A novel method for high level production of protein glutaminase by sfGFP tag in Bacillus subtilis

  • Zheng Zhang
  • , Yuxi Li
  • , Lihui Zheng
  • , Mingfei Jin
  • , Yelin Wu
  • , Rui Xu
  • , Yin Luo
  • , Jiajing Wu
  • , Wei Su
  • , Shijing Luo
  • , Yuchen Huang
  • , Cong Wang
  • , Zhongyi Chang
  • , Deming Jiang*
  • , Jing Huang
  • *Corresponding author for this work

Research output: Contribution to journalArticlepeer-review

13 Scopus citations

Abstract

Protein glutaminase (PG; EC 3.5.1.44) is a novel deamidase that helps to improve functional properties of food proteins. Currently, the highest activated PG enzyme activity was 26 U/mg when recombinantly expressed via the twin-arginine translocation (Tat) pathway in Corynebacterium glutamicum. In this study, superfolder green fluorescent protein (sfGFP) was used to replace traditional signal peptides to facilitate efficient heterologous expression and secretion of Propeptide-Protein glutaminase (PP) in Bacillus subtilis. The fusion protein, sfGFP-PP, was secreted from 12 h of fermentation and reached its highest extracellular expression at 28 h, with a secretion efficiency of about 93 %. Moreover, when fusing sfGFP with PP at the N-terminus, it significantly enhances PG expression up to 26 U/mL by approximately 2.2-fold compared to conventional signal-peptides- guided PP with 11.9 U/mL. Finally, the PG enzyme activity increased from 26 U/mL to 36.9 U/mL after promoter and RBS optimization. This strategy not only provides a new approach to increase PG production as well as extracellular secretion but also offers sfGFP as an effective N-terminal tag for increased secreted production of difficult-to-express proteins.

Original languageEnglish
Article number130092
JournalInternational Journal of Biological Macromolecules
Volume262
DOIs
StatePublished - Mar 2024

Keywords

  • Bacillus subtilis
  • Protein glutaminase
  • Secretion
  • Signal peptide
  • sfGFP

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