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Open Access Highly Accessed Research article

Bacterial diversity in faeces from polar bear (Ursus maritimus) in Arctic Svalbard

Trine Glad12*, Pål Bernhardsen12, Kaare M Nielsen1, Lorenzo Brusetti3, Magnus Andersen4, Jon Aars4 and Monica A Sundset2

Author Affiliations

1 Department of Pharmacy, University of Tromsø, 9037 Tromsø, Norway

2 Department of Arctic Biology and Institute of Medical Biology, University of Tromsø, 9037 Tromsø, Norway

3 Faculty of Science and Technology, Free University of Bozen/Bolzano, Bolzano, Italy

4 Norwegian Polar Institute, 9296 Tromsø, Norway

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BMC Microbiology 2010, 10:10  doi:10.1186/1471-2180-10-10

The electronic version of this article is the complete one and can be found online at: http://www.biomedcentral.com/1471-2180/10/10


Received:23 January 2009
Accepted:14 January 2010
Published:14 January 2010

© 2010 Glad et al; licensee BioMed Central Ltd.

This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract

Background

Polar bears (Ursus maritimus) are major predators in the Arctic marine ecosystem, feeding mainly on seals, and living closely associated with sea ice. Little is known of their gut microbial ecology and the main purpose of this study was to investigate the microbial diversity in faeces of polar bears in Svalbard, Norway (74-81°N, 10-33°E). In addition the level of blaTEM alleles, encoding ampicillin resistance (ampr) were determined. In total, ten samples were collected from ten individual bears, rectum swabs from five individuals in 2004 and faeces samples from five individuals in 2006.

Results

A 16S rRNA gene clone library was constructed, and all sequences obtained from 161 clones showed affiliation with the phylum Firmicutes, with 160 sequences identified as Clostridiales and one sequence identified as unclassified Firmicutes. The majority of the sequences (70%) were affiliated with the genus Clostridium. Aerobic heterotrophic cell counts on chocolate agar ranged between 5.0 × 104 to 1.6 × 106 colony forming units (cfu)/ml for the rectum swabs and 4.0 × 103 to 1.0 × 105 cfu/g for the faeces samples. The proportion of ampr bacteria ranged from 0% to 44%. All of 144 randomly selected ampr isolates tested positive for enzymatic β-lactamase activity. Three % of the ampr isolates from the rectal samples yielded positive results when screened for the presence of blaTEM genes by PCR. BlaTEM alleles were also detected by PCR in two out of three total faecal DNA samples from polar bears.

Conclusion

The bacterial diversity in faeces from polar bears in their natural environment in Svalbard is low compared to other animal species, with all obtained clones affiliating to Firmicutes. Furthermore, only low levels of blaTEM alleles were detected in contrast to their increasing prevalence in some clinical and commensal bacterial populations.

Background

The gastrointestinal microbiota of animals play an important role in the maintenance of health and modulation of disease. Previously, ecosystems have been characterized using microbiological methods based on culturing and phenotypic analysis of the isolates. Since the growth requirements of many bacteria are unknown, most of the gastrointestinal bacteria remain uncultivated. Molecular studies, avoiding the cultivation bias, yield more detailed insight into the diversity and characteristics of the intestinal ecosystems. Most cultivation independent studies have been conducted on the human gastrointestinal tract, but also animals including pigs, rats, chicken, termites, zebras, and ruminants such as reindeer, sheep, cows, and gazelles have been investigated [1-9]. As is the case with the intestinal ecosystems of many of the carnivore animals, the microbial ecology of the gastrointestinal tract of the polar bear is unknown and we know little about the microbial diversity and dominant species in these animals. The Barents Sea subpopulation of polar bears is located in an area which is sparsely populated by humans and thereby has little contact with human activities [10]. This enables us to study an ecosystem with little human impact.

Antibiotic resistant bacteria are known to originate in populations located in environments that seem not to have been exposed to the selective pressure of pharmaceutically produced antibiotics [11]. The β-lactam antibiotics are of the most widely used agents in clinical and veterinary practice, and resistance to these agents are commonly observed in clinical settings [12]. Some of the most common resistance genes are bla genes which encode β-lactamases that give high level resistance to β-lactam antibiotics, and within this group, the blaTEM genes are very important [13,14]. The blaTEM alleles encode resistance to ampicillin and other β-lactam antibiotics. Even though widespread in clinical settings, only few studies have determined the distribution of blaTEM genes in non-clinical environments, included the gastrointestinal tract of free ranging Arctic wild mammals [15-19]. In this study, we have examined the role of polar bear gut microbiota as a potential natural reservoir of the clinically important blaTEM genes.

Polar bears are major predators in the Arctic marine ecosystem. They are closely associated with sea ice, which they use as substrate for both hunting and movement [20]. The world population of polar bears is currently believed to be about 20,000-25,000 animals that can be divided into 19 subpopulations throughout the circumpolar Arctic [10]. The Barents Sea subpopulation is one of these, and inhabits the geographic regions of Svalbard, the Barents Sea and Franz Josef Land. The size of this subpopulation is estimated to be approximately 2650 individuals [21]. The polar bear has a monogastric digestive system with a simple and relatively short intestine typical of a carnivorous animal, and with the caecum completely lacking [22]. Polar bears are mostly carnivorous and feed mainly on seals, although white whales, narwhals, birds, bird eggs and carrion can be important food items during times of the year when seals are less available [23-30]. In Svalbard, polar bear predation on reindeer on land has also been observed [23].

To improve our understanding of the intestinal ecosystem of the polar bear we have studied the bacterial diversity and the prevalence of blaTEM alleles in faeces of polar bears in Svalbard, Norway (Fig. 1). We here present the results of the molecular characterization of the gastrointestinal microbiota of polar bears sampled through 16S rRNA gene cloning and sequencing.

thumbnailFigure 1. Map of Svalbard, Norway. The black circles indicate where the polar bears were captured.

Results

Bacterial diversity

Sequences were obtained from 161 clones and none of the sequences were identified as possible chimeras. All sequences were affiliated with the phylum Firmicutes, with 99% of the sequences belonging to the order Clostridiales (Table 1, Fig. 2). The majority of the sequences (70%) were affiliated to the genus Clostridium. Based on 97% sequence similarity, seventeen phylotypes were identified (Table 2) within the clone library, with the Chao1 index estimating the population richness to be twenty phylotypes. The Shannon-Weaver index, a measure of diversity, was 1.9, and the coverage was 97%. The most abundant phylotype contained 42% of the sequences, and the nearest relative (99.9%) was Clostridium perfringens. Four phylotypes (6% of the sequences) were novel, showing < 97% similarity to sequences representing the phylotypes nearest cultivated relative. Phylotype PBM_a8 contained five sequences and the nearest cultivated relative (96.6%) was Clostridium bartlettii. The nearest cultivated relative (95.3%) to phylotype PBF_b32 which contained two sequences was Ruminococcus hansenii. The other two phylotypes (PBF_b35 and PBM_a2) contained only one sequence each and the nearest relative belonged to the phylum Firmicutes (95.1%) and to unclassified bacteria (96.6%), respectively.

thumbnailFigure 2. Phylogenetic tree of the 17 phylotypes recovered from the clone library obtained from faeces from three polar bears in Svalbard, Norway (bold). Evolutionary distance was calculated using the Kimura-2 parameter model for nucleotide change and the tree was constructed using the neighbor-joining method. Statistical significance of branching was verified by bootstrapping. The scale bar represents a 5% estimated sequence divergence, and reference sequences were obtained from the GenBank Database.

Table 1. Distribution and abundance of 16S rRNA gene sequences in the clone library

Table 2. Polar bear 16S rRNA gene clones representing 17 valid phylotypes

Aerobic heterotrophic cell counts and β-lactamase activity

The aerobic heterotrophic cell counts ranged from 5.0 × 104 to 1.6 × 106 cfu/ml for the rectum swabs, and from 4.0 × 103 to 1.0 × 105 cfu/g for the faeces samples (Table 3 and 4). The coliform counts for the faeces samples ranged from 3.2 × 103 to 8.0 × 104 cfu/g. There was no growth of ampicillin resistant bacteria in the faeces samples. For the rectal swabs, the proportion of ampr bacteria ranged between 3% and 44% (Table 3). A total of 144 randomly selected ampr isolates cultivated from rectal swab samples were tested for β-lactamase activity by the nitrocefin test and all isolates showed β-lactamase activity.

Table 3. Aerobic heterotrophic, coliform, and ampicillin resistant cells counts (cfu/ml) in rectum swabs from polar bears in Svalbard

Table 4. Aerobic heterotrophic, coliform, and ampicillin resistant cell counts (cfu/g) in faeces from polar bears in Svalbard a

Detection of blaTEM genes in ampr isolates

The absence of PCR inhibitory substances in the DNA extracted from ampr isolates was tested by running 16S rRNA gene PCR on extracted DNA from each of 100 single isolates. As much as 98 of the amplifications were positive, indicating that bacterial DNA is amplifiable in 98% of the samples. Subsequently, 144 ampr isolates from the rectal samples were screened for the presence of blaTEM genes with primers designed for the TEM-1 allele and derivatives [15], and 4 of the ampr isolates were positive. For all four positive isolates, sequencing of the flanking regions demonstrated the presence of blaTEM inserted in a Tn3 backbone. The four isolates were identified as E. coli by ID32 E (bioMérieux, Marcy l'Etoile, France) and 16S rRNA gene sequencing.

Detection of blaTEM genes in total genomic DNA extracts

Total genomic DNA was extracted from the rectal swab from polar bear no. 4 (Table 5). The sample was negative for blaTEM PCR and positive when screened for 16S rRNA genes, confirming the general suitability of DNA for PCR. Total genomic DNA was also extracted from faeces from three of the polar bears (no. 6-8, Table 5) sampled in 2006, and one of the three faecal samples was negative, while one was positive, and one out of five DNA extractions from the third sample (bear no. 7) was positive (Fig. 3).

Table 5. Year of sampling, sex, age, condition, and samples obtained for the polar bear used in this study

thumbnailFigure 3. PCR with blaTEM specific primers on total DNA extracted from polar bear faeces. Lane 1 and 14, 1 kb Plus DNA ladder (Invitrogen, California, USA); lane 2, bear no. 6; lanes 3-7, five parallel DNA extraction from faeces from bear no 7; lane 8, bear no. 8; lane 9-13 positive controls (TEM-3, TEM-6, TEM-9, TEM-10, SHV-2).

Discussion

The Barents Sea subpopulation of polar bears has little contact with human activities [10], and the samples investigated in this study were collected from the subpopulation in their natural environment in Svalbard, Norway. Fresh faeces were collected from live, sedated bears and immediately frozen. There is a potential loss of bacteria when samples are stored before cultivation of bacteria. The pure faeces samples were stored at -70°C and the rectum swabs were stored in 20% glycerol at the same temperature. Achá et al [31] found that there was not a great loss of bacterial number and species when pure faeces samples were stored at -70°C compared to faeces samples mixed with a cryoprotectant such as glycerol, as long as the samples were not repeatedly thawed and analysed in shorter intervals. The samples processed in this study were not repeatedly thawed and analysed and we expect little loss of bacterial number and species compared to if the samples were mixed with glycerol before storing.

The 16S rRNA gene libraries were made from DNA extracted from faeces, and the samples were pooled after PCR to ensure that bacterial DNA from all animals was equally represented. The number of PCR cycles were reduced to a minimum, as the frequency of formation of chimeric molecules increases by the number of PCR cycles [32]. We used 30 cycles for the amplification of the 16S rRNA genes, and did not detect possible chimeras using the Chimera Detection Program. Seventeen different phylotypes were identified among the 161 sequences analysed (Table 2). The coverage of the combined libraries was 97%, which indicate that we have detected the majority of the present microbioma in the faeces. In a study based on faecal microbial communities of 106 individual mammals representing 60 species from 13 taxonomic orders, including captive bears and pandas, Ley et al [33] observed that host diet and phylogeny both influence bacterial diversity, which increases from carnivorous to omnivorous to herbivorous animals. In captive carnivores between 19 and 75 OTUs were observed using the 96% similarity criteria, while in herbivore animals up to 223 OTUs were detected. Within members of the Ursidae family including carnivorous, herbivorous and omnivorous bears, the number of OTUs ranged from 14 to 34 which is consistent with our findings.

Only four of the seventeen phylotypes were < 97% related to any known cultivated species (Table 2). This is in contrast to observations made in other studies that the microbial diversity reflected by cultivation represents only a minor fraction of the microbial diversity. In a study of the microbial diversity in reindeer, 92.5% of the bacterial diversity represented novel taxonomic groupings [7]. A study on the microbial community composition of the intestinal tract of chickens, 85% of the phylotypes did not have sequence similarity to any cultured species [1], and in the pig gastrointestinal microbiota, 83% of the identified phylotypes were not likely represented by a known bacterial species [4]. Analysis of the polar bear faeces in this study showed a homogenous microbial flora dominated by Clostridia class. These bacteria are well characterized as they are dominant in the human gut and thereby in the interest of many scientists [34].

All 161 sequences obtained from polar bears were affiliated with the phylum Firmicutes (Table 1, Fig. 2). All except one sequence affiliated with the order Clostridiales, and 93% to the family Clostridiaceae. The low level of diversity observed in the polar bear clone library is in contrast to the diversity observed in colon content from another Arctic carnivorous animal belonging to the same order as polar bears, the hooded seal (Cystophora cristata) [35]. Sequences that affiliated with the phyla Bacteroides, Firmicutes, Fusobacteria, and Proteobacteria were identified in the colon content from the seals. The dominant phylum was the Bacteroides to which 68% of the sequences were affiliated, while 21% were affiliated to the Firmicutes [35]. The same molecular methods were used to analyse both the polar bear and seal samples, indicating that the methods are not selective towards Firmicutes. Jores et al [36] found Clostridium in 44% of the samples when cultivating faeces from polar bears in Svalbard. In faeces from a herbivorous mammal, the wild gorilla, 71% of the phylogenetic lineage was Firmicutes [37]. Ley et al [33] observed that the microbial faecal bacterial communities from bears on different diets cluster together, independent of the diet. However, these observations were made in animals kept in zoo's and might not reflect the situation in the wild. Eight of the 673 sequences (GenBank/EMBL/DDBJ database, NCBI) from polar bear faeces collected in zoo's [33] were compared to the sequences obtained in this study (Fig. 2). The eight zoo polar bear sequences included in Fig. 2 represent eight out of 100 phylotypes (analysed by FastgroupII) and contain 59% of the 673 zoo polar bear sequences. Only two of the sequences, representing 10% of all the sequences, cluster together with sequences from our study, indicating a difference between the microbioma in faeces of wild and captive polar bears.

We investigated the prevalence of blaTEM alleles in faeces from polar bears with little human impact in Svalbard, Norway. We have earlier investigated the prevalence of blaTEM alleles in Arctic soils and sediments, and in colon content of Arctic seals and found low prevalence of the alleles [15,35]. This current cultivation study of faeces from polar bears did not give any growth on plates with ampicillin (Table 4). The blaTEM alleles are likely to be found in coliform bacteria, but the selective growth on MacConkey agar with ampicillin yielded < 0.3% ampr cfu (Table 4). However, from 3% to 44% of the isolates from the rectal swabs were phenotypically ampr. A random selection of ampr isolates all showed β-lactamase activity, but when tested by blaTEM PCR, only 4 out of 144 isolates were positive. This indicates a low level of blaTEM alleles. The four isolates were all identified as E. coli, and the blaTEM alleles were inserted in a Tn3 transposon which is found in a wide variety of bacteria. The presence of blaTEM alleles has previously been reported in wild animals in Portugal, where they detected the alleles in E. coli isolated from faeces from deer, fox, owl, and birds of prey [38]. Others have identified blaTEM in faecal E. coli isolates from pigs, dogs, and cats [17,39]. The blaTEM PCR on total DNA extracted was negative for the two rectal swabs, and two of the three faecal samples were blaTEM PCR positive (Fig. 3). Previous studies on Arctic soil samples suggest that the detection limit for total DNA extracted was < 21 blaTEM alleles (pUC18) per PCR sample [15]. The diversity analysis of polar bear faeces showed a dominance of clostridiales in which there has been no reports of β-lactamase production. This is consistent with the low levels of blaTEM alleles detected in the samples.

Conclusions

This study showed that the bacterial diversity in faeces from polar bears in their natural environment in the pristine Svalbard area were low, all obtained clones affiliated to Firmicutes. As with any PCR-based method, 16S rRNA gene clone libraries are biased [40] and the gastrointestinal microbiota of more polar bears should be studied to give a more complete picture of the microbial diversity. Furthermore, only low levels of blaTEM alleles were detected in contrast to their increasing prevalence in some clinical and commensal bacterial populations.

Methods

Sampling

Ten samples from ten polar bears were collected on two occasions. Faeces were sampled from five individuals March 30th-April 12th 2004 and from five individuals March 30th-April 9th 2006 (Table 5). Sampling occurred on both occasions at the coast or the surrounding sea ice at Spitsbergen and Nordaustlandet in Svalbard, Norway (Fig. 1). Bears were caught by remote injection of a dart (Palmer Cap-Chur Equipment) containing the drug Zoletil® (Virbac, Carros Cedex, France) fired from a helicopter [41]. Animal handling methods were approved by the National Animal Research Authority (Norwegian Animal Health Authority, P.O. Box 8147 Dep., N-0033 Oslo, Norway). The sex, reproductive status, and a series of standardized morphometric measurements were collected from each bear (Table 5). In 2004, the samples were collected by swabbing rectum and the samples were kept frozen in LB-broth (Luria Broth, Fluka BioChemica) with 20% glycerol. In 2006, faeces was collected with a sterile glove and kept in sterilized plastic bags. The amount of sample ranged from 0.2 g to 2 g. All samples were kept in containers at -20°C during transport to the laboratory, where they were stored at -70°C until analysed.

16S rRNA Clone Library

The amount of sampled material was limited due to little faeces in the rectum of the polar bears, and only three faeces samples gave sufficient DNA yield to make 16S rRNA gene clone libraries. A 16S rRNA gene clone library was made with DNA extracted from faeces from bear no. 6, 7 and 8. Total genomic DNA was extracted using the QIAmp DNA stool kit (Qiagen, Solna, Sweden) according to the protocol provided by the producer, and DNA quantified using a NanoDrop® ND-1000 Spectrophotometer (260 nm) (Thermo Fisher Scientific, Waltham, USA). Two parallel 16S rRNA gene PCR amplifications on DNA from each of the three animals were performed, using primers 16S-27F and 16S-1494R (Table 6), in a reaction mixture containing 1× HotStartTaq DNA master mix (Qiagen), 0.3 μM of each primer, and 20 ng of extracted DNA solution in a final volume of 50 μl. PCR amplification was initiated by denaturation at 95°C for 15 min and then 30 cycles of 94°C for 30 s, 50°C for 30 s, and 72°C for 2 min, with a final extension at 72°C for 10 min. The 16S rRNA gene amplicons were pooled and cloned using the TOPO TA Cloning® Kit for Sequencing (Invitrogen, California, USA), and transformed by heat-shock into One Shot® Competent Escherichia coli cells (Invitrogen). Positive clones were randomly selected and recombinant plasmids extracted using QIA prep spin miniprep kit (Qiagen). Extracted DNA was quantified using a NanoDrop ND-1000 Spectrophotometer (260 nm), and sequenced on a 3130 Genetic analyzer (Applied Biosystems, Foster City, USA) using the ABI BigDye Terminator chemistry. The sequencing primers (Invitrogen) used were M13 forward primer, M13 reverse primer, and the universal bacterial 16S rRNA primer Bact338, corresponding to nucleotide position 338-355 of E. coli (Table 6).

Table 6. Primers used for PCR and sequencing

Sequence analysis

The 16S rRNA gene sequences were assembled using the program Lasergene™ Seqman v. 7.1.0. (DNASTAR Inc.). Putative chimeric sequences were evaluated using the Chimera Detection Program which is part of the SimRank 2.7 package available through the Ribosomal Database Project (RDP) [42]. Sequences generated were first compared to sequences obtained from the RDP II (Classifier: Naive Bayesian rRNA Classifier Version 1.0, November 2003; The nomenclature taxonomy of Garrity and Lilburn, release 6.0) and then compared to GenBank sequences using BLAST (Basic Local Alignment Search Tool) [43]. The 16S rRNA gene sequences were automatically aligned by CLUSTAL-W in the software package BioEdit (v. 5.0.9) to give a uniform length. Phylogenetic analysis was performed using the neighbour-joining method with the Kimura2-parameter correction model in the software MEGA (v. 4.0) [44]. Statistical significance of branching was verified by bootstrapping [45] involving construction and analysis of 1000 trees from the data set in the software MEGA. Sequences were assigned to operational taxonomic units (OTUs) based on a 97% sequence similarity criterion [46]. Standard diversity and richness indices, including the Shannon-Weaver index [47] (a nonparametric diversity index combining estimates of richness, i.e. total numbers of ribotypes) and evenness (relative abundance of each OTU, indicating diversity) and the Chao1 index [48] (a nonparametric estimator of the minimum OTU richness) were calculated using the FastGroupII web-based bioinformatics platform for analyses of 16S rRNA gene based libraries [49]. The coverage of the clone library was calculated with the formula [1-(n/N)] [50] where n is the number of phylotypes (OTUs) represented by one clone and N is the total number of clones. The sequence data for the clones have been submitted to the GenBank/EMBL/DDBJ database (NCBI) with accession numbers FJ375772 to FJ375932.

Determination of cultivable, coliform, and ampicillin resistant counts

Faeces samples were thawed and suspended in saline immediately before cultivation of aerobic bacteria. For both rectal swabs and faeces samples, colony forming units were determined for aerobic heterotrophic cells on chocolate medium (agar, horse blood, glucose, Vitox SR 090A, Vitox, SR 090H (Oxoid); University hospital, Tromsø, Norway) and for ampr aerobic heterotrophic cells on chocolate medium supplemented with 50 mg/l of ampicillin (Sigma). Coliform cells were determined for faeces samples on MacConkey medium (Fluka BioChemika), and for ampr coliform cells on MacConkey medium supplemented with 50 mg/l of ampicillin. All plates were enumerated after 48 h of incubation at 37°C. Means and standard deviations (SD) for the cfu's were calculated on the basis of nine replicates for each of the bear samples analysed.

Identification of β-lactamase activity with the nitrocefin-test

Extracellular β-lactamase activity was determined by the nitrocefin test method. A solution (0.5 g/l) of nitrocefin (chromogenic β-lactamase substrate, Calbiochem, San Diego, USA) was prepared according to the manufacturer's instruction. Ten μl of the solution was added to single colonies and a colour change from yellow to pink within 30 minutes after application indicated β-lactamase activity.

DNA extraction and test PCR amplification of 16S rRNA genes

DNA was extracted from randomly chosen colonies by a boiling lysis method [51]. The general suitability of DNA for PCR was confirmed with amplification of the 16S rRNA gene, using the primers 16S-27F and 16S-1494R (Table 6). The amplification was performed as explained above, with the following conditions; denaturation at 95°C for 15 min and then 5 cycles of 94°C for 4 min, 50°C for 45 s, and 72°C for 1 min, and then 30 cycles of 92°C for 45 s, 55°C for 45 s, and 72°C for 1 min, with a final extension at 72°C for 10 min.

PCR amplification of potential blaTEM genes in ampr isolates

The amplification of blaTEM alleles in individual bacterial isolates was performed in a reaction mixture containing 1× HotStartTaq DNA master mix (Qiagen), 0.2 μM of each primer, and 2 μl of the crude DNA solution in a final volume of 30 μl. Reactions were denatured at 95°C for 15 min and then subjected to 30 cycles of 94°C for 45 s, 61°C for 45 s, and 72°C for 1 min, with a final extension at 72°C for 10 min. For all blaTEM PCR analyses, the primers BlaF and BlaR (Table 6) were used to amplify a product of 828 bp (TEM-1 allele of E. coli) [15]. The following controls were used: five strains of E. coli carrying the bla alleles TEM-1, TEM-3, TEM-6, TEM-9, and TEM-10 as positive controls, and one strain carrying the SHV-2 allele as negative control. The specificity of the primers were confirmed by 'in silico' amplification and by aligning the primer binding region of approximately 100 sequence polymorphic blaTEM alleles [15].

Sequencing of 16S rRNA, blaTEM, and blaTEM flanking regions

The identity of putative ampr positive isolates was determined by sequencing, with primers 16S-27F, 16S-1494R, and Bact 338 (Table 6), on a 3130 Genetic analyzer using the ABI BigDye Terminator chemistry. To confirm the presence of and determine the location of blaTEM in the DNA extract from ampr isolates, sequencing of the immediate flanking regions of the blaTEM gene was performed using the sequencing primers TemI3, TemI5a or TemI5b (Table 6) as described in [15].

Authors' contributions

TG has participated in its design and coordination, participated in the analysis, and drafting and revising the manuscript. MAS conceived part of the study, participated in its design and analysis, and revising the manuscript. KN conceived part of the study, participated in its design and revision of the manuscript. PB performed molecular genetic analyses/cultivations and drafting of the manuscript. LB has participated in the analysis and interpretation of data, and revising the manuscript. JA has been involved in acquisition of data and revising the manuscript. MA has been involved in acquisition of data and revising the manuscript. All authors read and approved the final manuscript.

Acknowledgements

This study was funded by the Norwegian Research Council and Roald Amundsen Centre for Arctic Research (University of Tromsø, Norway). The sequencing laboratory at the Faculty of Medicine, University of Tromsø is acknowledged for their sequencing of the bacterial 16S rRNA genes. Control strains used for the blaTEM PCR analyses and the identification of E. coli by ID32 E were kindly provided by Prof. Arnfinn Sundsfjord, University Hospital of North Norway, Tromsø, Norway.

References

  1. Bjerrum L, Engberg RM, Leser TD, Jensen BB, Finster K, Pedersen K: Microbial community composition of the ileum and cecum of broiler chickens as revealed by molecular and culture-based techniques.

    Poult Sci 2006, 85(7):1151-1164. PubMed Abstract | Publisher Full Text OpenURL

  2. Brooks SPJ, McAllister M, Sandoz M, Kalmokoff ML: Culture-independent phylogenetic analysis of the faecal flora of the rat.

    Can J Microbiol 2003, 49:589-601. PubMed Abstract | Publisher Full Text OpenURL

  3. Koike S, Yoshitani S, Kobayashi Y, Tanaka K: Phylogenetic analysis of fiber-associated rumen bacterial community and PCR detection of uncultured bacteria.

    FEMS Microbiol Lett 2003, 229(1):23-30. PubMed Abstract | Publisher Full Text OpenURL

  4. Leser TD, Amenuvor JZ, Jensen TK, Lindecrona RH, Boye M, Moller K: Culture-independent analysis of gut bacteria: the pig gastrointestinal tract microbiota revisited.

    Appl Environ Microbiol 2002, 68(2):673-690. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  5. Nelson KE, Zinder SH, Hance I, Burr P, Odongo D, Wasawo D, Odenyo A, Bishop R: Phylogenetic analysis of the microbial populations in the wild herbivore gastrointestinal tract: insights into an unexplored niche.

    Environ Microbiol 2003, 5(11):1212-1220. PubMed Abstract | Publisher Full Text OpenURL

  6. Ohkuma M, Kudo T: Phylogenetic diversity of the intestinal bacterial community in the termite Reticulitermes speratus.

    Appl Environ Microbiol 1996, 62(2):461-468. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  7. Sundset MA, Præsteng K, Cann I, Mathiesen SD, Mackie RI: Novel rumen bacterial diversity in two geographically separated sub-species of reindeer.

    Microb Ecol 2007, 54(3):424-438. PubMed Abstract | Publisher Full Text OpenURL

  8. Sundset MA, Edwards J, Cheng Y, Senosiain R, Fraile M, Northwood KS, Præsteng K, Glad T, Mathiesen S, Wright A-DG: Molecular diversity of the rumen microbiome of Norwegian reindeer on natural summer pasture.

    Microb Ecol 2009, 57:335-348. PubMed Abstract | Publisher Full Text OpenURL

  9. Tajima K, Aminov RI, Nagamine T, Ogata K, Nakamura M, Matsui H, Benno Y: Rumen bacterial diversity as determined by sequence analysis of 16S rDNA libraries.

    FEMS Microbiol Ecol 1999, 29(2):159-169. Publisher Full Text OpenURL

  10. Aars J, Lunn NJ, Derocher AE: Polar bears. In Proceedings of the 14th working meeting of the IUCN/SSC Polar Bear Specialist Group, 20-24 June 2005, Seattle, Washington, USA. IUCN, Gland, Switzerland and Cambridge, UK; 2006. OpenURL

  11. Seveno N, Smalla K, van Elsas JD, Collard J-M, Karagouni A, Kallifidas D, Wellington E: Occurrence and reservoirs of antibiotic resistance genes in the environment.

    RevMed Microbiol 2002, 13(1):15-27. OpenURL

  12. Singh G: β-Lactams in the new millennium. Part-I: monobactams and carbapenems.

    Mini Rev Med Chem 2004, 4:69-92. PubMed Abstract | Publisher Full Text OpenURL

  13. Bush K: Characterization of beta-lactamases.

    Antimicrob Agents Chemother 1989, 33(3):259-263. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  14. Livermore DM: beta-Lactamases in laboratory and clinical resistance.

    Clin Microbiol Rev 1995, 8(4):557-584. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  15. Brusetti L, Glad T, Borin S, Myren P, Rizzi A, Johnsen PJ, Carter P, Daffonchio D, Nielsen KM: Low prevalence of blaTEM genes in Arctic environments and agricultural soil and rhizosphere.

    Microb Ecol Health D 2008, 20(1):27-36. Publisher Full Text OpenURL

  16. Demaneche S, Sanguin H, Pote J, Navarro E, Bernillon D, Mavingui P, Wildi W, Vogel TM, Simonet P: Antibiotic-resistant soil bacteria in transgenic plant fields.

    Proc Natl Acad Sci 2008, 105(10):3957-3962. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  17. Carattoli A, Lovari S, Franco A, Cordaro G, Di Matteo P, Battisti A: Extended-spectrum beta-lactamases in Escherichia coli isolated from dogs and cats in Rome, Italy, from 2001 to 2003.

    Antimicrob Agents Chemother 2005, 49(2):833-835. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  18. Osterblad M, Norrdahl K, Korpimaki E, Huovinen P: Antibiotic resistance: How wild are wild mammals?

    Nature 2001, 409(6816):37-38. PubMed Abstract | Publisher Full Text OpenURL

  19. Gilliver MA, Bennett M, Begon M, Hazel SM, Hart CA: Enterobacteria: Antibiotic resistance found in wild rodents.

    Nature 1999, 401(6750):233-234. PubMed Abstract | Publisher Full Text OpenURL

  20. Mauritzen M: Patterns and processes in female polar bear space use. PhD thesis. University of Oslo, Norway; 2002. OpenURL

  21. Aars J, Marques T, Buckland S, Andersen M, Belikov S, Boltunov A, Wiig Ø: Estimating the Barents Sea polar bear subpopulation size.

    Mar Mamm Sci 2009, 25(1):35-52. Publisher Full Text OpenURL

  22. Larsen AK, Marhaug T, Sundset MA, Storeheier PV, Mathiesen SD: Digestive adaptations in the polar bear - an anatomical study of the gastrointestinal system of the polar bear related to its ability to adapt to future climatic changes in the Arctic.

    Polar Res Tromsø 2004, 10-11. OpenURL

  23. Derocher AE, Wiig Ø, Bangjord G: Predation of Svalbard reindeer by polar bears.

    Polar Biol 2000, 23(10):675-678. Publisher Full Text OpenURL

  24. Donaldson G, Chapdelaine G, Andrews J: Predation of thick-billed murres, Uria lomvia, at 2 breeding colonies by polar bears, Ursus maritimus, and whalruses, Odobenus rosmarus.

    Can Field Nat 1995, 109:112-114. OpenURL

  25. Gjertz I, Lydersen C: Polar bear predation on ringed seals in the fast-ice of Hornsund, Svalbard.

    Polar Res 1986, 4:65-68. Publisher Full Text OpenURL

  26. Lowry L, Burns J, Nelson R: Polar bear, Ursus maritimus, predation on belugas, Delphinapterus leucas, in the Bering and Chukchi seas.

    Can Field Nat 1987, 101:141-146. OpenURL

  27. Rugh D, Shelden K: Polar bears, Ursus maritimus, Feeding on beluga whaled, Delphinapterus leucas.

    Can Field Nat 1993, 107:235-237. OpenURL

  28. Smith T: Polar bear predation of ringed and bearded seals in the land-fast sea ice habitat.

    Can J Zool 1980, 58:2201-2209. Publisher Full Text OpenURL

  29. Smith T, Sjare B: Predation of belugas and narwhals by polar bears in nearshore areas of the Canadian High Arctic.

    Arctic 1990, 43:99-102. OpenURL

  30. Stempniewicz L: The polar bear Ursus maritimus feeding in a seabird colony in Frans Josef Land.

    Polar Res 1993, 12:33-36. Publisher Full Text OpenURL

  31. Achá SJ, Kühn I, Mbazima G, Colque-Navarro P, Möllby R: Changes of viability and composition of the Escherichia coli flora in faecal samples during long time storage.

    J Microbiol Methods 2005, 63(3):229-238. PubMed Abstract | Publisher Full Text OpenURL

  32. Wang GC, Wang Y: Frequency of formation of chimeric molecules as a consequence of PCR coamplification of 16S rRNA genes from mixed bacterial genomes.

    Appl Environ Microbiol 1997, 63(12):4645-4650. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  33. Ley RE, Hamady M, Lozupone C, Turnbaugh PJ, Ramey RR, Bircher JS, Schlegel ML, Tucker TA, Schrenzel MD, Knight R, et al.: Evolution of mammals and their gut microbes.

    Science 2008, 320(5883):1647-1651. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  34. Eckburg PB, Bik EM, Bernstein CN, Purdom E, Dethlefsen L, Sargent M, Gill SR, Nelson KE, Relman DA: Diversity of the human intestinal microbial flora.

    Science 2005, 308(5728):1635-1638. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  35. Glad T, Nielsen KM, Nordgård L, Sundset M: Bacterial diversity and antibiotic resistance in the colon of the hooded seal.

    Reprod Nutr Dev 2007, 46(Suppl 1):S15-S16. OpenURL

  36. Jores J, Derocher AE, Staubach C, Aschfalk A: Occurrence and prevalence of Clostridium perfringens in polar bears from Svalbard, Norway.

    J Wildl Dis 2008, 44(1):155-158. PubMed Abstract | Publisher Full Text OpenURL

  37. Frey JC, Rothman JM, Pell AN, Nizeyi JB, Cranfield MR, Angert ER: Fecal bacterial diversity in a wild gorilla.

    Appl Environ Microbiol 2006, 72(5):3788-3792. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  38. Costa D, Poeta P, Saenz Y, Vinue L, Rojo-Bezares B, Jouini A, Zarazaga M, Rodrigues J, Torres C: Detection of Escherichia coli harbouring extended-spectrum beta-lactamases of the CTX-M, TEM and SHV classes in faecal samples of wild animals in Portugal.

    J Antimicrob Chemother 2006, 58(6):1311-1312. PubMed Abstract | Publisher Full Text OpenURL

  39. Saenz Y, Brinas L, Dominguez E, Ruiz J, Zarazaga M, Vila J, Torres C: Mechanisms of resistance in multiple-antibiotic-resistant Escherichia coli strains of human, animal, and food origins.

    Antimicrob Agents Chemother 2004, 48(10):3996-4001. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  40. v. Wintzingerode F, Göbel UB, Stackebrandt E: Determination of microbial diversity in environmental samples: pitfalls of PCR-based rRNA analysis.

    FEMS Microbiol Rev 1997, 21(3):213-229. PubMed Abstract | Publisher Full Text OpenURL

  41. Strirling I, Spencer C, Andriashek D: Immobilization of polar bears (Ursus maritimus) with TelazolR in the Canadian Arctic.

    J Wildl Dis 1989, 25:159-168. PubMed Abstract | Publisher Full Text OpenURL

  42. Cole JR, Chai B, Marsh TL, Farris RJ, Wang Q, Kulam SA, Chandra S, McGarrell DM, Schmidt TM, Garrity GM, et al.: The Ribosomal Database Project (RDP-II): previewing a new autoaligner that allows regular updates and the new prokaryotic taxonomy.

    Nucl Acids Res 2003, 31(1):442-443. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  43. Altschul SF, Madden TL, Schaffer AA, Zhang J, Zhang Z, Miller W, Lipman DJ: Gapped BLAST and PSI-BLAST: a new generation of protein database search programs.

    Nucl Acids Res 1997, 25(17):3389-3402. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL

  44. Tamura K, Dudley J, Nei M, Kumar S: MEGA4: Molecular evolutionary genetics analysis (MEGA) software version 4.0.

    Mol Biol Evol 2007, 24(8):1596-1599. PubMed Abstract | Publisher Full Text OpenURL

  45. Felsenstein J: Confidence limits on phylogenies: An approach using the bootstrap.

    Evolution 1985, 39(4):783-791. Publisher Full Text OpenURL

  46. Stackebrandt E, Goebel BM: Taxonomic note: a place for DNA-DNA reassociation and 16S rRNA sequence analysis in the present species definition in bacteriology.

    Int J Syst Bacteriol 1994, 44(4):846-849. OpenURL

  47. Shannon C, Weaver W: The mathematical theory of communication. University of Illinois Press, Urbana, USA; 1949.

  48. Chao A: Non-parametric estimation of the number of classes in a population.

    Scand J Stat 1984, 11:783-791. OpenURL

  49. Yu Y, Breitbart M, McNairnie P, Rohwer F: FastGroupII: A web-based bioinformatics platform for analyses of large 16S rDNA libraries.

    BMC Bioinformatics 2006, 7(1):57-65. PubMed Abstract | BioMed Central Full Text | PubMed Central Full Text OpenURL

  50. Good IJ: The population frequencies of species and the estimation of population parameters.

    Biometrika Trust 1953, 40(3/4):237-264. Publisher Full Text OpenURL

  51. Glad T, Klingenberg C, Flaegstad T, Ericson JU, Olsvik Ø: Rapid detection of the methicillin-resistance gene, mecA, in coagulase-negative staphylococci.

    Scand J Infect Dis 2001, 33(7):502-506. PubMed Abstract | Publisher Full Text OpenURL

  52. Ehlers B, Strauch E, Goltz M, Kubsch D, Wagner H, Maidhof H, Bendiek J, Appel B, Buhk HJ: Nachweis gentechnischer Veränderungen in Mais mittels PCR.

    Bundesgesundheitsbl 1997, 40(4):118-121. Publisher Full Text OpenURL

  53. Lane DJ: 16S/23S rRNAsequencing. Nucleic acid techniques in bacterial systematics. In Modern microbiological methods. Edited by Stackebrandt E, Goodfellow M. Chichester, UK: J Wiley & Sons; 1991:133. OpenURL

  54. Amann RI, Ludwig W, Schleifer KH: Phylogenetic identification and in situ detection of individual microbial cells without cultivation.

    Microbiol Rev 1995, 59(1):143-169. PubMed Abstract | Publisher Full Text | PubMed Central Full Text OpenURL