Disruption of SMC-related genes promotes recombinant cholesterol esterase production in Burkholderia stabilis

Kenji Konishi; Yoshiaki Yasutake; Shuji Muramatsu; Satomi Murata; Keitaro Yoshida; Koji Ishiya; Sachiyo Aburatani; Shin-Ichi Sakasegawa; Tomohiro Tamura

doi:10.1007/s00253-022-12277-3

Disruption of SMC-related genes promotes recombinant cholesterol esterase production in Burkholderia stabilis

Appl Microbiol Biotechnol. 2022 Dec;106(24):8093-8110. doi: 10.1007/s00253-022-12277-3. Epub 2022 Nov 18.

Authors

Kenji Konishi^{1

2}, Yoshiaki Yasutake^{3

4}, Shuji Muramatsu¹, Satomi Murata¹, Keitaro Yoshida³, Koji Ishiya³, Sachiyo Aburatani³, Shin-Ichi Sakasegawa¹, Tomohiro Tamura^{5

6}

Affiliations

¹ Asahi Kasei Pharma Corporation, Shizuoka, 410-2321, Japan.
² Laboratory of Molecular Environmental Microbiology, Graduate School of Agriculture, Hokkaido University, Sapporo, 060-8589, Japan.
³ Bioproduction Research Institute, National Institute of Advanced Industrial Science and Technology (AIST), Sapporo, 062-8517, Japan.
⁴ Computational Bio Big-Data Open Innovation Laboratory (CBBD-OIL), AIST, Tokyo, 169-8555, Japan.
⁵ Laboratory of Molecular Environmental Microbiology, Graduate School of Agriculture, Hokkaido University, Sapporo, 060-8589, Japan. t-tamura@aist.go.jp.
⁶ Bioproduction Research Institute, National Institute of Advanced Industrial Science and Technology (AIST), Sapporo, 062-8517, Japan. t-tamura@aist.go.jp.

PMID: 36399168
DOI: 10.1007/s00253-022-12277-3

Abstract

Burkholderia stabilis strain FERMP-21014 secretes cholesterol esterase (BsChe), which is used in clinical settings to determine serum cholesterol levels. Previously, we constructed an expression plasmid with an endogenous constitutive promoter to enable the production of recombinant BsChe. In this study, we obtained one mutant strain with 13.1-fold higher BsChe activity than the wild type, using N-methyl-N'-nitro-N-nitrosoguanidine as a mutagen. DNA-sequencing analysis revealed that the strain had lost chromosome 3 (∆Chr3), suggesting that the genes hindering BsChe production may be encoded on Chr3. We also identified common mutations in the functionally unknown BSFP_068720/30 genes in the top 10 active strains generated during transposon mutagenesis. As BSFP_068720/30/40 comprised an operon on Chr3, we created the BSFP_068720/30/40 disruption mutant and confirmed that each disruption mutant containing the expression plasmid exhibited ~ 16.1-fold higher BsChe activity than the wild type. Quantitative PCR showed that each disruption mutant and ΔChr3 had a ~ 9.4-fold higher plasmid copy number than the wild type. Structural prediction models indicate that BSFP_068730/40 is structurally homologous to the structural maintenance of chromosomes (SMC) protein MukBE, which is responsible for chromosome segregation during cell division. Conversely, BSFP_068720/30/40 disruption did not lead to a Chr3 drop-out. These results imply that BSFP_068720/30/40 is not a SMC protein but is involved in destabilizing foreign plasmids to prevent the influx of genetic information from the environment. In conclusion, the disruption of BSFP_068720/30/40 improved plasmid stability and copy number, resulting in exceptionally high BsChe production. KEY POINTS: • Disruption of BSFP_068720/30/40 enabled mass production of Burkholderia Che/Lip. • BSFP_068730/40 is an SMC protein homolog not involved in chromosome retention. • BSFP_068720/30/40 is likely responsible for the exclusion of exogenous plasmids.

Keywords: Burkholderia; Cholesterol esterase; Condensin; Lipase; Plasmid stability; Structural maintenance of chromosomes (SMC).

MeSH terms

Chromosomes
Internationality*
Sterol Esterase*

Substances

Sterol Esterase

Supplementary concepts

Burkholderia stabilis