Intracellular Transposition and Capture of Mobile Genetic Elements following Intercellular Conjugation of Multidrug Resistance Conjugative Plasmids from Clinical Enterobacteriaceae Isolates

ABSTRACT Mobile genetic elements (MGEs) are often associated with antimicrobial resistance genes (ARGs). They are responsible for intracellular transposition between different replicons and intercellular conjugation and are therefore important agents of ARG dissemination. Detection and characterization of functional MGEs, especially in clinical isolates, would increase our understanding of the underlying pathways of transposition and recombination and allow us to determine interventional strategies to interrupt this process. Entrapment vectors can be used to capture active MGEs, as they contain a positive selection genetic system conferring a selectable phenotype upon the insertion of an MGE within certain regions of that system. Previously, we developed the pBACpAK entrapment vector that results in a tetracycline-resistant phenotype when MGEs translocate and disrupt the cI repressor gene. We have previously used pBACpAK to capture MGEs in clinical Escherichia coli isolates following transformation with pBACpAK. In this study, we aimed to extend the utilization of pBACpAK to other bacterial taxa. We utilized an MGE-free recipient E. coli strain containing pBACpAK to capture MGEs on conjugative, ARG-containing plasmids following conjugation from clinical Enterobacteriaceae donors. Following the conjugative transfer of multiple conjugative plasmids and screening for tetracycline resistance in these transconjugants, we captured several insertion sequence (IS) elements and novel transposons (Tn7350 and Tn7351) and detected the de novo formation of novel putative composite transposons where the pBACpAK-located tet(A) is flanked by ISKpn25 from the transferred conjugative plasmid, as well as the ISKpn14-mediated integration of an entire 119-kb, blaNDM-1-containing conjugative plasmid from Klebsiella pneumoniae. IMPORTANCE By analyzing transposition activity within our MGE-free recipient, we can gain insights into the interaction and evolution of multidrug resistance-conferring MGEs following conjugation, including the movement of multiple ISs, the formation of composite transposons, and cointegration and/or recombination between different replicons in the same cell. This combination of recipient and entrapment vector will allow fine-scale experimental studies of factors affecting intracellular transposition and MGE formation in and from ARG-encoding MGEs from multiple species of clinically relevant Enterobacteriaceae.

ABSTRACT Mobile genetic elements (MGEs) are often associated with antimicrobial resistance genes (ARGs). They are responsible for intracellular transposition between different replicons and intercellular conjugation and are therefore important agents of ARG dissemination. Detection and characterization of functional MGEs, especially in clinical isolates, would increase our understanding of the underlying pathways of transposition and recombination and allow us to determine interventional strategies to interrupt this process. Entrapment vectors can be used to capture active MGEs, as they contain a positive selection genetic system conferring a selectable phenotype upon the insertion of an MGE within certain regions of that system. Previously, we developed the pBACpAK entrapment vector that results in a tetracycline-resistant phenotype when MGEs translocate and disrupt the cI repressor gene. We have previously used pBACpAK to capture MGEs in clinical Escherichia coli isolates following transformation with pBACpAK. In this study, we aimed to extend the utilization of pBACpAK to other bacterial taxa. We utilized an MGE-free recipient E. coli strain containing pBACpAK to capture MGEs on conjugative, ARG-containing plasmids following conjugation from clinical Enterobacteriaceae donors. Following the conjugative transfer of multiple conjugative plasmids and screening for tetracycline resistance in these transconjugants, we captured several insertion sequence (IS) elements and novel transposons (Tn7350 and Tn7351) and detected the de novo formation of novel putative composite transposons where the pBACpAK-located tet(A) is flanked by ISKpn25 from the transferred conjugative plasmid, as well as the ISKpn14-mediated integration of an entire 119-kb, bla NDM-1 -containing conjugative plasmid from Klebsiella pneumoniae. IMPORTANCE By analyzing transposition activity within our MGE-free recipient, we can gain insights into the interaction and evolution of multidrug resistance-conferring MGEs following conjugation, including the movement of multiple ISs, the formation of composite transposons, and cointegration and/or recombination between different replicons in the same cell. This combination of recipient and entrapment vector will allow finescale experimental studies of factors affecting intracellular transposition and MGE formation in and from ARG-encoding MGEs from multiple species of clinically relevant Enterobacteriaceae.
KEYWORDS entrapment vector, insertion sequence, antimicrobial resistance, transposon, bla NDM-1 A ntimicrobial resistance (AMR) is a major global public health problem and is likely to get worse without the rapid development of new antibiotics and additional therapeutic options. Every use of antimicrobials provides a selective pressure for the evolution of AMR and associated mobile genetic elements (MGEs).
MGEs, such as conjugative plasmids and integrative and conjugative elements (ICEs), are responsible for the dissemination of antimicrobial resistance genes (ARGs) among bacteria, and they often contain multiple ARGs. ARGs are mobilized onto conjugative MGEs via the activity of smaller MGEs, including insertion sequences (ISs), that are capable of intracellular transposition. Transposons containing ARGs against lastresort antibiotics have been found on different plasmids in different bacterial species. For example, bla NDM-1 , conferring carbapenem resistance, and mcr-1, conferring colistin resistance, were found on ISAba125-and ISApl1-based composite transposons like Tn125 and Tn6330, respectively. Both composite transposons have been found on multiple plasmids in different bacterial species (1)(2)(3)(4)(5).
MGEs are usually identified through the phenotypic changes conferred by the accessory genes, including ARGs, or changes caused by insertions of MGEs that result in the activation/inactivation of other genes. For example, insertions of IS26, IS5, IS903, and IS1 into the ompK36 porin gene and insertion of the ISEcp1-bla OXA-181 transposon into the mgrB gene were shown to result in carbapenem and colistin resistance, respectively, in Klebsiella pneumoniae (6)(7)(8). Bioinformatic analysis can also identify MGEs by comparative genomics of whole-genome sequencing (WGS) data and by interrogating WGS data with available databases of MGEs (9, 10); however, this approach can rarely give information on the transposition activity of these MGEs. Contextualization of AMR genes on MGEs from short-read sequencing data is also notoriously difficult (11).
Another approach is to use entrapment vectors to capture MGEs based solely on their transposition activity. Entrapment vectors contain a genetic system that will confer a selective phenotype when MGEs transpose into a defined region of DNA (12)(13)(14). Previously, we developed a single-copy-number entrapment vector called pBACpAK and demonstrated that it can detect the insertion of MGEs in both laboratory and clinical Escherichia coli isolates (15,16). pBACpAK contains a cI-te(A) gene system in which the l repressor (encoded by cI) constitutively inhibits the expression of the tet(A) gene by binding to the P RM promoter, blocking the expression of tet(A) (17). When an MGE inserts into the cI gene, the expression of the repressor is interrupted, leading to the expression of tet(A) and a tetracycline resistance phenotype (Fig. 1). Several IS elements and a novel translocatable unit (TU) carrying a functional trimethoprim resistance gene, dfrA8, were captured by using the pBACpAK entrapment vector previously (15).
In this study, we used pBACpAK to identify active MGEs from conjugative plasmids that had transferred via conjugation to a transposon-free, differentially resistant recipient E. coli strain from carbapenemase-producing clinical Enterobacteriaceae donor strains (Fig. 1). Multiple novel MGEs were detected from the screening of tetracycline-resistant transconjugants, giving insights into the interaction and evolution of MGEs carrying ARGs.

RESULTS
Characterization of donor and recipient strains. Based on bioinformatic analysis of the WGS data of 59 carbapenemase-producing Enterobacteriaceae clinical strains, 8 clinical isolates (7 K. pneumoniae and 1 E. coli) were selected as donors in this study, as summarized in Table 1, with the raw data shown in Table S2 in the supplemental material. Their resistance phenotypes against rifampicin (Rif) and fusidic acid (Fus) were subsequently determined to make sure that both antibiotics could be used for selection of transconjugants following a filter-mating experiment. All 8 clinical strains showed no growth on Luria-Bertani (LB) agar supplemented with rifampicin and fusidic acid (Table 1). pBACpAK was electroporated into E. coli strain MDS, which was subsequently sequentially evolved to rifampicin and then fusidic acid resistance. The strain was then screened on LB agar containing tetracycline to check for the rate of mutations in the cI gene. No tetracycline-resistant colonies were found on any plates from three replicates after 72 h of incubation.
Developing the E. coli MDS::pBACpAK strain into rifampicin and fusidic acid resistance was done to use the resistant phenotypes as selective markers for recipient strains, reducing the chance for false-positive transconjugants due to spontaneous mutations in the donor strains. E. coli MDS::pBACpAK with rifampicin and fusidic acid resistance was selected and denoted E. coli MDS Rif Fus::pBACpAK. E. coli MDS Rif Fus::pBACpAK was shown to have point mutations (underlined) in the rpoB (D516G [a mutation of D to G at position 516]; GAC!GGC) and fusA (L466F; CTC!TTC) genes, which are known to confer resistance to rifampicin and fusidic acid, respectively (18,19).
Transfer of conjugative plasmids from clinical isolates to E. coli MDS Rif Fus:: pBACpAK. Filter mating between clinical isolates and E. coli MDS Rif Fus::pBACpAK was carried out, and transconjugants were selected on LB agar supplemented with FIG 1 Capture of MGEs from conjugative plasmids by using pBACpAK. The conjugative plasmid from carbapenemase-producing Enterobacteriaceae clinical strains were transferred to an E. coli MDS Rif Fus::pBACpAK recipient strain through conjugation. Transconjugants were selected on LB agar supplemented with chloramphenicol, rifampicin, ampicillin, and fusidic acid. If the MGE, located on the conjugative plasmid, translocated into the cI gene on pBACpAK, it would disrupt the expression of the l repressor, conferring tetracycline resistance due to the derepression of the P R promoter. Clones with an insertion of MGEs therefore can be selected on tetracycline-containing agar. The gray and red arrowed boxes represent cI and tet(A) genes, respectively, which point in the direction of transcription. MGE, l repressors, and tetracycline resistance protein are shown as orange, gray, and red rectangles. The blue, yellow, green, and brown rectangles represent donor, recipient, transconjugant, and tetracycline-resistant transconjugant cells, respectively. Chl r , chloramphenicol resistance; Rif r , rifampicin resistance; Amp r , ampicillin resistance; Fus r , fusidic acid resistance; Tet r , tetracycline resistance. chloramphenicol, rifampicin, ampicillin, and fusidic acid (LB CRAF agar). Several transconjugant colonies were found from all mating pairs. The donor-only group showed no growth on LB agar supplemented with chloramphenicol, rifampicin, and fusidic acid, while the recipient-only group showed no growth on LB ampicillin plates. Both control groups also showed no growth on any LB CRAF agar plates. The cI-tet(A) fragments were successfully amplified from all mating pairs except the K. pneumoniae strain K68-18 and E. coli MDS Rif Fus::pBACpAK pair, which verified that transconjugants from 7 donors contained conjugative plasmids (conferring an ampicillin resistance phenotype) and the pBACpAK entrapment vector.
Most clones showed an insertion in the cI repressor genes; however, E. coli MDS-50825040-TC-Tet-2-3 and E. coli MDS-50627996-TC-Tet-2 showed an ISKpn25 insertion between tet(A) and oriV and an IS26 insertion in the sopA gene on pBACpAK, respectively. The tetracycline resistance phenotype in both clones was a result of a deletion in the cI repressor gene (6-bp and 786-bp deletions). E. coli MDS-50825040-TC-Tet-3-7 and E. coli MDS-50825040-TC-Tet-4-38 each had an insertion of ISKpn25, one in the cI repressor gene and the other one between tet(A) and oriV. For clones that were analyzed by WGS, translocation of MGEs into chromosomal DNA was determined by using breseq, which showed no additional insertion within the chromosome of the recipient in any tetracycline-resistant transconjugants.

DISCUSSION
Entrapment vectors have been used to capture MGEs in multiple bacterial species, both Gram positive and Gram negative, such as Paracoccus pantotrophus, Rhodococcus fascians, Agrobacterium tumefaciens, Corynebacterium glutamicum, and E. coli (15,(24)(25)(26). As this approach relies on the transposition activity of MGEs, it has the potential to identify new MGEs that have not been previously delineated (24,27,28). In our study, we have identified 2 novel transposons (Tn7350 and Tn7351) in transconjugants from the conjugations between carbapenemase-producing clinical Enterobacteriaceae isolates and E. coli MDS Rif Fus::pBACpAK. Both of these transposons, plus the region absent in Tn7351 compared to Tn7350, are flanked by GAAC inverted or direct repeats. GAAC represents the conserved target site of IS91 insertion sequences (29,30). ISSbo1, which is present on both Tn7350 and Tn7351, is a member of the IS91 family of insertion sequences (31) and is therefore likely to be responsible for the movement of these novel transposons; however, experimental verification is still needed to confirm this.
Prior to the filter-mating experiment, we characterized each carbapenemase-producing Enterobacteriaceae strain by using the bioinformatic tools Mobile Element Finder, ResFinder, and PlasmidFinder to analyze their WGS data to use as criteria for a selection of donor strains. Our results showed that we detected novel MGEs with pBACpAK that were not reported by these tools, as they are not present in the databases, but it could also capture other known MGEs that were missed by these tools, such as ISSbo1 in K. pneumoniae 50675619, ISKpn25 in K. pneumoniae 50825040, and IS26 in K. pneumoniae 50627996 (Table S2).
Previously, the pBACpAK entrapment vector was developed and used in laboratory and clinical E. coli isolates, as it was designed based on the pCC1BAC vector containing the E. coli F factor single-copy origin of replication so that entrapment of larger DNA fragments would be more stable than if we had used a high-copy-number plasmid. In this study, we proposed another approach that could extend the uses of pBACpAK to the detection of MGEs from other bacterial species through a filter-mating experiment between clinical Enterobacteriaceae isolates as donors and the differentially marked E. coli MDS Rif Fus::pBACpAK as a recipient. This allows the capture of MGEs located on conjugative plasmids/transposons from any bacterial species that can transfer MGEs via conjugation (or transformation) to our MGE-free E. coli recipient strain. Conjugative elements, especially from clinical isolates, tend to carry not only multiple ARGs but also smaller MGEs; it has been shown, for example, that bacterial plasmids tend to contain a significantly higher number of IS elements than their chromosomal DNA (32).
This approach also extends the uses of pBACpAK in terms of resistance phenotype, since pBACpAK uses the chloramphenicol resistance gene as a selective marker for the vector and a tetracycline resistance phenotype to screen for clones with MGE insertion. Therefore, it cannot be used directly with E. coli strains with either a chloramphenicol or tetracycline resistance phenotype. As only resistance genes associated with conjugative elements will be transferred to the recipient in filter mating, it will reduce the background resistance phenotypes from the clinical isolates. This was shown in our study where K. pneumoniae 50627996 and E. coli 50676002 had the tetracycline resistance phenotype, but the transconjugants from both clinical isolates were susceptible to tetracycline, allowing us to screen for MGEs on other conjugative elements from both strains.
The conjugation and subsequent detection of MGE movement in transconjugants demonstrate both how MGEs like IS elements and Tns can translocate from one bacterial cell to another with the help of conjugative elements and the consequences of rapid dissemination to other replicons in the recipient cell. The translocation of IS elements can have direct consequences for resistance to their host. ISKpn26 has recently been shown to insert into acrR, leading to inactivation of the AcrAB-TolC multidrug efflux pump and resistance to tigecycline in carbapenemase (KPC-2)-producing ST11 K. pneumoniae isolates from Chinese hospitals (33). ISKpn14 and ISKpn25 have previously been shown in several studies to be associated with colistin resistance through an insertion that disrupts the expression of the mgrB regulator gene, which results in overexpression of PhoPQ, activating the pmrHFIJKLM operon and modification of lipopolysaccharide, a drug target of colistin (34)(35)(36)(37)(38). While the translocation of ISs in our entrapment vector is also detected by interrupting a gene (cI) leading to a tetracycline resistance phenotype, the translocation of MGEs following conjugation can also result in the formation of new composite transposons and variations of known MGEs containing antibiotic resistance accessory genes. In our study, we observed the formation of two independently derived putative novel composite transposons containing the pBACpAK-located tet(A) tetracycline resistance gene flanked by copies of ISKpn25. The tet(A) in these clones may have the potential to be disseminated as a composite transposon. It could also move through an intermediate circular structure containing one copy of ISKpn25 and the tet(A) gene, such as translocatable units (mainly reported in IS26-family PCTs) and unconventional circularized structures (UCSs) (39,40). However, the estimation of copy numbers of the tet(A) resistance gene in E. coli MDS-50825040-TC-Tet-3-7 and E. coli MDS-50825040-TC-Tet 4-38 (Table S3) showed that they had the same copy number as the chloramphenicol resistance gene on pBACpAK, suggesting that it was unlikely that tet(A) was being mobilized, and potentially amplified, from pBACpAK at detectable levels in the bacterial population analyzed; however, planned evolutionary studies will reveal if this gene is able to be acquired by the larger conjugative plasmid.
Comparing the sequences of Tn7359 from E. coli MDS-50825040-TC-Tet-3-1 and plasmid p2 from K. pneumoniae showed that plasmid p2 contained only one copy of ISKpn14. The Tn7359 composite transposon would therefore form via transposition into pBACpAK. ISKpn14 is an IS1 family IS element, which can transpose through both conservative transposition and replicative transposition (Fig. 5) (41,42). An insertion of Tn7359 on pBACpAK could occur as a result of a replicative transposition without a resolution of the cointegrate between the conjugative plasmid and the pBACpAK vector. It could also occur as a two-step event by first inserting only ISKpn14 through replicative transposition, as suggested by an insertion of ISKpn14 in E. coli MDS-50825040-TC-Tet-2-1. The ISKpn14-containing pBACpAK and ISKpn14-containing conjugative plasmid could subsequently combine through a targeted conservative transposition or homologous recombination at the ISKpn14 of both replicons (Fig. 5).
The entrapment of Tn7359 by pBACpAK is the first time, to our knowledge, an entrapment vector captured an entire ARG-containing conjugative plasmid. Even though the captured element was not originally a transposon, the structure of the p50825040-pBACpAK cointegrate now fits the definition of a composite transposon, consisting of two IS elements flanking a DNA fragment (21,43). It also shows how  [41]) where the cointegrate did not resolve, so it combined p50825040 with pBACpAK. (B) It could also form through targeted conservative transposition or homologous recombination between the ISKpn14-containing pBACpAK and p50825040. The ISKpn14-containing pBACpAK could form either through the transposition of ISKpn14 into the cI repressor gene or the resolution of the p50825040-pBACpAK cointegrate, indicated by the green dashed-line arrows. The yellow, green, and red arrowed boxes represent cI, ISKpn14, and tet(A), respectively. The gray and orange circles represent pBACpAK and p50825042, respectively. multidrug resistance conjugative plasmids could extend their genetic complement through fusion with other plasmids, something that has recently been reported in a K. pneumoniae isolate containing the IncFIB:IncHI1B hybrid plasmid pEBSI036-1-NDM-VIR from an Egyptian hospital (44). The p50825040 conjugative plasmid from the donor would receive the tet(A) tetracycline resistance gene due to a fusion with the pBACpAK vector. Several studies also discovered plasmid fusion mediated by IS elements, such as IS257-mediated generation of multidrug resistance plasmids pSK818 and pSK697 in Streptococcus epidermis and ISKpn19-mediated cointegration between plasmid pBJ114-46 and pBJ114-141 in E. coli (45,46). Previously, all entrapment vector studies used cI-tet(A) primers and primer walking to identify MGEs in the tetracycline resistance clones. However, we found that the cItet(A) region of some samples could not be amplified by both standard and long PCR protocols, so they could not be sequenced by Sanger sequencing. We therefore used WGS sequencing to characterize these clones. We found that E. coli MDS-50825040-TC-Tet-3-7 and Tet 4-38 had double insertions of ISKpn25 both at the cI gene and downstream from tet(A). Insertions of MGEs in other locations, not in the cI-tet(A) region, on pBACpAK were found in the WGS analysis of E. coli MDS-50627996-TC-Tet-2 as well, including an IS26 insertion in sopA and a 786-bp deletion in the cI gene, resulting in tetracycline resistance and a failed cI-tet(A) PCR, as it lost a cI-tet(A)-F1 primer binding site. E. coli MDS-50825040-TC-Tet-2-3 showed a wild-type cI-tet(A) PCR amplicon in colony PCR screening. This plasmid was then extracted and used to represent the wildtype pBACpAK in XhoI plasmid digestion to compare with other tetracycline-resistant transconjugants. However, XhoI plasmid digestion showed that the 3-kb cI-tet(A) band of E. coli MDS-50825040-TC-Tet-2-3 shifted up to more than 10 kb (Fig. S3); it was therefore sent for WGS sequencing, which showed a 6-bp deletion in the cI gene, conferring tetracycline resistance, and the insertion of ISKpn25 at a site downstream from tet(A).
With the advancement of the sequencing technologies and the declining cost, using WGS sequencing to analyze all tetracycline resistance clones is becoming a viable option, as it will give information on translocation of MGEs into other locations, including the recipient chromosomal DNA. In our study, the WGS data did not show MGE insertions in the host chromosomal DNA. Such insertions are likely in a cellular population but in this case were not selected for, as our assay screened for transconjugants with a tetracycline resistance phenotype that would occur only in cells with an inactivating mutation or insertion of an MGE into the cI repressor gene on the pBACpAK vector.
In conclusion, we have demonstrated an approach to use the pBACpAK entrapment vector to capture MGEs from conjugative elements through a filter-mating experiment between clinical Enterobacteriaceae isolates and the E. coli MDS Rif Fus::pBACpAK recipient, which extended the utility of pBACpAK to other bacterial species. We also showed here that pBACpAK had the potential to capture large (120-kb) MGEs, including conjugative plasmids. Our results also demonstrated several aspects of MGE evolution after conjugation, including the rapid movement of IS elements and transposons, the formation of drug-resistance putative composite transposons, and a plasmid fusion likely mediated by IS elements.

MATERIALS AND METHODS
Bacterial strains and culture conditions. All bacterial strains used in the study are listed in Table 3. All bacterial strains were grown at 37°C in Luria-Bertani (LB) medium supplemented with appropriate antibiotics (Sigma-Aldrich, UK) with concentrations as follows: chloramphenicol at 12.5 mg/mL, rifampicin at 20 mg/mL, ampicillin at 100 mg/mL, fusidic acid at 400 mg/mL, and tetracycline at 5 mg/mL.
Clinical isolates in this study were selected from a carbapenemase-producing Enterobacteriaceae (CPE) collection at the Norwegian National Advisory Unit on Detection of Antimicrobial Resistance (20). The whole-genome sequencing (WGS) data of these isolates (BioProject accession number PRJNA295003) were used to initially screen for strains that either did not contain tetracycline resistance genes or contained tetracycline resistance genes on chromosome-derived contigs by using ResFinder and mlplasmids (47,48). The numbers of plasmids, MGEs, and b-lactamase genes associated with plasmid-derived contigs were also determined by using Mobile Element Finder, PlasmidFinder, and mlplasmids (10,48,49) and were used as criteria to select 8 potential donors for the filter-mating experiments with our E. coli MDS Rif Fus::pBACpAK recipient (see below).
Preparation of E. coli MDS Rif Fus::pBACpAK recipient strain. For recipient cells, the E. coli MDS strain (Scarab Genomics, USA) was used, as it has been genetically modified to remove all mobile DNA and error-prone DNA polymerases (50), reducing the possibility of false positives from the transposition of MGEs from an E. coli host and de novo mutations within cI during screening.
E. coli MDS::pBACpAK was prepared by introducing a pBACpAK entrapment vector into E. coli MDS electrocompetent cells (Scarab Genomics, USA) through electroporation. Amounts of 50 mL of the electrocompetent cells and 10 ng of pBACpAK plasmid were mixed in a prechilled 1.5-mL microcentrifuge tube and transferred to a prechilled, 0.1-cm electroporation cuvette (Bio-Rad, UK). The cells were then electroporated, and 950 mL of prewarmed SOC medium (New England Biolabs, UK) was added into the cuvette. The cell mixture was transferred to a 50-mL tube and incubated in a 37°C shaker for 1 h. After the incubation, cells were grown on LB agar containing chloramphenicol and incubated overnight. The transformants were screened and checked for the presence of pBACpAK by performing cI-tet(A) PCR with cI-tetA-F1 and ERIS primers (Table S1).
To generate E. coli MDS Rif::pBACpAK, E. coli MDS::pBACpAK was subcultured in LB broth containing chloramphenicol (for selection of pBACpAK) and incubated overnight. An aliquot of 100 mL of the overnight culture was plated onto LB agar supplemented with 20 mg/mL rifampicin and incubated overnight. The colonies grown on the selective plates were subcultured onto another fresh rifampicin  (20). b Chl r , chloramphenicol resistance; Rif r , rifampicin resistance; Fus r , fusidic acid resistance; Amp r , ampicillin resistance.
selective plate to confirm their rifampicin resistance phenotype. E. coli MDS Rif Fus::pBACpAK was then generated from E. coli MDS Rif::pBACpAK with the same process but with LB agar supplemented with 400 mg/mL fusidic acid. Rifampicin and fusidic acid resistance in E. coli MDS Rif Fus::pBACpAK were confirmed by PCR amplification and sequencing of genes previously shown to be responsible for the resistance phenotypes and subsequently confirmed by WGS of E. coli MDS Rif Fus::pBACpAK transconjugants.
Filter mating between clinical isolate donors and E. coli MDS Rif Fus::pBACpAK recipient. The frequency of spontaneous mutation of E. coli MDS Rif Fus::pBACpAK exposed to tetracycline was determined by spreading an overnight culture of E. coli MDS Rif Fus::pBACpAK on 3 LB agar plates supplemented with rifampicin, fusidic acid, chloramphenicol, and tetracycline and incubating at 37°C for 3 days.
Filter mating was performed by following the protocol described previously (51). The donors (Enterobacteriaceae clinical isolates) ( Table 3) and the recipient (E. coli MDS Rif Fus::pBACpAK) were grown overnight in 5 mL LB broth supplemented with appropriate antibiotics in separate 50-mL tubes. Each overnight culture was subcultured into 10 mL of fresh LB broth with no antibiotics with an optical density at 600 nm (OD 600 ) of 0.1 and incubated at 37°C until mid-exponential phase (OD 600 of 0.5 to 0.6). The cells were centrifuged and resuspended in 500 mL of LB broth. The donor and recipient cells were then mixed together and 150 mL spread on a 0.45-mm-pore-size sterilized nitrocellulose filter (Sartorius, UK) on antibiotic-free LB agar plates. Control groups were also included by adding only the donor or recipient strain to filters. After 5 h, the filters were transferred into 50-mL tubes. Cells on the filters were resuspended in 1 mL of prewarmed LB broth by vortexing the tubes at high speed for 1 min. The cell suspension was spread onto plates containing LB agar supplemented with chloramphenicol, rifampicin, ampicillin, and fusidic acid (LB CRAF agar) to select for transconjugants. Ampicillin was used to select for the transfer of the b-lactamase-containing plasmid(s) to the recipient strain. The transconjugants were confirmed by subculturing on fresh selective LB CRAF agar plates and carrying out a cI-tet(A) colony PCR (cI-tetA-F1 and ERIS primers) to confirm that they were recipient cells (Table S1).
Screening for transconjugants with insertion of MGEs within pBACpAK. All transconjugants were subcultured into 5 mL of LB CRAF broth and incubated for 4 h in a 37°C shaker. An aliquot of 500 mL of culture was plated onto two plates of LB agar supplemented with chloramphenicol, rifampicin, ampicillin, fusidic acid, and tetracycline (LB CRAFT agar). One of them was incubated at 37°C, while the other one was incubated at room temperature. The 4-h culture was returned to the 37°C shaker overnight, and then 100 mL of the overnight culture was spread onto another two LB CRAFT agar plates and incubated at 37°C or room temperature separately. The overnight culture was also used to subculture into 5 mL of fresh LB CRAF broth and the same plating and subculture repeated for another 3 days. All plates were checked for colony growth every day for a week, and any resulting colonies were subcultured on fresh LB CRAFT agar to confirm the tetracycline resistance phenotype.
All confirmed tetracycline resistance transconjugants were screened for insertion of MGEs into the cI-tet(A) region of pBACpAK by colony PCR with cI-tetA-F1 and ERIS primers (Table S1) as described previously (15). The colony PCR was first performed with a standard PCR protocol using 2Â Biomix red (Bioline, UK) with an elongation time of 3 min to amplify up to 6 kb to initially rule out clones with mutations irrelevant in this study (point mutations, deletions, and small insertions). Clones that failed to amplify using the standard PCR were repeated with Q5 high-fidelity 2Â mastermix (New England Biolabs, UK) with a 10-min elongation time to amplify up to 20 kb. The amplicons with more than a 500bp increase in the size of the cI-tet(A) amplicon compared to a wild-type cI-tet(A) amplicon (1.35 kb) were sequenced by the Sanger sequencing service from Genewiz, Germany. BLASTN, BLASTX, and ISFinder were used to compare the sequences to nucleotide, protein, and IS element databases, respectively (52,53).
Genetic analysis of tetracycline-resistant transconjugants. Clones that failed to amplify a product with cI-tetA-F1 and ERIS primers with both standard and long colony PCR protocols were initially analyzed by extracting their plasmids and comparing their XhoI plasmid digestion pattern with the wildtype XhoI pBACpAK digestion pattern. WGS was performed by using MiSeq version 3 with 600 cycles (300-bp paired-end reads) at the Norwegian Sequencing Centre (Oslo University Hospital, Ullevål, Oslo, Norway). Genomic DNA was extracted from the bacterial pellet using the QIAcube automated station (Qiagen, Norway) following the QIAamp DNA mini-QIAcube kit protocol. DNA libraries were prepared using Nextera DNA flex tagmentation (Illumina).
The raw reads were processed with AfterQC version 0.9.7 to trim and filter low-quality reads (54), followed by de novo genome assembly with SPAdes 3.13.1 (55). The contigs containing pBACpAK were identified by using BLAST to compare the assembled contigs with pBACpAK sequences. Insertion of MGEs in chromosomal DNA of the E. coli recipient was checked by using breseq version 0.35.6 to map the filtered reads with the E. coli MDS reference genome (accession number AP012306) (56). The comparison of Tn7350-, Tn7351-, and Tn7359-containing pBACpAK sequences with their best match from BLASTN was performed with BLAST Ring Image Generator (BRIG) version 0.95 (57). The estimation of gene copy number was done by determining the number of filtered reads mapped to each gene with BWA version 0.7.17 and SAMtools version 1.11 (58,59) and normalized by dividing the read counts by the size of each gene. The copy numbers of each gene were calculated by dividing each normalized read count by the normalized read counts of the reference genes (the chloramphenicol resistance gene and repE for pBACpAK and the bla NDM-1 resistance gene and repA for the conjugative plasmid).
Data availability. Novel transposons were assigned the following Tn numbers by The Transposon Registry (43): Tn7350 (OK245453), Tn7351 (OK245454), and Tn7359 (accession number SAMN21542911). The WGS data were deposited at the National Center for Biotechnology Information (NCBI) with accession numbers SAMN21542910 to SAMN21542916.

SUPPLEMENTAL MATERIAL
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