Pathogens (Jan 2024)

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

  • Irene Cano,
  • Gareth Wood,
  • David Stone,
  • Mathilde Noyer,
  • Lydie Canier,
  • Isabelle Arzul

DOI
https://doi.org/10.3390/pathogens13020132
Journal volume & issue
Vol. 13, no. 2
p. 132

Abstract

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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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