Bioluminescence of the insect pathogen Xenorhabdus luminescens

Author:

Schmidt T M1,Kopecky K1,Nealson K H1

Affiliation:

1. Center for Great Lakes Studies, University of Wisconsin-Milwaukee 53204.

Abstract

Luminescence of batch cultures of Xenorhabdus luminescens was maximal when cultures approached stationary phase; the onset of in vivo luminescence coincided with a burst of synthesis of bacterial luciferase, the enzyme responsible for luminescence. Expression of luciferase was aldehyde limited at all stages of growth, although more so during the preinduction phase. Luciferase was purified from cultures of X. luminescens Hm to a specific activity of 4.6 x 10(13) guanta/s per mg of protein and found to be similar to other bacterial luciferases. The Xenorhabdus luciferase consisted of two subunits with approximate molecular masses of 39 and 42 kilodaltons. A third protein with a molecular mass of 24 kilodaltons copurified with luciferase, and in its presence, either NADH or NADPH was effective in stimulating luminescence, indicating that this protein is an NAD(P)H oxidoreductase. Luciferases from two other luminous bacteria, Vibrio harveyii (B392) and Vibrio cholerae (L85), were partially purified, and their subunits were separated in 5 M urea and tested for complementation with the subunits prepared from X. luminescens Hb. Positive complementation was seen with luciferase subunits among all three species. The slow decay kinetics of the Xenorhabdus luciferase were attributed to the alpha subunit.

Publisher

American Society for Microbiology

Subject

Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology

Reference29 articles.

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4. Mutationally altered bacterial Iuciferase: implications for subunit functions;Cline T. W.;Biochemistry,1972

5. Nucleotide sequence of the IuxA gene of Vibrio harveyi and the complete amino acid sequence of the alpha subunit of bacterial Iuciferase;Cohn D. H.;J. Biol. Chem.,1985

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