Heterologous expression of mtf and mtc genes of Pseudanabaena foetida var. intermedia is sufficient to produce 2-methylisoborneol in Escherichia coli

Author:

Dayarathne Kaushalya1ORCID,Ishikawa Toshiki1ORCID,Watanabe Satoru2ORCID,Ishikawa Yuuma3ORCID,Aikeranmu Kadeer1,Kitagawaa Hina1,Komatsubara Natsumi1,Yamaguchi Masatoshi1ORCID,Kawai-Yamada Maki1ORCID

Affiliation:

1. Graduate School of Science and Engineering, Saitama University, Shimo-Okubo, Sakura-ku, Saitama-city , Saitama, Japan

2. Department of Bioscience, Tokyo University of Agriculture, 1-chōme-1-1 Sakuragaoka, Setagaya-city , Tokyo, Japan

3. Institute for Molecular Physiology, Heinrich-Heine-Universität, Cluster of Excellence on Plant Sciences (CEPLAS) , Düsseldorf, Germany

Abstract

ABSTRACT Microbial volatile metabolite 2-methylisoborneol (2-MIB) causes odor and taste issues in drinking water, making it unappealing for human consumption. It has been suggested that 2-MIB biosynthesis consists of two main steps, namely, methylation of geranyl diphosphate into 2-methyl geranyl diphosphate by geranyl diphosphate methyl transferase (GPPMT) and subsequent cyclization into 2-MIB by 2-MIB synthase (MIBS). Pseudanabaena foetida var. intermedia is a 2-MIB-producing cyanobacterium whose GPPMT and MIBS enzymes are encoded by adjacent mtf and mtc genes . The present study identified a 2-MIB-related gene cluster composed of cnb A, mtf , mtc , and cnb B genes in P . foetida var. intermedia . The two homologous cyclic nucleotide-binding protein genes, cnb A and cnb B, were detected adjacent to the mtf and mtc genes, respectively. The nucleotide sequence of the cnb A- mtf-mtc-cnb B gene cluster showed 99.55% identity with 2-MIB synthesis-associated gene cluster of Pseudanabaena sp. dqh15. RT-PCR results revealed that mtf and mtc genes are co-expressed, while cnb A and cnb B genes are expressed independently in P . foetida var. intermedia . To investigate whether only mtf and mtc genes are sufficient for 2-MIB synthesis, the two-gene unit ( mtf-mtc ) was introduced into Escherichia coli strain JM109 via overexpression vector pYS1C. Gas chromatograph-mass spectrometry results showed that the E. coli strain transformed with mtf-mtc was able to produce 2-MIB. The intracellular 2-MIB level in P . foetida var. intermedia was higher than the extracellular 2-MIB level, while the transformed E. coli strain showed an opposite trend. Growth inhibition was observed in the 2-MIB-producing transformed E. coli strain. IMPORTANCE Contamination of drinking water with odiferous microbial metabolite 2-MIB is a worldwide concern. Removal of 2-MIB from drinking water burdens the water purification process. Therefore, it is important to search for alternative methods, such as suppressing the production of 2-MIB by aquatic microorganisms. For that, it is necessary to expand the current knowledge about the mechanism of 2-MIB synthesis at the genetic level. This study revealed that mtf and mtc genes of the 2-MIB-related gene cluster are transcribed as a single unit in P . foetida var. intermedia , and the expression of both mtf and mtc genes is essential and sufficient for 2-MIB synthesis in E. coli heterologous gene expression system.

Funder

MEXT | Japan Society for the Promotion of Science

Publisher

American Society for Microbiology

Subject

Infectious Diseases,Cell Biology,Microbiology (medical),Genetics,General Immunology and Microbiology,Ecology,Physiology

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