Genome-wide study of Cerrena unicolor 87613 laccase gene family and their mode prediction in association with substrate oxidation

Long-Bin Zhang; Wu-Wei-Jie Yang; Ting-Ting Qiu

doi:10.1186/s12864-023-09606-9

Genome-wide study of Cerrena unicolor 87613 laccase gene family and their mode prediction in association with substrate oxidation

BMC Genomics. 2023 Aug 30;24(1):504. doi: 10.1186/s12864-023-09606-9.

Authors

Long-Bin Zhang^{1

2}, Wu-Wei-Jie Yang^{3

4}, Ting-Ting Qiu^{3

4}

Affiliations

¹ Fujian Key Laboratory of Marine Enzyme Engineering, Fuzhou University, Fuzhou, 350116, Fujian, China. longbinzhang@fzu.edu.cn.
² College of Biological Science and Engineering, Fuzhou University, Fuzhou, 350116, Fujian, China. longbinzhang@fzu.edu.cn.
³ Fujian Key Laboratory of Marine Enzyme Engineering, Fuzhou University, Fuzhou, 350116, Fujian, China.
⁴ College of Biological Science and Engineering, Fuzhou University, Fuzhou, 350116, Fujian, China.

Abstract

Background: Laccases are green biocatalysts with wide industrial applications. The study of efficient and specific laccase producers remains a priority. Cerrena species have been shown to be promising basidiomycete candidates for laccase production. Although two sets of Cerrena genome data have been publicly published, no comprehensive bioinformatics study of laccase gene family in C. unicolor has been reported, particularly concerning the analysis of their three-dimensional (3D) structures and molecular docking to substrates, like ABTS and aflatoxin B₁ (AFB₁).

Results: In this study, we conducted a comprehensive genome-wide analysis of laccase gene family in C. unicolor 87613. We identified eighteen laccase genes (CuLacs) and classified them into three clades using phylogenetic analysis. We characterized these laccases, including their location in contig 5,6,9,12,15,19,26,27, gene structures of different exon-intron arrangements, molecular weight ranging from 47.89 to 141.41 kDa, acidic pI value, 5-15 conserved protein motifs, signaling peptide of extracellular secretion (harbored by 13 CuLacs) and others. In addition, the analysis of cis-acting element in laccase promoters indicated that the transcription response of CuLac gene family was regulatable and complex under different environmental cues. Furthermore, analysis of transcription pattern revealed that CuLac8, 12 and CuLac2, 13 were the predominant laccases in response to copper ions or oxidative stress, respectively. Finally, we focused on the 3D structure analysis of CuLac proteins. Seven laccases with extra transmembrane domains or special sequences were particularly interesting. Predicted structures of each CuLac protein with or without these extra sequences showed altered interacting amino acid residues and binding sites, leading to varied affinities to both ABTS and AFB₁. As far as we know, it is the first time to discuss the influence of the extra sequence on laccase's affinity to substrates.

Conclusions: Our findings provide robust genetic data for a better understanding of the laccase gene family in C. unicolor 87613, and create a foundation for the molecular redesign of CuLac proteins to enhance their industrial applications.

Keywords: 3D structure; Cerrena unicolor; Gene family; Genome; Laccase; Molecular docking; Transcriptional response.

MeSH terms

Genome-Wide Association Study*
Laccase* / genetics
Molecular Docking Simulation
Phylogeny

Substances

Laccase
2,2'-azino-di-(3-ethylbenzothiazoline)-6-sulfonic acid

Supplementary concepts

Cerrena unicolor
Cebus unicolor

Abstract

MeSH terms

Substances

Supplementary concepts

Grants and funding