Application of Dynamic Regulation to Increase L-Phenylalanine Production in Escherichia coli
Author(s) -
Jie Wu,
Yongfei Liu,
Sheng Zhao,
Jibin Sun,
Zhaoxia Jin,
Dawei Zhang
Publication year - 2019
Publication title -
journal of microbiology and biotechnology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.601
H-Index - 64
eISSN - 1738-8872
pISSN - 1017-7825
DOI - 10.4014/jmb.1901.01058
Subject(s) - escherichia coli , fermentation , phenylalanine , enzyme , strain (injury) , biochemistry , metabolic engineering , titer , yield (engineering) , chemistry , biology , amino acid , gene , genetics , materials science , antibody , metallurgy , anatomy
Current strategies of strain improvement processes are mainly focused on enhancing the synthetic pathways of the products. However, excessive metabolic flux often creates metabolic imbalances, which lead to growth retardation and ultimately limit the yield of the product. To solve this problem, we applied a dynamic regulation strategy to produce L-phenylalanine (LPhe) in Escherichia coli . First, we constructed a series of Phe-induced promoters that exhibited different strengths through modification of the promoter region of yrP . Then, two engineered promoters were separately introduced into a Phe-producing strain xllp1 to dynamically control the expression level of one pathway enzyme AroK. Batch fermentation results of the strain xllp3 showed that the titer of Phe reached 61.3 g/l at 48 h, representing a titer of 1.36- fold of the strain xllp1 (45.0 g/l). Moreover, the L-Phe yields on glucose of xllp3 (0.22 g/g) were also greatly improved, with an increase of 1.22-fold in comparison with the xllp1 (0.18 g/ g). In summary, we successfully improved the titer of Phe by using dynamic regulation of one key enzyme and this strategy can be applied for improving the performance of strains producing other aromatic amino acids and derived compounds.
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