Construction of intein-mediated hGMCSF expression vector and its purification in Pichia pastoris

英特因 毕赤酵母 重组DNA 串联亲和纯化 蛋白质纯化 标志标签 融合基因 分子生物学 表达式向量 生物化学 化学 亲和层析 生物 融合蛋白 蛋白质剪接 基因 毕赤酵母 质粒 蛋白质工程 酵母 靶蛋白 大肠杆菌 蛋白质标签 核糖核酸 RNA剪接
作者
K. Sudhakar Babu,Aju Antony,T. Muthukumaran,S. Meenakshisundaram
出处
期刊:Protein Expression and Purification [Elsevier BV]
卷期号:57 (2): 201-205 被引量:20
标识
DOI:10.1016/j.pep.2007.10.004
摘要

As a novel attempt for the intracellular recombinant protein over expression and easy purification from Pichia pastoris, the therapeutic cytokine human granulocyte macrophage colony stimulating factor (hGMCSF) gene was fused to an intein-chitin-binding domain (gene from pTYB11 vector) fusion tag by overlap extension PCR and inserted into pPICZB vector, allowing for the purification of a native recombinant protein without the need for enzymatic cleavage. The fusion protein under the AOX1 promoter was integrated into the P. pastoris genome (SMD 1168) and the recombinant Pichia clones were screened for multicopy integrants. Expression of hGMCSF was done using glycerol and methanol based synthetic medium by three stage cultivation in a bioreactor. Purification of the expressed hGMCSF fusion protein was done after cell disruption and binding of the solubilized fusion protein to chitin affinity column, followed by DTT induced on column cleavage of hGMCSF from the intein tag. In this study, final biomass of 89 g dry cell weight/l and purified hGMCSF of 120 mg/l having a specific activity of 0.657 x 10(7) IU/mg was obtained. This strategy has an edge over the other--His or--GST based fusion protein purification where non-specific protein binding, expensive enzymatic cleavage and further purification of the enzyme is required. It distinguishes itself from all other purification systems by its ability to purify, in a single chromatographic step.

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