Cloning of a Genetically Unstable Cytochrome P-450 Gene Cluster Involved in Degradation of the Pollutant Ethyl tert -Butyl Ether by Rhodococcus ruber

Author:

Chauvaux Sylvie1,Chevalier Fabien2,Le Dantec Corinne3,Fayolle Françoise4,Miras Isabelle1,Kunst Frank2,Beguin Pierre1

Affiliation:

1. Unité Microbiologie et Environnement and URA 2172,1

2. Laboratoire de Génomique des Microorganismes Pathogènes,2 and

3. Laboratoire de Référence des Mycobactéries,3Institut Pasteur, 75724 Paris Cedex 15, and

4. Département de Microbiologie, Institut Français du Pétrole, 92852 Rueil-Malmaison Cedex,4 France

Abstract

ABSTRACT Rhodococcus ruber (formerly Gordonia terrae ) IFP 2001 is one of a few bacterial strains able to degrade ethyl tert- butyl ether (ETBE), which is a major pollutant from gasoline. This strain was found to undergo a spontaneous 14.3-kbp chromosomal deletion, which results in the loss of the ability to degrade ETBE. Sequence analysis of the region corresponding to the deletion revealed the presence of a gene cluster, ethABCD , encoding a ferredoxin reductase, a cytochrome P-450, a ferredoxin, and a 10-kDa protein of unknown function, respectively. The EthB and EthD proteins could be easily detected by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and were induced by ETBE in the wild-type strain. Upstream of ethABCD lies ethR , which codes for a putative positive transcriptional regulator of the AraC/XylS family. Transformation of the ETBE-negative mutant by a plasmid carrying the ethRABCD genes restored the ability to degrade ETBE. Complementation was abolished if the plasmid carried ethRABC only. The eth genes are located in a DNA fragment flanked by two identical direct repeats of 5.6 kbp. The ETBE-negative mutants carry a single copy of this 5.6-kbp repeat, suggesting that the 14.3-kbp chromosomal deletion resulted from a recombination between the two identical sequences. The 5.6-kbp repeat is a class II transposon carrying a TnpA transposase, a truncated form of the recombinase TnpR, and a terminal inverted repeat of 38 bp. The truncated TnpR is encoded by an IS 3 -interrupted tnpR gene.

Publisher

American Society for Microbiology

Subject

Molecular Biology,Microbiology

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