4.7 Article

High titer production of tetracenomycins by heterologous expression of the pathway in a Streptomyces cinnamonensis industrial monensin producer strain

期刊

METABOLIC ENGINEERING
卷 11, 期 6, 页码 319-327

出版社

ACADEMIC PRESS INC ELSEVIER SCIENCE
DOI: 10.1016/j.ymben.2009.06.004

关键词

Heterologous expression; Tetracenomycin; Precursor supply; Polyketide; Monensin; Crotonyl-CoA reductase; Streptomyces

资金

  1. National Institutes of Health [GM50542]
  2. Eli Lilly and Company

向作者/读者索取更多资源

Streptomyces cinnamonensis C730.1 and C730.7, are industrially mutagenized strains that produce moderate and high levels of the polyketide polyether antibiotic monensin A, respectively, in an oil-based fermentation medium. The possibility that these strains could be used for high titer production of a heterologous polyketide product was investigated by expression of the entire tetracenomycin (TCM) biosynthetic pathway using an integrative plasmid, pSET154. Expression in C730.1 led to stable production of similar to 0.44g/l TCM C (the final biosynthetic product) and similar to 2.69 g/l TCM A2 (the penultimate biosynthetic product), and resulted in a 40% decrease in monensin production. Expression in the C730.7 led to higher levels of TCMs, similar to 0.6 g/l TCM C and similar to 4.35 g/l TCM A2, without any detectable decrease in the higher titer monensin production. Abrogation of monensin production in this strain through deletion of the corresponding bio synthetic genes did not lead to higher levels of TCM products. In the case of the C730.7 host, 85% of the TCMC and virtually all of the TCMA2 were intracellular, suggesting feedback inhibition leads to the accumulation of the final pathway intermediate. These observations contrast those made for the native producer Streptomyces glaucescens where the predominant product is TCM C and TCM titers are significantly lower levels (similar to 0.3 g/l), and demonstrate the potential utility of S. cinnamonensis strains as heterologous hosts for high level expression of a variety of polyketide synthase derived products. (C) 2009 Elsevier Inc. All rights reserved.

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