Affiliation:
1. 0000 0004 1760 4804 grid.411389.6 School of Life Sciences Anhui Agricultural University 230036 Hefei China
2. 0000 0001 0085 4987 grid.252245.6 Institute of Physical Science and Information Technology, School of Life Sciences Anhui University 230601 Hefei China
3. 0000 0001 2163 4895 grid.28056.39 State Key Laboratory of Bioreactor Engineering East China University of Science and Technology 200237 Shanghai China
Abstract
Abstract
In this work, we found that the Lrp/AsnC family protein SACE_5717 negatively regulated erythromycin biosynthesis in S. erythraea. Disruption of SACE_5717 led to a 27% improvement in the yield of erythromycin in S. erythraea A226. SACE_5717 directly repressed its own gene expression, as well as that of the adjacent gene SACE_5716 by binding to the target sequence 5′-GAACGTTCGCCGTCACGCC-3′. The predicted LysE superfamily protein SACE_5716 directly influenced the export of lysine, histidine, threonine and glycine in S. erythraea. Arginine, tyrosine and tryptophan were characterized as the effectors of SACE_5717 by weakening the binding affinity of SACE_5717. In the industrial S. erythraea WB strain, deletion of SACE_5717 (WBΔSACE_5717) increased erythromycin yield by 20%, and by 36% when SACE_5716 was overexpressed in WBΔSACE_5717 (WBΔSACE_5717/5716). In large-scale 5-L fermentation experiment, erythromycin yield in the engineered strain WBΔSACE_5717/5716 reached 4686 mg/L, a 41% enhancement over 3323 mg/L of the parent WB strain.
Funder
National Natural Science Foundation of China
National Program on Key Basic Research Project
Initial Foundation of Scientific Research in Anhui Agricultural University
Publisher
Oxford University Press (OUP)
Subject
Applied Microbiology and Biotechnology,Biotechnology,Bioengineering
Cited by
14 articles.
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