Your search keyword '"Multiplex Polymerase Chain Reaction veterinary"' showing total 311 results

1. Novel genotyping assay for a 212-kb deletion from the BBS9 gene, and frequency of the allele in pig populations in Vietnam.

Author

Tinh NH, Hop NV, Phuong PT, Tam TLH, Quoc NB, Son TH, and Bui APN

Subjects

Animals, Swine genetics, Vietnam, Gene Frequency, Genotype, Bardet-Biedl Syndrome genetics, Bardet-Biedl Syndrome veterinary, Alleles, Genotyping Techniques veterinary, Genotyping Techniques methods, Multiplex Polymerase Chain Reaction veterinary

Abstract

Piglet lethality is one of the major concerns in pig breeding programs. Deletion of a 212-kb region within the Bardet-Biedl syndrome 9 ( BBS9 ) gene has been linked to a reduction in the number of piglets born alive per litter. The BBS9 mutant gene carrier-by-carrier mating scheme could result in mummification of piglets carrying 2 copies of the BBS9 mutant allele, which ultimately affects the reproductive performance of the sow. Our aim was to develop a simple, rapid, and cost-efficient method that could be applied in a BBS9 mutant gene carrier screening program in low- and middle-income countries within basic laboratory settings. Here, we report an optimized multiplex PCR assay that we have established successfully for detection of a 212-kb deletion within the BBS9 genomic sequence. We genotyped 420 animals from Yorkshire, Duroc, and Landrace purebred populations in Vietnam. We found that while the BBS9 mutant allele was not identified in Duroc pigs, the frequency of BBS9 carriers was 10% in both Yorkshire and Landrace populations. We subsequently validated our results using Sanger sequencing. Our multiplex PCR method could be utilized as a BBS9 screening test in pig breeding programs., Competing Interests: Declaration of conflicting interestsThe authors declared no potential conflicts of interest with respect to the research, authorship, and/or publication of this article.

Published

2024

2. Multiplex PCR assay for the accurate and rapid detection and differentiation of Lactococcus garvieae and L. petauri.

Author

Ustaoglu D, Öztürk RÇ, Ture M, Colussi S, Pastorino P, Vela AI, Kotzamanidis C, Volpatti D, Acutis PL, and Altinok I

Subjects

Animals, Sensitivity and Specificity, Lactococcus genetics, Lactococcus isolation & purification, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods, Fish Diseases microbiology, Fish Diseases diagnosis, Gram-Positive Bacterial Infections veterinary, Gram-Positive Bacterial Infections microbiology, Gram-Positive Bacterial Infections diagnosis

Abstract

Lactococcosis is a common bacterial fish disease caused by Lactococcus garvieae, L. petauri and L. formosensis. Although there are different PCR-based techniques to identify the etiological agent, none of these can differentiate these two bacteria without sequencing PCR-amplified fragments. In the present study, we developed a multiplex PCR assay for simultaneous detection and differentiation of L. garvieae and L. petauri. The specificity of the primers was validated against the bacterial DNA of the targeted and non-targeted bacteria. The sizes of the PCR amplicons were obtained as 204 bp for the DUF1430 domain-containing protein gene of L. garvieae, 465 bp for the Lichenan permease IIC component gene of L. petauri, and 302 bp for the teichoic acid biosynthesis protein F gene of both L. garvieae and L. petauri. The PCR amplicons were clearly separated by agarose gel electrophoresis. The multiplex PCR assay did not produce any amplification products with the DNA of the non-targeted bacteria. The multiplex PCR detection limits for L. garvieae and L. petauri were 5 and 4 CFU in pure culture and 50 and 40 CFU/g in spiked tissue samples, respectively. It takes less than 2 h from plate-cultured bacteria and 3 h from tissue samples to get results. In conclusion, the developed multiplex PCR assay is a rapid, specific, accurate, and cost-effective method for the detection and differentiation of L. garvieae and L. petauri and is suitable to be used for routine laboratory diagnosis of L. garvieae and L. petauri., (© 2024 The Author(s). Journal of Fish Diseases published by John Wiley & Sons Ltd.)

Published

2024

3. Bovine tuberculosis in Central Ethiopian slaughterhouses and the identification of causative mycobacteria by multiplex real-time PCR.

Author

Fromsa A, Conlan AJK, Srinivasan S, Zeleke M, Worku D, Lakew M, Abdela MG, Bahiru G, Wood JLN, Bakker D, Gumi B, Ameni G, and Kapur V

Subjects

Animals, Cattle, Ethiopia epidemiology, Cross-Sectional Studies, Prevalence, Risk Factors, Mycobacterium bovis genetics, Mycobacterium bovis isolation & purification, Mycobacterium bovis classification, Female, Tuberculosis, Bovine microbiology, Tuberculosis, Bovine epidemiology, Tuberculosis, Bovine diagnosis, Abattoirs, Multiplex Polymerase Chain Reaction veterinary, Real-Time Polymerase Chain Reaction

Abstract

Background: Bovine tuberculosis (bTB) is a chronic disease caused by members of the Mycobacterium tuberculosis complex (MTBC) that ultimately leads to the development of progressive granulomatous lesions. Although the disease is widespread, especially in crossbred cattle in Ethiopia, routine investigations and surveillance are lacking. Thus, the aim of this study was to determine the prevalence, associated risk factors, and species of mycobacteria causing bTB in slaughtered cattle at four slaughterhouses in Central Ethiopia., Methods: Postmortem examination of 7,640 cattle was conducted using a cross-sectional slaughterhouse survey. A total of 388 tuberculous-like lesions (TBLs) were collected from 173 animals and cultured. Six target genes were used to differentiate mycobacterial species using multiplex real-time PCR (mRT-PCR). Multivariate logistic regression analyses and related odds ratios (ORs) were used to gauge the strength of the associations between risk factors, TBL incidence and culture growth., Results: The prevalence of TBL was 2.3% (95% CI = 2.0-2.6). Logistic regression analysis indicated an increased risk of TBL in crossbred cattle (OR = 11.8, 95% CI: 6.4, 21.2, p < 0.001). Animals slaughtered at Adama (OR = 3.2, 95% CI: 1.2, 7.3, p = 0.009) or Burayu (OR = 5.8, 95% CI: 3.9, 8.9, p < 0.001) had a greater risk of TBL than those slaughtered at Sululta. There were significantly more TBL-positive lesions in the lungs and lymph nodes related to the lung (OR = 7.1; 95% CI: 2.7, 24.5, p < 0.001) and the head lymph node (OR = 5.6; 95% CI: 1.8, 21.7; p = 0.006) compared to gut associated lymph nodes. Among the 173 TBL-positive animals, 36% (95% CI = 28.8, 43.2), and among the 388 TBL-positive tissues, 24.2% (95% CI = 20, 29) were culture and mRT-PCR positive. All the culture-generated isolates were positive for M. bovis in mRT-PCR. Among them, two animals had mixed infections including one zebu cattle tested positive for both M. caprae and M. bovis, and a crossbred cow tested positive for both M. tuberculosis and M. bovis in mRT-PCR. This suggests persistent transmission within the cattle population, posing a substantial public health threat., Conclusion: This study revealed an eleven-fold greater risk of bTB-related lesions in crossbred cattle compared to local zebu cattle. This finding highlights the necessity for targeted interventions, continuous vigilance, and thorough carcass inspection to mitigate public health risks., (© 2024. The Author(s).)

Published

2024

4. The first isolation of Clostridium massiliodielmoense from a dead beef cow in Japan and pitfalls to be aware of in identifying the Clostridium species.

Author

Mada T, Umeda A, Kodama A, and Takamatsu D

Subjects

Animals, Cattle, Japan, Female, Diarrhea microbiology, Diarrhea veterinary, Multiplex Polymerase Chain Reaction veterinary, Clostridium isolation & purification, Clostridium genetics, Cattle Diseases microbiology, Cattle Diseases diagnosis, Clostridium Infections veterinary, Clostridium Infections microbiology, Clostridium Infections diagnosis, RNA, Ribosomal, 16S genetics

Abstract

Clostridium sp. was detected in the organs of a cow with black watery diarrhea in Japan. Results identifying this species were inconsistent; Clostridium novyi type A infection was suggested by PCR assay targeting Clostridium fliC region (fliC-multiplex PCR), while 16S rRNA gene sequencing identified the isolated bacteria as Clostridium massiliodielmoense. Sequencing of fliC-multiplex PCR products from the isolates revealed the presence of fliC region in C. massiliodielmoense, which had 92.7% nucleotide similarity to that of C. novyi type A JCM 1406 T , leading to the false positive detection of C. novyi by the PCR. This is the first C. massiliodielmoense isolation from clinical specimens, suggesting the need for further research on its pathogenicity and improvement in fliC-multiplex PCR.

Published

2024

5. Molecular Survey of Tick-Borne Haemoparasites of Dogs by Multiplex Polymerase Chain Reaction from Punjab, India.

Author

Singh H, Padmaja M, Thomas AM, Panwar H, Nasrul SI, Jyoti, and Singh NK

Subjects

Dogs, Animals, India epidemiology, Prevalence, Ehrlichiosis veterinary, Ehrlichiosis epidemiology, Ehrlichiosis diagnosis, RNA, Ribosomal, 18S genetics, Male, Female, Sensitivity and Specificity, Coccidiosis veterinary, Coccidiosis epidemiology, Coccidiosis parasitology, Coccidiosis diagnosis, Dog Diseases parasitology, Dog Diseases epidemiology, Dog Diseases diagnosis, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Babesia genetics, Babesia isolation & purification, Babesiosis epidemiology, Babesiosis parasitology, Babesiosis diagnosis, Tick-Borne Diseases veterinary, Tick-Borne Diseases epidemiology, Tick-Borne Diseases parasitology, Ehrlichia canis genetics, Ehrlichia canis isolation & purification

Abstract

Purpose: Tick-transmitted parasites as Babesia gibsoni, Babesia vogeli, Ehrlichia canis, and Hepatozoon canis are major health concern for dogs. Owing to prevalence and infection severity, there is need of sensitive, specific, and affordable test for their simultaneous detection., Methods: Prevalence of B. gibsoni, B. vogeli, E. canis, and H. canis infections was assessed on 719 blood samples by microscopy and multiplex PCR assay targeting 18S rRNA (B. gibsoni & H. canis), ITS1 & 5.8S rRNA (B. vogeli) and VirB9 gene (E. canis). An internal control (canine-actin) was also included to increase the accuracy of assay and effect of associated risk factors with disease prevalence was also studied., Results: Microscopic prevalence of B. gibsoni, B. vogeli, E. canis and H. canis was 5.0%, 0.1%, 1.4% and 1.0%, respectively, whereas with multiplex PCR assay, the corresponding values were 8.9%, 1.1%, 2.6% and 5.1% besides concurrent infections of B. gibsoni & H. canis (0.4%), B. gibsoni & E. canis (0.4%), E. canis & H. canis (0.3%) and B. gibsoni & B. vogeli (0.1%). Analytical sensitivity of developed assay was 0.1pg (B. gibsoni & H. canis), 0.01pg (B. vogeli), and 1.0pg (E. canis). A ″fair″ (B. vogeli & H. canis) to ″substantial″ (B. gibsoni & E. canis) agreement between two tests was observed with data as statistically significant. Breed, sex and location were significantly associated with B. gibsoni infection., Conclusion: The developed multiplex PCR assay offers a potential solution to detect these pathogens simultaneously, aiding in timely diagnosis and effective disease management in suspected dogs., (© 2024. The Author(s), under exclusive licence to Springer Nature Switzerland AG.)

Published

2024

6. Development of a 1-step multiplex PCR assay for the detection of S. Enteritidis, S. Pullorum, S. Typhimurium, and S. Infantis associated with poultry production.

Author

Liu B, Meng C, Han S, Li Q, Miao X, Wang Z, Xu C, Kang X, Jiao X, and Pan Z

Subjects

Animals, Salmonella isolation & purification, Salmonella genetics, Sensitivity and Specificity, Serogroup, Animal Husbandry methods, Salmonella Infections, Animal microbiology, Salmonella Infections, Animal diagnosis, Poultry Diseases microbiology, Poultry Diseases diagnosis, Chickens microbiology, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods

Abstract

Salmonellosis in poultry is detrimental to the advancement of the breeding industry and poses hazards to human health. Approximately 2,600 Salmonella varieties exist, among which S. Enteritidis, S. Pullorum, S. Typhimurium, and S. Infantis are prevalent serotypes in the poultry industry in recent years. They can also infect humans by contaminating poultry eggs and meat. Therefore, identifying these serotypes is crucial for successful preventive and control interventions. The White-Kauffmann-Le Minor scheme is time-consuming and requires expensive reagents. Whole-genome sequencing (WGS) and other molecular biology techniques require skilled technical staff. In comparison, the polymerase chain reaction (PCR) is more accurate, rapid, and inexpensive, thus proving suitable for widespread application in the poultry industry. Here, we selected 4 specific primers: lygD, mdh, ipaJ, and SIN&#95;02055, which correspond to detecting S. Enteritidis, S. Typhimurium, S. Pullorum, and S. Infantis, respectively. They were integrated into a 1-step multiplex PCR method. We optimized the PCR method by utilizing specificity test results to determine the optimal annealing temperature (57°C). The PCR method exhibited excellent sensitivity for genomic DNA and bacterial cultures. We used the developed method to determine 157 clinical Salmonella isolates from various stages of the poultry production chain. The results aligned with serotype data generated via WGS analysis, demonstrating the method's excellent accuracy. In conclusion, this study developed a 1-step multiplex PCR method that simultaneously identifies S. Enteritidis, S. Typhimurium, S. Pullorum, and S. Infantis, allowing routine mass detection in the grass-root poultry industry., Competing Interests: DISCLOSURES The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

7. Molecular detection of lumpy skin disease virus in naturally infected cattle and buffaloes: unveiling the role of tick vectors in disease spread.

Author

Zeedan GSG, Abdalhamed AM, Allam AM, and Abdel-Shafy S

Subjects

Animals, Cattle, Egypt epidemiology, Real-Time Polymerase Chain Reaction veterinary, Arachnid Vectors virology, Multiplex Polymerase Chain Reaction veterinary, Female, Cattle Diseases virology, Cattle Diseases transmission, Cattle Diseases epidemiology, Male, Rhipicephalus virology, Buffaloes virology, Lumpy skin disease virus isolation & purification, Lumpy skin disease virus genetics, Lumpy Skin Disease virology, Lumpy Skin Disease transmission, Lumpy Skin Disease epidemiology, Lumpy Skin Disease diagnosis

Abstract

Lumpy skin disease (LSD) is a viral disease that affects cattle and buffaloes in Egypt, causing considerable economic losses in the animal sector. This study aimed to investigate the recent outbreak of LSDV in cattle and buffaloes and evaluate the potential role of the hard tick Rhipicephalus annulatus in their transmission through isolation and molecular characterization by multiplex PCR (mPCR) and real-time quantitative PCR (rt-qPCR) assays. A total of 50 skin biopsies (cattle n = 30, buffaloes n = 20), 110 nasal swabs (cattle n = 76, buffaloes n = 44), and 129 blood samples (cattle n = 84, buffaloes n = 45) were collected. In addition, 145 hard ticks of different stages were collected from cattle and buffaloes of different breeds and ages in different governorates in Egypt from November 2021 to June 2022. Multiplex PCR and real-time quantitative PCR (rt-qPCR) assays based on SYBR Green and targets (P32, VP32, G protein, and viral fusion protein) were used. We identified positive results in 17 out of 30 cattle skin biopsies (56.6%), 1 out of 7 buffalo skin scabs (14.3%), and 5 out of 45 buffalo blood samples (11.11%) using mPCR and RT-qPCR methods. We successfully isolated LSDV from hard ticks and cattle infested with ticks and exhibited characteristic signs of LSD on the chorioallantois membrane (CAM) of specific pathogen-free embryonated chicken eggs (SPF-ECE). The isolates were confirmed by multiplex PCR and RT-qPCR. The cyclic threshold (Ct) with correlation-slandered curve values of rt-qPCR ranging from 10.2 to 36.5 showed the amount of LSDV-DNA in different samples. The study's findings demonstrated the widespread circulation of LSDV in both cattle and buffaloes in Egypt and provided strong evidence that hard ticks R. annulatus play a role in the transmission of LSDV in susceptible animals., (© 2024. The Author(s).)

Published

2024

8. Multiplex qPCR development for the simultaneous and rapid detection of largemouth bass virus and infectious spleen and kidney necrosis virus in aquaculture.

Author

Cao W, Huang B, Xu Q, Xie H, Gao J, Mai X, Lin X, Tian C, Huang X, and Zhang H

Subjects

Animals, Reproducibility of Results, Bass virology, Real-Time Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction veterinary, Fish Diseases virology, Fish Diseases diagnosis, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, DNA Virus Infections veterinary, DNA Virus Infections diagnosis, DNA Virus Infections virology, Sensitivity and Specificity, Aquaculture, Iridoviridae isolation & purification, Iridoviridae genetics

Abstract

Largemouth bass virus (LMBV) and infectious spleen and kidney necrosis virus (ISKNV) are both belong to Iridoviridae that cause considerable economic losses in the fish industry. There is no reported literature that can detect these two viruses simultaneously. In this study, we established a multiplex quantitative polymerase chain reaction (qPCR) assay that can specifically and simultaneously detect both LMBV and ISKNV in fish samples. The specificity experiment showed that the method only amplified LMBV and ISKNV but not the other 10 common fish viruses. The slope (m), efficiency (E) and linearity (R 2 ) determined from the generated standard curve were all within the optimal range of qPCR values. The detection limit of the multiplex qPCR assay was as low as 4 copies/μL for LMBV DNA and 7 copies/μL for ISKNV DNA, respectively. The established method exhibited adequate repeatability and reproducibility, and the intra- and inter-assay coefficients of variation were both less than 3 %. The accuracy of the multiplex qPCR method was validated using 229 fish samples and was more precise than that of the conventional PCR assay. In summary, the established multiplex qPCR assay can simultaneously detect LMBV and ISKNV to monitor the risk of infection LMBV and ISKNV and control the disease early., Competing Interests: Declaration of Competing Interest The authors have no conflict of interest to declare., (Copyright © 2024. Published by Elsevier B.V.)

Published

2024

9. A Duplex PCR Assay for Rapid Detection of Klebsiella pneumoniae and Chryseobacterium in Large Yellow Croaker Fish.

Author

Hu G, Yin L, Luo X, Miao Y, and Yu J

Subjects

Animals, Perciformes microbiology, Klebsiella Infections veterinary, Klebsiella Infections diagnosis, Klebsiella Infections microbiology, Flavobacteriaceae Infections veterinary, Flavobacteriaceae Infections microbiology, Flavobacteriaceae Infections diagnosis, Aquaculture, DNA, Bacterial isolation & purification, DNA, Bacterial genetics, Polymerase Chain Reaction methods, Sensitivity and Specificity, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods, DNA Primers, Klebsiella pneumoniae isolation & purification, Klebsiella pneumoniae genetics, Chryseobacterium isolation & purification, Chryseobacterium genetics, Fish Diseases microbiology, Fish Diseases diagnosis

Abstract

Both Klebsiella pneumoniae and Chryseobacterium cause an increasing number of diseases in fish, resulting in great economic losses in aquaculture. In addition, the disease infected with Klebsiella pneumoniae or Chryseobacterium exhibited the similar clinical symptoms in aquatic animals. However, there is no effective means for the simultaneous detection of co-infection and discrimination them for these two pathogens. Here, we developed a duplex polymerase chain reaction (PCR) method based on the outer membrane protein A ( ompA ) gene of Klebsiella pneumoniae and Chryseobacterium . The specificity and validity of the designed primers were confirmed experimentally using simplex PCR. The expected amplicons for Klebsiella pneumoniae and Chryseobacterium had a size of 663 and 1404 bp, respectively. The optimal condition for duplex PCR were determined to encompass a primer concentration of 0.5 μM and annealing temperature of 57°C. This method was analytical specific with no amplification being observed from the genomic DNA of Escherichia coli , Vibrio harveyi , Pseudomonas plecoglossicida , Aeromonas hydrophila and Acinetobacter johnsonii . The limit of detection was estimated to be 20 fg of genomic DNA for Chryseobacterium and 200 fg for Klebsiella pneumoniae , or 100 colony-forming units (CFU) of bacterial cells in both cases. The duplex PCR was capable of simultaneously amplifying target fragments from genomic DNA extracted from the bacteria and fish liver. For practical validation of the method, 20 diseased fish were collected from farms, among which 4 samples were PCR-positive for Klebsiella pneumoniae and Chryseobacterium . The duplex PCR method developed here is time-saving, specific, convenient, and may prove to be an invaluable tool for molecular detection and epidemiological investigation of Klebsiella pneumoniae and Chryseobacterium in the field of aquaculture.

Published

2024

10. Detection of Bartonella spp. in farmed deer (Artiodactyla: Cervidae) using multiplex assays in the Qinghai-Tibet Plateau, China.

Author

Miao Y, Guo W, Zhang W, Chen Z, Mian D, Li R, Xu A, Chen M, and Li D

Subjects

Animals, China epidemiology, Prevalence, Tibet epidemiology, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, DNA, Bacterial genetics, Bartonella genetics, Bartonella isolation & purification, Bartonella classification, Deer microbiology, Bartonella Infections epidemiology, Bartonella Infections veterinary, Bartonella Infections microbiology, Phylogeny

Abstract

In this study, we investigated the prevalence of Bartonella in deer from Qilian County, Qinghai Province, China. Blood samples were collected from 69 red deer, 40 white-lipped deer, and 27 sika deer. The detection of Bartonella spp. has been conducted. The overall prevalence of Bartonella was 33.6% (46/135). Species-specific prevalence was 50.72% in red deer (35/69), 20.00% in white-lipped deer (8/40), and 11.11% in sika deer (3/27). There were significant differences in the prevalence rates among the different species of deer. The amplicon sequence comparison revealed a high homology of the ruminant-associated Bartonella spp. Nanopore sequencing further confirmed the results. Bartonella reads were presented in each of the qPCR-positive samples. Phylogenetic analysis indicated that the Bartonella sequences detected in deer blood were closely related to ruminant-borne Bartonella spp. In summary, we reported the Bartonella prevalence of different deer species in Qinghai, and there were at least one species of ruminant-associated Bartonella , B. schoenbuchensis ., Importance: This is the first report about Bartonella infections in the deer population from China. We found that there were two species of Bartonella and an unidentified species of Bartonella among the unculturing strains carried by these deer populations. We first used Nanopore sequencing to detect Bartonella from deer blood samples and indicated that Nanopore sequencing is beneficial to detect pathogens due to its advantage of real-time and high sensitivity., Competing Interests: The authors declare no conflict of interest.

Published

2024

11. Rapid diagnosis of canine respiratory coronavirus, canine influenza virus, canine distemper virus and canine parainfluenza virus with a Taqman probe-based multiplex real-time PCR.

Author

Zhou H, Li H, Sun X, Lin J, Zhang C, Zhao J, Zhao L, and Zhou M

Subjects

Animals, Dogs, Distemper Virus, Canine genetics, Distemper Virus, Canine isolation & purification, Coronavirus, Canine genetics, Coronavirus, Canine isolation & purification, DNA Primers genetics, Orthomyxoviridae Infections diagnosis, Orthomyxoviridae Infections veterinary, Orthomyxoviridae Infections virology, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Sensitivity and Specificity, Real-Time Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction veterinary, Dog Diseases diagnosis, Dog Diseases virology

Abstract

Canine Infectious Respiratory Disease Complex (CIRDC) is a highly infectious diseases. Canine respiratory coronavirus (CRCoV), Canine influenza virus (CIV), Canine distemper virus (CDV), and Canine parainfluenza virus (CPiV) are crucial pathogens causing CIRDC. Due to the similar clinical symptoms induced by these viruses, differential diagnosis based solely on symptoms can be challenging. In this study, a multiplex real-time PCR assay was developed for detecting the four RNA viruses of CIRDC. Specific primers and probes were designed to target M gene of CRCoV, M gene of CIV, N gene of CDV and NP gene of CPiV. The detection limit is 10 copies/μL for CIV or CRCoV, while the detection limit of CDV or CPiV is 100 copies/μL. Intra-group and inter-group repeatability coefficient of variation (CV) were both less than 2 %. A total of 341 clinical canine samples were analyzed, and the results indicated that the method developed in our study owns a good consistency and better specificity compared with the conventional reverse transcription PCR. This study provides a new method to enable the simultaneous detection of all four pathogens in a single reaction, improving the efficiency for monitoring the prevalence of four viruses in CIRDC, which benefits the control of CIRDC., Competing Interests: Declaration of Competing Interest The authors declare that there are no conflicts of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

12. Establishment and application of multiplex PCR for rapid detection of three mink diarrhea-associated viruses.

Author

Yu Y, Yao Y, Song Y, Shan H, and Han X

Subjects

Animals, China, Circovirus genetics, Circovirus isolation & purification, Bocavirus genetics, Bocavirus isolation & purification, Mink enteritis virus genetics, Mink enteritis virus isolation & purification, Molecular Diagnostic Techniques methods, Molecular Diagnostic Techniques veterinary, Mink virology, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Sensitivity and Specificity, Diarrhea virology, Diarrhea veterinary, Diarrhea diagnosis, DNA Primers genetics, Feces virology

Abstract

In this report, a multiplex PCR method was developed for the detection of three diarrhea-associated viruses in mink, including circovirus (MCV), bocavirus (MBoV), and enteritis virus (MEV). Three compatible sets of primers specific for each virus were designed respectively based on their conserved sequences. After optimization of the crucial factors such as primer concentration and annealing temperature in single and multiple amplification, three specific fragments were simultaneously amplified with the highest sensitivity and specificity in one PCR reaction. The fragments amplified were 259 bp (MCV)，455 bp (MBoV) and 671 bp (MEV). The sensibility of this one-step multiplex PCR is about 10 times lower than that of regular singleplex PCR. There were no cross-reactions with some relevant pathogens like mink coronavirus, canine distemper virus, and aleutian mink disease virus. In our study we analyzed viral DNA in mink fecal samples by multiplex PCR assay from China, which revealed the occurrence of MCV, MBoV, and MEV as 3.1 %, 5.7 %, and 9.8 %, respectively. The testing results of multiplex PCR agreed with the singleplex PCR results with a coincidence rate of 100 %. These results indicated that the method could provide technical support for rapid detection of the three diarrhea-associated viruses, and epidemiological investigation of mink viral diarrhea., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

13. Microscopic detection and molecular characterization of Sarcocystis miescheriana in wild boars (Sus scrofa): first report from Greece.

Author

Dimzas D, Rubiola S, Pacifico L, Veneziano V, Chiesa F, Chassalevris T, and Diakou A

Subjects

Animals, Greece epidemiology, Swine, DNA, Protozoan genetics, Microscopy, Prevalence, Sequence Analysis, DNA, DNA, Mitochondrial genetics, Multiplex Polymerase Chain Reaction veterinary, Electron Transport Complex IV genetics, Diaphragm parasitology, Sarcocystis genetics, Sarcocystis isolation & purification, Sarcocystis classification, Sarcocystosis veterinary, Sarcocystosis parasitology, Sarcocystosis epidemiology, Sus scrofa parasitology, Swine Diseases parasitology, Swine Diseases epidemiology

Abstract

The genus Sarcocystis includes protozoan parasites with an indirect life cycle. Sarcocystis spp. can infect various animal species and humans, causing sarcocystosis, a parasitosis of economic importance and zoonotic concern. Wild boars can act as intermediate hosts for Sarcocystis miescheriana and the zoonotic Sarcocystis suihominis that infects humans by consumption of raw or undercooked infected swine meat. In the present study, the diaphragmatic muscle tissue of 123 wild boars hunted in Greece was examined to determine the frequency of Sarcocystis spp. The samples were examined by tissue compression and molecular techniques. Under light microscopy, 34 out of 123 (27.6%) wild boars tested positive for Sarcocystis spp., while a higher infection prevalence (75%) was revealed by multiplex PCR performed in 100 of the samples. The partial mtDNA cox1 gene (~ 1100 bp) of 20 samples tested positive for S. miescheriana by multiplex PCR was amplified and sequenced. Sarcocystis miescheriana was identified as the only species involved in these infections. This is the first study on the prevalence of Sarcocystis spp. in wild animals in Greece. Further, large-scale surveys are needed to assess the prevalence and species of this parasite in Greece and to design efficient control and preventive measures in a One Health perspective., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2024

14. Multiplex fluorescent amplification-refractory mutation system PCR method for the detection of 10 genetic defects in Holstein cattle and its comparison with the KASP genotyping assay.

Author

Khan MYA, Dai D, Su X, Tian J, Zhou J, Ma L, Wang Y, Wen W, and Zhang Y

Subjects

Animals, Cattle genetics, Cattle Diseases genetics, Multiplex Polymerase Chain Reaction veterinary, Genotype, Polymerase Chain Reaction veterinary, Mutation, Genotyping Techniques veterinary, Genotyping Techniques methods

Abstract

The common deleterious genetic defects in Holstein cattle include haplotypes 1-6 (HH1-HH6), haplotypes for cholesterol deficiency (HCD), bovine leukocyte adhesion deficiency (BLAD), complex vertebral malformation (CVM) and brachyspina syndrome (BS). Recessive inheritance patterns of these genetic defects permit the carriers to function normally, but homozygous recessive genotypes cause embryo loss or neonatal death. Therefore, rapid detection of the carriers is essential to manage these genetic defects. This study was conducted to develop a single-tube multiplex fluorescent amplification-refractory mutation system (mf-ARMS) PCR method for efficient genotyping of these 10 genetic defects and to compare its efficiency with the kompetitive allele specific PCR (KASP) genotyping assay. The mf-ARMS PCR method introduced 10 sets of tri-primers optimized with additional mismatches in the 3' end of wild and mutant-specific primers, size differentiation between wild and mutant-specific primers, fluorescent labeling of universal primers, adjustment of annealing temperatures and optimization of primer concentrations. The genotyping of 484 Holstein cows resulted in 16.12% carriers with at least one genetic defect, while no homozygous recessive genotype was detected. This study found carrier frequencies ranging from 0.0% (HH6) to 3.72% (HH3) for individual defects. The mf-ARMS PCR method demonstrated improved detection, time and cost efficiency compared with the KASP method for these defects. Therefore, the application of mf-ARMS PCR for genotyping Holstein cattle is anticipated to decrease the frequency of lethal alleles and limit the transmission of these genetic defects., (© 2024 Stichting International Foundation for Animal Genetics.)

Published

2024

15. Comparison of bacteriological culture method and multiplex real-time PCR for detection of mastitis.

Author

Kahya Demirbilek S, Yıldız M, Akkoç A, Mutlu AM, Ardıçlı Ö, and Aner H

Subjects

Female, Animals, Cattle, Bacteriological Techniques methods, Bacteriological Techniques veterinary, Milk microbiology, Bacteria isolation & purification, Bacteria genetics, Bacteria classification, Mastitis, Bovine microbiology, Mastitis, Bovine diagnosis, Real-Time Polymerase Chain Reaction veterinary, Real-Time Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods

Abstract

This study includes the evaluation of multiplex real-time PCR (rPCR) kit, which was developed to provide rapid diagnosis of mastitis infections, by working with milk samples of 2 different sources of mastitis and comparing the results with the classical bacteriological culture method (BC). A total of 273 bacteria were isolated in 226 samples (47.88%) out of 472 samples by BC. These were 139 (50.91%) Staphylococcus spp., 61 (22.34%) Streptococcus spp., 15 (5.49%) E. coli, 8 (2.93%) Enterococcus spp., 50 (18.31%) other bacteria. When we look at the multiplex rPCR results; 1052 positive were obtained for the gene regions of 14 different bacteria, 1 yeast, and 1 β-lactamase gene examined in 472 samples. While no searched gene region was found by rPCR in 78 (16.5%) of the 472 samples studied, at least 1 gene was detected in 394 (83.5%) samples. These 1052 positive samples by rPCR were; 263 (28.43%) Staphylococcus spp., 51 (5.51%) S. aureus, 57 (6.16%) Enterococcus spp., 49 (5.29%) C. bovis, 16 (1.73%) S. dysgalactiae, 84 (9.08%) S. agalactiae, 71 (7.67%) S. uberis, 73 (7.89%) E. coli, 14 (1.51%) Prototheca spp., 39 (4.21%) T. pyogenes/P. indolicus, 5 (0.54%) S. marcescens, 15 (1.62%) K. oxytoca/pneumonia, 117 (12.64%) Mycoplasma spp., 31 (3.35%) M. bovis, 40 (4.32%) yeast, and 127 samples (26.90%) were β-lactamase positive. When the antibiotic resistance of the isolates was evaluated, 78 (31.96%) tetracycline, 72 (29.5%) penicillin, and 60 (24.59%) clindamycin resistance were observed predominantly in Gram-positive isolates, while 6 (23.07%) tigecycline, 6 (23.07%) netilmicin, 6 (23.07%) pipercillin resistance was found in gram-negative isolates. While a bacteria and/or yeast gene was found by rPCR in 187 of 246 (76.01%) samples with no bacterial growth, a bacterium was isolated with BC in only 20 (8.84%) samples whose gene region was not found by rPCR. As a result, the multiplex rPCR system used in the diagnosis of mastitis has been found to be quite reliable as it can detect a large number of bacteria in a very short time compared to classical methods. Therefore, we advise the use of rPCR and/or culture for confirmation of clinical signs in mastitis and at routine mastitis surveillance., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier Ltd. All rights reserved.)

Published

2024

16. Detection and differentiation of seven porcine respiratory pathogens using a multiplex ligation-dependent probe amplification assay.

Author

Zhou Y, Yu H, Zhao X, Ni J, Gan S, Dong W, Du J, Zhou X, Wang X, and Song H

Subjects

Animals, Swine, Sensitivity and Specificity, Respiratory Tract Infections veterinary, Respiratory Tract Infections virology, Respiratory Tract Infections microbiology, Respiratory Tract Infections diagnosis, Porcine respiratory and reproductive syndrome virus isolation & purification, Porcine respiratory and reproductive syndrome virus genetics, Virus Diseases veterinary, Virus Diseases virology, Virus Diseases diagnosis, Nucleic Acid Amplification Techniques veterinary, Nucleic Acid Amplification Techniques methods, Swine Diseases virology, Swine Diseases microbiology, Swine Diseases diagnosis, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods

Abstract

Respiratory diseases due to viral or bacterial agents, either alone or in combination, cause substantial economic burdens to the swine industry worldwide. Rapid and reliable detection of causal pathogens is crucial for effective epidemiological surveillance and disease management. This research aimed to employ the multiplex ligation-dependent probe amplification (MLPA) assay for simultaneous detection of seven distinct pathogens causing respiratory problems in swine, porcine reproductive and respiratory syndrome virus (PRRSV), swine influenza virus (SIV), porcine respiratory coronavirus (PRCV), porcine circovirus type 2 (PCV2), Pasteurella multocida, Actinobacillus pleuropneumoniae, and Glässerella parasuis. The results indicated no probe cross-reactivity among the seven target agents with other swine pathogens. The detection limits ranged from 5 to 34 copies per assay for the target organisms. The MLPA assay was evaluated with 88 samples and compared to real-time or multiplex PCR for the target pathogens. The MLPA assay demonstrated high relative test sensitivities (100 %) and reasonable to good relative specificities at 62.5 %, 95.1 %, 86.8 %, and 97.6 % for PRRSV, P. multocida, G. parasuis, and PCV2, respectively, relative to comparator PCR assays. In 71 samples where MLPA and comparator PCR assays matched exactly, infections were detected in 64 samples (90.1 %), with PRRSV being the most commonly found virus and 50.7 % of the samples showing co-infection with two to five of the pathogens. This approach serves as a valuable tool for conducting differential diagnoses and epidemiological investigations of pathogen prevalence within swine populations., (Copyright © 2024. Published by Elsevier Ltd.)

Published

2024

17. Improving the detection of integrative conjugative elements in bovine nasopharyngeal swabs using multiplex recombinase polymerase amplification.

Author

Conrad CC, Funk T, Andrés-Lasheras S, Yevtushenko C, Claassen C, Otto SJG, Waldner C, Zaheer R, and McAllister TA

Subjects

Animals, Cattle, Interspersed Repetitive Sequences genetics, Cattle Diseases microbiology, Cattle Diseases diagnosis, DNA, Bacterial genetics, Drug Resistance, Bacterial genetics, Bovine Respiratory Disease Complex microbiology, Conjugation, Genetic, Sensitivity and Specificity, Mannheimia haemolytica genetics, Mannheimia haemolytica isolation & purification, Pasteurellaceae genetics, Pasteurellaceae isolation & purification, Nasopharynx microbiology, Recombinases genetics, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary

Abstract

Bovine respiratory disease (BRD) is an important health and economic burden to the cattle industry worldwide. Three bacterial pathogens frequently associated with BRD (Mannheimia haemolytica, Pasteurella multocida, and Histophilus somni) can possess integrative and conjugative elements (ICEs), a diverse group of mobile genetic elements that acquire antimicrobial resistance (AMR) genes (ARGs) and decrease the therapeutic efficacy of antimicrobial drugs. We developed a duplex recombinase polymerase amplification (RPA) assay to detect up to two variants of ICEs in these Pasteurellaceae. Whole genome sequence analysis of M. haemolytica, P. multocida, and H. somni isolates harbouring ICEs revealed the presence of tnpA or ebrB next to tet(H), a conserved ARG that is frequently detected in ICEs within BRD-associated bacteria. This real-time multiplex RPA assay targeted both ICE variants simultaneously, denoted as tetH&#95;tnpA and tetH&#95;ebrB, with a limit of detection (LOD) of 29 (95% CI [23, 46]) and 38 genome copies (95% CI [30, 59]), respectively. DNA was extracted from 100 deep nasopharyngeal swabs collected from feedlot cattle on arrival. Samples were tested for ICEs using a real-time multiplex RPA assay, and for M. haemolytica, P. multocida, H. somni, and Mycoplasma bovis using both culture methods and RPA. The assay provided sensitive and accurate identification of ICEs in extracted DNA, providing a useful molecular tool for timely detection of potential risk factors associated with the development of antimicrobial-resistant BRD in feedlot cattle., Competing Interests: Declaration of competing interest The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2024. Published by Elsevier B.V.)

Published

2024

18. Rapid differentiation of infectious salmon anemia virus avirulent (HPR0) from virulent (HPRΔ) variants using multiplex RT-qPCR.

Author

Rounsville TF Jr, Polinski MP, Marini AG, Turner SM, Vendramin N, Cuenca A, Pietrak MR, Peterson BC, and Bouchard DA

Subjects

Animals, Orthomyxoviridae Infections veterinary, Orthomyxoviridae Infections virology, Orthomyxoviridae Infections diagnosis, Virulence, Real-Time Polymerase Chain Reaction veterinary, Real-Time Polymerase Chain Reaction methods, Isavirus genetics, Isavirus isolation & purification, Fish Diseases virology, Fish Diseases diagnosis, Salmo salar virology, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods

Abstract

Infectious salmon anemia virus (ISAV; Isavirus salaris ) causes an economically important disease of Atlantic salmon ( Salmo salar L.). ISA outbreaks have resulted in significant losses of farmed salmon globally, often with a sudden onset. However, 2 phenotypically distinct variants of ISAV exist, each with divergent disease outcomes, associated regulations, and control measures. ISAV-HPRΔ, also known as ISAV-HPR deleted, is responsible for ISA outbreaks; ISAV-HPR0, is avirulent and is not known to cause fish mortality. Current detection methodology requires genetic sequencing of ISAV-positive samples to differentiate phenotypes, which may slow responses to disease management. To increase the speed of phenotypic determinations of ISAV, we developed a new, rapid multiplex RT-qPCR method capable of 1) detecting if a sample contains any form of ISAV, 2) discriminating whether positive samples contain HPRΔ or HPR0, and 3) validating RNA extractions with an internal control, all in a single reaction. Following assay development and optimization, we validated this new multiplex on 31 ISAV strains collected from North America and Europe (28 ISAV-HPRΔ, 3 ISAV-HPR0). Finally, we completed an inter-laboratory comparison of this multiplex qPCR with commercial ISAV testing and found that both methods provided equivalent results for ISAV detection., Competing Interests: Declaration of conflicting interestsThe authors declared no potential conflicts of interest with respect to the research, authorship, and/or publication of this article.

Published

2024

19. Characterization of Actinobacillus pleuropneumoniae biovar 2 isolates reportedly reacted with the serovar 4 antiserum, and development of a multiplex PCR for O-antigen typing.

Author

To H, Maldonado J, Tsutsumi N, Gottschalk M, Frey J, and Nagai S

Subjects

Animals, Swine, Serogroup, Multiplex Polymerase Chain Reaction veterinary, O Antigens genetics, Serotyping veterinary, Actinobacillus pleuropneumoniae, Actinobacillus Infections veterinary, Swine Diseases

Abstract

We have analyzed the capsule (CPS) and the lipopolysaccharide O-Antigen (O-Ag) biosynthesis loci of twelve Spanish field isolates of Actinobacillus pleuropneumoniae biovar 2, eleven of them previously typed serologically as serovar 4 and one non-typable (NT) (Maldonado et al., 2009, 2011). These isolates have the common core genes of the type I CPS locus, sharing >98% identity with those of serovar 2. However, the former possesses the O-Ag locus as serovar 4, and the latter possesses the O-Ag locus as serovar 7. The main difference found between the CPS loci of the 11 isolates and that of serovar 2 reference strain S1536 are two deletions, one of an 8 bp sequence upstream of the coding sequence and one of 111 bp sequence at the 5' end of the cps2G gene. The deletion mutations mentioned lead to a defect in the production of CPS in these isolates, which contributed to their previous mis-identification. In order to complement the serotyping of A. pleuropneumoniae in diagnostics and epidemiology, we have developed a multiplex PCR for the comprehensive O-Ag typing of all A. pleuropneumoniae isolates., Competing Interests: Declaration of Competing Interest We declare that we have no conflict of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

20. Comparison of Giardia duodenalis point-of-care antigen faecal tests to reference laboratory assays in non-symptomatic dogs.

Author

Ktenas S, Roeber F, Meggiolaro MN, Ktenas A, Ward MP, and Šlapeta J

Subjects

Humans, Dogs, Animals, Point-of-Care Systems, Multiplex Polymerase Chain Reaction veterinary, Real-Time Polymerase Chain Reaction veterinary, Antigens, Protozoan genetics, DNA, Feces parasitology, Giardia lamblia genetics, Giardiasis diagnosis, Giardiasis veterinary, Giardiasis parasitology, Dog Diseases diagnosis, Dog Diseases parasitology

Abstract

Giardia duodenalis is one of the most prevalent enteric parasites of dogs. Point-of-care antigen tests (POC) are rapid and do not require additional equipment, or a specialised diagnostic laboratory. The aim of this study was to compare diagnostic tests available in veterinary practices and in a diagnostic laboratory for the detection of G. duodenalis on a cohort of group-housed dogs from New South Wales, Australia. Two different POC tests were used for the detection of G. duodenalis. Laboratory tests used were the multiplexed-tandem PCR panel (MT-PCR) that includes detection of G. duodenalis DNA, and two reference tests (an in-house TaqMan real-time PCR and a direct immunofluorescence assay, DFA). Canine faecal samples (n = 40) were tested simultaneously for the detection of G. duodenalis. Using either DFA or TaqMan real-time PCR as reference tests, 77.5% (31/40) and 82.5% (33/40) of dogs tested positive, respectively. Agreement (Kappa) between the DFA and TaqMan real-time PCR was 0.84 (95% CI 0.64 to 1.00). There was substantial G. duodenalis test outcome agreement between the two POC tests, Kappa = 0.75. Combining the two POC tests yielded 77% sensitivity and 100% specificity with DFA as reference, and for TaqMan real-time PCR it was 73% sensitivity and 100% specificity. The MT-PCR was in excellent agreement with each reference test, DFA or TaqMan real-time PCR. Due to the high specificity of both POC tests, they can be confidently used as rule-in diagnostics. Confirmatory testing that detects different biological parameters such as DNA, e.g. PCR (inc. MT-PCR), should be implemented before concluding that a dog is negative for the presence of G. duodenalis., Competing Interests: Declaration of Competing Interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Editorial Board of Veterinary Parasitology (JS)., (Copyright © 2024 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2024

21. Development of a Multiplex PCR Assay for Rapid Differentiation of Fowlpox and Pigeonpox Viruses.

Author

Özgünlük İ, Yücetepe AG, Çetiner B, Keskin O, and Özyörük F

Subjects

Animals, Turkeys, Fowlpox virology, Fowlpox diagnosis, Species Specificity, Phylogeny, Bird Diseases virology, Bird Diseases diagnosis, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods, Columbidae, Fowlpox virus genetics, Fowlpox virus isolation & purification, Poxviridae Infections veterinary, Poxviridae Infections virology, Poxviridae Infections diagnosis, Poultry Diseases virology, Poultry Diseases diagnosis, Avipoxvirus genetics, Avipoxvirus isolation & purification, Avipoxvirus classification, Chickens

Abstract

The aim of this study was to develop a multiplex PCR assay capable of rapidly differentiating two major Avipoxvirus (APV) species, Fowlpox virus (FWPV) and Pigeonpox virus (PGPV), which cause disease in bird species. Despite the importance of a rapid differentiation assay, no such assay exists that can differentiate the APV species without sequencing. To achieve this, species-specific target DNA fragments were selected from the fpv122 gene of FWPV and the HM89&#95;gp120 gene of PGPV, which are unique to each genome. Nine samples collected from unvaccinated chickens, pigeons, and a turkey with typical pox lesions were genetically identified as FWPV and PGPV. The designed primers and target DNA fragments were validated using in silico analyses with the nucleotide Basic Local Alignment Search Tool. The multiplex PCR assay consisted of species-specific primers and previously described PanAPV primers (genus-specific) and was able to differentiate FWPV and PGPV, consistent with the phylogenetic outputs. This study represents the first successful differentiation of FWPV and PGPV genomes using a conventional multiplex PCR test. This assay has the potential to facilitate the rapid diagnosis and control of APV infections.

Published

2024

22. Equine Piroplasmosis in Asymptomatic Horses of Western Iran: Comparison of Microscopic Examination and Multiplex PCR.

Author

Mohammad-Naseri A, Shokrani H, and Rahmani-Shahraki A

Subjects

Animals, Horses, Iran epidemiology, Male, Female, Prevalence, DNA, Protozoan genetics, Theileriasis epidemiology, Theileriasis diagnosis, Theileriasis parasitology, Sensitivity and Specificity, Horse Diseases parasitology, Horse Diseases diagnosis, Horse Diseases epidemiology, Babesiosis epidemiology, Babesiosis diagnosis, Babesiosis parasitology, Babesia genetics, Babesia isolation & purification, Babesia classification, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Theileria genetics, Theileria isolation & purification, Theileria classification, Microscopy methods

Abstract

Purpose: Piroplasmosis is responsible for anemia, fever, loss of physical activity and even death in equines. In epidemiological studies, accurate diagnostic tests are essential for detecting asymptomatic carriers. This study aimed to investigate the prevalence of infection in asymptomatic horses from Lorestan province, western Iran by developing a multiplex PCR., Methods and Results: Blood samples were examined by microscopy and multiplex PCR targeting the SSU rRNA gene of Theileria equi and Babesia caballi. Out of the total of 165 horses, 19 (11.51%) and 31 (18.78%) cases were positive for piroplasms by microscopy and PCR, respectively. The detection rates of both genera were significantly higher in multiplex PCR compared to microscopy (p < 0.0001). Compared with multiplex PCR, the sensitivities of microscopy for the detection of Babesia were only 28.5%. The prevalence of T. equi infection was significantly higher in summer (p = 0.035). The prevalence of B. caballi was significantly higher in males (p = 0.038)., Conclusion: Findings indicate that the multiplex PCR described here is a sensitive technique for the detection of piroplasm DNA in carriers. Furthermore, asymptomatic carriers must be considered as an important source of infection for equids living in this region., (© 2024. The Author(s), under exclusive licence to Springer Nature Switzerland AG.)

Published

2024

23. Bacteriological evaluation and advanced SYBR-green multiplex real-time PCR assay for detection of minced meat adulteration.

Author

El-Sheikh SH, Whab RMA, ElDaly RA, Raslan MT, Fahmy HA, and El-Demerdash AS

Subjects

Animals, Cattle, Horses, Swine, Dogs, Real-Time Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction veterinary, Escherichia coli, Food Contamination analysis, Meat, Diamines, Quinolines, Benzothiazoles

Abstract

Background: Minced meat is a valuable source of nutrients, but it is vulnerable to contamination by microorganisms commonly present in the environment. In addition, there is a risk of adulteration with cheaper meat sources, which can be harmful to consumers., Aim: It is crucial to identify meat adulteration with distinct microbiological analysis for legal, economic, religious, and public health purposes., Methods: A total of 100 minced meat samples were collected from several markets in Sharkia Governorate, Egypt. These samples were then subjected to bacteriological testing and an advanced multiplex PCR method. This method enables the detection of bovine, equine, porcine, and dog species in meat samples with just one step., Results: The adulterated samples had a higher total bacterial count and pH values compared to pure bovine meat. These differences in bacterial count and pH values were statistically significant, with p- values of 0.843 (log 10 ) and 0.233, respectively. The frequency of Escherichia coli occurrence was 13%, and the O111 serotype was predominant in the adulterated samples. Listeria monocytogenes and Staphylococcus aureus were isolated with prevalence rates of 3% and 29%, respectively. Besides, the SYBR-green multiplex real-time PCR assay used in this study detected adulteration with dog, equine, and porcine meats in the examined samples at rates of 9%, 5%, and 4%, respectively., Conclusion: This method provides a sensitive and specific approach to detect issues related to well-being and safety., Competing Interests: All authors declare that there is no conflict of interest.

Published

2024

24. Molecular identification and characterisation of Mannheimia haemolytica.

Author

Kayal A, Nahar N, Barker L, Tran T, Williams M, Blackall PJ, Turni C, and Omaleki L

Subjects

Cattle, Animals, Bacteria genetics, Serotyping methods, Serotyping veterinary, Ruminants, Multiplex Polymerase Chain Reaction veterinary, Mannheimia haemolytica, Cattle Diseases microbiology, Respiratory Tract Diseases veterinary

Abstract

Mannheimia haemolytica is known as one of the major bacterial contributors to Bovine Respiratory Disease (BRD) syndrome. This study sought to establish a novel species-specific PCR to aid in identification of this key pathogen. As well, an existing multiplex PCR was used to determine the prevalence of serovars 1, 2 or 6 in Australia. Most of the 65 studied isolates originated from cattle with a total of 11 isolates from small ruminants. All problematic field isolates in the identification or serotyping PCRs were subjected to whole genome sequencing and bioinformatic analysis. The field isolates were also subjected to rep-PCR fingerprinting. A total of 59 out of the 65 tested isolates were conformed as M. haemolytica by the new species-specific PCR which is based on the rpoB gene. The confirmed M. haemolytica field isolates were assigned to serovars 1 (24 isolates), 2 (seven isolates) and 6 (26 isolates) while two of the isolates were negative in the serotyping PCR. The two non-typeable isolates were assigned to serovar 7 and 14 following whole genome sequencing and bioinformatic analysis. The rep-PCR typing resulted in five major clusters with serovars 1 and 6 often within the same cluster. The M. haemolytica-specific PCR developed in this work was species specific and should be a valuable support for frontline diagnostic laboratories. The serotyping results support the relative importance of serovars 1 and 6 in bovine respiratory disease., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2023 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2024

25. Is Brucella excreted in cattle faeces? - Evidence from Punjab, India.

Author

Sharma V, Kaur P, Aulakh RS, Sharma R, Verma R, and Singh BB

Subjects

Cattle, Animals, Humans, RNA, Ribosomal, 16S genetics, Brucella abortus, Multiplex Polymerase Chain Reaction veterinary, India epidemiology, Brucellosis epidemiology, Brucellosis veterinary

Abstract

Brucellosis is a neglected zoonosis that affects animals and people in much of the underdeveloped world. The disease is endemic in cattle in Punjab, India and controlling it is a public health challenge. Dairy farmers and farm labour commonly handle cattle faeces with bare hands and personal protective equipments are not used. No studies have been conducted about the shedding of Brucella species in faeces of sero positive cattle in the state. This study aimed to isolate and identify the Brucella species from faeces of sero positive cattle in Punjab, India. Faecal samples were collected from 350 Brucella sero positive cattle in Ludhiana district of Punjab, India. Isolation was performed using a pre-enriched Brucella selective broth medium as well as Brucella selective medium agar plates containing horse serum and Brucella selective supplements. Isolates were identified using Gram staining technique and rapid slide agglutination test, and then confirmed by using bcsp31 and 16s rRNA genus specific PCR. Isolates were further identified up to species level by using Bruce-Ladder multiplex PCR. Fourteen Brucella species were isolated, all of which showed coccobacilli on gram staining, positive rapid slide agglutination test and amplification of bcsp31 and 16s rRNA genes. Of the 14 isolates, 11 were identified as Brucella abortus and 3 were identified as Brucella melitensis. The study demonstrates that animal faeces could pose a potential risk for animal and human health and faeces of seropositive cattle must be handled with care., Competing Interests: Declaration of Competing Interest None declared., (Copyright © 2023 Elsevier Ltd. All rights reserved.)

Published

2024

26. PCR-based methods in detection and identification of dermatophytes in dogs and cats with suspected dermatophytosis in 2021 in Poland.

Author

Jańczak D, Górecki P, and Maj AK

Subjects

Humans, Animals, Cats, Dogs, Poland epidemiology, Microsporum genetics, Trichophyton genetics, Multiplex Polymerase Chain Reaction veterinary, Mammals genetics, Arthrodermataceae genetics, Dermatomycoses diagnosis, Dermatomycoses epidemiology, Dermatomycoses veterinary, Cat Diseases diagnosis, Cat Diseases epidemiology, Dog Diseases diagnosis, Dog Diseases epidemiology, Tinea diagnosis, Tinea epidemiology, Tinea veterinary

Abstract

Dermatophytes from Microsporum, Trichophyton and Epidermophyton genera are divided into geophilic, zoophilic and anthropophilic species which cause skin infection in humans and wide group of animals, mainly mammals. Main species causing dermatophytosis in dogs and cats are Microsporum and Trichophyton. Conventional mycological diagnostic technique includes Saburaud Dextrose Agar (SAD) and others medium cultures, 10% KOH mount and direct microscopy of hairs and scraping. Molecular diagnostic become more frequent in veterinary practice due to shortening of waiting time. In this study we based on two PCR methods. The nested PCR amplified CHS1 gene for dermatophytes detection, and multiplex PCR coding ITS1 and ITS2 fragments for species identification of detected derpatophytes. Most frequently detected species was Microsporum canis, mainly in young cats. Geophilic Microsporum gypseum and anthropophilic Trichophyton rubrum was found primarily in dogs. Molecular methods in dermatophytosis identification are rapid in contrast to routinely, long lasting culture.

Published

2023

27. Virulence gene profiles and antimicrobial susceptibility of Salmonella Brancaster from chicken.

Author

Khoo E, Roslee R, Zakaria Z, and Ahmad NI

Subjects

Animals, Virulence genetics, Salmonella genetics, Anti-Bacterial Agents pharmacology, Chloramphenicol, Ampicillin, Tetracycline, Microbial Sensitivity Tests veterinary, Multiplex Polymerase Chain Reaction veterinary, Streptomycin, Drug Resistance, Multiple, Bacterial, Chickens genetics, Salmonella enterica genetics

Abstract

Background: The current conventional serotyping based on antigen-antisera agglutination could not provide a better understanding of the potential pathogenicity of Salmonella enterica subsp. enterica serovar Brancaster. Surveillance data from Malaysian poultry farms indicated an increase in its presence over the years., Objective: This study aims to investigate the virulence determinants and antimicrobial resistance in S. Brancaster isolated from chickens in Malaysia., Methods: One hundred strains of archived S. Brancaster isolated from chicken cloacal swabs and raw chicken meat from 2017 to 2022 were studied. Two sets of multiplex polymerase chain reaction (PCR) were conducted to identify eight virulence genes associated with pathogenicity in Salmonella (invasion protein gene [ invA ], Salmonella invasion protein gene [ sipB ], Salmonella- induced filament gene [ sifA ], cytolethal-distending toxin B gene [ cdtB ], Salmonella iron transporter gene [ sitC ], Salmonella pathogenicity islands gene [ spiA ], Salmonella plasmid virulence gene [ spvB ], and inositol phosphate phosphatase gene [ sopB ]). Antimicrobial susceptibility assessment was conducted by disc diffusion method on nine selected antibiotics for the S. Brancaster isolates. S. Brancaster, with the phenotypic ACSSuT-resistance pattern (ampicillin, chloramphenicol, streptomycin, sulphonamides, and tetracycline), was subjected to PCR to detect the corresponding resistance gene(s)., Results: Virulence genes detected in S . Brancaster in this study were invA , sitC , spiA , sipB , sopB , sifA , cdtB , and spvB . A total of 36 antibiogram patterns of S . Brancaster with a high level of multidrug resistance were observed, with ampicillin exhibiting the highest resistance. Over a third of the isolates displayed ACSSuT-resistance, and seven resistance genes (β-lactamase temoneira [ bla TEM ], florfenicol/chloramphenicol resistance gene [ floR ], streptomycin resistance gene [ strA ], aminoglycoside nucleotidyltransferase gene [ ant(3″)-Ia ], sulfonamides resistance gene [ sul-1 , sul-2 ], and tetracycline resistance gene [ tetA ]) were detected., Conclusion: Multidrug-resistant S. Brancaster from chickens harbored an array of virulence-associated genes similar to other clinically significant and invasive non-typhoidal Salmonella serovars, placing it as another significant foodborne zoonosis., Competing Interests: The authors declare no conflicts of interest., (© 2023 The Korean Society of Veterinary Science.)

Published

2023

28. Development of multiplex PCR assay for simultaneous detection of African swine fever, porcine circo and porcine parvo viral infection from clinical samples.

Author

Pegu SR, Deb R, Das PJ, Sengar GS, Yadav AK, Rajkhowa S, Paul S, and Gupta VK

Subjects

Animals, Swine, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods, African Swine Fever diagnosis, Coinfection diagnosis, Coinfection veterinary, Circoviridae Infections diagnosis, Circoviridae Infections veterinary, Swine Diseases diagnosis, Virus Diseases diagnosis, Parvoviridae Infections, Parvovirus, Porcine genetics

Abstract

A diagnostic method for simultaneously detecting and distinguishing African Swine Fever (ASF), porcine circovirus type 2 (PCV2), and porcine parvovirus (PPV) in clinical specimens is critical for differential diagnosis, monitoring, and control in the field. Three primer pairs were designed and used to create a multiplex PCR assay. In addition, 356 porcine post mortem tissue samples from various parts of India's North Eastern region were tested by the developed multiplex PCR assay to demonstrate its accuracy. Using the designed primers, each of the ASF, PCV2 and PPV target genes was amplified, but no other porcine virus genes were detected. The assay's limit of detection was 10 2 copies/µl of PCV2, PPV, or ASFV. The detection of PCV2, PPV, and ASF in postmortem tissue samples revealed that they are co-circulating in India's North-Eastern region. The percentage positivity (PP) for PCV2, PPV and ASF single infection were 7.02% (25/356), 3.93% (14/356), and 3.37% (12/356), respectively, while the PP for PCV2& PPV co-infection was 2.80% (10/356), ASF & PCV2 co infection was 1.4% (5/356) and the ASF, PPV& PCV2 co-infection was1.40% (5/356). The results also indicate that the ASF can infect pigs alongside PCV and PPV.

Published

2023

29. Molecular differentiation of Sarcocystis miescheriana and Sarcocystis suihominis using a new multiplex PCR targeting the mtDNA cox1 gene in wild boars in southern Italy.

Author

Pacifico L, Rubiola S, Buono F, Sgadari M, D'Alessio N, Scarcelli S, Sgroi G, Buglione M, Chiesa F, Restucci B, Fioretti A, Prakas P, and Veneziano V

Subjects

Animals, DNA, Mitochondrial analysis, DNA, Mitochondrial chemistry, Italy epidemiology, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Phylogeny, Sus scrofa genetics, Swine, Electron Transport Complex IV genetics, Sarcocystis genetics, Sarcocystosis epidemiology, Sarcocystosis veterinary, Sarcocystosis parasitology, Swine Diseases diagnosis, Swine Diseases epidemiology, Swine Diseases parasitology

Abstract

The increase of wild boar populations density and their meat consumption across Europe could expose humans to a plethora of foodborne diseases as sarcocystosis, caused by the zoonotic protozoan Sarcocystis suihominis. Humans become infected by eating raw or undercooked pig (Sus scrofa domesticus) containing S. suihominis sarcocysts. Despite this, to date very few data are available on the risk of infection by this parasite to wild boar (Sus scrofa) meat consumers. Thus, the present study aimed to assess the occurrence of Sarcocystis spp. in wild boars from southern Italy, applying both histology and a new multiplex PCR assay targeting the cox1 gene. Between 2019 and 2020, 997 muscle tissues (i.e., n = 269 oesophagus, n = 277 diaphragms, n = 298 hearts, n = 153 tongues) from 311 wild boars were collected and screened by a combined histological and molecular approach. Overall, 251 (80.7%) animals tested were positive for Sarcocystis spp., and S. miescheriana whose definitive hosts are canids, was the only molecularly identified species. A statistically significant difference (p < 0.05) in the prevalence of Sarcocystis infection was found according to the wild boar age and muscle tissue. Findings outlined the low zoonotic potential of infection to humans via wild boar meat consumption in Italy and the importance of the application of new molecular methods in distinguishing different Sarcocystis species., Competing Interests: Declaration of Competing Interest None., (Copyright © 2023. Published by Elsevier Ltd.)

Published

2023

30. Clinical evaluation of a dermatophyte RT-PCR assay and its impact on the turn-around-time: A prospective study.

Author

Debuysschere C, Blairon L, Cupaiolo R, Beukinga I, and Tré-Hardy M

Subjects

Animals, Prospective Studies, Reverse Transcriptase Polymerase Chain Reaction veterinary, DNA, Fungal, Sensitivity and Specificity, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Trichophyton genetics, Onychomycosis diagnosis, Onychomycosis veterinary, Arthrodermataceae genetics

Abstract

Onychomycosis is an important public health problem whose prevalence continues to grow and impact public health at several levels. Nevertheless, today the main diagnostic methods used in routine practice have many drawbacks. The aim of this study was to evaluate, for the first time, the clinical performance of a new multiplex polymerase chain reaction (PCR) (Novaplex®) in the identification of the causative agent on nail samples, and its impact on the turnaround time, compared to our traditional laboratory methods. From June 2022 to December 2022, all nail samples sent to our laboratory for suspected onychomycosis were included in this prospective study. We collected for each sample the results obtained with the Novaplex® PCR method and with the traditional direct microscopy examination and culture. Each discordant result was checked using a third method, which is another PCR method (DermaGenius® kit) as a resolver. For culture-positive samples, a turnaround time was calculated and compared to the one obtained with the Novaplex® method. A total of 131 samples were included. Among them, 5 were positive (3.8%) on direct microscopy, 33 were positive (25.2%) after culture, and 98 were negative (74.8%). All positive (n = 33) and negative (n = 69) cultures were also positive/negative with the Novaplex® PCR. Twenty-nine samples were positive with the Novaplex® method but negative with culture (discordant results). The percentage agreement between the culture and the Novaplex® methods was 77.9% (102 out of 131). While tested with the resolver (DermaGenius® PCR), 28 out of 29 discordant results were similarly found positive. The percentage agreement between the two PCR methods (Novaplex® and DermaGenius®) was 96.6%. The Novaplex® PCR method evaluated proved to be very reliable and allowed the direct identification of 62 out of 131 positive samples (47.3%) with the following distribution: 79.0% of Trichophyton rubrum complex, 11.3% of Trichophyton mentagrophytes complex, 6.5% of both Trichophyton rubrum complex and Trichophyton mentagrophytes complex, and 3.2% of Candida albicans. The median time [± 95% CI] for positive culture (between incubation and validation of the final identification) was 15 [12-23] days, while the turnaround time for the Novaplex® method adapted to our clinical laboratory routine is ≤7 days. Laboratory confirmation of onychomycosis is crucial and should always be obtained before starting treatment. The evaluated PCR method offered a rapid, reliable, robust, and inexpensive method of identification of the causative agent compared to traditional methods., (© The Author(s) 2023. Published by Oxford University Press on behalf of The International Society for Human and Animal Mycology.)

Published

2023

31. Simultaneous and rapid detection of avian respiratory diseases of small poultry using multiplex reverse transcription-Polymerase Chain Reaction assay.

Author

Piri-Gharaghie T, Ghajari G, Lahijani NT, Pecho RDC, Hussam F, Castillo-Acobo RY, and Aghassizadeh-Sherbaf M

Subjects

Animals, Poultry, Reverse Transcriptase Polymerase Chain Reaction veterinary, Reproducibility of Results, Reverse Transcription, Chickens, Sensitivity and Specificity, Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods, Bird Diseases, Virus Diseases veterinary, Respiratory Tract Infections veterinary, Poultry Diseases diagnosis

Abstract

Major viral infections, such as Newcastle disease virus, infectious bronchitis virus, avian influenza virus, and infectious bursal disease virus, inflict significant injury to small poultry and tremendous economic damage to the poultry sector. This research aims to develop a multiplex reverse transcriptase polymerase chain reaction (m-RT-PCR) approach to simultaneously determine these important viral pathogens. The conserved segment of various viral genetic sequences was used to design and synthesize specific primers. Moreover, as positive controls, recombinant vectors were synthesized in this investigation. The d-optimal approach was used to improve PCR conditions in this investigation. Positive controls and clinical samples were used to assess the m-PCR assay's specificity, sensitivity, repeatability, and reproducibility. According to the sensitivity test findings, the m-PCR technique could generate the 8 target genes from viral genomes using 1 × 102. In addition, 8 viral pathogens were detected from the infected samples. The findings also suggest that live animal oral swabs were not significantly different from tissue sampling of a dead animal (P < 0.05), and this kit had a high sensitivity for analyzing both types of samples. The suggested m-PCR test may detect and evaluate viral infection in birds with excellent specificity, sensitivity, and throughput., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2023

32. A novel one-step multiplex PCR protocol to detect avian haemosporidian parasites in the subgenus Haemoproteus (Kruse, 1890) used to quantify parasite prevalence in domestic pigeons (Columba livia) in Turkey.

Author

Ciloglu A, Yildirim A, Pekmezci D, Yetismis G, Sursal Simsek N, Simsek E, Duzlu O, Onder Z, Delibasi Kokcu N, Pekmezci GZ, Ellis VA, and Inci A

Subjects

Animals, Columbidae genetics, Columbidae parasitology, Multiplex Polymerase Chain Reaction veterinary, Prevalence, Turkey, DNA, Protozoan genetics, Parasites genetics, Protozoan Infections, Animal diagnosis, Protozoan Infections, Animal epidemiology, Protozoan Infections, Animal parasitology, Bird Diseases diagnosis, Bird Diseases epidemiology, Haemosporida genetics

Abstract

Infections of avian haemosporidian parasites are regularly identified by molecular methods including multiplex PCR, which allows researchers to distinguish mixed infections of parasites from multiple genera. Here we extend the utility of a previously designed multiplex PCR by designing a primer set specific to parasites of the subgenus Haemoproteus (genus: Haemoproteus). The updated one-step multiplex PCR protocol we describe here allows for the detection of the genera Plasmodium and Leucocytozoon and the two subgenera (Haemoproteus and Parahaemoproteus) of the genus Haemoproteus. A sensitivity analysis showed that the multiplex PCR could amplify DNA of parasites in the subgenus Haemoproteus at very low levels of infection. We used this multiplex PCR to identify haemosporidian infections in 250 adult domestic pigeons (Columba livia) in Turkey. All samples were also screened by microscopy and a widely used nested PCR to compare with the results of multiplex PCR, to detect low levels of parasitemia, and to identify possible abortive infections. In total, 71 pigeons (28.4%) were found to be infected by all three methods. The multiplex PCR protocol successfully detected and discriminated both subgenera Haemoproteus and Parahaemoproteus infections. We compared our results with previous host species records to assess the host specificity of the parasite lineages we found. Our findings provide novel data on the prevalence of avian haemosporidians in domestic pigeons and demonstrate the utility of the new one-step multiplex PCR protocol for the determination of mixed avian haemosporidian infections. We expect that this protocol will contribute to a better understanding of the distribution, epizootiology, and ecology of avian haemosporidians., (© 2022. The Author(s), under exclusive licence to Springer Nature B.V.)

Published

2023

33. A novel time-saving multiplex PCR assay for detecting and discriminating the most common canine Babesia species in Europe.

Author

Remesar S, Méndez A, Benito A, Prieto A, García-Dios D, López CM, Panadero R, Díez-Baños P, Morrondo P, and Díaz P

Subjects

Dogs, Animals, Multiplex Polymerase Chain Reaction veterinary, Europe epidemiology, Babesia genetics, Babesiosis diagnosis, Babesiosis epidemiology, Dog Diseases diagnosis, Dog Diseases epidemiology

Abstract

In Europe, most cases of canine babesiosis are caused by Babesia canis, Babesia vogeli (large piroplasms) and Babesia vulpes (small piroplasm). Molecular diagnosis is recommended due to its high sensitivity. Species identification after sequencing allows applying a rapid and efficient treatment, leading to a better prognosis; however, it is expensive and time-consuming. Thus, the objective of the present study was to develop a time-saving multiplex polymerase chain reaction (PCR) for simultaneously detecting and discriminating between large and small forms without sequence analysis. A new multiplex PCR was designed and tested using blood samples from 79 dogs showing clinical signs compatible with babesiosis which were previously analysed using blood smears and molecular methods. Multiplex PCR successfully discriminated between both Babesia groups showing bands of 700 and 890 bp for B. canis/B. vogeli and B. vulpes, respectively. No significant differences in the results of both PCR were detected and a substantial agreement between protocols (κ = 0.64) was found. Our multiplex PCR represents a reliable tool for detecting infections by the major Babesia spp. in dogs from Europe. Since no sequence analysis is required for identifying the species involved, this PCR allows the rapid administration of an appropriate treatment, thus improving the survival rate of the infected animals. In addition, it will represent a helpful tool for unravelling the real prevalence and distribution of B. vulpes and its implication in clinical cases., Competing Interests: Declaration of Competing Interest The authors declared no potential conflicts of interest with respect to the research, authorship, and/or publication of this article., (Copyright © 2023 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2023

34. Multiplex PCR for rapid differential diagnosis of co-prevalent species of Theileria (Theileria annulata and Theileria orientalis) in cattle.

Author

Marwaha S, Brar B, Jain VK, Poonia R, and Prasad M

Subjects

Cattle, Animals, Multiplex Polymerase Chain Reaction veterinary, Diagnosis, Differential, DNA, Protozoan genetics, Theileria genetics, Theileria annulata genetics, Theileriasis diagnosis, Theileriasis epidemiology, Theileriasis parasitology, Cattle Diseases diagnosis, Cattle Diseases parasitology

Abstract

Theileriosis is a tick-borne disease that causes enormous losses in the dairy industry. There are several species of Theileria that can infect bovines. Generally, more than one species are prevalent in any geographical area; thus, chances of co-infections are high. Differentiation of these species may not be possible by microscopic examination or serological tests. Therefore, in this study, a multiplex PCR assay was standardized and evaluated for rapid and simultaneous differential detection of two species of Theileria viz., Theileria annulata and Theileria orientalis. Species-specific primers were designed to target the merozoite piroplasm surface antigen gene (TAMS1) of T. annulata and the major piroplasm surface protein gene of T. orientalis, yielding specific amplicon of 229 bp and 466 bp, respectively. The sensitivity of multiplex PCR was 10 2 and 10 3 copies for T. annulata and T. orientalis, respectively. The simplex and multiplex PCRs were specific and showed no cross-reactivity with other hemoprotozoa for either primer. For comparative evaluation, blood samples from 216 cattle were tested by simplex and multiplex PCR for both species. Using multiplex PCR, 131 animals were found infected for theileriosis, of which 112 were infected with T. annulata, five were infected with T. orientalis, and 14 had mixed infections. This is the first report of T. orientalis from Haryana, India. Representative sequences of T. annulata (ON248941) and T. orientalis (ON248942) were submitted in GenBank. The standardized multiplex PCR assay used in this study was specific, sensitive, for the screening of field samples., (© 2023. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2023

35. Isolation, identification, molecular typing, and drug resistance of Escherichia coli from infected cattle and sheep in Xinjiang, China.

Author

Gu X, Ma X, Wu Q, Tao Q, Chai Y, Zhou X, Han M, Li J, Huang X, Wu T, Zhang X, Zhong F, Cao Y, and Zhang L

Subjects

Animals, Cattle, Sheep, Escherichia coli, Phylogeny, RNA, Ribosomal, 16S, China epidemiology, Multiplex Polymerase Chain Reaction veterinary, Molecular Typing veterinary, Drug Resistance, Escherichia coli Infections epidemiology, Escherichia coli Infections veterinary, Escherichia coli Infections microbiology, Cattle Diseases epidemiology, Cattle Diseases microbiology, Sheep Diseases epidemiology

Abstract

Background: Escherichia coli infections are common in Xinjiang, a major region of cattle and sheep breeding in China. Therefore, strategies are required to control E. coli. The aim of this study was to investigate the phylogenetic groups, virulence genes, and antibiotic resistance characteristics of E. coli isolates., Methods: In this study, 116 tissue samples were collected from the organs of cattle and sheep that were suspected of having E. coli infections between 2015 and 2019. Bacteria in the samples were identified using a biochemical identification system and amplification of 16S rRNA, and the phylogenetic groupings of E. coli isolates were determined by multiplex polymerase chain reactions. In addition, PCR detection and analysis of virulence factors, antibiotic resistance genes, and drug-resistant phenotypes of E. coli isolates were performed., Results: A total of 116 pathogenic E. coli strains belonging to seven phylogenetic groups were isolated, with the majority of isolates in groups A and B1. Among the virulence genes, curli-encoding crl had the highest detection rate of 97.4%, followed by hemolysin-encoding hlyE with the detection rate of 94.82%. Antimicrobial susceptibility test results indicated that the isolates had the highest rates of resistance against streptomycin (81.9%)., Conclusion: These characteristics complicate the prevention and treatment of E. coli-related diseases in Xinjiang., (© 2023 The Authors. Veterinary Medicine and Science published by John Wiley & Sons Ltd.)

Published

2023

36. Simultaneous detection of three important viruses affecting tilapia using a multiplex PCR assay.

Author

Prasartset T and Surachetpong W

Subjects

Animals, Multiplex Polymerase Chain Reaction veterinary, Sensitivity and Specificity, Tilapia, Fish Diseases diagnosis, Viruses

Published

2023

37. Comparison of multiplex copro PCR with coproscopy followed by PCR on recovered eggs for the detection of Echinococcus granulosus and Taenia spp. infection in dogs.

Author

Yasur-Landau D, Genad O, Salant H, Dvir E, Mazuz ML, and Baneth G

Subjects

Animals, Dogs, DNA, Echinococcus granulosus genetics, Feces parasitology, Multiplex Polymerase Chain Reaction veterinary, Ovum, Taenia genetics, Dog Diseases diagnosis, Dog Diseases parasitology, Taeniasis diagnosis, Taeniasis veterinary, Echinococcosis diagnosis, Echinococcosis veterinary

Abstract

Echinococcosis and taeniasis are important helminth diseases that carry considerable impact on human and animal health. Domestic dogs and other canids are definitive hosts for several parasites of this group, including Echinococcus granulosus, Taenia multiceps, T. ovis, T. hydatigena and E. multilocularis. Detection of infection in dog populations is imperative for estimating the risk to susceptible humans and animals, and for its mitigation through prevention measures in dogs, other animals and humans. To date, identification of taeniid eggs, antigens or DNA in fecal samples are the most practical diagnostic modalities available for canine definitive hosts. Although widely used for this purpose, there is limited information comparing copro PCR and combined coproscopy-PCR protocols for the detection of taeniids. In the current study, a widely used multiplex PCR was performed on a large number of dog fecal samples using DNA extracted directly from feces. The samples were also tested by fecal flotation and coproscopy, eggs were isolated from microscopically-positive samples and extracted DNA was tested using the same multiplex PCR. The total number of taeniid positive samples detected using both methods was 46/317 (14.5%), including 10/317 (3.2%) E. granulosus positive samples. Both copro PCR and coproscopy have identified an equal number of samples as taeniid positive (n = 32). However, for the purpose of identification to species level, the copro PCR was significantly more sensitive than coproscopy followed by PCR on isolated eggs (sensitivity 0.7 vs. 0.41, p = 0.012), with 32/317 (10.1%) and 19/317 (6%) positive samples identified, respectively. The difference in identification of E. granulosus was highly apparent, as the majority of the E. granulosus positive samples (8/10) were detected by the copro PCR only. Coproscopy and egg PCR have identified 5/317 (1.6%) positive samples not detected by the copro PCR, including only a single sample (0.3%) positive for E. granulosus. Adding these positive samples to those identified by the copro PCR did not significantly improve the overall sensitivity (p = 0.074). Therefore, using both copro PCR and coproscopy in parallel may not be advantageous for taeniid detection and identification, at least until the egg PCR is further optimized and performs better. These results should be weighed against the different advantages that coproscopy based approach may offer., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2023 Elsevier B.V. All rights reserved.)

Published

2023

38. Multiplex gel-based PCR assay for the simultaneous detection of 5 genotypes of porcine astroviruses.

Author

Zhang Q, Liu Q, Opriessnig T, Wen D, Gu K, and Jiang Y

Subjects

Animals, Swine, Multiplex Polymerase Chain Reaction veterinary, Genotype, Sensitivity and Specificity, Astroviridae Infections diagnosis, Astroviridae Infections epidemiology, Astroviridae Infections veterinary, Swine Diseases diagnosis, Swine Diseases epidemiology

Abstract

Porcine astrovirus (PAstV) has been associated experimentally with diarrhea in piglets, but much more knowledge is needed about this virus. PAstV has high genetic variability, and 5 genotypes have been identified, namely PAstV1-5. To obtain information on the epidemiology of PAstV, we established a multiplex PAstV PCR assay to detect and differentiate the 5 PAstV genotypes simultaneously. The assay utilized specific primers for each genotype, producing fragments of 307, 353, 205, 253, and 467 bp, representing PAstV1-5, respectively. Our multiplex PCR assay amplified all 5 DNA fragments from single or mixed viral genomes without cross-reactions with other PAstV genotypes or other viruses in pigs. The limit of detection of the multiplex PCR assay was 5 × 10 2 copies/μL for PAstV1 and PAstV4, and 5 × 10 3 copies/μL for PAstV2, PAstV3, and PAstV5. We examined 76 pig fecal specimens with our multiplex PCR assay. PAstV was detected in 36 of 76 (47.4%) samples; ≥2 PAstVs were found in 20 of 76 (26.3%) samples. The multiplex PCR assay results were essentially the same as the results using a monoplex PAstV PCR assay, with a coincidence rate of >96%. Our multiplex PCR method provides a simple, sensitive, and specific detection tool for PAstV detection and epidemiologic surveys.

Published

2023

39. Application of a Multiplex PCR Assay for Molecular Identification of Pathogenic and Non-Pathogenic Leptospires based on lipL32 and 16S rRNA Genes.

Author

Khaki P, Rahimi Zarchi F, Moradi Bidhendi S, and Gharakhani M

Subjects

Animals, Multiplex Polymerase Chain Reaction veterinary, RNA, Ribosomal, 16S genetics, Genes, rRNA, Leptospira genetics, Leptospirosis diagnosis, Leptospirosis veterinary

Abstract

Leptospirosis is a serious zoonotic infection and the most prevalence disease is in the tropical and subtropical region. The definitive diagnosis of Leptospirosis, caused by spirochetes of the genus Leptospira infection is already using culture methods, serological tests such as the microscopic agglutination test (MAT) and molecular detection methods (PCR) are possible. In this study, we used multiplex PCR method for detection of pathogenic and non - pathogenic Leptospira based on lipL32 and 16S rRNA genes. All serovars were obtained from the Leptospira Reference Laboratory of Microbiology Department, Razi Vaccine and Serum Research Institute, Karaj, Iran. The PCR product for the lipL32 and 16S rRNA genes was 272 bp and 240 bp respectively. The sensitivity amplification for the multiplex assay was 10 -6 pg / μl for 16S rRNA gene and 10 -4 pg / μl for lipL32 gene. The sensitivity for multiplex PCR was 10 -3 pg / μl. The results supported the idea that multiplex PCR can be used to detect Leptospira samples. This method was also able to differentiate between saprophytic and pathogenic leptospires and was able to do so much easily than conventional methodologies. Due to the slow growth of Leptospira and the importance of time in diagnosis, molecular methods such as PCR are suggested., Competing Interests: The authors declare that they have no conflict of interest.

Published

2023

40. Identification of staphylococcal cassette chromosome mec in Staphylococcus aureus and non-aureus staphylococci from dairy cattle in Belgium: Comparison of multiplex PCR and whole genome sequencing.

Author

Tchamba CN, Touzain F, Fergestad M, De Visscher A, L'Abee-Lund T, De Vliegher S, Wasteson Y, Blanchard Y, Argudín MA, Mainil J, and Thiry D

Subjects

Animals, Cattle, Anti-Bacterial Agents pharmacology, Bacterial Proteins genetics, Belgium, Cefoxitin pharmacology, Chromosomes, Microbial Sensitivity Tests veterinary, Multiplex Polymerase Chain Reaction veterinary, Staphylococcus genetics, Staphylococcus aureus genetics, Whole Genome Sequencing veterinary, Cattle Diseases epidemiology, Cattle Diseases microbiology, Methicillin-Resistant Staphylococcus aureus, Staphylococcal Infections epidemiology, Staphylococcal Infections veterinary

Abstract

The present study compared multiplex PCR (mPCR) and Whole Genome Sequencing (WGS) using the SCCmecFinder database to identify the Staphylococcal Cassette Chromosome (SCC) mec in five Staphylococcus aureus (SA) and nine non-aureus staphylococci (NAS) isolated from dairy cattle. mPCR identified an SCCmecIV in four SA and one NAS, but could not differentiate between SCCmecII and IV in the fifth SA, that all harbored the mecA gene and were phenotypically resistant to cefoxitin. SCCmecFinder confirmed the presence of an SCCmecIVc(2B) in four SA and of the SCCmecIVa(2B) in the fifth SA and the one NAS. Both methods also detected one untypeable SCCmec in another cefoxitin-resistant NAS harboring the mecA gene and a pseudo SCCmec in one cefoxitin-sensitive NAS harboring one mecC-related gene. No SCCmec elements were identified either in one cefoxitin-sensitive NAS harboring the mecA2 gene, or in five NAS (one resistant and four sensitive to cefoxitin) harboring the mecA1 gene. SCCmecFinder could even not identify the presence of any mecA1 gene in these five NAS, whose presence was nevertheless confirmed by ResFinder. The conclusions of this study are: (i) mPCR and WGS sequencing using SCCmecFinder are complementary methodologies to identify SCCmec; (ii) SCCmecFinder and ResFinder to a lesser extent cannot identify all mec gene allotypes; (iii) a specific classification of the SCCmec in NAS would be epidemiologically helpful; (iv) presence of a mecA gene and a complete SCCmec is linked to cefoxitin resistance, whereas presence of other mec genes and of pseudo or no SCCmec is not., Competing Interests: Declaration of Competing Interest The authors declare no conflict of interest., (Copyright © 2023 Elsevier Ltd. All rights reserved.)

Published

2023

41. Simultaneous detection and differentiation of three oncogenic viral diseases of chicken by use of multiplex PCR.

Author

Kannaki TR, Edigi P, Yalagandula N, and Haunshi S

Subjects

Animals, Chickens genetics, Multiplex Polymerase Chain Reaction veterinary, Multiplex Polymerase Chain Reaction methods, Oncogenic Viruses genetics, Marek Disease diagnosis, Marek Disease pathology, Neoplasms, Poultry Diseases diagnosis, Poultry Diseases pathology

Abstract

Avian oncogenic or tumor diseases are common in poultry industry causing significant economic loss. Marek's disease (MD), avian leukosis (AL) and Reticuloendotheliosis (RE) are the three major viral oncogenic infections that are difficult to differentiate with gross lesions. Multiplex PCR for simultaneous detection and differentiation of these three viruses was developed and validated. The primers targeting the genes of pp38 , pol and LTR for MDV, ALV and REV were designed to yield 206, 429, and 128 bp, respectively. The sensitivity of the PCR primers was checked with serial dilution of positive template DNA for each virus and found to be in the range of 10 -5 to 10 -7 of 1 µg/µl of initial template DNA. Out of 114 suspected tumor samples screened, 8 samples were positive for MDV, 13 samples were positive for ALV and 31 samples positive for REV. Five samples were positive for both MD and ALV; 3 samples were positive for MD and REV and 25 samples were positive for ALV and REV. Eight samples were positive for all three viruses. Multiplex PCR demonstrated to be a useful technique for simultaneous, rapid detection and differentiation of major tumor causing and immunosuppressive viral diseases of chicken.

Published

2022

42. Prevalence of three Mycoplasma sp. by multiplex PCR in cattle with and without respiratory disease in central Mexico.

Author

Maya-Rodríguez LM, Carrillo-Casas EM, Rojas-Trejo V, Trigo-Tavera F, and Miranda-Morales RE

Subjects

Cattle, Animals, Multiplex Polymerase Chain Reaction veterinary, Prevalence, Mexico epidemiology, Respiration Disorders veterinary, Respiratory Tract Diseases veterinary, Mycoplasma bovis genetics, Cattle Diseases diagnosis, Cattle Diseases epidemiology

Abstract

This study aimed to identify Mycoplasma bovis, Myc. dispar, and Myc. bovirhinis, which are involved in bovine respiratory disease through a multiplex PCR as an alternative to culture's features that hamper Mycoplasma isolation. Nasal swabs were taken from 335 cattle with and without respiratory disease background (RDB) from dairy herds in the central region of Mexico. Each sample was divided in two; the first part was processed for the direct DNA extraction of the nasal swab and the second for Mycoplasma isolation, culture, and then the multiplex PCR was performed. In the nasal swabs, Myc. bovis was identified in 21.1%; Myc. dispar, in 11.8%; and Myc. bovirhinis, in 10.8% in cattle with RDB. Isolates were identified as Myc. bovis, 20.1%; Myc. dispar, 11.8%; and Myc. bovirhinis, 6.1%. There is a strong correlation between the presence of Mycoplasma identified by PCR and the clinical history of the disease (ρ < 0.0000). In animals without RDB, Myc. bovirhinis was the only species detected in 6.1% of the samples processed directly for multiplex PCR, and in 2% of the isolates. There is an excellent correlation (kappa 0.803) between the isolation and the 16S PCR and a high correlation (kappa 0.75) between the isolation and the multiplex PCR. Therefore, we conclude that the PCR multiplex test is highly sensitive and may be used for the diagnosis and surveillance of the three species in biological samples and mycoplasma isolates., (© 2022. The Author(s), under exclusive licence to Springer Nature B.V.)

Published

2022

43. Single-tube Multiplex Nested PCR System for Efficient Detection of Pathogenic Microorganisms in SPF Rodents.

Author

Xu WJ, Pan YJ, Li WJ, Peng LN, Liang DL, Zhang M, Ding W, and Wang ZX

Subjects

Animals, DNA Primers genetics, DNA, Bacterial genetics, DNA, Ribosomal genetics, Sensitivity and Specificity, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Rodentia

Abstract

PCR testing is increasingly important for microbial control in SPF facilities. However, most current PCR methods are timeconsuming and require compromise between high sensitivity and high multiplexing. We developed a one-tube multiplex nested PCR strategy (MN-PCR) for simultaneous direct (that is, without culturing) detection of multiple pathogens. We first aligned sequences for the 16S rDNA genes of selected target bacteria and a panel of closely related organisms. From these data, we designed a pair of universal primers and multiple sets of species-specific PCR primers to amplify the target sequences; the universal primers were modified to include various degenerate bases and locked nucleic acids. In a single tube, 16S rDNA sequences were amplified by using the nested PCR primers under high temperature (that is, above 65°C) during the first stage of the MN-PCR procedure, when the target-species-specific PCR primers do not support amplification due to their short length. In addition, the concentration of the nested PCR primers during the first stage was adjusted to ensure that they were consumed and did not yield visible bands themselves. During the second stage, the enriched 16S rDNA sequences then served as templates for amplification of the species-specific fragments by using the multiple PCR primers at low annealing temperatures (that is, below 60°C). The results showed that our MN-PCR method detected as little as 1 fg of target bacterial DNA in a 20-μL reaction volume, whereas conventional multiplex PCR detected a minimum of 1 pg only. Compared with traditional multiplex PCR assays, our MN-PCR system is an effective and efficient culture-free process.

Published

2022

44. Genomic characterization of Tenacibaculum maritimum O-antigen gene cluster and development of a multiplex PCR-based serotyping scheme.

Author

Lopez P, Bridel S, Saulnier D, David R, Magariños B, Torres BS, Bernardet JF, and Duchaud E

Subjects

Animals, Fishes microbiology, Genome-Wide Association Study veterinary, Genomics, Multigene Family, Multiplex Polymerase Chain Reaction veterinary, O Antigens genetics, Serotyping methods, Serotyping veterinary, Fish Diseases diagnosis, Fish Diseases epidemiology, Flavobacteriaceae Infections microbiology, Flavobacteriaceae Infections veterinary, Tenacibaculum genetics

Abstract

Tenacibaculum maritimum is a devastating bacterial pathogen affecting a large variety of marine fish species. It is responsible for significant economic losses in aquaculture farms worldwide. Different typing methods have been proposed to analyse bacterial diversity and population structure. Serological heterogeneity has been observed and up to four different serotypes have been described so far. However, the underlying molecular factors remain unknown. By combining conventional serotyping and genome-wide association study, we identified the genomic loci likely involved in the O-antigen biosynthesis. This finding allowed the development of a robust multiplex PCR-based serotyping scheme able to detect subgroups within each serotype and therefore performs better than conventional serotyping. This scheme was successfully applied to a large number of isolates from worldwide origin and retrieved from a large variety of fish species. No obvious correlations were observed between the mPCR-based serotype and the host species or the geographic origin of the isolates. Strikingly, the distribution of mPCR-based serotypes does not follow the core genome phylogeny. Nevertheless, this simple and cost-effective mPCR-based serotyping method could be useful for different applications such as population structure analysis, disease surveillance, vaccine formulation and efficacy follow-up., (© 2022 The Authors. Transboundary and Emerging Diseases published by Wiley-VCH GmbH.)

Published

2022

45. Multiplex PCR assay based on the citE2 gene and intergenic sequence for the rapid detection of Salmonella Pullorum in chickens.

Author

Liu Z, Yu Y, Fotina T, Petrov R, Klishchova Z, Fotin A, and Ma J

Subjects

Animals, Chickens genetics, DNA, Intergenic, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Salmonella, Salmonella enteritidis genetics, Sensitivity and Specificity, Salmonella Infections, Animal diagnosis, Salmonella Infections, Animal genetics, Salmonella enterica genetics

Abstract

Salmonella is one of the most common Gram-negative pathogens and seriously threatens chicken farms and food safety. This study aimed to establish a multiplex polymerase chain reaction (PCR) approach for the identification of different Salmonella enterica subsp. enterica. The citE2 gene and interval sequence of SPS4&#95;00301-SPS4&#95;00311 existed in all S. enterica subsp. enterica serovars by genomic comparison. By contrast, a 76 bp deletion in citE2 was found only in Salmonella Pullorum. Two pairs of special primers designed from citE2 and interval sequence were used to establish the multiplex PCR system. The optimized multiplex PCR system could distinguish Salmonella Pullorum and non-Salmonella Pullorum. The sensitivity of the optimized multiplex PCR system could be as low as 6.25 pg/μL and 10 4 colony-forming units (CFU)/mL for genomic DNA and Salmonella Pullorum cells, respectively. The developed multiplex PCR assay distinguished Salmonella Pullorum from 33 different Salmonella enterica subsp. enterica serotypes and 13 non-target species. The detection of egg samples artificially contaminated with Salmonella Pullorum, Salmonella Enteritidis, and naturally contaminated 69 anal swab samples showed that results were consistent with the culture method. These features indicated that the developed multiplex PCR system had high sensitivity and specificity and could be used for the accurate detection of Salmonella Pullorum in clinical samples., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

46. Genotyping, antibiotic resistance and prevalence of Arcobacter species in milk and dairy products.

Author

Lameei A, Rahimi E, Shakerian A, and Momtaz H

Subjects

Animals, Anti-Bacterial Agents pharmacology, Drug Resistance, Microbial, Genotype, Humans, Milk, Multiplex Polymerase Chain Reaction veterinary, Prevalence, RNA, Ribosomal, 16S, Virulence Factors genetics, Arcobacter genetics

Abstract

Background: Arcobacter spp. has been considered an emerging foodborne pathogen and a hazard to human health. The dairy chain has been isolated from different sources; nevertheless, data on Arcobacter occurrence in raw milk and dairy products in Iran are still scant., Objective: The present study investigates the prevalence, antimicrobial susceptibility and the presence of virulence genes of Arcobacters species isolated from milk and dairy products., Methods: Then, a total of 350 raw milk samples and 400 dairy product samples were collected from dairy supply centers in Isfahan, Iran. Presumptive Arcobacter strains were obtained by enriching samples in Oxoid Arcobacter enrichment broth (AEB) followed by the filtration of enrichment product through 0.45-μm pore size membrane filters laid onto non-selective blood at 30°C under microaerophilic conditions. Molecular identification of Arcobacter cryaerophilus and A. butzleri was performed by Polymerase chain reaction (PCR) amplification of the 16S rRNA gene, followed by sequencing. The disc diffusion method was used to determine the antimicrobial susceptibility of isolates. Targeted resistance and virulence genes were detected using multiplex PCR., Results: The results show a low recovery rate of Arcobacter spp. in milk. Arcobacters were found in all types of milk, except raw camel milk, but were absent from all dairy products. Arcobacter butzleri was the predominant species in raw milk. Detection of virulence genes shows that all virulence genes targeted were found among A. butzleri, and six (cadF, cj1349, irgA, mviN, pldA, tlyA) were found among A. cryaerophilus. All A. butzleri strains and some A. cryaerophilus strains isolated from milk were resistant to amoxicillin-clavulanic acid and tetracycline. All A. cryaerophilus isolates from milk were susceptible to gentamycin, streptomycin, erythromycin and ciprofloxacin. The distribution of resistance genes in Arcobacter strains in milk shows that all isolates carried tet(O) and bla OXA-61 genes., Conclusions: In conclusion, the results indicate a low recovery rate of Arcobacter spp. in milk and milk products. However, a significant number of Arcobacter strains with putative virulence genes may be potential pathogens for humans and an overall increase in Arcobacter resistance to first-line antibiotics. These results highlight the need for regular surveillance of Arcobacter strains in milk and milk products in Iran., (© 2022 The Authors. Veterinary Medicine and Science published by John Wiley & Sons Ltd.)

Published

2022

47. Isolation and molecular confirmation of Brucella suis biovar 2 from slaughtered pigs: an unanticipated biovar from domestic pigs in Egypt.

Author

Elmonir W, Abdel-Hamid NH, Hamdy MER, Beleta EIM, El-Diasty M, Melzer F, Wareth G, and Neubauer H

Subjects

Animals, Egypt epidemiology, Female, Male, Multiplex Polymerase Chain Reaction veterinary, Sus scrofa genetics, Swine, Brucella suis genetics, Brucellosis epidemiology, Brucellosis veterinary, Swine Diseases epidemiology

Abstract

Background: Brucella suis is a zoonotic pathogen with a serious impact on public health and the pig industry worldwide. Information regarding B. suis in pigs in Egypt is scarce. This study aimed to investigate the prevalence of B. suis in slaughtered domestic pigs at El-Basatin abattoir in Cairo, Egypt. A total of 1,116 domestic pigs slaughtered in 2020 were sampled for Brucella isolation and identification. Identified Brucella isolates were molecularly confirmed at species, and biovar levels using Bruce ladder PCR and Suis ladder multiplex PCR. Additionally, high-risk practices of 16 abattoir workers (4 veterinarians, 10 butchering and evisceration workers, and 2 scalding workers) were investigated using a pre-piloted structured questionnaire., Results: Brucella isolates were recovered from 1.3% of examined pigs (n = 14) at consistently low rates (1.1-2.9%) across the year of sampling from February to December 2020. All isolates were confirmed as B. suis biovar (bv) 2. Remarkably, 92.9% (13/14) of isolates showed atypical ability to produce H 2 S and hence were considered as B. suis bv2 atypical phenotype. The prevalence was higher in males (1.8%) than in females (0.9). However, this difference was not significant (Odds ratio = 1.9; CI 95% 0.7 - 5.7; P = 0.2). No detectable pathological lesions were associated with B. suis bv2 infection in examined pigs. All strains were isolated from cervical lymph nodes, highlighting a potential oral transmission. High-risk practices were recorded among swine abattoir workers in this study: 75% do not wear gloves or disinfect their knives daily, and 18.8% were willing to work with open wound injuries., Conclusions: To the best of our knowledge, this is the first isolation of B. suis bv2 in Egypt. Detection of H 2 S producing B. suis bv2 atypical phenotype is alarming as it may result in misinterpretation of these isolates as highly human pathogenic B. suis bv1 in Egypt and possibly elsewhere. Further epidemiological tracing studies are crucial for the detection of the origin of this biovar. Including pigs in the national surveillance program of brucellosis, and an education program for swine abattoir workers about occupational risk of B. suis is a need in Egypt., (© 2022. The Author(s).)

Published

2022

48. Development and validation of multiplex SYBR Green real-time PCR assays for detection and molecular surveillance of four tick-borne canine haemoparasites.

Author

Padmaja M, Singh H, Panwar H, Jyoti, Singh NK, and Singh NK

Subjects

Animals, Benzothiazoles, Diamines, Dogs, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Quinolines, Real-Time Polymerase Chain Reaction veterinary, Dog Diseases diagnosis, Dog Diseases epidemiology, Dog Diseases parasitology, Ticks

Abstract

Two multiplex SYBR Green based real-time PCR assays were standardized and evaluated to detect DNA from four canine haemoparasites (Babesia gibsoni, Babesia vogeli, Ehrlichia canis and Hepatozoon canis), along with internal controls from dogs from selected districts of Punjab state, India. Amplicons of 126 bp, 337 bp, 234 bp and 106 bp corresponding to B. gibsoni (18S rRNA gene), B. vogeli (18S rRNA gene), E. canis (virB9 gene), and H. canis (18S rRNA gene) were obtained, without any non-specific amplification. Microscopic evaluation of 200 blood samples from dogs revealed the prevalence of B. gibsoni, E. canis and H. canis as 1.5%, 1.5% and 1.0%, respectively, while with the multiplex real-time PCR assays the values for B. gibsoni, B. vogeli, E. canis, and H. canis were 8.0%, 1.5%, 3.5% and 23.5%, respectively, with concurrent infections of B. gibsoni and H. canis (3.5%); E. canis and H. canis (2.0%) and B. gibsoni, B. vogeli, E. canis, and H. canis (0.5%). The diagnostic sensitivity of the multiplex real-time PCR assays with respect to microscopy in the detection of B. gibsoni, E. canis and H. canis was 100% while the specificity for B. gibsoni, B. vogeli, E. canis, and H. canis was 93%, 100%, 98% and 77%, respectively, revealing the respective strength of agreement as ″fair″, ″slight″, ″moderate″ and ″slight″ by kappa value statistics, and the data were statistically significant, for detection of B. gibsoni and E. canis infections, by Fisher's exact test. The analytical sensitivity of the multiplex PCR assays in detection of DNAs was 8.59 × 10 5 and 9.9 × 10 6 copies for B. vogeli and E. canis, respectively, and 1.15 × 10 6 and 3.41 × 10 5 copies for B. gibsoni and H. canis, respectively. Assessment of risk factors viz. age, sex, breed, season and locations showed no significant association with the prevalence of these haemoparasites except for B. vogeli, E. canis and H. canis where significant associations were found for location, age and breed, respectively by multiplex real-time PCR assays., (Copyright © 2022. Published by Elsevier GmbH.)

Published

2022

49. Multiplex polymerase chain reaction for the detection and differentiation of 4 porcine circovirus 2 genotypes (PCV-2a, -2b, -2d, and -2e) in clinical samples.

Author

Park KH, Cho H, Oh T, Yang S, and Chae C

Subjects

Animals, DNA, Viral genetics, Genotype, Multiplex Polymerase Chain Reaction veterinary, Swine, Circoviridae Infections diagnosis, Circoviridae Infections veterinary, Circovirus genetics, Swine Diseases

Abstract

The objective of this study was to develop multiplex polymerase chain reaction (PCR) for the simultaneous detection of porcine circovirus 2 (PCV-2) and differentiation among 4 PCV-2 genotypes (2a, 2b, 2d, and 2e) in collected clinical lymph node samples. The multiplex PCR detected each of 4 PCV-2 genotypes (2a, 2b, 2d, and 2e) to a dilution of 2 × 10 1 copies/μL. PCV-2a, PCV-2b, PCV-2d, and PCV-2e were propagated in tissues prior to DNA extraction for use in multiplex PCR for the simultaneous detection and differentiation of 4 PCV-2 genotypes. The designed multiplex PCR effectively detected and differentiated various combinations of multiple infection, such as PCV-2a+2b, PCV-2a+2d, PCV-2b+2d, PCV-2a+2e, and PCV-2a+2b+2d, in clinical lymph node samples. The results of this study demonstrated that multiplex PCR testing of clinical samples developed herein was able to simultaneously detect and differentiate among the 4 PCV-2 genotypes (PCV-2a, 2b, 2d, and 2e)., (Copyright and/or publishing rights held by the Canadian Veterinary Medical Association.)

Published

2022

50. Detection and differentiation of Salmonella Enteritidis and Salmonella Typhimurium by multiplex quantitative PCR from different poultry matrices.

Author

Müştak IB and Müştak HK

Subjects

Animals, Chickens genetics, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Poultry genetics, Salmonella enteritidis genetics, Salmonella typhimurium genetics

Abstract

1. The aim of this study was to develop a multiplex quantitative polymerase chain reaction (qPCR) based molecular diagnostic kit for rapid diagnosis of Salmonella enterica serovar Enteritidis and S. enterica serovar Typhimurium serotypes, which are frequently isolated worldwide from poultry samples.2. Detection and discrimination of S. Enteritidis and S. Typhimurium were performed by targeting the sdf and the STM4492 (putative cytoplasmic protein) gene, respectively. The invA (invasion protein) gene was used to detect Salmonella spp. as a target gene, since it is considered a standard. In this study, a total of 200 bacterial strains (178 Salmonella spp . strains and 22 other genera) were used to test the specificity and sensitivity of the developed kit. The limit of detection (LOD) of the assays was determined to be 10 0 -10 1  cfu/25 g from chicken meat samples artificially contaminated by litter and 10 0 -10 1  cfu/ml for cloacal swab samples.3. The multiplex qPCR results were 100% compatible with conventional serotyping results while the specificity and sensitivity values were 100%. These findings indicated that the newly developed multiplex qPCR technique can provide an alternative method to conventional serotyping of S. Enteritidis and S. Typhimurium in laboratories lacking adequate infrastructure.

Published

2022