- Research article
- Open Access
Multilocus variable-number tandem-repeat genotyping of Renibacterium salmoninarum, a bacterium causing bacterial kidney disease in salmonid fish
© Matejusova et al.; licensee BioMed Central Ltd. 2013
- Received: 26 April 2013
- Accepted: 15 November 2013
- Published: 6 December 2013
Bacterial kidney disease (BKD), caused by Renibacterium salmoninarum, is a bacterial disease of fish, which is both geographically widespread and difficult to control. Previously, application of various molecular typing methods has failed to reliably discriminate between R. salmoninarum isolates originating from different host species and geographic areas. The current study aimed to utilize multilocus variable number tandem repeats (VNTR) to investigate inter-strain variation of R. salmoninarum to establish whether host-specific populations exist in Atlantic salmon and rainbow trout respectively. Such information would be valuable in risk assessment of transmission of R. salmoninarum in a multispecies aquaculture environment.
The present analysis utilizing sixteen VNTRs distinguished 17 different haplotypes amongst 41 R. salmoninarum isolates originating from Atlantic salmon and rainbow trout in Scotland, Norway and the US. The VNTR typing system revealed two well supported groups of R. salmoninarum haplotypes. The first group included R. salmoninarum isolates originating from both Atlantic salmon and rainbow trout circulating in Scottish and Norwegian aquaculture, in addition to the type strain ATCC33209T originating from Chinook salmon in North America. The second group comprised isolates found exclusively in Atlantic salmon, of mainly wild origin, including isolates NCIB1114 and NCIB1116 associated with the original Dee disease in Scotland.
The present study confirmed that VNTR analysis can be successfully applied to discriminate R. salmoninarum strains. There was no clear distinction between isolates originating from Atlantic salmon and rainbow trout as several haplotypes in group 1 clustered together R. salmoninarum isolates from both species. These findings indicate a potential exchange of pathogens between Atlantic salmon and rainbow trout in Scottish and Norwegian aquaculture during the last 20 years. In a scenario of expansion of rainbow trout farming into the marine environment, appropriate biosecurity measures to minimize disease occurrence are advised. The present results also suggest that R. salmoninarum isolates circulating in European aquaculture over the last 20 years are genetically distant to the wild strains originally causing BKD in the rivers Dee and Spey.
- Bacterial kidney disease
Renibacterium salmoninarum is a Gram-positive bacterium, belonging to the Micrococcus-Arthrobacter subgroup of the actinomycetes [2–4] and the causative agent of bacterial kidney disease (BKD), a chronic systemic disease of salmonid fish in both marine and freshwater environments . Bacterial kidney disease was first reported in wild Atlantic salmon (Salmo salar) in the Rivers Dee and Spey (Scotland, United Kingdom) in 1930 [6, 7] and similar disease signs were reported from North America in 1935 in brook trout (Salvelinus fontinalis), brown trout (Salmo trutta) and rainbow trout (Oncorhynchus mykiss) [8, 9]. Renibacterium salmoninarum has an intracellular lifecycle and transmission, both horizontally through contact with infected fish/water or vertically inside fish ova, has been confirmed in many salmonid species [10–14]. Recent epidemiological studies have identified an association between the spread of BKD and anthropogenic activities [15, 16].
Bacterial kidney disease is geographically widespread and has been reported from most countries where salmonid fish are cultured or naturally occurring. The disease is known to have the potential to cause high mortalities [17, 18] and represents one of the most difficult bacterial diseases of fish to control due to its slow progression and lack of effective treatment. In Scotland, farmed Atlantic salmon and rainbow trout may be infected in both seawater and freshwater environments , although the contribution of wild fish to infection transmission is considered low .
Sensitive R. salmoninarum typing tools are required to improve BKD control through identification of sources of infection and transmission routes. Molecular typing methods, such as direct sequencing of the intergenic spacer (ITS1 and ITS) of ribosomal RNA and randomly amplified polymorphic DNA (RAPD) analysis [20–23], have shown a limited power to distinguish R. salmoninarum strains. Amplification of length polymorphisms in the tRNA intergenic spacer (tDNA-ILPs) has, however, offered improved discriminatory power with some potential for identification of R. salmoninarum isolates known to come from the same hatchery .
In Scotland, BKD and infection with R. salmoninarum are regulated under The Aquatic Animal Health (Scotland) Regulation 2009. From the available farm data, it appears that BKD persists longer on rainbow trout farms , compared with Atlantic salmon farms [16, 19]. To date, all typing systems have failed to distinguish between R. salmoninarum strains originating from Atlantic salmon and rainbow trout [20, 22, 23], suggesting that individual isolates may represent a risk to both host species. Confirmation of this, applying a more sensitive typing tool, would be beneficial, for example, in a scenario of an expansion of rainbow trout sea water aquaculture. Application of appropriate biosecurity measures could then be applied to minimise risk of pathogen transmission.
In recent years, multilocus variable number tandem repeat analysis, based on amplification of short repetitive DNA sequences, has been found to be a rapid and simple typing technique that enables differentiation of bacterial strains displaying otherwise low genomic variation. The method has been used to discriminate between closely related strains of various human pathogenic microorganisms such as Clostridium difficile, Bartonella henselae, or Streptococcus agalactiae as well as fish pathogenic species such as Francisella noatunensis. The primary purpose of this study was therefore to investigate the genetic variation in R. salmoninarum isolated from Atlantic salmon and rainbow trout farms in Scotland using multilocus variable number tandem repeat analysis (VNTR). Additional samples from other countries were also included in the present study to put any observed variation into context and identify whether the present VNTR typing scheme can distinguish between R. salmoninarum collected from different geographic areas.
Characterization of tandem repeat loci
Number of alleles and variation in repeat span per polymorphic locus
Marker locus name*
Number of alleles
Repeat number/span (bp)
Renibacterium salmoninarum isolates haplotype identified using multilocus tandem repeat sequencing
Country of origin
Environment (wild/farmed fish)
Data of isolation
MT1470, MT1511b, MT2119c, MT2622c
FW, SW (F)
MT452a, MT839, MT1351, MT1363, MT1880, MT2979, MT3277a, MT3314, MT3315b, MT3402, N4245, N6642, N6552d, N6553d, N6694, N6765, N6863e, N6864e
FW, SW (F)
FW, SW (F)
MT3106, MT3479, TERV
FW, SW (F)
Phylogenetic relationships among R. salmoninarumisolates inferred from VNTRs
Group 2 represents R. salmoninarum isolates obtained uniquely from Atlantic salmon originating from Scotland and Norway. These isolates differed from group 1 at loci BKD396 and BKD1935. A moderately supported cluster within group 2, comprising strains O-Q, represented isolates exclusively from wild Atlantic salmon, including the Dee disease isolates NCIMB 1114 and 1116 associated with first occurrence of BKD in Scotland.
The present VNTR typing scheme was also applied to investigate whether Scottish R. salmoninarum isolates can be distinguished from isolates originating from Norway. Within group 1, some association with country of origin was observed for haplotypes A, C, and G, uniquely obtained from Scottish aquaculture, while haplotype E represented R. salmoninarum from Norway. On the contrary, the most common haplotype B contained isolates obtained from aquaculture establishments in both countries.
The present study describes development and application of a VNTR typing system for R. salmoninarum, a bacterium affecting salmonid aquaculture worldwide and discusses the potential implications for disease management. In comparison to other genotyping methods used to study R. salmoninarum such as RAPD, tDNA-ILPs [20–23], multilocus VNTR typing offers a considerable improvement. Using a combination of sixteen VNTRs, 17 different haplotypes can be identified among 41 R. salmoninarum isolates. The discriminatory power of the present combined VNTR scheme was high, characterized by HGDI index of 0.81, indicating that two unrelated isolates will on 81% of occasions fall into different haplotypes. In contrast, no more than nine different tDNA-ILP profiles could be identified from a much larger collection of R. salmoninarum isolates . In addition, VNTR represents a more reproducible typing system in comparison to techniques relying on random amplification under low-stringency parameters and accurate data from individual isolates can readily be shared between different laboratories. Although the discriminatory power of VNTR when applied to R. salmoninarum is lower than has been achieved with some human pathogenic bacteria such as Bartonella or Streptococcus[26, 27], these later studies are based on significantly larger data sets usually gathered from wider geographic areas. If a larger R. salmoninarum data set becomes available in future, the VNTRs described in the present study should be applied to test its ability to trace disease outbreaks and connect individual infected farms with a source of infection.
The developed VNTR typing system separated the studied isolates into two well-supported groups. Group 1 clustered together 12 out of 17 R. salmoninarum haplotypes, including a wide range of isolates from Scotland, Norway and North America, from three different species of salmonid fish, spanning the period between 1974 and 2009. Several haplotypes of group 1 (B, D, E and G) comprised multiple isolates causing disease in both Atlantic salmon and rainbow trout, suggesting a relatively common historical transfer of the pathogen between these fish species. On the other hand, some association was found between rainbow trout and R. salmoninarum haplotype A and between Atlantic salmon and R. salmoninarum haplotypes C, F, H, I and L-Q. However, with the exception of haplotypes A and C, these haplotypes were represented by single isolations.
The present study concludes that using a data set of 41 isolates representing bacterium circulating in Scotland over a period of more than 20 years, there was no consistent division of R. salmoninarum isolates into two host specific populations. This result is consistent with the possibility that individual R. salmoninarum strains can infect both host species in environments where both species co-occur. The transfer of R. salmoninarum free stock to the marine environment could in theory eliminate disease transmission. However, the possibility that a carrier would be not detected, as a consequence of a potentially low infection prevalence and low diagnostic sensitivity of tests for asymptomatic stock, have to be considered . The spatial separation of marine rainbow trout and Atlantic salmon farms into separate disease management areas in marine environment, as described in , can further reduce the risk of pathogen transfer between host species.
All previous R. salmoninarum typing systems have failed to reliably discriminate between European and US isolates [20, 22, 23]. This study identified the type strain ATCC33209T originating from Oregon (US) as a unique strain (haplotype J) and its position within group 1 supports previous studies suggesting intercontinental spread of this pathogen related to anthropogenic activities such as movement of fish during expansion of the rainbow trout industry in Europe . The present genotyping system could, however, clearly separate R. salmoninarum strains M-Q (group 2), indicating an origin not associated with ATCC33209T. The majority of these strains were of wild origin and have not been reported in wild or farmed fish since their original description in the 1930s. The locus BKD1935 was previously described by  referred to as the Exact Tandem Repeat A (ETR-A). It was demonstrated that the ETR-A can successfully separate the wild-fish isolates such as NCIMB1114 and NCIMB1116 (tandem repeat 1) from the farmed isolates such as MT452 and MT1363 (tandem repeat 2). Further investigation on a larger data set, focusing on loci BKD396 and BKD1935, which are solely responsible for differentiation between groups 1 and 2, might bring more insight into a relationship between farmed and wild R. salmoninarum strains and confirm the origin of R. salmoninarum in Scottish aquaculture.
Cross-species infectivity of R. salmoninarum strains also has wider implications for marine ecosystems; including possible transfer of R. salmoninarum from farmed to wild fish or vice versa. In Scotland, recent studies provided evidence of a relatively low prevalence of R. salmoninarum in wild fish captured in close proximity to farms, suggesting that the transmission of this pathogen between wild and farmed fish is limited [16, 31]. However, this scenario might not apply for other regions or countries such as England or Norway  and the described VNTR typing system can be utilized to identify and understand farmed and wild fish interactions in terms of R. salmoninarum transmission if a larger data set should become available.
Preparation of Renibacterium isolates and DNA extraction
Twenty-five R. salmoninarum isolates from confirmed disease outbreaks on Scottish farms were selected for this study. Number and selection of Scottish R. salmoninarum isolates represents the geographic range, habitat, frequency of disease outbreaks in the salmonid aquaculture sector, supply of fish stock and takes into account difficulties of bacteria culturing from asymptomatic fish and resuscitation of archived material. In addition, 14 Norwegian isolates and two isolates derived from the first successful cultivation of R. salmoninarum from the River Dee  were included. Isolate details including country of origin, date of isolation, host species and environment are summarized in Additional file 2: Table S2.
For Scottish strains, lyophilised cultures were resuscitated onto Mueller-Hinton L-cysteine agar (MHCA) containing polymyxin-B-sulphate, D-cycloserine, oxolinic acid and cycloheximide and incubated at 15°C for several weeks to allow growth. Suspensions of culture in 0.85% sterile saline were made to a turbidity of McFarland 1, serially diluted to 10-4 in sterile saline and 0.1 ml volume of the dilutions spread onto MHCA to achieve single colony purification. The Gram appearance and purity of individual colonies was confirmed before sub-culturing onto fresh MHCA and additional checks for purity and identity (API ZYM, ELISA using the Bios Chile kit) were carried out. At 4–6 weeks, each agar culture was scraped from the plate and suspended in sterile saline before pelleting at 2,400 × g. Genomic DNA was extracted from bacterial cultures using the MagAttract DNA mini M48 kit (Qiagen) and quantified using a ND-1000 Nanodrop Spectrophotometer (NanoDrop Technologies). For Norwegian strains, cryo-preserved isolates (−80°C) were resuscitated on kidney disease (KD) medium  followed by KD broth culture to an approximate turbidity of McFarland 1 prior to extraction of genomic DNA using the Gentra Puregene cell kit (Qiagen).
Tandem repeat identification and amplification
The complete genome sequence of R. salmoninarum reference strain ATCC33209T (Accession number NC_010168) was utilized to identify the repetitive DNA sequence regions using the Microorganisms Tandem Repeat Database (http://minisatellites.u-psud.fr)  and Tandem Repeats Finder (TRF version 4.03) (http://tandem.bu.edu) . Tandem repeats with at least two repeat units per locus and a repeat unit length of between 4 and 80 bp were selected for further analysis.
Primers for amplification of each locus were designed using OligoPerfect™ Designer (http://tool.invitrogen.com) and their specificity tested using BLAST (blastn) searches. Loci were amplified using the primer pairs listed in Additional file 1: Table S1. Each reaction consisted of 1 × PCR buffer (Bioline), 1.5 mM MgCl2, 200 μM dNTPs, 10 μM of each primer, 1 U BioTaq (Bioline) in a final volume of 20 μl. The cycling conditions were 35 cycles of: 95°C for 1 min, 50 or 55°C (see Additional file 1: Table S1) for 1 min, 72°C for 1 min, followed by a final elongation step of 72°C for 5 min. Amplified products were visualized on a 1% ethidium bromide-stained agarose gel (Invitrogen) and purified using ExoSAP IT or ExoStar 1-Step (GE Healthcare). Approximately 15 ng of purified PCR product was sequenced, utilising the same primers as in the amplification reaction using the GenomeLab DTCS Quick Start kit (Beckman Coulter) and the automated CEQ8800 DNA Sequencer (Beckman Coulter).
Tandem repeat analysis
Each type (size) of repeat, identified by sequencing, at each locus was assigned a unique allele identifier. Data were imported from a Microsoft Office Excel 2003 generated comma-separated-value data file and analysed using version 2.14.0 of the R statistical computing environment . The permutations of alleles across 16 polymorphic loci were used to define distinct haplotypes.
Gross differences between haplotypes (identified using 16 polymorphic loci) were measured with the Hamming distance  and used to construct an unrooted neighbor-joining tree using version 1.6-0 of the supplementary R package phangorn . To simplify interpretation of results, haplotypes were named A-Q on the basis of their respective position in the phylogenetic tree. Support for clusters was evaluated using the bootstrap test of phylogeny (1000 repeats) and clusters with values of less than 50% collapsed . The clustering of very closely related haplotypes, defined as those differing at only one locus, was examined using eBURST v 3.0 . Homoplasy and extent of recombination events were investigated using Splits Decomposition, as implemented in Splitstree v 4 , by depicting conflicting signals in the data caused by recombination events. The resulting network was consistent with the phylogenetic analysis, and no reticulation was evident, indicating that the evolutionary relationships have not been affected by recombination or homoplasy (data not shown).
The discriminatory power of a typing system was estimated using the Hunter-Gaston discriminatory index HGDI . The index provides a probability that two randomly sampled unrelated isolates will be placed into different typing groups/haplotypes. The minimum number of loci required to distinguish all the strains was determined.
The authors would like to thank Drs. Sandy G. Murray and David Bruno (Marine Scotland Science, Aberdeen, United Kingdom) for valuable comments which greatly improved the manuscript draft.
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