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Benzylpenicillin-producing Trichophyton erinacei and methicillin resistant Staphylococcus aureus carrying the mecC gene on European hedgehogs – A pilot-study

Abstract

Background

A high carriage rate of methicillin-resistant Staphylococcus aureus with the mecC gene (mecC-MRSA) has been described among Wild European hedgehogs (Europeaus erineaus). Due to this frequent occurrence, it has been suggested that hedgehogs could be a natural reservoir for mecC-MRSA. However, the reason why hedgehogs carry mecC-MRSA remains unknown, but it has been hypothesized that mecC-MRSA could have evolved on the skin of hedgehogs due to the co-occurrence with antibiotic producing dermatophytes. The aim of this pilot-study was therefore to investigate if hedgehogs in Sweden carry Trichophyton spp. and to provide evidence that these dermatophytes are able to produce penicillin or similar substances. In addition, the study aimed to identify if dermatophytes co-occurred with mecC-MRSA.

Methods

Samples were collected from hedgehogs (Europeaus erineaus) that were euthanized or died of natural causes. All samples were screened for dermatophytes and mecC-MRSA using selective cultivation methods. Suspected isolates were characterized using PCR-based methods, genome sequencing and bioinformatic analyses. Identification of penicillin was performed by ultra-high-performance liquid chromatography-tandem mass spectrometry.

Results

In total 23 hedgehogs were investigated, and it was shown that two carried Trichophyton erinacei producing benzyl-penicillin, and that these hedgehogs also carried mecC-MRSA. The study also showed that 60% of the hedgehogs carried mecC-MRSA.

Conclusion

The pilot-study demonstrated that Trichophyton erinacei, isolated from Swedish hedgehogs, can produce benzylpenicillin and that these benzylpenicillin-producing T. erinacei co-occurred with mecC-MRSA. The study also reconfirmed the high occurrence of mecC-MRSA among hedgehogs.

Peer Review reports

Background

Staphylococcus aureus is a commensal of humans and many animals, but it is also an opportunistic pathogen [1]. However, due to the spread of antibiotic resistant strains the ability to treat S. aureus infections has been undermined, and of particular concern is the emergence of methicillin-resistant S. aureus (MRSA). MRSA has low sensitivity for all clinically used beta-lactam antibiotics, except the fifth generation cephalosporins [2]. When MRSA first emerged in the 1980s it was primarily associated with hospital infections (HA-MRSA), but soon after reports on community associated infections (CA-MRSA) occurred [3]. Today MRSA also occurs in animals and has spread particularly among farm animals, primarily pigs, where occurrence mainly is due to asymptomatic carriage of some specific livestock-adapted clonal linages (LA-MRSA) [4].

All MRSA were originally associated with the mecA gene (mecA-MRSA), which encodes for an altered penicillin-binding protein (PBP), PBP2a [5]. However, in 2011, a mecA homologue, mecALGA251, was identified with about 69% nucleotide identity to mecA that codes for an alternative PBP called PBP2c [6]. The mecALGA251 gene was later renamed mecC (mecC-MRSA) and mecC-MRSA was first described from bulk milk samples in UK and human samples in Denmark, UK, and Ireland [6, 7]. Subsequent studies have described mecC-MRSA from a diverse set of regions and animal species, but almost exclusively from Europe [8,9,10,11,12,13]. Overall, there appears to be a low incidence of mecC-MRSA in most sectors, including in human healthcare settings, but an increasing trend in human clinical cases has been observed in Denmark [14]. At first domestic animals in Europe, primarily dairy cattle, were linked to mecC-MRSA and it was therefore suggested that dairy cattle could be the original reservoir [15, 16]. However, the wide distribution of mecC-MRSA in different wild animal species challenged that narrative and it was therefore suggested that rodents, insectivores, or small carnivores could be the origin of mecC-MRSA [17]. This hypothesis appears too be supported by a Swedish study showing a high occurrence of mecC-MRSA, 64%, in wild European hedgehogs (Europeaus erineaus) in 2017 [8]. A recent nationwide study in Denmark further strengthens that mecC-MRSA is associated with hedgehogs as it showed a carriage rate of 61% [11]. In Sweden, all MRSA are notifiable to the authorities and only 132 instances of MRSA from animals, not counting hedgehogs, have been reported between 2006 and through 2018. For comparison, 3864 MRSA cases were reported from humans in 2018 alone [18]. Cases with mecC-MRSA has remained rare in Sweden both among humans and animals, with only 92 and 14 cases respectively reported since 2011 and up to 2018, when excluding hedgehogs. The first mecC-MRSA in Sweden was isolated already in 2003 from a hedgehog suffering from S. aureus septicemia but it was not described as such until 2012 [19]. After the first report three mecC-MRSA isolates were reported from dairy cows in 2010, and since 2011 it has been reported from cats, dogs, dairy cows, dairy and pet goats, and humans [18, 20].

In the 1960s a study conducted by Smith and Marples [21] reported a high proportion, 86%, of penicillin-resistant S. aureus in wild European hedgehogs (E. erineaus) in New Zealand. This study also noted that 45% of hedgehogs had chronic mycotic infections caused by dermatophytes. Since an earlier study had demonstrated penicillin-like production by dermatophytes [22], Smith and Marples hypothesized that hedgehogs could be a potential natural reservoir of penicillin-resistant S. aureus and that antibiotics produced by their dermatophytes could have selected for this resistance phenotype. Subsequently, they were able to show that Trichophyton spp. dermatophytes from hedgehogs’ skin likely produce a penicillin-like substance [23].

Based on the described high occurrence of mecC-MRSA and Trichophyton spp. on hedgehogs and that the dermatophytes have been suggested to produce penicillin-like substances we aimed to investigate if Swedish hedgehogs carry Trichophyton spp. that produce penicillin or a similar substance, and if Trichophyton spp. co-occurs with MRSA.

Results

Recovery and characterization of dermatophytes

Twenty-three hedgehogs from Gotland County (n = 14), Skåne County (n = 6), and Uppsala County (n = 3) were investigated in the pilot-study and two, both originating from Gotland County, were found to carry dermatophytes. None of the sampled hedgehogs showed any visible signs of ongoing mycotic infection. The identified dermatophytes had identical Internal Transcribed Spacer (ITS) sequences and were identical to the T. erinacei type strain CBS 511.73 ITS sequence (GenBank AB105793) originally isolated from a European hedgehog in New Zealand (Fig. 1). The two ITS sequences were also identical to those of several T. erinacei isolates recovered from pet hedgehogs in Spain [24], represented in Fig. 1 by the isolate T-127 (GenBank KU852597), as well as additional T. erinacei isolates from other countries.

Fig. 1
figure 1

Neighbor-joining tree of ITS sequences from the two Trichophyton isolates recovered in the present study compared to ITS sequences from isolates of T. erinacei and closely related species. The scale is number of nucleotide differences in the 586 bp compared. Support from 10k bootstrap replicates is shown as a percentage at branch divisions. The more distantly related T. rubrum is included as an outgroup. The tree was created in MEGA 6

Both identified T. erinacei isolates were confirmed to carry the genes, pcbAB, pcbC and penDE, which encodes penicillin biosynthesis enzymes (Fig. 2), and expression of the pcbAB and pcbC genes was confirmed by quantitative reverse transcription real-time PCR (RT-qPCR) and subsequent melt-curve analysis. The length and identity of the genes were identical between both isolates but differed from those in the Penicillium chrysogenum Wisconsin 54-1255 reference strain (Fig. 2). Gene sizes were as follows; 11280bp for pcbAB, 1002bp for pcbC, 651bp for penDE in T. erinacei isolates, while 11376bp for pcbAB, 996bp for pcbC, 1275bp for penDE in the Wisconsin 54-1255 (Fig. 2). Amino acid comparisons between the two isolates and Wisconsin 54-1255 showed 60%, 70%, and 66% similarity for pcbAB, pcbC and penDE respectively (Fig. 2). Similar comparisons to Trichophyton species, listed in Table 1, showed similarities of 92-98%, 98-99% and 92-94% for pcbAB, pcbC and penDE respectively.

Fig. 2
figure 2

Comparison of the genes pcbAB, pcbC and penDE in penicillin biosynthesis gene cluster (PGC). T. erinacei isolates from Swedish European hedgehogs (B) against the PGC in Penicillium chrysogenum Wisconsin 54-1255 strain (A) and the PCG identified in T. rubrum (NZ_ACPH00000000.1), T. violaceum (LHPN00000000.1), T. verrucosum (NZ_ACYE00000000.1), T. mentagrophytes (BFBS00000000.1), T. interdigitale (AOKY00000000.1), T. equinum (ABWI00000000.1), T. benhamiae (ABSU00000000.1), T. tonsurans (ACPI00000000.1) (C). The percentages given represent the similarity on amino acid level compared to the T. erinacei hedgehog isolates

Table 1 Trichophyton species and their respective reference IDs used to compare penicillin biosynthesis genes

Identification of benzylpenicillin

In the mass chromatograms from ultra-high-performance liquid chromatography-tandem mass spectrometry (UHPLC-MS/MS) analyses (Fig. 3a–c), the characteristic daughter ion transitions m/z 335 [M+H]+ > 91, 335 [M+H]+ > 98, 335 [M+H]+ > 114, 335 [M+H]+ > 160 and 335 [M+H]+ > 176 are shown. The blank control (Fig. 3a) showed no chromatographic peaks but the sample 18MIK164927 (Fig. 3b) peaks were observed in all transitions at the retention time 2.96 min. These results agreed with those of the benzylpenicillin reference standard (Fig. 3c). In addition, the peak area ratios for the daughter ions were compared and these results were also consistent. The second isolate 19MIK191009 was also analyzed and the result from this analysis indicated presence of benzylpenicillin, but the peak responses were too weak for a definite identification.

Fig. 3
figure 3

Mass chromatograms from UHPLC-MS/MS analyses. The characteristic SRM transitions m/z 335 [M+H]+ > 91, 335 [M+H]+ > 98, 335 [M+H]+ > 114, 335 [M+H]+ > 160 and 335 [M+H]+ > 176. a blank control, b sample 18MIK164927 and c reference standard of benzylpenicillin

Recovery and characterization of mecC-MRSA

Of the 23 sampled hedgehogs 14 (60%) carried mecC-MRSA with 11 originating from Gotland county and 3 from Skåne County, with no MRSA positive hedgehogs found in Uppsala County. Because two isolates were lost at the laboratory during handling twelve isolates were available for genome sequencing. Both hedgehogs from Gotland positive for T. erinacei also carried mecC-MRSA which belonged to sequence types (ST) ST425 and ST1254. In total 5 different STs were identified, with the three isolates from Skåne County belonging to ST130 and the remaining isolates from Gotland County belonging to ST130 (n = 6), ST425 (n = 2), ST1943 (n = 1) and ST2631 (n = 1) (Fig. 4). Except for ST1943 and ST2361 that differed in one allele all recovered STs differed in ≥5 alleles. Using core-genome multi-locus sequence typing (cgMLST) and visualizing the difference in the number of alleles between isolates using a minimum spanning tree based on 1915 alleles, it was shown that the five STs differed significantly from each other (Fig. 3). Furthermore, there were >32 allele differences within each ST (Fig. 4). All mecC-MRSA isolates carried the staphylococcal cassette chromosome mec (SCCmec) type XI, blaZLGA251, and were negative for PVL.

Fig. 4
figure 4

Minimum spanning tree (MST) of core genome MLST (cgMLST) relationship of methicillin resistant S. aureus carrying the mecC gene (mecC-MRSA) from European hedgehogs in Sweden. The cgMLST is based on target genes extracted from the mecC-MRSA genome LGA251, accession number FR821779, using the SeqSphere + software, which identified 1915 alleles present in all compared isolates. Nodes represent isolates (one isolate per node), Numbers in nodes denotes the multi-locus sequence type (7-MLST) as defined by the scheme at https://pubmlst.org/ and colours represent the origin of the isolate, Gotland County (Red) and Skåne County (Blue). Isolates encompassed in the solid box belong to ST425 while those in dashed box belong to ST130. Numbers on the lines between isolates indicate differences in alleles between isolates and line lengths are based on the allele differences in a logarithmic scale. Nodes marked in bold are mecC-MRSA isolates co-occurring with benzylpenicillin-producing T. erinacei isolates. The mecC-MRSA reference strain LGA251 (yellow) belonging to ST425, isolated from a dairy cow bulk milk sample in UK [6], is included in the figure for comparison

Discussion

In the current study we could show that Swedish hedgehogs can carry benzylpenicillin producing T. erinacei. However, it was suggested already in the 1960s that T. erinacei, then called T. mentagrophytes var. erinacei, potentially could produce a penicillin-like substance [23]. This 1960s study was however limited in that it only showed that the investigated substance inhibited growth of penicillin-sensitive S. aureus strains and that the activity of the substance was hampered by penicillinase. In our study, genome sequencing was used to confirm the presence of the penicillin biosynthesis genes in the recovered T. erinacei isolates and RT-qPCR was used to show that the genes were expressed. In addition, UHPLC-MS/MS verified that the isolate 18MIK164927 produced benzylpenicillin (Fig. 3), but that the second isolate 19MIK191009 only had a weak peak response (data not shown). The weak peak response for 19MIK191009 was not unexpected as fungal strains grown under standard conditions may only produce small quantities of benzylpenicillin since production is normally triggered by stress or environmental conditions. As an example, commercial production of benzylpenicillin in Penicillum species relies on extensive genetic and environmental optimization with current strains producing 100.000 times more penicillin than the P. notatum strain originally described by Fleming [25]. Other studies have also confirmed production of antimicrobials by dermatophytes from other settings, but this is to our knowledge the first time for T. erinacei [26]. Albeit only two hedgehogs carried T. erinacei previous studies on hedgehogs have shown that this dermatophyte species is widespread among hedgehogs, especially during the winter months [27,28,29]. The higher incidence of T. erinacei during winter months, when hedgehogs hibernate, could explain the lower number of positive samples in the current study, since all hedgehogs included were sampled in spring to early autumn.

The identification of penicillin-producing T. erinacei in hedgehogs is important since this dermatophyte might influence the skin bacterial flora of the hedgehogs by imposing a selection pressure on or working in a symbiotic relationship with the flora. The selective pressure, or symbiosis, could facilitate the emergence of resistant variants of bacteria such as mecC-MRSA, and both hedgehogs that carried penicillin-producing T. erinacei also carried mecC-MRSA (Fig. 4). A previous study has however described that the PBP2c produced by mecC has lower affinity for penicillin than the PBP2a produced by mecA [28], which could contradict the hypothesis of a possible connection between mecC-MRSA and penicillin-producing T. erinacei. However, the selection of mecC-MRSA on hedgehogs could be influenced by the presence of the blaZLGA251 gene which produces beta-lactamase and is in close proximity to the mecC on the SCCmec XI. In the current study, as in previous ones, the isolates were all positive for the SCCmec XI and carried blaZLGA251. In opposition to mecA-MRSA it has also been shown that broad-spectrum beta-lactam resistance for mecC-MRSA is due to the combined presences of mecC and blaZLGA251 on the SCCmec XI [30]. It is also worth to note that mecA-MRSA might also have evolved due to selection pressure from penicillin rather than through the more modern methicillin [31].

In accordance with previous studies, we found that mecC-MRSA is common, 60%, among wild hedgehogs [8, 11]. We were also able to show that the mecC-MRSA isolates belonged to five distinct 7-MLST types and that it was a high diversity between and within STs based on cgMLST (Fig. 4). The high diversity indicates that occurrence in hedgehogs is not due to nosocomial spread at rescue centers or a local endemic spread fueled by release of animals. In addition, the recent Danish study showed the same high mecC-MRSA incidence on hedgehogs not connected to rescue centers [11]. Previous studies also emphasized the high mecC-MRSA occurrence and diversity in this animal species, but based on spa-types rather than high-resolution genome sequencing [8, 11]. Furthermore, the STs identified in this study have all previously been shown to be connected to mecC-MRSA except for ST1254, and all isolates in this study carried the SCCmec XI, which is the SCCmec linked to mecC [16, 17]. The mecC-MRSA associated STs identified in this study, and others, also overlaps with those identified from clinical cases in humans, dairy cattle, goats, and companion animals in Sweden [18, 32]. These combined studies therefore all lend further support to the suggestion that mecC-MRSA could be a wildlife associated MRSA (WA-MRSA), rather than a LA-MRSA, with the main reservoir being European hedgehogs [17]. If European hedgehogs, which primarily are native to Northern and Western Europe, are the main reservoirs for mecC-MRSA it would also help explain why mecC-MRSA mainly has been found in Europe [16, 17]. However, it is worth noticing that other wildlife reservoirs might exist as a recent Spanish study showed a relatively high incidence of mecC-MRSA in wild rabbits [33].

To understand the occurrence and evolution of mecC-MRSA and its connection to penicillin-producing T. erinacei and to hedgehogs, additional studies are warranted as the current pilot-study is limited in the number of samples and isolates investigated. Such studies should be; i) more extensive sampling of hedgehog populations from wider geographic areas and during hibernation, as well as pet hedgehogs, to ascertain a statistically viable correlation between mecC-MRSA and penicillin producing T. erinacei, ii) investigation of the influence of the penicillin-production of T. erinacei on mecC-MRSA, mecA-MRSA, and penicillin-sensitive S. aureus strains in-vitro, iii) investigation of other wildlife species for occurrence of mecC-MRSA to establish if occurrence is exclusively linked to hedgehogs and iv) determination of resistance profiles of additional microflora from hedgehogs that are carriers of penicillin-producing T. erinacei which would provide an insight on the mechanics of antimicrobial resistance in nature.

Conclusions

The current study shows that European hedgehogs in Sweden can carry benzylpenicillin-producing T. erinacei and that the hedgehogs that carry these dermatophytes also carries mecC-MRSA. In addition, the study confirms the high occurrence and diversity of mecC-MRSA in the European hedgehog population. The results emphasize the further need to study the association, host-adaption and potential shared evolution of mecC-MRSA, T. erinacei and European hedgehogs.

Methods

Collection and sampling of hedgehogs

In July 2018, custodians at two rescue centres in Gotland County and Skåne County were invited to send dead hedgehogs to the National Veterinary Institute (SVA) for the study. Included hedgehogs were euthanized due to injury or illness or had already died of natural causes upon arriving at the rescue centres. Euthanasia was performed by trained personal through intraperitoneal injection with pentobarbital according to Swedish legislation. In addition to the two rescue centres the study participants also collected dead hedgehogs found as roadkill in Uppsala County. Ethical approval according to national legislation (SJVFS 2015:38) was not required since samples were collected from wildlife where the cause of death, natural or euthanized, was unrelated and occurred prior to inclusion in the study. The study adhered to the Animal Research: Reporting of In Vivo Experiments (ARRIVE) guidelines.

Sampling was carried out between July 2018 and ended in October 2019. Sampling during winter months was not feasible since the animals were in hibernation. All hedgehogs were shipped to the laboratory within 24–48h of death and subsequently sampled within 24 h. For dermatophytes, quills and skin scrapings were taken and for MRSA, oral cavity, nostril, skin, and perineum of hedgehogs were swabbed using Copan EswabsTM (Copan).

Fungi cultivation and identification

Samples were inoculated on Sabouraud agar (SAB) with Chloramphenicol, pH 7, (National veterinary Institute, SVA) and modified Dixon agar (SVA), and then incubated at 27 °C for 15 days. Cultures were macroscopically analysed for dermatophytes and all fungi cultures characteristic of dermatophytes were further subjected to microscopy. Prior to microscopy, a drop of MYCETBLUETM stain was placed at the centre of a microscope glass slide and a piece of cellophane tape was used to collect and apply a culture in the stain on the glass slide. The slide was then incubated at room temperature for 15 min and viewed under a light microscope at 100-400X magnification to verify presence of dermatophytes based on the morphology of macro- and microconidia.

MRSA isolation and identification

Copan EswabsTM (Copan) were briefly vortexed, and 0.2 mL of the suspension was added to 4.8 mL trypticase soy broth (TSB) supplemented with 4% NaCl, 1% mannitol, and 10 mg/L aztreonam, and incubated overnight at 37 °C. To select for MRSA, 10 μL of the overnight culture was streaked on MRSA 2 Brilliance agar (Oxoid), Mannitol salt agar (SVA) and horse blood agar (SVA), respectively, and plates were incubated at 37 °C overnight.

Suspected MRSA-colonies were subjected to Matrix Assisted Laser Desorption and Ionization- Time of flight (Bruker Maldi-TOF Biotyper System) to confirm species, and presences of mecA/mecC/PVL/nuc was confirmed using a real-time quadruplex PCR [34].

DNA extraction, sequencing, and bioinformatics

Verified dermatophytes were cultured on SAB without antibiotics at 30 °C for 14 days to obtain pure cultures. Colonies of the pure cultures were homogenised by a mortar and pestle in liquid nitrogen followed by total DNA extraction using DNeasy Plant Mini Kit (Qiagen) according to manufacturer’s instructions.

MRSA isolates were cultured on horse blood agar and genomic DNA was extracted from a 1 μL loopful of colonies using EZ1 tissue kit (Qiagen) on a EZI advanced XL (Qiagen).

DNA from dermatophyte and MRSA were prepared using Nextera XT DNA library preparation kit (Illumina) and genome sequencing was performed on a MiSeq Illumina platform, as 2x250 bp paired-end reads aiming for a minimum average coverage of 40X. The quality of sequence data was analysed using the FastQC program [35].

Sequence data from S. aureus were subsequently run through an assembly, species determination, and antibiotic resistance classification pipeline composed of Trimmomatic 0.36 [36], SPAdes 3.5.0 [37], Pilon 1.2.3 [38], Kraken using mini-Kraken 8GB-database [39], and ARIBA [40] using the ResFinder database (http://www.genomicepidemiology.org/). SCCmec cassette typing was performed using SCCmecFinder (https://cge.cbs.dtu.dk). 7-MLST and core genome MLST (cgMLST) was performed using the Ridom SeqSphere+ software [41], with the genome of LGA251, accession number FR821779 used to define an ad-hoc cgMLST scheme with default settings in SeqSphere+.

For the assembly of dermatophyte sequencing data, the same pipeline as for MRSA was used but excluding ARIBA and Kraken. To identify the dermatophyte species, the ITS region of Trichophyton rubrum (refseq: NZ_ACPH00000000.1) was used in a BLAST+ search against the dermatophyte assemblies. Matches to ITS with the highest score, coverage, identity, and lowest E-value were extracted from respective contigs and used in species identification performed by matching against the ISHAM Barcoding Database (http://its.mycologylab.org/). Reference T. erinacei ITS sequences from the ISHAM Barcoding Database were retrieved, sequences were aligned by the ClustalW algorithm and their relatedness investigated by the Neighbor joining algorithm in Mega 6 [42] excluding positions with gaps and otherwise with default settings. The resulting tree was evaluated by generating 10,000 bootstrap replicates.

Identification and expression of penicillin biosynthesis genes (PGs)

To identify the penicillin biosynthesis gene cluster (PGC) containing the genes, pcbAB, pcbC and penDE in the recovered T. erinacei, the PGC sequence from the Penicillium chrysogenum isolate Wisconsin54-1255 (accession number EF601124.1) was used as reference for a BLAST+ analysis of the generated contigs. The full ORFs for the corresponding homologues in the analysed assembly were extracted from a contig producing BLAST hits for all three genes using NCBI ORFfinder tool (https://0-www-ncbi-nlm-nih-gov.brum.beds.ac.uk/orffinder/) and Snapgene (GSL Biotech, snapgene.com). Gene orthologues from available Trichophyton species (Table 1) were compared to genes from the recovered strains at amino acid level using the NCBI BlastP suite.

To evaluate expression of the penicillin biosynthesis genes, colonies from a 14-day pure culture were homogenised by a mortar and pestle in liquid nitrogen followed by extraction of total RNA using Trizol (Thermofisher) and phenol-chloroform extraction method. The resultant RNA was treated with DNase 1 (Thermo Scientific™) according to manufacturer’s instructions. Expression of two genes, pcbAB and pcbC was investigated using iTaq Universal One-Step RT-qPCR Kit, in triplicates with in-house deigned primers sets using Primer3 with default settings (http://bioinfo.ut.ee/primer3-0.4.0/) (Table 2). These primers were designed only for use on pure cultures and were not evaluated for specificity in other contexts. Dnase treated RNA, fungi genomic DNA (used as positive control), were analysed and RNA without the DNase treatment was used as a quality control for the efficiency of eliminating DNA remnants post extraction. The thermal cycling program was as follows; 10 min at 50 °C, 1 min at 95 °C followed by 40 cycles of 15 sec at 95 °C and 1 min at 60 °C subsequent melt-curve analysis of 60 °C–95 °C with 0.5 °C increment for 4 sec per step as an indicator to confirm the specific amplification of a single target consistent with the product produced in the positive control .

Table 2 Oligonucleotide primer sets for RT-qPCR

Identification of benzylpenicillin

Scrapings from 14-day cultures of each Trichophyton isolate were stored in absolute methanol at -80 °C awaiting chemical analysis. A blank control sample was included which was treated identical to the hedgehog samples. The methanol extract (supernatant) of each sample (40 μL) was diluted with 160 μL MilliQ-water, vortexed for 1 min and transferred to a vial. For substance identification and comparison, a prepared standard (1 ng/mL in methanol:MilliQ-water (20/80, v/v)) of a European pharmacopoeia reference material of benzylpenicillin sodium (certified reference standard, from Sigma-Aldrich Corporation, Germany) was used.

Benzylpenicillin analysis was performed with a UHPLC-MS/MS system composed of an Acquity UPLC coupled to a Xevo TQ-Sμ mass spectrometer (Waters Corporation, MA, USA) with an electrospray interface. The chromatographic system used consisted of a C18 guard column (Waters Corp.) and an Acquity BEH C18 column (2.1 x 100 mm, 1.7 μm) (Waters Corp.) both at 65 °C. The mobile phase consisted of A) 0.1 % formic acid in water and B) methanol and it was delivered as a gradient. The gradient started at 30% B to 0.40 min, then continued with a linear increase over time to 80% B at 4.00 min, and 95% B at 4.50 min. At 5.50 min the gradient switched to 10% B and was held constant for 1.5 min for equilibration. The flow rate was 0.400 mL/min and the injection volume 10 μL. The analyte was analysed with a positive capillary voltage of 1.2 kV and a cone voltage of 18 V. The desolvation temperature was 500 °C and desolvation gas flow was 1000 L/h. The ionization was positive electrospray and benzylpenicillin was detected as [M+H]+. The mass spectrometric analysis mode was selected reaction monitoring (SRM) using daughter ion transitions characteristic for benzylpenicillin. The SRM transitions for the qualitative detection were m/z 335 > 91, m/z 335 > 98, m/z 335 > 114, m/z 335 > 160 and m/z 335 > 176 (collision energy 44 eV, 32 eV, 30 eV, 10 eV and 12 eV respectively). The results were evaluated using the software TargetLynx (Waters Corp.). The evaluation of data was done using the EC. 657/2002. Commission Decision 2002/657/EC as guideline.

Availability of data and materials

The data and isolates generated during the current study are available from the authors upon reasonable request. Sequence reads T. erinacei and mecC-MRSA isolates have been deposited in the European Nucleotide Archive under the accession number PRJEB37151 and PRJEB37163, respectively.

Abbreviations

cgMLST:

core-genome Multi-locus sequence typing

ITS:

Internal Transcribed Spacer

MRSA:

Methicillin-resistant Staphylococcus aureus

PCR:

Polymerase Chain Reaction

PGC:

penicillin biosynthesis gene cluster

RT-qPCR:

Reverse transcription quantitative PCR

SAB:

Sabouraud agar

SCCmec:

Staphylococcal chromosomal cassettes mec

SRM:

Selected reaction monitoring

ST:

Sequence types

UHPLC-MS/MS:

Ultra-high-performance liquid chromatography-tandem mass spectrometry

MLST:

Multi-locus sequence typing

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Acknowledgements

The authors are grateful to Wildlife rehabilitator Eva Fallström and VMD Lotta Persson for collecting and sending dead and euthanized hedgehogs to SVA. We also would like to thank Mattias Myrenås and Annica Landén for assistance in the laboratory.

Conflict of Interest Statement

Nothing to declare.

Funding

The study was funded by The Royal Swedish Academy of Agriculture and Forestry (GFS2018-0069) and was co-financed by the National Veterinary Institute (SVA), Uppsala, Sweden. Funders had no influence on the design, analysis and reporting of the study. Open Access funding provided by Swedish University of Agricultural Sciences.

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Authors

Contributions

Faruk Dube (FD) Robert Söderlund (RS), Matilda Lampinen Salomonsson (MS), Karin Troell (KT), Stefan Börjesson (SB): RS, KT and SB conceived, designed, and executed the study. FD wrote the first draft of the manuscript and performed the microbiology laboratory analyses with SB assistants, and bioinformatic analyses were performed by RS, FD, and SB. All work, analysis and writing related to UHPLC-MS/MS analyses was done by MS. The data and results were analysed by FD, RS, KT and SB. The manuscript was critically revised by RS, KT, MS and SB and SB finalized the manuscript. All authors read and approved the manuscript.

Corresponding author

Correspondence to Faruk Dube.

Ethics declarations

Ethics approval and consent to participate

Ethical approval according to national legislation (SJVFS 2015:38) was not necessary as the samples were collected from dead wildlife where the cause of death was not related to the preformed study. The included hedgehogs were either found as roadkill, was dead on arrival or died during the stay at the participating centres, or euthanized due to poor condition on arrival or deteriorating health during the stay at the centres.

Representatives for rescue centres gave consent via e-mail to participate in the study to Stefan Börjesson. When representatives accepted participation, they were provided with material and instructions on how to package and send deceased hedgehogs to SVA, all costs related to transport and packing were paid by SVA.

Consent for publication

All people involved in the manuscript and study was informed about the intent to publish and have given their approval.

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Nothing to declare.

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Dube, F., Söderlund, R., Lampinen Salomonsson, M. et al. Benzylpenicillin-producing Trichophyton erinacei and methicillin resistant Staphylococcus aureus carrying the mecC gene on European hedgehogs – A pilot-study. BMC Microbiol 21, 212 (2021). https://0-doi-org.brum.beds.ac.uk/10.1186/s12866-021-02260-9

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