Frontiers in Microbiology (Aug 2022)

The characteristics of protein-glutaminase from an isolated Chryseobacterium cucumeris strain and its deamidation application

  • Ruidan Qu,
  • Ruidan Qu,
  • Tian Dai,
  • Jiajing Wu,
  • Aitian Tian,
  • Yanfang Zhang,
  • Li Kang,
  • Wei Ouyang,
  • Congli Jin,
  • Jinjin Niu,
  • Zhen Li,
  • Zhongyi Chang,
  • Deming Jiang,
  • Jing Huang,
  • Hongliang Gao

DOI
https://doi.org/10.3389/fmicb.2022.969445
Journal volume & issue
Vol. 13

Abstract

Read online

Protein-glutaminase (PG), a deamidation enzyme commercially derived from Chryseobacterium proteolyticum, is used to improve the solubility and other functional properties of food proteins. In this study, a new PG-producing strain, Chryseobacterium cucumeris ZYF120413-7, was isolated from soil, and it had a high PG yield and a short culture time. It gave the maximum PG activity with 0.557 U/ml on Cbz-Gln-Gly after 12 h of culture, indicating that it was more suitable for PG production. The enzyme activity recovery and purification fold were 32.95% and 161.95-fold, respectively, with a specific activity of 27.37 U/mg. The PG was a pre-pro-protein with a 16 amino acids putative signal peptide, a pro-PG of 118 amino acids, and a mature PG of 185 amino acids. The amino acid sequence identity of PG from strain ZYF120413-7 was 74 and 45%, respectively, to that of PG from C. proteolyticum 9670T and BH-PG. The optimum reaction pH and temperature of PG was 6 and 60°C, respectively. Enzyme activity was inhibited by Cu2+. The optimum PG substrate was Cbz-Gln-Gly, and the Km and Vmax values were 1.68 mM and 1.41 μM mg protein−1 min−1, respectively. Degree of deamidation (DD) of soy protein isolate (SPI) treated by purified PG was 40.75% within the first 2 h and 52.35% after 18 h. These results demonstrated that the PG from C. cucumeris ZYF120413-7 was a promising protein-deamidating enzyme for improving the functionality of food proteins.

Keywords