High-level production of chitinase by multi-strategy combination optimization in Bacillus licheniformis

Zhimin Qi; Bo Lei; Min Xiong; Weijia Li; Yongqing Liao; Dongbo Cai; Xin Ma; Ruibin Zhang; Shouwen Chen

doi:10.1007/s11274-024-03995-z

High-level production of chitinase by multi-strategy combination optimization in Bacillus licheniformis

World J Microbiol Biotechnol. 2024 Apr 26;40(6):181. doi: 10.1007/s11274-024-03995-z.

Authors

Zhimin Qi¹, Bo Lei¹, Min Xiong¹, Weijia Li¹, Yongqing Liao¹, Dongbo Cai¹, Xin Ma¹, Ruibin Zhang², Shouwen Chen³

Affiliations

¹ State Key Laboratory of Biocatalysis and Enzyme Engineering, Environmental Microbial Technology Center of Hubei Province, College of Life Sciences, Hubei University, 368 Youyi Avenue, Wuhan, Hubei, 430062, PR China.
² State Key Laboratory of Biocatalysis and Enzyme Engineering, Environmental Microbial Technology Center of Hubei Province, College of Life Sciences, Hubei University, 368 Youyi Avenue, Wuhan, Hubei, 430062, PR China. zhangruibin1990@126.com.
³ State Key Laboratory of Biocatalysis and Enzyme Engineering, Environmental Microbial Technology Center of Hubei Province, College of Life Sciences, Hubei University, 368 Youyi Avenue, Wuhan, Hubei, 430062, PR China. mel212@126.com.

PMID: 38668833
DOI: 10.1007/s11274-024-03995-z

Abstract

In view of the extensive potential applications of chitinase (ChiA) in various fields such as agriculture, environmental protection, medicine, and biotechnology, the development of a high-yielding strain capable of producing chitinase with enhanced activity holds significant importance. The objective of this study was to utilize the extracellular chitinase from Bacillus thuringiensis as the target, and Bacillus licheniformis as the expression host to achieve heterologous expression of ChiA with enhanced activity. Initially, through structural analysis and molecular dynamics simulation, we identified key amino acids to improve the enzymatic performance of chitinase, and the specific activity of chitinase mutant D116N/E118N was 48% higher than that of the natural enzyme, with concomitant enhancements in thermostability and pH stability. Subsequently, the expression elements of ChiA(D116N/E118N) were screened and modified in Bacillus licheniformis, resulting in extracellular ChiA activity reached 89.31 U/mL. Further efforts involved the successful knockout of extracellular protease genes aprE, bprA and epr, along with the gene clusters involved in the synthesis of by-products such as bacitracin and lichenin from Bacillus licheniformis. This led to the development of a recombinant strain, DW2△abelA, which exhibited a remarkable improvement in chitinase activity, reaching 145.56 U/mL. To further improve chitinase activity, a chitinase expression frame was integrated into the genome of DW2△abelA, resulting in a significant increas to 180.26 U/mL. Optimization of fermentation conditions and medium components further boosted shake flask enzyme activity shake flask enzyme activity, achieving 200.28 U/mL, while scale-up fermentation experiments yielded an impressive enzyme activity of 338.79 U/mL. Through host genetic modification, expression optimization and fermentation optimization, a high-yielding ChiA strain was successfully constructed, which will provide a solid foundation for the extracellular production of ChiA.

Keywords: Bacillus licheniformis; Chitinase; Fermentation optimization; Host modification; Protein engineering.

MeSH terms

Bacillus licheniformis* / enzymology
Bacillus licheniformis* / genetics
Bacillus thuringiensis / enzymology
Bacillus thuringiensis / genetics
Bacitracin
Bacterial Proteins* / genetics
Bacterial Proteins* / metabolism
Chitinases* / biosynthesis
Enzyme Stability
Hydrogen-Ion Concentration
Molecular Dynamics Simulation
Multigene Family
Recombinant Proteins / biosynthesis
Temperature

Substances

Bacitracin
Bacterial Proteins
Chitinases
Recombinant Proteins

Grants and funding

2021YFC2100200/National Key Research and Development Program of China