Phase variation in Xenorhabdus luminescens: cloning and sequencing of the lipase gene and analysis of its expression in primary and secondary phases of the bacterium.

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J Bacteriol. 1993 March; 175(6): 1665-1673

research-article

Phase variation in Xenorhabdus luminescens: cloning and sequencing of the lipase gene and analysis of its expression in primary and secondary phases of the bacterium.

H Wang and B C Dowds

Department of Biology, St. Patrick's College, Maynooth, County Kildare, Ireland.

ABSTRACT

The phenomenon of phase variation in the insect-pathogenic bacteriumXenorhabdus luminescens was investigated. Differential activityof the lipase enzyme (EC 3.1.1.3) was observed between the twophases of the bacteria. The enzyme was found to be secretedinto the culture medium, and about five to six times greaterspecific activity was secreted by the primary phase than bythe secondary form. The lipase gene (lip-1) was cloned and sequenced.The data imply that there is only a single Tween 80-utilizinglipase gene in X. luminescens K122. The sequence revealed atranslation product of 645 amino acids, from which a hydrophobicleader sequence of 24 amino acids is removed during processing.The structure of the gene was shown to be the same in the primaryand secondary forms of X. luminescens. In addition, transcriptionwas found to start at the same position, 169 bp upstream ofthe translation initiation codon, in the two forms of the bacteria.Equal amounts of lipase RNA accumulated in the two forms, andat least as much lipase protein was secreted by the secondaryform as by the primary. This suggests that the difference inspecific activity between the enzymes secreted by the two phasesprobably arises from a posttranslational type of regulation.

J Bacteriol. 1993 March; 175(6): 1665-1673

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