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Development of a Multiplex-PCR probe system for the proper identification of Klebsiella variicola Microbial genetics, genomics and proteomics

BMC Microbiology (2015) 15(1)
DOI: 10.1186/s12866-015-0396-6
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Abstract

Background: Klebsiella variicola was very recently described as a new bacterial species and is very closely related to Klebsiella pneumoniae; in fact, K. variicola isolates were first identified as K. pneumoniae. Therefore, it might be the case that some isolates, which were initially classified as K. pneumoniae, are actually K. variicola. The aim of this study was to devise a multiplex-PCR probe that can differentiate isolates from these sister species. Result: This work describes the development of a multiplex-PCR method to identify K. variicola. This development was based on sequencing a K. variicola clinical isolate (801) and comparing it to other K. variicola and K. pneumoniae genomes. The phylogenetic analysis showed that K. variicola isolates form a monophyletic group that is well differentiated from K. pneumoniae. Notably, the isolate K. pneumoniae 342 and K. pneumoniae KP5-1 might have been misclassified because in our analysis, both clustered with K. variicola isolates rather than with K. pneumoniae. The multiplex-PCR (M-PCR-1 to 3) probe system could identify K. variicola with high accuracy using the shared unique genes of K. variicola and K. pneumoniae genomes, respectively. M-PCR-1 was used to assay a collection of multidrug-resistant (503) and antimicrobial-sensitive (557) K. pneumoniae clinical isolates. We found K. variicola with a prevalence of 2.1% (23/1,060), of them a 56.5% (13/23) of the isolates were multidrug resistant, and 43.5% (10/23) of the isolates were antimicrobial sensitive. The phylogenetic analysis of rpoB of K. variicola-positive isolates identified by multiplex-PCR support the correct identification and differentiation of K. variicola from K. pneumoniae clinical isolates. Conclusions: This multiplex-PCR provides the means to reliably identify and genotype K. variicola. This tool could be very helpful for clinical, epidemiological, and population genetics studies of this species. A low but significant prevalence of K. variicola isolates was found, implying that misclassification had occurred previously. We believe that our multiplex-PCR assay could be of paramount importance to understand the population dynamics of K. variicola in both clinical and environmental settings.

Figures

  • Table 1 Amplification conditions, oligonucleotide combinations, sequence and amplification fragment of multiplex-PCR for K. variicola identification
  • Figure 1 The maximum-likelihood gene phylogenies of K. variicola and K. pneumoniae. Bootstrapping of the gene tree was implemented to evaluate the support of the K. variicola and K. pneumoniae groups. The numbers next to the nodes are the bootstrap values, and the length of the branches has no meaning.
  • Figure 2 Amplification by PCR of shared unique genes to K. variicola variicola using the genomes of control strains such as K. pneumoniae ATCC ATCC 33531 and K. oxytoca ATCC 49134. B) Amplification of shared unique ge above. Lane 1, ϕX174/Hae III; Lane 2, mtnC gene (KmtnC-F and -R oligonucle oligonucleotides); Lane 4, thiopurine S-methyltransferase gene (KV1000-F and -R oligonucleotides); Lanes 1 to 6, rpoB gene (CM7 and rpoB-M) in co Lane 7, rpoB oligonuclotides without DNA (CM7 and rpoB-M); Lane 8, Transfer gene (KP888-F and R oligonucleotides) (Table 1).
  • Figure 3 Multiplex-PCR amplification of oligonucleotides combinations used for identification of K. variicola. A) Lane 1, molecular weight 1 kb; Lane 2, oligonucleotide combination named M-PCR-1 (KV770-F/KV770-R, KP888-F/KP888-R and KmtnC-F/KmtnC-R); Lane 3, oligonucleotide combination named M-PCR-2 (KV1615-F/KV1615-R, KP878-F/KP878-R and KmtnC-F/KmtnC-R); Lane 4, oligonucleotide combination named M-PCR-3 (KV1000-F/KV1000-F, KP888-F/KP888-R and KmtnC-F/KmtnC-R) (Table 1). B) M-PCR-1 assayed on environmental endophytic K. variicola isolates. Lane 1, molecular weight ΦX174 DNA-Hae III; Lane 2, K. pneumoniae ATCC 13883 and K. variicola 801, DNA’s combination; Lane 3, K. variicola T29A; Lane 4, K. variicola 6A2; Lane 5, K. variicola CFNE 2006; Lane 6, K. variicola 3; Lane 7, K. variicola F2R9; Lane 8, K. variicola VI; Lane 9, negative control (without DNA).
  • Table 2 Characteristics of endophytic and clinical K. variicola isolates
  • Figure 4 The maximum-likelihood phylogeny of the rpoB sequences. The tree was rooted with the sequences from Escherichia coli K-12 MG1655 and Salmonella enterica Ty21. To evaluate the support of the nodes, a bootstrap analysis of 100 replicates was conducted. For clarity, only the bootstrap values for the main groups are shown. The scale bar represents substitutions per site.
  • Figure 5 PFGE and dendrogram analysis that includes K. variicola and and clinical), species, hospital and city, origin of sample, PFGE pattern and

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Garza-Ramos, U., Silva-Sánchez, J., Martínez-Romero, E., Tinoco, P., Pina-Gonzales, M., Barrios, H., … Tellez-Sosa, J. (2015). Development of a Multiplex-PCR probe system for the proper identification of Klebsiella variicola Microbial genetics, genomics and proteomics. BMC Microbiology, 15(1). https://doi.org/10.1186/s12866-015-0396-6

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