Manipulation Strategy to Increase Expression Level of Soluble Recombinant Protein Penicillin G Acylase (PGA) in Bacterial Host Escherichia coli: A Review Article

Achmad Makin Amin, Sismindari, Sunni Sofiah Aniqah, Lutfia Nadiatuz Zakiyah, Muthi’ah Rasyidah, Purwanto
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Abstract

The strategy of producing PGA on a massive scale with high levels of soluble protein can be through recombinant genetic techniques and expressed in a certain host. E. coli is still a popular bacterial host to produce a recombinant protein which has advantages such as fast growth, low production cost, and high expression rate. Apart from its advantages, E. coli as a production host also has disadvantages including the expression of recombinant proteins often failing to form the proper folding conformation which makes the protein biologically inactive. Many strategies can be developed to overcome these problems, such as the selection of the host strain (E. coli HB101 & JM109), fusion protein to enhance the recovery of soluble protein (MBP & NusA), optimization of fermentation (low-temperature incubation), and optimization of the protein isolation process for the recovery of active PGA (Freeze-thawing method).
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提高可溶性重组蛋白青霉素 G 乙酰化酶 (PGA) 在细菌宿主大肠杆菌中的表达水平的操作策略:综述文章
大规模生产高水平可溶性 PGA 蛋白的策略是通过基因重组技术,并在一定的宿主中进行表达。大肠杆菌仍然是生产重组蛋白的常用细菌宿主,它具有生长快、生产成本低、表达率高等优点。除了优点之外,大肠杆菌作为生产宿主也有缺点,包括表达的重组蛋白往往不能形成正确的折叠构象,从而使蛋白失去生物活性。为克服这些问题,可开发多种策略,如选择宿主菌株(大肠杆菌 HB101 和 JM109)、融合蛋白以提高可溶性蛋白的回收率(MBP 和 NusA)、优化发酵(低温培养)以及优化蛋白分离过程以回收活性 PGA(冻融法)。
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