Your search keyword '"Detection"' showing total 361 results

1. Establishment of a RAA-CRISPR Cas12a based diagnostic method for peste des petits ruminants virus N gene and M gene.

Author

Xu, Jiao, Wang, Yingli, Zhang, Yongqiang, Wang, Shujuan, Su, Na, Chang, Xing, Ren, Weijie, Zou, Yanli, Liu, Shan, Li, Lin, Li, Jinming, Bao, Jingyue, and Wang, Zhiliang

Subjects

*REVERSE transcriptase polymerase chain reaction, *PESTE des petits ruminants, *COMMUNICABLE diseases, *DETECTION limit, *CRISPRS

Abstract

Peste des petis ruminants (PPR) is an acute, highly contagious fatal disease affecting both domestic and wild small ruminants, caused by Morbillivirus caprinae (also known as peste des petis ruminants virus (PPRV)). Herein, a rapid method based on recombinase aided amplification-clustered regularly interspaced short palindromic repeats-Cas12a (RAA-CRISPR Cas12a) to detect PPRV was developed. CRISPR RNAs and RAA primers for PPRV-N (nucleocapsid) and PPRV-M (matrix) fragments were designed. The reaction system was constructed following screening and optimization. Detection could be completed within in 50 minutes at 37°C. Detection of gradient dilutions of plasmids carrying of PPRV N and M gene fragments indicated a minimum limit of detection of 10 copies/μL. There were no cross-reactions with related viruses and all tested lineages of PPRV were detected successfully. The method also showed good repeatability. The detection of clinical samples (previously detected using reverse transcription polymerase chain reaction (RT-PCR)) indicated good consistency between the RAA-CRISPR Cas12a method and RT-PCR. Thus, the RAA-CRISPR Cas12a method for rapid PPRV diagnosis has strong specificity, high sensitivity, and stable repeatability. Moreover, the results can be observed visually under blue or UV light or using lateral flow strips without complex instruments. [ABSTRACT FROM AUTHOR]

Published

2024

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

Author

Chen, Qiang, Zhang, Li-Juan, Song, Tie-Ying, and Ge, Jun-Qing

Subjects

*HEMORRHAGIC diseases, *DETECTION limit, *GENE targeting, *EELS, *EARLY diagnosis

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. • A visual loop-mediated isothermal amplification (LAMP) assay was developed for specific detection of AngHV. • The AngHV LAMP assay is more sensitive than conventional PCR. • The LAMP assay has great potential for early diagnosis of AngHV infection in the farm. [ABSTRACT FROM AUTHOR]

Published

2024

3. Development of TaqMan RT-qPCR for the detection of regulated citrus viruses and viroids in Aotearoa New Zealand.

Author

Yan, Juncong, Tang, Joe, Perez-Egusquiza, Zoila, and Thompson, Jeremy R.

Subjects

*CITRUS, *VIROIDS, *ORANGES, *MOSAIC viruses, *PLANT performance, *VIRUS diseases, *INTERNAL auditing

Abstract

The major citrus species include several economically important fruits, such as orange, mandarin, lemon, limes, grapefruit and pomelos. Since the 1980 s, total production and consumption of citrus has grown strongly with the current annual worldwide production at over 105 million tonnes. New Zealand's citrus exports, for instance, had an estimated worth of NZ$ 11.6 million (approx. US$ 7 million) in 2020. Citrus plants are prone to viral diseases, which can lead to substantial economic losses. In New Zealand, the citrus Import Health Standard (IHS) has identified 22 viruses and viroids that are subject to regulation and requires citrus nursery stock to be free of these pathogens. As such, there is a need for reliable, sensitive, and rapid detection methods to screen for these viruses and viroids during post entry quarantine. In this study, we developed TaqMan RT-qPCR assays for the detection of nine of these regulated viruses and viroids, namely citrus leaf rugose virus (CiLRV), citrus leprosis virus C (CiLV-C), citrus leprosis virus C2 (CiLV-C2), citrus leprosis virus N (CiLV-N), citrus psorosis virus (CPsV), citrus yellow mosaic virus (CYMV), citrus bent leaf viroid (CBLVd), citrus viroid V (CVd-V), and citrus viroid VI (CVd-VI). These assays have been validated and found to be highly sensitive, specific, and reliable. The implementation of these assays will facilitate the safe importation of citrus nursery stock, thus safeguarding the country's horticultural and economic interests. • New TaqMan RT-qPCR assays for the detection of nine emerging Citrus viruses and viroids. • Assays developed using latest global sequence data to ensure detection of all known isolates. • Validated assays with high sensitivity, specificity, and reliability. • Assays duplexed without loss in performance to include a plant internal control (Nad5). [ABSTRACT FROM AUTHOR]

Published

2024

4. Visual, rapid, and cost-effective BK virus detection system for renal transplanted patients using gold nanoparticle coupled loop-mediated isothermal amplification (nanoLAMP).

Author

Kumar, Sunil, Raman, Srishty, Sesham, Kishore, Gupta, Abhishek, Yadav, Raj Kanwar, Mridha, Asit Ranjan, and Yadav, Subhash Chandra

Subjects

*GOLD nanoparticles, *BK virus, *SV40 (Virus), *JOHN Cunningham virus, *VIRUS diseases, *KIDNEY transplantation

Abstract

A substantial percentage of kidney transplant recipients show transplant failure due to BK virus-induced nephropathy. This can be clinically controlled by the rapid and timely detection of BK virus infection in immune-compromised patients. We report a rapid (two hours from sample collection, processing, and detection), cost-effective (< 2$), highly sensitive and BKV-specific nanoLAMP (loop-mediated isothermal amplification) diagnostic methodology using novel primers and gold nanoparticles complex-based visual detection. The standardized nanoLAMP showed an analytical sensitivity of 25 copies/µl and did not cross-react with closely related JC and SV40 viruses. This nanoLAMP showed diagnostic sensitivity and specificity as 91% and 96%, respectively, taking 50 BK virus-negative (confirmed by qPCR from the plasma of healthy donors) and 57 positive BKV patient samples (confirmed by clinical parameters and qPCR assay). This simple two-step, low-cost, and quick (1–2 h/test) detection would be advantageous over the currently used diagnostic methodology. It may change the paradigm for polyomavirus infection-based failure of renal transplant. [Display omitted] • A rapid, cost-effective (< 2$), highly sensitive and BKV-specific nanoLAMP method. • This showed an analytical sensitivity of 25 copies/µl/per reaction and specific. • This showed clinical sensitivity (91%), and specificity (96%), respectively. • This simple two-step method would be advantageous over the current diagnostics. [ABSTRACT FROM AUTHOR]

Published

2024

5. Development and application of monoclonal antibody-based dot-ELISA and colloidal gold immunochromatographic strip for rapid, specific, and sensitive detection of tomato brown rugose fruit virus.

Author

Zhao, Xinru, Wu, Jiayu, Ma, Ziyue, Shi, Yujie, Fang, Zhu, Wu, Jianxiang, Yang, Xiuling, and Zhou, Xueping

Subjects

*COLLOIDAL gold, *REVERSE transcriptase polymerase chain reaction, *FRUIT

Abstract

Tomato brown rugose fruit virus (ToBRFV) is an emerging tobamovirus that has become a great concern to tomato production industry. Due to the lack of resistant cultivars, precise detection of ToBRFV is essential to prevent the spread of ToBRFV. In this study, we produced highly sensitive and specific monoclonal antibodies against ToBRFV and established dot-enzyme-linked immunosorbent assay (dot-ELISA) and colloidal gold immunochromatographic strip (CGICS)-based methods for ToBRFV detection. These two methods could specifically detect ToBRFV without cross-reaction with seven tested tobamoviruses and three frequently occurring tomato-infecting viruses. Sensitivity analysis showed that the limit of detection of the established dot-ELISA and CGICS methods reached up to 1:6400 and 1:10,000 (w/v, g/mL) dilution of ToBRFV-infected tomato tissue, respectively. Further analyses using field-collected tomato foliar and fruit samples showed that the results obtained by dot-ELISA and CGICS were consistent with those obtained by reverse transcription polymerase chain reaction. The established methods here allow for specific, sensitive, and robust detection of ToBRFV, and will be helpful for precise monitoring and early warning of ToBRFV. • Highly sensitive and specific monoclonal antibodies against ToBRFV were produced. • Monoclonal antibody-based dot-ELISA and immunostrip have been developed for rapid, specific, and sensitive detection of ToBRFV. • The developed methods do not cross react with the tested seven tobamoviruses and other three tomato-infecting viruses. • The methods are feasible in detecting both foliar and fruit tomato samples. [ABSTRACT FROM AUTHOR]

Published

2024

6. Establishment of a p30-based lateral flow assay for African swine fever virus detection.

Author

Hang Vu, Thi Thu, Le, Van Phan, Jeong, Dae Gwin, Yeom, Minjoo, Oh, Jinsik, Kang, BoKyu, Park, Song-Kyu, and Song, Daesub

Subjects

*AFRICAN swine fever virus, *COLLOIDAL gold, *SWINE farms, *SWINE breeding, *SMALL farms, *AFRICAN swine fever, *MONOCLONAL antibodies

Abstract

African swine fever virus (ASFV) has continuously devastated the global pig industry. Viral persistence causes problems in large pig farms and kills small farms. Timely diagnostic tools play an important role in controlling outbreaks and minimizing losses. In this study, we developed a lateral flow assay to detect ASFV on-site. The VDRG® ASFV Ag Rapid Kit was established using two monoclonal antibodies (mAbs) against the p30 protein. The conjunction pad of the kit was coated with a mixture of the mAb and colloidal gold. This rapid kit was capable of detecting 11.5 ng of antigen and 0.16 HAD 50 of virus from samples, in 20 min for the entire procedure. It passed cross-specific tests using common viruses that cause infectious diseases in pigs. ASFV was detected after 4 days in experimental infection in pigs by the kit. The specificity and sensitivity of the kit for clinical samples were 99.88% and 84.52% (93.8% for samples with a Ct value below 30), respectively. Finally, the kit can detect 100% positive herd outbreaks. The VDRG® ASFV Ag Rapid Kit presents a useful point-of-care tool for ASFV detection. • A lateral flow assay was established using two mAbs against the ASFV p30 protein. • Nanoscale colloidal gold was used for visual detection. • The assay was validated in experimental infection samples and clinical samples. [ABSTRACT FROM AUTHOR]

Published

2023

7. Universal primer multiplex PCR assay for detection and genotyping of porcine astroviruses.

Author

Zhang, Qiuya, Wen, Dan, Liu, Qin, Opriessnig, Tanja, Yu, Xiaoya, and Jiang, Yonghou

Subjects

*ASTROVIRUSES, *POLYMERASE chain reaction, *MIXED infections, *DETECTION limit, *GENOTYPES, *PHYTOPLASMAS, *SWINE farms

Abstract

Porcine astroviruses (PAstV) are members of the family Astroviridae , Mamastravirus genus and have been identified to have five genotypes (PAstV1–5). These viruses are highly prevalent in pigs and can cause enteric disease as well as neurological or respiratory symptoms depending on their genotypes. At present, the epidemiological impacts of some PAstV genotypes on pigs are largely unknown and hence continuously monitoring of these PAstVs may be needed. The purpose of this research was to develop an improved and efficient detection tool for PAstVs and to evaluate the developed method using clinical samples. Initially, a set of five chimeric primers (CP), each comprising genotype specific primer pairs with an identical universal adapter at the 5' end, and a universal primer (UP) that is identical to universal adapter sequence, were designed. With these tools in place, a novel multiplex PCR system with universal primer was established for the simultaneous detection of the five types of PAstV. This method can specifically detect PAstV genotypes, with a limit of detection (LOD) of 5 copies/μL for each genotype irrespective of single or mixed target template. Using this new assay, 273 pig fecal samples were investigated for further assay evaluation. Among all samples, the positive rate was 70.0% with PAstV4 in 56.8% of the samples, PAstV2 in 38.8%, PAstV1 in 16.8%, and PAstV5 in 11.0%. More than one PAstV in a sample were detected in 39.2% of the samples. The consistency rate between the novel multiplex PCR and singleplex PCRs was 96.4–100%. Given its rapidity, specificity and sensitivity, the novel multiplex PCR is a useful approach for demonstrating single or mixed genotype infections of PAstV. • A novel multiplex PAstV PCR was developed for detection and genotyping of PAstV. • This assay showed a high specificity and sensitivity with a detection limit of 5 copies per reaction. • This assay was proved to be a reliable diagnostic method for the detection and differentiation of five PAstV genotypes. [ABSTRACT FROM AUTHOR]

Published

2023

8. "Rapid diagnosis of Cucumber mosaic virus in banana plants using a fluorescence-based real-time isothermal reverse transcription-recombinase polymerase amplification assay".

Author

Srivastava, Nishant, Kapoor, Reetika, Kumar, Rakesh, Kumar, Shailender, R.K., Saritha, Kumar, Sandeep, and Baranwal, Virendra K.

Subjects

*CUCUMBER mosaic virus, *POLYMERASES, *PLANT viruses, *MESSENGER RNA, *CYTOMEGALOVIRUS diseases, *PLANT RNA

Abstract

• A highly sensitive fluorescence-based real-time RT-exo-RPA assay has been developed for the rapid detection of Cucumber mosaic virus (CMV). • The assay has been validated for the detection of CMV from the crude leaf extracts of a large number of banana samples. • The RT-exo-RPA assay is a simple technique and can be completed within 10–20 min. Cucumber mosaic virus (CMV) is a widespread plant virus infecting important vegetables, plantation and flower crops. Currently, CMV is detected by enzyme-linked immunosorbent assays (ELISA) and reverse transcription-polymerase chain reaction (RT-PCR) assays. ELISA requires polyclonal antibodies and is time-consuming. PCR requires skilled manpower and complex procedures of RNA isolation as well as a thermal cycler. To overcome these difficulties, a portable rapid, simple and visual fluorescence-based reverse transcription-recombinase polymerase amplification (portable RT-exo-RPA) assay for the detection of CMV was developed. A specific primer pair of 30–33 bp targeting a conserved region of the coat protein (CP) gene of CMV and a probe to function in the RT-exo-RPA assays were designed and synthesized. A total of 62 symptomatic as well as 58 asymptomatic banana plant samples, collected from banana orchards located in Jalgaon, Maharashtra, India, were evaluated for CMV infections using crude leaf extracts as templates by a reverse transcription-recombinase polymerase amplification (RT-RPA) assay as well as a real-time RT-exo-RPA assay and the results were compared with those of a reverse transcription-polymerase chain reaction (RT-PCR) assay using purified total plant RNAs as templates. CMV was as efficiently detected using the crude leaf extract template in the RT-RPA and real-time RT-exo-RPA assays as using the purified RNA template in the RT-PCR assay. To dispense with the use of real-time PCR, a portable RT-exo-RPA assay was developed and the alternative methods for the visualization of CMV detection using either a fluorometer or direct viewing with a UV transilluminator were evaluated. To our knowledge, this is the first report of the rapid and reliable diagnosis of CMV infections by a real-time RT-exo-RPA assay using a crude leaf extract as template. [ABSTRACT FROM AUTHOR]

Published

2019

9. Development of a bead-based immunoassay using virus-like particles for detection of alphaviral humoral response.

Author

Ricks, Keersten M., Shoemaker, Charles J., Dupuy, Lesley C., Flusin, Olivier, Voorhees, Matthew A., Fulmer, Ashley N., Badger, Catherine V., Schmaljohn, Connie S., and Schoepp, Randal J.

Subjects

*VIRUS-like particles, *VENEZUELAN equine encephalomyelitis, *EMERGING infectious diseases, *VIRAL antibodies, *IMMUNOASSAY, *ENCEPHALITIS viruses

Abstract

• VLP coupling to microspheres is a viable approach for viral antibody detection in immunoassays. • VEEV IgG detection, this method was 2-log more sensitive than traditional plate-based ELISA, even with the same antigen. • Microspheres can accommodate multiple VLP architectures. • MAGPIX permits multiplexed detection of both IgG and IgM against VEEV and CHIKV humoral response in human clinical samples. There is a pressing need for sustainable and sensitive immunodiagnostics for use in public health efforts to understand and combat the threat of endemic and emerging infectious diseases. In this proof-of-concept work, we describe an immunodiagnostic approach based on the utilization of virus-like particles (VLPs) in a magnetic bead-based platform for multiplexed detection of antiviral humoral response. A retroviral-based VLP, that presents Venezuelan equine encephalitis virus E1/E2 glycoprotein antigen on its surface, was synthesized and coupled to magnetic beads to create VLP-conjugated microspheres (VCMs). Using these VCMs, IgM and IgG antibodies were detectable in nonhuman primate (NHP) and human clinical serum samples at dilutions of 1 × 10 Basile et al. [4] and greater. We also extended the VCM methodology to an Old World alphavirus, chikungunya virus, demonstrating the flexibility of this approach toward different VLP architectures. When multiplexed on the MAGPIX® platform, this method provided differential detection between Old World and New World alphaviral IgM. This flexible, immunodiagnostic method, based on the MAGPIX® platform, demonstrates compatibility of particulate antigens with bead-based assays, improves sensitivity by up to 2-logs, and has faster sample-to-answer time over traditional methods. [ABSTRACT FROM AUTHOR]

Published

2019

10. A reverse transcription-insulated isothermal PCR assay for the detection of duck hepatitis A virus type 3 based on the POCKIT™ system.

Author

Ren, Yupeng, Yue, Hua, Zhu, Lin, Kan, Ruici, Tang, Cheng, and Zhang, Bin

Subjects

*HEPATITIS viruses, *DUCK plague, *DETECTION limit, *HEPATITIS

Abstract

• It is the first time that an insulated isothermal (ii)PCR for DHAV-3 detection was developed. • The RT-iiPCR method is more sensitive and specific than many other reported methods. • It is processed in a small device that is convenient and portable. • The RT-iiPCR assay is highly suited to field diagnosis. Duck hepatitis A virus type 3 (DHAV-3) infection is characterized by severe hepatitis. In recent years, DHAV-3 has become widespread in Asia and has led to economic losses. Conventional methods for DHAV-3 detection usually depend on the use of larger equipment that is not portable and is not fit for on-site diagnoses. In this study, a rapid reverse transcription insulated isothermal (RT-iiPCR) technique was developed for the on-site detection of DHAV-3 based on the POCKIT™ system in a convenient device. The concentration of primer pairs and probes were optimized for amplification of the DHAV-3 VP3 gene of DHAV-3, with no amplification of 12 other duck pathogens. The detection limit of viral RNA was 3.85 × 101 copies/μL, and the analytical sensitivity and specificity levels were both 100% in the detection of 40 liver samples. Furthermore, 97.5% of the RT-iiPCR results were in agreement with those of rRT-PCR, with a kappa value of 0.93. This method is time-saving and better suited to field diagnoses because of its portable device. [ABSTRACT FROM AUTHOR]

Published

2019

11. Development of a triplex real-time RT-PCR assay for detection and differentiation of three US genotypes of porcine hemagglutinating encephalomyelitis virus.

Author

Wang, Leyi, Eggett, Therese E., Lanka, Saraswathi, Fredrickson, Richard L., Li, Ganwu, Zhang, Yan, Yoo, Dongwan, and Bowman, Andrew S.

Subjects

*PORCINE epidemic diarrhea virus, *GENOTYPES, *MOLECULAR probes, *NUCLEOTIDE sequence, *DETECTION limit, *RESPIRATORY diseases, *RNA viruses

Abstract

• A triplex real time RT-PCR was developed for detection and differentiation of three genotypes of PHEV. • The developed triplex real time RT-PCR assay showed high specificity and sensitivity. • The triplex real time RT-PCR assay correctly genotyped clinical samples and is useful to monitor PHEV. Porcine hemagglutinating encephalomyelitis virus (PHEV) is a single-stranded, positive-sense RNA virus. PHEV mainly causes two types of clinical manifestations representing vomiting and wasting and encephalomyelitis in piglets. However, our recent findings provide strong evidence that PHEV can also cause respiratory disease in older pigs. Genomic analysis of new PHEV strains identified in our former study further classifies PHEV into three genotypes. Detection and differentiation of these new mutants are critical in monitoring PHEV evolution in the field. In the present study, we report the development of a triplex real-time RT-PCR assay for detection and differentiation of three PHEV genotypes, 1, 2, and 3. Three sets of primers and probes were designed; one set of primers and probe targeting the conserved regions of the 3′ end nucleocapsid for detection of all three genotypes and another two sets of primers and probes targeting the regions of NS2 with different patterns of deletions for detection of both genotypes 1 and 3, or genotype 3 only. Genotype 1 was positive when two probe dyes showed signals, genotype 2 was positive when only one probe dye showed a signal, and genotype 3 was positive when all three probes showed signals. The detection limit of the developed triplex real-time RT-PCR was as low as 8 or 9 DNA copies for three sets of primers and probes. The specificity test showed no cross reaction with other porcine viruses. Positive field-samples were correctly typed by this new assay, which was further confirmed by DNA sequencing. The triplex real-time RT-PCR provides a rapid and sensitive method to detect and differentiate all three US genotypes of PHEV from clinical samples. [ABSTRACT FROM AUTHOR]

Published

2019

12. A validated semi-nested PCR for rapid detection of scale drop disease virus (SDDV) in Asian sea bass (Lates calcarifer).

Author

Charoenwai, Onanong, Meemetta, Watcharachai, Sonthi, Molrudee, Dong, Ha Thanh, and Senapin, Saengchan

Subjects

*GIANT perch, *VIRUS diseases, *SEA basses, *EPINEPHELUS, *BASSES (Fish), *MARINE fishes

Abstract

• A snPCR was developed for detection of SDDV in L. calcarifer. • The method has detection limit of 100 copies/μL and highly specific for SDDV. • This is the first validated method for SDDV detection for field samples. • The snPCR might be useful for active surveillance in L. calcarifer farming countries. Scale drop diseases virus (SDDV), a newly characterized virus of farmed Asian sea bass (Lates calcarifer), has been reported in several countries in Southeast Asia. However, no fully validated detection method is publicly available for disease diagnosis and surveillance. Here, we described a newly developed semi-nested PCR (snPCR) method for detection of the virus from field samples. The designed primers targeting a gene encoding ATPase generated amplicons of 738 bp and 412 bp in the first and second step PCR, respectively. The established protocol could detect down to 100 viral copies/μL template and was 100-fold more sensitive than single step PCR. A Specificity test against extracted DNA from ten bacterial pathogens, tissues from viral infected specimens and fish host revealed no cross amplification. The SDDV snPCR method could detect the virus from all clinical samples showing symptoms of scale drop disease (n = 25) and all samples from outbreaks of an unknown disease (n = 6) whereas all clinically healthy fish sea bass (n = 161) and grouper (n = 45) collected from different provinces tested negative. The newly established protocol might be useful for Asian sea bass farming countries to initiate disease diagnosis and surveillance. [ABSTRACT FROM AUTHOR]

Published

2019

13. Simultaneous detection of five pig viruses associated with enteric disease in pigs using EvaGreen real-time PCR combined with melting curve analysis.

Author

Wen, Dan, Liu, Gaopeng, Opriessnig, Tanja, Yang, Zongqi, and Jiang, Yonghou

Subjects

*ROTAVIRUSES, *CIRCOVIRUS diseases, *PORCINE epidemic diarrhea virus, *ENTEROVIRUSES, *VIRAL diarrhea, *VIRUS diseases

Abstract

• A low-cost and sensitive real-time PCR assay for enteric disease-associated porcine viruses was developed. • This assay could be used for the detection of one or more diarrhea-causing pig viruses in one reaction. • Diagnostic assay is suitable for epidemiological survey of viral diarrhea infection in high-throughput clinical samples. In recent years, a series of porcine diarrhea viruses such as porcine epidemic diarrhea virus (PEDV), transmissible gastroenteritis virus (TGEV), rotaviruses of group A (RVA), rotaviruses of group C (RVC), and porcine circovirus 2 (PCV2) caused enormous economic losses all over the world. While any of these viruses is capable to cause disease alone, there is often concurrent infection with more than one virus on pig farms. In this study, a multiplex real-time PCR method based on EvaGreen fluorescent dye and melting curve analysis was established to simultaneously detect these five viruses in a single closed tube. Five distinct melt peaks were obtained with different melting temperature (Tm) value corresponding to each of the five viruses. This method was highly sensitive to detect and distinguish TGEV, RVA, RVC, PEDV and PCV2 with the limits of detection ranging from 5 to 50 copies/μL. The intra-assay and inter-assay reproducibility were good with coefficient of variation of Tm and cycle threshold values less than 0.32% and 2.86%, respectively. Testing of 90 field samples by the single and multiplex real-time PCR assays demonstrated a concordance of 91.1%. Thus, the EvaGreen multiplex real-time PCR is a rapid, sensitive and low-cost diagnostic tool for differential detection and routine surveillance of TGEV, RVA, RVC, PEDV and PCV2 in pigs. [ABSTRACT FROM AUTHOR]

Published

2019

14. Development of a SYBR green-based real-time RT-PCR assay for rapid detection of the emerging swine acute diarrhea syndrome coronavirus.

Author

Ma, Lei, Zeng, Fanwen, Cong, Feng, Huang, Bihong, Huang, Ren, Ma, Jingyun, and Guo, Pengju

Subjects

*DIARRHEA, *SWINE diseases, *POLYMERASE chain reaction, *VIRAL genomes, *CORONAVIRUS diseases

Abstract

Abstract Swine acute diarrhea syndrome coronavirus (SADS-CoV) is a novel coronavirus which was associated with severe diarrhea disease in pigs. SADS-CoV was first detected and identified as the causative agent of a devastating swine disease outbreak in southern China in 2017. Routine monitoring and early detection of the source of infection is therefore integral to the prevention and control of SADS-CoV infection. In this study, a SYBR green-based real-time reverse transcription quantitative polymerase chain reaction (RT-qPCR) technique was established for rapid detection and monitoring of this emerging virus. Specific primers were designed based on the conserved region within the M gene of the viral genome. The lowest detection limit of the RT-qPCR assay was 10 copies/μL. This assay was specific and had no cross-reaction with other 11 swine viruses. The positive rate of 84 clinical samples for the SYBR green-based RT-qPCR and the conventional RT-PCR was 73.81% (62/84) and 53.57% (45/84), respectively. These results demonstrated that the SYBR green-based RT-qPCR technique was an effectively diagnostic method with higher sensitivity than probe-based RT-qPCR and gel-based RT-PCR for detection and epidemiological investigations of SADS-CoV. [ABSTRACT FROM AUTHOR]

Published

2019

15. Development of a LAMP assay with a portable device for real-time detection of begomoviruses under field conditions.

Author

Wilisiani, Fariha, Tomiyama, Aika, Katoh, Hiroshi, Hartono, Sedyo, Neriya, Yutaro, Nishigawa, Hisashi, and Natsuaki, Tomohide

Subjects

*BEGOMOVIRUSES, *VEGETABLES, *CUCURBITACEAE, *TOMATOES, *FLUORIMETER

Abstract

Abstract The emergence of begomovirus infection is one of the most important problems affecting production of a variety of vegetable crops worldwide. Infection by begomoviruses has been detected and spread rapidly on Cucurbitaceae and Solanaceae plants in Indonesia. A rapid and simple detection assay for begomoviruses under field conditions for routine sampling of plants is needed. Primers for a loop-mediated isothermal amplification (LAMP) assay were designed based on the sequences of three Indonesian begomoviruses, namely Tomato leaf curl New Delhi virus (ToLCNDV), Pepper yellow leaf curl Indonesia virus (PepYLCIV), and Tomato yellow leaf curl Kanchanaburi virus (TYLCKaV), infecting Cucurbitaceae and Solanaceae plants. LAMP assays using a Genelyzer™ III portable fluorometer with a toothpick method successfully detected these begomoviruses in infected melon, pepper, and eggplant samples. LAMP assays conducted during a field survey for detection of the three begomoviruses on 104 fresh leaves indicated that most of the samples were positive; the findings were confirmed by PCR using universal primers of begomovirus as a common detection method. These results demonstrate that this simple and rapid LAMP assay using a fluorometer portable device may be used to achieve real-time detection of begomoviruses under field conditions. [ABSTRACT FROM AUTHOR]

Published

2019

16. A multiplex reverse transcription PCR assay for simultaneous detection of six main RNA viruses in tomato plants.

Author

Liu, Huan, Wu, Kuan, Wu, Wei, Mi, Weili, Hao, Xingan, and Wu, Yunfeng

Subjects

*TOMATOES, *VIRUS diseases, *POLYMERASE chain reaction, *TOBACCO mosaic disease, *TOBACCO mosaic virus

Abstract

Highlights • A method for simultaneously detecting six tomato virus diseases was established, which is reliable, convenient, and economical. • The addition of the internal control gene EF-1α to the detection system can effectively avoid false negatives. • The detection sensitivity of this method is close to that of simplex RT-PCR, which can be used for the diagnosis of tomato virus disease. Abstract Tomato virus diseases occur all around the world, causing serious yield losses. To detect these viruses quickly and provide a basis for disease control, a multiplex reverse transcription polymerase chain reaction system was established for simultaneous detection of Tobacco mosaic virus (TMV), Cucumber mosaic virus (CMV), Tomato spotted wilt virus (TSWV), Tomato chlorosis virus (ToCV), Potato virus Y (PVY) and Potato virus X (PVX) in tomato plants, with 6 pairs of specific primers being designed based on the coat protein (CP) genes of these viruses. Transcriptional elongation factor-1α (EF-1α) from tomato was added to the multiplex RT-PCR reaction system to prevent false negatives. The concentration of the primers, annealing temperature, annealing time, extension time and amplification cycles were optimized. Expected fragments of 159 bp (ToCV), 262 bp (PVY), 362 bp (EF-1α), 430 bp (TMV), 500 bp (TSWV), 600 bp (CMV) and 705 bp (PVX) were amplified by this multiplex RT-PCR system, and their origin was confirmed by DNA sequencing. This method will have a wide application in virus detection of field samples. [ABSTRACT FROM AUTHOR]

Published

2019

17. A novel multiplex PCR for virus detection by melting curve analysis.

Author

Liu, Pengcheng, Lu, Lijuan, Xu, Menghua, Zhong, Huaqing, Jia, Ran, Su, Liyun, Cao, Lingfeng, Dong, Zuoquan, Dong, Niuniu, Zhou, Linfu, and Xu, Jin

Subjects

*POLYMERASE chain reaction, *FLUORESCENT antibody technique, *VIRUSES, *FLUOROPHORES, *PLASMIDS

Abstract

Highlights • Taqman probe based melting curve analysis can detect and distinguish six respiratory viruses simultaneously. • The multiplex PCR established here has a good analytical sensitivity and specificity. • The accordance rate between the multiplex PCR and direct fluorescent antibody testing was high. • Taqman probe based melting curve analysis is well suited to multiple virus detection. Abstract Background Rapid and accurate laboratory diagnoses of viral infections are crucial for the management and treatment of patients with viral infections. Conventional methods for virus detection are labourious, time consuming, and only a single virus can be analysed in one assay. Objectives The objective of this study was to develop a novel real-time PCR method for multiple virus detection by melting curve analysis using Taqman probes in a single reaction. Study design As a model, six respiratory viruses were detected in one tube using three fluorophores. The specificity was assessed by cross-reaction tests with other common respiratory pathogens. The analytical sensitivity was assessed by testing the limit of detection of the assay using artificial plasmids as the positive template. The clinical evaluation of the established assay was evaluated for the detection of respiratory viruses in clinical samples, and the results were compared with direct fluorescent antibody testing (DFA). Results The six respiratory viruses were clearly distinguished by their respective melting temperature values in the corresponding fluorescence detection channels. No cross reactions were observed by cross reaction tests. The detection limits of this assay were 2 to 2 × 103 copies per reaction for each virus. The clinical evaluation of this assay was demonstrated by analysing 352 clinical samples, and 67(19.0%) samples were positive for at least one virus. The accordance rate between the established PCR and DFA testing was high, and ranged from 94.57% to 100%. Conclusions Taqman probe-based melting curve analysis is well suited for detection of multiple viruses in clinical and research laboratories because of its high throughput, reliability, and cost savings. [ABSTRACT FROM AUTHOR]

Published

2018

18. Subtype specific virus enrichment with immunomagnetic separation method followed by NGS unravels the mixture of H5 and H9 avian influenza virus.

Author

Noh, Eun Bi, Heo, Gyeong-Beom, Lee, Kwang-Nyeong, Kang, Yong-Myung, An, Se-Hee, Kim, Nayeong, and Lee, Youn-Jeong

Subjects

*AVIAN influenza A virus, *IMMUNOMAGNETIC separation, *MOSAIC viruses, *AVIAN influenza, *VETERINARY services, *NUCLEOTIDE sequencing, *MIXTURES

Abstract

Wild bird avian influenza type A virus (AIV) surveillance is important for the early detection of highly pathogenic AIVs and for providing early warnings to the poultry industry and veterinary services to implement more effective control measures against these viruses. Some field samples are often found to contain more than two kinds of AIV. Correct determination of the HA/NA subtype and complete nucleotide sequences of the component viruses in those samples are often critical for timely and accurate understanding of the field situation, but it is not easy to define the genomic structure of the constituent viruses unambiguously because AIV has eight segmented genomes. In this study, with immunomagnetic beads incorporating polyclonal antibodies of chicken for subtype-specific viral enrichment, we could selectively decrease the density of one of the two constituent viruses in a sample of different subtypes, H5 and H9, artificially generated; this was represented in the changes of Ct values with subtype specific real-time RT-PCR. Following this, with NGS, we could recover nearly complete genomic sequences and arrange the consensus sequences of gene segments of the constituent viruses confidently with the quantitative variable like genome coverage, linked along the gene segments and associated with the number of viral copies in a sample. • Wild bird feces can be cross-contaminated with multiple avian influenza viruses due to the gathering and defecation of bird flocks. • The genomic characterization of avian influenza viruses mixed in a wild bird fecal sample is challenging, but it would be crutial in cases of highly pathgenicity avian influenza virusses. • The two different avian influenza viruses could be selectively purified using the immunomagnetic separation method in an HA subtype-specific manner. • The effectiveness of this assay was confirmed by the successful determination of the subtypes and genomic sequences of the component viruses through next-generation sequencing. [ABSTRACT FROM AUTHOR]

Published

2023

19. Development of a TaqMan-based real-time PCR for detecting duck adenovirus 3.

Author

Wan, Chunhe, Chen, Cuiteng, Cheng, Longfei, Fu, Guanghua, Shi, Shaohua, Liu, Rongchang, Chen, Hongmei, Fu, Qiuling, and Huang, Yu

Subjects

*ADENOVIRUS diseases, *DUCKS, *POLYMERASE chain reaction, *IMMUNOSPECIFICITY, *DETECTION limit, *DIAGNOSIS, *DISEASES

Abstract

Highlights • A TaqMan-based real-time PCR method for the detection of DAdV-3 was developed. • The method showed high sensitivity, specificity and reproducibility. • DAdV-3-positive can be found in embryos and newly hatched ducklings. Abstract Recently, a novel duck adenovirus (designated as duck adenovirus 3, DAdV-3) was discovered in Muscovy ducks, China. Here, we developed a TaqMan-based real-time PCR assay (qPCR) for the detection of DAdV-3 infection. After the optimization of the qPCR conditions, the lower limit of detection for DAdV-3 infection was 40.9 copies/μl. No cross-reactivity was observed with other duck-derived pathogens. Intra- and inter-assay variability was less than 2.30%. DAdV-3 was detected in embryos and newly hatched ducklings by qPCR assay, the findings provided evidence of possible vertical transmission of DAdV-3. The developed qPCR analysis showed high specificity, sensitivity, and reproducibility, thereby indicating that it can be used in future investigations on the pathogenesis and epidemiology of DAdV-3. [ABSTRACT FROM AUTHOR]

Published

2018

20. Rapid detection of milk vetch dwarf virus by loop-mediated isothermal amplification.

Author

Zhang, Jun, Liu, Xiaowei, Li, Wei, Zhang, Jing, Xiao, Zhixin, Zhou, Zhicheng, Liu, Tianbo, Li, Ying, Wang, Fenglong, Zhang, Songbai, and Yang, Jinguang

Subjects

*ASTRAGALUS (Plants), *PLANT viruses, *GENE amplification, *VIRAL genetics, *POLYMERASE chain reaction, *VIRUSES

Abstract

Highlights • We demonstrated the use of LAMP for the amplification of genomic MDV DNA for the first time. • The LAMP method for the detection of MDV is cost-effective, rapid, and easy to perform. • We obtained the optimal reaction conditions. • The LAMP method is suitable for detecting MDV not only in laboratory but also in the field. Abstract Milk vetch dwarf virus (MDV) is a member of the genus Nanovirus , and its genome is composed of multiple circular 1-kb ssDNA components. In this study, we first determined that the diseased tobacco samples obtained in Zhucheng, Shandong Province were naturally infected with MDV using a polymerase chain reaction (PCR) assay. Subsequently, loop-mediated isothermal amplification (LAMP) was developed for the detection of MDV for the first time. The Mg2+ and dNTP concentrations and the reaction temperature and time of the LAMP were optimized to 8 mM, 1.8 mM, 65 °C, and 60 min, respectively. The best ratio of the inner primers (FIP and BIP) to the outer primers (F3 and B3) was 2:1. The LAMP detection limit was 100 times greater than that of PCR. The nucleotide amplification could be clearly observed by adding SYBR Green I. The positive and negative reactions exhibit distinctly different colors in daylight; however, the positive reactions exhibit green fluorescence under a UV lamp. Therefore, the method is stable, sensitive and specific. [ABSTRACT FROM AUTHOR]

Published

2018

21. Development of recombinase polymerase amplification assays for the rapid detection of peste des petits ruminants virus.

Author

Zhang, Yongning, Wang, Jianchang, Zhang, Zhou, Mei, Lin, Wang, Jinfeng, Wu, Shaoqiang, and Lin, Xiangmei

Subjects

*POLYMERASES, *VIRUSES, *ENZYMES, *GENETIC vectors, *GENE expression

Abstract

Peste des petits ruminants (PPR) is a severe infectious disease of small ruminants caused by PPR virus (PPRV). Rapid and sensitive detection of PPRV is critical for controlling PPR. This report describes the development and evaluation of a conventional reverse transcription recombinase polymerase amplification (RT-RPA) assay and a real-time RT-RPA assay, targeting the PPRV N gene. Sensitivity analysis revealed that the conventional RT-RPA assay could detect 852 copies of standard PPRV RNA per reaction at 95% probability within 20 min at 41 °C, and the real-time RT-RPA assay could detect 103 copies of RNA molecules per reaction at 95% probability. Specificity analysis showed that both assays have no cross-reactivity with nucleic acid templates prepared from other selected viruses or common pathogens. Clinical evaluation using 162 ovine and hircine serum and nasal swab samples showed that the performance of both the real-time RT-RPA assay and the conventional RT-RPA assay were comparable to that of real-time RT-PCR. The overall agreements between real-time RT-PCR and real-time RT-RPA, and conventional RT-RPA were 99.4% (161/162) and 98.8% (160/162), respectively. The R 2 value of real-time RT-RPA and real-time RT-PCR was 0.900 by linear regression analysis. Our results suggest that both RT-RPA assays have a potential application in the rapid, sensitive and specific detection of PPRV. [ABSTRACT FROM AUTHOR]

Published

2018

22. Genome sequence and detection of peach rosette mosaic virus.

Author

Ho, Thien, Harris, Audra, Katsiani, Asimina, Khadgi, Archana, Schilder, Annemiek, and Tzanetakis, Ioannis E.

Subjects

*MOSAIC viruses, *PLANT genetics, *GENOMES, *PLANT viruses, *GENETICS

Abstract

Peach rosette mosaic disease was first described in the 1940s affecting peach and plum. It was later determined that peach rosette mosaic virus (PRMV) is the causal agent of the disease. PRMV, a member of the genus Nepovirus, infects several perennial crops including stone fruit, grape and blueberry as well as several weed species found in orchards around the world. The molecular characterization of the virus is limited to partial genome sequences making it difficult to develop reliable and sensitive molecular detection tests; the reason that detection is routinely performed using ELISA with antibodies risen against a single virus isolate. Given the potential economic impact of the virus and the modes of transmission which, in addition to nematodes, include seed we studied PRMV in more depth using a modified dsRNA extraction protocol to obtain the virus genome. We determined the full nucleotide sequence and developed a protocol that detects conserved regions present in RNA 1 and RNA 2, making it an excellent alternative to the detection protocols used today. [ABSTRACT FROM AUTHOR]

Published

2018

23. Improved TaqMan real-time assays for detecting hepatitis A virus.

Author

Chou, Kyson X. and Williams-Hill, Donna M.

Subjects

*HEPATITIS A virus, *GENOMES, *ENTEROVIRUSES, *GENETICS, *NUCLEOTIDE sequence

Abstract

Rapid advancement in genomics and bioinformatics in recent years holds great promise for research and development in many disciplines including public health. For the detection of pathogens, methods based on nucleic acid amplification need to be re-evaluated periodically to ensure the validity of signature primers and probes as more and more outbreak strains are sequenced and collected into databases in public domains. In this study, a previous assay designed computationally for detecting hepatitis A virus (HAV) was re-examined. Alignment of 57 complete or near complete HAV genomes allowed identification of conserved sequences for developing new primers and TaqMan probes. Two sets of real-time reverse transcription PCR reagents were developed by targeting highly conserved regions with primers and probes having optimal melting temperatures and minimum secondary structures. These two assays had 10 to 1000 fold lower detection limits than the previous assay when tested using representative human HAV genotypes IA, IB, and IIIA. The better of the two improved assays had a detection limit of 3.7 × 10 −2 to 6.6 × 10 −2 TCID 50 or less. The improved detection sensitivity was likely due to improvement in the following four areas: 1) The Gardner1 probe has a single nucleotide mismatch at the 5′ end in all 19 strains of genotypes IIIA and IIIB. 2) For the Gardner1 forward primer, there is a mismatch corresponding to the 3′ end of the oligonucleotides in two strains belonging to genotype IA. 3) The Gardner1 probe had a melting temperature of 66.2 °C, which is less than the optimum of 68–70 °C (Dorak, 2006). 4) The Gardner1 forward and reverse primers had high potential of forming primer dimers. The improved HAV detection assays developed in this study would support better food safety surveillance initiatives and response to disease outbreaks of viral food-borne illness. [ABSTRACT FROM AUTHOR]

Published

2018

24. Reverse transcription loop-mediated isothermal amplification for species-specific detection of tomato chlorotic spot orthotospovirus.

Author

Sui, Xuelian, Zhang, Shouan, Wu, Zujian, and Ling, Kai-Shu

Subjects

*REVERSE transcriptase polymerase chain reaction, *GENE amplification, *TOMATO diseases & pests, *TOMATO spotted wilt virus disease, *SYMPTOMS, *VIRUSES

Abstract

Tomato chlorotic spot orthotospovirus (TCSV) is an emerging orthotospovirus that can cause severe disease on tomato plants. There are at least four orthotospoviruses infecting tomato, and mixed infection of two or more orthotospoviruses in a single tomato plant is quite common in the field. With similarity in the symptomatology and cross serological reactivity among tomato-infecting orthotospoviruses, especially between TCSV and groundnut ringspot orthotospovirus (GRSV), the current serological tests could not achieve definite and accurate species-specific determination in disease diagnosis. Here, a one-step reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed for TCSV. Under optimum conditions, the virus was detected in as little as 0.2 ng of total RNA or in 1:10,000 dilution of a simple diluted tissue extract, which was ten times more sensitive than a conventional RT-PCR assay. The RT-LAMP assay was highly specific for TCSV, with no cross reaction with the other two orthotospoviruses: GRSV and tomato spotted wilt orthotospovirus (TSWV). These results demonstrate that this simple and sensitive RT-LAMP could be used to achieve species-specific detection for TCSV under field conditions. [ABSTRACT FROM AUTHOR]

Published

2018

25. 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, Wenzhi, Zhou, Yong, Fan, Yuding, Jiang, Nan, Cain, Kenneth, and Zeng, Lingbing

Subjects

*GENE amplification, *INFECTIOUS pancreatic necrosis virus, *CAPSIDS, *AQUACULTURE, *VIRUSES, KIDNEY necrosis

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. [ABSTRACT FROM AUTHOR]

Published

2018

26. Development of a SYBR green-based real-time quantitative PCR assay to detect PCV3 in pigs.

Author

Chen, Gui-hua, Tang, Xiao-yu, Sun, Yuan, Zhou, Ling, Li, Di, Bai, Yang, Mai, Kai-jie, Li, Yi-yun, Wu, Qi-wen, and Ma, Jing-yun

Subjects

*SWINE, *CIRCOVIRUS diseases, *SKIN inflammation, *POLYMERASE chain reaction, *DETECTION limit

Abstract

Porcine circovirus 3 (PCV3) has been reported in cases of porcine dermatitis and nephropathy syndrome, reproductive failure, cardiac and multi-systemic inflammation. A SYBR green-based real-time quantitative PCR (qPCR) assay was established in this study to detect PCV3 in 203 clinical samples from suckling piglets affected by congenital tremors in China. The limit of detection (LOD) of PCV3 was 1.73 × 10 4 copies/μL for gel electrophoresis and 1.73 × 10 2 copies/μL for SYBR green-based real-time qPCR. The melt curve analysis showed a single melt peak at 82.5 °C.The intra-assay coefficient of variation was up to 1.83% and the inter-assay coefficient of variation was up to 2.27%. The PCV3 positive detection rate of 203 clinical samples for the SYBR green-based real-time qPCR and the conventional PCR was 86.70% (176/203) and 26.60% (54/203), respectively. Each tissue detected in the SYBR green-based real-time qPCR showed a higher positive rate than that detected in the conventional PCR. These results indicated that the SYBR green-based real-time qPCR assay is a powerful method with high sensitivity, specificity and reproducibility for epidemiological investigations of PCV3. [ABSTRACT FROM AUTHOR]

Published

2018

27. Development of a simple and rapid reverse transcription-loop mediated isothermal amplification (RT-LAMP) assay for sensitive detection of Citrus tristeza virus.

Author

Warghane, Ashish, Misra, Pragati, Bhose, Sumit, Biswas, Kajal Kumar, Sharma, Ashwani Kumar, Reddy, M. Krishna, and Ghosh, Dilip Kumar

Subjects

*CITRUS diseases & pests, *CITRUS tristeza virus, *GENETIC transcription, *GENE amplification, *BIOLOGICAL assay, *ETIOLOGY of diseases, *VIRUSES

Abstract

Tristeza is a devastating disease of citrus and reported to be present in almost all countries where it is cultivated as a commercial crop. The etiological agent of this disease is Citrus tristeza virus (CTV), a member of the genus Closterovirus with in the family Closteroviridae . The pathogen is restricted to the phloem tissue of the infected citrus plant and has a monopartite ss (+) RNA genome of ∼20 kb size. Till date, there is no effective control measure available for this virus. Management of tristeza depends on destruction of CTV infected field plants, production of virus-free planting material for new orchard establishment and controlling viruliferous aphid vectors responsible for field spread of the pathogen. Availability of rapid diagnostic assay is essential for rapid and efficient detection of the pathogen. In the present investigation, RT-LAMP (reverse transcription-loop mediated isothermal amplification), a highly sensitive, robust and low cost assay has been developed for rapid detection of CTV in infected citrus plant samples. Based on conserved nucleotide sequences available in GenBank and specific to p25 gene (major coat protein gene) of predominant CTV isolates of India, four primer sets (CTV-F3, CTV-B3, CTV-FIP and CTV-BIP) ware designed and custom synthesized. The amplified LAMP products obtained after maintaining isothermal condition of 65° C for 60 min duration could be visible easily with necked eyes in presence of SYBR Green I (100X). Subsequently, LAMP products were verified by electrophoresis run in 1.5% agarose gel. The RT-LAMP results obtained with known CTV isolates maintained in screen house of CCRI, Nagpur were validated using field samples and thereafter it was further confirmed by conventional RT-PCR (reveres transcription-polymerase chain reaction) assay. The sensitivity of CTV-RT-LAMP protocol standardized in the present study was 100 times more than conventional one step RT-PCR assay. It also has maximum detection limit up to 0.0001 ng RNA in individual reaction mixture. CTV-RT-LAMP assay is a simple, sensitive, rapid and less costly detection technique. This assay could be used for CTV diagnosis in pathology laboratories having limited facility and resources and even by citrus nurseries situated in remote locations. As per our knowledge and available literature, the present study reports first time about the usefulness of RT-LAMP assay for detection of CTV from India. [ABSTRACT FROM AUTHOR]

Published

2017

28. β-Propiolactone (BPL)-inactivation of SARS-Co-V-2: In vitro validation with focus on saliva from COVID-19 patients for scent dog training.

Author

Pilchová, Veronika, Prajeeth, Chittappen Kandiyil, Jendrny, Paula, Twele, Friederike, Meller, Sebastian, Pink, Isabell, Fathi, Anahita, Addo, Marylyn Martina, Volk, Holger Andreas, Osterhaus, Albert, von Köckritz-Blickwede, Maren, and Schulz, Claudia

Subjects

*COVID-19, *DOG training, *SALIVA, *ODORS, *DETECTOR dogs, *VIRUS isolation, *SARS-CoV-2

Abstract

β-Propiolactone (BPL) is an organic compound widely used as an inactivating agent in vaccine development and production, for example for SARS-CoV, SARS-CoV-2 and Influenza viruses. Inactivation of pathogens by BPL is based on an irreversible alkylation of nucleic acids but also on acetylation and cross-linking between proteins, DNA or RNA. However, the protocols for BPL inactivation of viruses vary widely. Handling of infectious, enriched SARS-CoV-2 specimens and diagnostic samples from COVID-19 patients is recommended in biosafety level (BSL)− 3 or BSL-2 laboratories, respectively. We validated BPL inactivation of SARS-CoV-2 in saliva samples with the objective to use saliva from COVID-19 patients for training of scent dogs for the detection of SARS-CoV-2 positive individuals. Therefore, saliva samples and cell culture medium buffered with NaHCO 3 (pH 8.3) were comparatively spiked with SARS-CoV-2 and inactivated with 0.1 % BPL for 1 h (h) or 71 h (± 1 h) at 2–8 °C, followed by hydrolysis of BPL at 37 °C for 1 or 2 h, converting BPL into non-toxic beta-hydroxy-propionic acid. SARS-CoV-2 inactivation was demonstrated by a titre reduction of up to 10^4 TCID 50 /ml in the spiked samples for both inactivation periods using virus titration and virus isolation, respectively. The validated method was confirmed by successful inactivation of pathogens in saliva samples from COVID-19 patients. Furthermore, we reviewed the currently available literature on SARS-CoV-2 inactivation by BPL. Accordingly, BPL-inactivated, hydrolysed samples can be handled in a non-laboratory setting. Furthermore, our BPL inactivation protocols can be adapted to validation experiments with other pathogens. • 0.1 % β-propiolactone (BPL) inactivates SARS-CoV-2 in saliva from COVID-19 patients. • BPL inactivation retains COVID-19 odour imprint required for detection dog training. • BPL inactivation protocols for SARS-CoV and SARS-CoV-2 in literature vary widely. [ABSTRACT FROM AUTHOR]

Published

2023

29. Development of one step colorimetric RT-LAMP assays for rapid detection of Apple mosaic virus and Prunus necrotic ringspot virus.

Author

Wani, Latief A., Jawa, Priyanka, and Khan, Jawaid A.

Subjects

*REVERSE transcriptase, *MOSAIC viruses, *ISOTHERMAL temperature, *ROSACEAE, *NUCLEIC acids, *DETECTION limit

Abstract

Apple mosaic virus (ApMV) and Prunus necrotic ringspot virus (PNRSV), belonging to genus Ilarvirus, cause significant losses to rose and other plants of the family Rosaceae. They are easily transmitted through mechanical or vegetative means. In our previous study, the occurrence of ApMV and PNRSV in rose plants was reported. In this study, as a first step towards the development of a colorimetric Reverse Transcriptase – Loop Mediated Isothermal Amplification (RT-LAMP) assay, two primer sets were designed, each containing six primers (F3, B3, FIP, BIP, LF and LB) targeting the coat protein genes of ApMV and PNRSV. After incubation of RT-LAMP reaction mix at an isothermal temperature (65 °C/30 min), the amplified products were visually confirmed with the nucleic acid intercalation dye SYBR Green I and the indicator dye Hydroxy-Naphthol Blue. The developed assays were virus specific and showed no cross amplification. Their sensitivity was 103 times higher than that of the corresponding RT-PCRs. The LAMP assays developed in this study are inexpensive, rapid and reliable for the early detection of ApMV and PNRSV, and could therefore be used in plant quarantine to control the risk of their spread. • RT-LAMP assay for the detection of ApMV infection was developed for the first time. • An efficient one-step colorimetric RT-LAMP assay was developed for the detection of PNRSV in rose plants. • Detection limits of ApMV and PNRSV were 103 times higher than RT-PCR assays. • Both RT-LAMP assays were economical, rapid and specific for detection of ApMV and PNRSV infections under field conditions. [ABSTRACT FROM AUTHOR]

Published

2023

30. One-step reverse transcription loop-mediated isothermal amplification assay for detection of Apple chlorotic leaf spot virus.

Author

Peng, Dandan, Xie, Jipeng, Qiang, Wei, Ling, Kai-Shu, Guo, Liyun, Fan, Zaifeng, and Zhou, Tao

Subjects

*LEAF spots, *REVERSE transcriptase, *GENE amplification, *APPLE microbiology, *CHLOROSIS (Plants), *VIRUSES

Abstract

A reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed for the detection of Apple chlorotic leaf spot virus (ACLSV). In this method, a set of four primers was designed based on the conserved regions in the coat protein gene of ACLSV, and the primers were synthesized for the RT-LAMP assay using total RNA extracted from ACLSV-infected leaf tissues. The optimal reaction temperature and assay time were determined to be 64 °C and 75 min, respectively. The sensitivity of RT-LAMP reactions was reliable up to a maximum dilution of 1:3125, which was more sensitive than the RT-PCR assay. The successful application of RT-LAMP to field-collected apple samples demonstrated its potential for broader applications in effectively diagnosing diseases and, consequently, its potential to control ACLSV from spreading further, particularly in many developing countries around the world. To our knowledge, this is the first application of RT-LAMP for the detection of ACLSV. [ABSTRACT FROM AUTHOR]

Published

2017

31. A multiplex PCR for detection of six viruses in ducks.

Author

Wang, Yongjuan, Zhu, Shanyuan, Hong, Weiming, Wang, Anping, and Zuo, Weiyong

Subjects

*DUCKS, *VIRUS diseases in poultry, *POLYMERASE chain reaction, *GENE amplification, *VIRAL proteins, *DISEASES, *VIRUSES

Abstract

In this study, six pairs of specific primers that can amplify DNA fragments of different sizes were designed and synthesized according to viral protein gene sequences published in GenBank. Then, a multiplex PCR method was established for rapid detection of duck hepatitis virus 1, duck plague virus, duck Tembusu virus, muscovy duck parvovirus, muscovy duck reovirus, and duck H9N2 avian influenza virus, and achieve simple and rapid detection of viral diseases in ducks. Single PCR was used to confirm primer specificity, and PCR conditions were optimized to construct a multiplex PCR system. Specificity and sensitivity assays were also developed. The multiplex PCR was used to detect duck embryos infected with mixed viruses and those with clinically suspected diseases to verify the feasibility of the multiplex PCR. Results show that the primers can specifically amplify target fragments, without any cross-amplification with other viruses. The multiplex PCR system can amplify six DNA fragments from the pooled viral genomes and specifically detect nucleic acids of the six duck susceptible viruses when the template amount is 10 2 copies/μl. In addition, the system can be used to detect viral nucleic acids in duck embryos infected with the six common viruses. The detection results for clinical samples are consistent with those detected by single PCR. Therefore, the established multiplex PCR method can perform specific, sensitive, and high-throughput detection of six duck-infecting viruses and can be applied to clinical identification and diagnosis of viral infection in ducks. [ABSTRACT FROM AUTHOR]

Published

2017

32. Development of reliable detection assays for blueberry mosaic- and blackberry vein banding- associated viruses based on their population structures.

Author

Thekke-Veetil, Thanuja and Tzanetakis, Ioannis E.

Subjects

*MOSAIC viruses, *BLUEBERRIES, *BLACKBERRIES, *RNA viruses, *MEDICAL protocols, *DISEASES

Abstract

Blueberry mosaic associated virus (BlMaV), the presumed causal agent of the homonymous disease and blackberry vein banding associated virus (BVBaV), a component of the blackberry yellow vein disease complex, are recently characterized RNA viruses. There is a need for efficient and sensitive detection protocols for the two viruses, not only for screening during the nursery propagation process but also in commercial fields to better understand virus epidemiology and minimize disease spread. RNA viruses display significant nucleotide variation forming quasi-species. Therefore, sequence-based detection methodologies, even though sensitive, may lead to false negative results. For this reason, information on the genetic diversity of virus populations is essential to develop diagnostic assays that have the potential to detect all variants. Detection assays for BlMaV and BVBaV were developed based on existing genetic diversity data and were validated by screening samples from different geographical areas in the United States. These detection tests provide sensitivity and specificity and will serve as the protocols of choice for virus screening in Vaccinium and Rubus certification programs in the United States and elsewhere. Given the increasing global trade of both blueberry and blackberry these tests will be valuable in avoiding virus introductions to new areas. [ABSTRACT FROM AUTHOR]

Published

2017

33. Evaluation of a rapid detection for Coxsackievirus B3 using one-step reverse transcription loop-mediated isothermal amplification (RT-LAMP).

Author

Monazah, A., Zeinoddini, M., and Saeeidinia, A.R.

Subjects

*COXSACKIEVIRUSES, *MYOCARDITIS, *PICORNAVIRUSES, *RNA, *CANCER cells

Abstract

Coxsackievirus B3 (CVB3) is a member of the genus Enterovirus within the family Picornaviridae and is an important pathogen of viral myocarditis, which accounts for more than 50% viral myocarditis cases. VP1 is major capsid protein that this region has a low homology in both amino acid and nucleotide sequences among Enteroviruses . Therefore we have chosen this region for designed a set of RT-LAMP primers for CVB3 detection. For this the total RNA was extracted from 24-h post infected-HeLa cells with complete cytopathic effect (CPE), and applied to a one-step reverse transcription loop-mediated isothermal amplification reaction (RT-LAMP) using CVB3-specific primers. The optimization of RT-LAMP reaction was carried out with three variables factors including MgSO 4 concentration, temperature and time of incubation. Amplification was analyzed by using 2% agarose gel electrophoresis and ethidium bromide and SYBR Green staining. Our results were shown the ladder-like pattern of the VP1 gene amplification. The LAMP reaction mix was optimized and the best result observed at 4 mM MgSO 4 and 60 °C for 90 min incubation. RT-LAMP had high sensitivity and specificity for detection of CVB3 infection. This method can be used as a rapid and easy diagnostic test for detection of CVB3 in clinical laboratories. [ABSTRACT FROM AUTHOR]

Published

2017

34. Enhancing the sensitivity of Dengue virus serotype detection by RT-PCR among infected children in India.

Author

Ahamed, Syed Fazil, Vivek, Rosario, Kotabagi, Shalini, Nayak, Kaustuv, Chandele, Anmol, Kaja, Murali-Krishna, and Shet, Anita

Subjects

*DENGUE, *DIAGNOSIS of fever, *SEROTYPES, *REVERSE transcriptase polymerase chain reaction, *VIRAL envelopes, *CHILDREN, *CAPSIDS, *DISEASES

Abstract

Dengue surveillance relies on reverse transcription-polymerase chain reaction (RT-PCR), for confirmation of dengue virus (DENV) serotypes. We compared efficacies of published and modified primer sets targeting envelope ( Env ) and capsid-premembrane ( C-prM ) genes for detection of circulating DENV serotypes in southern India. Acute samples from children with clinically-diagnosed dengue were used for RT-PCR testing. All samples were also subjected to dengue serology (NS1 antigen and anti-dengue-IgM/IgG rapid immunochromatographic assay). Nested RT-PCR was performed on viral RNA using three methods targeting 654 bp C-prM, 511 bp C-prM and 641 bp Env regions, respectively. RT-PCR-positive samples were validated by population sequencing. Among 171 children with suspected dengue, 121 were dengue serology-positive and 50 were dengue serology-negative. Among 121 serology-positives, RT-PCR detected 91 (75.2%) by CprM654, 72 (59.5%) by CprM511, and 74 (61.1%) by Env641 . Among 50 serology-negatives, 10 (20.0%) were detected by CprM654 , 12 (24.0%) by CprM511 , and 11 (22.0%) by Env641 . Overall detection rate using three methods sequentially was 82.6% (100/121) among serology-positive and 40.0% (20/50) among serology-negative samples; 6.6% (8/120) had co-infection with multiple DENV serotypes. We conclude that detection of acute dengue was enhanced by a modified RT-PCR method targeting the 654 bp C-prM region, and further improved by using all three methods sequentially. [ABSTRACT FROM AUTHOR]

Published

2017

35. One-step reverse transcription loop-mediated isothermal amplification for the detection of Maize chlorotic mottle virus in maize.

Author

Chen, Ling, Jiao, Zhiyuan, Liu, Dongmei, Liu, Xingliang, Xia, Zihao, Deng, Congliang, Zhou, Tao, and Fan, Zaifeng

Subjects

*CORN viruses, *AMPLIFICATION reactions, *NECROSIS, *REVERSE transcriptase, *DNA primers, *NUCLEOTIDE sequencing

Abstract

Maize chlorotic mottle virus (MCMV) is spreading in many regions worldwide, causing maize lethal necrosis when co-infected with a potyvirid. In this study, one-step reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed to detect MCMV in maize. A set of four specific primers was designed based on the conserved coat protein gene sequences of MCMV. The RT-LAMP could be completed within 60 min under isothermal condition at 63 °C. The sensitivity test showed that the RT-LAMP was about 10-fold more sensitive than RT-PCR and no cross-reactivity was detected with other viral pathogens infecting maize in China. Moreover, the results of RT-LAMP could be visually inspected by SYBR Green I staining in a closed-tube, facilitating high-throughput application of MCMV detection. This method was further verified by testing field-collected samples. These results suggested that the developed MCMV RT-LAMP technique is a rapid, efficient and sensitive method which could be used as a routine screen for MCMV infection. [ABSTRACT FROM AUTHOR]

Published

2017

36. Evaluation of an integrated cell culture RT-PCR assay to detect and quantify infectious lymphocystis disease virus.

Author

Valverde, Estefania J., Borrego, Juan J., and Castro, Dolores

Subjects

*CELL culture, *IRIDOVIRUSES, *REVERSE transcriptase polymerase chain reaction, *SPARUS aurata

Abstract

The lymphocystis disease virus (LCDV), a member of the Iridoviridae family, infects a wide range of fish species including gilthead seabream ( Sparus aurata L.), the most important species cultured in the Mediterranean. LCDV is difficult to propagate in cell culture and does not produce clear and consistent cytopathic effects (CPE), especially in samples collected from subclinically infected fish. An integrated cell culture reverse transcription-polymerase chain reaction (ICC-RT-PCR) assay, followed by dot-blot hybridization of the RT-PCR products, was developed to improve the detection of infectious LCDV. The sensitivity of the ICC-RT-PCR assay, which can be performed in 7 d, was at least 100-fold higher than viral diagnosis obtained by CPE development. The developed assay thus allows the determination of infectious titres in samples with low viral loads, including those from asymptomatic carrier fish, in which no CPE was recorded after a 14-d incubation period. The ICC-RT-PCR assay enables rapid, specific and sensitive detection and quantification of infectious LCDV, and may be a valuable tool in the study of aspects of LCDV infection including transmission or epizootiology. [ABSTRACT FROM AUTHOR]

Published

2016

37. Rapid and sensitive detection of Lily symptomless virus by reverse transcription loop-mediated isothermal amplification.

Author

He, Xiangfeng, Xue, Fei, Xu, Shufa, and Wang, Wenhe

Subjects

*GENE amplification, *COAT proteins (Viruses), *REVERSE transcriptase polymerase chain reaction, *VIRUS diseases of plants, *LILIES, *VIRUSES

Abstract

Lily symptomless virus (LSV) is one of the most prevalent viruses that infect lily plants worldwide. A rapid and sensitive reverse transcription loop-mediated isothermal amplification (RT-LAMP) assay was developed for detection of LSV, using two primer pairs that specifically amplified the conserved sequence of LSV coat protein. The optimum reaction conditions were as follows: 4 mM MgCl 2 and 0.8 M betaine with incubation at 64 °C for 30 min. The limit of detection of LSV from infected lily leaves was 10-fold higher for RT-LAMP than for conventional RT-PCR. Moreover, RT-LAMP detected LSV in not only symptomatic, but also in symptomless tissues of infected plants. These findings indicate that our RT-LAMP method for LSV can serve as a low-cost, simple, and rapid alternative to conventional detection assays. [ABSTRACT FROM AUTHOR]

Published

2016

38. Development and evaluation of a one-step reverse transcription loop-mediated isothermal amplification for detection of Citrus leaf blotch virus.

Author

Liu, Huan, Wu, Wei, Tan, Jiaqi, Li, Yue, Mi, Weili, Jiang, Lijun, and Wu, Yunfeng

Subjects

*CITRUS, *MICROBIAL genes, *PATHOGENIC microorganisms, *LEAVES, *KIWIFRUIT

Abstract

Citrus leaf blotch virus (CLBV) is a type member of the genus Citrivirus belonging to Betaflexiviridae. In this study, a reverse transcription loop-mediated isothermal amplification (RT-LAMP) method was developed to detect CLBV; this technology has been widely used in the detection of various plant pathogenic microorganisms and exogenous genes. The sensitivity of the RT-LAMP method was increased 100-fold compared to that of the conventional RT-PCR. In addition, this method was fast, simple and specific; it could provide better technical support for field diagnosis, customs quarantine and the control measures of CLBV. To our knowledge, this is the first report detecting CLBV using RT-LAMP. [ABSTRACT FROM AUTHOR]

Published

2019

39. Development of a rapid and sensitive reverse transcription real-time quantitative PCR assay for detection and quantification of grass carp reovirus II.

Author

Li, Jiahao, Wu, Huiliang, Xu, Wei, Wang, Yajun, Wang, Hao, Wang, Yingying, Li, Yingying, Shi, Cunbin, Bergmann, Sven M., Mo, Xubing, Wang, Qing, and Yin, Jiyuan

Subjects

*POLYMERASE chain reaction, *CTENOPHARYNGODON idella, *REOVIRUSES, *HEMORRHAGIC diseases, *RNA viruses, *TRANSGENIC organisms, *SENSITIVITY & specificity (Statistics)

Abstract

Hemorrhagic disease of grass carp, which is induced by grass carp reovirus II (GCRV-II), leads to mass mortality in grass carp culture and causes enormous economic loss. However, there is currently no quantitative analysis method for the detection of GCRV-II, which is greatly restricted the etiological and epidemiological study of the disease. In this study a reverse transcription TaqMan PCR (RT-qPCR) assay was developed for the quantitative detection of GCRV-II. The probe and primers targeted location is the segment 6 (S6) region of the GCRV-II genome which is highly conserved. Standard curves were drawn and criteria were confirmed after the determination of the optimum reaction conditions. The species-specific assay showed that the method is highly specific and has no cross reactions with other pathogens. The assay was sufficiently sensitive to detect as low as 10 copies of virus RNA. Moreover, the method has a very good repeatability for batches and inter-batches sample detection. Then the method was applied to detect the virus in tissue samples from clinically infected grass carp, compared with conventional RT-seminested PCR, the RT-qPCR represents a specific value for detection rate of positive samples. In summary, the RT-qPCR was applied and achieved high sensitivity and specificity for GCRV-II detection. • The new detection method is the most sensitive and rapid GCRV-II diagnostic method at present. • This detection can apply accurate quantitative analysis for GCRV-II detection. • Upgrade the existing fluorescence quantitative methods to improve specificity and no cross reaction with other pathogens. • The RT-qPCR method has a good effect on the detection of clinical samples. [ABSTRACT FROM AUTHOR]

Published

2023

40. A peptide-based ELISA for detection of antibodies against novel goose astrovirus type 1.

Author

Ren, Dan, Zhang, Xinyun, Zhang, Wei, Lian, Mingjun, Meng, Xianchen, Li, Tuofan, Xie, Quan, Shao, Hongxia, Wan, Zhimin, Qin, Aijian, Gao, Wei, and Ye, Jianqiang

Subjects

*MONOCLONAL antibodies, *GEESE, *IMMUNOGLOBULINS, *PEPTIDES, *B cells, *IMMUNOFLUORESCENCE

Abstract

Goose gout disease is a high morbidity and mortality disease caused by novel serotype 1 goose astrovirus (GAstV-1), which has resulted in huge economic loss to the goose industry of China. However, few diagnostic methods have been developed for serological surveillance of GAstV-1. In our previous study, several novel B cell epitopes were identified in the ORF2 protein of GAstV-1. In this study, one novel peptide of 627–646 aa in the ORF2 recognized by monoclonal antibody (mAb) 6C6 was used as an antigen to develop an efficient peptide-based ELISA (pELISA) for detection of antibodies against GAstV-1. Specificity analysis showed that the pELISA only reacted with sera against GAstV-1, but not with sera against other pathogens tested. The sensitivity of the pELISA in detecting positive sera was higher than that of the IFA (Indirect immunofluorescence assay). The coefficients of variation (CV) of the intra-assay and inter-assay were both < 10%, indicating that the reproducibility of pELISA was good. For detection of clinical samples, the pELISA had 87.5% concordance with the IFA. Our data demonstrate that the pELISA generated here provides an accurate, rapid, and economical method for the detection antibodies against GAstV-1 for serological surveillance. • A novel peptide (627–646aa) derived in ORF2 was used as an coating antigen in the pELISA. • The established pELISA showed efficient specificity and sensitivity for detection of antibodies against novel GAstV-1. • The pELISA provided a reliable tool for serological surveillance for the infection of GAstV-1. [ABSTRACT FROM AUTHOR]

Published

2023

41. Development of a TaqMan-based real-time PCR assay for the detection of Novel GPV.

Author

Niu, Xiaoyu, Chen, Hao, Yang, Jing, Yu, Xianglong, Ti, Jinfeng, Wang, Aihua, and Diao, Youxiang

Subjects

*DUCKS, *MOLECULAR diagnosis, *POLYMERASE chain reaction, *EPIDEMIOLOGY, *QUANTITATIVE research, *DISEASES

Abstract

The newly emerged disease, duck beak atrophy and dwarfism syndrome (BADS), is caused by novel goose parovirus (N-GPV). Although N-GPV infection has severe consequences, few methods for detecting this virus have been developed. Therefore, the availability of rapid and reliable molecular diagnostic methods would aid future studies of this novel virus. Clinical specimens from 138 suspected cases of N-GPV infection and 120 cloacal swabs from breeding ducks were used in this study. The targeted sequence of N-GPV cloned into the pMD18-T vector was used to generate the N-GPV DNA standard curve. The specificity of the assay was validated using duck plague virus, GPV, duck hepatitis virus, avian influenza virus, duck reovirus, tembusu virus, and fowl adenovirus. The lowest limit of detection was 8.8 × 10 1 copies/μL with a good linear standard curve (Y = −3.3682X + 37.220, R 2 = 0.9953) over a wide range of input DNA, of which the concentration was between 8.8 × 10 1 to 8.8 × 10 8 copies/μL. The results show that the real-time PCR assay is a highly sensitive, specific, reproducible, and versatile method for quantitatively detecting N-GPV DNA, and thus can be used to detect this virus, thereby facilitating epidemiological investigations of animals with BADS. [ABSTRACT FROM AUTHOR]

Published

2016

42. Development and validation of a multiplex conventional PCR assay for simultaneous detection and grouping of porcine bocaviruses.

Author

Zheng, Xiaowen, Liu, Gaopeng, Opriessnig, Tanja, Wang, Zining, Yang, Zongqi, and Jiang, Yonghou

Subjects

*PARVOVIRUSES, *DETECTION of microorganisms, *POLYMERASE chain reaction, *WASTING syndrome, *SWINE diseases

Abstract

Porcine bocavirus (PBoV), a newly described porcine parvovirus, has received attention because it can be commonly identified in clinically affected pigs including pigs with post-weaning multisystemic wasting syndrome (PWMS) and pigs with diarrhea. In recent years, novel PBoVs have been identified and were classified into three genogroups, but the ability to detect and classify these novel PBoVs is not comprehensive to date. In this study, a multiplex conventional PCR assay for simultaneous detection and grouping of PBoVs was developed by screening combinations of mixed primer pairs followed by optimization of the PCR conditions. This method exclusively amplifies targeted fragments of 531 bp from the VP1 gene of PBoV G1, 291 bp from the NP1 gene of PBoV G2, and 384 bp from the NP1/VP1 gene of PBoV G3. The assay has a detection limit of 1.0 × 10 3 copies/μL for PBoV G1 4.5 × 10 3 for PBoV G2 and 3.8 × 10 3 for PBoV G3 based on testing mixed purified plasmid constructs containing the specific viral target fragments. The performance of the multiplex PCR assay was comparable to that of the single PCRs which used the same primer pairs. Using the newly established multiplex PCR assay, 227 field samples including faeces, serum and tissue samples from pigs were investigated. All three PBoV genogroups were detected in the clinical samples with a detection rate of 1.3%, 2.6% and 12.3%, respectively for PBoV G1, G2 and G3. Additionally, coinfections with two or more PBoV were detected in 1.7% of the samples investigated. These results indicate the multiplex PCR assay is specific, sensitive and rapid, and can be used for the detection and differentiation of single and multiple infections of the three PBoV genogroups in pigs. [ABSTRACT FROM AUTHOR]

Published

2016

43. Development of a rapid diagnostic assay for the detection of tomato chlorotic dwarf viroid based on isothermal reverse-transcription-recombinase polymerase amplification.

Author

Hammond, Rosemarie W. and Zhang, Shulu

Subjects

*VIROIDS, *DETECTION of microorganisms, *TOMATO diseases & pests, *DNA primers, *PLANT cells & tissues

Abstract

A molecular diagnostic assay utilizing reverse transcription-recombinase polymerase amplification (RT-RPA) at an isothermal constant temperature of 39 °C and target-specific primers and probe were developed for the rapid, sensitive, and specific detection of tomato chlorotic dwarf viroid (TCDVd) in infected leaf and seed tissues. The performance of the AmplifyRP ® Acceler8™ RT-RPA diagnostic assay, utilizing a lateral flow strip contained within an amplicon detection chamber, was evaluated and the results were compared with a standard RT-PCR assay. The AmplifyRP ® Acceler8™ assay was specific for TCDVd in leaf and seed tissues, its sensitivity was comparable to conventional RT-PCR in leaf tissues, and it does not require extensive sample purification, specialized equipment, or technical expertise. This is the first report utilizing an RT-RPA assay to detect viroids and the assay can be used both in the laboratory and in the field for TCDVd detection. [ABSTRACT FROM AUTHOR]

Published

2016

44. Development of a novel immuno-PCR for detection of avian leukosis virus.

Author

Xie, Quan, Zhang, Jianjun, Shao, Hongxia, Wan, Zhimin, Tian, Xiaoyan, Yang, Jialiang, Pang, Mayun, Qian, Kun, Gao, Wei, Wang, Chengming, Qin, Aijian, and Ye, Jianqiang

Subjects

*AVIAN leukosis, *DETECTION of microorganisms, *POLYMERASE chain reaction, *POULTRY industry & economics, *LIGATURE (Surgery)

Abstract

Avian leukosis virus (ALV) is an important pathogen for various neoplasms, including lymphoid, myeloid, and erythroid neoplasms, and it causes significant economic loss in the poultry industry. Several efficient methods for the detection of ALV have been reported. However, these previously developed approaches are based on either PCR or immunoassays. Here, we used a proximity ligation technique and combined PCR with the immunoassay to develop a novel immuno-PCR (Im-PCR) approach for the detection of ALV. Our data showed that the Im-PCR had high specificity and sensitivity to ALV. The Im-PCR method selectively reacted to ALV but not to the other avian viruses tested. The limit of detection of Im-PCR could reach 0.5 TCID 50 . Moreover, the results of Im-PCR were in agreement with results from commercial ELISA when the clinical cloaca samples were used for ALV detection. The present results demonstrate that the novel Im-PCR method can be efficiently applied to detect ALV in a clinical setting. Our data also highlight that Im-PCR may have promising applications in the diagnosis of pathogens. [ABSTRACT FROM AUTHOR]

Published

2016

45. Towards next-generation sequencing analytics for foodborne RNA viruses: Examining the effect of RNA input quantity and viral RNA purity.

Author

Yang, Zhihui, Leonard, Susan R., Mammel, Mark K., Elkins, Christopher A., and Kulka, Michael

Subjects

*RNA viruses, *NUCLEOTIDE sequencing, *FOOD microbiology, *DETECTION of microorganisms, *DNA copy number variations

Abstract

Detection and identification of viruses in food samples are technically challenging due largely to the low viral copy number in contaminated food items, and the lack of effective culture enrichment methods that are amenable to regulatory applications for many of the common foodborne viruses. Using an Illumina MiSeq platform and two hepatitis A virus (HAV) cell-culture adapted strains as a representative enteric virus species, this study examined the limits of single-stranded RNA (ssRNA) viral detection following next-generation sequencing without pre-amplification of the viral genome. Complete viral genome sequences were obtained from HAV samples of varying purities and with an input as low as 2 ng total RNA containing 1.4 × 10 5 copies of viral RNA. In addition, single nucleotide variations were reproducibly detected over the range of concentrations examined, and their identity confirmed by alternate sequencing technology. In summary, next-generation sequencing technology has the potential for sensitive detection/identification of a viral genome at a low copy number. This study provides a benchmark for metagenomic sequencing application as is required for virus detection in complex food matrices using a culture-independent diagnostic approach. [ABSTRACT FROM AUTHOR]

Published

2016

46. Development of multiplex polymerase chain reaction assay for simultaneous detection of clostero-, badna- and mandari-viruses along with huanglongbing bacterium in citrus trees.

Author

Meena, Ram Prasnna and Baranwal, V.K.

Subjects

*CITRUS greening disease, *CANDIDATUS liberibacter asiaticus, *CYMBIDIUM mosaic virus, *DNA primers, *POLYMERASE chain reaction, *MOLECULAR size

Abstract

Citrus trees harbor a large number of viral and bacterial pathogens. Citrus yellow vein clearing virus (CYVCV), Indian citrus ringspot virus (ICRSV), Citrus yellow mosaic virus (CYMV), Citrus tristeza virus (CTV) and a bacterium, Candidatus Liberibacter asiaticus ( C La) associated with huanglongbing (HLB) disease, the most prevalent pathogens in citrus orchards of different regions in India and are responsible for debilitating citriculture. For detection of these viral and bacterial pathogens a quick, sensitive and cost effective detection method is required. With this objective a multiplex polymerase chain reaction (mPCR) assay was developed for simultaneous detection of four viruses and a bacterium in citrus. Several sets of primers were designed for each virus based on the retrieved reference sequences from the GenBank. A primer pair published previously was used for greening bacterium. Each pair of primers was evaluated for their sensitivity and differentiation by simplex and mPCR. The constant amplified products were identified on the basis of molecular size in mPCR and were compared with standard PCR. The amplicons were cloned and results were confirmed with sequencing analysis. The mPCR assay was validated using naturally infected field samples for one or more citrus viruses and the huanglongbing bacterium. The mPCR assay developed here will aid in the production of virus free planting materials and rapid indexing for certification of citrus budwood programme. [ABSTRACT FROM AUTHOR]

Published

2016

47. Optimizing a custom tiling microarray for low input detection and identification of unamplified virus targets.

Author

Yu, Christine, Wales, Samantha Q., Mammel, Mark K., Hida, Kaoru, and Kulka, Michael

Subjects

*FOODBORNE diseases, *DNA microarrays, *FOOD contamination, *COXSACKIEVIRUS diseases, *NOROVIRUSES

Abstract

Viruses are major pathogens causing foodborne illnesses and are often present at low levels in foods, thus requiring sensitive techniques for their detection in contaminated foods. The lack of efficient culture methods for many foodborne viruses and the potential for multi-species viral contamination have driven investigation toward non-amplification based methods for virus detection and identification. A custom DNA microarray (FDA_EVIR) was assessed for its sensitivity in the detection and identification of low-input virus targets, human hepatitis A virus, norovirus, and coxsackievirus, individually and in combination. Modifications to sample processing were made to accommodate low input levels of unamplified virus targets, which included addition of carrier cDNA, RNase treatment, and optimization of DNase I-mediated target fragmentation. Amplification-free detection and identification of foodborne viruses were achieved in the range of 250–500 copies of virus RNA. Alternative data analysis methods were employed to distinguish the genotypes of the viruses particularly at lower levels of target input and the single probe-based analysis approach made it possible to identify a minority species in a multi-virus complex. The oligonucleotide array is shown to be a promising platform to detect foodborne viruses at low levels close to what are anticipated in food or environmental samples. [ABSTRACT FROM AUTHOR]

Published

2016

48. Standardization of a cytometric p24-capture bead-assay for the detection of main HIV-1 subtypes.

Author

Merbah, Mélanie, Onkar, Sayali, Grivel, Jean-Charles, Vanpouille, Christophe, Biancotto, Angélique, Bonar, Lydia, Sanders-Buell, Eric, Kijak, Gustavo, Michael, Nelson, Robb, Merlin, Kim, Jerome H., Tovanabutra, Sodsai, and Chenine, Agnès-Laurence

Subjects

*CYTOMETRY, *BIOLOGICAL assay, *HIV infections, *THERAPEUTICS, *MONOCLONAL antibodies, *BLOOD plasma

Abstract

The prevailing method to assess HIV-1 replication and infectivity is to measure the production of p24 Gag protein by enzyme-linked immunosorbent assay (ELISA). Since fluorescent bead-based technologies offer a broader dynamic range and higher sensitivity, this study describes a p24 capture Luminex assay capable of detecting HIV-1 subtypes A–D, circulating recombinant forms (CRF) CRF01_AE and CRF02_AG, which together are responsible for over 90% of HIV-1 infections worldwide. The success of the assay lies in the identification and selection of a cross-reactive capture antibody (clone 183-H12-5C). Fifty-six isolates that belonged to six HIV-1 subtypes and CRFs were successfully detected with p -values below 0.021; limits of detection ranging from 3.7 to 3 × 104 pg/ml. The intra- and inter-assay variation gave coefficient of variations below 6 and 14%, respectively. The 183-bead Luminex assay also displayed higher sensitivity of 91% and 98% compared to commercial p24 ELISA and a previously described Luminex assay. The p24 concentrations measured by the 183-bead Luminex assay showed a significant correlation ( R = 0.92, p < 0.0001) with the data obtained from quantitative real time PCR. This newly developed p24 assay leverages the advantages of the Luminex platform, which include smaller sample volume and simultaneous detection of up to 500 analytes in a single sample, and delivers a valuable tool for the field. [ABSTRACT FROM AUTHOR]

Published

2016

49. Immunostained plaque assay for detection and titration of rabies virus infectivity.

Author

Park, Jun-Sun, Um, Jihye, Choi, Young-Ki, Lee, Yeong Seon, Ju, Young Ran, and Kim, Su Yeon

Subjects

*PLAQUE assay technique, *FLUORESCENT antibody technique, *VOLUMETRIC analysis, *RABIES virus, *MONOCLONAL antibodies, *IMMUNOSTAINING

Abstract

The fluorescent antibody test (FAT) is the most commonly used method for detection of the rabies virus (RV). The plaque assay can only be applied to fixed RVs, and cannot be used for street RVs. In this study, plaque formation allowing the determination of both fixed and street RVs was achieved using the immune plaque assay. The immune plaque assay carried out using both fixed and street RVs showed the formation of clear and countable plaques after immunostaining with anti-RV P monoclonal antibody and HRP-conjugated anti-mouse IgG. Plaque size increased with incubation time, and the plaque morphology differed according to viral strain. Fixed RVs had the dot-shaped regular plaque morphology and street RVs had the small irregular-shape plaque morphology. In addition, no significant differences were observed between the growth kinetics of the KGH strain when the virus was titrated using the FAT and the immune plaque assay. It allowed the successful detection and quantification of both street and fixed RVs through the production of clear, countable plaques, making it easy to obtain objective results. The assay is an applicable tool for the detection of RVs in various investigations, including virus neutralizing antibody testing, cell-to-cell spread, and viral drug sensitivity testing. [ABSTRACT FROM AUTHOR]

Published

2016

50. Development of a triplex real-time RT-PCR assay for detection and differentiation of three US genotypes of porcine hemagglutinating encephalomyelitis virus

Author

Saraswathi Lanka, Andrew S. Bowman, Dongwan Yoo, Leyi Wang, Ganwu Li, Richard L. Fredrickson, Yan Zhang, and Therese E. Eggett

Subjects

0301 basic medicine, Genotype, Swine, PHEV, Encephalomyelitis, 030106 microbiology, Mutant, Real time RT-PCR, Genome, Viral, Biology, Sensitivity and Specificity, Article, DNA sequencing, 03 medical and health sciences, chemistry.chemical_compound, Limit of Detection, Virology, medicine, Animals, Betacoronavirus 1, Swine Diseases, RNA virus, medicine.disease, biology.organism_classification, Detection, 030104 developmental biology, Real-time polymerase chain reaction, chemistry, Differentiation, Porcine hemagglutinating encephalomyelitis virus, Coronavirus Infections, Multiplex Polymerase Chain Reaction, DNA

Abstract

Highlights • A triplex real time RT-PCR was developed for detection and differentiation of three genotypes of PHEV. • The developed triplex real time RT-PCR assay showed high specificity and sensitivity. • The triplex real time RT-PCR assay correctly genotyped clinical samples and is useful to monitor PHEV., Porcine hemagglutinating encephalomyelitis virus (PHEV) is a single-stranded, positive-sense RNA virus. PHEV mainly causes two types of clinical manifestations representing vomiting and wasting and encephalomyelitis in piglets. However, our recent findings provide strong evidence that PHEV can also cause respiratory disease in older pigs. Genomic analysis of new PHEV strains identified in our former study further classifies PHEV into three genotypes. Detection and differentiation of these new mutants are critical in monitoring PHEV evolution in the field. In the present study, we report the development of a triplex real-time RT-PCR assay for detection and differentiation of three PHEV genotypes, 1, 2, and 3. Three sets of primers and probes were designed; one set of primers and probe targeting the conserved regions of the 3′ end nucleocapsid for detection of all three genotypes and another two sets of primers and probes targeting the regions of NS2 with different patterns of deletions for detection of both genotypes 1 and 3, or genotype 3 only. Genotype 1 was positive when two probe dyes showed signals, genotype 2 was positive when only one probe dye showed a signal, and genotype 3 was positive when all three probes showed signals. The detection limit of the developed triplex real-time RT-PCR was as low as 8 or 9 DNA copies for three sets of primers and probes. The specificity test showed no cross reaction with other porcine viruses. Positive field-samples were correctly typed by this new assay, which was further confirmed by DNA sequencing. The triplex real-time RT-PCR provides a rapid and sensitive method to detect and differentiate all three US genotypes of PHEV from clinical samples.

Published

2019