反义RNA抑制ackA、pta和poxB对大肠杆菌醋酸酯分泌和重组β干扰素表达的影响

Mohammad Hossein Morowvat
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摘要

大肠杆菌(E.coli)是生产重组蛋白最广泛使用的宿主之一。获得高产品产量和生产率的主要问题是醋酸(醋酸盐)作为一种有害的代谢副产物的积累。在本研究中,采用一种基于反义的代谢工程方法来抑制醋酸盐的排泄问题。材料与方法:设计了含有人重组干扰素β (rhINF-β)编码基因和3个针对醋酸激酶、磷酸转乙酰酶和丙酮酸氧化酶B的反义寡核苷酸的重组质粒。研究了重组质粒在大肠杆菌中对细胞生理、rhf -β产生和乙酸酯分泌的影响。结果:与对照细胞相比,反义调节细胞的靶酶mRNA水平降低。由于质粒的构建,培养基中乙酸酯的浓度降低。反义RNA的表达不影响细胞生长,呈负向。此外,与不含反义基因的对照质粒相比,反义调控菌株的rhf -β产量增加。结论:乙酸途径的反义策略在大肠杆菌代谢工程中的应用是成功的。反义技术对产率的提高表明,该策略可成功应用于大肠杆菌表达系统的高密度发酵中,以过表达其他重组蛋白。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Effects of ackA, pta and poxB inhibition by antisense RNA on acetate excretion and recombinant beta interferon expression in Escherichia coli
Introduction : Escherichia coli (E.coli) is one of the most widely used hosts for the production of recombinant proteins. The main problem in getting high product yields and productivity is the accumulation of acetic acid (acetate) as an unwanted metabolic by-product. In this study, an antisense-based strategy as a metabolic engineering approach was employed to hamper the acetate excretion problem. Materials and Methods : A recombinant plasmid containing the encoding genes for human recombinant interferon beta (rhINF-β) and three antisense oligonucleotides against acetate kinase, phosphotransacetylase and pyruvate oxidase B was designed. The effects of recombinant plasmid on the cell physiology, rhINF-β production and acetate excretion were studied in E. coli. Results: The mRNA levels of the targeted enzymes were lowered in antisense-regulated cells compared to the control cells. The concentration of acetate in culture media was decreased due to the constructed plasmid. The expression of antisense RNA did not affect the cell growth, negatively. Besides, the rhINF-β production was enhanced in antisense-regulated strain compared to the control plasmid without antisense genes. Conclusion: Application of an antisense strategy on the acetate pathway was successful in metabolically engineering E. coli. This enhancement of production yield by antisense technology suggests that this strategy may be successfully applied to high cell density fermentations of E. coli expression system to overexpress other recombinant proteins.
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