First characterization of the parasite
            <i>Haplosporidium costale</i>
            in France and development of a real‐time PCR assay for its rapid detection in the Pacific oyster,
            <i>Crassostrea gigas</i>

Arzul, Isabelle; Garcia, Céline; Chollet, Bruno; Serpin, Delphine; Lupo, Coralie; Noyer, Mathilde; Tourbiez, Delphine; Chloé, Berland; Dégremont, Lionel; Marie‐Agnès, Travers

doi:10.1111/tbed.14541

Cited by 7 publications

(3 citation statements)

References 65 publications

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“…Alignments with 18S–ITS1–5.8S–ITS2–28S partial sequences of Haplosporidium costale from Crassostrea virginica (KF790901–2 [ 50 ]) and from C. gigas (MZ666374 [ 51 ]), of Haplosporidium sp. from Saccostrea glomerata (KF790894–900 [ 50 ]), and of Haplosporidium littoralis (KJ150289 [ 52 ]) were used to compare and to allocate the start and stop nucleotide locations of rRNAs.…”

Section: Resultsmentioning

confidence: 99%

Haplosporidium pinnae Parasite Detection in Seawater Samples

et al. 2023

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In this study, we investigated the presence of the parasite Haplosporidium pinnae, which is a pathogen for the bivalve Pinna nobilis, in water samples from different environments. Fifteen mantle samples of P. nobilis infected by H. pinnae were used to characterize the ribosomal unit of this parasite. The obtained sequences were employed to develop a method for eDNA detection of H. pinnae. We collected 56 water samples (from aquaria, open sea and sanctuaries) for testing the methodology. In this work, we developed three different PCRs generating amplicons of different lengths to determine the level of degradation of the DNA, since the status of H. pinnae in water and, therefore, its infectious capacity are unknown. The results showed the ability of the method to detect H. pinnae in sea waters from different areas persistent in the environment but with different degrees of DNA fragmentation. This developed method offers a new tool for preventive analysis for monitoring areas and to better understand the life cycle and the spread of this parasite.

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Section: Resultsmentioning

confidence: 99%

Haplosporidium pinnae Parasite Detection in Seawater Samples

et al. 2023

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“…[ 88 , 89 ], Haplosporidium spp. [ 90 ], and Mikrocytos mackini [ 91 ]. The susceptibility of Pacific oyster to Marteilia refringens , Bonamia ostreae , and Bonamia exitiosa is still undetermined [ 92 , 93 ].…”

Section: Discussionmentioning

confidence: 99%

Identification and Characterization of Infectious Pathogens Associated with Mass Mortalities of Pacific Oyster (Crassostrea gigas) Cultured in Northern China

Zhang

Huang

Zheng

et al. 2023

Biology

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The Pacific oyster (Crassostrea gigas) aquaculture industry increased rapidly in China with the introduction and promotion of triploid oysters in recent years. Mass mortalities affecting different life stages of Pacific oysters emerged periodically in several important production areas of Northern China. During 2020 and 2021, we conducted a passive two-year investigation of infectious pathogens linked to mass mortality. Ostreid herpesvirus-1 (OsHV-1) was detected to be associated with mass mortalities of hatchery larvae, but not juveniles and adults in the open sea. Protozoan parasites, such as Marteilia spp., Perkinsus spp. and Bonamia spp. were not detected. Bacterial isolation and identification revealed that Vibrio natriegens and Vibrio alginolyticus were the most frequently (9 out of 13) identified two dominant bacteria associated with mass mortalities. Pseudoalteromonas spp. was identified as the dominant bacteria in three mortality events that occurred during the cold season. Further bacteriological analysis was conducted on two representative isolates of V. natriegens and V. alginolyticus, designated as CgA1-1 and CgA1-2. Multisequence analysis (MLSA) showed that CgA1-1 and CgA1-2 were closely related to each other and nested within the Harveyi clade. Bacteriological investigation revealed faster growth, and more remarkable haemolytic activity and siderophore production capacity at 25 °C than at 15 °C for both CgA1-1 and CgA1-2. The accumulative mortalities of experimental immersion infections were also higher at 25 °C (90% and 63.33%) than at 15 °C (43.33% and 33.33%) using both CgA1-1 and CgA1-2, respectively. Similar clinical and pathological features were identified in samples collected during both naturally and experimentally occurring mortalities, such as thin visceral mass, discolouration, and connective tissue and digestive tube lesions. The results presented here highlight the potential risk of OsHV-1 to hatchery production of larvae, and the pathogenic role of V. natriegens and V. alginolyticus during mass mortalities of all life stages of Pacific oysters in Northern China.

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“…Control DNA for B. exitiosa , B. ostreae , and other species of parasites were sourced from the collection of the Ifremer ASIM Laboratory (France). The presence of the parasite on infected molluscs was confirmed by conventional PCR combined with sequencing [ 21 , 39 , 40 ], except for the samples infected with M. mackini and the one co-infected with H. nesloni and H. costale , which were only tested by real-time PCR. However, the status of those two samples was confirmed by the donor laboratory.…”

Section: Methodsmentioning

confidence: 99%

Loop-Mediated Isothermal Amplification for the Fast Detection of Bonamia ostreae and Bonamia exitiosa in Flat Oysters

Cano,

Wood,

Stone

et al. 2024

Pathogens

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The haplosporidian parasites Bonamia ostreae (BO) and B. exitiosa (BE) are serious oyster pathogens. Two independent laboratories evaluated fluorescence real-time loop-mediated isothermal amplification (LAMP) assays for rapidly detecting these parasites. Specific LAMP assays were designed on the BO actin-1 and BE actin genes. A further generic assay was conceived on a conserved region of the 18S gene to detect both Bonamia species. The optimal reaction temperature varied from 65 to 67 °C depending on the test and instrument. Melting temperatures were 89.8–90.2 °C, 87.0–87.6 °C, and 86.2–86.6 °C for each of the BO, BE, and generic assays. The analytical sensitivity of these assays was 50 copies/µL in a 30 min run. The BO and BE test sensitivity was ~1 log lower than a real-time PCR, while the generic test sensitivity was similar to the real-time PCR. Both the BO and BE assays were shown to be specific; however, the generic assay potentially cross-reacts with Haplosporidium costale. The performance of the LAMP assays evaluated on samples of known status detected positives within 7–20 min with a test accuracy of 100% for the BO and generic tests and a 95.8% accuracy for BE. The ease of use, rapidity and affordability of these tests allow for field deployment.

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First characterization of the parasite Haplosporidium costale in France and development of a real‐time PCR assay for its rapid detection in the Pacific oyster, Crassostrea gigas

Cited by 7 publications

References 65 publications

Haplosporidium pinnae Parasite Detection in Seawater Samples

Haplosporidium pinnae Parasite Detection in Seawater Samples

Identification and Characterization of Infectious Pathogens Associated with Mass Mortalities of Pacific Oyster (Crassostrea gigas) Cultured in Northern China

Loop-Mediated Isothermal Amplification for the Fast Detection of Bonamia ostreae and Bonamia exitiosa in Flat Oysters

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