Biofilm exclusion of uropathogenic bacteria by selected asymptomatic bacteriuria Escherichia coli strains
- 1 June 2007
- journal article
- Published by Microbiology Society in Microbiology
- Vol. 153 (6) , 1711-1719
- https://doi.org/10.1099/mic.0.2006/004721-0
Abstract
Butane monooxygenase (sBMO) has been purified to homogeneity from the Gram-negative β-proteobacterium ‘Pseudomonas butanovora’ and confirmed to be a three-component diiron monooxygenase system. The reconstituted enzyme complex oxidized C3–C6 linear and branched aliphatic alkanes, which are growth substrates for ‘P. butanovora’. The sBMO complex was composed of an iron-containing hydroxylase (BMOH), a flavo-iron sulfur-containing NADH-oxidoreductase (BMOR) and a small regulatory component protein (BMOB). The physical characteristics of sBMO were remarkably similar to the sMMO family of soluble multicomponent diiron monooxgenases. However, the catalytic properties of sBMO were quantitatively different in regard to inactivation in the presence of substrate and product distribution. BMOH was capable of ethene oxidation when supplied with H2O2 and ethene (known as the peroxide shunt), but this activity was at least three orders of magnitude less than that observed for the hydroxylase of sMMO of Methylosinus trichosporium OB3b. BMOH and BMOR were efficient in the oxidation of ethene in the absence of BMOB with regard to rate of reaction and product yield. Regiospecificity of sBMO was strongly biased towards primary hydroxylation, with ≥80 % of the hydroxylations occurring at the terminal carbon atom.Keywords
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