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Expression and purification of antimicrobial peptide CM4 by N~(pro) fusion technology in E. coli

机译:N〜(pro)融合技术在大肠杆菌中表达和纯化抗菌肽CM4

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Antimicrobial peptide CM4 is a small cationic peptide with broad-spectrum activities against bacteria, fungi, and tumor cells. Different strategies have been developed to produce small antibacterial peptides using recombinant techniques. To date, no efforts to obtain large quantities of active recombinant CM4 have been reported. In order to establish a bacterium-based CM4 production system, CM4 was cloned into pET28a and expressed with N~(pro) mutant (EDDIE) fusion. CM4 expressed as EDDIE are deposited as inclusion bodies. On in vitro refolding by switching from chemotropic to kosmotropic conditions, the fusion partner is released from the C-terminal end of the autoprotease by self-cleavage, leaving CM4 protein with an authentic N terminus. Purified CM4 was separated on Ni~(2+)-chelating chromatography column and cation-exchange chromatography column. Mass spectroscopic analysis indicated the protein to be 4132.56 Dalton, which equalled the theoretically expected mass. N-terminal sequencing of CM4 showed the sequence corresponded to the native protein. The recombinant CM4 exhibited the same antimicrobial and anti-tumor activity as reported previously. The expression strategy presented in this study allows convenient high yield and easy purification of recombinant CM4 with native sequences.
机译:抗菌肽CM4是一种小的阳离子肽,对细菌,真菌和肿瘤细胞具有广谱活性。已经开发出使用重组技术生产小的抗菌肽的不同策略。迄今为止,尚未报道获得大量活性重组CM4的努力。为了建立基于细菌的CM4生产系统,将CM4克隆到pET28a中并与N〜(pro)突变体(EDDIE)融合表达。表示为EDDIE的CM4作为包涵体保存。在从趋化条件切换到趋同条件的体外重折叠中,融合伴侣通过自身裂解作用从自体蛋白酶的C末端释放,从而使CM4蛋白具有真实的N末端。在Ni〜(2+)螯合色谱柱和阳离子交换色谱柱上分离纯化的CM4。质谱分析表明该蛋白质为4132.56道尔顿,等于理论上的预期质量。 CM4的N端测序表明该序列与天然蛋白相对应。重组CM4表现出与先前报道的相同的抗微生物和抗肿瘤活性。在这项研究中提出的表达策略允许方便的高产量和容易纯化具有天然序列的重组CM4。

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