Bioengineering (Aug 2023)

Trehalose Production Using Three Extracellular Enzymes Produced via One-Step Fermentation of an Engineered <i>Bacillus subtilis</i> Strain

  • Xi Sun,
  • Jun Yang,
  • Xiaoping Fu,
  • Xingya Zhao,
  • Jie Zhen,
  • Hui Song,
  • Jianyong Xu,
  • Hongchen Zheng,
  • Wenqin Bai

DOI
https://doi.org/10.3390/bioengineering10080977
Journal volume & issue
Vol. 10, no. 8
p. 977

Abstract

Read online

At present, the double-enzyme catalyzed method using maltooligosyltrehalose synthase (MTSase) and maltooligosyltrehalose trehalohydrolase (MTHase) is the mainstream technology for industrial trehalose production. However, MTSase and MTHase are prepared mainly using the heterologous expression in the engineered Escherichia coli strains so far. In this study, we first proved that the addition of 3 U/g neutral pullulanase PulA could enhance the trehalose conversion rate by 2.46 times in the double-enzyme catalyzed system. Then, a CBM68 domain was used to successfully assist the secretory expression of MTSase and MTHase from Arthrobacter ramosus S34 in Bacillus subtilis SCK6. At the basis, an engineered strain B. subtilis PSH02 (amyE::pulA/pHT43-C68-ARS/pMC68-ARH), which co-expressed MTSase, MTHase, and PulA, was constructed. After the 24 h fermentation of B. subtilis PSH02, the optimum ratio of the extracellular multi-enzymes was obtained to make the highest trehalose conversion rate of 80% from 100 g/L maltodextrin. The high passage stability and multi-enzyme preservation stability made B. subtilis PSH02 an excellent industrial production strain. Moreover, trehalose production using these extracellular enzymes produced via the one-step fermentation of B. subtilis PSH02 would greatly simplify the procedure for multi-enzyme preparation and be expected to reduce production costs.

Keywords