期刊论文详细信息
The Journal of General and Applied Microbiology
Isolation and characterization of a bacterial strain that degrades cis-dichloroethenein the absence of aromatic inducers
Kenta Yonezuka2  Daisuke Kasai2  Jun Shimodaira3  Akira Hosoyama3  Shoko Ohji3  Eiji Masai2  Nobuyuki Fujita3  Atsushi Yamazoe3  Takayuki Ezaki1  Masao Fukuda2  Naoto Araki2  Mitsuru Numata3 
[1] Department of Microbiology, Gifu University Graduate School of Medicine;Department of Bioengineering, Nagaoka University of Technology;Biological Resource Center, National Institute of Technology and Evaluation
关键词: cis-dichloroethene;    Pseudomonas;    toluene dioxygenase;    trichloroethene;   
DOI  :  10.2323/jgam.2015.12.002
学科分类:微生物学和免疫学
来源: Applied Microbiology, Molecular and Cellulrar Biosciences Research Foundation
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【 摘 要 】

Bacteria capable of degrading cis-dichloroethene (cDCE) were screened from cDCE-contaminated soil, and YKD221, a bacterial strain that exhibited a higher growth on minimal salt agar plates in the presence of cDCE than in the absence of cDCE, were isolated. Phylogenetic studies of the 16S rRNA as well as gyrB, rpoD, and recA in YKD221 indicated that this strain is closely related to the type strains of Pseudomonas plecoglossicida, monteilii, and putida. An average nucleotide identity analysis indicated that YKD221 is most closely related to P. putida strains, including the type strain, which suggests that YKD221 belongs to P. putida. Although the genome of YKD221 was very similar to that of P. putida F1, a toluene-degrading strain, the YKD221 genome has 15 single-nucleotide polymorphisms and 4 insertions compared with the F1 genome. YKD221 caused the release of sufficient chloride ions from cDCE to suggest that the strain is able to completely dechlorinate and degrade cDCE. YKD221 also degraded trichloroethene but was unable to degrade trans-dichloroethene and tetrachloroethene. The degradation activity of YKD221 was elevated after growth on toluene. Inactivation of todC1, which encodes for a large subunit of the catalytic terminal component in toluene dioxygenase, resulted in a complete loss of growth on toluene and cDCE degradation activity. This is the first evidence of the involvement of todC1C2BA-coded toluene dioxygenase in cDCE degradation. YKD221 did not appear to grow on cDCE in a minimal salt liquid medium. However, YKD221 did exhibit an enhanced increase in cell concentration and volume of cells during growth on minimal salt agar plates with cDCE when first grown in LB medium. This behavior appears to have led us to misinterpret our initial results on YKD221 as an indication of improved growth in the presence of cDCE.

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