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[通过囊泡吸附剂上的色谱法分离重组蛋白]

[Separation of recombinant proteins by chromatography on vesicular sorbents].

作者信息

Kliushnichenko V E, Vul'fson A N, Titel C, Ehwald R, Miroshnikov A I

机构信息

Humboldt-University, Department of Biology, Berlin.

出版信息

Bioorg Khim. 1994 Aug-Sep;20(8-9):894-8.

PMID:7826416
Abstract

Vesicle chromatography, a recently developed method for separation of biomolecules, uses the vesicular packing (VP) material (clusters of microcapsules derived from plant cells), which was tested with respect to its application for the recombinant protein separation. Since VP has a well-defined separation limit, biomolecules are distributed in two separate peaks: large molecules are excluded and small molecules permeate through cell walls into the empty cell lumen. Recombinant proteins frequently form oligomers, which differ from monomers not only in size but also chemically and biologically. In the present study, separations of the recombinant proinsulin fusion protein oligomer and monomer, the recombinant human gamma-interferon monomer and dimer and recombinant tumour necrosis factor-alpha were investigated. For peak identification, the fractions and starting samples of the recombinant proteins were analysed by HPLC. The separations occurred without any sorption effects and with high efficiency and resolution of the protein peaks at a short column (10 cm). The VP is characterised by a high load ability, which favours the scale-up purification of the recombinant proteins. The combination of VP and HPLC is a considerable advance in biotechnology separation.

摘要

囊泡色谱法是一种最近开发的生物分子分离方法,它使用囊泡填充(VP)材料(源自植物细胞的微胶囊簇),并对其在重组蛋白分离中的应用进行了测试。由于VP具有明确的分离极限,生物分子分布在两个单独的峰中:大分子被排除在外,小分子透过细胞壁进入空的细胞腔。重组蛋白经常形成寡聚体,其与单体不仅在大小上不同,而且在化学和生物学上也不同。在本研究中,对重组胰岛素原融合蛋白寡聚体和单体、重组人γ干扰素单体和二聚体以及重组肿瘤坏死因子-α的分离进行了研究。为了进行峰鉴定,通过HPLC分析重组蛋白的馏分和起始样品。分离过程中没有任何吸附作用,并且在短柱(10 cm)上蛋白质峰具有高效率和分辨率。VP的特点是负载能力高,这有利于重组蛋白的放大纯化。VP和HPLC的结合是生物技术分离方面的一项重大进展。

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