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Pseudomonas C12B, an SDS degrading strain, harbours a plasmid coding for degradation of medium chain length n-alkanes
Authors:Jan Kostal  Miloslav Suchanek  Hana Klierova  Katerina Demnerova  Blanka Kralova  Dani L McBeth
Institution:1Institute of Chemical Technology, Dept. of Biochemistry and Microbiology, Technicka 5, Praha, 6 16000, Czech Republic;2The City University of New York Medical School, Dept. of Microbiology and Immunology, 138th St. at Convent Ave., New York, NY 10031, USA
Abstract:Pseudomonas C12B is able to degrade alkyl sulfates, alkylbenzene sulfonates, and linear alkanes and alkenes. Mitomycin C curing experiments and conjugation experiments demonstrated that the ability to utilize n-alkanes (C9–C12) and n-alkenes (C10 and C12) of medium chain length was plasmid-encoded. The plasmid was designated pDEC. Its size was estimated at several hundreds kb according to mobility in agarose gels. The plasmid did not confer resistance to the antibiotics tested. Analysis of alkylsulfatases P1 and P2 in original and cured strains confirmed that both enzymes are encoded by the chromosome. The ability of Pseudomonas C12B to utilize alkylbenzene sulfonates also appears to be encoded by the chromosome. pDEC could be transferred only to cured derivatives of Pseudomonas C12B, but not to strains of P. aeruginosa, P. putida, or Acinetobacter sp. Cured derivatives of Pseudomonas C12B could not serve as hosts for the broad host range plasmid CAM–OCT. The enzyme system encoded by the putative dec genes present on plasmid pDEC differs from the system coded by the alk genes of plasmid OCT in the size range of hydrocarbons preferentially used.
Keywords:Bacteria  Biodegradation  Olefins  Paraffins  Sulfur compounds  Molecular structure  Gels  Antibiotics  Enzymes  Chromosomes  Surface active agents  Curing  Alkyl sulfate  Alkylbenzene sulfonate
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