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首页> 外文期刊>Bulletin of the Korean Chemical Society >High-Level Expression and Purification of Tag-free Peptides Containing Multiple Disulfide Bond in Pichia pastoris
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High-Level Expression and Purification of Tag-free Peptides Containing Multiple Disulfide Bond in Pichia pastoris

机译:含有多种二硫键在Pichia Pastoris中的无标签肽的高水平表达和纯化

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Eukaryotic expression systems are used widely and have the advantages of protein processing, proteolytic cleavage, disulfide bond formation, and posttranslational modification in contrast to the prokaryotic expression system. In the present study, peptide gene (olive flounder beta-defensin or hepcidin) was inserted into the vector of pPIC9K, which involved the secretion signal and promoter AOX1. The colonies with high copy numbers of the target gene for high-level expression were selected by G418. Approximately 30 mg/L for beta-defensin and 25 mg/L for hepcidin was obtained from the culture medium supernatant. An ammonium sulfate salting-out method was used for purification; this one-step purification simplified the procedures, and the purification effect was good in terms of the purity and yield. The proteins from yeast itself could be isolated easily using the ammonium sulfate salting-out method.
机译:与原核表达系统相比,真核表达系统被广泛使用并且具有蛋白质加工,蛋白水解裂解,二硫键形成和后期改性的优点。 在本研究中,将肽基因(橄榄树博β-防御素或肝素)插入PPIC9K的载体中,涉及分泌信号和启动子AX1。 通过G418选择具有高级别表达的靶基因的高拷贝数的菌落。 从培养基上清液中获得约30mg / L对于肝蛋白的β-defensin和25mg / L. 硫酸铵盐酸铵法用于纯化; 这种一步纯化简化了该程序,并且在纯度和产率方面纯化效果良好。 酵母本身的蛋白质可以使用硫酸铵盐析方法容易地分离。

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