Identification of the di-n-butyl phthalate-biodegrading strains and the biodegradation pathway in strain LMB-1


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DNA isolated from a greenhouse soil (Nanjing, Jiangsu Province, China) was suitable for PCR amplification of gene segment coding for the 16S rRNA. Diverse PCR products were characterized by cloning and sequencing, and analysis of bacterial colonies showed the presence over 26 phyla. The most bacteria belonged to Proteobacteria, Actinobacteria, Gemmatimonadetes, Acidobacteria and Planctomycetes. Furthermore, after the enrichment procedure of DBP-degrading microorganisms, 4 strains were isolated from the soil sample with di-n-butyl phthalate (DBP) biodegradability, and they were identified to be Rhizobium sp., Streptomyces sp., Pseudomonas sp. and Acinetobacter sp. Analysis of the degradation products by LC-MS led to identification of metabolites of DBP in strain LMB-1 (identified as Rhizobium sp.) which suggests that DBP was degraded through β-oxidation, demethylation, de-esterification and cleavage of aromatic ring.

作者简介

Y. Fang

Laboratory of Biosystems and Microanalysis, State Key Laboratory of Bioreactor Engineering

Email: zhouying@ecust.edu.cn
中国, Meilong RD 130, Shanghai, 200237

L.-S. Zhang

Laboratory of Biosystems and Microanalysis, State Key Laboratory of Bioreactor Engineering

Email: zhouying@ecust.edu.cn
中国, Meilong RD 130, Shanghai, 200237

J. Wang

Laboratory of Biosystems and Microanalysis, State Key Laboratory of Bioreactor Engineering

Email: zhouying@ecust.edu.cn
中国, Meilong RD 130, Shanghai, 200237

Y. Zhou

Laboratory of Biosystems and Microanalysis, State Key Laboratory of Bioreactor Engineering

编辑信件的主要联系方式.
Email: zhouying@ecust.edu.cn
中国, Meilong RD 130, Shanghai, 200237

B.-C. Ye

Laboratory of Biosystems and Microanalysis, State Key Laboratory of Bioreactor Engineering; School of Chemistry and Chemical Engineering

Email: zhouying@ecust.edu.cn
中国, Meilong RD 130, Shanghai, 200237; Xinjiang, 832000

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