N-terminal domain truncation yielded a unique dimer of polysaccharide hydrolase with enhanced enzymatic activity, stability and calcium ion independence

La Xiang; Xinlin Hu; Chao Du; Lian Wu; Zhenghui Lu; Jiahai Zhou; Guimin Zhang

doi:10.1016/j.ijbiomac.2024.131352

N-terminal domain truncation yielded a unique dimer of polysaccharide hydrolase with enhanced enzymatic activity, stability and calcium ion independence

Int J Biol Macromol. 2024 May;266(Pt 2):131352. doi: 10.1016/j.ijbiomac.2024.131352. Epub 2024 Apr 2.

Authors

La Xiang¹, Xinlin Hu², Chao Du¹, Lian Wu³, Zhenghui Lu², Jiahai Zhou⁴, Guimin Zhang⁵

Affiliations

¹ College of Life Science and Technology, Beijing University of Chemical Technology, Beijing, People's Republic of China; State Key Laboratory of Biocatalysis and Enzyme Engineering, School of Life Sciences, Hubei University, Hubei, People's Republic of China.
² State Key Laboratory of Biocatalysis and Enzyme Engineering, School of Life Sciences, Hubei University, Hubei, People's Republic of China.
³ State Key Laboratory of Bio-organic and Natural Products Chemistry, Shanghai Institute of Organic Chemistry, Shanghai, People's Republic of China.
⁴ CAS Key Laboratory of Quantitative Engineering Biology, Shenzhen Institute of Synthetic Biology, Shenzhen Institutes of Advanced Technology, Chinese Academy of Sciences, Shenzhen, People's Republic of China. Electronic address: jiahai@siat.ac.cn.
⁵ College of Life Science and Technology, Beijing University of Chemical Technology, Beijing, People's Republic of China; State Key Laboratory of Biocatalysis and Enzyme Engineering, School of Life Sciences, Hubei University, Hubei, People's Republic of China. Electronic address: zhangguimin@mail.buct.edu.cn.

PMID: 38574926
DOI: 10.1016/j.ijbiomac.2024.131352

Abstract

Domain engineering, including domain truncation, fusion, or swapping, has become a common strategy to improve properties of enzymes, especially glycosyl hydrolases. However, there are few reports explaining the mechanism of increased activity from a protein structure perspective. Amy703 is an alkaline amylase with a unique N-terminal domain. Prior studies have shown that N-Amy, a mutant without an N-terminal domain, exhibits improved activity, stability, and calcium ion independence. In this study, we have used X-ray crystallography to determine the crystal structure of N-Amy and used AlphaFold2 to model the Amy703 structure, respectively. We further used size exclusion chromatography to show that Amy703 existed as a monomer, whereas N-Amy formed a unique dimer. It was found that the N-terminus of one monomer of N-Amy was inserted into the catalytic domain of its symmetrical subunit, resulting in the expansion of the catalytic pocket. This also significantly increased the pK_a of the hydrogen donor Glu350, thereby enhancing substrate binding affinity and contributing to increased N-Amy activity. Meanwhile, two calcium ions were found to bind to N-Amy at different binding sites, which also contributed to the stability of protein. Therefore, this study provided new structural insights into the mechanisms of various glycosyl hydrolases.

Keywords: Calcium-independent; Dimer; N-terminal domain.

MeSH terms

Calcium* / chemistry
Calcium* / metabolism
Catalytic Domain
Crystallography, X-Ray
Enzyme Stability*
Glycoside Hydrolases / chemistry
Glycoside Hydrolases / genetics
Glycoside Hydrolases / metabolism
Models, Molecular
Protein Domains
Protein Multimerization*

Substances

Calcium
Glycoside Hydrolases