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采用L-组氨酸和1-苄基-L-组氨酸亲和配体的色谱法纯化人乳头瘤病毒16型E6/E7质粒疫苗

Chromatographic HPV-16 E6/E7 plasmid vaccine purification employing L-histidine and 1-benzyl-L-histidine affinity ligands.

作者信息

Amorim Lúcia F A, Gaspar Rita, Pereira Patrícia, Černigoj Urh, Sousa Fani, Queiroz João António, Sousa Ângela

机构信息

CICS-UBI - Centro de Investigação em Ciências da Saúde, Universidade da Beira Interior, Covilhã, Portugal.

BIASeparationsd.o.o., Ajdovščina, Slovenia.

出版信息

Electrophoresis. 2017 Nov;38(22-23):2975-2980. doi: 10.1002/elps.201700147. Epub 2017 Aug 14.

DOI:10.1002/elps.201700147
PMID:28683160
Abstract

Affinity chromatography based on amino acids as interacting ligands was already indicated as an alternative compared to ion exchange or hydrophobic interaction for plasmid DNA purification. Understanding the recognition mechanisms occurring between histidine-based ligands and nucleic acids enables more efficient purification of a DNA vaccine, as the binding and elution conditions can be adjusted in order to enhance the purification performance. Decreasing pH to slightly acidic conditions increases the positive charge of histidine ligand, what influences the type of interaction between chromatographic support and analytes. This was proven in this work, where hydrophobic effects established in the presence of ammonium sulfate were affected at pH 5.0 in comparison to pH 8.0, while electrostatic and cation-π interactions were intensified. Histidine ligand at pH 5.0 interacts with phosphate groups or aromatic rings of plasmid DNA. Due to different responses of RNA and pDNA on mobile phase changes, the elution order between RNA and pDNA was changed with mobile phase pH decrease from 8.0 to 5.0. The phenomenon was more evident with L-histidine ligand due to more hydrophilic character, leading to an improved selectivity of L-histidine-modified chromatographic monolith, allowing the product recovery with 99% of purity (RNA removal). With the 1-benzyl- L-histidine ligand, stronger and less selective interactions with the nucleic acids were observed due to the additional hydrophobicity associated with the phenyl aromatic ring. Optimization of sample displacement chromatography parameters (especially (NH ) SO concentration) at slightly acidic pH enabled excellent isolation of pDNA, by the removal of RNA in a negative mode, with binding capacities above 1.5 mg pDNA per mL of chromatographic support.

摘要

与离子交换或疏水相互作用相比,基于氨基酸作为相互作用配体的亲和色谱已被指出是质粒DNA纯化的一种替代方法。了解基于组氨酸的配体与核酸之间发生的识别机制能够更有效地纯化DNA疫苗,因为可以调整结合和洗脱条件以提高纯化性能。将pH降低到略呈酸性的条件会增加组氨酸配体的正电荷,这会影响色谱支持物与分析物之间的相互作用类型。这项工作证明了这一点,与pH 8.0相比,在pH 5.0时硫酸铵存在下建立的疏水作用受到影响,而静电和阳离子-π相互作用增强。pH 5.0时的组氨酸配体与质粒DNA的磷酸基团或芳香环相互作用。由于RNA和质粒DNA对流动相变化的响应不同,随着流动相pH从8.0降至5.0,RNA和质粒DNA之间的洗脱顺序发生了变化。由于L-组氨酸配体具有更强的亲水性,这种现象更为明显,从而提高了L-组氨酸修饰的整体色谱柱的选择性,使得产品回收率达到99%的纯度(去除RNA)。对于1-苄基-L-组氨酸配体,由于与苯芳香环相关的额外疏水性,观察到与核酸的相互作用更强但选择性更低。在略呈酸性的pH下优化样品置换色谱参数(尤其是硫酸铵浓度)能够出色地分离质粒DNA,通过负模式去除RNA,每毫升色谱支持物的结合容量超过1.5毫克质粒DNA。

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