Skip to main content

ORIGINAL RESEARCH article

Front. Microbiol., 11 January 2016
Sec. Antimicrobials, Resistance and Chemotherapy

Study of the Aminoglycoside Subsistence Phenotype of Bacteria Residing in the Gut of Humans and Zoo Animals

  • 1Laboratory of Microbiology, Wageningen University, Wageningen, Netherlands
  • 2RIKILT, Wageningen University, Wageningen, Netherlands
  • 3National Institute of Public Health and Environment, Bilthoven, Netherlands

Recent studies indicate that next to antibiotic resistance, bacteria are able to subsist on antibiotics as a carbon source. Here we evaluated the potential of gut bacteria from healthy human volunteers and zoo animals to subsist on antibiotics. Nine gut isolates of Escherichia coli and Cellulosimicrobium sp. displayed increases in colony forming units (CFU) during incubations in minimal medium with only antibiotics added, i.e., the antibiotic subsistence phenotype. Furthermore, laboratory strains of E. coli and Pseudomonas putida equipped with the aminoglycoside 3′ phosphotransferase II gene also displayed the subsistence phenotype on aminoglycosides. In order to address which endogenous genes could be involved in these subsistence phenotypes, the broad-range glycosyl-hydrolase inhibiting iminosugar deoxynojirimycin (DNJ) was used. Addition of DNJ to minimal medium containing glucose showed initial growth retardation of resistant E. coli, which was rapidly recovered to normal growth. In contrast, addition of DNJ to minimal medium containing kanamycin arrested resistant E. coli growth, suggesting that glycosyl-hydrolases were involved in the subsistence phenotype. However, antibiotic degradation experiments showed no reduction in kanamycin, even though the number of CFUs increased. Although antibiotic subsistence phenotypes are readily observed in bacterial species, and are even found in susceptible laboratory strains carrying standard resistance genes, we conclude there is a discrepancy between the observed antibiotic subsistence phenotype and actual antibiotic degradation. Based on these results we can hypothesize that aminoglycoside modifying enzymes might first inactivate the antibiotic (i.e., by acetylation of amino groups, modification of hydroxyl groups by adenylation and phosphorylation respectively), before the subsequent action of catabolic enzymes. Even though we do not dispute that antibiotics could be used as a single carbon source, our observations show that antibiotic subsistence should be carefully examined with precise degradation studies, and that its mechanistic basis remains inconclusive.

Introduction

Antibiotic resistance is a global health problem, and resistance is prevalent in bacteria isolated from both human and animal sources (van den Bogaard and Stobberingh, 2000; Sommer et al., 2009). Also, other natural habitats, for example soil, represent a common reservoir of resistance genes (Dantas et al., 2008). Recent metatranscriptome analyses have revealed that antibiotic resistance genes are expressed in a broad range of natural habitats, even in the absence of obvious antibiotic selection pressure (Versluis et al., 2015). Furthermore, metagenomic studies of ancient environments have revealed that antibiotic resistance is a natural phenomenon that predates the anthropogenic selective pressure of clinical antibiotic use (D’Costa et al., 2011).

It has long been speculated that, for example in clinically relevant strains, genes conferring resistance to aminoglycoside antibiotics were derived from organisms producing aminoglycosides, suggesting that members of the Actinomycetes could have provided the initial pool of aminoglycoside resistance genes (Benveniste and Davies, 1973; Wright, 2007). Aminoglycosides are useful in the treatment of Gram-negative aerobic bacilli, staphylococci, and other Gram-positive bacterial infections (Yao and Moellering, 2007). The initial site of aminoglycoside action is the outer bacterial membrane, where the cationic antibiotic molecules create fissures in the outer cell membrane. These fissures result in leakage of intracellular contents, and enhanced antibiotic uptake. Once inside the bacterial cell, aminoglycosides inhibit protein synthesis by binding to the 30S ribosomal subunit (Gonzalez et al., 1998). Resistance to aminiglycosides is often due to enzymatic inactivation by acetyltransferases, nucleotidyltransferases and phosphotransferases. Other resistance mechanisms include loss of permeability, structural alteration of the ribosomal target and the presence of efflux pumps (Azucena and Mobashery, 2001). Streptomycin, a representative of aminoglycoside antibiotics produced naturally by bacteria, has been shown to participate in microbial survival pathways. These pathways can be defined as the capacity of bacterial metabolism to modulate antibiotic resistance (Martinez and Rojo, 2011). This could indicate that aminoglycosides, apart from inhibiting bacterial growth, could stimulate the acquisition of aminoglycoside resistance genes. This can play an important role in the survival of microorganisms, as indicated for the acetyltransferase involved in aminoglycoside resistance in Providencia stuartii (Goldberg et al., 1999; Barlow and Hall, 2002).

Recently a large and diverse group of bacteria from soil, seawater, and the gut of humans and farm animals were found to not merely resist the toxic effects of antibiotics, but also to use antibiotics including aminoglycosides as a single carbon source. This phenotype is commonly referred to as “antibiotic subsistence” (Dopazo et al., 1988; Dantas et al., 2008; Barnhill et al., 2011; Xin et al., 2012). In addition, the concept of bacteria subsisting on antibiotics has been referred to as “antibiotic-resistant extremophiles” (Gabani et al., 2012) or “antibiotrophs” (Woappi et al., 2014) These alternative terms depict the microorganisms as being able to subsist under harsh environmental conditions, e.g., elevated antibiotic concentrations or the use of antibiotics as the sole carbon source. In disagreement with the accumulating body of literature supporting the possibility of bacterial subsistence on antibiotics, Walsh et al. (2013) tested whether soil bacteria could subsist on antibiotics. As no degradation of antibiotics occurred, Walsh et al. (2013) concluded that soil bacteria could not utilize antibiotics (including streptomycin, trimethoprim, penicillin, and carbapenicillin) as a carbon source.

To date, no genes have been identified that could enable bacteria to use antibiotics as a single carbon source, and therefore the relationship between antibiotic resistance and antibiotic subsistence remains unclear (Dantas and Sommer, 2012). To this end, and since the gut microbiota of humans and animals has been described as a reservoir of antibiotic resistance, we studied the potential of gut bacteria to display the antibiotic subsistence phenotype using a range of antibiotics. Almost all of the bacteria able to subsist on antibiotics grew on an aminoglycoside, and therefore we focused on aminoglycosides to address mechanistic aspects of the subsistence phenotype that could be readily approached using laboratory model organisms.

Materials and Methods

Samples and Antibiotics Used

We evaluated the antibiotic subsistence phenotype of bacteria subsisting on a range of antibiotics: ampicillin, chloramphenicol, erythromycin, kanamycin, streptomycin and tetracycline (1mg/ml) (Sigma-Aldrich, Zwijndrecht, The Netherlands). Fecal samples from two healthy human volunteers and six species of exotic zoo animals (Burgers’ Zoo – Arnhem, the Netherlands) with no previous antibiotic administration (6 months) were used as inocula (Table 1). Fecal samples from zoo animals were taken by the zookeepers following internal standard regulations. The samples were collected immediately after defecation into a sterile container, and then stored at 4°C (for 0.5–4 h) before being transferred to –80°C.

TABLE 1
www.frontiersin.org

TABLE 1. Human and zoo animal fecal isolates with subsistence phenotype on antibiotics.

Isolating Bacteria with the Subsistence Phenotype

Fecal samples (∼200 mg) were suspended in 5 ml of M9 minimal salts medium (Sigma–Aldrich) and centrifuged twice (5 min at 18,400 g) to prevent carry-over of dissolved carbon from the fecal material. Washed bacterial cells were then suspended in 5 ml of fresh M9 medium, and 50 μl inoculated into 5 ml M9 medium supplemented with 1 mg/ml of a single antibiotic (98–99% purity) and incubated at 37°C for 24 h. Then, the cultures were serially transferred twice to a fresh media with antibiotic, followed by plating on Luria Broth agar (LB agar), to quantify the bacterial growth based on enumeration of colony forming units (CFU) on the LB plates were counted after 8, 24, 48 h of incubation at 37°C. The subsistence phenotype criteria was identified based on a twofold increase of CFUs over multiple transfers. A single colony was selected and tested to confirm the subsistence phenotype. Glucose (1 mg/ml) was used as a positive control, while M9 medium lacking any carbon source served as negative control for growth. All experiments were performed in duplicate.

Identification of Bacterial Isolates with the Subsistence Phenotype

Bacteria subsisting on antibiotics were selected for DNA amplification using the 27F and 1492R primers. PCR was carried out with FastStart Taq DNA polymerase (Roche) in a reaction mixture containing 10X Fast Taq buffer + MgCl2, dNTPs (10 mM each, Roche), 10 pmol of both primers in a final volume of 49 μl; finally add the template of DNA (1 μl). For the amplification reaction, after 5 min at 95°C, 35 identical cycles (30 s of denaturation at 95°C, 40 s of annealing at 52°C, 90 s of elongation at 72°C) were followed by a final elongation step of 7 min at 72°C. The amplified fragments were selected for partial sequence analysis of the 16S rRNA gene (∼800 bp) using the 1392R primer, and sequences were deposited in GenBank with accession numbers KT989026, KT989027, KT989028, KT989029, KT989030, KT989031, KT989032, KT989033, KT989034, KT989035 (Table 1). Furthermore, all isolates were tested for their antibiotic resistance phenotype by dilution agar test as recommended by Clinical and Laboratory Standards Institute (2014).

Experimental Controls to Differentiate Between Aminoglycoside Resistance and the Subsistence Phenotype

In order to differentiate between antibiotic resistance and antibiotic subsistence, we used transformants containing a gene encoding aminoglycoside 3′ phosphotransferase II (APH (3′) II) (Berg et al., 1975), one of the most common aminoglycoside-modifying enzymes in prokaryotes, as a control. In detail, chemically competent cells of two different strains of E. coli (DH5α and TOP10) were transformed by heat-shock with cloning vectors pRSF-1b (Novagen, Billerica, MA, USA) and pCR-2.1TOPO (Invitrogen, Carlsbad, CA, USA), respectively, both containing an APH (3′) II gene. Also, we used Pseudomonas putida TEC1 transformed with the cloning vector pUTmini-Tn5-Km1 (de Lorenzo et al., 1990; Leprince et al., 2012). Transformed and non-transformed strains were tested for their ability to resist and subsist on the aminoglycoside antibiotics kanamycin and neomycin using the protocol described above.

Effect of Deoxynojirimycin (DNJ) on the Aminoglycoside Subsistence Phenotype

To evaluate the involvement of glycosyl hydrolases (GH) in the subsistence phenotype on aminoglycoside we selected deoxynojirimycin (DNJ) (Laboratory of Organic Chemistry, Leiden University, The Netherlands), which is one of the simplest natural carbohydrate mimics that can competitively inhibit specific glycosidic enzymes (Hughes and Rudge, 1994). We tested the capacity of E. coli (DH5α) transformed with pRSF-1b plasmid-encoded APH (3′) II gene, to grow on kanamycin or glucose (1 mg/ml) as a single carbon source in the presence of DNJ (range of 0.00001–10 mM of DNJ) and monitored growth for 24 h. All the experiments were performed in triplicate and used 96-well plates. Growth was measured by OD = 600 nm for 24 h continuously during incubation at 37°C with agitation at 75 rpm.

Kanamycin Degradation by Escherichia coli

To investigate kanamycin degradation by E. coli we performed an LC-MS/MS analysis. The experimental control was carried out using E. coli (DH5α) with and without cloning vector pRSF-1b in the presence of kanamycin (99.25% Kanamycin A Sulfate, EvoPureTM, GENTAUR Netherlands) (1 mg/ml). An aliquot was taken at 0, 4, 8, 24 h, and analyzed in duplicate using LC-MS/MS. In detail, the samples were diluted 100 times in 0,065% heptafluorbutyric acid, with an expected concentration of 10 mg/L. Octamethylkanamycine was added as an internal standard to the diluted samples at a concentration of 10 mg/L. Fifty microliter of the diluted sample was injected using a 2690 separations module high-performance liquid chromatography (HPLC) system (Waters Corporation, USA) coupled to a Quattro Micro tandem mass detector (Waters-Micromass, Manchester, UK). For the analysis samples were separated using a Symmetry C18 (150 mm × 3 mm, 5 μm) chromatographic column from Waters (Milford, PA, USA) working at 30°C and at a flow rate of 0.4 ml/min. The mobile phase was water containing 0.065% heptafluorbutyric acid (A) mixed on a gradient mode with methanol containing 0.065% heptafluorbutyric acid (B), as follows: initiated at 100% A, from 100 to 55% A in 5 min, from 55 to 40% A in 11.5 min, kept isocratic at 60% B for 5 min, from 60% B to 0% B in 1 min for equilibration of the column (initial conditions). The mass spectrometer was operated in electrospray positive mode, and data acquisition was in multiple reactions monitoring mode (MRM). Source settings were as follows: capillary voltage 2.7 kV, cone voltage 25 V, source temperature 120°C, desolvation temperature 400°C, cone nitrogen gas flow 60 L/h, desolvation gas flow 600 L/h. Argon was used as the collision gas at 3.2 × 10-3 mbar. Calibration was done by means of a calibration curve (0, 2, 5, 10, and 20 mg/L) in 0.065% heptafluorbutyric acid. Quantification of kanamycin in the samples was done on the calibrators by means of isotope dilution using octamethylkanamycin. The bacterial culture was also plated on LB agar for growth assessment (CFU/ml) as described above.

Results

Gut Bacteria of Human and Zoo Animals Displayed Subsistence Phenotype

Nine isolates from human and animal fecal samples displayed subsistence phenotypes when cultivated with a single antibiotic as the sole carbon source: six on kanamycin, two on streptomycin, and one isolate displayed the subsistence phenotype on both erythromycin and kanamycin (Table 1). The subsistence phenotype was measured by plating and counting CFU increases, with a twofold increase of CFUs used to identify the phenotype. The isolates were classified by partial sequence analysis of 16S rRNA genes, and seven isolates were identified as E. coli and three as Cellulosimicrobium sp. The Cellulosimicrobium sp. are members of the family Promicromonosporaceae within the Actinobacteria, and were most closely related to Cellulosimicrobium cellulans and C. funkei (Table 1), which are all related to human pathogens (Funke et al., 1995; Kaper et al., 2004; Petkar et al., 2011). All nine isolates were resistant to two or more of the following antibiotics: ampicillin, chloramphenicol, tetracycline, erythromycin, streptomycin, and kanamycin (Table 1).

Experimental Controls to Differentiate Aminoglycoside Resistance and Subsistence Phenotype

Since nine isolates displayed the subsistence phenotype on aminoglycosides, mainly kanamycin, we included an experimental control in an attempt to differentiate between antibiotic resistance and antibiotic subsistence. This was performed by equipping laboratory strains with a plasmid-encoded APH (3′) II gene. All transformants of E. coli and P. putida, but none of the non-transformed strains, displayed the subsistence phenotype on kanamycin and neomycin (Table 2). Growth of the strains on glucose was similar to that in the presence of aminoglycosides, whereas no growth was observed in M9 medium to which no carbon source was added (Table 2).

TABLE 2
www.frontiersin.org

TABLE 2. Growth experiments (48 h, performed in duplicate) of non-resistant and resistant E. coli and P. putida strains on media containing no carbon source, glucose, or aminoglycosides (kanamycin, neomycin) in M9 minimal salts medium.

Effect of Deoxynojirimycin on the Aminoglycoside Subsistence Phenotype

In order to evaluate the involvement of GH in the subsistence phenotype on aminoglycoside, we tested the capacity of E. coli (DH5α) transformed with pRSF-1b plasmid- encoded APH (3′) II gene to grow on kanamycin or glucose as a single carbon source in the presence of DNJ (range of 0.00001–10 mM). Cultivability was measured by plating and counting CFUs during 24 h. We found that in the presence of DNJ and glucose, the bacteria showed initial growth retardation which was then rapidly overcome (Figure 1A). In contrast, adding DNJ to a minimal medium containing only kanamycin as a carbon source arrested growth completely. This suggested that glycosyl-hydrolases are required for the subsistence phenotype on kanamycin (Figure 1B).

FIGURE 1
www.frontiersin.org

FIGURE 1. Growth dynamics (in triplicate) of transformed E. coli in M9 medium containing glucose (1 mg/ml) (A) and kanamycin (B) in the presence of different concentrations of DNJ (in mM).

Kanamycin Degradation by Escherichia coli

Finally, we studied kanamycin degradation by E. coli (DH5α) in the presence or absence of the plasmid encoded APH (3) II gene using 1 mg/ml of high purity kanamycin (Evopure, 99.25%) in M9 medium. Bacterial growth was calculated using the plate counting method, and kanamycin was measured by LC-MS/MS. It was observed that the number of CFUs increased during the first 8 h, although no degradation of the antibiotic was observed (Table 3).

TABLE 3
www.frontiersin.org

TABLE 3. Concentration of kanamycin and colony forming units (CFUs) obtained in M9 minimal media with kanamycin (EvoPureTM-1 mg/ml) with and without resistant E. coli during LC-MS/MS experiments over time.

Discussion

We observed that two groups of bacteria, E. coli and Cellulosimicrobium sp., present in the gut microbiota of healthy human volunteers and zoo animals, displayed the subsistence phenotype on aminoglycosides and erythromycin as a single carbon source. The subsistence phenotype was defined as an increase of CFUs over multiple transfers compared to the inoculum incubated in the same media without a carbon source. In order to avoid the presence of residual carbon sources, we included a pre-washing step to prevent carry-over of dissolved carbon from the fecal material and used new sterile glass material and freshly prepared media. In addition, we included serial two-fold dilutions of glucose and kanamycin (1–0.0625 mg/ml) and observed the subsistence phenotype at all antibiotic concentrations including those more similar to amounts found in natural habitats (Trieu-Cuot and Courvalin, 1986; data not shown).

Subsistence phenotypes were found previously in P. fluorescens isolates obtained from lake sediments, which were described to utilize benzylpenicillin as a carbon, nitrogen and energy source (Johnsen, 1977). Soil bacteria from the orders Pseudomonadales and Burkholderiales have also been isolated based on their capacity to grow on a range of antibiotics as a single carbon source (Dantas et al., 2008). In another environment including clinical and non-clinical samples, Barnhill et al. (2011) observed that multi-resistant Salmonella spp. were also able to subsist on antibiotics, highlighting the potential prevalence of the antibiotic subsistence phenotype in a clinical context. Xin et al. (2012) showed that two members of the Enterobacteria group (e.g., Klebsiella pneumoniae and Escherichia fergusonii) isolated from fecal material of healthy volunteers were able to subsist and bio-degraded chloramphenicol as a sole carbon source. However, all the strains in the study were chloramphenicol susceptible, which indicates that the subsistence and resistance mechanisms were independent in this particular case.

In our study, since the majority of the bacteria seemed to subsist on aminoglycosides, we studied laboratory strains of E. coli and P. putida with a plasmid-encoded APH (3′) II gene in order to differentiate aminoglycoside resistance and the subsistence phenotype. Our results showed that a common resistance gene facilitates the subsistence phenotype on aminoglycosides, and these results indicated that resistance and subsistence mechanism might be linked. Similar subsistence phenotypes were obtained with P. putida TEC1 using the cloning vector pUTmini-Tn5-Km1 (de Lorenzo et al., 1990; Leprince et al., 2012), which similarly contains an APH (3′) II gene.

Previous studies have shown that kanamycin is stable under culture conditions for at least a week (Ryan et al., 1970). Stability has been attributed to its structure where a six-aminocyclitol ring is attached to aminosugar side chains through glycosidic bonds. We hypothesized that an intrinsic metabolic capacity to break down and utilize phosphorylated aminoglycosides is present in various bacteria. In the genomes of E. coli and P. putida a multitude of genes predicted to encode GH exist (40–50 in E. coli and 26 in P. putida), with typically between 20 and 22 GH gene families annotated in E. coli. The encoded enzymes could potentially be involved in breaking the glycosidic bonds in the aminoglycosides, releasing an accessible carbon source. Due to the large number of GH encoding genes though single and combinatorial gene knockouts would not be numerically feasible. It is also likely that this approach may not deliver the necessary result due to potential functional redundancy of these enzymes. In our study we showed that a specific glycosyl-hydrolase inhibiting iminosugar (DNJ) abolishes the subsistence phenotype on aminoglycosides. This suggests that glycosyl-hydrolase activity could be necessary for the hydrolysis of the glycosidic bond and subsequent release of the aminosugars from the aminoglycoside, and hence indicates an involvement of GH in the antibiotic subsistence phenotype.

Since we found several indications of aminoglycoside subsistence phenotypes in line with previous observations, we applied the LC-MS/MS method to study kanamycin degradation. However, no degradation of kanamycin was observed in our study. Our findings thus align with the previous observations by Walsh et al. (2013) suggesting that due to the lack of antibiotic degradation, the subsistence phenotype cannot be linked to the use of the antibiotic as a sole carbon source.

So far, no genes have been identified in the catabolic pathways of Kanamycin (http://www.ebi.ac.uk/chebi/chebiOntology.do?chebiId=CHEBI:6104). However, Stancu and Grifoll (2011), showed that several groups of Gram-positive and Gram-negative bacteria (including members of the Enterobacteriaceae family), displayed particular metabolic capabilities such as hydrocarbon degradation since these were able to grow on Poeni crude oil as a single carbon source. In addition, they show that Gram-negative bacteria possessed between two and four catabolic genes involved in degradation of saturated, monoaromatic, and polyaromatic hydrocarbons. Interestingly, these groups of bacteria were resistant to hydrophilic antibiotics such as ampicillin and kanamycin, and cellular and molecular modifications were induced by the antibiotic.

Since subsistence phenotypes on a range of antibiotics are readily observed, it is possible that antibiotic resistance genes frequently allow not only resistance, but also simultaneously facilitate antibiotic subsistence. Dantas and Sommer (2012) investigated the connection between subsistomes and resistomes, and indicated that thus far not a single gene involved in antibiotic subsistence has been identified. Although active aminoglycoside efflux pumps have been observed in E. coli (Mingeot-Leclercq et al., 1999), it is hypothesized that this mechanism is not actively involved in the E. coli clones subsisting on the antibiotics. This is because such activity would hinder accumulation of the drugs in the cytoplasm, where they are required for catabolism to occur.

Another potential subsistence mechanism that we considered was ribosomal protein mutations in spontaneous kanamycin resistant E. coli strains. It has been indicated that resistance to kanamycin and neomycin by ribosomal protein mutation is uncommon since this antibiotic binds to multiple sites on 30S and 50S ribosomal subunits, and high level resistance cannot be achieved by a single mutation (Kucers et al., 1997). However, aminoglycoside modifying enzymes encoded by plasmids including the acetyltransferases, adenyltransferases, and phosphotransferases encoded by plasmids (Neu, 1992) may inactivate antibiotics (i.e., by acetylation of amino groups, adenylation and phosphorylation of hydroxyl groups), before the subsequent action of the catabolic enzymes.

Based on our results we conclude that gut bacteria isolated were not able to degrade kanamycin and utilize it as a carbon source. Nevertheless, we observed that the presence of an aminoglycoside resistance gene supports the aminoglycoside subsistence phenotype, and GH seem to be required. This could indicate a possible link between the resistance and the subsistence phenotype. In addition, as we only tested one type of aminoglycoside modifying enzyme, we cannot assume that all the aminoglycoside modifying enzymes act in the same way. The different mechanisms of enzymatic modification could have different consequences. Further studies of kanamycin degradation linked to the evaluation of the subsistence phenotype and other aminoglycoside modifying enzymes may therefore provide further insight to the underlying subsistence mechanism.

Bacteria need to adapt to the growth medium in order to be able to metabolize the nutrients, and during the lag phase they are not completely inactive. They grow in size and develop primary metabolites (such as proteins, enzymes, and RNA) as well as coenzymes and division factors required for making new cells. These factors together with the mechanisms involved in antibiotic resistance could also be hypothesized to facilitate the antibiotic subsistence phenotype. It also may well be that bacteria simply need to be resistant to the antimicrobial in order to be able to exploit trace levels of non-toxic breakdown products. Future analyses including experimental evolution of antibiotic subsistence will help to further unravel the possible mechanisms involved in this phenotype. Nevertheless, since we were able to identify a bacterial strain that displayed the subsisting phenotype with both aminoglycoside (kanamycin) and macrolide (erythromycin) antibiotics, expansion of future studies to include resistance genes and metabolic pathways of macrolides as well as aminoglycosides could be of special interest.

Author Contributions

TB: designed and performed the experiments, analyzed, and interpreted the data and wrote the paper. TZ and GB: performed the LC-MS/MS experiments, analyzed the data, and revised the work critically for intellectual content. HS and MP: supervised the project, substantial contribution to revising it critically, and final approval of the version to be published.

Conflict of Interest Statement

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Acknowledgments

We are grateful to D. Aga, B. Atnafie, and J. Nyagwange for their experimental contributions, Dr. Audrey Leprince for strains and helpful suggestions and Dr. Joan Edwards for carefully checked the grammar issues. We thank the Dutch Organization for Health Research and Development (ZonMW, SEDAR project number 50-41700-98-034) as well as the European Community’s Seventh Framework Programme (EvoTAR project, grant agreement number FP7-HEALTH 2011-282004) for financial support.

References

Azucena, E., and Mobashery, S. (2001). Aminoglycoside-modifying enzymes: mechanisms of catalytic processes and inhibition. Drug Resist. Updat. 4, 106–117. doi: 10.1054/drup.2001.0197

PubMed Abstract | CrossRef Full Text | Google Scholar

Barlow, M., and Hall, B. G. (2002). Phylogenetic analysis shows that the OXA beta-lactamase genes have been on plasmids for millions of years. J. Mol. Evol. 55, 314–321. doi: 10.1007/s00239-002-2328-y

PubMed Abstract | CrossRef Full Text | Google Scholar

Barnhill, A. E., Weeks, K. E., Xiong, N., Day, T. A., and Carlson, S. A. (2011). Identification of multiresistant Salmonella isolates capable of subsisting on antibiotics. Appl. Environ. Microbiol. 76, 2678–2680. doi: 10.1128/AEM.02516-09

PubMed Abstract | CrossRef Full Text | Google Scholar

Benveniste, R., and Davies, J. (1973). Mechanisms of antibiotic resistance in bacteria. Annu. Rev. Biochem. 42, 471–506. doi: 10.1146/annurev.bi.42.070173.002351

CrossRef Full Text | Google Scholar

Berg, D. E., Davies, J., Allet, B., and Rochaix, J. D. (1975). Transposition of R factor genes to bacteriophage lambda. Proc. Natl. Acad. Sci. U.S.A. 72, 3628–3632.

Google Scholar

Clinical and Laboratory Standards Institute (2014). Methods for Dilution Antimicrobial Susceptibility Tests for Bacteria that Grow Aerobically, 9th Edn. Wayne, PA: Clinical and Laboratory Standards Institute.

Google Scholar

Dantas, G., Sommer, M. O., Oluwasegun, R. D., and Church, G. M. (2008). Bacteria subsisting on antibiotics. Science 320, 100–103. doi: 10.1126/science.1155157

PubMed Abstract | CrossRef Full Text | Google Scholar

Dantas, G., and Sommer, M. O. A. (2012). “Ecological and clinical consequences of antibiotic subsistence by environmental microbes,” in Antimicrobial Resistance in the Environment, 1st Edn, eds G. Dantas and M. O. A. Sommer (Hoboken, NJ: John Wiley & Sons).

Google Scholar

D’Costa, V. M., King, C. E., Kalan, L., Morar, M., Sung, W. W., Schwarz, C., et al. (2011). Antibiotic resistance is ancient. Nature 477, 457–461. doi: 10.1038/nature10388

PubMed Abstract | CrossRef Full Text | Google Scholar

de Lorenzo, V., Herrero, M., Jakubzik, U., and Timmis, K. N. (1990). Mini-Tn5 transposon derivatives for insertion mutagenesis, promoter probing, and chromosomal insertion of cloned DNA in gram-negative eubacteria. J. Bacteriol. 172, 6568–6572.

PubMed Abstract | Google Scholar

Dopazo, C. P., Lemos, M. L., Lodeiros, C., Bolinches, J., Barja, J. L., and Toranzo, A. E. (1988). Inhibitory activity of antibiotic-producing marine bacteria against fish pathogens. J. Appl. Bacteriol. 65, 97–101. doi: 10.1111/j.1365-2672.1988.tb01497.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Funke, G., Ramos, C. P., and Collins, M. D. (1995). Identification of some clinical strains of CDC coryneform group A-3 and A-4 bacteria as Cellulomonas species and proposal of Cellulomonas hominis sp. nov. for some group A-3 strains. J. Clin. Microbiol. 33, 2091–2097.

PubMed Abstract | Google Scholar

Gabani, P., Prakash, D., and Singh, O. V. (2012). Emergence of antibiotic-resistant extremophiles (AREs). Extremophiles 16, 697–713. doi: 10.1007/s00792-012-0475-7

PubMed Abstract | CrossRef Full Text | Google Scholar

Goldberg, M., Pribyl, T., Juhnke, S., and Nies, D. H. (1999). Energetic and topology of CzcA, a cation/proton antiporter of the resistance-nodulation-cell division protein family. J. Biol. Chem. 274, 26065–26070. doi: 10.1074/jbc.274.37.26065

CrossRef Full Text | Google Scholar

Gonzalez, U. S., Pharm, D., and Spencer, J. P. (1998). Aminoglycoside: a practical review. Am. Fam. Physician 58, 1811–1820.

Google Scholar

Hughes, A. B., and Rudge, A. J. (1994). Deoxynojirimycin: synthesis and biological activity. Nat. Prod. Rep. 14, 135–162. doi: 10.1039/np9941100135

CrossRef Full Text | Google Scholar

Johnsen, J. (1977). Utilization of benzylpenicillin as carbon, nitrogen and energy source by a Pseudomonas fluorescens strain. Arch. Microbiol. 115, 271–275. doi: 10.1007/BF00446452

PubMed Abstract | CrossRef Full Text | Google Scholar

Kaper, J. B., Nataro, J. P., and Mobley, H. L. (2004). Pathogenic Escherichia coli. Nat. Rev. Microbiol. 2, 123–140. doi: 10.1038/nrmicro818

PubMed Abstract | CrossRef Full Text | Google Scholar

Kucers, A., Crowe, S., Grayson, M. L., and Hoy, J. (eds) (1997). The Use of Antibiotics: A Clinical Review of Antibacterial, Antifungal and Antiviral Drugs, 5th Edn. Oxford: Butterworth Heinemann, 452–457.

Google Scholar

Leprince, A., de Lorenzo, V., Voller, P., Van Passel, M. W., and Martins Dos Santos, V. A. (2012). Random and cyclical deletion of large DNA segments in the genome of Pseudomonas putida. Environ. Microbiol. 14, 1444–1453. doi: 10.1111/j.1462-2920.2012.02730.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Martinez, J. L., and Rojo, F. (2011). Metabolic regulation of antibiotic resistance. FEMS Inmun. Med. Microbiol. 35, 768–789. doi: 10.1111/j.1574-6976.2011.00282.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Mingeot-Leclercq, M. P., Glupczynski, Y., and Tulkens, P. M. (1999). Aminoglycosides: activity and resistance. Antimicrob. Agents Chemother. 43, 727–737.

Google Scholar

Neu, H. C. (1992). The crisis of antibiotic resistance. Science 257, 1064–1073. doi: 10.1126/science.257.5073.1064

CrossRef Full Text | Google Scholar

Petkar, H., Li, A., Bunce, N., Duffy, K., Malnick, H., and Shah, J. J. (2011). Cellulosimicrobium funkei: first report of infection in a nonimmunocompromised patient and useful phenotypic tests for differentiation from Cellulosimicrobium cellulans and Cellulosimicrobium terreum. J. Clin. Microbiol. 49, 1175–1178. doi: 10.1128/JCM.01103-10

PubMed Abstract | CrossRef Full Text | Google Scholar

Ryan, K. J., Needham, G. M., Dunsmoor, C. L., and Sherris, J. C. (1970). Stability of antibiotics and chemotherapeutics in agar plates. Appl. Microbiol. 20, 447–451.

PubMed Abstract | Google Scholar

Sommer, M. O., Dantas, G., and Church, G. M. (2009). Functional characterization of the antibiotic resistance reservoir in the human microflora. Science 325, 1128–1131. doi: 10.1126/science.1176950

PubMed Abstract | CrossRef Full Text | Google Scholar

Stancu, M. M., and Grifoll, M. (2011). Multidrug resistance in hydrocarbon-tolerant Gram-positive and Gram-negative bacteria. J. Gen. Appl. Microbiol. 57, 1–18. doi: 10.2323/jgam.57.1

PubMed Abstract | CrossRef Full Text | Google Scholar

Trieu-Cuot, P., and Courvalin, P. (1986). Evolution and transfer of aminoglycoside resistance genes under natural conditions. J. Antimicrob. Chemother. 18, 93–102.

PubMed Abstract | Google Scholar

van den Bogaard, A. E., and Stobberingh, E. E. (2000). Epidemiology of resistance to antibiotics links between animals and humans. Int. J. Antimicrob. Agents 14, 327–335. doi: 10.1016/S0924-8579(00)00145-X

CrossRef Full Text | Google Scholar

Versluis, D., D’Andrea, M. M., Ramiro Garcia, J., Leimena, M. M., Hugenholtz, F., and Zhang, J. (2015). Mining microbial metatranscriptomes for expression of antibiotic resistance genes under natural conditions. Sci. Rep. 5:11981. doi: 10.1038/srep11981

PubMed Abstract | CrossRef Full Text | Google Scholar

Walsh, F., Amyes, S. G. B., and Duffy, B. (2013). Challenging the concept of bacteria subsisting on antibiotics. Int. J. Antimicrob. Agents 41, 558–563. doi: 10.1016/j.ijantimicag.2013.01.021

PubMed Abstract | CrossRef Full Text | Google Scholar

Woappi, Y., Gabani, P., Singh, A., and Singh, O. V. (2014). Antibiotrophs: the complexity of antibiotic-subsisting and antibiotic-resistant microorganisms. Crit. Rev. Microbiol. doi: 10.3109/1040841X.2013.875982 [Epub ahead of print].

PubMed Abstract | CrossRef Full Text | Google Scholar

Wright, G. D. (2007). The antibiotic resistome: the nexus of chemical and genetic diversity. Nat. Rev. Microbiol. 5, 175–186. doi: 10.1038/nrmicro1614

PubMed Abstract | CrossRef Full Text | Google Scholar

Xin, Z., Fengwei, T., Gang, W., Xiaoming, L., Qiuxiang, Z., Hao, Z., et al. (2012). Isolation, identification and characterization of human intestinal bacteria with the ability to utilize chloramphenicol as the sole source of carbon and energy. FEMS Microbiol. Ecol. 82, 703–712. doi: 10.1111/j.1574-6941.2012.01440.x

PubMed Abstract | CrossRef Full Text | Google Scholar

Yao, J., and Moellering, R. (2007). “Antibacterial agents,” in Manual of Clinical Microbiology, eds P. Murray, E. Baron, J. Jorgensen, M. Landry, and M. Pfaller (Washington, DC: American Society for Microbiology Press), 1077–1113.

Google Scholar

Keywords: antibiotic resistance, antibiotic subsistence, antibiotic subsistence phenotype, aminoglycosides, single carbon source

Citation: Bello Gonzalez TdJ, Zuidema T, Bor G, Smidt H and van Passel MWJ (2016) Study of the Aminoglycoside Subsistence Phenotype of Bacteria Residing in the Gut of Humans and Zoo Animals. Front. Microbiol. 6:1550. doi: 10.3389/fmicb.2015.01550

Received: 25 September 2015; Accepted: 21 December 2015;
Published: 11 January 2016.

Edited by:

Tzi Bun Ng, The Chinese University of Hong Kong, China

Reviewed by:

Eddie Cytryn, Agricultural Research Organization, Volcani Center, Israel
Daniela Ceccarelli, Central Veterinary Institute – Wageningen University and Research Centre, Netherlands

Copyright © 2016 Bello Gonzalez, Zuidema, Bor, Smidt and van Passel. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.

*Correspondence: Teresita de J. Bello González, teresita.bellogonzalez@wur.nl

Disclaimer: All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article or claim that may be made by its manufacturer is not guaranteed or endorsed by the publisher.