Your search keyword '"Fish Diseases diagnosis"' showing total 58 results

1. Development of a loop-mediated isothermal amplification (LAMP) assay for rapid and visual detection of Anguillid herpesvirus 1.

Author

Chen Q, Zhang LJ, Song TY, and Ge JQ

Subjects

Animals, China, DNA Primers genetics, Aquaculture, Eels virology, Temperature, DNA, Viral genetics, DNA, Viral isolation & purification, Nucleic Acid Amplification Techniques methods, Nucleic Acid Amplification Techniques veterinary, Sensitivity and Specificity, Fish Diseases diagnosis, Fish Diseases virology, Molecular Diagnostic Techniques methods, Molecular Diagnostic Techniques veterinary, Herpesviridae isolation & purification, Herpesviridae genetics, Herpesviridae Infections veterinary, Herpesviridae Infections diagnosis, Herpesviridae Infections virology

Abstract

China has the largest aquaculture eel production in the world. High-density cultivation pattern often results in an outbreak of epidemic diseases. Since the 1990s, eel "mucus sloughing and hemorrhagic septicemia disease" was often broke out in China, and brought huge economic losses to eel breeders. Anguillid herpesvirus 1 (AngHV) was detected and isolated from the diseased eel, and proved to be the pathogen of the disease. In this study, a loop-mediated isothermal amplification (LAMP) assay was developed for rapid, sensitive, and specific detection of AngHV. A set of six primers targeting the ORF51 gene of AngHV was designed, which could effectively detect purified AngHV virions, AngHV-infected cells, or eel tissue samples. The suitable reaction temperature is 63℃, and the reaction time is 40 min. There was no cross-reaction with eel and other fish viruses, including Infectious pancreatic necrosis virus (IPNV), Marine birnavirus (MABV), Rana grylio virus (RGV), Cyprinid herpesvirus 3 (CyHV-3), and Eel iridovirus (EIV). The lower detection limit of the AngHV LAMP assay is 10 copies of AngHV genome DNA, which is at least 100 times more sensitive than conventional PCR in detecting AngHV. The assay could effectively detect AngHV from collected samples with typical clinical symptoms of AngHV infection. It suggested that the LAMP assay could be used in specific detection of AngHV and has great potential for early diagnosis of AngHV infection in the farm., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

2. Development of real-time recombinase polymerase amplification (RPA) and RPA combined with lateral flow dipstick (LFD) assays for the rapid and sensitive detection of cyprinid herpesvirus 3.

Author

Li Y, Li R, Mo X, Wang Y, Yin J, Bergmann SM, Ren Y, Pan H, Shi C, Zhang D, and Wang Q

Subjects

Animals, Recombinases metabolism, Fish Diseases diagnosis, Fish Diseases virology, Herpesviridae isolation & purification, Herpesviridae genetics, Herpesviridae Infections veterinary, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Carps virology, Sensitivity and Specificity, Nucleic Acid Amplification Techniques veterinary, Nucleic Acid Amplification Techniques methods

Abstract

In this issue, we established rapid, cost-effective, and simple detection methods including recombines polymerase amplification with lateral flow dipstick (RPA-LFD) and real-time RPA for cyprinid herpesvirus 3(CyHV-3), and evaluated their sensitivity, specificity, and applicability, the real-time RPA method could achieve sensitive diagnosis of CyHV-3 within 1.3 copies per reaction, respectively. The real-time RPA method is 10-fold more sensitive than RPA-LFD method. The exact number of CyHV-3 can be calculated in each sample by real-time RPA. The sera from koi also can be tested in these methods. In addition, no cross-reaction was observed with other related pathogens, including carp oedema virus (CEV), spring viraemia of carp virus (SVCV), cyprinid herpesvirus 1(CyHV-1), cyprinid herpesvirus 2(CyHV-2), type I grass carp reovirus (GCRV-I), type II GCRV (GCRV-II), type III GCRV (GCRV-III), and Aeromonas hydrophila., (© 2024 John Wiley & Sons Ltd.)

Published

2024

3. Rapid and sensitive detection of large yellow croaker iridovirus by real-time RPA and RPA-LFD.

Author

Liu X, Cao Y, Wang J, Cao S, Lu L, and Jiang Y

Subjects

Animals, DNA, Viral genetics, Capsid Proteins genetics, Perciformes virology, Fish Diseases virology, Fish Diseases diagnosis, DNA Virus Infections veterinary, DNA Virus Infections diagnosis, DNA Virus Infections virology, Iridovirus isolation & purification, Iridovirus genetics, Nucleic Acid Amplification Techniques veterinary, Nucleic Acid Amplification Techniques methods, Sensitivity and Specificity

Abstract

Large yellow croaker (Larimichthys crocea) is a vital marine-cultured species in China. Large yellow croaker iridovirus (LYCIV) can cause a high mortality rate in L. crocea. Rapid and convenient detection of LYCIV is an urgent demand for diagnosis. In this study, rapid and simple recombinase polymerase amplification (RPA), real-time RPA and RPA combined with lateral flow dipstick (RPA-LFD) methods were developed for the detection of LYCIV based on the conserved sequence of the LYCIV major capsid protein (MCP) gene. With these optimized RPA analyses, LYCIV detection could be completed within 20 min at 40°C. Both RPA and real-time RPA could detect viral DNA as low as 10 2 copies/μL, while the detection limit of RPA-LFD was 10 1 copies/μL, and there was no cross-reaction with other aquatic pathogens (KHV, CyHV-2, GCRV-JX01, SVCV, LCDV and LMBV). In practical evaluation of RPA, real-time RPA and RPA-LFD methods, the results showed consistency with the general PCR detection. In short, the developed RPA, real-time RPA and RPA-LFD analyses could be simple, rapid, sensitive and reliable methods for field diagnosis of LYCIV infection and have significant potential in the protection of LYCIV infection., (© 2024 John Wiley & Sons Ltd.)

Published

2024

4. Development and application of a recombinase-aided amplification combined with a lateral flow dipstick assay for rapid visual detection of anguillid herpesvirus 1.

Author

Chen X, Chen H, and Ge JQ

Subjects

Animals, Recombinases, Sensitivity and Specificity, Nucleic Acid Amplification Techniques veterinary, Nucleic Acid Amplification Techniques methods, Fish Diseases diagnosis, Herpesviridae

Abstract

Eel (Anguilla sp.) is an important freshwater-cultured species with high economic value in China. Anguillid herpesvirus 1 (AngHV-1) has been proven to be the pathogen of "mucus sloughing and haemorrhagic septicaemia disease" in eels, resulting in significant mortality and substantial losses to the eel industry. Current diagnostic methods for detecting AngHV-1 are limited to laboratory-based tests, for example, conventional end-point PCR and qPCR. Therefore, there is an urgent need to develop an accurate, rapid, and simple detection method for on-site diagnosis of AngHV-1. In this study, we developed a recombinase-aided amplification combined lateral flow dipstick (RAA-LFD) assay for the detection of AngHV-1. The RAA-LFD assay can be performed within a temperature range of 18-45°C, with a reaction time of just 10 min for amplification. Importantly, the established RAA-LFD assay exhibited no reactivity with other common aquatic viral pathogens, indicating its high specificity. The limit of detection for this method is 10 2 copies of AngHV-1, which is more sensitive than the established conventional end-point PCR method similarly targeting ORF95. Clinical detection of the diseased samples demonstrated that the accuracy of RAA-LFD was significantly higher than that of the conventional end-point PCR. In conclusion, the developed RAA-LFD assay has proven to be a convenient, rapid, sensitive, and reliable tool for on-site diagnosis of AngHV-1. This advancement will be invaluable for the prevention and control of AngHV-1 in the eel farming industry., (© 2023 John Wiley & Sons Ltd.)

Published

2024

5. Reverse transcription loop-mediated isothermal amplification (RT-LAMP) combined with colorimetric gold nanoparticle (AuNP) probe assay for visual detection of tilapia lake virus (TiLV) in Nile and red hybrid tilapia.

Author

Kampeera J, Dangtip S, Suvannakad R, Khumwan P, Senapin S, and Kiatpathomchai W

Subjects

Animals, Fish Diseases virology, Gold therapeutic use, RNA Virus Infections diagnosis, RNA Virus Infections virology, Reverse Transcription, Sensitivity and Specificity, Aquaculture methods, Cichlids, Colorimetry veterinary, Fish Diseases diagnosis, Metal Nanoparticles therapeutic use, Molecular Diagnostic Techniques veterinary, Nucleic Acid Amplification Techniques veterinary, RNA Virus Infections veterinary, RNA Viruses isolation & purification

Abstract

Tilapia is one of the major aquaculture species with a global economic significance. Despite a high scale of production worldwide, mortality in many tilapia cultures has recently become a problem concerned with not only intensive farming but also the prevalence of infectious pathogens. Tilapia lake virus (TiLV) has emerged as a serious single-stranded RNA disease agent that thus far has continued to cause a number of incidences across the continents. Conventional PCR-based molecular detection techniques, despite having high sensitivity for TiLV, are not best suited for the onsite identification of infected fish mainly due to their requirement of laboratory resources and extended assay turnaround time. To address this practical limitation, we have developed a novel colorimetric assay based on reverse transcription-loop-mediated isothermal amplification (RT-LAMP) and gold nanoparticle (AuNP)-labelled oligonucleotide reporter probe targeting the viral genomic segment 9 that enables the assay to be completed within an hour. This technique has been shown to be compatible with a rapid nucleic extraction method that does not demand centrifugation steps or any benchtop laboratory equipment. When validated with field-acquired tilapia samples, our RT-LAMP-AuNP assay exhibited a near-perfect agreement with the semi-nested RT-PCR assay recommended by OIE with Cohen's κ coefficient of .869, yet requiring significantly less time to perform., (© 2021 John Wiley & Sons Ltd.)

Published

2021

6. Development of cross-priming amplification (CPA) combined with colorimetric and lateral flow dipstick visualization for scale drop disease virus (SDDV) detection.

Author

Prasitporn T, Senapin S, Vaniksampanna A, Longyant S, and Chaivisuthangkura P

Subjects

Animals, Colorimetry, Cross-Priming, DNA Virus Infections diagnosis, Fish Diseases virology, Naphthalenesulfonates, Serologic Tests methods, DNA Virus Infections veterinary, Fish Diseases diagnosis, Iridoviridae isolation & purification, Nucleic Acid Amplification Techniques methods

Abstract

Scale drop disease virus (SDDV) is one of the most important pathogens that causes scale drop disease (SDD) in Asian sea bass (Lates calcarifer). The outbreaks of this disease are one of the factors causing substantial losses in Asian sea bass aquaculture. In this study, the uracil-DNA glycosylase (UDG)-supplemented cross-priming amplification (UCPA) combined with a colorimetric detection method using the hydroxynaphthol blue (HNB) and lateral flow dipstick (LFD) for detection of SDDV was developed. The UDG was utilized to prevent carryover contamination, and the CPA reactions can be readily observed by HNB and LFD. The CPA primers and probe were designed to target the major capsid protein (MCP) gene of the SDDV. The optimized UCPA conditions were performed at the temperature of 61°C for 60 min. The UCPA assays demonstrated specificity to SDDV without cross-reaction to other tested viruses including red-spotted grouper nervous necrosis virus (RGNNV), infectious spleen and kidney necrosis virus (ISKNV) and Lates calcarifer herpes virus (LCHV), and other bacterial species commonly found in aquatic animals. The sensitivity of the UCPA-HNB and UCPA-LFD was 100 viral copies/µl and 10 pg of extracted total DNA, which was 10-fold more sensitive than that of conventional PCR. The UCPA-HNB and UCPA-LFD assays could be used to detect the SDDV infection in all 25 confirmed SDDV-infected fish samples. Therefore, the UCPA coupled with HNB and LFD was rapid, simple and effective and might be applied for diagnosis of SDDV infection., (© 2021 John Wiley & Sons Ltd.)

Published

2021

7. Application of the FTA elute card coupled with visual colorimetric loop-mediated isothermal amplification for the rapid diagnosis of Streptococcus agalactiae in farmed tilapia (Oreochromis niloticus).

Author

Pepey E, Taukhid T, Keck N, Lusiastuti A, Avarre JC, Sundari G, Sarter S, and Caruso D

Subjects

Animals, Colorimetry methods, Fish Diseases microbiology, Molecular Diagnostic Techniques methods, Nucleic Acid Amplification Techniques methods, Streptococcal Infections diagnosis, Streptococcal Infections microbiology, Cichlids, Colorimetry veterinary, Fish Diseases diagnosis, Molecular Diagnostic Techniques veterinary, Nucleic Acid Amplification Techniques veterinary, Streptococcal Infections veterinary, Streptococcus agalactiae isolation & purification

Abstract

A method combining the FTA Elute card and visual colorimetric loop-mediated isothermal amplification (FTA-e/LAMP) was tested to diagnose Streptococcus agalactiae infections in vitro and in vivo. FTA-e/LAMP consists of two main steps: first, the FTA card is used to extract DNA and then a colorimetric loop-mediated isothermal amplification (LAMP) reaction is carried out on the extracted DNA. In vitro sensitivity was 1.9 x 10 2  CFU/mL, and regarding specificity, all nine S. agalactiae strains tested positive. All Streptococcus spp. tested negative, except for S. dysgalactiae, thereby indicating the need for another set of primers to distinguish this species from S. agalactiae. To diagnose S. agalactiae infections using FTA-e/LAMP in vivo, two experimental trials on juvenile Oreochromis niloticus infected with bovine or piscine strains were carried out. Sensitivity in symptomatic fish was 100%, and 50.7% of fish without signs were positive. All negative control fish tested negative (n = 28). No bacteria were detected after 16 days post-infection (dpi). Accuracy during the first week (1-7 dpi) was 89% and decreased to 44% thereafter (10-22 dpi). FTA-e/LAMP results suggest that this method is a promising tool for early and fast diagnosis of S. agalactiae on tilapia farms., (© 2021 John Wiley & Sons Ltd.)

Published

2021

8. Simultaneous detection of multiple bacterial and viral aquatic pathogens using a fluorogenic loop-mediated isothermal amplification-based dual-sample microfluidic chip.

Author

Zhou QJ, Lu JF, Su XR, Jin JL, Li SY, Zhou Y, Wang L, Shao XB, Wang YH, Yan MC, Li MY, and Chen J

Subjects

Animals, Crustacea microbiology, Crustacea virology, DNA Virus Infections diagnosis, DNA Virus Infections veterinary, DNA Virus Infections virology, Fish Diseases diagnosis, Fish Diseases microbiology, Fish Diseases virology, Fishes microbiology, Fishes virology, Gram-Negative Bacterial Infections diagnosis, Gram-Negative Bacterial Infections microbiology, Gram-Negative Bacterial Infections veterinary, Limit of Detection, Molecular Diagnostic Techniques methods, Mollusca microbiology, Mollusca virology, Nucleic Acid Amplification Techniques methods, Reproducibility of Results, Sensitivity and Specificity, Aeromonas hydrophila isolation & purification, Densovirinae isolation & purification, Edwardsiella tarda isolation & purification, Iridoviridae isolation & purification, Microfluidics methods, Molecular Diagnostic Techniques veterinary, Nucleic Acid Amplification Techniques veterinary, Vibrio isolation & purification, White spot syndrome virus 1 isolation & purification

Abstract

Rapid and user-friendly diagnostic tests are necessary for early diagnosis and immediate detection of diseases, particularly for on-site screening of pathogenic microorganisms in aquaculture. In this study, we developed a dual-sample microfluidic chip integrated with a real-time fluorogenic loop-mediated isothermal amplification assay (dual-sample on-chip LAMP) to simultaneously detect 10 pathogenic microorganisms, that is Aeromonas hydrophila, Edwardsiella tarda, Vibrio harveyi, V. alginolyticus, V. anguillarum, V. parahaemolyticus, V. vulnificus, infectious hypodermal and haematopoietic necrosis virus, infectious spleen and kidney necrosis virus, and white spot syndrome virus. This on-chip LAMP provided a nearly automated protocol that can analyse two samples simultaneously, and the tests achieved limits of detection (LOD) ranging from 10 0 to 10 -1  pg/μl for genomic DNA of tested bacteria and 10 -4 to 10 -5  pg/μl for recombinant plasmid DNA of tested viruses, with run times averaging less than 30 min. The coefficient of variation for the time-to-positive value was less than 10%, reflecting a robust reproducibility. The clinical sensitivity and specificity were 93.52% and 85.53%, respectively, compared to conventional microbiological or clinical methods. The on-chip LAMP assay provides an effective dual-sample and multiple pathogen analysis, and thus would be applicable to on-site detection and routine monitoring of multiple pathogens in aquaculture., (© 2020 John Wiley & Sons Ltd.)

Published

2021

9. Development of a real-time recombinase polymerase amplification assay for rapid detection of Aeromonas hydrophila.

Author

Qu Y, Wang Q, Li Y, Wang Y, Yin J, Ren Y, Liu C, Liu X, Wang Y, and Zeng W

Subjects

Animals, Fish Diseases virology, Gram-Negative Bacterial Infections diagnosis, Gram-Negative Bacterial Infections virology, Nucleic Acid Amplification Techniques methods, Aeromonas hydrophila isolation & purification, Fish Diseases diagnosis, Gram-Negative Bacterial Infections veterinary, Nucleic Acid Amplification Techniques veterinary

Abstract

Aeromonas hydrophila is ubiquitous in the aquaculture industry and a constant cause of severe disease and economic losses. The early diagnosis of these infections is crucial for disease surveillance and prevention. We developed a real-time recombinase polymerase amplification (real-time RPA) assay for detection of A. hydrophila using the haemolysin gene. The assay was performed at 37°C for 20 min and was highly specific with no cross-reaction with other fish pathogens or with other Aeromonas species. The assay detection limit was 10 2 copies of the Aeromonas hydrophila per reaction. Compared with traditional culture-based method or real-time PCR, the diagnostic sensitivity and specificity of the real-time RPA were 73.7 and 100%, as well as 64.7 and 93%. Our newly developed real-time RPA was specific and sensitive and can be used in large-scale and point-of-care field investigations of A. hydrophila infections to enable earlier diagnoses., (© 2020 John Wiley & Sons Ltd.)

Published

2021

10. Non-lethal loop-mediated isothermal amplification assay as a point-of-care diagnostics tool for Neoparamoeba perurans, the causative agent of amoebic gill disease.

Author

Cano I, McCullough R, Mulhearn B, Gunning S, Waine A, Joiner C, and Paley R

Subjects

Amebiasis diagnosis, Amebiasis parasitology, Animals, Fish Diseases parasitology, Gills parasitology, Nucleic Acid Amplification Techniques methods, Amebiasis veterinary, Amoebozoa isolation & purification, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques veterinary, Point-of-Care Systems, Salmo salar

Abstract

Neoparamoeba perurans is the causative agent of amoebic gill disease (AGD). Two loop-mediated isothermal amplification (LAMP) assays targeting the parasite 18S rRNA and the Atlantic salmon EF1α, used as internal control, were designed. The N. perurans LAMP assay did not amplify close relatives N. pemaquidensis and N. branchiphila, or the host DNA. This assay detected 10 6 copies of the parasite 18S rRNA gene under 13 min and 10 3 copies under 35 min. Five "fast-and-dirty" DNA extraction methods were compared with a reference method and further validated by TaqMan™ qPCR. Of those, the QuickExtract buffer was selected for field tests. Seventy-one non-lethal gill swabs were analysed from AGD-clinically infected Atlantic salmon. The pathogen was detected under 23 min in fish of gill score >2 and under 39 min for lower gill scores. About 1.6% of the tests were invalid (no amplification of the internal control). 100% of positives were obtained from swabs taken from fish showing gill score ˃3, but only ~50% of positives for lower gill scores. The present LAMP assay could be implemented as a point-of-care test for the on-site identification of N. perurans; however, further work is required to improve its performance for lower scores., (© 2020 Crown copyright. Journal of Fish Diseases published by John Wiley & Sons Ltd. This article is published with the permission of the Controller of HMSO and the Queen’s Printer for Scotland.)

Published

2020

11. Detection of Vibrio anguillarum and Vibrio alginolyticus by Singleplex and Duplex Loop-Mediated Isothermal Amplification (LAMP) Assays Targeted to groEL and fklB Genes.

Author

Siddique MP, Jang WJ, Lee JM, Hasan MT, Kim CH, and Kong IS

Subjects

Animals, Fish Diseases diagnosis, Humans, Vibrio genetics, Vibrio Infections diagnosis, Vibrio alginolyticus classification, Vibrio alginolyticus genetics, Bacterial Proteins genetics, Chaperonin 60 genetics, Fish Diseases microbiology, Nucleic Acid Amplification Techniques methods, Vibrio isolation & purification, Vibrio Infections microbiology, Vibrio Infections veterinary

Abstract

Singleplex and duplex loop-mediated isothermal amplification (LAMP) assays were developed for detecting Vibrio anguillarum, a major bacterial pathogen of fish, and Vibrio alginolyticus, a pathogen of fish and humans, separately and simultaneously from contaminated seawater by targeting the groEL gene of V. anguillarum, which encodes a molecular chaperone protein, and the fklB gene of V. alginolyticus, which encodes a 22 kilodalton (kDa) peptidyl prolyl isomerase. The optimal reaction conditions to produce consistent results were 65 °C for 30 min, 63 °C for 30 min, and 63 °C for 40 min for the groEL (singleplex for V. anguillarum), fklB (singleplex for V. alginolyticus), and groEL + flkB (duplex) LAMP assays, respectively, analyzed via visual detection methods (use of calcein, and SYBR Green I) and agarose gel electrophoresis. The assays were found to be species-specific, as closely related Vibrio spp. were not detected. The limits of detection (LoDs) of the LAMP assays for DNA template from pure culture and artificially contaminated seawater were 10 and 14 fg (groEL assay; for V. anguillarum), 12.5 and 17 fg (fklB assay; for V. alginolyticus), and 50 and 70 fg (duplex assay) per reaction, respectively, which were much better than the LoDs of conventional polymerase chain reaction (PCR). Singleplex and duplex LAMP assays were found to be rapid, species-specific, and sensitive for the detection of V. anguillarum and V. alginolyticus and are applicable to laboratory and field diagnostics.

Published

2019

12. Establishment of loop-mediated isothermal amplification for rapid and convenient detection of Mycobacterium marinum complex.

Author

Tsai MA, Wang PC, Yoshida S, Aono A, Mitarai S, Wada T, and Chen SC

Subjects

Animals, Buruli Ulcer diagnosis, Buruli Ulcer microbiology, DNA, Bacterial analysis, DNA, Bacterial genetics, Fish Diseases diagnosis, Fish Diseases microbiology, Genes, Bacterial genetics, Mycobacterium genetics, Mycobacterium isolation & purification, Mycobacterium marinum genetics, Sensitivity and Specificity, Water Microbiology, Mycobacterium marinum isolation & purification, Nucleic Acid Amplification Techniques methods

Abstract

Mycobacterium marinum is a zoonotic pathogen that can cause dermatological infection mainly from contaminated water or fish. Some well-known genetically similar species and subspecies are M. lifrandii and M. pseudoshottsii from amphibians and fish in aquaculture, and M. ulcerans, a causative agent of a neglected tropical disease (NTD), Buruli ulcer. They are believed to survive in water as their major niche, which might be related to their source of infection, but detailed ecological surveillance of the species complex remains to be done. Herein, we present a new detection system for M. marinum complex based on isothermal DNA amplification that can be conducted conveniently with high sensitivity and specificity. The target was a chromosomal gene, mrsA, including a restriction polymorphism between M. ulcerans (except for the most ancestral subspecies, M. ulcerans subsp. shinshuense) and the other species. The system was able to detect less than 500 fg (approximately 70 copies) of genomic DNA of M. marinum, within 60 min, and caused no amplification from mycobacterial species other than M. marinum complex species. It was also verified that restriction of the amplified DNA fragments was able to discriminate M. ulcerans as expected. This easy, quick, and convenient system is expected to facilitate detection of M. marinum complex from various resources., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

13. Development of a simple and rapid reverse transcription-loopmediated isothermal amplification (RT-LAMP) assay for sensitive detection of tilapia lake virus.

Author

Yin J, Wang Q, Wang Y, Li Y, Zeng W, Wu J, Ren Y, Tang Y, Gao C, Hu H, and Bergmann SM

Subjects

Animals, Aquaculture, DNA Primers genetics, DNA Virus Infections diagnosis, Fish Diseases virology, Lakes virology, RNA, Viral genetics, Reverse Transcription, Sensitivity and Specificity, Temperature, DNA Virus Infections veterinary, DNA Viruses isolation & purification, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques methods, Tilapia virology

Abstract

Recently, substantial mortality of farmed and wild tilapia caused by tilapia lake virus (TiLV) infection has been observed worldwide. However, sensitive and reliable diagnostic method is limited. A reverse transcription-loopmediated isothermal amplification (RT-LAMP) assay has been applied for the detection of TiLV nucleotide sequence. Six primers targeting two locations on the target gene based on a highly conserved sequence in the segment 1 (S1) region of the TiLV genome have been designed. The optimized RT-LAMP reaction was maintained at the isothermal condition of 63°C for 45 min. And the amplifications could be verified by turbidity or a colour change with the addition of SYBR Green I. Subsequently, RT-LAMP products could be observed by a ladder pattern following gel electrophoresis. The species-specific assay showed that the method was sensitive enough to detect as low as 1.6 copies of viral particle, and the assay was highly specific because no cross-reactivity was observed with other pathogens, and had a diagnostic sensitivity and specificity of 100% when TiLV-positive samples and non-target virus were tested. In summary, all the results demonstrate that this RT-LAMP is a rapid, effective and sensitive method for TiLV detection in tilapia aquaculture., (© 2019 John Wiley & Sons Ltd.)

Published

2019

14. Development of a loop-mediated isothermal amplification assay for the detection and quantification of epizootic epitheliotropic disease virus (salmonid herpesvirus-3).

Author

Zhang Q, Shavalier M, Standish I, Glenney GW, Loch TP, and Faisal M

Subjects

Animals, DNA, Viral genetics, Fish Diseases virology, Gills virology, Herpesviridae genetics, Herpesviridae Infections diagnosis, Sensitivity and Specificity, Skin virology, Temperature, Fish Diseases diagnosis, Herpesviridae isolation & purification, Herpesviridae Infections veterinary, Nucleic Acid Amplification Techniques methods, Trout virology

Abstract

Epizootic Epitheliotropic Disease Virus (EEDV; Salmonid Herpesvirus-3) causes a serious disease hatchery-reared lake trout (Salvelinus namaycush), threatening restoration efforts of this species in North America. The current inability to replicate EEDV in vitro necessitates the search for a reproducible, sensitive, and specific assay that allows for its detection and quantitation in a time- and cost-effective manner. Herein, we describe a loop-mediated isothermal amplification (LAMP) assay that was developed for the quantitative detection of EEDV in infected fish tissues. The newly developed LAMP reaction was optimized in the presence of calcein, and the best results were produced using 2 mM MgCl 2 , 1.8 mM dNTPs and at an incubation temperature of 67.1 °C. This method was highly specific to EEDV, as it showed no cross-reactivity with several fish viruses, including Salmonid Herpesvirus -1 , -2, -4, and -5, Infectious Pancreatic Necrosis Virus, Spring Viremia of Carp Virus, Infectious Hematopoietic Necrosis Virus, Golden Shiner Reovirus, Fathead Minnow Nidovirus, and Viral Hemorrhagic Septicemia Virus. The analytical sensitivity of the EEDV-LAMP method was estimated to be as low as 16 copies of plasmid per reaction. When infected fish tissue was used, a positive reaction could be obtained when an infected gill tissue sample that contained 430 viral copies/μg was diluted up to five orders of magnitude. The sensitivity and specificity of the newly developed LAMP assay compared to the SYBR Green qPCR assay were 84.3% and 93.3%, respectively. The quantitative LAMP for EEDV had a correlation coefficient (R 2  = 0.980), and did not differ significantly from the SYBR Green quantitative PCR assay (p > 0.05). Given its cost- and time-effectiveness, this quantitative LAMP assay is suitable for screening lake trout populations and for the initial diagnosis of clinical cases., (Copyright © 2018. Published by Elsevier B.V.)

Published

2019

15. An effective established biosensor of bifunctional probes-labeled AuNPs combined with LAMP for detection of fish pathogen Streptococcus iniae.

Author

Zhou Y, Xiao J, Ma X, Wang Q, and Zhang Y

Subjects

Animals, Bacterial Proteins analysis, Biosensing Techniques instrumentation, Fish Diseases microbiology, Limit of Detection, Sensitivity and Specificity, Streptococcal Infections diagnosis, Streptococcal Infections microbiology, Zebrafish, Aquaculture methods, Fish Diseases diagnosis, Gold chemistry, Metal Nanoparticles chemistry, Nucleic Acid Amplification Techniques, Streptococcal Infections veterinary, Streptococcus iniae isolation & purification

Abstract

In purpose of valid Streptococcus iniae detection, we established a colorimetric biosensor using gold nanoparticles (AuNPs) labeled with dual functional probes and along with loop-mediated isothermal amplification (LAMP) assay (LAMP-AuNPs). Based on the characteristics of self-aggregation and bio-conjugation with ligands, AuNPs were chosen for observable color change in tandem with LAMP amplification method to reach high sensitivity and easy operation. Meanwhile, the improvement of dual probes that could fully utilize the LAMP product gave the biosensor a stable result exhibition. LAMP-AuNPs targeting gene ftsB, one of the ATP transporter-related genes, turned out favorable specificity in cross reaction among other fish pathogens. The detect limit of 10 2 CFU revealed a better sensitivity compared with polymerase chain reaction (PCR) method and AuNPs lateral flow test strip (LFTS). It was also proved to be effective by zebrafish infection model trials with less than 2-h time consumption and nearly no devices which make it a convenient biosensor for point-to-care S. iniae detection.

Published

2018

16. Rapid detection and differentiation of carp oedema virus and cyprinid herpes virus-3 in koi and common carp.

Author

Soliman H and El-Matbouli M

Subjects

Animals, Fish Diseases virology, Herpesviridae classification, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Poxviridae classification, Poxviridae Infections diagnosis, Poxviridae Infections virology, Carps, Fish Diseases diagnosis, Herpesviridae isolation & purification, Herpesviridae Infections veterinary, Nucleic Acid Amplification Techniques veterinary, Poxviridae isolation & purification, Poxviridae Infections veterinary

Abstract

Carp oedema virus (CEV) and koi herpes virus (KHV) are of major concern to common carp breeders and koi enthusiasts worldwide. The viruses cause diseases that exhibit similar external signs; thus, it is difficult to distinguish between them clinically. In this study, we developed and optimized rapid and accurate single- and multiplex isothermal diagnostic tools, based on recombinase polymerase amplification (RPA), for detection and differentiation of CEV and KHV. The assays were combined with a lateral flow dipstick to enable visual detection of amplification products and simplify post-amplification analysis. Both CEV- and KHV-RPA assays were specific for their target virus. The lower detection limits of the assays were similar to those of established diagnostic PCR tests for the viruses. A sample preparation method was optimized to eliminate the need for total DNA extraction from fish tissues. The estimated time to perform these RPA assays, from receiving the sample to having a result, is 50 min, compared to 10 and 7 hr for CEV- and KHV-PCR tests, respectively. The assays can be performed in field situations to improve screening of fish and reduce spread of these viruses and thereby enhance the common carp and koi industries., (© 2018 John Wiley & Sons Ltd.)

Published

2018

17. Recombinase polymerase amplification assay combined with a lateral flow dipstick for rapid detection of Tetracapsuloides bryosalmonae, the causative agent of proliferative kidney disease in salmonids.

Author

Soliman H, Kumar G, and El-Matbouli M

Subjects

Animals, Fish Diseases parasitology, Kidney Diseases diagnosis, Kidney Diseases parasitology, Parasitic Diseases, Animal parasitology, Sensitivity and Specificity, Time Factors, Chromatography, Affinity methods, Fish Diseases diagnosis, Kidney Diseases veterinary, Myxozoa isolation & purification, Nucleic Acid Amplification Techniques methods, Parasitic Diseases, Animal diagnosis, Salmonidae

Abstract

Background: The myxozoan Tetracapsuloides bryosalmonae, the causative agent of proliferative kidney disease (PKD), is responsible for considerable losses in farmed and wild fish populations in Europe and North America. Recently, T. bryosalmonae was detected in many European countries, and strategy to control the disease in the wild and farmed fish population is yet to be developed. Recombinase polymerase amplification (RPA) is a novel isothermal nucleic acid amplification technology that does not require any thermal cycling, and lateral flow dipstick (LFD) is a rapid, cost-effective, and easy-to-handle assay that enables stable detection., Results: In this study, we developed and optimized a rapid and sensitive RPA assay combined with an LFD for the detection of T. bryosalmonae. The PKD-RPA assay was specific to T. bryosalmonae, as no cross-reaction or false positive signals were observed with any of the other tested DNAs. The developed PKD-RPA assay was ten times more sensitive than an existing diagnostic polymerase chain reaction (PCR) assay for this parasite. The estimated time to perform PKD-RPA assay is 25 min compared to 4 h for PKD-PCR assay., Conclusions: A novel PKD-RPA assay for the detection of T. bryosalmonae was developed. The assay offers considerable advantages including speed, sensitivity, specificity and visual detection. Applying the PKD-RPA assay combined with an LFD enhances the surveillance and early detection of T. bryosalmonae in salmonids.

Published

2018

18. Development of cross-priming amplification coupled with vertical flow visualization for rapid detection of infectious spleen and kidney necrosis virus (ISKNV) in mandarin fish, Siniperca chuatsi.

Author

Liu W, Zhou Y, Fan Y, Jiang N, Cain K, and Zeng L

Subjects

Animals, DNA, Viral, Iridoviridae classification, Reproducibility of Results, Sensitivity and Specificity, DNA Virus Infections veterinary, Fish Diseases diagnosis, Fish Diseases virology, Fishes virology, Iridoviridae genetics, Nucleic Acid Amplification Techniques

Abstract

Infectious spleen and kidney necrosis virus (ISKNV) has been recognized as the causative agent of the most serious disease in cultured mandarin fish, Siniperca chuatsi, in China. Disease outbreaks have resulted in substantial losses to the aquaculture industry. Currently, reliable laboratory detection and identification methods are available for this virus. However, rapid detection methods applicable for on-site diagnosis of this infectious agent are unavailable. To address this need, a nearly instrument-free, cost-effective and simple detection method was developed and optimized and incorporates cross priming amplification coupled with vertical flow visualization for rapid identification of ISKNV (ISKNV-CPA-VF). Results show that cross circulation amplification targeting the conserved region of the major capsid protein (MCP) regiment of the ISKNV genome had a sensitivity 10 times greater than traditional PCR at 64 °C within 60 min. The optimized concentration of dNTPs and the concentration for Mg 2+ were 1.0 mmol/L and 10 mmol/L, respectively. No cross-reactions with other viruses or bacteria were observed. When combined with the nucleic acid strip detection technology, visual detection of ISKNV amplified products was realized within 3-5 min following amplification. The simplicity and nearly instrument-free method for this ISKNV-CPA-VF assay shows great potential for on-site diagnostics of ISKNV infection in Siniperca chuatsi., (Copyright © 2017 Elsevier B.V. All rights reserved.)

Published

2018

19. Rapid and Sensitive Detection of Lymphocystis Disease Virus Genotype VII by Loop-Mediated Isothermal Amplification.

Author

Valverde EJ, Cano I, Castro D, Paley RK, and Borrego JJ

Subjects

Animals, DNA Primers genetics, DNA Virus Infections diagnosis, DNA Virus Infections virology, Fish Diseases diagnosis, Genotype, Iridoviridae classification, Iridoviridae genetics, Sea Bream virology, DNA Virus Infections veterinary, Fish Diseases virology, Iridoviridae isolation & purification, Nucleic Acid Amplification Techniques methods

Abstract

Lymphocystis disease virus (LCDV) infections have been described in gilthead seabream (Sparus aurata L.) and Senegalese sole (Solea senegalensis, Kaup), two of the most important marine fish species in the Mediterranean aquaculture. In this study, a rapid, specific, and sensitive detection method for LCDV genotype VII based on loop-mediated isothermal amplification (LAMP) was developed. The LAMP assay, performed using an apparatus with real-time amplification monitoring, was able to specifically detect LCDV genotype VII from clinically positive samples in less than 12 min. In addition, the assay allowed the detection of LCDV in all asymptomatic carrier fish analysed, identified by qPCR, showing an analytical sensitivity of ten copies of viral DNA per reaction. The LCDV LAMP assay has proven to be a promising diagnostic method that can be used easily in fish farms to detect the presence and spread of this iridovirus.

Published

2017

20. Electrochemical detection of Piscirickettsia salmonis genomic DNA from salmon samples using solid-phase recombinase polymerase amplification.

Author

Del Río JS, Svobodova M, Bustos P, Conejeros P, and O'Sullivan CK

Subjects

Animals, Biosensing Techniques instrumentation, Biotinylation, DNA Primers chemistry, Electrodes, Enzymes, Immobilized chemistry, Fish Diseases microbiology, Gold chemistry, Horseradish Peroxidase chemistry, Limit of Detection, Piscirickettsia isolation & purification, Piscirickettsiaceae Infections diagnosis, Piscirickettsiaceae Infections microbiology, Recombinases chemistry, Salmon microbiology, DNA, Bacterial analysis, Electrochemical Techniques, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques, Piscirickettsia genetics, Piscirickettsiaceae Infections veterinary

Abstract

Electrochemical detection of solid-phase isothermal recombinase polymerase amplification (RPA) of Piscirickettsia salmonis in salmon genomic DNA is reported. The electrochemical biosensor was constructed by surface functionalization of gold electrodes with a thiolated forward primer specific to the genomic region of interest. Solid-phase RPA and primer elongation were achieved in the presence of the specific target sequence and biotinylated reverse primers. The formation of the subsequent surface-tethered duplex amplicons was electrochemically monitored via addition of streptavidin-linked HRP upon completion of solid-phase RPA. Successful quantitative amplification and detection were achieved in less than 1 h at 37 °C, calibrating with PCR-amplified genomic DNA standards and achieving a limit of detection of 5 · 10 -8  μg ml -1 (3 · 10 3 copies in 10 μl). The presented system was applied to the analysis of eight real salmon samples, and the method was also compared to qPCR analysis, observing an excellent degree of correlation. Graphical abstract Schematic of use of electrochemical RPA for detection of Psiricketessia salmonis in salmon liver.

Published

2016

21. Shewanella putrefaciens in cultured tilapia detected by a new calcein-loop-mediated isothermal amplification (Ca-LAMP) method.

Author

Suebsing R, Kampeera J, Sirithammajak S, Pradeep PJ, Jitrakorn S, Arunrut N, Sangsuriya P, Saksmerprome V, Senapin S, Withyachumnarnkul B, and Kiatpathomchai W

Subjects

Animals, Aquaculture, Fish Diseases diagnosis, Gram-Negative Bacterial Infections diagnosis, Gram-Negative Bacterial Infections microbiology, Sensitivity and Specificity, Water Microbiology, Fish Diseases microbiology, Gram-Negative Bacterial Infections veterinary, Nucleic Acid Amplification Techniques methods, Shewanella putrefaciens isolation & purification, Tilapia

Abstract

Shewanella putrefaciens is being increasingly isolated from a wide variety of sources and is pathogenic to many marine and freshwater fish. For better control of this pathogen, there is a need for the development of simple and inexpensive but highly specific, sensitive, and rapid detection methods suitable for application in field laboratories. Our colorogenic loop-mediated isothermal amplification (LAMP) assay combined with calcein (Ca-LAMP) for unaided visual confirmation of LAMP amplicons is a simple method for fish pathogen detection in cultured tilapia. Here, we describe the detection of S. putrefaciens using the same platform. As before, the method gave positive results (orange to green color change) in 45 min at 63°C with sensitivity 100 times higher than that of a conventional PCR assay, with no cross-amplification of other known fish bacterial pathogens tested. Using the assay with 389 samples of gonads, fertilized eggs, and fry of farmed Nile and red tilapia Oreochromis spp., 35% of samples were positive for S. putrefaciens. The highest prevalence was found in samples of gonads (55%) and fertilized eggs (55%) from adult breeding stocks, indicating that S. putrefaciens could be passed on easily to fry used for stocking production ponds. Tissue tropism assays revealed that the spleen showed the highest colonization by S. putrefaciens in naturally infected tilapia and that it would be the most suitable organ for screening and monitoring fish stocks for presence of the bacteria.

Published

2015

22. Development and evaluation of a loop-mediated isothermal amplification assay for the detection of channel catfish virus.

Author

Liu GX, Lin L, Wang M, and Liu XQ

Subjects

Animals, Fish Diseases diagnosis, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Nucleic Acid Amplification Techniques methods, Fish Diseases virology, Herpesviridae Infections veterinary, Ictaluridae virology, Ictalurivirus genetics, Nucleic Acid Amplification Techniques veterinary

Published

2015

23. Establishment and application of cross-priming isothermal amplification coupled with lateral flow dipstick (CPA-LFD) for rapid and specific detection of red-spotted grouper nervous necrosis virus.

Author

Su ZD, Shi CY, Huang J, Shen GM, Li J, Wang SQ, and Fan C

Subjects

Animals, DNA Primers genetics, Fishes, Nodaviridae genetics, Sensitivity and Specificity, Temperature, Time Factors, Chromatography, Affinity methods, Fish Diseases diagnosis, Nodaviridae isolation & purification, Nucleic Acid Amplification Techniques methods, Point-of-Care Systems

Abstract

Background: Red-spotted grouper nervous necrosis virus (RGNNV) is an important pathogen that causes diseases in many species of fish in marine aquaculture. The larvae and juveniles are more easily infected by RGNNV and the cumulative mortality is as high as 100 % after being infected with RGNNV. This virus imposes a serious threat to aquaculture of grouper fry. This study aimed to establish a simple, accurate and highly sensitive method for rapid detection of RGNNV on the spot., Methods: In this study, the primers specifically targeting RGNNV were designed and cross-priming isothermal amplification (CPA) system was established. The product amplified by CPA was detected through visualization with lateral flow dipstick (LFD). Three important parameters, including the amplification temperature, the concentration of dNTPs and the concentration of Mg(2+) for the CPA system, were optimized. The sensitivity and specificity of this method for RGNNV were tested and compared with those of the conventional RT-PCR and real-time quantitative RT-PCR (qRT-PCR)., Results: The optimized conditions for the CPA amplification system were determined as follows: the optimal amplification temperature, the optimized concentration of dNTPs and the concentration for Mg(2+) were 69 °C, 1.2 mmol/L and 5 mmol/L, respectively. The lowest limit of detection (LLOD) of this method for RGNNV was 10(1) copies/μL of RNA sample, which was 10 times lower than that of conventional RT-PCR and comparable to that of RT-qPCR. This method was specific for RGNNV in combination with SJNNV and had no cross-reactions with 8 types of virus and bacterial strains tested. This method was successfully applied to detect RGNNV in fish samples., Conclusions: This study established a CPA-LFD method for detection of RGNNV. This method is simple and rapid with high sensitivity and good specificity and can be widely applied for rapid detection of this virus on the spot.

Published

2015

24. Colorimetric Method of Loop-Mediated Isothermal Amplification with the Pre-Addition of Calcein for Detecting Flavobacterium columnare and its Assessment in Tilapia Farms.

Author

Suebsing R, Kampeera J, Sirithammajak S, Withyachumnarnkul B, Turner W, and Kiatpathomchai W

Subjects

Animals, Aquaculture, Colorimetry methods, Fish Diseases diagnosis, Flavobacteriaceae Infections diagnosis, Flavobacteriaceae Infections microbiology, Flavobacterium classification, Colorimetry veterinary, Fish Diseases microbiology, Flavobacteriaceae Infections veterinary, Flavobacterium isolation & purification, Fluoresceins chemistry, Nucleic Acid Amplification Techniques veterinary, Tilapia

Abstract

Flavobacterium columnare, the causative agent of columnaris disease in fish, affects many economically important freshwater fish species. A colorimetric method of loop-mediated isothermal amplification with the pre-addition of calcein (LAMP-calcein) was developed and used to detect the presence of F. columnare in farmed tilapia (Nile Tilapia Oreochromis niloticus and red tilapia [Nile Tilapia × Mozambique Tilapia O. mossambicus]) and rearing water. The detection method, based on a change in color from orange to green, could be performed within 45 min at 63°C. The method was highly specific, as it had no cross-detections with 14 other bacterial species, including other fish pathogens and two Flavobacterium species. The method has a minimum detection limit of 2.2 × 10(2) F. columnare CFU; thus, it is about 10 times more sensitive than conventional PCR. With this method, F. columnare was detected in gonad, gill, and blood samples from apparently healthy tilapia broodstock as well as in samples of fertilized eggs, newly hatched fry, and rearing water. The bacteria isolated from the blood were further characterized biochemically and found to be phenotypically identical to F. columnare. The amplified products from the LAMP-calcein method had 97% homology with the DNA sequence of F. columnare.

Published

2015

25. Development of a loop-mediated isothermal amplification assay for rapid detection of Nocardia salmonicida, the causative agent of nocardiosis in fish.

Author

Xia L, Zhang H, Lu Y, Cai J, Wang B, and Jian J

Subjects

Animals, DNA Primers genetics, Electrophoresis, Agar Gel, Nocardia Infections microbiology, Polymerase Chain Reaction methods, RNA, Ribosomal, 16S, Sensitivity and Specificity, Fish Diseases diagnosis, Nocardia genetics, Nocardia isolation & purification, Nocardia Infections diagnosis, Nucleic Acid Amplification Techniques methods

Abstract

Nocardia salmonicida is one of the main pathogens of fish nocardiosis. The purpose of this study was to build a loop-mediated isothermal amplification (LAMP) method for the rapid and sensitive detection of N. salmonicida. A set of four primers were designed from the 16S-23S rRNA intergenic spacer region of N. salmonicida, and conditions for LAMP were optimized as incubating all the reagents for 60 min at 64°C. LAMP products were judged with agar gel electrophoresis as well as with the naked eye after the addition of SYBR Green I. Results showed the sensitivity of the LAMP assay was 1.68 × 10(3) CFU/ml (16.8 CFU per reaction) and 10-fold higher than that of PCR. The LAMP method was also effectively applied to detect N. salmonicida in diseased fish samples, and it may potentially facilitate the surveillance and early diagnosis of fish nocardiosis.

Published

2015

26. Detection of fish pathogens by loop-mediated isothermal amplification (LAMP) technique.

Author

Soliman H, Saleh M, and El-Matbouli M

Subjects

Animals, Nucleic Acid Amplification Techniques standards, Fish Diseases diagnosis, Fish Diseases etiology, Nucleic Acid Amplification Techniques methods

Abstract

Rapid detection of fish pathogens is mandatory for applying the crucial preventive and control measures to reduce fish losses and, consequently, minimize the economic impact of diseases on the fish farm owners. The currently used molecular diagnostic tools of fish infectious agents, such as PCR and RT-PCR, are sensitive and specific but still have some drawbacks. These tools are usually time consuming and laborious, need skilled persons, and require sophisticated devices to be performed. Therefore, next-generation tools for rapid diagnosis of fish infectious diseases were developed to conquer these shortages. One of these novel tools is the loop-mediated isothermal amplification (LAMP) technique. LAMP is considered a more advantageous tool than PCR because it needs only a heating block or a thermostatically controlled water bath as a source of constant temperature. It is considered to be more specific than the PCR assay as it uses 4-6 primers, which may diminish the occurrence of false-positive results. The time required for the amplification process by LAMP is ranging from 30 min to 1 h comparing to 3-5 h in the case of PCR. The visual detection methods coupled with the LAMP assay eliminates the post-run processing for detection of the amplification products. Its sensitivity is either comparable with the PCR or better than it. A variety of LAMP assays were developed for simple and rapid detection of a diversity of fish pathogens. Herein, we describe how to perform a LAMP assay and troubleshoot any potential problem arising during the process.

Published

2015

27. Development of a rapid cyprinid herpesvirus 2 detection method by loop-mediated isothermal amplification.

Author

Liang LG, Xie J, and Luo D

Subjects

Animals, DNA Primers genetics, Fish Diseases diagnosis, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Sensitivity and Specificity, Fish Diseases virology, Goldfish, Herpesviridae isolation & purification, Herpesviridae Infections veterinary, Nucleic Acid Amplification Techniques methods

Abstract

Cyprinid herpesvirus 2 (CyHV2) is a pathogen that causes severe disease and high mortality in goldfish and Prussian carp. We developed a six primer loop-mediated isothermal amplification (LAMP) assay targeting the intercapsomeric triplex protein gene. CyHV-2 DNA was 10-fold serially diluted (10(8)-10(0) copies μl(-1)) and was used as the template to determine primer sensitivity. LAMP assays were performed with DNA templates from other pathogens to determine specificity. The LAMP assay had an unequivocal detection limit of 10 copies μl(-1), which was 100 times lower than that of the polymerase chain reaction. Other pathogen strains were not amplified by the LAMP primers, indicating good specificity. SYBR Green I was added to visually detect the amplification products. Assay applicability was evaluated in 120 samples of Carassius auratus gibelio, and a positive rate of 92·5% was obtained. In conclusion, a conventional LAMP assay has high convenience, rapidity, sensitivity and specificity for detecting CyHV-2 in infected aquatic organisms. Significance and impact of the study: Herpesviral haematopoietic necrosis, caused by cyprinid herpesvirus 2 (CyHV-2), is a severe disease of goldfish and Prussian carp associated with high mortality. We developed a loop-mediated isothermal amplification (LAMP) assay to detect CyHV-2 at relatively low plasmid DNA copy levels. The results show that the LAMP assay has a number of advantages (simple, sensitive, rapid and specific) over the conventional polymerase chain reaction and can be applied in the laboratory and field. Particularly, the method is highly applicable to facilitate surveillance and early diagnosis of CyHV-2., (© 2014 The Society for Applied Microbiology.)

Published

2014

28. Development and evaluation of reverse transcription loop-mediated isothermal amplification assay for the detection of the fathead minnow nidovirus.

Author

Zhang Q, Standish I, Winters AD, Puzach C, Ulferts R, Ziebuhr J, and Faisal M

Subjects

Animals, Coronavirus Infections diagnosis, Coronavirus Infections virology, DNA Primers genetics, Fish Diseases virology, Nidovirales genetics, North America, Sensitivity and Specificity, Spike Glycoprotein, Coronavirus genetics, Coronavirus Infections veterinary, Cyprinidae virology, Fish Diseases diagnosis, Nidovirales isolation & purification, Nucleic Acid Amplification Techniques methods, Reverse Transcription, Viral Load methods

Abstract

Fathead minnow nidovirus (FHMNV) is a serious baitfish-pathogenic virus in North America. Studies to trace the spread of the virus and determine its host range are hampered by the absence of reliable diagnostic assays. In this study, a one-step, reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed that targets a region in the FHMNV spike protein gene. The assay was optimized, and the best results were obtained at 8 mM of Mg(2+) with an incubation time of 40 min at 63 °C in the presence of calcein. The analytical sensitivity of the RT-LAMP method was estimated to be as low as 5 viral copies and was 1000-fold more sensitive than the conventional reverse transcription polymerase chain reaction (RT-PCR) method. The diagnostic sensitivity and specificity of the developed RT-LAMP assay versus the RT-PCR assay was 100% and 95.7%, respectively. A quantitative RT-LAMP of FHMNV with a high correlation coefficient (r(2)=0.9926) was also developed and the result of quantitation of viral copies in tissue samples of infected fish showed that the viral loads of the infected fish tissue samples reached up to 4.7×10(10) copies per mg. It is anticipated that the developed RT-LAMP and quantitative RT-LAMP methods will be instrumental for diagnosis and surveillance of FHMNV., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2014

29. Development of loop-mediated isothermal amplification method for detection of Kudoa septempunctata (Myxozoa: Multivalvulida) in olive flounder (Paralichthys olivaceus).

Author

Jeon CH, Wi S, Song JY, Choi HS, and Kim JH

Subjects

Animals, Aquaculture, Fish Diseases parasitology, Muscles parasitology, Sensitivity and Specificity, Spores isolation & purification, Fish Diseases diagnosis, Flounder parasitology, Myxozoa isolation & purification, Nucleic Acid Amplification Techniques methods, Parasitic Diseases, Animal diagnosis

Abstract

A loop-mediated isothermal amplification (LAMP) assay was developed and validated for early, rapid, and sensitive detection of Kudoa septempunctata, a myxosporean parasite found in olive flounder (Paralichthys olivaceus). Recently, several outbreaks associated with ingestion of raw olive flounder muscles harboring mature K. septempunctata spores have been reported, and it is becoming obvious that fresh K. septempunctata spores can cause problems in humans when ingested. Thus, it is necessary to develop reliable detection method of K. septempunctata, to prevent outbreaks and ensure food safety. The LAMP assay has advantages over other molecular detection methods for detecting K. septempunctata in olive flounder muscle, in terms of simplicity, rapidity, and sensitivity. The reaction condition was optimized as 63 °C, 45 min, with three sets of specific primers. The results can be simply confirmed with the naked eye after adding SYBR Green I or by conventional electrophoresis followed by ethidium bromide staining. This LAMP assay did not show any cross-reaction with other kudoid myxosporeans (Kudoa lateolabracis, Kudoa thyrsites) can be found in olive flounder muscles and was validated by testing Kudoa septempunctata spore-spiked samples and field samples. The results showed that the LAMP assay is ten times more sensitive than the conventional polymerase chain reaction in this study and can be applied for early detection for monitoring and epidemiological studies of K. septempunctata in olive flounder aquaculture farms.

Published

2014

30. A loop-mediated isothermal amplification assay for rapid detection of cyprinid herpesvirus 2 in gibel carp (Carassius auratus gibelio).

Author

Zhang H, Zeng L, Fan Y, Zhou Y, Xu J, and Ma J

Subjects

Animals, Base Sequence, Fish Diseases virology, Goldfish, Molecular Sequence Data, Time Factors, Fish Diseases diagnosis, Fish Diseases genetics, Herpesviridae Infections diagnosis, Herpesviridae Infections genetics, Herpesvirus 2, Human genetics, Nucleic Acid Amplification Techniques methods

Abstract

A rapid and sensitive loop-mediated isothermal amplification (LAMP) assay for Cyprinid herpesvirus 2 (CyHV-2) detection in gibel carp was developed. Following cloning and sequencing of the putative DNA helicase gene of CyHV-2 isolate from China, a set of four specific primers was designed based on the sequence. The MgCl2 concentration and the reaction temperature were optimized to 6 mM, 64°C, respectively. LAMP products were detected by visual inspection of a color change due to addition of SYBR Green I stain. The specificity and sensitivity of the LAMP assay were determined. No cross-reaction was observed with other fish DNA viruses including eel herpesvirus, koi herpesvirus, and Chinese giant salamander iridovirus. The LAMP assay was found to be equally sensitive as nested PCR. A comparative evaluation of 10 fish samples using LAMP and nested PCR assays showed an overall correlation in positive and negative results for CyHV-2. These results indicate that the LAMP assay is simple, sensitive, and specific and has a great potential use for CyHV-2 detection in the laboratory and field.

Published

2014

31. Development and evaluation of a loop-mediated isothermal amplification assay for diagnosis of Cyprinid herpesvirus 2.

Author

He J, Shi X, Yu L, Zheng X, Lan W, Jia P, Wang J, and Liu H

Subjects

Animals, DNA Primers genetics, DNA, Viral genetics, Goldfish, Herpesviridae genetics, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Sensitivity and Specificity, DNA, Viral isolation & purification, Fish Diseases diagnosis, Fish Diseases virology, Herpesviridae isolation & purification, Herpesviridae Infections veterinary, Nucleic Acid Amplification Techniques methods

Abstract

Goldfish Haematopoietic Necrosis caused by Cyprinid herpesvirus 2 (CyHV-2) is a severe fish disease with high level of mortality. This is the first study on detection of this disease by loop-mediated isothermal amplification (LAMP). A set of six primers targeting terminase gene (accession no. EU349285.1) was determined after a serial of tests. Detection limit was 1.09 × 10(-4)μg/μL, which was superior to conventional PCR and real-time PCR. No cross reaction with 28 other viruses or bacteria commonly found in fish was observed. The application of commercial kit and instrument for the LAMP assay could reduce the risk of cross contamination, which is suitable for detection of infection under field conditions., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

32. Evaluation of colorimetric loop-mediated isothermal amplification assay for visual detection of Streptococcus agalactiae and Streptococcus iniae in tilapia.

Author

Suebsing R, Kampeera J, Tookdee B, Withyachumnarnkul B, Turner W, and Kiatpathomchai W

Subjects

Animals, Fish Diseases diagnosis, Streptococcal Infections diagnosis, Streptococcal Infections microbiology, Streptococcus genetics, Streptococcus agalactiae genetics, Streptococcus agalactiae isolation & purification, Tilapia microbiology, Colorimetry methods, Fish Diseases microbiology, Nucleic Acid Amplification Techniques methods, Streptococcal Infections veterinary, Streptococcus isolation & purification

Abstract

Unlabelled: Streptococcus agalactiae and Strep. iniae are bacterial pathogens that cause streptococcosis in many fish species. An accelerated colorimetric loop-mediated isothermal amplification (LAMP) assay with pre-addition of calcein was established, and the transmission and detection of Strep. agalactiae and Strep. iniae in tilapia under natural aquatic environment were investigated. A positive reaction was observed by a colour change from orange to green through the naked eyes after completion at 63°C for 30 min with 10 times higher sensitivity than that of nested PCR assays and without cross-amplification with other fish bacterial pathogens. All sample types of Nile and red tilapia (broodstock, fertilized egg, fry) were Strep. agalactiae- and Strep. iniae positive by this new method, implying that they could be vertically transmitted. With its application for screening broodstock and fry before stocking and for monitoring fish health in grow-out ponds, the method would become very useful in fish farming industry., Significance and Impact of the Study: The application of colorimetric LAMP with pre-addition of calcein offers simple, rapid and sensitive technique with applicability for small field laboratories. This technique explored the possible vertical transmission mode of Strep. agalactiae and Strep. iniae under natural aquatic environment. It could be such preliminary data provided for the screening broodstock before breeding and/or the specific-pathogen-free production., (© 2013 The Society for Applied Microbiology.)

Published

2013

33. Development of a rapid assay to detect the dinoflagellate Amyloodinium ocellatum using loop-mediated isothermal amplification (LAMP).

Author

Picón-Camacho SM, Thompson WP, Blaylock RB, and Lotz JM

Subjects

Animals, Base Sequence, DNA genetics, Fish Diseases diagnosis, Fish Diseases parasitology, Fishes, Nucleic Acid Amplification Techniques methods, Sensitivity and Specificity, Time Factors, Water parasitology, Dinoflagellida isolation & purification, Nucleic Acid Amplification Techniques veterinary

Abstract

Amyloodinium ocellatum is a highly pathogenic dinoflagellate parasite with global distribution that causes high mortalities in the culture of tropical and sub-tropical marine and estuarine fishes. Diagnosis typically occurs through gross examination following the onset of morbidity, at which point treatment is of limited benefit. In the present study, a new molecular diagnostic tool for the rapid detection of A. ocellatum (AO) was developed using the loop-mediated isothermal amplification method (LAMP). The AO-LAMP assay designed is highly specific using a set of four primers - two outer and two inner primers targeting six different regions on the 5' end of the Small Subunit rDNA region (SSU rDNA) of A. ocellatum. The AO-LAMP assay, optimized for 25-30 min at 62°C, amplified the DNA from A. ocellatum extracted from both water and gill tissue samples and did not amplify DNA from four closely related dinoflagellate sp ecies. The detection limit of the AO-LAMP assay was 10 fg, exceptionally higher than the conventional PCR (1 pg). In addition, the standardized AO-LAMP assay was capable of detecting single tomonts and trophonts; the assay was not affected by the presence of possible inhibitory substances present in environmental water samples or gill samples. The AO-LAMP assay developed in the present study provides a novel useful tool for the simple, rapid and sensitive detection of A. ocellatum in water and gill tissue samples, which could assist in the early detection and improved control of A. ocellatum infections in aquaculture systems., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

34. Specific and rapid diagnosis of Edwardsiella tarda by a novel loop-mediated isothermal amplification targeting the upstream region of hlyb gene.

Author

Xie GS, Huang J, Zhang QL, Shi CY, Wang XH, and Liu QH

Subjects

Animals, Base Sequence, Enterobacteriaceae Infections diagnosis, Enterobacteriaceae Infections microbiology, Fish Diseases diagnosis, Fish Diseases microbiology, Fishes, Gene Expression Regulation, Bacterial, Molecular Structure, Nucleic Acid Amplification Techniques methods, Sensitivity and Specificity, Species Specificity, Bacterial Proteins genetics, Carrier Proteins genetics, Edwardsiella tarda genetics, Edwardsiella tarda isolation & purification, Enterobacteriaceae Infections veterinary, Hemolysin Proteins genetics, Nucleic Acid Amplification Techniques veterinary

Abstract

Edwardsiella tarda has become one of the most severe pathogens in aquaculture industries throughout the world; therefore, a specific and rapid identification method for this bacterium is urgently needed. In the present study, a novel loop-mediated isothermal amplification (LAMP) was developed by targeting the upstream region of the hlyb gene of E. tarda, which was then named as UH-LAMP. The Mg(2+) concentrations, the reaction temperature, and the reaction time of UH-LAMP were optimized to 10 mM, 65°C, and 45 min, respectively. The detection limit of the UH-LAMP was 100-times higher than that of conventional polymerase chain reaction (10 versus 1000 CFU/test). Furthermore, the new UH-LAMP assay showed no cross-reactivity to the E. ictaluri belonging to the other species in the genus Edwardsiella. The high specificity of the assay was also confirmed by testing the nine strains of E. tarda collected from different geographical locations and the other 20 bacteria species. The assay can be performed in a simple water bath or a heat block and the detection result can be visualized by adding a fluorescent reagent to the reaction mixture. Taken together, our preliminary results indicate that this UH-LAMP assay provided a rapid, sensitive, and species-specific diagnostic tool for E. tarda and can easily be applied for the diagnosis under clinical or onsite conditions.

Published

2013

35. Development of a reverse transcription loop-mediated isothermal amplification assay for detecting nervous necrosis virus in olive flounder Paralichthys olivaceus.

Author

Suebsing R, Oh MJ, and Kim JH

Subjects

Animals, Clinical Laboratory Techniques economics, DNA Primers genetics, Fish Diseases epidemiology, Fish Diseases virology, Nucleic Acid Amplification Techniques economics, Prevalence, RNA Virus Infections diagnosis, RNA Virus Infections epidemiology, RNA Virus Infections virology, Republic of Korea epidemiology, Sensitivity and Specificity, Time Factors, Veterinary Medicine economics, Virology economics, Virology methods, Clinical Laboratory Techniques methods, Fish Diseases diagnosis, Flatfishes virology, Nodaviridae isolation & purification, Nucleic Acid Amplification Techniques methods, RNA Virus Infections veterinary, Veterinary Medicine methods

Abstract

In this study, a reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed for the rapid, sensitive, and inexpensive detection of nervous necrosis virus (NNV) in olive flounder, Paralichthys olivaceus, in Korea. A set of six specific primers was designed to target the RNA 2 gene encoding the coat protein of Korean NNV strains. The RT-LAMP reaction successfully detected NNV after 30 min at 65 degrees C. When the sensitivities among RT-LAMP, RT-PCR, and nested RTPCR were compared, the RT-LAMP was shown to be able to detect the RNA template at 2.58 × 10(-2) TCID50/ml, whereas the RT-PCR and nested RT-PCR were only able to detect the RNA template at 2.58 × 10(2) TCID50/ml and 2.58 TCID50/ml, respectively. Thus, the sensitivity of the RT-LAMP assay was higher than those of the RT-PCR assays. In the specificity test of the RT-LAMP, 2 genotypes of NNVs (SJNNV and RGNNV) were positive; however, no other fish viruses were positive with the primers, indicating that the RT-LAMP assay is only specific to NNV. A total of 102 olive flounder were collected from hatcheries between 2009 and 2011. The occurrence of NNV in olive flounder was determined to be 53.9% (55/ 102) by the RT-LAMP. On the other hand, the prevalence based on the nested RT-PCR and RT-PCR results was 33.8% (34/102) and 20.6% (21/102), respectively. This result indicates that the RT-LAMP assay developed in this study is suitable for early field diagnosis of NNV with high sensitivity.

Published

2012

36. Development of a visual loop-mediated isothermal amplification method for rapid detection of the bacterial pathogen Pseudomonas putida of the large yellow croaker (Pseudosciaena crocea).

Author

Mao Z, Qiu Y, Zheng L, Chen J, and Yang J

Subjects

Animals, China, DNA Primers genetics, DNA, Bacterial chemistry, DNA, Bacterial genetics, Fish Diseases microbiology, Molecular Sequence Data, Pseudomonas Infections diagnosis, Sensitivity and Specificity, Sequence Analysis, DNA, Veterinary Medicine methods, Bacteriological Techniques methods, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques methods, Perciformes microbiology, Pseudomonas Infections veterinary, Pseudomonas putida genetics, Pseudomonas putida isolation & purification

Abstract

In recent years, the large yellow croaker (Pseudosciaena crocea), an important marine fish farmed in the coastal areas of Zhejiang province, east China, has become severely endangered as a result of the bacterial pathogen Pseudomonas putida. This paper reports the development of a visual loop-mediated isothermal amplification (LAMP) assay for rapid detection of the pathogen. Four primers, F3, B3, FIP and BIP, were designed on the basis of DNA sequence of the rpoN gene of P. putida. After optimization of the reaction conditions, the detection limit of LAMP assay was 4.8cfu per reaction, 10-fold higher than that of conventional PCR. The assay showed high specificity to discriminate all P. putida isolates from nine other Gram-negative bacteria. The assay also successfully detected the pathogen DNA in the tissues of infected fish. For visual LAMP without cross-contamination, SYBR Green I was embedded in a microcrystalline wax capsule and preset in the reaction tubes; after the reaction the wax was melted at 85°C to release the dye and allow intercalation with the amplicons. The simple, highly sensitive, highly specific and cost-effective characteristics of visual LAMP may encourage its application in the rapid diagnosis of this pathogen., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

37. Development of loop-mediated isothermal amplification method for rapid detection of Streptococcus iniae, the causative agent of streptococcicosis in fish.

Author

Cai SH, Wang B, Lu YS, Jian JC, and Wu ZH

Subjects

Animals, Aquaculture, Base Sequence, DNA Primers genetics, DNA, Bacterial isolation & purification, Fish Diseases microbiology, Fishes microbiology, Sensitivity and Specificity, Streptococcus genetics, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques methods, Streptococcus isolation & purification

Abstract

Streptococcus iniae is a major pathogen that causes sever economic losses in tilapia aquaculture. A set of four specific primers was designed by targeting lctO gene. With Bst DNA polymerase, the target DNA can be clearly amplified for 60 min at 64 °C in a simple water bath. The sensitivity of the LAMP assay for the detection of S. iniae is about 12.4 cells per reaction in both of pure cultures and added fish tissues cultures. LAMP products could be judged with agar gel or naked eye after addition of SYBR Green I. There were no cross-reactions with other bacterial strains indicating high specificity of the LAMP. The LAMP method was also applied to detect S. iniae-infected tilapia tissues effectively. The LAMP assay reported here indicates the potential usefulness of the technique as a valuable simple, rapid alternative procedure for the detection of S. iniae during streptococcicosis monitoring of cultured fish., (Copyright © 2012 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2012

38. Genomics and molecular genetics of Clonorchis sinensis: current status and perspectives.

Author

Huang SY, Zhao GH, Fu BQ, Xu MJ, Wang CR, Wu SM, Zou FC, and Zhu XQ

Subjects

Animals, Clonorchiasis epidemiology, Clonorchiasis parasitology, Clonorchiasis prevention & control, Expressed Sequence Tags, Fish Diseases diagnosis, Fish Diseases epidemiology, Fishes parasitology, Genetic Variation, Humans, MicroRNAs analysis, Nucleic Acid Amplification Techniques veterinary, Nucleic Acids analysis, Polymerase Chain Reaction veterinary, Snails parasitology, Transcriptome, Clonorchiasis diagnosis, Clonorchis sinensis genetics, Genome, Helminth, Molecular Sequence Annotation methods, Nucleic Acid Amplification Techniques methods, Polymerase Chain Reaction methods

Abstract

Clonorchiasis caused by Clonorchis sinensis is an important foodborne parasitosis of humans and animals, and is predominantly a hepatobiliary disease. Globally, nearly 35 million people were infected with C. sinensis, with approximately 15 million being in China. Patients would chronically present fatigue, jaundice, abdominal discomfort, along with the increased risk of developing into a form of cholangiocarcinoma that is fatal to humans. Treatment of clonorchiasis by praziquantel has been very successful, but this is dependent on early accurate diagnosis and correct species identification. The present article reviews the current status of knowledge in genomics and functional genomics of C. sinensis, and summarizes the main DNA-based techniques for the specific diagnosis of C. sinensis infection and studies of genetic variation in C. sinensis, and provides perspectives for future studies. The advances in genomics and molecular genetics of C. sinensis shed new sight on our understanding of population structure of C. sinensis as well as the prevention and control of clonorchiasis., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published

2012

39. Evaluation of rapid and sensitive reverse transcription loop-mediated isothermal amplification method for detecting infectious pancreatic necrosis virus in chum salmon (Oncorhynchus keta).

Author

Suebsing R, Oh MJ, and Kim JH

Subjects

Animals, Base Sequence, Birnaviridae Infections diagnosis, Birnaviridae Infections virology, Fish Diseases virology, Infectious pancreatic necrosis virus genetics, Nucleic Acid Amplification Techniques methods, RNA, Viral genetics, Sensitivity and Specificity, Time Factors, Birnaviridae Infections veterinary, Fish Diseases diagnosis, Infectious pancreatic necrosis virus isolation & purification, Nucleic Acid Amplification Techniques veterinary, Oncorhynchus keta

Abstract

Reverse transcription loop-mediated isothermal amplification (RT-LAMP) was developed for detecting Infectious pancreatic necrosis virus (IPNV) in chum salmon (Oncorhynchus keta) in Korea. The RT-LAMP is a novel approach of nucleic acid gene amplification with high specificity, sensitivity, and rapidity under isothermal conditions. Based on the VP2/NS gene sequence of VR-299 and Jasper strains, a set of 6 IPNV-specific primers was designed to recognize 8 diverse sequences of the IPNV RNA. The assay was successfully optimized to detect IPNV at 65°C in 30 min. The detection limit was 0.075 tissue culture infectious dose infecting 50% of inoculated cultures per milliliter (TCID(50)/ml) from IPNV-infected rainbow trout gonad (RTG)-2 cells, whereas nested reverse transcription polymerase chain reaction (nRT-PCR) had a sensitivity of 7.5 TCID(50)/ml. Using RT-LAMP assay, field samples were analyzed and the results compared with those of nRT-PCR assay. Two hundred and sixty-six out of 659 (40.4%) samples were IPNV-positive by RT-LAMP, whereas 182 of 659 samples (27.6%) were IPNV-positive by nRT-PCR. The results indicate that RT-LAMP can be a useful tool for early field diagnosis of IPNV.

Published

2011

40. Rapid and sensitive detection of Streptococcus iniae by loop-mediated isothermal amplification (LAMP).

Author

Han HJ, Jung SJ, Oh MJ, and Kim DH

Subjects

Animals, DNA, Bacterial isolation & purification, Fish Diseases microbiology, Fishes microbiology, Limit of Detection, Nucleic Acid Amplification Techniques methods, Sensitivity and Specificity, Streptococcal Infections diagnosis, Streptococcus genetics, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques veterinary, Streptococcal Infections veterinary, Streptococcus isolation & purification

Published

2011

41. Reverse transcriptase loop-mediated isothermal amplification assay for infectious hematopoietic necrosis virus in Oncorhynchus keta.

Author

Suebsing R, Jeon CH, Oh MJ, and Kim JH

Subjects

Animals, Cell Line, Fish Diseases diagnosis, Reverse Transcriptase Polymerase Chain Reaction veterinary, Rhabdoviridae Infections diagnosis, Rhabdoviridae Infections virology, Sensitivity and Specificity, Fish Diseases virology, Infectious hematopoietic necrosis virus, Nucleic Acid Amplification Techniques veterinary, Oncorhynchus keta, Rhabdoviridae Infections veterinary

Abstract

A reverse transcriptase loop-mediated isothermal amplification (RT-LAMP) assay was developed for detecting infectious hematopoietic necrosis virus (IHNV) from chum salmon Oncorhynchus keta in South Korea with high specificity, sensitivity and rapidity. A set of 6 IHNV-specific primers was designed, based on the G-protein sequence of IHNV (PRT strain), recognizing 8 distinct sequences of the target RNA. The assay was optimized to detect IHNV at 63 degrees C for 30 min. The limit of detection was 0.01 fg of RNA extracted from IHNV-infected CHSE-214 cells, compared with 1.0 fg for nested RT-PCR. The applicability of this RT-LAMP assay was further tested by comparison with nested RT-PCR using field samples. Of 473 samples tested, 191 samples (40.38%) were IHNV-positive by RT-LAMP, whereas 162 samples (34.25%) were IHNV-positive by nested RT-PCR. These results indicate that, because of its high sensitivity and rapidity, the RT-LAMP assay is useful for early diagnosis of IHN.

Published

2011

42. An integrated microfluidic loop-mediated-isothermal-amplification system for rapid sample pre-treatment and detection of viruses.

Author

Wang CH, Lien KY, Wang TY, Chen TY, and Lee GB

Subjects

Animals, Biosensing Techniques instrumentation, Equipment Design, Equipment Failure Analysis, Fish Diseases diagnosis, Nodaviridae genetics, Systems Integration, Temperature, Fish Diseases virology, Microfluidic Analytical Techniques instrumentation, Nodaviridae isolation & purification, Nucleic Acid Amplification Techniques instrumentation, RNA, Viral genetics, RNA, Viral isolation & purification, Viral Load instrumentation

Abstract

This study presents a novel automatic assay for targeted ribonucleic acid (RNA) extraction and a one-step reverse transcription loop-mediated-isothermal-amplification (RT-LAMP) process for the rapid detection of viruses from tissue samples by utilizing an integrated microfluidic system. By utilizing specific probe-conjugated magnetic beads, target RNA samples can be specifically recognized and hybridized onto the surface of the magnetic beads which are mixed with whole tissue lysates, followed by the synthesis of complementary deoxyribonucleic acid (cDNA) and isothermal amplification of target genes simultaneously with the incorporation of two specific primer sets. The nervous necrosis virus (NNV), the most common aquaculture pathogen, with a mortality rate in infected fish ranging from 80% to 100%, has been selected to verify the performance of the developed miniature system. Experimental results showed that the sensitivity of the integrated microfluidic LAMP system is about 100-fold higher when compared to a conventional one-step reverse-transcript polymerase chain reaction (RT-PCR) process. Significantly, the entire protocol from sample pre-treatment to target gene amplification can be completed within 60 min in an automatic manner without cross-reactions with other tested virus, bacteria and eukaryotic cells. Consequently, this integrated microfluidic LAMP system may provide a powerful platform for rapid purification and detection of virus samples., (Copyright © 2010 Elsevier B.V. All rights reserved.)

Published

2011

43. Sensitive and rapid detection of Clonorchis sinensis infection in fish by loop-mediated isothermal amplification (LAMP).

Author

Cai XQ, Xu MJ, Wang YH, Qiu DY, Liu GX, Lin A, Tang JD, Zhang RL, and Zhu XQ

Subjects

Animals, Cathepsin B genetics, Clonorchiasis diagnosis, DNA Primers genetics, Fish Diseases parasitology, Fishes, Helminth Proteins genetics, Sensitivity and Specificity, Clonorchiasis veterinary, Clonorchis sinensis isolation & purification, Fish Diseases diagnosis, Nucleic Acid Amplification Techniques methods, Parasitology methods

Abstract

The fish-borne clonorchiasis caused by the oriental liver fluke Clonorchis sinensis is endemic in a number of countries with over 35 million people being infected globally. Rapid and accurate detection of C. sinensis in its intermediate host fish is important for the control and prevention of clonorchiasis in areas where the disease is endemic. In the present study, we established a loop-mediated isothermal amplification (LAMP) approach for the sensitive and rapid detection of C. sinensis metacercariae in fish. The specificity and sensitivity of primers designed from the C. sinensis cathepsins B3 gene were evaluated, and specific amplification products were obtained with C. sinensis, while no amplification products were detected with DNA of related trematodes, demonstrating the specificity of the assay. The LAMP assay was proved to be 100 times more sensitive than a conventional polymerase chain reaction for detection of C. sinensis. The established LAMP assay provides a useful tool for the rapid and sensitive detection of C. sinensis in fish, which has important implications for the effective control of human clonorchiasis.

Published

2010

44. Rapid and sensitive detection of infectious spleen and kidney necrosis virus by loop-mediated isothermal amplification combined with a lateral flow dipstick.

Author

Ding WC, Chen J, Shi YH, Lu XJ, and Li MY

Subjects

Animals, DNA Primers genetics, DNA Virus Infections diagnosis, DNA Virus Infections virology, DNA, Viral genetics, Fish Diseases virology, Iridoviridae genetics, Molecular Sequence Data, Sensitivity and Specificity, Sequence Analysis, DNA, Time Factors, DNA Virus Infections veterinary, Fish Diseases diagnosis, Iridoviridae isolation & purification, Molecular Diagnostic Techniques methods, Nucleic Acid Amplification Techniques methods

Abstract

Loop-mediated isothermal amplification (LAMP) allows rapid amplification of nucleic acids under isothermal conditions. In this report, a 20-min LAMP amplification of the DPOL gene of infectious spleen and kidney necrosis virus (ISKNV) using a biotin-labeled primer was combined with lateral flow dipstick (LFD) chromatography for rapid and simple visual detection of ISKNV-specific amplicons. The LFD process involves a 5-min specific hybridization with an FITC-labeled DNA probe to confirm the presence of complement ISKNV amplicons that were biotinated in LAMP. The resulting DNA duplexes, consisting of labeled probes and amplicons, migrate along the LFD strip by chromatography for 5 min and are trapped at the test line and visualized by biotin labeling. The detection limit of ISKNV by LAMP-LFD was 10 copies. The results show that the LAMP-LFD method has the advantages of better sensitivity and speed and less dependence on equipment than the standard PCR for specifically detecting low levels of ISKNV DNA, and this can be useful in the field as a routine diagnostic tool.

Published

2010

45. Development and evaluation of a loop-mediated isothermal amplification assay for rapid detection of lymphocystis disease virus.

Author

Li Q, Yue Z, Liu H, Liang C, Zheng X, Zhao Y, Chen X, Xiao X, and Chen C

Subjects

Animals, Benzothiazoles, Capsid Proteins genetics, DNA Primers genetics, DNA Virus Infections diagnosis, Diamines, Electrophoresis, Agar Gel, Fish Diseases virology, Fluorescent Dyes pharmacology, Iridoviridae genetics, Organic Chemicals pharmacology, Quinolines, Sensitivity and Specificity, Staining and Labeling methods, Temperature, Time Factors, DNA Virus Infections veterinary, Fish Diseases diagnosis, Flatfishes virology, Iridoviridae isolation & purification, Nucleic Acid Amplification Techniques methods

Abstract

A loop-mediated isothermal amplification (LAMP) assay was developed for the detection of lymphocystis disease virus (LCDV). A set of five specific primers, two inner and two outer primers and a loop primer, were designed on the basis of the major capsid protein gene of LCDV. The reaction time and temperatures were optimized for 60 min at 63 degrees C, respectively. LAMP amplification products were detected by a ladder-like appearance on agarose gel electrophoresis or a naked-eye inspection of a color change in the reaction tube by addition of SYBR Green I. The assay was specific for LCDV, and there was no cross-reactivity with white spot syndrome virus (WSSV) or six other Iridoviridae viruses (epizootic hematopoietic necrosis virus, EHNV; tiger frog virus, TFV; Bohle iridovirus, BIV; soft-shelled turtle iridovirus, STIV; infectious spleen and kidney necrosis virus, ISKNV; red sea bream iridovirus, RSIV). The detection limit of the LAMP assay was 15 fg, which was similar to that of real-time quantitative polymerase chain reaction (PCR) and 10-fold higher than the conventional PCR. The LAMP assay was evaluated using 109 clinical samples, and the results indicated the suitability and simplicity of the test as a rapid, field diagnostic tool for detection of LCDV. The LCDV LAMP assay has potential for early diagnosis of LCDV infection., (2009 Elsevier B.V. All rights reserved.)

Published

2010

46. Immunocapture and direct binding loop mediated isothermal amplification simplify molecular diagnosis of Cyprinid herpesvirus-3.

Author

Soliman H and El-Matbouli M

Subjects

Animals, Aquaculture, Fish Diseases virology, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Sensitivity and Specificity, Time Factors, Carps virology, Fish Diseases diagnosis, Herpesviridae classification, Herpesviridae genetics, Herpesviridae immunology, Herpesviridae isolation & purification, Herpesviridae Infections veterinary, Nucleic Acid Amplification Techniques methods

Abstract

Loop mediated isothermal amplification (LAMP) assay is used for rapid diagnosis of Cyprinid herpesvirus-3, formerly designated koi herpesvirus (KHV), with comparable sensitivity to PCR. To reduce the time required for the LAMP assay, an immunocapture (IC) and direct binding (DB) techniques were developed to exclude the DNA extraction step in molecular diagnostic procedures of the virus. Both techniques were evaluated by using PCR and CyHV-3-LAMP assays. The DB-LAMP/PCR assays were more sensitive (detecting 0.1 virus particles/ml) than the IC-LAMP/PCR assays (detecting 1 virus particle/ml). By using the SYBR Green I stain and the DB/LAMP assay the complete CyHV-3 diagnostic process can be achieved within 90 min compared to more than 5 h for the routine PCR assay. Both assays (IC/DB) could amplify successfully CyHV-3 from clinical samples which prove its application to diagnostic tests. The DB-LAMP assay is a simple, rapid, sensitive technique and applicable to the diagnosis of CyHV-3 in the field.

Published

2009

47. Reverse transcription loop-mediated isothermal amplification for rapid and sensitive detection of nervous necrosis virus in groupers.

Author

Sung CH and Lu JK

Subjects

Animals, DNA Primers genetics, Fish Diseases virology, Fishes, Nodaviridae genetics, RNA Virus Infections diagnosis, RNA Virus Infections virology, Sensitivity and Specificity, Temperature, Time Factors, Fish Diseases diagnosis, Nodaviridae isolation & purification, Nucleic Acid Amplification Techniques methods, RNA Virus Infections veterinary

Abstract

The reverse transcription loop-mediated isothermal amplification (RT-LAMP) method is a sensitive nucleic acid diagnostic method that can amplify rapidly a target template; it can be applied for the diagnosis of viral disease in grouper aquaculture. In this study, two outer and two inner primers were designed from nervous necrosis virus (NNV) coat protein gene sequence. The reaction temperature and time for the detection of NNV were optimized at 65 degrees C for 60min. The detection limit of RT-LAMP is 10(-6) NNV-RNA from infected groupers, and more sensitive than the one-step RT-PCR and nested RT-PCR. The combination of RNA rapid extraction and RT-LAMP, the process can be completed within 2h. Thus, the RT-LMAP is a rapid, sensitive, specific and efficient method for detection of NNV in groupers.

Published

2009

48. Rapid, sensitive and simple detection method for koi herpesvirus using loop-mediated isothermal amplification.

Author

Yoshino M, Watari H, Kojima T, Ikedo M, and Kurita J

Subjects

Animals, Base Sequence, DNA Primers, DNA, Viral analysis, Deoxyribonucleases, Type II Site-Specific, Diphosphates, Fish Diseases virology, Gills virology, Herpesviridae genetics, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Magnesium Compounds, Molecular Sequence Data, Polymerase Chain Reaction, Sensitivity and Specificity, Time Factors, Carps virology, Fish Diseases diagnosis, Herpesviridae isolation & purification, Herpesviridae Infections veterinary, Nucleic Acid Amplification Techniques methods

Abstract

New methods were developed for the detection of koi herpesvirus (KHV, CyHV-3) by LAMP, which were compared with the PCR for specificity and sensitivity. We designed two primer sets targeting a specific sequence within the 9/5 PCR amplicon (9/5 LAMP) and the upper region of the SphI-5 PCR amplicon (SphI-5 LAMP), including a sequence highly conserved among the strains. The amplification was monitored in real-time based on the increase in turbidity, with magnesium pyrophosphate as the by-product. The reactions were carried out under isothermal conditions at 65 degrees C for 60 min. The detection limit of both LAMP was six copies, equal to the modified SphI-5 PCR. No cross-reactivity with other fish pathogenic viruses and bacteria was observed. SphI-5 LAMP was found to have a quicker response in terms of the reaction velocity than 9/5 LAMP. Therefore, we consider SphI-5 LAMP to be superior for routine use. Additionally, LAMP was found applicable to crude extract from gills and other organs. LAMP methods are superior in terms of sensitivity, specificity, rapidity and simplicity, and are potentially a valuable diagnostic tool for KHV infections.

Published

2009

49. A sensitive loop-mediated isothermal amplification (LAMP) method for detection of Renibacterium salmoninarum, causative agent of bacterial kidney disease in salmonids.

Author

Gahlawat SK, Ellis AE, and Collet B

Subjects

Actinomycetales Infections diagnosis, Actinomycetales Infections microbiology, Animals, Base Sequence, DNA Primers genetics, Kidney microbiology, Molecular Sequence Data, Nucleic Acid Amplification Techniques methods, Sensitivity and Specificity, Actinomycetales Infections veterinary, Fish Diseases diagnosis, Fish Diseases microbiology, Micrococcaceae genetics, Nucleic Acid Amplification Techniques veterinary, Salmonidae

Abstract

Loop-mediated isothermal amplification (LAMP) is a novel technique for nucleic acid amplification with high specificity, sensitivity and rapidity and does not require expensive equipment or reagents. In the present study, we developed and evaluated a LAMP method for the rapid detection of Renibacterium salmoninarum causing the bacterial kidney disease in salmonids. This method was more sensitive than quantitative real-time polymerase chain reaction (qPCR). Using DNA template extracted from cultured R. salmoninarum, the LAMP method gave an amplification signal from template diluted to 10(-8) while the limit of detection of qPCR was10(-7). The LAMP method was also highly specific and did not amplify DNA purified from five other Gram-positive and -negative bacterial fish pathogens. The method also worked well using extracts of macrophages infected with R. salmoninarum and kidney material from rainbow trout, which were positive for R. salmoninarum by qPCR and crude R. salmoninarum culture. There was some evidence for inhibitors of the LAMP reaction in the kidney samples, which was overcome by diluting the sample.

Published

2009

50. Rapid diagnosis of turbot reddish body iridovirus in turbot using the loop-mediated isothermal amplification method.

Author

Zhang Q, Shi C, Huang J, Jia K, Chen X, and Liu H

Subjects

Amino Acid Sequence, Animals, Base Sequence, China, DNA Primers genetics, DNA Virus Infections virology, Enzyme Activators pharmacology, Fish Diseases virology, Iridoviridae genetics, Magnesium pharmacology, Molecular Sequence Data, Sensitivity and Specificity, Sequence Alignment, Temperature, Time Factors, DNA Virus Infections veterinary, Fish Diseases diagnosis, Flatfishes virology, Iridoviridae isolation & purification, Nucleic Acid Amplification Techniques methods

Abstract

Turbot reddish body iridovirus (TRBIV) is a new piscine iridovirus that infects the turbot, Scophthalmus maximus, cultured in northern China and can cause high mortality. In this study, a loop-mediated isothermal amplification (LAMP) method was developed for the specific detection of this virus using primers designed from an Msp I restriction DNA fragment of the TRBIV genome. Mg(2+) concentrations, the reaction temperature, and the reaction time of LAMP were optimized to 6mM, 65 degrees C, and 60 min, respectively. The detection limit of the LAMP method was as low as seven copies and was 100 times more sensitive than the conventional PCR technique. Visual inspection of LAMP amplifications demonstrated that the positive and negative reactions exhibit distinct and different colors in daylight, which means that gel electrophoresis is not necessary to judge the presence or absence of the virus. LAMP can be conducted in 1h and requires only a simple heating device for incubation. Thus, the LAMP-TRBIV detection protocol has great potential for use in the detection of TRBIV in both the laboratory and the farm.

Published

2009