Table of contents
1. Introduction
2. Bacterial fish pathogens
3. Isolation of fish pathogens: the culture-dependent approach
4. Approaches to characterization
4.1 Phenotype
4.2 Immunological methods
4.3 Chemotaxonomy
4.3.1
Lactococccus piscium
4.3.2
Mycobacterium neoarum
4.3.3
Nocardia
4.3.4
Renibacterium salmoninarum
4.4 Molecular/genetic methods
5. New species of fish pathogens recognized by 16S rRNA sequencing
5.1 New and uncultured fish pathogens: “Candidatus”
6. Taxonomic developments associated with specific bacterial fish pathogens
6.1 Motile aeromonas septicaemia
6.2
Aeromonas salmonicida
6.3 Enteric redmouth (ERM)
6.4 Vibriosis
7. The role of phylogenetics in bacterial fish pathology
8. Conclusions
9. References
1. Introduction
"What's in a name?" (William Shakespeare; Romeo and Juliet)
The Swedish botanist Carl Linnaeus (1707-1778), who was also known as Carolus Linnaeus and Carl von Linné, is undoubtedly the Father of Taxonomy, and was responsible for developing a system for naming and ranking living organisms. His lasting contribution was the development of a simplified naming system in Latin with consistency across all living organisms, i.e. the binomial system, in which each organism has a unique two-word name - incorporating genus and species. A simplistic view is that Linnaeus made order out of chaos. Yet, for Linnaeus and his contemporaries, the process was comparatively easy, and involved only large organisms, which were clearly visible to the naked eye (= macro-organisms) and easily seen morphological characteristics (= a category of phenotypic characters). Thus, these early classifications (= the process of arranging organisms into groups) were based on limited but easily visible data, and the outcomes were largely obvious, for example a dog is notably different from a horse and would therefore belong in separate species.
The founding father of microbiology, the Dutch textile merchant and lens maker, Antonie van Leeuwenhoek (1632-1723), observed small organisms initially from the proximity of his teeth (= bacteria and protozoa?), and these entities were termed "animalcules", which he wrote about in a letter to the Royal Society of London in 1676. His careful illustrations suggested morphological variation between the cells. Yet, another two centuries were to pass before serious attempts at naming and ordering bacteria started. Thus, bacterial taxonomy has progressed from the simplistic approach involving a small number of readily observable characteristics, such as morphology as deduced from observation using light microscopes, to the modern applications of molecular biology. With improvements in knowledge, there have been refinements in taxonomic processes and an increase in reliability. It should be remembered that taxonomy (= the theory of classification, nomenclature and identification) is a man-made process, i.e. the organisms included in any classification have not chosen to be placed in the groups that have been created by human beings. Nevertheless if done properly, taxonomy has value in:
• Understanding biodiversity, namely the range of organisms in a given habitat
• Communication between scientists, thus enabling exchange of information about similar organisms
• Cataloguing information - the name is the key to a catalogue of information about the organism
• Enabling identification, such that new isolates may be readily and reliably identified
• Providing an insight into evolutionary pathways (= phylogenetics).
To be effective, taxonomy should be
- based on a high information content
- reproducible, and
- stable,
otherwise confusion will surely result.
Since the start of bacterial taxonomic processes in the nineteenth century, there has been a progression in the type of information used in the procedure. It may be argued that early bacteriologists had considerable taxonomic insight judging from the conclusions reached from the comparatively simple data that were available. However, taxonomy is a dynamic science, with new developments/methods being incorporated into processes including the descriptions of bacterial species. Since the 1950 s, bacterial taxonomy has evolved rationally, encompassing numerical methods
1
2
, chemotaxonomy (e.g.
3
4
), and molecular techniques
5
. Taxonomy has progressed from a highly artificial process involving limited amounts of phenotypic data to the recognition of more natural relationships between organisms, based on comparatively large amounts of varied and reliable data covering multiple aspects of the biology of an organism, and including phenotypic, chemotaxonomic, genotypic and phylogenetic date, i.e. a polyphasic approach. However, the current dominance of 16S rRNA gene sequencing although revolutionising some aspects of bacterial classification needs to be treated cautiously as overreliance on the approach may lead to erroneous conclusions
5
. Nevertheless, it is apparent that sequencing methods are instrumental with the explosion of new species names, which have greeted the arrival of the twenty-first century. Whereas, the information content of many of the new species descriptions is generally high, an unwelcome trend is that many new taxa (= taxonomic groups) are described solely after the study of only single strains. Therefore, the diversity/variability within the new taxon cannot be adequately assessed. Also, it is impossible to determine whether a single strain is effectively an outlier or a median representative of the group (in future years, will it be regarded as typical or atypical of the group?). However, taxonomy is often ignored by many microbiologists in other specialisms, and there may well be concern that basic principles could be forgotten, e.g. is the purity and authenticity of cultures always verified before use? Where culturing is not possible, there is the possibility of analyzing the nucleic acids, determining species composition, and even proposing new taxa, i.e. by the use of culture-independent approaches.
4. Approaches to characterization
4.1 Phenotype
Traditionally, bacteria were characterized phenotypically, and undoubtedly for some groups, e.g. the Enterobacteriaceae, a wealth of knowledge emerged particularly from the 1950's onwards. Currently, emphasis on phenotype has declined with a concomitant move towards molecular-based approaches. Nevertheless, phenotypic data have a role in polyphasic studies whereby many facets of the biology of an organism are studied
14
. Phenotyping leads the way with diagnoses worldwide; emphasis often being placed on commercial kits and the use of manufacturer's probabilistic databases to achieve an acceptable identification. Although the approach has standardized diagnoses, the weakness is that most identification systems have been developed for medically important bacteria that grow within 24-48 h at 35-37°C. Consequently, the reliability of these kits for use with fish pathogens which need lower incubation temperatures for longer periods needs to be questioned
6
15
. In particular, the API 20E system includes the use of sugar fermentation reactions, which may be influenced by the presence of plasmids
6
. Moreover, there may be confusion over the interpretation of the profiles. For example, some of the profiles of A. hydrophila are similar to those of A. allosaccharophila and A. sobria; Yersinia ruckeri may be confused with Hafnia alvei; moreover Tenacibaculum maritimum and Pseudomonas anguilliseptica are indistinguishable by API 20E
6
. Problems may result when data from rapid commercial kits are used in conjunction with conventional diagnostic schemes, which have been developed for traditional and often laborious phenotypic characters. Also, some of the traditional tests, e.g. the Voges Proskauer reaction, are not noted for their reproducibility and may introduce errors into the taxonomic process and lead to mis-identification
16
.
Undoubtedly, selective media have proved useful for the recovery of some fish pathogens, with an example including selective kidney disease medium (SKDM) for Renibacterium salmoninarum
17
. However, selective media are only available for a minority of all fish pathogens, therefore recovery is dependent on more general culturing methods. Specially developed diagnostic procedures have aided identification of some group, e.g. the glucose motility deep cultures have benefitted the recovery and identification of V. anguillarum
18
.
4.2 Immunological methods
The development and availability of standardized immunological (antibodies and kits) reagents have improved diagnoses considerably
6
19
20
, and enhanced the reliability of methods for the detection of pathogens, including Mycobacterium spp., Photobacterium damselae subsp. piscicida
21
, Piscirickettsia salmonis
22
, R. salmoninarum
23
and Streptococcus iniae
24
. Tentative diagnoses, including of asymptomatic infections, may result from use of monospecific polyclonal or monoclonal antibodies in a range of antibody-based procedures, including the indirect fluorescent antibody test (iFAT), whole-cell (slide) agglutination, precipitin reactions, complement fixation, immunodiffusion, antibody-coated latex particles, co-agglutination using antibody-coated staphylococcal cells, passive haemagglutination, immuno-India ink technique (Geck) or enzyme linked immunosorbent assay (ELISA; reviewed by
25
), the latter of which may also be used for serology, i.e. detecting antibodies in the host to specific pathogens
26
. Antibody-based methods are used effectively for detecting exposure to fish viruses, such as Koi herpes virus
27
, but bacterial pathogens pose a more complicated picture with cross reactivities likely unless specific known molecules/antigens are used to coat the ELISA plates rather than whole pathogens
19
. Techniques are often sensitive, specific, rapid and reliable, and in some cases may be used in the field
6
. This is in marked contrast to molecular biology, which may be much slower and relies on specialist, well equipped laboratories.
4.3 Chemotaxonomy
Chemotaxonomy involves the investigation of chemical constituents of bacteria, and is particularly useful for the study of Gram-positive bacteria. The molecules studied include fatty acids, polar lipids, lipopolysaccharide (nature of the chain length of the fatty acid and the sugar in the Lipid A moiety;
28
), menaquinones, naphthoquinones, ubiquinones, mycolic acids, peptidoglycan, polyamines, teichoic and teichuronic acids and isoprenoid quinones
29
. Mycolic acids, which are useful taxonomic markers, are present in Gram-positive bacteria with high G+C ratios of their DNA
4
, and have been reported for a range of fish pathogens, including Mycobacterium chelonei subsp. piscarium
3
and M. shottsii
30
. The length of the mycolate side chain has been correlated to 16S rRNA gene sequence homology
31
. Specific examples for which reliable chemotaxonomic data exist for Gram-positive bacterial fish pathogens are detailed below:
4.3.1 Lactococccus piscium
The long chain cellular fatty acids of Lactococcus piscium were reported to be straight chain saturated, mono-unsaturated and cyclopropane-ring types. The major acids corresponded to hexadecanoic acid, ∆ 11-octadecanoic acid and ∆ 11-methylenoctadecanoic acid
32
.
4.3.2 Mycobacterium neoarum
The cell wall chemotype has been given as IVA, with glycolated muramic acids, mycolic acids and MK-9, as the predominant isoprenoid quinone, being present
33
.
4.3.3 Nocardia
Nocardia salmonicida contains LL-diaminopimelic acid (DAP) and glycine but not meso-DAP, arabinose or galactose in the cell wall (i.e. Type I). The major cellular fatty acids are hexdecanoic, octadecanoic, octadecanoic and 10-methyloctadecanoic acid
34
.
N. seriolae contains meso-diaminopimelic acid, arabinose and galactose, indicative of chemotype IVA. Mycolic acids containing 44-58 carbon atoms are present. The cellular fatty acids are dominated by n-C16:0, n-C16:1 and n-C18:1; 10-methyl-C19:0 is also present as a major component in some isolates. The predominant isoprenoid quinone is tetrahydrogenated menaquinone with eight isoprene units
34
.
4.3.4 Renibacterium salmoninarum
Chemotaxonomic traits of R. salmoninarum have been highlighted in part because of the comparative difficulty with obtaining conventional phenotypic test results. Thus, the cell wall peptidoglycan was deduced to contain D-alanine, D-glutamic acid, glycine and lysine as the diamino acids
35
. The principal cell wall sugar was glucose, although arabinose, mannose and rhamnose were also present; mycolic acids were absent
36
. Methyl-branched fatty acids form > 92% of the total fatty acid component of the cells, with 12-methyltetradecanoic (anteiso-C15), 13-methyldecanoic (iso-C15) and 14-methylhexadecanoic (anteiso-C17) as the major components. Straight chain fatty acids generally account for 1% of the total fatty acids, and unsaturated fatty acids are not detected at all. Over 81% of the total fatty acids are composed of the lower melting point anteiso acids, which may contribute to membrane fluidity at low temperatures. Unsaturated menaquinones with nine isoprene units are present. All strains contain diphosphatydylglycerol, 2 major and 6 or 7 minor glycolipids and two unidentified minor phospholipids
37
.
4.4 Molecular/genetic methods
Molecular/genetic methods involving 16S rRNA gene sequencing
38
, reverse transcriptase-sequencing
39
40
and polymerase chain reaction (PCR)-based gene sequencing
41
have been useful additions to the armoury of techniques applicable to bacterial taxonomy
29
31
. DNA hybridization, which is regarded as the "gold standard" for demonstrating the presence or absence of new species, was introduced into bacterial taxonomy during the 1960s (e.g.
42
). Genotypic classification involving sequencing of the 16S and 23S RNA genes (the latter is less popular) is regarded as the definitive standard for determining phylogenetic relationships of bacteria
29
38
. In particular, the genes are regarded as having all the attributes of useful, relevant and stable biological markers being present and homologous in all bacteria. Also, they are not prone to the effects of gene transfer
29
. Yet, the exact homology values have a profound effect on interpretation of the outputs. Thus, homology values of ≤ 98.7% (97% according to
31
) indicates membership of different species, and this correlates well with DNA hybridization results. Yet, occasionally higher homology values may be attributed to distinct species groupings
43
. By themselves, 16S rRNA gene sequences are insufficient to describe a new species, but may be used indicatively and in conjunction with DNA:DNA hybridization
31
. However, sequencing has permitted the recognition of new variants. For example, sequencing revealed a new variant among Israeli isolates of Streptococcus iniae
44
. Moreover, 16S rRNA cataloguing has been useful in providing information about the position of species in existing classifications. Thus, small-subunit rRNA sequencing and DNA:DNA hybridization revealed that Pasteurella piscicida was related to Photobacterium damsela leading to the proposal that the pathogen be re-classified as Ph. damsela(e) subsp. piscicida
45
. Furthermore, R. salmoninarum was deduced to be a member of the actinomycete subdivision, being related to Arthrobacter, Brevibacterium, Cellulomonas, Jonesia, Micrococcus, Promicromonospora, Stomatococcus and Terrabacter
46
47
. The evolutionary relationship of R. salmoninarum to Arthrobacter was reinforced as the result of genome sequencing, which suggested that the genome of the former had been reduced significantly since its divergence from a common ancestor
48
.
Nucleic acid fingerprinting methods, including amplified fragment-length polymorphism PCR (AFLP), pulsed field gel electrophoresis (PFGE), random amplified polymorphic DNA (RAPD), rep-PCR (repetitive element primed PCR), REP-PCR (repetitive extragenic palindromic-PCR), ERIC-PCR (enterobacterial repetitive intergenic consensus sequences-PCR), BOX-PCR (derived from the boxA element) and ribotyping, provide information at or below the subspecies level
31
. Of these, AFLP and ribotyping are extremely useful and standardized.
It is unfortunate that with the increasing use of molecular methods, the description of bacterial groups has been often met with the use of minimal phenotypic data, which causes problems for diagnostics especially in laboratories, which are not equipped for molecular biology
6
. In these situations where distinguishing phenotypic feature have not been or could not be provided then the species should be referred to as a geno[mo]species. Nevertheless, molecular methods have revolutionized taxonomy, and led to the description of an increasing number of new taxa. The methodologies may be culture-independent, allowing for the study of uncultured organisms but there are issues with genomic fluidity
29
. "Candidatus" describes uncultured prokaryotes for which phylogenetic relationships have been determined, and authenticity confirmed by methods such as in situ probing
29
.
Sequencing of the 16S rDNA is becoming an accepted procedure for the identification of fish pathogens, for example V. harveyi
49
and confirming its synonymy with V. carchariae
9
10
, and has been instrumental in the recognition of new pathogens, including Streptococcus dysgalactiae
50
, S. parauberis (previously recognised as S. uberis genotype II;
51
) and Vagococcus salmoninarum
8
52
, and confirmed the presence of Lactococcus garvieae in Taiwan
53
.
DNA:DNA and RNA:DNA hybridization, 16S RNA cataloguing, and 5S and 16S rRNA sequencing techniques have been used with increasing regularity and success. A review of PCR with emphasis on validation of the techniques and problems with diagnosis has been published
54
. PCR has been used successfully to identify hard-to-isolate fish pathogens, such as Mycobacterium spp. in sea bass (Dicentrarchus labrax)
55
and M. chelonei in a cichlid oscar (Astronotus ocellatus)
56
. Moreover, PCR has been useful with distinguishing different species from within the same genus, such as Lactococcus garvieae from L. lactis
57
, from related genera, i.e. L. garvieae, S. difficilis, S. iniae and S. parauberis
58
, and with an admirable level of specificity
59
.
The sensitivity of PCR is clearly a positive attribute particularly with slow growing and/or nutritionally fastidious pathogens that are otherwise difficult to study in the laboratory. Of relevance, a PCR was developed
60
61
, which detected only 22 cells of R. salmoninarum; a sensitivity of 10 cells was reported by others
62
. Similarly, PCR detected only 102 colony forming units (CFU) of N. seriolae in yellowtail
63
.
A recent development is multi locus sequence analysis (MLSA), which permits the genotypic examination of micro-organisms by comparison of the sequences of multiple, i.e. 12 or more, house-keeping genes. The benefit of using multiple genes is that the outputs are more informative and less likely to generate results that are distorted by recombination of single loci
29
. The resulting phylogenetic trees are capable of recognizing deeply branching clusters and permit the delineation of groups within a species or genus
64
.
5. New species of fish pathogens recognized by 16S rRNA sequencing
16S rRNA sequencing has helped the description of fish pathogens where phenotypic characterization alone does not permit their incorporation in classifications. For example, a new disease of Atlantic salmon (Salmo salar) was linked to the Streptobacillus moniliformis and the fusobacteria group on the basis of sequence homology; biochemical traits did not permit identification
65
. The newly described cause of a mycobacteriosis in Chesapeake Bay (USA) striped bass (Morone saxatilis) was equated to a new species, M. shottsii, with confirmation by 16S rRNA sequence homology in which the pathogen was linked most closely to M. marinum and M. ulcerans (similarity = 99.2%)
30
. In one study, M. gordonae was identified by 16S rRNA sequencing
66
. Furthermore, phylogenetic analysis based on 16S rRNA gene sequencing together with partial sequences from the 65 kDa heat-shock protein (hsp65) and the beta-subunit of the bacterial RNA polymerase (rpoB) genes and the 16S-23S internal transcribed spacer 1 (ITS 1) region named other novel mycobacteria as M. stomatepiae and M. barombii
67
.
During an examination of 16S rRNA sequences, two isolates of motile aeromonads from diseased elvers in Spain were described as a new species, Aeromonas allosaccharophila
68
, albeit phenotypically heterogeneous
69
. This heterogenicity has caused problems for reliable phenotypic-based diagnoses.
Francisella became recognized as the cause of a new disease of Atlantic cod (Gadus morhua) in Norway in which the affected fish displayed white granuloma in the viscera and skin. Isolates were recovered, and determined to possess the key phenotypic characters of Francisella, viz. non-motile, strictly aerobic Gram-negative intracellular coccobacilli which produced H2S from cysteine-containing media
70
. 16S rRNA sequencing revealed a 99.17% homology to Francisella philomiragia
71
, although a slightly higher value of 99.3% was published
70
with the proposal for a new subspecies, i.e. Francisella philomiragia subsp. noatunensis, to accommodate the organisms. There was 92.2-99.0% homology with Francisella philomiragia housekeeping genes, groEL, shdA, rpoB, rpoA, pgm and atpA. A DNA:DNA hybridization of 68% was recorded between the fish pathogen and Francisella philomiragia
70
.
Pasteurella skyensis was recovered from diseased Atlantic salmon in Scotland, linked to the family Pasteurellaceae by phenotypic analysis, and elevated to a new species largely as a result of 16S rRNA sequencing that identified the closest neighbour as Pasteurella phocoenarum (homology = 97.1%;
72
).
Piscirickettsia salmonis was named to accommodate isolates from diseased salmon in Chile, of which LF-89 was studied in detail
73
with 16S rRNA conforming to the gamma subdivision of the Proteobacteria with similarities to the family Rickettsiales, and in particular Wolbachia persica (similarity = 86.3%) and Coxiella burnetii (similarity = 87.5%) more than to representatives of Ehrlichia, Rickettsia or Rochalimaea leading to the description of a new genus and species
73
. Other rickettsias not conforming exactly with Piscirickettia salmonis have been described. For example, an organism recovered from white sea bass (Atractascion nobilis) was reported to have a 96.3-98.7% 16S rDNA homology with Piscirickettsia salmonis
74
, which was considered by the authors to be too low for a confirmed identity. A Tasmanian isolate from Atlantic salmon was distinct from Piscirickettsia in terms of sequence alignment of the 16S rRNA, and for the present regarded as a rickettsial-like organism (RLO;
75
).
Pseudomonas plecoglossicida, the causal agent of bacterial ascites of ayu (Plecoglossus altivelis), was described as a new species as a result of 16S rRNA gene sequence analysis confirming distinctiveness from P. putida biovar A. DNA:DNA hybridization confirmed the isolates to be a new centre of variation insofar as < 50% homology was recorded with other pseudomonads, including P. putida
76
.
Streptococcus phocae was recognized as a cause of systemic disease in Atlantic salmon farmed in Chile. Phenotypic testing linked the pathogen with the streptococci, notably Gemella, but analysis of 16S rRNA genes provided a link to S. phocae
77
.
Tenacibaculum soleae was recovered from diseased sole (Solea senegalensis) in Spain, and confirmed as a new species largely on account of 16S rRNA homology values of 94.8-96.7% with other members of the genus
78
.
Two groups of bacteria were recovered from Atlantic salmon with winter ulcer disease/syndrome
79
, of which one cluster was found to be closest to Moritella marina (43% re-association by DNA:DNA hybridization), and was named as V. viscosus. By 16S rDNA sequencing, the closest match was with Moritella
79
and M. marina (99.1% sequence homology) so that the organism was re-classified to Moritella, but as a new species, as M. viscosa
80
, despite the high sequence homology
29
. Separately, 19 Icelandic and one Norwegian isolate from shallow skin lesions on Atlantic salmon, and the type strain of V. marinus NCIMB 1144 were identified as V. marinus after an examination of phenotypic data and analyses by numerical taxonomy
81
. On the basis of 16S rRNA sequencing, the species was transferred to Moritella as M. marina
82
.
5.1 New and uncultured fish pathogens: "Candidatus"
Molecular techniques have permitted the recognition of uncultured pathogens belonging to new groupings for which the name of "Candidatus" has been used. "Candidatus arthromitus" has been recovered from rainbow trout (Oncorhynchus mykiss) with summer enteritic syndrome, which is a gastro-enteritis
83
84
. The organism was observed in histological preparations to which nested polymerase chain reaction was used, with confirmation by sequencing
85
. "Candidatus piscichlamydia salmonis" was detected by RT-DGGE in intracellular inclusions, i.e. epitheliocysts, in Atlantic salmon with proliferative gill inflammation
86
. "Candidatus clavochlamydia salmonicola" is an intracellular organism, causing epitheliocystis in Atlantic salmon, which was recognized as novel as a result of 16S rRNA sequencing
87
.
6. Taxonomic developments associated with specific bacterial fish pathogens
From the early literature, a question-mark has hung over the reliability of some bacterial names insofar as there was often negligible evidence to support the use of those names. Concern may also be expressed about the value of studies based on only single isolates where concern about the reasons for choice of the culture may be aired. Some of the controversy surrounding specific diseases/pathogens follows:
6.1 Motile aeromonas septicaemia
Aeromonas hydrophila (= A. formicans and A. liquefaciens) would appear to have worldwide distribution and to be a pathogen, causing motile aeromonas septicaemia, of many species of freshwater fish. Indeed, there are reports of a spread into marine fish, notably ulcer disease of cod
88
. Since its initial recognition in the literature, a wealth of knowledge has been accumulated about many facets of its biology (see
6
). A new variant A. hydrophila subsp. dhakenis, which was originally recovered from children with diarrhoeae in Bangladesh, was determined to be pathogenic to rainbow trout
89
. However overall, there has been some doubt about the role of A. hydrophila as a pathogen, and in some cases it may well be present in fish tissue only as a secondary invader
6
. Moreover with developments in the taxonomy of motile aeromonads
90
, the accuracy of some of the early published identifications may be justifiably questioned. Could other motile aeromonads be associated with fish disease and may have been confused previously with A. hydrophila
89
?
It is clear that there is phenotypic, serological and genotypic heterogeneity within the descriptions of fish pathogenic A. hydrophila [e.g. 91, 92], and other motile aeromonads have been implicated as the aetiological agents of (fish) diseases. Thus, 8 isolates reported as pathogenic to eel in Spain were identified by numerical taxonomy as A. jandaei
93
94
. Certainly, the current approach of allocating species names as a result of the examination of 16S rRNA gene sequences has encompassed fish pathogenic motile aeromonads. For example, isolates from diseased fish which were recovered in Aeromonas DNA Hybridization Group 2 (= A. hydrophila) were equated with a new group, A. bestiarum
95
. Subsequently, A. sobria (A. sobria biovar sobria and A. veronii biovar sobria were reported as pathogenic to rainbow trout
89
. Indeed, A. sobria has been previously found to have a role as a fish pathogen, with isolates recovered from wild spawning gizzard shad (Dorosoma cepedianum) in Maryland, USA during 1987
15
96
. Also, A. veronii has been recovered from Siberian sturgeon (Acipenser baerii) with identification of the pathogen resulting from phenotyping and 16S rRNA gene sequencing
97
.
6.2 Aeromonas salmonicida
Aeromonas salmonicida is one of the oldest described fish pathogens, being isolated initially from diseased hatchery-maintained brown trout (Salmo trutta) in Germany, and named as "Bacillus der Forellenseuche" or bacillus of trout contagious disease. The history of the organism reveals a plethora of synonyms including Bacillus devorans, Bacterium salmonica, Bacterium salmonicida, Bacillus truttae and Bacillus salmonicida
6
. The 7th edition of Bergey's Manual of Determinative Bacteriology (1957) placed the pathogen in the genus Aeromonas within the family Pseudomonadaceae
98
. Later, there was a transfer to the family Vibrionaceae and subsequently to its own family, i.e. the Aeromonadaceae
99
. Re-classification was based primarily on phenotyping
100
. Thus in 1953, the first detailed description of the pathogen was published, and from an examination of 10 isolates, it was concluded that Bacterium salmonicida was homogeneous in cultural and biochemical characteristics
100
. Numerous studies have addressed the homogeneity of the species (e.g.
101
). The basic description is of an organism, which comprises non-motile (motility and flaA and flaB flagellar genes have been reported
52
82
), fermentative, Gram-negative rods, which produce a brown water-soluble pigment on tryptone-containing agar, do not grow at 37°C, and produce catalase and oxidase
6
. Cultures have the ability to dissociate into rough, smooth and G-phase (= intermediate) colonies
102
. The pathogen has spread from its dominance in salmonids to cyprinids and marine flatfish
6
. An ongoing issue surrounds the intraspecies structure, i.e. the validity of subspecies achromogenes, masoucida, pectinolytica, salmonicida and smithia, and the status of so-called atypical isolates.
A. salmonicida subsp. salmonicida, isolates of which have been obtained almost exclusively from outbreaks of furunculosis in salmonids, is regarded as homogeneous, and is referred to as "typical"
103
; all other isolates are considered as heterogeneous and "atypical"
6
. So called atypical strains may demonstrate weak, slow or non-pigment production
104
105
, catalase
106
or oxidase-negativity [e.g. 106, 107], nutritional fastidiousness for blood products
108
, slow growth, i.e. ≥ 5 days compared with 1-2 days for typical isolates
106
108
, and be pathogenic for fish other than salmonids, e.g. cyprinids (e.g.
106
108
109
) and marine flatfish, namely dab (Limanda limanda), plaice (Pleuronectes platessa), flounder (Platichthys flesus) and turbot (Scophthalmus maximus)
110
111
112
, and cause ulceration rather than furunculosis
6
113
. The deviation in characteristics from the typical to atypical isolates has made typing difficult
114
115
116
. Even 16S rDNA sequencing has not helped with the clustering of atypical forms (e.g.
117
).
Smith
118
recognized heterogeneity in the species description of A. salmonicida. She examined six isolates of non-pigmented A. salmonicida, which were clustered as Group I in her numerical taxonomy study, for which a separate new species name was proposed, i.e. A. achromogenes, but the proposal was not adopted widely. A second non-pigmented group was described by Kimura
119
, and named as A. salmonicida subsp. masoucida. Schubert
120
considered these non-pigmented isolates as subspecies, and coined the names of A. salmonicida subsp. achromogenes and A. salmonicida subsp. masoucida, respectively. Pigmented strains (= typical) were classified as A. salmonicida subsp. salmonicida
120
. The precise relationship of the subspecies has been the subject of detailed discussion. In particular, it was contended that subsp. achromogenes and masoucida were more closely related to A. hydrophila than to A. salmonicida
121
. Later, it was mooted that subsp. masoucida bridged typical A. salmonicida and A. hydrophila
122
. Yet, A. salmonicida subsp. masoucida is non-motile, sensitive to A. salmonicida bacteriophages, possesses an antigenic profile specific to A. salmonicida, and shares a DNA homology of 103% with A. salmonicida
92
. By PCR, a combination of achromogenes with masoucida could be justified, but this was not substantiated by ribotyping and RAPD analyses
114
. Phenotypic data suggest a case for combining subsp. masoucida with salmonicida, and subsp. achromogenes with Haemophilus piscium, which is the causal agent of ulcer disease of trout
123
. Examination of the small subunit rRNA gene sequences revealed 99.9% homology of an authentic strain of H. piscium with A. salmonicida subsp. salmonicida
124
. So far, the comparative uniqueness of subsp. smithia has been indicated from several studies (e.g.
114
). The complication is with aberrant strains of A. salmonicida from fish species other than salmonids.
DNA homology was used to reveal that all isolates of A. salmonicida (including A. salmonicida subsp. masoucida) were highly related, i.e. 96-106% homology, when hybridized against A. salmonicida subsp. salmonicida
92
. It was opined that A. salmonicida subsp. masoucida and some atypical isolates did not warrant separate subspecies status, because they were regarded as variants of other well-recognized groups. Also as a result of genotypic analyses, it was reported that typical and atypical isolates of A. salmonicida were very closely related, with minimal divergence
125
. Using DNA:DNA re-association, it was concluded that typical A. salmonicida were recovered in a homogeneous group, whereas the atypical representatives were more diverse
126
. From numerical taxonomy and DNA:DNA hybridization, similar conclusions resulted regarding the homogeneity of typical isolates of A. salmonicida
101
. However using 16S rRNA sequencing techniques, it was reported that subspecies achromogenes and masoucida were indistinguishable, and only differed from subspecies salmonicida by two bases
68
.
The relation of A. salmonicida to other aeromonads has been discussed. Eddy
127
focused on the inability of A. salmonicida to produce 2,3-butanediol from glucose, and the absence of motility, which were in contrast to the genus description
128
. A new genus, i.e. Necromonas, was proposed with two species, namely N. salmonicida for the typical isolates and N. achromogenes for the non-pigmented strains
118
. This proposal was not formally widely accepted, although Cowan
129
used the suggestion in his landmark identification scheme for medically important bacteria. Subsequent serological and bacteriophage sensitivity data supported the relationship between A. salmonicida and the motile aeromonads. Common antigens between A. hydrophila and A. salmonicida subsp. masoucida and other isolates of A. salmonicida were reported
122
130
. Furthermore, serological cross-reactions between A. salmonicida and motile aeromonads were discussed
131
. Moreover, A. hydrophila cultures were found to be sensitive to A. salmonicida bacteriophages
132
133
. The outcome of all the studies is that DNA homology supports the classification of A. salmonicida in the genus Aeromonas (e.g.
92
122
126
).
There are certainly outstanding questions about the validity and taxonomic placing of Haemophilus piscium
123
, but an authentic reference strain was not deposited any in any recognized culture collection at the time of its first isolation. Later, it was concluded that the organism was not a bona fide
Haemophilus because of the lack of requirement for haemin or NAD
134
. In particular H. piscium differed from the type species of the genus, H. influenzae, in the inability to reduce nitrate or alkaline phosphatase and to grow at 37°C, in conjunction with a higher G+C ratio of the DNA. It was commented that there was only a low similarity between H. piscium and other Haemophilus spp. in a numerical taxonomic study
135
. A link with atypical, achromogenic A. salmonicida was made
122
. This link was reinforced by bacteriophage sensitivity, when it was concluded that H. piscium is an atypical A. salmonicida
136
. Other workers have supported this view (e.g.
114
). However with the absence of an authentic, original type strain, the definitive taxonomic position of H. piscium is only speculative.
A lack of congruence has been reported between the results of molecular (PCR, RAPD and ribotyping) and phenotypic methods in taxonomy of aeromonads
114
. Moreover, there are problems of inter-laboratory differences and lack of standardisation in test methods
137
. The outcome is that the definitive classification of A. salmonicida has not been achieved, to date.
6.3 Enteric redmouth (ERM)
There has been discussion about the taxonomic position of the aetiological agent of ERM. Strong agglutination with Salmonella enterica subsp arizonae O group 26, and a weak reaction with O group 29 was reported
138
. In addition, biochemical similarities with enterics, notably Enterobacter liquefaciens, Serratia marcescens subsp. kiliensis as well as Salmonella enterica subsp. arizonae were mentioned
138
. Serological cross-reactions were also recorded with Hafnia alvei
139
. Nevertheless, a new species, i.e. Yersinia ruckeri was described although there was only a 30-31% DNA homology with Y. enterocolitica and Y. pseudotuberculosis
140
. This compares to DNA homologies of 24-28% and 31% with Serratia marcescens and Serratia liquefaciens, respectively
141
. Indeed, it has been suggested that the causal agent of ERM should belong in a new genus of the Enterobacteriaceae
142
. A complication developed when a new non-motile form of the pathogen was recovered from rainbow trout. By 16S rRNA sequencing and a homology of 100%, the organisms were linked to Y. ruckeri but regarded as a new biogroup
143
. Similar non-motile variants were also recovered from previously vaccinated rainbow trout in Spain
144
.
6.4 Vibriosis
The causal agent of "red-pest" in eels was first designated as Bacterium anguillarum
6
. Subsequently, an outbreak among eels in Sweden led to the use of the name Vibrio anguillarum. Numerous studies have pointed to heterogeneity in V. anguillarum initially with the delineation of two sub-groupings/biotypes (e.g.
12
). This increased to 3
145
and then 4 sub-groups/phena within the species definition
146
147
. Ribotyping has confirmed the heterogeneity
148
, although a single taxon, homogeneous by ribotyping but heterogeneous by LPS profiles, plasmid composition, serogrouping, and BIOLOG-GN fingerprints and API 20E profiles was described
149
150
. Biotype II became recognized as a separate species, i.e. V. ordalii
151
, which is homogeneous by plasmid profiling, ribotyping and serogrouping, accommodates two LPS groups, but is heterogeneous by BIOLOG-GN fingerprints and API 20E profiles
150
.
Serology has been widely used for diagnosis, but has complicated the understanding of V. anguillarum
151
, and the establishment of serotypes has to some extent traversed species boundaries. With V. anguillarum, serogroup 02 and 05, there are common antigens with V. ordalii
152
and V. harveyi
149
, respectively. Initially, three serotypes were recognised for isolates from salmonids from the northwest USA, Europe, and the Pacific-northwest (USA)
103
. This number increased to 6
128
, and then 10
153
and upwards
148
154
. Serogroup O1 dominates the number of isolates available for study and the relative importance to fish pathology
149
155
156
157
. Serogroup O2 has been further subdivided into serogroup O2a and O2b
158
.
V. anguillarum was re-classified initially to Beneckea
12
and then to a newly proposed genus Listonella
13
, but the changes were not widely accepted.