Use of Green Fluorescent Protein To Tag and Investigate Gene Expression in Marine Bacteria

Stretton, Serina; Techkarnjanaruk, Somkiet; McLennan, Alan M.; Goodman, Amanda E.

doi:10.1128/aem.64.7.2554-2559.1998

Cited by 74 publications

(36 citation statements)

References 46 publications

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“…Green fluorescent protein (GFP)‐expressing strains are now frequently used for tracking specific microbial strains in ecosystems. Bacteria marked with gfp have been employed to study the distribution and dynamics of bacterial populations in soils (Errampalli et al ., 1998; Tresse et al ., 1998), aqueous systems (Stretton et al ., 1998), rhizospheres (Gage et al ., 1996; Bloemberg et al ., 1997; Tombolini et al ., 1997), activated‐sludge (Eberl et al ., 1997; Olofsson et al ., 1998) and biofilms (Möller et al ., 1998; Skillman et al ., 1998). Furthermore, GFPs can be used to visualize gene expression (Cubitt et al ., 1995; Andersen et al ., 1998; Jaspers et al., 2001).…”

Section: Introductionmentioning

confidence: 99%

Effect of integration of a GFP reporter gene on fitness of Ralstonia eutropha during growth with 2,4‐dichlorophenoxyacetic acid

Füchslin

Rüegg

Meer

et al. 2003

Environmental Microbiology

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Green fluorescent proteins (GFPs) are frequently used as marker and reporter systems to assess the fate and activity of microbial strains with the ability to degrade xenobiotic compounds. To evaluate the potential of this tool for tracking herbicide-degrading microorganisms in the environment a promoterless gfp was linked to the tfd C promoter, which is activated during degradation of the herbicide 2,4-dichlorophenoxyacetic acid (2,4-D), and integrated into the chromosome of the 2,4-D-degrading strain Ralstonia eutropha JMP 134. The effects of the inserted gfp gene on the kinetics of 2,4-D degradation by R. eutropha in batch and chemostat culture were compared to those of the wild-type strain. In batch culture with 2,4-D as the only carbon and energy source the maximum specific growth rate of the gfp-marked strain did not differ significantly from the wild type. However, compared to the wild type, the 2,4-D steady-state concentration in 2,4-D-limited chemostat cultures of the gfp-marked strain was higher at all dilution rates tested. The reduced competitiveness of the gfp-marked strain at low substrate concentrations was confirmed in a competition experiment for 2,4-D in continuous culture at a dilution rate of 0.075 h-1. Reproducibly, the gfp-marked strain was displaced by the wild-type strain. The study clearly demonstrates that fitness of constructs cannot be assessed by measuring micro max with selected substrates in batch cultures only but that a thorough kinetic analysis is needed, which also considers slow, carbon-limited growth conditions as they occur in the environment.

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Section: Introductionmentioning

confidence: 99%

Effect of integration of a GFP reporter gene on fitness of Ralstonia eutropha during growth with 2,4‐dichlorophenoxyacetic acid

Füchslin

Rüegg

Meer

et al. 2003

Environmental Microbiology

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“…Thus, K. ascorbata SUD165/26 was labeled with green £uorescent protein (GFP) from the jelly¢sh Aquoria victoria, and with luciferase (Lux) from the bacterium Vibrio harveyi. GFP and Lux are both very sensitive, easily detected and can be quanti¢ed with a spectro£uorimeter or a luminometer [13,14], thereby providing a simple and accurate means of monitoring and localizing selected bacteria in a complex environment.…”

Section: Introductionmentioning

confidence: 99%

Biological activity and colonization pattern of the bioluminescence-labeled plant growth-promoting bacterium Kluyvera ascorbata SUD165/26

Zalec

Glick

2001

FEMS Microbiology Ecology

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Kluyvera ascorbata SUD165/26 is a spontaneous siderophore-overproducing mutant of K. ascorbata SUD165, which was previously isolated from nickel-contaminated soil and shown to significantly enhance plant growth in soil contaminated with high levels of heavy metals. To develop a better understanding of the functioning of K. ascorbata SUD165/26 in the environment, and to trace its distribution in the rhizosphere, isolates of this bacterium were labeled with either green fluorescent protein or luciferase. When the plant growth-promoting activities of the labeled strains were assayed and compared with the activities of the unlabeled strain, none of the monitored parameters had changed to any significant extent. When the spatial colonization patterns of the labeled bacteria on canola roots were determined after seed application, it was observed that the bacterium was tightly attached to the surface of both roots and seeds, and formed aggregates. The majority of the bacterial population inhabited the upper two thirds of the roots, with no bacteria detected around the root tips.

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“…10% of the cells had lost the plasmid (data not shown). Other studies using bacteria tagged with a plasmidbased gfp construct also demonstrated that during colonization of substrates, part of the population lost their ability to express GFP (Gage et al 1996;Stretton et al 1998). To guarantee stable expression in long term in planta studies, the gene encoding GFP should be introduced into the bacterial chromosome, which is more stable than those plasmidborne (Errampalli et al 1999).…”

Section: Discussionmentioning

confidence: 99%

Colonization of siliques and seeds of rapid cycling Brassica oleracea plants by Xanthomonas campestris pv. campestris after spray-inoculation of flower clusters

et al. 2019

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Colonization of siliques and seeds of rapid cycling Brassica oleracea plants by Xanthomonas campestris pv. campestris after spray-inoculation of flower clusters Abstract Glasshouse experiments were conducted to study the colonization of seedpods (siliques) and seeds of rapid cycling Brassica oleracea plants after spraying inoculum on clusters of recently opened flowers with Xanthomonas campestris pv. campestris (Xcc) at densities of 10 7 -10 8 cfu ml −1 . A green fluorescent protein (GFP) tagged Xcc strain was used to allow visualization of the bacteria by epifluorescence stereo microscopy (ESM) and confocal laser scanning microscopy (CLSM). The GFP-tagged strain showed reduced virulence compared to the untagged parental strain, but was still able to cause black rot symptoms. Two to three days after sprayinoculation, sepals, stamen and petals were colonized by Xcc, as observed by ESM. In green siliques a GFP-signal was observed on valves, septa and seeds, despite the fact that a high percentage of Xcc cells had lost their ability to express GFP as found by dilution-plating. Densities of Xcc in infected silique tissues were up to 10 9 cfu g −1 . A fluorescent signal using ESM was found in seeds harvested from symptomatic siliques after incubation of seeds on blotting paper wetted with broth to enhance the multiplication of Xcc. Xcc was found in association with the seed coat and in a single seed, also in the endosperm and embryo, indicating deep-seated seed infection. The estimated incidence of contaminated seeds in both years was ca. 7%. The estimated incidence of deep-seated infections, still detectable after warm water treatment of seeds, was also high (2-3.8%). It is concluded that spray-inoculation of flower clusters with Xcc can result in the infection of sepals and reproductive organs, and in deep-seated seed infections.

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Use of Green Fluorescent Protein To Tag and Investigate Gene Expression in Marine Bacteria

Cited by 74 publications

References 46 publications

Effect of integration of a GFP reporter gene on fitness of Ralstonia eutropha during growth with 2,4‐dichlorophenoxyacetic acid

Effect of integration of a GFP reporter gene on fitness of Ralstonia eutropha during growth with 2,4‐dichlorophenoxyacetic acid

Biological activity and colonization pattern of the bioluminescence-labeled plant growth-promoting bacterium Kluyvera ascorbata SUD165/26

Colonization of siliques and seeds of rapid cycling Brassica oleracea plants by Xanthomonas campestris pv. campestris after spray-inoculation of flower clusters

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