Abstract

Acute hepatopancreatic necrosis disease (AHPND) is a component cause of early mortality syndrome (EMS) of shrimp. In 2013, the causative agent was found to be unique isolates of Vibrio parahaemolyticus (VPAHPND) that contained a 69 kbp plasmid (pAP1) carrying binary Pir-like toxin genes PirvpA and PirvpB. In Thailand, AHPND was first recognized in 2012, prior to knowledge of the causative agent, and it subsequently led to a precipitous drop in shrimp production. After VPAHPND was characterized, a major focus of the AHPND control strategy was to monitor broodstock shrimp and post larvae for freedom from VPAHPND by nucleic acid amplification methods, most of which required use of expensive and sophisticated equipment not readily available in a shrimp farm setting. Here, we describe a simpler but equally sensitive approach for detection of VPAHPND based on loop-mediated isothermal amplification (LAMP) combined with unaided visual reading of positive amplification products using a DNA-functionalized, ssDNA-labled nanogold probe (AuNP). The target for the special set of six LAMP primers used was the VPAHPND PirvpA gene. The LAMP reaction was carried out at 65°C for 45 min followed by addition of the red AuNP solution and further incubation at 65°C for 5 min, allowing any PirvpA gene amplicons present to hybridize with the probe. Hybridization protected the AuNP against aggregation, so that the solution color remained red upon subsequent salt addition (positive test result) while unprotected AuNP aggregated and underwent a color change from red to blue and eventually precipitated (negative result). The total assay time was approximately 50 min. The detection limit (100 CFU) was comparable to that of other commonly-used methods for nested PCR detection of VPAHPND and 100-times more sensitive than 1-step PCR detection methods (104 CFU) that used amplicon detection by electrophoresis or spectrophotometry. There was no cross reaction with DNA templates derived from non-AHPND bacteria commonly found in shrimp ponds (including other Vibrio species). The new method significantly reduced the time, difficulty and cost for molecular detection of VPAHPND in shrimp hatchery and farm settings.

Highlights

  • Mortality syndrome (EMS) refers to unusually high mortality in cultivated shrimp within approximately 35 days after stocking of rearing ponds

  • The name was changed to acute hepatopancreatic necrosis disease (AHPND) when the causative agent was later discovered to be unique isolates of Vibrio parahaemolyticus (VPAHPND) that carry a 69 kbp plasmid that contains binary Pir-like toxin genes PirvpA and PirvpB [3,4,5,6]

  • Tests for the optimal loop-mediated isothermal amplification (LAMP) reaction temperature using 100 ng of DNA template from the VPAHPND isolated 5HP revealed that 65°C gave a slightly better result by agarose gel electrophoresis (AGE) analysis than 60 or 63°C (Fig 2)

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Summary

Introduction

Mortality syndrome (EMS) refers to unusually high mortality in cultivated shrimp within approximately 35 days after stocking of rearing ponds. After its first appearance in Thailand on the eastern coast of the Gulf of Thailand in late 2012, shrimp production dropped from a high of approximately 600,000 metric tons in 2011 to less than 200,000 in 2014 (FishStat; Food and Agriculture Organization of the United Nations) from a combination AHPND mortality and farmer reluctance to stock ponds until a solution was found. Molecular tools such as polymerase chain reaction (PCR) based on targeting the toxin genes PirvpA and PirvpB have been reported for early detection and prevention of AHPND spread. Loop-mediated isothermal amplification (LAMP) achieves synthesis of large amounts of DNA in a shorter time and in a simpler manner without sacrificing sensitivity or specificity, and it requires only a heating block or hot water bath rather than an expensive thermocycler

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