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High-Yield Soluble Expression and Simple Purification of the Antimicrobial Peptide OG2 Using the Intein System in Escherichia coli

机译:使用Intein系统在大肠杆菌中高纯度可溶表达和抗菌肽OG2的简单纯化

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摘要

OG2 is a modified antimicrobial peptide, that is, derived from the frog peptide Palustrin-OG1. It has high antimicrobial activity and low cytotoxicity, and it is therefore promising as a therapeutic agent. Both prokaryotic (Escherichia coli) and eukaryotic (Pichia pastoris) production host systems were used to produce OG2 in our previous study; however, it was difficult to achieve high expression yields and efficient purification. In this study, we achieved high-yield OG2 expression using the intein fusion system. The optimized OG2 gene was cloned into the pTWIN1 vector to generate pTWIN-OG2-intein2 (C-terminal fusion vector) and pTWIN-intein1-OG2 (N-terminal fusion vector). Nearly 70% of the expressed OG2-intein2 was soluble after the IPTG concentration and induction temperature were decreased, whereas only 42% of the expressed of intein1-OG2 was soluble. Up to 75 mg of OG2-intein2 was obtained from a 1 l culture, and 85% of the protein was cleaved by 100 mM DTT. Intein1-OG2 was less amenable to cleavage due to the inhibition of cleavage by the N-terminal amino acid of OG2. The purified OG2 exhibited strong antimicrobial activity against E. coli K88. The intein system is the best currently available system for the cost-effective production of OG2.
机译:OG2是修饰的抗菌肽,即衍生自青蛙肽Palustrin-OG1。它具有高抗菌活性和低细胞毒性,因此有望用作治疗剂。在我们先前的研究中,原核(大肠杆菌)和真核(巴斯德毕赤酵母)生产宿主系统都用于生产OG2。然而,难以实现高表达产量和有效纯化。在这项研究中,我们使用了intein融合系统实现了高产量OG2表达。将优化的OG2基因克隆到pTWIN1载体中以产生pTWIN-OG2-intein2(C末端融合载体)和pTWIN-intein1-OG2(N末端融合载体)。在降低IPTG浓度和诱导温度后,将近70%的OG2-intein2表达可溶,而仅42%的intein1-OG2表达可溶。从1微升培养物中获得最多75微克的OG2-intein2,并且100微升MTT裂解了85%的蛋白质。由于OG2的N-末端氨基酸对切割的抑制,Intein1-OG2较不易于切割。纯化的OG2对大肠杆菌K88表现出强大的抗菌活性。内含肽系统是目前可用于生产具有成本效益的OG2的最佳系统。

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