PEGylation inhibited the production of multi-PEGylated forms and resulted in a relatively low yield of selective mono-PEGylated form. Pore diffusion may play an important role in solid-phase PEGylation. These results suggest the possibility of a reaction and purification process development based on the mechanistic model for PEGylated proteins on ion exchange chromatography.

摘要

蛋白质聚乙二醇化的机制很复杂,取决于蛋白质反应物的结构。因此,很难设计出一种能够以高产率产生所需聚乙二醇化形式的反应过程。同样,必须针对每种产品专门构建蛋白质聚乙二醇化后的有效纯化工艺。基于我们之前开发的模型 Chem. Eng. Technol. 2005, 28, 1387-1393,研究了驱动基于静电相互作用的色谱(离子交换色谱)的聚乙二醇化蛋白质(随机聚乙二醇化溶菌酶和单聚乙二醇化牛血清白蛋白)的保留和结合机制。与未修饰的分子相比,每种蛋白质的聚乙二醇化都会导致洗脱体积向较小的方向移动,但不会显著影响结合位点的数量。聚乙二醇化蛋白质保留体积的移动与计算得到的蛋白质分子周围聚乙二醇层的厚度相关。在柱上进行随机聚乙二醇化(固相聚乙二醇化),并在同一柱上分离聚乙二醇化蛋白质。固相聚乙二醇化抑制了多聚乙二醇化形式的产生,导致选择性单聚乙二醇化形式的产率相对较低。孔扩散可能在固相聚乙二醇化中起重要作用。这些结果表明,基于蛋白质在离子交换色谱上的聚乙二醇化的机制模型,可以开发反应和纯化工艺。

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PEG chain length impacts yield of solid-phase protein PEGylation and efficiency of PEGylated protein separation by ion-exchange chromatography: insights of mechanistic models.聚乙二醇(PEG)链长影响固相蛋白 PEG 化的产率和离子交换色谱法分离 PEG 化蛋白的效率:机制模型的见解。
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