Simultaneous Monitoring of Cell Number and Metabolic Activity of Specific Bacterial Populations with a Dual gfp-luxAB Marker System

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Applied and Environmental Microbiology, February 1999, p. 813-821, Vol. 65, No. 2
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Simultaneous Monitoring of Cell Number and Metabolic Activity of Specific Bacterial Populations with a Dual gfp-luxAB Marker System

Annika Unge, Riccardo Tombolini, Lars Mølbak, and Janet K. Jansson^*

Department of Biochemistry, Stockholm University, S-10691 Stockholm, Sweden

Received 18 May 1998/Accepted 12 November 1998

A dual marker system was developed for simultaneous quantification of bacterial cell numbers and their activity with the luxABand gfp genes, encoding bacterial luciferase and green fluorescentprotein (GFP), respectively. The bioluminescence phenotype ofthe luxAB biomarker is dependent on cellular energy status. Sincecellular metabolism requires energy, bioluminescence output isdirectly related to the metabolic activity of the cells. By contrast,GFP fluorescence has no energy requirement. Therefore, by combiningthese two biomarkers, total cell number and metabolic activityof a specific marked cell population could be monitored simultaneously.Two different bacterial strains, Escherichia coli DH5 $alpha$ and Pseudomonasfluorescens SBW25, were chromosomally tagged with the dual markercassette, and the cells were monitored under different conditionsby flow cytometry, plate counting, and luminometry. During log-phasegrowth, the luciferase activity was proportional to the numberof GFP-fluorescent cells and culturable cells. Upon entrance intostationary phase or during starvation, luciferase activity decreaseddue to a decrease in cellular metabolic activity of the population,but the number of GFP-fluorescing cells and culturable cells remainedrelatively stable. In addition, we optimized a procedure for extractionof bacterial cells from soil, allowing GFP-tagged bacteria insoil samples to be quantitated by flow cytometry. After 30 daysof incubation of P. fluorescens SBW25::gfp/lux in soil, the cellswere still maintained at high population densities, as determinedby GFP fluorescence, but there was a slow decline in luciferaseactivity, implicating nutrient limitation. In conclusion, thedual marker system allowed simultaneous monitoring of the metabolicactivity and cell number of a specific bacterial population andis a promising tool for monitoring of specific bacteria in situin environmentalsamples.

^* Corresponding author. Mailing address: Department of Biochemistry, Stockholm University, S-10691 Stockholm, Sweden. Phone:46-8-16 2469. Fax: 46-8-15 3679. E-mail: janet{at}biokemi.su.se.

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