Bacterial Activity in the Rhizosphere Analyzed at the Single-Cell Level by Monitoring Ribosome Contents and Synthesis Rates

ABSTRACT The growth activity of Pseudomonas putida cells colonizing the rhizosphere of barley seedlings was estimated at the single-cell level by monitoring ribosomal contents and synthesis rates. Ribosomal synthesis was monitored by using a system comprising a fusion of the ribosomal Escherichia coli rrnBP1 promoter to a gene encoding an unstable variant of the green fluorescent protein (Gfp). Gfp expression in a P. putida strain carrying this system inserted into the chromosome was strongly dependent on the growth phase and growth rate of the strain, and cells growing exponentially at rates of ≥0.17 h−1 emitted growth rate-dependent green fluorescence detectable at the single-cell level. The single-cell ribosomal contents were very heterogeneous, as determined by quantitative hybridization with fluorescently labeled rRNA probes in P. putida cells extracted from the rhizosphere of 1-day-old barley seedlings grown under sterile conditions. After this, cells extracted from the root system had ribosomal contents similar to those found in starved cells. There was a significant decrease in the ribosomal content of P. putida cells when bacteria were introduced into nonsterile bulk or rhizosphere soil, and the Gfp monitoring system was not induced in cells extracted from either of the two soil systems. The monitoring system used permitted nondestructive in situ detection of fast-growing bacterial microcolonies on the sloughing root sheath cells of 1- and 2-day-old barley seedlings grown under sterile conditions, which demonstrated that it may be possible to use the unstable Gfp marker for studies of transient gene expression in plant-microbe systems.

Download Full-text

Chimeric green fluorescent protein-aequorin as bioluminescent Ca2+ reporters at the single-cell level

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.97.13.7260 ◽

2000 ◽

Vol 97 (13) ◽

pp. 7260-7265 ◽

Cited By ~ 189

Author(s):

V. Baubet ◽

H. Le Mouellic ◽

A. K. Campbell ◽

E. Lucas-Meunier ◽

P. Fossier ◽

...

Keyword(s):

Green Fluorescent Protein ◽

Single Cell ◽

Fluorescent Protein ◽

Single Cell Level ◽

Cell Level ◽

Green Fluorescent

Download Full-text

Heteroresistance at the Single-Cell Level: Adapting to Antibiotic Stress through a Population-Based Strategy and Growth-Controlled Interphenotypic Coordination

mBio ◽

10.1128/mbio.00942-13 ◽

2014 ◽

Vol 5 (1) ◽

Cited By ~ 33

Author(s):

Xiaorong Wang ◽

Yu Kang ◽

Chunxiong Luo ◽

Tong Zhao ◽

Lin Liu ◽

...

Keyword(s):

Growth Rate ◽

Single Cell ◽

Task Allocation ◽

Bacterial Population ◽

Population Based ◽

Phenotypic Heterogeneity ◽

Single Cell Level ◽

Bacterial Survival ◽

Cell Level ◽

Resistant Cells

ABSTRACT Heteroresistance refers to phenotypic heterogeneity of microbial clonal populations under antibiotic stress, and it has been thought to be an allocation of a subset of “resistant” cells for surviving in higher concentrations of antibiotic. The assumption fits the so-called bet-hedging strategy, where a bacterial population “hedges” its “bet” on different phenotypes to be selected by unpredicted environment stresses. To test this hypothesis, we constructed a heteroresistance model by introducing a bla CTX-M-14 gene (coding for a cephalosporin hydrolase) into a sensitive Escherichia coli strain. We confirmed heteroresistance in this clone and that a subset of the cells expressed more hydrolase and formed more colonies in the presence of ceftriaxone (exhibited stronger “resistance”). However, subsequent single-cell-level investigation by using a microfluidic device showed that a subset of cells with a distinguishable phenotype of slowed growth and intensified hydrolase expression emerged, and they were not positively selected but increased their proportion in the population with ascending antibiotic concentrations. Therefore, heteroresistance—the gradually decreased colony-forming capability in the presence of antibiotic—was a result of a decreased growth rate rather than of selection for resistant cells. Using a mock strain without the resistance gene, we further demonstrated the existence of two nested growth-centric feedback loops that control the expression of the hydrolase and maximize population growth in various antibiotic concentrations. In conclusion, phenotypic heterogeneity is a population-based strategy beneficial for bacterial survival and propagation through task allocation and interphenotypic collaboration, and the growth rate provides a critical control for the expression of stress-related genes and an essential mechanism in responding to environmental stresses. IMPORTANCE Heteroresistance is essentially phenotypic heterogeneity, where a population-based strategy is thought to be at work, being assumed to be variable cell-to-cell resistance to be selected under antibiotic stress. Exact mechanisms of heteroresistance and its roles in adaptation to antibiotic stress have yet to be fully understood at the molecular and single-cell levels. In our study, we have not been able to detect any apparent subset of “resistant” cells selected by antibiotics; on the contrary, cell populations differentiate into phenotypic subsets with variable growth statuses and hydrolase expression. The growth rate appears to be sensitive to stress intensity and plays a key role in controlling hydrolase expression at both the bulk population and single-cell levels. We have shown here, for the first time, that phenotypic heterogeneity can be beneficial to a growing bacterial population through task allocation and interphenotypic collaboration other than partitioning cells into different categories of selective advantage.

Download Full-text

Stratified Growth in Pseudomonas aeruginosa Biofilms

Applied and Environmental Microbiology ◽

10.1128/aem.70.10.6188-6196.2004 ◽

2004 ◽

Vol 70 (10) ◽

pp. 6188-6196 ◽

Cited By ~ 230

Author(s):

Erin Werner ◽

Frank Roe ◽

Amandine Bugnicourt ◽

Michael J. Franklin ◽

Arne Heydorn ◽

...

Keyword(s):

Pseudomonas Aeruginosa ◽

Protein Synthesis ◽

Fluorescent Protein ◽

Anaerobic Growth ◽

Synthetic Activity ◽

Gene Encoding ◽

Rate Dependent ◽

Air Interface ◽

Transmission Electron ◽

Green Fluorescent

ABSTRACT In this study, stratified patterns of protein synthesis and growth were demonstrated in Pseudomonas aeruginosa biofilms. Spatial patterns of protein synthetic activity inside biofilms were characterized by the use of two green fluorescent protein (GFP) reporter gene constructs. One construct carried an isopropyl-β-d-thiogalactopyranoside (IPTG)-inducible gfpmut2 gene encoding a stable GFP. The second construct carried a GFP derivative, gfp-AGA, encoding an unstable GFP under the control of the growth-rate-dependent rrnBp 1 promoter. Both GFP reporters indicated that active protein synthesis was restricted to a narrow band in the part of the biofilm adjacent to the source of oxygen. The zone of active GFP expression was approximately 60 μm wide in colony biofilms and 30 μm wide in flow cell biofilms. The region of the biofilm in which cells were capable of elongation was mapped by treating colony biofilms with carbenicillin, which blocks cell division, and then measuring individual cell lengths by transmission electron microscopy. Cell elongation was localized at the air interface of the biofilm. The heterogeneous anabolic patterns measured inside these biofilms were likely a result of oxygen limitation in the biofilm. Oxygen microelectrode measurements showed that oxygen only penetrated approximately 50 μm into the biofilm. P. aeruginosa was incapable of anaerobic growth in the medium used for this investigation. These results show that while mature P. aeruginosa biofilms contain active, growing cells, they can also harbor large numbers of cells that are inactive and not growing.

Download Full-text

Detection of uncoupled circadian rhythms in individual cells of Lemna minor using a dual-color bioluminescence monitoring system

10.1101/2020.06.10.143727 ◽

2020 ◽

Author(s):

Emiri Watanabe ◽

Minako Isoda ◽

Tomoaki Muranaka ◽

Shogo Ito ◽

Tokitaka Oyama

Keyword(s):

Circadian Rhythms ◽

Single Cell ◽

Monitoring System ◽

Lemna Minor ◽

Single Cell Level ◽

Cell Level ◽

Dual Color ◽

Stochastic Phenomena ◽

Circadian Behavior ◽

Bioluminescent Reporters

SummaryThe plant circadian oscillation system is based on the circadian clock of individual cells and coordinates the circadian behavior of the plant body. To observe the cellular circadian behavior of both the oscillator and its output in plants, we developed the dual-color bioluminescence monitoring system that automatically measured the luminescence of two luciferase reporters simultaneously at a single-cell level. We selected a yellow-green-emitting firefly luciferase (LUC+) and a red-emitting luciferase (PtRLUC) that is a mutant form of Brazilian click beetle ELUC. We used AtCCA1::LUC+ and CaMV35S::PtRLUC to observe the cellular behavior of the oscillator and output, respectively. These bioluminescent reporters were introduced into the cells of a duckweed, Lemna minor, by particle bombardment. Time series of the bioluminescence of individual cells in a frond were obtained using a dual-color bioluminescence monitoring system with a green-pass- and red-pass filter. Luminescence intensities from the LUC+ and PtRLUC of each cell were calculated from the filtered luminescence intensities. We succeeded in reconstructing the bioluminescence behaviors of AtCCA1::LUC+ and CaMV35S::PtRLUC in the same cells. Under prolonged constant light conditions, AtCCA1::LUC+ showed a robust circadian rhythm in individual cells in an asynchronous state in the frond, as previously reported in studies using other plants. In contrast, CaMV35S::PtRLUC stochastically showed circadian rhythms in a synchronous state. Thus, we clearly demonstrated the uncoupling between the oscillator and output in individual cells. This dual-color bioluminescence monitoring system is a powerful tool to analyze various stochastic phenomena accompanying large cell-to-cell variation in gene expression.Significance statementWe succeeded in establishing the world’s first dual-color bioluminescence monitoring system at a single-cell level that enables simultaneous measurement of the luminescence activities of two reporter genes in plants. This system is a strong tool to analyze stochastic phenomena, and we clearly demonstrated the uncoupling of rhythmic behavior between two bioluminescent reporters in individual cells that stochastically occurred in the same plant.

Download Full-text

Generation of genetic tools for gauging multiple gene expression at single cell level

Applied and Environmental Microbiology ◽

10.1128/aem.02956-20 ◽

2021 ◽

Author(s):

Marta Mellini ◽

Massimiliano Lucidi ◽

Francesco Imperi ◽

Paolo Visca ◽

Livia Leoni ◽

...

Keyword(s):

Gene Expression ◽

Image Processing ◽

Single Cell ◽

Fluorescent Protein ◽

Single Cells ◽

Phenotypic Heterogeneity ◽

Single Cell Level ◽

Cell Level ◽

Multiple Gene ◽

Genetic Tools

Key microbial processes in many bacterial species are heterogeneously expressed in single cells of bacterial populations. However, the paucity of adequate molecular tools for live, real-time monitoring of multiple gene expression at the single cell level has limited the understanding of phenotypic heterogeneity. In order to investigate phenotypic heterogeneity in the ubiquitous opportunistic pathogen Pseudomonas aeruginosa, a genetic tool that allows gauging multiple gene expression at the single cell level has been generated. This tool, named pRGC, consists in a promoter-probe vector for transcriptional fusions that carries three reporter genes coding for the fluorescent proteins mCherry, green fluorescent protein (GFP) and cyan fluorescent protein (CFP). The pRGC vector has been characterized and validated via single cell gene expression analysis of both constitutive and iron-regulated promoters, showing clear discrimination of the three fluorescence signals in single cells of a P. aeruginosa population, without the need of image-processing for spectral crosstalk correction. In addition, two pRGC variants have been generated for either i) integration of the reporter gene cassette into a single neutral site of P. aeruginosa chromosome, that is suitable for long-term experiments in the absence of antibiotic selection, or ii) replication in bacterial genera other than Pseudomonas. The easy-to-use genetic tools generated in this study will allow rapid and cost-effective investigation of multiple gene expression in populations of environmental and pathogenic bacteria, hopefully advancing the understanding of microbial phenotypic heterogeneity. IMPORTANCE Within a bacterial population single cells can differently express some genes, even though they are genetically identical and experience the same chemical and physical stimuli. This phenomenon, known as phenotypic heterogeneity, is mainly driven by gene expression noise and results in the emergence of bacterial sub-populations with distinct phenotypes. The analysis of gene expression at the single cell level has shown that phenotypic heterogeneity is associated with key bacterial processes, including competence, sporulation and persistence. In this study, new genetic tools have been generated that allow easy cloning of up to three promoters upstream of distinct fluorescent genes, making it possible to gauge multiple gene expression at the single cell level by fluorescent microscopy, without the need of advanced image-processing procedures. A proof of concept has been provided by investigating iron-uptake and iron-storage gene expression in response to iron availability in P. aeruginosa.

Download Full-text

Fluorescent protein-based FRET sensor for intracellular monitoring of redox status in bacteria at single cell level

Analytical and Bioanalytical Chemistry ◽

10.1007/s00216-014-8165-1 ◽

2014 ◽

Vol 406 (28) ◽

pp. 7195-7204 ◽

Cited By ~ 12

Author(s):

Bobin George Abraham ◽

Ville Santala ◽

Nikolai V. Tkachenko ◽

Matti Karp

Keyword(s):

Single Cell ◽

Fluorescent Protein ◽

Redox Status ◽

Single Cell Level ◽

Cell Level

Download Full-text

The critical size is set at a single-cell level by growth rate to attain homeostasis and adaptation

Nature Communications ◽

10.1038/ncomms2015 ◽

2012 ◽

Vol 3 (1) ◽

Cited By ~ 112

Author(s):

Francisco Ferrezuelo ◽

Neus Colomina ◽

Alida Palmisano ◽

Eloi Garí ◽

Carme Gallego ◽

...

Keyword(s):

Growth Rate ◽

Single Cell ◽

Critical Size ◽

Single Cell Level ◽

Cell Level

Download Full-text

A Combination of Direct Viable Counting, Fluorescence in situ Hybridization, and Green Fluorescent Protein Gene Expression for Estimating Plasmid Transfer at the Single Cell Level

Microbes and Environments ◽

10.1264/jsme2.21.101 ◽

2006 ◽

Vol 21 (2) ◽

pp. 101-111 ◽

Cited By ~ 5

Author(s):

Milko Jorquera ◽

Nobuyasu Yamaguchi ◽

Katsuji Tani ◽

Masao Nasu

Keyword(s):

Gene Expression ◽

In Situ Hybridization ◽

Green Fluorescent Protein ◽

Protein Gene ◽

Fluorescent Protein ◽

Green Fluorescent Protein Gene ◽

Single Cell Level ◽

Cell Level ◽

Green Fluorescent

Download Full-text

An image-based, dual fluorescence reporter assay to evaluate the efficacy of shRNA for gene silencing at the single-cell level

F1000Research ◽

10.12688/f1000research.3-60.v1 ◽

2014 ◽

Vol 3 ◽

pp. 60 ◽

Cited By ~ 1

Author(s):

Shin-ichiro Kojima ◽

Gary G. Borisy

Keyword(s):

Single Cell ◽

Fluorescent Protein ◽

Selection Marker ◽

Target Sequence ◽

Fluorescence Intensity Ratio ◽

Single Cell Level ◽

Reporter Assay ◽

Red Fluorescent Protein ◽

Dual Fluorescence ◽

Cell Level

RNA interference (RNAi) is widely used to suppress gene expression in a specific manner. The efficacy of RNAi is mainly dependent on the sequence of small interfering RNA (siRNA) in relation to the target mRNA. Although several algorithms have been developed for the design of siRNA, it is still difficult to choose a really effective siRNA from among multiple candidates. In this article, we report the development of an image-based, quantitative, ratiometric fluorescence reporter assay to evaluate the efficacy of RNAi at the single-cell level. Two fluorescence reporter constructs are used. One expresses the candidate small hairpin RNA (shRNA) together with an enhanced green fluorescent protein (EGFP); the other expresses a 19-nt target sequence inserted into a cassette expressing a red fluorescent protein (either DsRed or mCherry). Effectiveness of the candidate shRNA is evaluated as the extent to which it knocks down expression of the red fluorescent protein. Thus, the red-to-green fluorescence intensity ratio (appropriately normalized to controls) is used as the read-out for quantifying the siRNA efficacy at the individual cell level. We tested this dual fluorescence assay and compared predictions to actual endogenous knockdown levels for three different genes (vimentin, lamin A/C and Arp3) and twenty different shRNAs. For each of the genes, our assay successfully predicted the target sequences for effective RNAi. To further facilitate testing of RNAi efficacy, we developed a negative selection marker (ccdB) method for construction of shRNA and red fluorescent reporter plasmids that allowed us to purify these plasmids directly from transformed bacteria without the need for colony selection and DNA sequencing verification.

Download Full-text

In Situ Detection of High Levels of Horizontal Plasmid Transfer in Marine Bacterial Communities

Applied and Environmental Microbiology ◽

10.1128/aem.64.7.2670-2675.1998 ◽

1998 ◽

Vol 64 (7) ◽

pp. 2670-2675 ◽

Cited By ~ 101

Author(s):

Cecilia Dahlberg ◽

Maria Bergström ◽

Malte Hermansson

Keyword(s):

Gene Transfer ◽

Pseudomonas Putida ◽

Single Cell ◽

Fluorescent Protein ◽

Detection System ◽

Plasmid Transfer ◽

Conjugative Plasmid ◽

Epifluorescence Microscopy ◽

Single Cell Level ◽

Cell Level

ABSTRACT Gene transfer of the conjugative plasmid pBF1 fromPseudomonas putida to indigenous bacteria in seawater was investigated with a detection system for gene transfer based on the green fluorescent protein (GFP) (C. Dahlberg et al., Mol. Biol. Evol. 15:385–390, 1998). pBF1 was tagged with the gfp gene controlled by a lac promoter which is down regulated in the donor cell by a chromosomal repressor (lacI q). The plasmid donor cells (Pseudomonas putida KT2442) subsequently do not express gfp. Transfer to recipient strains lacking the repressor results in expression of gfp. The transconjugant can subsequently be detected by epifluorescence microscopy on a single-cell level. By using this method, transfer of pBF1::gfp and expression of the gfpgene were first shown to occur during nutrient-limiting conditions to several defined recipient bacteria in artificial seawater. Second, we measured transfer of pBF1 from P. putida to the marine bacterial community directly in seawater samples, on a single-cell level, without limiting the detection of gene transfer to the culturable fraction of bacteria. Plasmid transfer was detected on surfaces and in bulk seawater. Seawater bacteria with different morphologies were shown to receive the plasmid. Gene transfer frequencies of 2.3 × 10−6 to 2.2 × 10−4 transconjugants per recipient were recorded after 3 days of incubation.

Download Full-text