The regulatory control of the bacterial luminescence system—A new view
- 1 July 1989
- journal article
- research article
- Published by Wiley in Journal of Bioluminescence and Chemiluminescence
- Vol. 4 (1) , 317-325
- https://doi.org/10.1002/bio.1170040144
Abstract
We have recently shown that the transcription of the PR lux operon for Vibrio fischeri luminescence is positively controlled by the htpR (σ32) protein. It was suggested that the LexA protein might negatively control the lux genes. This paper extends these findings. It was found that Escherichia coli cells that contain the entire lux operon (pChv1) in RecA or LexA mutants which are unable to remove the LexA protein are considerable dimmer than the wild‐type strain. Mutants that do not make LexA or from a weakly bound LexA are very bright. The role of σ32 protein was studied on luxR‐luxl genes that are fused to β‐galactosidase. The addition of V. fischeri inducer brings about the formation of β‐galactosidase activity in htpR+ but not in htpR− strains of E. coli/pMJ3. Similar to the effect of starvation on the induction of luminescence in marine bacteria and in E. coli/pChv1 cells, β‐galactrosidase activity in such constructs is preferentially induced by low nutrient concentrations. A new model for the regulatory control of the V. fischeri luminescence system is discussed.Keywords
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