Simple and rapid detection of Photobacterium damselae ssp. piscicida by a PCR technique and plating method

Rajan, P. R.; Lin, John Han-You; Ho, Margaret S.; Yang, Huey‐Lang

doi:10.1046/j.1365-2672.2003.02119.x

Cited by 44 publications

(43 citation statements)

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“…piscicida strain O82352 was isolated from the kidney of yellowtail during an outbreak of pseudotuberculosis at a culture farm in Oita Prefecture, Japan, in 1998. The bacterium was identified using polymerase chain reaction (PCR) targeted at 16S ribosomal RNA and capsular polysaccharide [22,23]. The bacterium was precultured in 7 ml brain heart infusion (BHI) broth (Difco) supplemented with 1.5% NaCl (BHI) at 25°C with shaking at 100 rpm for 16 h. Then, 0.75 ml of the suspension was inoculated into 300 ml BHI broth, which was incubated at 25°C with shaking at 100 rpm.…”

Section: Methodsmentioning

confidence: 99%

Repeatable immersion infection with Photobacterium damselae subsp. piscicida reproducing clinical signs and moderate mortality

et al. 2009

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Pseudotuberculosis is a bacterial septicaemia caused by Photobacterium damselae subsp. piscicida in several marine fish species. Yellowtail Seriola quinqueradiata is the most sensitive fish species to this disease. The internal organs of naturally infected yellowtail exhibit whitish spots, tubercle-like tissue structures, consisting of bacterial accumulations. There have been many trials for experimental infection, however adequate method of infection that reproduces moderate mortality and primary clinical signs has not yet established. Present investigation evaluated an immersion infection method by using logarithmic culture-phase bacteria resulting in higher mortality than that using stationary culture-phase bacteria. Typical white spots on the spleen and kidney were also observed constantly in dead fish. Transmission electron microscopy and fluorescent antibody microscopy showed bacterial clusters not only in the spleen and kidney but also in the blood channels in the secondary gill filaments. These results were confirmed repeatedly by plural experiments. The use of logarithmic-phase bacteria in immersion infection is an appropriate technique to reproduce moderate mortality and primary clinical signs, which will be a reliable infection method also for the challenge test of pseudotuberculosis vaccine.

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Section: Methodsmentioning

confidence: 99%

Repeatable immersion infection with Photobacterium damselae subsp. piscicida reproducing clinical signs and moderate mortality

et al. 2009

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“…damselae, em especial nas seguintes características: ausência de atividade hemolítica em meio ágar sangue, e atividade negativa para redução do nitrato, urease, amilase e lípase (Romalde, 2002). Além disso, Rajan et al (2003) relataram ausência de crescimento em meio ágar tiossulfato citrato sais de bile sacarose (TCBS).…”

Section: Photobacterium Damselae Subsp Piscicidaunclassified

“…Nascimento et al (2014) também realizaram análises bacteriológicas, com base em fragmentos de órgãos internos, em 74 animais cultivados no Nordeste brasileiro, tendo obtido uma porcentagem de isolamento de 96% (71 peixes) de bactérias da família Vibrionaceae. Esses autores não relataram a presença de P. damselae, porém, utilizaram apenas ágar TCBS como meio de isolamento, o que restringiu a capacidade de isolar ambas as subespécies (Rajan et al, 2003;Korun & Timur, 2005). Ainda assim, Nascimento et al (2014) enfatizam que os exemplares de bijupirá analisados, embora aparentemente saudáveis, estão infectados com bactérias potencialmente patogênicas para peixes e humanos.…”

Section: Fotobacteriose No Brasilunclassified

“…Essa situação torna-se (Andreoni & Magnani, 2014), que é capaz de detectar a espécie, mas incapaz de diferenciar as subespécies; kits comerciais de testes imunoenzimáticos (Andreoni & Magnani, 2014); e PCR multiplex dos genes 16S rRNA e ureC, capazes de diferenciar as subespécies piscicida e damselae (Andreoni & Magnani, 2014). Rajan et al (2003) sugerem o uso combinado da detecção por PCR do gene 16S rRNA com a diferenciação em meio TCBS para discriminar as subespécies, uma vez que somente o gene 16S rRNA é incapaz de diferenciar as subespécies desse patógeno (Osorio et al, 1999). Já Hundenborn et al (2013) reportam sucesso na detecção e discriminação desse patógeno com o sistema MALDI-TOF de espectrofotometria de massa.…”

Section: Fotobacteriose No Brasilunclassified

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Detecção, controle e prevenção de fotobacteriose em cultivo de bijupirá

Gonçalves

Sanches

Martins

et al. 2016

Pesq. agropec. bras.

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Resumo -O objetivo deste trabalho foi analisar a detecção, o controle e a prevenção de fotobacteriose em cultivo de bijupirá. Essa doença é causada pela bactéria Photobacterium damselae, que, juntamente com outros fatores, pode estar sendo responsável pela estagnação no crescimento da produção nacional de bijupirá (Rachycentron canadum). Essa bactéria é considerada um dos principais patógenos de peixes marinhos cultivados, tendo sido responsável por importantes prejuízos econômicos em diversos países. No Brasil, essa bactéria ainda não recebeu a devida importância, apesar de já ter sido detectada como causadora de mortalidades nos cultivos de bijupirá. Photobacterium damselae possui duas subespécies, piscicida e damselae, que podem ser consideradas ameaças sanitárias, respectivamente, em relação à atividade econômica da piscicultura marinha e em relação à saúde humana. Neste trabalho, são apresentadas algumas estratégias de detecção, controle e prevenção. Enfatiza-se, também, a necessidade de um melhor acompanhamento sanitário nos cultivos de bijupirá e a importância da vacinação contra esse patógeno.Termos para indexação: Photobacterium damselae, Rachycentron canadum, aquicultura, piscicultura marinha, sanidade animal, zoonose. Detection, control, and prevention of photobacteriosis in cobia culture in BrazilAbstract -The objective of this work was to analyse the detection, control, and prevention of photobacteriosis in cobia culture. This disease is caused by Photobacterium damselae bacterium, which, along with other factors, might be responsible for the stagnation in the development of national cobia (Rachycentron canadum) culture. This bacterium is considered one of the most important pathogens in marine fish culture, and it was responsible for major economic losses in a variety of countries. In Brazil, this bacterium has not yet getten proper attention, even though it was shown to have caused mortality in several cultured cobia fish. Photobacterium damselae has two subspecies, piscicida and damselae, which may be considered sanitary threats both to marine aquaculture economic activities and to human health, respectively. This paper presents some detection, control, and prevention strategies. It also emphasizes the need for a better sanitary control in cobia culture and the importance of vaccination against this pathogen.

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“…A method based on duplex PCR of ureC and 16S rRNA genes was proposed by Osorio et al (2000), due to the lack of the ureC gene in the subspecies piscicida, but subspecies discrimination was based on indirect evidence (lack of amplification of ureC). Lately, a combined approach of PCR technique and plating method has been proposed (Rajan et al 2003). Other methods such as ribotyping (Magariños et al 1997), RAPD (Random Amplified Polymorphic DNA) (Magariños et al 2000), and amplified fragment length polymorphism (AFLP) (Thyssen et al 2000, Kvitt et al 2002 showed the ability to differentiate the 2 subspecies as well as to identify clusters of P. damselae subsp.…”

Section: Introductionmentioning

confidence: 99%

Direct identification of Photobacterium damselae subspecies piscicida by PCR-RFLP analysis

Zappulli

Patarnello²,

Patarnello³

et al. 2005

Dis. Aquat. Org.

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Fish pasteurellosis is an infectious disease that affects several teleost species living in temperate marine waters. The pathogen responsible, Photobacterium damselae subspecies piscicida, shows high genetic similarity with P. damselae subsp. damselae, making subspecies discrimination extremely laborious. Here we report for the first time a PCR-RFLP method for the identification of P. damselae subsp. piscicida without prior isolation in pure culture. Genomic sequence information was obtained through cloning and sequencing of RAPD products. Two P. damselae-specific primer pairs were developed and tested on 17 strains of P. damselae subsp. piscicida, 10 strains of P. damselae subsp. damselae, and 6 closely related control species. High sensitivity was achieved in PCR amplification on serially diluted samples (<180 fg of pure bacterial DNA or <10 fg, depending on the amplified fragment). Restriction analysis of PCR products showed a unique digestion profile for all P. damselae subsp. piscicida strains. The same PCR-RFLP method was implemented on total DNA samples extracted from experimentally infected sea bream and sea bass. Positive results were obtained on fish with clear signs of the disease as well as on challenged, but asymptomatic, fish. The method presented here might provide a useful tool for both prevention and rapid diagnosis of fish pasteurellosis. KEY WORDS: Photobacterium damselae subsp. piscicida · Fish pasteurellosis · PCR-RFLP · Diagnostic tool Resale or republication not permitted without written consent of the publisherDis Aquat Org 65: [53][54][55][56][57][58][59][60][61] 2005 a better prevention of the disease through control of the presence of the pathogen in the water and/or carrier fishes. Thus far, a broad variety of methods has been evaluated for highly sensitive, species-(subspecies) identification of the pathogen without prior isolation as pure culture. Tested methods include enzyme-linked immunosorbent assays (ELISA) and enzyme immuno-assay (EIA) techniques (Bakopoulos et al. 1997, plasmid DNA PCR (Aoki et al. 1997), 16S rRNA gene sequencing , and primers designed following random amplified polymorphic DNA (RAPD) (Dalla Valle et al. 2002). All these methods, however, could not reliably discriminate between the 2 subspecies. A method based on duplex PCR of ureC and 16S rRNA genes was proposed by Osorio et al. (2000), due to the lack of the ureC gene in the subspecies piscicida, but subspecies discrimination was based on indirect evidence (lack of amplification of ureC). Lately, a combined approach of PCR technique and plating method has been proposed (Rajan et al. 2003). Other methods such as ribotyping (Magariños et al. 1997), RAPD (Random Amplified Polymorphic DNA) (Magariños et al. 2000), and amplified fragment length polymorphism (AFLP) (Thyssen et al. 2000, Kvitt et al. 2002 showed the ability to differentiate the 2 subspecies as well as to identify clusters of P. damselae subsp. piscicida strains. However, these methods require DNA extraction from pure cultures and refe...

show abstract

Simple and rapid detection of Photobacterium damselae ssp. piscicida by a PCR technique and plating method

Cited by 44 publications

References 30 publications

Repeatable immersion infection with Photobacterium damselae subsp. piscicida reproducing clinical signs and moderate mortality

Repeatable immersion infection with Photobacterium damselae subsp. piscicida reproducing clinical signs and moderate mortality

Detecção, controle e prevenção de fotobacteriose em cultivo de bijupirá

Direct identification of Photobacterium damselae subspecies piscicida by PCR-RFLP analysis

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