Real-time PCR-based assay for quantitative detection of Hematodinium sp. in the blue crab Callinectes sapidus

Nagle, Laurent; Place, Allen R.; Schott, Eric J.; Jagus, Rosemary; Messick, Gretchen A.; Pitula, Joseph S.

doi:10.3354/dao02027

Cited by 23 publications

(26 citation statements)

References 26 publications

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“…Similarly, we have found that the addition of BSA can counteract the inhibitory effects of remaining environmental inhibitors during diagnosis of Hematodinium using RT PCR. Thus, the use of BSA in the RT PCR protocol for diagnosis and quantification of Hematodinium in environmental samples is essential when inhibition is likely, as has been reported by others (Nagle et al, 2009).…”

Section: Discussionmentioning

confidence: 89%

“…(H.J. Small unpublished results), and based on an alignment of available SSU rRNA gene sequences, the primers developed by Nagle et al (2009) would also amplify the DNA of all Hematodinium and Hematodinium-like spp., as well as that of many other Syndiniales. As such, the above assays are genus-specific at best, but may also cross react with organisms in closely related genera.…”

Section: )mentioning

confidence: 99%

“…Frischer et al (2006) and Nagle et al (2009) developed real-time PCR assays for the detection and enumeration of the Hematodinium sp. infecting C. sapidus targeting regions of the SSU rRNA gene.…”

Section: )mentioning

confidence: 99%

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Detection and quantification of the free-living stage of the parasitic dinoflagellate Hematodinium sp. in laboratory and environmental samples

Shields

Miller

et al. 2010

Harmful Algae

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Section: Discussionmentioning

confidence: 89%

Section: )mentioning

confidence: 99%

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Detection and quantification of the free-living stage of the parasitic dinoflagellate Hematodinium sp. in laboratory and environmental samples

Shields

Miller

et al. 2010

Harmful Algae

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“…The Qiagen DNeasy Blood and Tissue Kit, for example, has been shown to be very efficient (Bletz et al 2015) and could be used for future DNA extractions, but this would increase the cost and processing time of the assay considerably. Additionally, DNA extraction methods are unable to completely separate DNA from PCR inhibitors (Liu et al 2009, Nagle et al 2009). For this reason, dilutions were used in the PCR assays in order to decrease PCR inhibition.…”

Section: Discussionmentioning

confidence: 99%

Development of quantitative PCR assay for detection of the trematode parasite Proctoeces maculatus in the blue mussel Mytilus edulis

Markowitz

Williams²,

Krause³

2016

Dis. Aquat. Org.

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The digenean trematode Proctoeces maculatus is an important parasite of the blue mussel Mytilus edulis. The parasite reduces mussel quality and yield, negatively impacting mussel aquaculture efforts. Typically, the trematode is detected by visual observation. To provide a better diagnostic tool able to detect this parasite at any life stage and at low intensities, we designed a species-specific molecular assay to detect P. maculatus in M. edulis tissue. Primers targeting the 18S nuclear ribosomal DNA (rDNA) from P. maculatus were used to develop an endpoint polymerase chain reaction assay and a quantitative polymerase chain reaction (qPCR) assay. Analytical specificity of the assays was demonstrated using DNA from 4 other digenean trematodes. The qPCR assay was linear from 6.79 × 10 2 to 6.79 × 10 7 copies of the cloned target DNA and had a conservative detection limit of 68 copies. The qPCR assay detected single cercariae, and the number of isolated cercariae was linearly correlated with the threshold cycle (C T ). Diagnostic sensitivity of the PCR-based methods was 100%. The assays also detected the parasite in 6 additional samples from the 57 tested through microscopy. We used the assays to verify the presence of encapsulated sporocysts in the mantle and to document infected mussels from Dover, New Hampshire, extending the previously described northern range of the species. Thus, this work has important implications for detection of the parasite in aquaculture and in monitoring its potential spread with climate change.KEY WORDS: Digenean · Aquaculture · Bivalve · Marine · Northwest Atlantic Resale or republication not permitted without written consent of the publisherDis Aquat Org 122: [125][126][127][128][129][130][131][132][133][134][135][136] 2016 and visible abscesses (Sunila et al. 2004). The parasites deplete glycogen and triglyceride levels in the mantle and hepatopancreas of infected mussels (Dennis et al. 1974, Machkevsky & Shchepkina 1985 and cause major organ damage as they spread throughout the mussel (Machkevsky & Gaevskaja 2008). Intense infections cause mussels to gape and detach from the substrate (Machkevsky & Gaevskaja 2008). Thus, infected mussels may be unable to handle the stress of harvesting and processing involved in aquaculture (Cole 1935, Canzonier 1972. Infection slows mussel growth (Machkevsky 1988) and at the highest intensity levels, ultimately leads to mortality (Machkevsky 1982, Machkevsky & Gaevskaja 2008. P. maculatus was implicated in mass mortalities of Mytilus galloprovincialis Lamarck, 1819 in Laguna Vaneta, Italy (Munford et al. 1981), and in the Black Sea (Machkevsky & Parukhin 1981), where the disease is referred to as 'proctecosis' (Machkevsky & Gaevs kaja 2008).P. maculatus has been found along the Gulf Coast (Wardle 1980) and east coast of the USA as far north as Woods Hole, MA. After numerous attempts by previous resear chers to find P. maculatus at sites north of Woods Hole were unsuccessful (Uzmann 1953, Pondick 1983, it was concluded that Woods Hol...

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“…Based on the previous work of Nagel et al (2009), qPCR detection was used as an indicator of infection status in both hemolymph and muscle tissue. The ITS2 primer set and the protocol described in Hanif et al (2013) were used for all samples in this study.…”

Section: Quantitative Polymerase Chain Reactionmentioning

confidence: 99%

Disease ecology of Hematodinium perezi in a high salinity estuary: investigating seasonal trends in environmental detection

Lycett¹,

Pitula²

2017

Dis. Aquat. Org.

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The blue crab Callinectes sapidus has seen a general decline in population levels. One factor influencing mortality is infections by Hematodinium perezi, a dinoflagellate parasite. A 2 yr study was conducted in 2014 and 2015 to monitor H. perezi DNA within the Maryland (USA) coastal bays, comparing seasonal cycles in the abundance of parasite DNA in environmental samples to parasite presence in host blue crabs. A late summer to early fall peak in H. perezi infections in blue crabs was observed, consistent with previous work. Infection intensities matched this trend, showing a slow progression of low intensity infections early in the year, with a peak in moderate and heavy infections occurring between July and September, for both years. It was hypo thesized that the peak in water column occurrence would coincide with those months when infection intensities were highest in blue crabs. As the peaks in water column occurrence were in July 2014 and August−September 2015, this is consistent with sporulation being the primary contributor to environmental detection in summer months. An additional peak in environmental detection occurred in both years during the early spring months, the cause of which is currently unknown but may be related to infections in overwintering crabs or alternate hosts. Several new crusta cean hosts were identified within this estuary, including grass shrimp Palaemonetes spp. and the sand shrimp Crangon septemspinosa, as well as the mud crab Dyspanopeus sayi. Improved knowledge of this disease system will allow for better management of this important fishery. KEY WORDS: Blue crab · Crustacean · Environment · DNA · quantitative PCR · qPCR Resale or republication not permitted without written consent of the publisherDis Aquat Org 124: [169][170][171][172][173][174][175][176][177][178][179] 2017 Epizootic events where infection prevalence reached 100% have been observed in the field, after which infections disappeared from the crab popu lation presumably due to high mortality (Messick 1994).Along the Maryland coastline, there are several oceanic bays where summer mortality events have been attributed to infections by H. perezi. For the purpose of this study, these bays are denoted as a unified system known as the Maryland coastal bays (MCB), which includes Isle of Wight, Assawoman, Sinepuxent, and Chincoteague bays, though a portion of Chincoteague Bay is in Virginia. Seasonal cycles of infection in this system suggest higher rates of infection when water temperatures are at their highest or beginning to cool from their summer peak (Messick 1994, Messick et al. 1999, Messick & Shields 2000.Although the exact mechanism of disease transmission is still unknown, there have been reports of sporulation events, where heavily infected hosts release dinospores into the water column (Shields & Squyars 2000). Despite this known connection to environmental release, limited work has investigated the hypothesis that sporulation in highly infected blue crabs leads to greater detection in the water ...

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Real-time PCR-based assay for quantitative detection of Hematodinium sp. in the blue crab Callinectes sapidus

Cited by 23 publications

References 26 publications

Detection and quantification of the free-living stage of the parasitic dinoflagellate Hematodinium sp. in laboratory and environmental samples

Detection and quantification of the free-living stage of the parasitic dinoflagellate Hematodinium sp. in laboratory and environmental samples

Development of quantitative PCR assay for detection of the trematode parasite Proctoeces maculatus in the blue mussel Mytilus edulis

Disease ecology of Hematodinium perezi in a high salinity estuary: investigating seasonal trends in environmental detection

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