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A simple novel method for the preparation of noncovalent homodimeric, biologically active human interleukin 10 in Escherichia coli-Enhancing protein expression by degenerate PCR of 5 ' DNA in the open reading frame

机译:一种简单的新颖方法,通过在开放阅读框中通过简并PCR 5'DNA的方法在大肠杆菌中制备非共价同源二聚体,具有生物活性的人白介素10-增强蛋白质表达

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摘要

DNA inserts encoding human interleukin 10 (hIL-10), optimized for codon usage and secondary RNA structure, were purchased from several commercial sources and subcloned into a pMon vector. Despite the optimization, protein expression was nil. We therefore subjected the 5' segment of the cDNA encoding N-terminal amino acids 2-11 to degenerate PCR in order to create a small library of 130K theoretical cDNA combinations that would not change the respective amino acid sequence and tested their expression. After screening over 320 colonies 10 hIL-10 clones encoding the original amino acid sequence were identified. Three nucleotide substitutions were sufficient to ensure reasonable protein expression. Subsequently, hIL-10 was expressed in Escherichia coli, refolded and purified to homogeneity, yielding over 95% electrophoretically pure noncovalent homodimeric protein, which was biologically active in MC/9 cells. The yield of recombinant hIL-10 from 10 L of fermentation culture was 60 mg and a protocol for its long-term storage as a carrier-free lyophilized powder at -20 degrees was developed. (c) 2008 Published by Elsevier Inc.
机译:从多个商业渠道购买了针对密码子使用和二级RNA结构优化的编码人白介素10(hIL-10)的DNA插入片段,并将其亚克隆到pMon载体中。尽管进行了优化,蛋白质表达还是为零。因此,我们对编码N末端氨基酸2-11的cDNA的5'片段进行简并PCR,以创建一个130K理论cDNA组合的小文库,该组合不会改变相应的氨基酸序列,并测试了它们的表达。在筛选超过320个菌落之后,鉴定出编码原始氨基酸序列的10个hIL-10克隆。三个核苷酸取代足以确保合理的蛋白质表达。随后,hIL-10在大肠杆菌中表达,重折叠并纯化至均一,产生超过95%的电泳纯非共价同二聚体蛋白,该蛋白在MC / 9细胞中具有生物活性。来自10 L发酵培养物的重组hIL-10的产量为60 mg,并制定了将其作为无载体的冻干粉末于-20度长期保存的方案。 (c)2008年由Elsevier Inc.发布。

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