Descriptor: "Clinical Veterinary Microbiology" - Searchworks@Jio Institute Digital Library Search Results

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723 results on '"Clinical Veterinary Microbiology"'

1. Proposal of a Method for Harmonized Broth Microdilution Antimicrobial Susceptibility Testing of Avibacterium gallinarum

Author: Franziska Gütgemann, Anja Müller, Yury Churin, Arne Jung, Franziska Kumm, Annet Heuvelink, Min Yue, and Corinna Kehrenberg
Subjects: Microbiology (medical), Anti-Infective Agents, Humans, Reproducibility of Results, Microbial Sensitivity Tests, Pasteurellaceae, Clinical Veterinary Microbiology, Anti-Bacterial Agents
Abstract: Avibacterium (Av.) gallinarum is an opportunistic pathogen in poultry, which, however, has also been associated with human disease. There is currently no approved method for antimicrobial susceptibility testing of this pathogen, so this study aimed at developing a harmonized broth microdilution method for Av. gallinarum that is suitable for diagnostic laboratories. For this, the Av. gallinarum CCUG 12391(T) type strain and 42 field isolates were collected and their species was confirmed by using a species-specific PCR assay and biochemical reactions. To select epidemiologically unrelated isolates, ApaI macrorestriction analysis was performed. Preliminary growth experiments were conducted with six culture media, and based on the results, four media were selected to compile growth curves with four isolates. Independent repetitions of MIC determinations were then performed to evaluate the reproducibility of the values. Cation-adjusted Mueller-Hinton broth (CAMHB) was initially selected as broth medium, but did not show sufficient homogeneity of MICs. Therefore, CAMHB plus 1% chicken serum and 0.0025% NADH was selected and showed a good homogeneity of MICs after 20 h and 24 h of incubation at 35 ± 2°C. This was reflected in essential MIC agreements ranging between 96% and 100%. Testing of a larger Av. gallinarum collection (n = 43) revealed that easily readable MICs could be obtained for the type strain and all isolates. Some Av. gallinarum showed elevated MICs of enrofloxacin (n = 35), nalidixic acid (n = 35), penicillin (n = 2), tetracycline (n = 19), and/or trimethoprim-sulfamethoxazole (n = 1). By using PCR analyses, the following antimicrobial resistance genes were detected: bla(TEM), dfrA14, sul2, tet(B), tet(H). The study demonstrated that the proposed medium is suitable for a harmonized broth microdilution susceptibility testing of Av. gallinarum with a recommended incubation time of 20 to 24 h.
Published: 2022

2. Development and Validation of a Competitive ELISA Based on Bovine Monoclonal Antibodies for the Detection of Neutralizing Antibodies against Foot-and-Mouth Disease Virus Serotype A

Author: Yimei Cao, Kun Li, Xiangchuan Xing, Guoqiang Zhu, Yuanfang Fu, Huifang Bao, Xingwen Bai, Pu Sun, Pinghua Li, Jing Zhang, Xueqing Ma, Jian Wang, Zhixun Zhao, Dong Li, Zaixin Liu, and Zengjun Lu
Subjects: Microbiology (medical), Foot-and-Mouth Disease Virus, Foot-and-Mouth Disease, viruses, Animals, Antibodies, Monoclonal, Humans, Cattle, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, Serogroup, Antibodies, Neutralizing, Clinical Veterinary Microbiology
Abstract: The level of neutralizing antibodies in vaccinated animals is directly related to their level of protection against a virus challenge. The virus neutralization test (VNT) is a “gold standard” method for detecting neutralizing antibodies against foot-and-mouth disease virus (FMDV). However, VNT requires high-containment facilities that can handle live viruses and is not suitable for large-scale serological surveillance. In this study, a bovine broadly neutralizing monoclonal antibody (W145) against FMDV serotype A was successfully produced using fluorescence-based single-B-cell antibody technology. Using biotinylated W145 as a detector antibody and another bovine cross-reactive monoclonal antibody, E32, which was produced previously as a capture antibody, a competitive enzyme-linked immunosorbent assay for the detection of neutralizing antibodies (NAC-ELISA) against FMDV serotype A was developed. The specificity and sensitivity of the assay were evaluated to be 99.04% and 100%, respectively. A statistically significant correlation (r = 0.9334, P < 0.0001) was observed between the NAC-ELISA titers and the VNT titers, suggesting that the NAC-ELISA could detect neutralizing antibodies against FMDV serotype A and could be used to evaluate protective immunity.
Published: 2022

3. A Survey of Current Activities and Technologies Used to Detect Carbapenem Resistance in Bacteria Isolated from Companion Animals at Veterinary Diagnostic Laboratories-United States, 2020

Author: Michelle A, Waltenburg, Alicia, Shugart, John Dustin, Loy, Deepanker, Tewari, Shuping, Zhang, Stephen D, Cole, Maroya Spalding, Walters, and Megin, Nichols
Subjects: Microbiology (medical), Bacteria, Microbial Sensitivity Tests, Pets, United States, beta-Lactamases, Anti-Bacterial Agents, Clinical Veterinary Microbiology, Anti-Infective Agents, Bacterial Proteins, Carbapenems, Animals, Humans, Laboratories
Abstract: Carbapenems are antimicrobial drugs reserved for the treatment of severe multidrug-resistant Gram-negative bacterial infections. Carbapenem-resistant organisms (CROs) are an urgent public health threat and have been made reportable to public health authorities in many jurisdictions. Recent reports of CROs in companion animals and veterinary settings suggest that CROs are a One Health problem. However, standard practices of U.S. veterinary diagnostic laboratories (VDLs) to detect CROs are unknown. We assessed the capacity of VDLs to characterize carbapenem resistance in isolates from companion animals. Among 74 VDLs surveyed in 42 states, 23 laboratories (31%) from 22 states responded. Most (22/23, 96%) included ≥1 carbapenem on their primary antimicrobial susceptibility testing panel, and approximately one-third (9/23, 39%) performed phenotypic carbapenemase production testing or molecular identification of carbapenemase genes. Overall, 35% (8/23) of VDLs across eight states reported they would notify public health if a CRO was detected. Most (17/21, 81%) VDLs were not aware of CRO reporting mandates, and some expressed uncertainty about whether the scope of known mandates included CROs from veterinary sources. Although nearly all surveyed VDLs tested for carbapenem resistance, fewer had the capacity for mechanism testing or awareness of public health reporting requirements. Addressing these gaps is critical to monitoring CRO incidence and trends in veterinary medicine, preventing spread in veterinary settings, and mounting an effective One Health response. Improved collaboration and communication between public health and veterinary medicine is critical to inform infection control practices in veterinary settings and conduct a public health response when resistant isolates are detected.
Published: 2022

4. Whole-Genome Sequencing Evaluation of MALDI-TOF MS as a Species Identification Tool for Streptococcus suis

Author: Anna, Werinder, Anna, Aspán, Robert, Söderlund, Annette, Backhans, Marie, Sjölund, Bengt, Guss, and Magdalena, Jacobson
Subjects: Streptococcus suis, Whole Genome Sequencing, Swine, RNA, Ribosomal, 16S, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Animals, Serogroup, Clinical Veterinary Microbiology
Abstract: Streptococcus suis is an important bacterial pathogen in pigs that may also cause zoonotic disease in humans. The aim of the study was to evaluate matrix-assisted laser desorption ionization–time of flight mass spectrometry (MALDI-TOF MS) identification of S. suis case isolates from diseased pigs and tonsil isolates from healthy pigs and wild boar using sequence analysis methods. Isolates (n = 348) that had been classified as S. suis by MALDI-TOF MS were whole-genome sequenced and investigated using analyses of (i) the 16S rRNA gene, (ii) the recN gene, and (iii) whole-genome average nucleotide identity (ANI). Analysis of the 16S rRNA gene indicated that 82.8% (288 out of 348) of the isolates were S. suis, while recN gene analysis indicated that 75.6% (263 out of 348) were S. suis. ANI analysis classified 44.3% (154 out of 348) as S. suis. In total, 44% (153 out of 348) of the investigated isolates were classified as S. suis by all of the species identification methods employed. The mean MALDI-TOF MS score was significantly higher for the S. suis case isolates than for the tonsil isolates; however, the difference is of limited practical use. The results show that species confirmation beyond MALDI-TOF MS is needed for S. suis isolates. Since the resolution of 16S rRNA gene analysis is too low for Streptococcus spp., ANI analysis with a slightly lowered cutoff of 94% may be used instead of, or in addition to, recN gene analysis. Supplementation of the MALDI-TOF MS reference library with mass spectra from S. orisratti, S. parasuis, S. ruminantium, and additional S. suis serotypes should be considered in order to produce more accurate classifications.
Published: 2021

5. Analysis of Yersinia pseudotuberculosis Isolates Recovered from Deceased Mammals of a German Zoo Animal Collection

Author: S. Dreyer, C. Heydel, N. vom Ort, Andrea Barac, Jens A. Hammerl, Stefan Hertwig, A. Kuczka, H. Peters, Claudia Jäckel, and L. Grund
Subjects: 0301 basic medicine, Microbiology (medical), Serotype, zoo animals, prophage, animal diseases, 030106 microbiology, Yersinia pseudotuberculosis Infections, Virulence, Yersinia, virulence factor, Clinical Veterinary Microbiology, diversity, Microbiology, 03 medical and health sciences, Plasmid, plasmid, Germany, Pulsed-field gel electrophoresis, Animals, Humans, Yersinia pseudotuberculosis, antimicrobial resistance, genome, Pathogen, Yersinia enterocolitica, Mammals, biology, biology.organism_classification, 030104 developmental biology, Animals, Zoo, Mobile genetic elements
Abstract: Yersinia pseudotuberculosis is an important pathogen for both humans and animals. It can infect livestock, as well as pets and wild animals. During recent years, a number of reports have described the isolation of Y. pseudotuberculosis from zoo animals, mainly birds and mammals, for which the infection was mostly lethal. Between 2005 and 2019, there were at least 17 cases of deceased mammals, belonging to five different species, which suffered from a Y. pseudotuberculosis infection at the Zoo Wuppertal, Germany. Since only scarce information exists on the properties of Y. pseudotuberculosis from zoo animals, we characterized eight isolates, covering all infected species, in detail. All isolates were members of biotype 1, but belonged to five serotypes, five sequence types (STs), and seven core-genome multilocus sequence types (cgMLSTs). Using pulsed-field gel electrophoresis (PFGE) analysis and whole-genome sequencing (WGS), the seven isolates could be discriminated from each other. They differed significantly regarding their virulence genes and mobile genetic elements. While the virulence plasmid pYV existed in all serotypes (five isolates), a complete high-pathogenicity island (HPI) was detected only in the serotypes O:1a, O:1b, and O:13 (four isolates), but not in O:2a and O:2b. Similarly, the content of other plasmids and prophages varied greatly between the isolates. The data demonstrate that the deceased mammals were infected by seven individual isolates and not by a single type predominating in the zoo animals.
Published: 2021

6. Application of Four Genotyping Methods to Mycoplasma bovis Isolates Derived from Western Canadian Feedlot Cattle

Author: Andrea Kinnear, Tim A. McAllister, Rahat Zaheer, Matthew Waldner, Karen B. Register, and Murray D. Jelinski
Subjects: 0301 basic medicine, Microbiology (medical), Mycoplasma bovis, Canada, Genotype, 040301 veterinary sciences, In silico, Biology, medicine.disease_cause, Genome, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, Mycoplasma, medicine, Animals, Clade, Genotyping, Phylogeny, Genetics, Phylogenetic tree, 04 agricultural and veterinary sciences, beef, feedlot, 030104 developmental biology, genotyping, Multilocus sequence typing, Cattle, Multilocus Sequence Typing
Abstract: Mycoplasma bovis is a significant pathogen of feedlot cattle, responsible for chronic pneumonia and polyarthritis syndrome (CPPS). M. bovis isolates (n = 129) were used to compare four methods of phylogenetic analysis and to determine if the isolates’ genotypes were associated with phenotypes. Metadata included the health status of the animal from which an isolate was derived (healthy, diseased, or dead), anatomical location (nasopharynx, lung, or joint), feedlot, and production year (2006 to 2018). Four in silico phylogenetic typing methods were used: multilocus sequence typing (MLST), core genome MLST (cgMLST), core genome single nucleotide variant (cgSNV) analysis, and whole-genome SNV (wgSNV) analysis. Using Simpson’s diversity index (D) as a proxy for resolution, MLST had the lowest resolution (D = 0.932); cgSNV (D = 0.984) and cgMLST (D = 0.987) generated comparable results; and wgSNV (D = 1.000) provided the highest resolution. Visual inspection of the minimum spanning trees found that the memberships of the clonal complexes and clades had similar structural appearances. Although MLST had the lowest resolution, this methodology was intuitive and easy to apply, and the PubMLST database facilitates the comparison of sequence types across studies. The cg methods had higher resolution than MLST, and the graphical interface software was user-friendly for nonbioinformaticians, but the proprietary software is relatively expensive. The wgSNV approach was the most robust for processing poor-quality sequence data while offering the highest resolution; however, application of its software requires specialized training. None of the four methods could associate genotypes with phenotypes.
Published: 2021

7. Distribution of Novel Og Types in Shiga Toxin-Producing Escherichia coli Isolated from Healthy Cattle

Author: Hiroshi Nakajima, Sunao Iyoda, Tadasuke Ooka, Thi Thu Huong Nguyen, Ritsuko Ohata, Hisahiro Kawai, and Atsushi Iguchi
Subjects: Microbiology (medical), Serotype, Shiga-Toxigenic Escherichia coli, biology, Escherichia coli Proteins, In silico, Locus (genetics), Serogroup, biology.organism_classification, medicine.disease_cause, Clinical Veterinary Microbiology, Microbiology, Feces, Gene cluster, Multiplex polymerase chain reaction, medicine, Animals, Cattle, Shigella, Serotyping, Escherichia coli, Escherichia coli Infections, Shigella boydii
Abstract: Shiga toxin-producing Escherichia coli (STEC) is an important foodborne pathogen. Although most cases of STEC infection in humans are due to O157 and non-O157 serogroups, there are also reports of infection with STEC strains that cannot be serologically classified into any O serogroup (O-serogroup untypeable [OUT]). Recently, it has become clear that even OUT strains can be subclassified based on the diversity of O-antigen biosynthesis gene cluster (O-AGC) sequences. Cattle are thought to be a major reservoir of STEC strains belonging to various serotypes; however, the internal composition of OUT STEC strains in cattle remains unknown. In this study, we screened 366 STEC strains isolated from healthy cattle by using multiplex PCR kits including primers that targeted novel O-AGC types (Og types) found in OUT E. coli and Shigella strains in previous studies. Interestingly, 94 (25.7%) of these strains could be classified into 13 novel Og types. Genomic analysis revealed that the results of the in silico serotyping of novel Og-type strains were perfectly consistent with those of the PCR experiment. In addition, it was revealed that a dual Og8+OgSB17-type strain carried two types of O-AGCs from E. coli O8 and Shigella boydii type 17 tandemly inserted at the locus, with both antigens expressed on the cell surface. The results of this comprehensive analysis of cattle-derived STEC strains may help improve our understanding of the strains circulating in the environment. Additionally, the DNA-based serotyping systems used in this study could be used in future epidemiological studies and risk assessments of other STEC strains.
Published: 2021

8. Development of an Indirect Chemiluminescence Immunoassay Using a Multiepitope Recombinant Protein To Specifically Detect Antibodies against Foot-and-Mouth Disease Virus Serotype O in Swine

Author: Wei Liu, Sudan Ge, Yanyan Chang, Guanglei Zhang, Huiyun Chang, Yue Sun, Zhan Gao, and Shao Junjun
Subjects: 0301 basic medicine, Microbiology (medical), Serotype, Luminescence, Swine, 030106 microbiology, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, Serogroup, Virus, Clinical Veterinary Microbiology, 03 medical and health sciences, Medicine, Potency, Animals, Swine Diseases, biology, business.industry, Viral Vaccines, biology.organism_classification, Virology, Recombinant Proteins, Vaccination, Titer, 030104 developmental biology, Foot-and-Mouth Disease Virus, Foot-and-Mouth Disease, Inactivated vaccine, biology.protein, Antibody, Foot-and-mouth disease virus, business
Abstract: Foot-and-mouth disease virus (FMDV) has led to serious losses in animal husbandry worldwide. Seromonitoring of FMDV postvaccination is important for the control and eradication of foot-and-mouth disease (FMD) in regions and countries where vaccination is widespread. However, many commercial kits present high false-positive rates. In this study, a multiepitope-based indirect chemiluminescence immunoassay (ME-CLIA) was developed for specifically detecting antibodies against FMDV serotype O in swine sera. The developed method presented high diagnostic sensitivity and excellent diagnostic specificity, and it could detect a broad spectrum of antibodies against FMDV serotype O. The diagnostic performance, accuracy rate, and analytical sensitivity of ME-CLIA were compared with those of three commercial kits. The immune protection value of multiple-epitope recombinant vaccine detected using ME-CLIA was preliminarily determined by observation of clinical symptoms postimmunization challenge, the results of which indicated that the ME-CLIA can be employed as a matching detection method for evaluating multiple-epitope recombinant vaccine. The percent positive values of ME-CLIA determined using swine vaccinated with inactivated vaccine were significantly positively correlated with the titers of liquid-phase-blocking enzyme-linked immunosorbent assay (ELISA) (LBPE) (r = 0.8361; P
Published: 2021

9. Evaluation of Nanopore Sequencing as a Diagnostic Tool for the Rapid Identification of Mycoplasma bavis from Individual and Pooled Respiratory Tract Samples

Author: Eefke Weesendorp, Nick Vereecke, Jade Bokma, Mathilde L Pas, Freddy Haesebrouck, Filip Boyen, Sebastiaan Theuns, Bart Pardon, Hans Nauwynck, Marianne Vahl, Laurens Chantillon, and Ruud H. Deurenberg
Subjects: Microbiology (medical), Mycoplasma bovis, Pcr assay, Respiratory System, Biology, medicine.disease_cause, Clinical Veterinary Microbiology, Diagnostics & Crisis Organization, parasitic diseases, medicine, Credible interval, Animals, MALDI-TOF MS, bronchoalveolar lavage, selective-indicative agar, Mycoplasma Infections, Diagnostiek & Crisisorganisatie, Bayes Theorem, Virology, Confidence interval, Rapid identification, Nanopore Sequencing, Mycoplasma species, medicine.anatomical_structure, Pooled analysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Cattle, Nanopore sequencing, Bayesian latent class model, Respiratory tract
Abstract: Rapid identification of Mycoplasma bovis infections in cattle is a key factor to guide antimicrobial therapy and biosecurity measures. Recently, Nanopore sequencing became an affordable diagnostic tool for both clinically relevant viruses and bacteria, but the diagnostic accuracy for M. bovis identification is undocumented. Therefore, in this study Nanopore sequencing was compared to rapid identification of M. bovis with matrix-assisted laser desorption ionization-time of flight mass spectrometry (RIMM) and a triplex real-time PCR assay in a Bayesian latent class model (BLCM) for M. bovis in bronchoalveolar lavage fluid (BALf) samples obtained from calves. In practice, pooling of samples is often used to save money, but the influence on diagnostic accuracy has not been described for M. bovis. Therefore, a convenience sample of 17 pooled samples containing 5 individual BALf samples per farm was analyzed as well. The results for the pooled samples were compared with those for the individual samples to determine sensitivity and specificity. The BLCM showed good sensitivity (77.3% [95% credible interval, 57.8 to 92.8%]) and high specificity (97.4% [91.5 to 99.7%]) for Nanopore sequencing, compared to RIMM (sensitivity, 93.0% [76.8 to 99.5%]; specificity, 91.3% [82.5 to 97.0%]) and real-time PCR (sensitivity, 94.6% [89.7 to 97.7%]; specificity, 86.0% [76.1 to 93.6%]). Sensitivity and specificity of pooled analysis for M. bovis were 85.7% (95% confidence interval, 59.8 to 111.6%) and 90.0% (71.4 to 108.6%%), respectively, for Nanopore sequencing and 100% (100% to 100%) and 88.9% (68.4 to 109.4%) for RIMM. In conclusion, Nanopore sequencing is a rapid, reliable tool for the identification of M. bovis. To reduce costs and increase the chance of M. bovis identification, pooling of 5 samples for Nanopore sequencing and RIMM is possible.
Published: 2021

10. Evaluation of a Fecal Shedding Test To Detect Badger Social Groups Infected with Mycobacterium bovis

Author: David Porter, Elizabeth M. H. Wellington, Victoria Hibberd, Andrew R. J. Murphy, and Emma Rachel Travis
Subjects: Microbiology (medical), Disease reservoir, Veterinary medicine, Badger, animal diseases, Disease, Meles, molecular epidemiology, Clinical Veterinary Microbiology, biology.animal, Mustelidae, Animals, bovine tuberculosis, Feces, Disease Reservoirs, badger, QL, Mycobacterium bovis, Wales, Molecular epidemiology, biology, biology.organism_classification, bacterial infections and mycoses, United Kingdom, QR, England, cattle, environmental microbiology, Herd, disease reservoir, Tuberculosis, Bovine
Abstract: Bovine tuberculosis (bTB) is an economically important disease affecting the cattle industry in England and Wales. bTB, caused by Mycobacterium bovis, also causes disease in the Eurasian badger (Meles meles), a secondary maintenance host. Disease transmission between these two species is bidirectional. Infected badgers shed M. bovis in their feces. The Animal and Plant Health Agency (APHA) of the United Kingdom organized a comparative trial to determine the performance of tests in detecting M. bovis in badger feces for the Department for Environment, Food, and Rural Affairs (DEFRA)., Bovine tuberculosis (bTB) is an economically important disease affecting the cattle industry in England and Wales. bTB, caused by Mycobacterium bovis, also causes disease in the Eurasian badger (Meles meles), a secondary maintenance host. Disease transmission between these two species is bidirectional. Infected badgers shed M. bovis in their feces. The Animal and Plant Health Agency (APHA) of the United Kingdom organized a comparative trial to determine the performance of tests in detecting M. bovis in badger feces for the Department for Environment, Food, and Rural Affairs (DEFRA). Here, we assessed the performance of the existing Warwick Fast24-qPCR test and its modified version based on a high-throughput DNA extraction method (Fast96-qPCR). We found Fast24-qPCR to have a sensitivity of 96.7% (95% confidence interval [CI], 94.5 to 99%; n = 244) and a specificity of 99% (95% CI, 97.8 to 100%; n = 292). Fast96-qPCR requires further optimization. Determining the disease status of badger social groups requires multiple tests per group. Therefore, to increase specificity further, we independently repeated the Fast24-qPCR test on positive samples, increasing stringency by requiring a second positive result. Fast24-qPCR with repeat testing had a sensitivity of 87.3% (95% CI, 83.1 to 91.5%; n = 244), and a specificity of 100% (95% CI, 100 to 100; n = 201) on an individual-sample level. At the social-group level, this repeat testing gives Fast24-qPCR high herd specificity, while testing multiple samples per group provides high herd sensitivity. With Fast24-qPCR, we provide a social-group-level test with sufficient specificity and sensitivity to monitor shedding in badgers via latrine sampling, delivering a potentially valuable tool to measure the impacts of bTB control measures.
Published: 2020

11. A Novel Real-Time PCR-Based Screening Test with Pooled Fecal Samples for Bovine Johne’s Disease

Author: Yasuyuki Mori, Reiko Nagata, Yasutaka Minegishi, Shingo Kishizuka, Satoko Kawaji, Akiko Mita, Yumi Saruyama, and Masahiro Saito
Subjects: Microbiology (medical), Veterinary medicine, 040301 veterinary sciences, Cattle Diseases, Paratuberculosis, Enzyme-Linked Immunosorbent Assay, Real-Time Polymerase Chain Reaction, Sensitivity and Specificity, Clinical Veterinary Microbiology, Serology, law.invention, 0403 veterinary science, Feces, 03 medical and health sciences, law, medicine, Animals, Polymerase chain reaction, 030304 developmental biology, 0303 health sciences, biology, 04 agricultural and veterinary sciences, biology.organism_classification, medicine.disease, Mycobacterium avium subsp. paratuberculosis, Real-time polymerase chain reaction, Infectious disease (medical specialty), Herd, Cattle, Mycobacterium
Abstract: Johne’s disease (JD) is an economically important infectious disease in livestock farming caused by Mycobacterium avium subsp. paratuberculosis. As an alternative to serological tests, which are used mainly for the screening of whole herds, we developed a novel ResoLight-based real-time PCR (RL-PCR) assay with pooled fecal samples for the detection of fecal shedders in cattle herds. The RL-PCR assay included an internal amplification control (IC) which was amplified using the same primer pair as the target molecule M. avium subsp. paratuberculosis IS900 and differentiated based on melting temperatures. Individual fecal suspensions were pooled and concentrated by centrifugation to avoid a loss of sensitivity by the dilution effect. Combined with a DNA extraction kit (Johne-PureSpin; FASMAC), no inhibition of PCR amplification was observed with up to 15 fecal samples in a pool. The detection limit of RL-PCR at a pool size of 10 was 10 M. avium subsp. paratuberculosis organisms per gram of feces, which was comparable to that of individual testing. A total of 2,654 animals in 12 infected herds were screened by individual antibody-enzyme-linked immunosorbent assay (ELISA) and the RL-PCR assay using pooled feces. Fifty animals were diagnosed with JD through the screening by RL-PCR, compared with only 5 by ELISA (which were also positive in RL-PCR). In 7 JD-free herds, the results of 4 out of 327 pools (1.2%) were invalid due to the lack of IC amplification, and then animals were confirmed negative individually. Our results suggest that implementation of herd screening by pooled RL-PCR would advance the monitoring and control of JD in cattle herds.
Published: 2020

12. Whole-Genome Sequencing of Porcine Reproductive and Respiratory Syndrome Virus from Field Clinical Samples Improves the Genomic Surveillance of the Virus

Author: Chantale Provost, Carl A. Gagnon, and Christian Lalonde
Subjects: 0301 basic medicine, Microbiology (medical), Canada, Swine, 040301 veterinary sciences, viruses, animal diseases, Porcine Reproductive and Respiratory Syndrome, Genome, DNA sequencing, Virus, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, medicine, Animals, Porcine respiratory and reproductive syndrome virus, Gene, Phylogeny, Whole genome sequencing, biology, Strain (biology), Quebec, virus diseases, Genomics, 04 agricultural and veterinary sciences, respiratory system, medicine.disease, Porcine reproductive and respiratory syndrome virus, biology.organism_classification, Virology, 3. Good health, 030104 developmental biology, Coinfection
Abstract: Porcine reproductive and respiratory syndrome virus (PRRSV) is a major economic concern worldwide. There are currently large data sets available about the ORF5 gene of the virus, with thousands of sequences available, but little data are currently available on the full-length genome of PRRSV. We hypothesized that whole-genome sequencing (WGS) of the PRRSV genome would allow better epidemiological monitoring than ORF5 gene sequencing. PRRSV PCR-positive serum, oral fluid, and tissue clinical samples submitted to the diagnostic laboratory for routine surveillance or diagnosis of PRRSV infection in Québec, Canada, swine herds were used. The PRRSV reverse transcription-quantitative PCR Cq values of the processed samples varied between 11.5 and 34.34. PRRSV strain genomes were isolated using a poly (A)-tail method and were sequenced with a MiSeq Illumina sequencer. Ninety-two full-length PRRSV genomes were obtained from 88 clinical samples out of 132 tested samples, resulting in a PRRSV WGS success rate of 66.67%. Three important deletions in ORF1a were found in most wild-type (i.e., not vaccine-like) strains. The importance of these deletions remains undetermined. Two different full-length PRRSV genomes were found in four different samples (three serum samples and one pool of tissues), suggesting a 4.55% PRRSV strain coinfection prevalence in swine. Moreover, six PRRSV whole genomes (6.52% of PRRSV strains) were found to cluster differently than they did under the ORF5 classification method. Overall, WGS of PRRSV enables better strain classification and/or interpretation of results in 9.10% of clinical samples than ORF5 sequencing, as well as allowing interesting research avenues.
Published: 2020

13. Resolution of Streptococcus suis Serotypes 1/2 versus 2 and 1 versus 14 by PCR-Restriction Fragment Length Polymorphism Method

Author: Bronislav Šimek, Monika Zouharova, Jan Matiasovic, Marcelo Gottschalk, Natalie Kralova, Katarína Matiašková, Katerina Nedbalcova, and Ivana Kucharovicova
Subjects: 0301 basic medicine, Microbiology (medical), Serotype, Streptococcus suis, Swine, 030106 microbiology, Locus (genetics), Serogroup, Polymerase Chain Reaction, Clinical Veterinary Microbiology, 03 medical and health sciences, Human health, Streptococcal Infections, Animals, Serotyping, Gene, Pathogen, Genetics, biology, biology.organism_classification, 3. Good health, Restriction enzyme, 030104 developmental biology, Restriction fragment length polymorphism, Polymorphism, Restriction Fragment Length
Abstract: Streptococcus suis is an important pathogen of pigs but is also transmissible to humans, with potentially fatal consequences. Among 29 serotypes currently recognized, some are clinically and epidemiologically more important than others. This is particularly true for serotypes 2 and 14, which have a large impact on pig production and also on human health. Conventional PCR-based serotyping cannot distinguish between serotype 1/2 and serotype 2 or between serotype 1 and serotype 14. Although serotype 1/2 and serotype 2 have a very similar cps locus, they differ in a single-nucleotide substitution at nucleotide position 483 of the cpsK gene. Similarly, serotypes 1 and 14 have a very similar cps locus but also differ in the same nucleotide substitution of the cpsK gene. Fortunately, this cpsK 483G→C/T substitution can be detected by BstNI restriction endonuclease. A PCR-restriction fragment length polymorphism (RFLP) detection method amplifying a fragment of the cpsK gene digested by BstNI restriction endonuclease was developed and tested in reference strains of these serotypes and also in field isolates.
Published: 2020

14. Detection of Bovine Antibodies against a Conserved Capsid Epitope as the Basis of a Novel Universal Serological Test for Foot-and-Mouth Disease

Author: Stephen Berryman, Tobias J. Tuthill, Ginette Wilsden, Satya Parida, Emiliana Brocchi, Donald P. King, Anna B. Ludi, N. Howe, Krupali Parekh, Santina Grazioli, and Amin S. Asfor
Subjects: 0301 basic medicine, Microbiology (medical), Serotype, 040301 veterinary sciences, medicine.drug_class, diagnosis, conserved capsid, viruses, serology, Enzyme-Linked Immunosorbent Assay, Monoclonal antibody, Antibodies, Viral, Epitope, Virus, Serology, Clinical Veterinary Microbiology, 0403 veterinary science, FMDV, 03 medical and health sciences, Epitopes, Capsid, Antigen, medicine, Animals, Serologic Tests, epitope, biology, foot-and-mouth disease virus, 04 agricultural and veterinary sciences, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Virology, 030104 developmental biology, Foot-and-Mouth Disease, ELISA, Capsid Proteins, Cattle, Foot-and-mouth disease virus, conserved capsid epitope
Abstract: Diagnostic tests for foot-and-mouth disease (FMD) include the detection of antibodies against either the viral nonstructural proteins or the capsid. The detection of antibodies against the structural proteins (SP) of the capsid can be used to monitor seroconversion in both infected and vaccinated animals. However, SP tests need to be tailored to the individual FMD virus (FMDV) serotype and their sensitivity may be affected by antigenic variability within each serotype and mismatching between test reagents., Diagnostic tests for foot-and-mouth disease (FMD) include the detection of antibodies against either the viral nonstructural proteins or the capsid. The detection of antibodies against the structural proteins (SP) of the capsid can be used to monitor seroconversion in both infected and vaccinated animals. However, SP tests need to be tailored to the individual FMD virus (FMDV) serotype and their sensitivity may be affected by antigenic variability within each serotype and mismatching between test reagents. As a consequence, FMD reference laboratories are required to maintain multiple type-specific SP assays and reagents. A universal SP test would simplify frontline diagnostics and facilitate large-scale serological surveillance and postvaccination monitoring. In this study, a highly conserved region in the N terminus of FMDV capsid protein VP2 (VP2N) was characterized using a panel of intertype-reactive monoclonal antibodies. This revealed a universal epitope in VP2N which could be used as a peptide antigen to detect FMDV-specific antibodies against all types of the virus. A VP2-peptide enzyme-linked immunosorbent assay (VP2-ELISA) was optimized using experimental and reference antisera from immunized, convalescent, and naïve animals (n = 172). The VP2-ELISA is universal and simple and provided sensitive (99%) and specific (93%) detection of antibodies to all FMDV strains used in this study. We anticipate that this SP test could have utility for serosurveillance during virus incursions in FMD-free countries and as an additional screening tool to assess FMD virus circulation in countries where the disease is endemic.
Published: 2020

15. Validation of Bartonella henselae Western Immunoblotting for Serodiagnosis of Bartonelloses in Dogs

Author: James R. Wilson, Ricardo G. Maggi, Nandhakumar Balakrishnan, Michael R. Lappin, Sindhura Sevala, Bruno B Chomel, Adam J. Birkenheuer, Edward B. Breitschwerdt, Pradeep Neupane, and Henry S. Marr
Subjects: 0301 basic medicine, Microbiology (medical), Bartonella, 040301 veterinary sciences, Blotting, Western, Clinical Veterinary Microbiology, Serology, 0403 veterinary science, 03 medical and health sciences, Dogs, Antigen, Brucella canis, Bartonella Infections, medicine, Animals, Serologic Tests, Dog Diseases, Bartonella henselae, biology, Zoonosis, Bartonelloses, 04 agricultural and veterinary sciences, bacterial infections and mycoses, biology.organism_classification, medicine.disease, Rickettsia rickettsii, Antibodies, Bacterial, Virology, 030104 developmental biology
Abstract: Bartonella spp. are etiological agents of life-threatening zoonotic diseases in dogs worldwide. Due to the poor sensitivity of immunofluorescent-antibody assays (IFAs), a reliable serodiagnostic test for canine bartonelloses is of clinical importance. The utility of Western blotting (WB) for the serodiagnosis of canine bartonelloses has not been critically investigated. The objective of this study was to characterize WB immunodominant proteins that could be used to confirm a serodiagnosis of bartonelloses. Using agar-grown Bartonella henselae San Antonio type 2 (SA2) whole-cell proteins, sera derived from four dog groups were tested by WB to assess immunodominant protein recognition patterns: group I consisted of 92 serum samples (10 preexposure and 82 postexposure serum samples) from 10 adult beagles experimentally inoculated with Bartonella spp., group II consisted of 36 serum samples from Bartonella PCR-positive naturally infected dogs, group III consisted of 26 serum samples from Bartonella PCR-negative and IFA-negative dogs, and group IV consisted of serum samples from 8 Brucella canis IFA-positive and 10 Rickettsia rickettsii IFA-positive dogs. Following experimental inoculation, 9 (90%) group I dogs were variably seroreactive to one or more of six specific immunodominant proteins (13, 17, 29, 50, 56, and 150 kDa). There was a strong but variable recognition of these proteins among 81% of group II dogs. In contrast, 24/26 group III dogs were not reactive to any immunodominant protein. In this study, the sensitivity and diagnostic accuracy of B. henselae SA2 WB were higher than those of B. henselae SA2 IFA testing. Some B. henselae SA2 immunodominant proteins were recognized by dogs experimentally and naturally infected with Bartonella spp. other than B. henselae. Additional research is necessary to more fully define the utility of WB for the serodiagnosis of canine bartonelloses.
Published: 2020

16. Retraction for Kanabagatte Basavarajappa et al., 'Glycoprotein-Based Enzyme-Linked Immunosorbent Assays for Serodiagnosis of Infectious Laryngotracheitis'

Author: Haichen Song, Siba K. Samal, Chinta Lamichhane, and Mallikarjuna Kanabagatte Basavarajappa
Subjects: Microbiology (medical), chemistry.chemical_classification, Enzyme, chemistry, business.industry, Medicine, Infectious laryngotracheitis, Glycoprotein, business, Virology, Clinical Veterinary Microbiology
Abstract: For detection of infectious laryngotracheitis virus (ILTV) antibody, glycoprotein B-, C-, and D-based enzyme-linked immunosorbent assays (B-, C-, and D-ELISAs, respectively) were developed. The B- and D-ELISAs showed enhanced detection of anti-ILTV antibodies in infected chickens compared to that of the commercial ELISA. Furthermore, the D-ELISA was efficient in detecting seroconversion with vectored vaccine, using recombinant Newcastle disease virus (rNDV) expressing glycoprotein D (gD) as the vaccine vector.
Published: 2020

17. Comparison of Two Multilocus Sequence Typing Schemes for Mycoplasma bovis and Revision of the PubMLST Reference Method

Author: David P. Alt, Karen B. Register, Darrell O. Bayles, Murray D. Jelinski, Inna Lysnyansky, Matthew Waldner, William D. Boatwright, and Paola Pilo
Subjects: 0301 basic medicine, Microbiology (medical), Mycoplasma bovis, Genotype, 040301 veterinary sciences, Cattle Diseases, Locus (genetics), Computational biology, Biology, medicine.disease_cause, Genome, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, medicine, Animals, Typing, Phylogeny, Deer, Goats, 04 agricultural and veterinary sciences, Sequence types, 030104 developmental biology, Multilocus sequence typing, Cattle, Female, Multilocus Sequence Typing
Abstract: Mycoplasma bovis causes pneumonia, pharyngitis, otitis, arthritis, mastitis, and reproductive disorders in cattle and bison. Two multilocus sequence typing (MLST) schemes have been developed for M. bovis, with one serving as the PubMLST reference method, but no comparison of the schemes has been undertaken. Although the PubMLST scheme has proven to be highly discriminatory and informative, the recent discovery of isolates missing one of the typing loci, adh-1, raises concern about its suitability for continued use. The goal of our study was to compare the performance of the two MLST schemes and identify a new reference scheme capable of fully typing all isolates. We evaluated 448 isolates from diverse geographic and anatomic sites that collectively represent cattle, bison, deer, and a goat. The discrimination indexes (DIs) for the PubMLST and the alternative scheme are 0.909 (91 sequence types [STs]) and 0.842 (77 STs), respectively. Although the PubMLST scheme outperformed the alternative scheme, the adh-1 locus must be retired from the PubMLST scheme if it is to be retained as a reference method. The DI obtained using the six remaining PubMLST loci (0.897, 79 STs) fails to reach the benchmark recommended for a reference method (0.900), mandating the addition of a seventh locus. Comparative analysis of genome sequences from the isolates used here identified the dnaA locus from the alternative scheme as the optimal replacement for adh-1. This revised scheme, which will be implemented as the new PubMLST reference method, has a DI of 0.914 and distinguishes 88 STs from the 448 isolates evaluated.
Published: 2020

18. Rapid Identification of Mycoplasma bovis Strains from Bovine Bronchoalveolar Lavage Fluid with Matrix-Assisted Laser Desorption Ionization-Time of Flight Mass Spectrometry after Enrichment Procedure

Author: Jade Bokma, Marianne Vahl, Bart Pardon, Filip Boyen, Eefke Weesendorp, Piet Deprez, Ruud H. Deurenberg, Laura Van Driessche, and Freddy Haesebrouck
Subjects: 0301 basic medicine, Microbiology (medical), MALDI-TOF, Mycoplasma bovis, food.ingredient, 040301 veterinary sciences, 030106 microbiology, CATTLE, Mycoplasma bovirhinis, DRUG-USE, medicine.disease_cause, Mass spectrometry, Microbiology, Diagnostics & Crisis Organization, Clinical Veterinary Microbiology, 0403 veterinary science, CULTURE, 03 medical and health sciences, food, Mycoplasma, Mycoplasma dispar, medicine, Agar, Animals, Veterinary Sciences, Incubation, SPECIFICITY, medicine.diagnostic_test, Diagnostiek & Crisisorganisatie, Chemistry, Bayes Theorem, 04 agricultural and veterinary sciences, lipase activity, Rapid identification, Bronchoalveolar lavage, INFECTIONS, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, RISK-FACTORS, Cattle, RESPIRATORY PATHOGENS, SENSITIVITY, Bayesian latent class model, CALVES, Bronchoalveolar Lavage Fluid
Abstract: Mycoplasma bovis is a leading cause of pneumonia in modern calf rearing. Fast identification is essential to ensure appropriate antimicrobial therapy. Therefore, the objective of this study was to develop a protocol to identify M. bovis from bronchoalveolar lavage fluid (BALf) with matrix-assisted laser desorption ionization–time of flight mass spectrometry MALDI-TOF MS and to determine the diagnostic accuracy in comparison with other techniques. BALf was obtained from 104 cattle, and the presence of M. bovis was determined in the following three ways: (i) rapid identification of M. bovis with MALDI-TOF MS (RIMM) (BALf was enriched and after 24, 48, and 72 h of incubation and was analyzed using MALDI-TOF MS), (ii) triplex real-time PCR for M. bovis, Mycoplasma bovirhinis, and Mycoplasma dispar, and (iii) 10-day incubation on selective-indicative agar. The diagnostic accuracy of the three tests was determined with Bayesian latent class modeling (BLCM). After 24 h of enrichment, M. bovis was identified with MALDI-TOF MS in 3 out of 104 BALf samples. After 48 and 72 h of enrichment, 32/104 and 38/100 samples, respectively, were M. bovis positive. Lipase-positive Mycoplasma-like colonies were seen in 28 of 104 samples. Real-time PCR resulted in 28/104 positive and 12/104 doubtful results for M. bovis. The BLCM showed a sensitivity (Se) and specificity (Sp) of 86.6% (95% credible interval [CI], 69.4% to 97.6%) and 86.4% (CI, 76.1 to 93.8) for RIMM. For real-time PCR, Se was 94.8% (CI, 89.9 to 97.9) and Sp was 88.9% (CI, 78.0 to 97.4). For selective-indicative agar, Se and Sp were 70.5% (CI, 52.1 to 87.1) and 93.9% (CI, 85.9 to 98.4), respectively. These results suggest that rapid identification of M. bovis with MALDI-TOF MS after an enrichment procedure is a promising test for routine diagnostics in veterinary laboratories.
Published: 2020

19. Rapid Sequence-Based Characterization of African Swine Fever Virus by Use of the Oxford Nanopore MinION Sequence Sensing Device and a Companion Analysis Software Tool

Author: Vivian O'Donnell, Kimberly A. Dodd, Frederic R. Grau, Gregory A. Mayr, Tracy L. Sturgill Samayoa, and Roger W. Barrette
Subjects: 0301 basic medicine, Microbiology (medical), Swine, 040301 veterinary sciences, Early detection, Genome, Viral, African swine fever virus, Genome, DNA sequencing, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, Animals, Analysis software, African Swine Fever, Sequence (medicine), biology, Computational Biology, High-Throughput Nucleotide Sequencing, Reproducibility of Results, Sequence Analysis, DNA, 04 agricultural and veterinary sciences, biology.organism_classification, African Swine Fever Virus, Virology, Nanopore Sequencing, 030104 developmental biology, Minion, Reagent Kits, Diagnostic, Nanopore sequencing, Software
Abstract: African swine fever virus (ASFV) is the causative agent of a severe and highly contagious viral disease of pigs that poses serious economic consequences to the swine industry due to the high mortality rate and impact on international trade. There is no effective vaccine to control African swine fever (ASF), and therefore, efficient disease control is dependent on early detection and diagnosis of ASFV. The large size of the ASFV genome (∼180 kb) has historically hindered efforts to rapidly obtain a full-genome sequence. Rapid acquisition of data is critical for characterization of the isolate and to support epidemiological efforts. Here, we investigated the capacity of the Oxford Nanopore MinION sequence sensing device to act as a rapid sequencing tool. When coupled with our novel companion software script, the African swine fever fast analysis sequencing tool (ASF-FAST), the analysis of output data was performed in real time. Complete ASFV genome sequences were generated from cell culture isolates and blood samples obtained from experimentally infected pigs. Removal of the host-methylated DNA from the extracted nucleic acid facilitated rapid ASFV sequence identification, with reads specific to ASFV detected within 6 min after the initiation of sequencing. Regardless of the starting material, sufficient sequence was available for complete genome resolution (up to 100%) within 10 min. Overall, this paper highlights the use of Nanopore sequencing technology in combination with the ASF-FAST software for the purpose of rapid and real-time resolution of the full ASFV genome from a diagnostic sample.
Published: 2019

20. Differentiation of Community-Associated and Livestock-Associated Methicillin-Resistant Staphylococcus aureus Isolates and Identification of

Author: Seyed A, Ghorashi, Jane, Heller, Quincy, Zhang, and Shafi, Sahibzada
Subjects: Methicillin-Resistant Staphylococcus aureus, Livestock, Swine, Animals, Microbial Sensitivity Tests, Staphylococcal Infections, Staphylococcal Protein A, Polymerase Chain Reaction, Clinical Veterinary Microbiology
Abstract: Infections due to methicillin-resistant Staphylococcus aureus (MRSA) are present worldwide and represent a major public health concern. The capability of PCR followed by high-resolution melt (HRM) curve analysis for the detection of community-associated and livestock-associated MRSA strains and the identification of staphylococcal protein A (spa) locus was evaluated in 74 MRSA samples which were isolated from the environment, humans, and pigs on a single piggery. PCR-HRM curve analysis identified four spa types among MRSA samples and differentiated MRSA strains accordingly. A nonsubjective differentiation model was developed according to genetic confidence percentage values produced by tested samples, which did not require visual interpretation of HRM curve results. The test was carried out at different settings, and result data were reanalyzed and confirmed with DNA sequencing. PCR-HRM curve analysis proved to be a robust and reliable test for spa typing and can be used as a tool in epidemiological studies.
Published: 2019

21. Implication of Broadly Neutralizing Bovine Monoclonal Antibodies in the Development of an Enzyme-Linked Immunosorbent Assay for Detecting Neutralizing Antibodies against Foot-and-Mouth Disease Virus Serotype O

Author: Sheng Wang, Zengjun Lu, Pu Sun, Xueqing Ma, Zhiyong Li, Yingli Chen, Kun Li, Xiangchuan Xing, Huifang Bao, Zaixin Liu, Dong Li, Yuanfang Fu, Yimei Cao, Shasha Zhou, Jing Zhang, Xingwen Bai, and Pinghua Li
Subjects: Veterinary Medicine, 0301 basic medicine, Microbiology (medical), Serotype, 040301 veterinary sciences, medicine.drug_class, Enzyme-Linked Immunosorbent Assay, Biology, Antibodies, Viral, Monoclonal antibody, Sensitivity and Specificity, Peripheral blood mononuclear cell, Virus, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, medicine, Animals, Neutralizing antibody, B cell, Antibodies, Monoclonal, Viral Vaccines, 04 agricultural and veterinary sciences, biology.organism_classification, Antibodies, Neutralizing, Virology, 030104 developmental biology, medicine.anatomical_structure, Vaccines, Inactivated, Foot-and-Mouth Disease Virus, Foot-and-Mouth Disease, biology.protein, Cattle, Foot-and-mouth disease virus, Antibody
Abstract: Vaccination with inactivated vaccines is still the main measure to control foot-and-mouth disease (FMD) in areas where the disease is endemic, and the level of neutralizing antibody in vaccinated animals is directly related to their protection against virus challenge. Currently, neutralizing antibody is mainly detected using the virus neutralization test (VNT) based on cell culture, which is laborious and time-consuming and requires restrictive biocontainment facilities. In this study, two broadly neutralizing antibodies (bnAbs), E46 and F128, were successfully produced using techniques for the isolation of single B cells from peripheral blood mononuclear cells (PBMCs) from bovines sequentially immunized with three topotypes of foot-and-mouth disease virus (FMDV) serotype O. Based on these bnAbs, a blocking enzyme-linked immunosorbent assay (ELISA) for detecting neutralizing antibodies (NA-ELISA) against FMDV serotype O was developed. The specificity and sensitivity of the test were estimated to be 99.21% and 100%, respectively. A significant correlation (P
Published: 2019

22. Comparative Phenotypic and Genotypic Analysis of Edwardsiella Isolates from Different Hosts and Geographic Origins, with Emphasis on Isolates Formerly Classified as E. tarda, and Evaluation of Diagnostic Methods

Author: Timothy J. Welch, Patricia S. Gaunt, Lester H. Khoo, Cova R. Arias, James Steadman, Thomas P. Loch, David J. Wise, Julio C. García, Geoffrey C. Waldbieser, Noemí Buján, Cynthia B. Stine, Stephen R. Reichley, Matt J. Griffin, Cynthia Ware, Terrence E. Greenway, Mark L. Lawrence, Benjamin R. LaFrentz, Anil J. Thachil, and Rocco C. Cipriano
Subjects: 0301 basic medicine, Microbiology (medical), Genotype, Biology, DNA gyrase, Clinical Veterinary Microbiology, Fish Diseases, 03 medical and health sciences, Bacterial Proteins, RNA, Ribosomal, 16S, Multiplex polymerase chain reaction, Animals, Edwardsiella tarda, Gene, Genetics, Superoxide Dismutase, business.industry, Enterobacteriaceae Infections, Sequence Analysis, DNA, 16S ribosomal RNA, biology.organism_classification, Biotechnology, Phylogeography, Phenotype, 030104 developmental biology, DNA Gyrase, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Edwardsiella, Identification (biology), business, Multiplex Polymerase Chain Reaction
Abstract: Edwardsiella spp. are responsible for significant losses in important wild and cultured fish species worldwide. Recent phylogenomic investigations have determined that bacteria historically classified as Edwardsiella tarda actually represent three genetically distinct yet phenotypically ambiguous taxa with various degrees of pathogenicity in different hosts. Previous recognition of these taxa was hampered by the lack of a distinguishing phenotypic character. Commercial test panel configurations are relatively constant over time, and as new species are defined, appropriate discriminatory tests may not be present in current test panel arrangements. While phenobiochemical tests fail to discriminate between these taxa, data presented here revealed discriminatory peaks for each Edwardsiella species using matrix-assisted laser desorption ionization–time of flight (MALDI-TOF) methodology, suggesting that MALDI-TOF can offer rapid, reliable identification in line with current systematic classifications. Furthermore, a multiplex PCR assay was validated for rapid molecular differentiation of the Edwardsiella spp. affecting fish. Moreover, the limitations of relying on partial 16S rRNA for discrimination of Edwardsiella spp. and advantages of employing alternative single-copy genes gyrB and sodB for molecular identification and classification of Edwardsiella were demonstrated. Last, sodB sequencing confirmed that isolates previously defined as typical motile fish-pathogenic E. tarda are synonymous with Edwardsiella piscicida , while atypical nonmotile fish-pathogenic E. tarda isolates are equivalent to Edwardsiella anguillarum . Fish-nonpathogenic E. tarda isolates are consistent with E. tarda as it is currently defined. These analyses help deconvolute the scientific literature regarding these organisms and provide baseline information to better facilitate proper taxonomic assignment and minimize erroneous identifications of Edwardsiella isolates in clinical and research settings.
Published: 2017

23. Association of Atypical Enteropathogenic Escherichia coli with Diarrhea and Related Mortality in Kittens

Author: Chitrita DebRoy, Megan E. Jacob, Sandra J. Strong, Victoria E. Watson, James R. Flowers, and Jody L. Gookin
Subjects: Diarrhea, 0301 basic medicine, Microbiology (medical), Parenteral Nutrition, medicine.medical_specialty, Fluid administration, genetic structures, Colon, 030106 microbiology, Physiology, Cat Diseases, Clinical Veterinary Microbiology, Enteropathogenic Escherichia coli, 03 medical and health sciences, Intestinal inflammation, Intestine, Small, medicine, Animals, Escherichia coli Infections, Feces, Intimin, Virulence, business.industry, Gastrointestinal pathology, Disease Models, Animal, Cats, Histopathology, sense organs, medicine.symptom, business, Multiplex Polymerase Chain Reaction
Abstract: Diarrhea is responsible for the death of approximately 900,000 children per year worldwide. In children, typical enteropathogenic Escherichia coli (EPEC) is a common cause of diarrhea and is associated with a higher hazard of death. Typical EPEC infection is rare in animals and poorly reproduced in experimental animal models. In contrast, atypical EPEC (aEPEC) infection is common in both children and animals, but its role in diarrhea is uncertain. Mortality in kittens is often attributed to diarrhea, and we previously identified enteroadherent EPEC in the intestines of deceased kittens. The purpose of this study was to determine the prevalence and type of EPEC in kittens and whether infection was associated with diarrhea, diarrhea-related mortality, gastrointestinal pathology, or other risk factors. Kittens with and without diarrhea were obtained from two shelter facilities and determined to shed atypical EPEC at a culture-based prevalence of 18%. In contrast, quantitative PCR detected the presence of the gene for intimin ( eae ) in feces from 42% of kittens. aEPEC was isolated from kittens with and without diarrhea. However, kittens with diarrhea harbored significantly larger quantities of aEPEC than kittens without diarrhea. Kittens with aEPEC had a significantly greater severity of small intestinal and colonic lesions and were significantly more likely to have required subcutaneous fluid administration. These findings identify aEPEC to be prevalent in kittens and a significant primary or contributing cause of intestinal inflammation, diarrhea, dehydration, and associated mortality in kittens.
Published: 2017

24. Targeted Enrichment for Pathogen Detection and Characterization in Three Felid Species

Author: Martin Löchelt, Justin S. Lee, Timo Kehl, Sue VandeWoude, Christina Boucher, Thomas Harrison, Trey Kind, Basir Shariat, and Ryan S. Mackie
Subjects: 0301 basic medicine, Microbiology (medical), Pathogen detection, Computational biology, Biology, Cat Diseases, Genome, DNA sequencing, Clinical Veterinary Microbiology, Serology, 03 medical and health sciences, 0302 clinical medicine, Animals, Multiplex, Pathogen, pathogen genomics, Oligonucleotide, Ecology, multiplex diagnostic assay, High-Throughput Nucleotide Sequencing, Bacterial Infections, 030104 developmental biology, Molecular Diagnostic Techniques, Virus Diseases, targeted enrichment, 030220 oncology & carcinogenesis, Cats, Nucleic acid, next-generation sequencing, Nucleic Acid Amplification Techniques
Abstract: Traditional diagnostic assays often lack sensitivity and can be difficult to multiplex across many pathogens. Next-generation sequencing (NGS) can overcome some of these problems but has limited application in the detection of low-copy-number pathogens in complex samples. Targeted genome capture (TGC) utilizes oligonucleotide probes to enrich specific nucleic acids in heterogeneous extracts and can therefore increase the proportion of NGS reads for low-abundance targets. While earlier studies have demonstrated the utility of this technology for detection of novel pathogens in human clinical samples, the capacity and practicality of TGC-NGS in a veterinary diagnostic setting have not yet been evaluated. Here we report the use of TGC-NGS assays for the detection and characterization of diverse feline pathogen taxa. We detected 31 pathogens comprising nine pathogen taxa in 28 felid samples analyzed. This included 20 pathogens detected via traditional PCR and 11 additional pathogens that had not been previously detected in the same samples. Most of the pathogens detected were sequenced at sufficient breadth and depth to confidently classify them at the species or subspecies level. Target nucleic acids were enriched from a low of 58-fold to 56 million-fold relative to host nucleic acids. Despite the promising performance of these assays, a number of pathogens detected by conventional PCR or serology were not isolated by TGC-NGS, suggesting that further validation is required before this technology can be used in lieu of quality-controlled standard assays. We conclude that TGC-NGS offers great potential as a broad multiplex pathogen characterization assay in veterinary diagnostic and research settings.
Published: 2017

25. Detection of Antigenic Variants of Subtype H3 Swine Influenza A Viruses from Clinical Samples

Author: Andrew S. Bowman, Lei Li, Larry A. Hanson, Xiu-Feng Wan, Brigitte E. Martin, Jacqueline M. Nolting, and David R. Smith
Subjects: 0301 basic medicine, Microbiology (medical), Swine, Population, Biology, Real-Time Polymerase Chain Reaction, medicine.disease_cause, Virus, Antigenic drift, Clinical Veterinary Microbiology, 03 medical and health sciences, Orthomyxoviridae Infections, Virology, Influenza A virus, medicine, Antigenic variation, Animals, education, Antigens, Viral, Immunoassay, Swine Diseases, education.field_of_study, Reverse Transcriptase Polymerase Chain Reaction, Influenza A Virus, H3N2 Subtype, Antigenic shift, Outbreak, Antigenic Variation, Vaccination, 030104 developmental biology
Abstract: A large population of genetically and antigenically diverse influenza A viruses (IAVs) are circulating among the swine population, playing an important role in influenza ecology. Swine IAVs not only cause outbreaks among swine but also can be transmitted to humans, causing sporadic infections and even pandemic outbreaks. Antigenic characterizations of swine IAVs are key to understanding the natural history of these viruses in swine and to selecting strains for effective vaccines. However, influenza outbreaks generally spread rapidly among swine, and the conventional methods for antigenic characterization require virus propagation, a time-consuming process that can significantly reduce the effectiveness of vaccination programs. We developed and validated a rapid, sensitive, and robust method, the polyclonal serum-based proximity ligation assay (polyPLA), to identify antigenic variants of subtype H3N2 swine IAVs. This method utilizes oligonucleotide-conjugated polyclonal antibodies and quantifies antibody-antigen binding affinities by quantitative reverse transcription-PCR (RT-PCR). Results showed the assay can rapidly detect H3N2 IAVs directly from nasal wash or nasal swab samples collected from laboratory-challenged animals or during influenza surveillance at county fairs. In addition, polyPLA can accurately separate the viruses at two contemporary swine IAV antigenic clusters (H3N2 swine IAV-α and H3N2 swine IAV-ß) with a sensitivity of 84.9% and a specificity of 100.0%. The polyPLA can be routinely used in surveillance programs to detect antigenic variants of influenza viruses and to select vaccine strains for use in controlling and preventing disease in swine.
Published: 2017

26. Evaluation of Genotypic and Phenotypic Protease Virulence Tests for Dichelobacter nodosus Infection in Sheep

Author: Richard Whittington, Om P. Dhungyel, and Andrew S. McPherson
Subjects: 0301 basic medicine, Microbiology (medical), Fastidious organism, AprV2, sheep, 040301 veterinary sciences, diagnosis, medicine.medical_treatment, Virulence, Sheep Diseases, Dichelobacter nodosus, footrot, Polymerase Chain Reaction, Microbiology, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, Bacterial Proteins, Foot rot, Genotype, medicine, elastase, Animals, Pathogen, Foot Rot, Protease, biology, Pancreatic Elastase, Serine Endopeptidases, Australia, protease, 04 agricultural and veterinary sciences, biology.organism_classification, Virology, qPCR, 030104 developmental biology, Flock
Abstract: Dichelobacter nodosus is a fastidious, strictly anaerobic bacterium, an obligate parasite of the ruminant hoof, and the essential causative agent of virulent ovine footrot. The clinical disease results from a complex interplay between the pathogen, the environment, and the host. Sheep flocks diagnosed with virulent but not benign footrot in Australia may be quarantined and required to undergo a compulsory eradication program, with costs met by the farmer. Virulence of D. nodosus at least partially depends on the elaboration of a protease encoded by aprV2 and manifests as elastase activity. Laboratory virulence tests are used to assist diagnosis because clinical differentiation of virulent and benign footrot can be challenging during the early stages of disease or when the disease is not fully expressed due to unfavorable pasture conditions. Using samples collected from foot lesions from 960 sheep from 40 flocks in four different geographic regions, we evaluated the analytical characteristics of qPCR tests for the protease gene alleles aprV2 and aprB2 , and compared these with results from phenotypic protease (elastase and gelatin gel) tests. There was a low level of agreement between clinical diagnosis and quantitative PCR (qPCR) test outcomes at both the flock and sample levels and poor agreement between qPCR test outcomes and the results of phenotypic virulence tests. The diagnostic specificity of the qPCR test was low at both the flock and individual swab levels (31.3% and 18.8%, respectively). By contrast, agreement between the elastase test and clinical diagnosis was high at both the flock level (diagnostic sensitivity [DSe], 100%; diagnostic specificity [DSp], 78.6%) and the isolate level (DSe, 69.5%; DSp, 80.5%).
Published: 2017

27. Evaluation of Veterinary-Specific Interpretive Criteria for Susceptibility Testing of Streptococcus equi Subspecies with Trimethoprim-Sulfamethoxazole and Trimethoprim-Sulfadiazine

Author: Jeffrey L. Watts, Theo Kanellos, Carmen Sadaka, Luca Guardabassi, and Joseph F. Boucher
Subjects: 0301 basic medicine, Microbiology (medical), Veterinary Medicine, Susceptibility testing, Streptococcus equi, 040301 veterinary sciences, animal diseases, 030106 microbiology, Antimicrobial susceptibility, Sulfadiazine, breakpoints, Microbial Sensitivity Tests, Subspecies, strangles, Trimethoprim, Microbiology, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, parasitic diseases, Trimethoprim, Sulfamethoxazole Drug Combination, medicine, Animals, horses, veterinary microbiology, Strangles, business.industry, Sulfamethoxazole, interpretive criteria, 04 agricultural and veterinary sciences, potentiated sulfonamides, bacterial infections and mycoses, 3. Good health, respiratory tract diseases, Anti-Bacterial Agents, Drug Combinations, business, medicine.drug
Abstract: Antimicrobial susceptibility test results for trimethoprim-sulfadiazine with Streptococcus equi subspecies are interpreted based on human data for trimethoprim-sulfamethoxazole. The veterinary-specific data generated in this study support a single breakpoint for testing trimethoprim-sulfamethoxazole and/or trimethoprim-sulfadiazine with S. equi . This study indicates trimethoprim-sulfamethoxazole as an acceptable surrogate for trimethoprim-sulfadiazine with S. equi .
Published: 2016

28. Single-Cell-Based Digital PCR Detection and Association of Shiga Toxin-Producing Escherichia coli Serogroups and Major Virulence Genes

Author: Tiruvoor G. Nagaraja, Jianfa Bai, Yin Wang, Colin Stoy, Lance W. Noll, Gary A. Anderson, Xuming Liu, Xiaorong Shi, Nanyan Lu, and Elizabeth Porter
Subjects: 0301 basic medicine, Microbiology (medical), DNA, Bacterial, Meat, Virulence Factors, 030106 microbiology, Virulence, Biology, medicine.disease_cause, Serogroup, Shiga Toxin 1, Polymerase Chain Reaction, Shiga Toxin 2, Microbiology, Shiga Toxin, Clinical Veterinary Microbiology, 03 medical and health sciences, Feces, fluids and secretions, STX2, medicine, Animals, Digital polymerase chain reaction, Gene, Escherichia coli, Intimin, Shiga-Toxigenic Escherichia coli, Escherichia coli Proteins, O Antigens, Shiga toxin, bacterial infections and mycoses, 030104 developmental biology, Genes, Bacterial, biology.protein, Food Microbiology, Cattle, Single-Cell Analysis
Abstract: Escherichia coli serogroups O157, O26, O45, O103, O111, O121, and O145, when carrying major virulence genes, the Shiga toxin genes stx(1) and stx(2) and the intimin gene eae, are important foodborne pathogens. They are referred to as the “top 7” Shiga toxin-producing E. coli (STEC) serogroups and were declared by the USDA as adulterants to human health. Since top 7 serogroup-positive cattle feces and ground beef can also contain nonadulterant E. coli strains, regular PCR cannot confirm whether the virulence genes are carried by adulterant or nonadulterant E. coli serogroups. Thus, traditional gold-standard STEC detection requires bacterial isolation and characterization, which are not compatible with high-throughput settings and often take a week to obtain a definitive result. In this study, we demonstrated that the partition-based multichannel digital PCR (dPCR) system can be used to detect and associate the E. coli serogroup-specific gene with major virulence genes and developed a single-cell-based dPCR approach for rapid (within 1 day) and accurate detection and confirmation of major STEC serogroups in high-throughput settings. Major virulence genes carried by each of the top 7 STEC serogroups were detected by dPCR with appropriately diluted intact bacterial cells from pure cultures, culture-spiked cattle feces, and culture-spiked ground beef. Furthermore, from 100 randomly collected, naturally shed cattle fecal samples, 3 O103 strains carrying eae and 2 O45 strains carrying stx(1) were identified by this dPCR assay and verified by the traditional isolation method. This novel and rapid dPCR assay is a culture-independent, high-throughput, accurate, and sensitive method for STEC detection and confirmation.
Published: 2019

29. Interleukin 8 and Pentaxin (C-Reactive Protein) as Potential New Biomarkers of Bovine Tuberculosis

Author: Jiang Yitong, Xiaoyu Guo, Jia Hong, Zhifang Zhang, Ming Li, Lichun Fang, Xin Ting, Xintao Gao, Weidong Lin, Zhu Hongfei, and Jiabo Ding
Subjects: Proteomics, 0301 basic medicine, Microbiology (medical), Proteome, 030106 microbiology, Enzyme-Linked Immunosorbent Assay, Sensitivity and Specificity, Clinical Veterinary Microbiology, 03 medical and health sciences, Tandem Mass Spectrometry, Animals, Interleukin 8, bovine tuberculosis, Mycobacterium bovis, IL-8, biology, Interleukin-8, C-reactive protein, Area under the curve, food and beverages, Reproducibility of Results, Blood Proteins, Prognosis, biology.organism_classification, Blood proteins, Molecular biology, C-Reactive Protein, 030104 developmental biology, biology.protein, biomarker, Biomarker (medicine), Cattle, CRP, Tuberculosis, Bovine, Nested polymerase chain reaction, Biomarkers, Chromatography, Liquid
Abstract: Bovine tuberculosis (bTB) is caused by Mycobacterium bovis. During the early stage of infection, greater than 15% of M. bovis-infected cattle shed mycobacteria through nasal secretions, which can be detected by nested PCR., Bovine tuberculosis (bTB) is caused by Mycobacterium bovis. During the early stage of infection, greater than 15% of M. bovis-infected cattle shed mycobacteria through nasal secretions, which can be detected by nested PCR. To compare the differences in the protein profiles of M. bovis-infected cattle that were nested PCR positive (bTBPCR-P) and M. bovis-infected cattle that were nested PCR negative (bTBPCR-N) and to screen for biomarkers that will facilitate the early and accurate detection of bTB, we investigated the protein expression profiles of serum and bovine purified protein derivative (PPD-B)-stimulated plasma among bTBPCR-P (n = 20), bTBPCR-N (n = 20), and uninfected cattle (NC; n = 20) by iTRAQ labeling coupled with two-dimensional liquid chromatography-tandem mass spectrometry (iTRAQ-2D LC-MS/MS). After comprehensive analysis, we selected 15 putative differentially expressed serum proteins and 15 plasma proteins for validation by parallel reaction monitoring (PRM) with the same cohort used in the iTRAQ analysis. Four serum and five PPD-B-stimulated proteins were confirmed in follow-up enzyme-linked immunosorbent assays. PPD-B-stimulated interleukin 8 (IL-8) displayed the potential to differentiate M. bovis-infected cattle from NC, with an area under the curve (AUC) value of 0.9662, while PPD-B-stimulated C-reactive protein (CRP) displayed the potential to differentiate bTBPCR-P from bTBPCR-N, with an AUC value of 1.00. Finally, double-blind testing with 244 cattle indicated that the PPD-B-stimulated IL-8 test exhibited good agreement with traditional tests (κ > 0.877) with a >90% relative sensitivity and a >98% relative specificity; the PPD-B-stimulated CRP test displayed good agreement with nested PCR (κ = 0.9117), with an observed 94% relative sensitivity and 97% relative specificity. Therefore, the PPD-B-stimulated IL-8 and CRP tests could be used to detect bTB and to differentiate bTBPCR-P from bTBPCR-N.
Published: 2019

30. Evaluation of an Indirect Enzyme-Linked Immunosorbent Assay Based on Recombinant Baculovirus-Expressed Rift Valley Fever Virus Nucleoprotein as the Diagnostic Antigen

Author: Bonto Faburay, Arss Secka, William C. Wilson, Barbara S. Drolet, Juergen A. Richt, and D. Scott McVey
Subjects: 0301 basic medicine, Microbiology (medical), Livestock, Rift Valley Fever, medicine.drug_class, Genetic Vectors, 030231 tropical medicine, Sheep Diseases, Enzyme-Linked Immunosorbent Assay, Biology, Antibodies, Viral, Monoclonal antibody, Sensitivity and Specificity, Clinical Veterinary Microbiology, law.invention, 03 medical and health sciences, 0302 clinical medicine, Plaque reduction neutralization test, Antigen, Neutralization Tests, law, medicine, Animals, Seroprevalence, Antigens, Viral, chemistry.chemical_classification, Antiserum, Sheep, Rift Valley fever virus, Virology, Recombinant Proteins, Nucleoprotein, Nucleoproteins, 030104 developmental biology, Enzyme, chemistry, Immunoglobulin G, Recombinant DNA, Baculoviridae
Abstract: The increasing risk of Rift Valley fever virus (RVFV) infection as a global veterinary and public health threat demands the development of safe and accurate diagnostic tests. The aim of this study was to assess the suitability of a baculovirus expression system to produce recombinant RVFV nucleoprotein (N) for use as serodiagnostic antigen in an indirect enzyme-linked immunosorbent assay (ELISA). The ability of the recombinant N antigen to detect RVFV antibody responses was evaluated in ELISA format using antisera from sheep and cattle experimentally infected with two genetically distinct wild-type RVFV strains and sera from indigenous sheep and goat populations exposed to natural RVFV field infection in The Gambia. The recombinant N exhibited specific reactivity with the N-specific monoclonal antibody and various hyperimmune serum samples from ruminants. The indirect ELISA detected N-specific antibody responses in animals with 100% sensitivity compared to the plaque reduction neutralization test (6 to 21 days postinfection) and with 97% and 100% specificity in sheep and cattle, respectively. There was a high level of correlation between the indirect N ELISA and the virus neutralization test for sheep sera (R2 = 0.75; 95% confidence interval [CI] = 0.73 to 0.92) and cattle sera (R2 = 0.80; 95% CI = 0.67 to 0.97); in addition, the N-specific ELISA detected RVFV seroprevalence levels of 26.1% and 54.3% in indigenous sheep and goats, respectively, in The Gambia. The high specificity and correlation with the virus neutralization test support the idea of the feasibility of using the recombinant baculovirus-expressed RVFV N-based indirect ELISA to assess RVFV seroprevalence in livestock in areas of endemicity and nonendemicity.
Published: 2019

31. Matrix-Assisted Laser Desorption Ionization–Time of Flight Mass Spectrometry Is a Superior Diagnostic Tool for the Identification and Differentiation of Mycoplasmas Isolated from Animals

Author: Joachim Spergser, Claudia Hess, Igor Loncaric, and Ana S. Ramírez
Subjects: 0301 basic medicine, Microbiology (medical), Veterinary Medicine, 040301 veterinary sciences, Parasitic Diseases, Animal, Vertebrate Animals, Matrix assisted laser desorption ionization time of flight, Computational biology, medicine.disease_cause, Mass spectrometry, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, medicine, Animals, Bacteriological Techniques, biology, 04 agricultural and veterinary sciences, Mycoplasma, Mycoplasmatales Infections, biology.organism_classification, Mycoplasmataceae, Acholeplasma, Matrix-assisted laser desorption/ionization, 030104 developmental biology, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Ureaplasma species, Identification (biology)
Abstract: In veterinary diagnostic laboratories, identification of mycoplasmas is achieved by demanding, cost-intensive, and time-consuming methods that rely on antigenic or genetic identification. Since matrix-assisted laser desorption ionization–time of flight mass spectrometry (MALDI-TOF MS) seems to represent a promising alternative to the currently practiced cumbersome diagnostics, we assessed its applicability for the identification of almost all mycoplasma species isolated from vertebrate animals so far. For generating main spectrum profiles (MSPs), the type strains of 98 Mycoplasma, 11 Acholeplasma, and 5 Ureaplasma species and, in the case of 69 species, 1 to 7 clinical isolates were used. To complete the database, 3 to 7 representatives of 23 undescribed Mycoplasma species isolated from livestock, companion animals, and wildlife were also analyzed. A large in-house library containing 530 MSPs was generated, and the diversity of spectra within a species was assessed by constructing dendrograms based on a similarity matrix. All strains of a given species formed cohesive clusters clearly distinct from all other species. In addition, phylogenetically closely related species also clustered closely but were separated accurately, indicating that the established database was highly robust, reproducible, and reliable. Further validation of the in-house mycoplasma library using 335 independent clinical isolates of 32 mycoplasma species confirmed the robustness of the established database by achieving reliable species identification with log scores of ≥1.80. In summary, MALDI-TOF MS proved to be an excellent method for the identification and differentiation of animal mycoplasmas, combining convenience, ease, speed, precision, and low running costs. Furthermore, this method is a powerful and supportive tool for the taxonomic resolution of animal mycoplasmas.
Published: 2019

32. Pathotyping the Zoonotic Pathogen Streptococcus suis: Novel Genetic Markers To Differentiate Invasive Disease-Associated Isolates from Non-Disease-Associated Isolates from England and Wales

Author: Wileman, TM, Weinert, LA, Howell, KJ, Wang, J, Peters, SE, Williamson, SM, Wells, JM, Langford, PR, Rycroft, AN, Wren, BW, Maskell, DJ, Tucker, AW, Bosse, JT, Li, Y, Cuccui, J, Terra, VS, Beddow, J, Maglennon, GA, Chaudhuri, RR, Howell, Kate J [0000-0001-8069-920X], Apollo - University of Cambridge Repository, and Biotechnology and Biological Sciences Research Council
Subjects: pathotyping, Streptococcus suis, Swine, Palatine Tonsil, Disease, Virulence markers, BACTERIAL PATHOGENS, Clinical Veterinary Microbiology, PIGS, 11 Medical and Health Sciences, Swine Diseases, 0303 health sciences, Surveillance, Virulence, virulence markers, England, Molecular Diagnostic Techniques, Carrier State, surveillance, LATEST DEVELOPMENTS, Life Sciences & Biomedicine, Microbiology (medical), Genetic Markers, Biology, Microbiology, molecular diagnostics, 03 medical and health sciences, 07 Agricultural and Veterinary Sciences, Streptococcal Infections, Multiplex polymerase chain reaction, Molecular diagnostics, THIOL-ACTIVATED HEMOLYSIN, Animals, Host-Microbe Interactomics, 030304 developmental biology, VLAG, Science & Technology, Wales, IDENTIFICATION, 030306 microbiology, CAPSULAR TYPES, STRAINS, 06 Biological Sciences, biology.organism_classification, Carriage, Genetic marker, WIAS, EXTRACELLULAR PROTEIN, Pathotyping, Asymptomatic carrier, MURAMIDASE-RELEASED PROTEIN, Multiplex Polymerase Chain Reaction, Genome, Bacterial
Abstract: Streptococcus suis is one of the most important zoonotic bacterial pathogens of pigs, causing significant economic losses to the global swine industry. S. suis is also a very successful colonizer of mucosal surfaces, and commensal strains can be found in almost all pig populations worldwide, making detection of the S. suis species in asymptomatic carrier herds of little practical value in predicting the likelihood of future clinical relevance., Streptococcus suis is one of the most important zoonotic bacterial pathogens of pigs, causing significant economic losses to the global swine industry. S. suis is also a very successful colonizer of mucosal surfaces, and commensal strains can be found in almost all pig populations worldwide, making detection of the S. suis species in asymptomatic carrier herds of little practical value in predicting the likelihood of future clinical relevance. The value of future molecular tools for surveillance and preventative health management lies in the detection of strains that genetically have increased potential to cause disease in presently healthy animals. Here we describe the use of genome-wide association studies to identify genetic markers associated with the observed clinical phenotypes (i) invasive disease and (ii) asymptomatic carriage on the palatine tonsils of pigs on UK farms. Subsequently, we designed a multiplex PCR to target three genetic markers that differentiated 115 S. suis isolates into disease-associated and non-disease-associated groups, that performed with a sensitivity of 0.91, a specificity of 0.79, a negative predictive value of 0.91, and a positive predictive value of 0.79 in comparison to observed clinical phenotypes. We describe evaluation of our pathotyping tool, using an out-of-sample collection of 50 previously uncharacterized S. suis isolates, in comparison to existing methods used to characterize and subtype S. suis isolates. In doing so, we show our pathotyping approach to be a competitive method to characterize S. suis isolates recovered from pigs on UK farms and one that can easily be updated to incorporate global strain collections.
Published: 2019

33. Serotype and Genotype (Multilocus Sequence Type) of Streptococcus suis Isolates from the United States Serve as Predictors of Pathotype

Author: Douglas Marthaler, Stephanie Rossow, April A. Estrada, Aaron Rendahl, Connie J. Gebhart, and Marcelo Gottschalk
Subjects: 0301 basic medicine, Microbiology (medical), Serotype, Genotype, Streptococcus suis, Swine, 030106 microbiology, multilocus sequence typing, Serogroup, Clinical Veterinary Microbiology, 03 medical and health sciences, Streptococcal Infections, Clinical information, medicine, Endocarditis, Animals, Sequence (medicine), Genetics, Swine Diseases, biology, pathotype, pathogenic, Sequence types, medicine.disease, biology.organism_classification, bacterial infections and mycoses, porcine, serotyping, 030104 developmental biology, North America, Multilocus sequence typing, MLST
Abstract: Streptococcus suis is a significant cause of mortality in piglets and growing pigs worldwide. The species contains pathogenic and commensal strains, with pathogenic strains causing meningitis, arthritis, endocarditis, polyserositis, and septicemia. Serotyping and multilocus sequence typing (MLST) are primary methods to differentiate strains, but the information is limited for strains found in the United States., Streptococcus suis is a significant cause of mortality in piglets and growing pigs worldwide. The species contains pathogenic and commensal strains, with pathogenic strains causing meningitis, arthritis, endocarditis, polyserositis, and septicemia. Serotyping and multilocus sequence typing (MLST) are primary methods to differentiate strains, but the information is limited for strains found in the United States. The objective of this study was to characterize the diversity of 208 S. suis isolates collected between 2014 and 2017 across North America (mainly the United States) by serotyping and MLST and to investigate associations between subtype and pathotype classifications (pathogenic, possibly opportunistic, and commensal), based on clinical information and site of isolation. Twenty serotypes were identified, and the predominant serotypes were 1/2 and 7. Fifty-eight sequence types (STs) were identified, and the predominant ST was ST28. Associations among serotypes, STs, and pathotypes were investigated using odds ratio and clustering analyses. Evaluation of serotype and ST with pathotype identified a majority of isolates of serotypes 1, 1/2, 2, 7, 14, and 23 and ST1, ST13, ST25, ST28, ST29, ST94, ST108, ST117, ST225, ST373, ST961, and ST977 as associated with the pathogenic pathotype. Serotypes 21 and 31, ST750, and ST821 were associated with the commensal pathotype, which is composed of isolates from farms with no known history of S. suis-associated disease. Our study demonstrates the use of serotyping and MLST to differentiate pathogenic from commensal isolates and establish links between pathotype and subtype, thus increasing the knowledge about S. suis strains circulating in the United States.
Published: 2019

34. Test Agreement among Biochemical Methods, Matrix-Assisted Laser Desorption Ionization–Time of Flight Mass Spectrometry, and 16S rRNA Sequencing for Identification of Microorganisms Isolated from Bovine Milk

Author: G. Goodell, David J. Wilson, Pamela R.F. Adkins, and John R. Middleton
Subjects: 0301 basic medicine, Microbiology (medical), Microorganism, 030106 microbiology, Biology, medicine.disease_cause, Clinical Veterinary Microbiology, Agar plate, 03 medical and health sciences, RNA, Ribosomal, 16S, medicine, Animals, Prospective Studies, Food science, Udder, Mastitis, Bovine, Bacteria, food and beverages, Bacterial Infections, biology.organism_classification, medicine.disease, 16S ribosomal RNA, Bacterial Typing Techniques, Mastitis, RNA, Bacterial, Matrix-assisted laser desorption/ionization, Milk, 030104 developmental biology, medicine.anatomical_structure, Staphylococcus aureus, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Cattle, Female
Abstract: The objective of this prospective study was a blinded comparison of three methods for the identification of bacteria isolated on Columbia blood agar from milk samples of dairy cows. Basic biochemical testing, matrix-assisted laser desorption ionization–time of flight mass spectrometry (MALDI-TOF MS), and 16S rRNA partial genome sequence analysis were compared for bacterial identification to the genus or species level. Milk samples submitted from a commercial dairy farm from recently calved cows or clinical mastitis cases were cultured, and 181 isolates were identified by biochemical testing, MALDI-TOF MS, and 16S rRNA sequence analysis (179 isolates; 2 isolates could not be recovered from storage). For Staphylococcus aureus and Escherichia coli, agreement was determined at the species level. For other microbes, agreement was determined at the genus level or at the group level for streptococcus-like organisms. The positive agreement among all 3 diagnostic methods was 94%, with 95% to 98% between each pair of methods. The overall (including negative agreement) agreement among all 3 methods ranged from 97% to 100%. MALDI-TOF MS is becoming more commonplace for the genus- and/or species-level identification of bacteria isolated from milk samples and, in some laboratories, has replaced conventional biochemical methods. The results of the present study suggest that when identifying pathogens at the genus or group level, conventional culture followed up with either secondary biochemical testing or MALDI-TOF MS is of practical value. For purposes of milk quality and udder health monitoring or research, any of the 3 methods is a valuable tool for genus-level identification of bacteria isolated from dairy cow milk.
Published: 2019

35. Detection and Differentiation of Two Koala Gammaherpesviruses by Use of High-Resolution Melt (HRM) Analysis Reveals Differences in Viral Prevalence and Clinical Associations in a Large Study of Free-Ranging Koalas

Author: Joanne M. Devlin, Alistair R. Legione, Paola K. Vaz, and Carol A. Hartley
Subjects: 0301 basic medicine, Microbiology (medical), Male, 040301 veterinary sciences, Physiology, Animals, Wild, Polymerase Chain Reaction, High Resolution Melt, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, Gammaherpesvirinae, Phascolarctos cinereus, Risk Factors, biology.animal, Chlamydia pecorum, medicine, Prevalence, Animals, Clinical significance, Phascolarctidae, Molecular Epidemiology, Chlamydia, biology, Molecular epidemiology, Australia, Genetic Variation, 04 agricultural and veterinary sciences, Herpesviridae Infections, biology.organism_classification, medicine.disease, 030104 developmental biology, Molecular Diagnostic Techniques, Koala retrovirus, Female
Abstract: The iconic koala (Phascolarctos cinereus) is host to two divergent gammaherpesviruses, phascolarctid gammaherpesviruses 1 and 2 (PhaHV-1 and -2), but the clinical significance of the individual viruses is unknown and current diagnostic methods are unsuitable for differentiating between the viruses in large-scale studies. To address this, we modified a pan-herpesvirus nested PCR to incorporate high-resolution melt analysis. We applied this assay in a molecular epidemiological study of 810 koalas from disparate populations across Victoria, Australia, including isolated island populations. Animal and clinical data recorded at sampling were analyzed and compared to infection status. Between populations, the prevalence of PhaHV-1 and -2 varied significantly, ranging from 1% to 55%. Adult and older animals were 5 to 13 times more likely to be positive for PhaHV-1 than juveniles (P < 0.001), whereas PhaHV-2 detection did not change with age, suggesting differences in how these two viruses are acquired over the life of the animal. PhaHV-1 detection was uniquely associated with the detection of koala retrovirus, particularly in females (P = 0.008). Both viruses were significantly associated (P < 0.05) with the presence of genital tract abnormalities (uterine/ovarian cysts and testicular malformation), reduced fertility in females, urinary incontinence, and detection of Chlamydia pecorum, although the strength of these associations varied by sex and virus. Understanding the clinical significance of these viruses and how they interact with other pathogens will inform future management of threatened koala populations.
Published: 2019

36. Accurate Detection of Avian Respiratory Viruses by Use of Multiplex PCR-Based Luminex Suspension Microarray Assay

Author: Abdeljelil Ghram, Issam Hmila, Pia Fällgren, Mikael Leijon, Nacira Laamiri, Jaouher Ben Ali, Siamak Zohari, Laboratoire d’Epidémiologie et de Microbiologie Vétérinaire (LR11IPT03), Institut Pasteur de Tunis, Réseau International des Instituts Pasteur (RIIP)-Réseau International des Instituts Pasteur (RIIP), Université de Carthage - University of Carthage, Statens Veterinarmedicinska Anstalt (SVA), Ecole Nationale Supérieure d'ingénieurs de Tunis (ENSIT), Université de Tunis, This work was supported by the Institut Pasteur de Tunis (LEMV project), the Ministry of Higher Education and Scientific Research (Tunisia), and by the National Veterinary Institute (SVA), Uppsala, Sweden., and We thank Hechmi Louzir, the head of the Institut Pasteur de Tunis, for his constant encouragements and Walter Fuchs (Friedrich Loeffler Institute, Greifswald Insel Riems, Germany) for providing the A489 ILTV strain. We extend many thanks to the supervisors and technician staff who provided laboratory assistance and helpful suggestions and advices.
Subjects: 0301 basic medicine, Microbiology (medical), Median Fluorescence Intensity, Microarray, viruses, 030106 microbiology, Biology, Sensitivity and Specificity, Newcastle disease, Virus, MESH: Bird Diseases, Clinical Veterinary Microbiology, Birds, MESH: Viruses, 03 medical and health sciences, MESH: Reverse Transcriptase Polymerase Chain Reaction, Multiplex polymerase chain reaction, Animals, Multiplex, MESH: Animals, Respiratory system, Respiratory Tract Infections, MESH: Multiplex Polymerase Chain Reaction, Bird Diseases, Reverse Transcriptase Polymerase Chain Reaction, Reproducibility of Results, Microarray Analysis, biology.organism_classification, Virology, Molecular biology, MESH: Sensitivity and Specificity, 3. Good health, Reverse transcription polymerase chain reaction, MESH: Reproducibility of Results, MESH: Virus Diseases, MESH: Microarray Analysis, [SDV.MP]Life Sciences [q-bio]/Microbiology and Parasitology, Virus Diseases, Viruses, MESH: Birds, MESH: Respiratory Tract Infections, Multiplex Polymerase Chain Reaction
Abstract: A novel oligonucleotide suspension microarray (Luminex microsphere system) was developed for the rapid detection of avian respiratory viruses of major clinical importance. This test was optimized and validated with 70 clinical samples. The developed tool was accurate for high-throughput detection and differentiation of the most important avian respiratory viruses: avian influenza virus (AIV), Newcastle disease virus (NDV), infection bronchitis virus (IBV), and infectious laryngotracheitis virus (ILTV) in single- and mixed-virus infections. A multiplex reverse transcriptase PCR (RT-PCR), followed by a monoplex or a multiplex Luminex assays, were realized using a Luminex 200 analyzer instrument. The sensitivity, specificity, and reproducibility of the multiplex DNA suspension microarray system were evaluated. The results showed no significant differences in the median fluorescence intensity (MFI) value in monoplex and multiplex Luminex assays. The sensitivity and specificity proved to be completely concordant with monoplex real-time RT-PCR. We demonstrated that the multiplex DNA suspension microarray system is an accurate, high-throughput, and relatively simple method for the rapid detection of the main respiratory viruses of poultry.
Published: 2016
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37. Serological and Molecular Detection of Senecavirus A Associated with an Outbreak of Swine Idiopathic Vesicular Disease and Neonatal Mortality

Author: Pablo Piñeyro, Daniel Linhares, Marisa L. Rotolo, Christopher Rademacher, David H. Baum, Luis G. Giménez-Lirola, Yaxuan Sun, Jeffrey J. Zimmerman, and Karen M. Harmon
Subjects: Serum, 0301 basic medicine, Microbiology (medical), Swine, Palatine Tonsil, Enzyme-Linked Immunosorbent Assay, Picornaviridae, Real-Time Polymerase Chain Reaction, Virus, Clinical Veterinary Microbiology, Disease Outbreaks, Serology, Feces, 03 medical and health sciences, Swine Vesicular Disease, Animals, Medicine, Serologic Tests, Longitudinal Studies, Seroconversion, Swine vesicular disease, biology, Reverse Transcriptase Polymerase Chain Reaction, business.industry, Outbreak, Virology, 030104 developmental biology, Molecular Diagnostic Techniques, Immunoglobulin G, Immunology, Herd, biology.protein, Antibody, business
Abstract: We performed a longitudinal field study in a swine breeding herd that presented with an outbreak of vesicular disease (VD) that was associated with an increase in neonatal mortality. Initially, a USDA Foreign Animal Disease (FAD) investigation confirmed the presence of Senecavirus A (SVA) and ruled out the presence of exotic agents that produce vesicular lesions, e.g., foot-and-mouth disease virus and others. Subsequently, serum samples, tonsil swabs, and feces were collected from sows ( n = 22) and their piglets ( n = 33) beginning 1 week after the onset of the clinical outbreak and weekly for 6 weeks. The presence of SVA RNA was evaluated in all specimens collected by reverse transcriptase quantitative PCR (RT-qPCR) targeting a conserved region of the 5′ untranslated region (5′-UTR). The serological response (IgG) to SVA was evaluated by the weekly testing of sow and piglet serum samples on a SVA VP1 recombinant protein (rVP1) indirect enzyme-linked immunosorbent assay (ELISA). The rVP1 ELISA detected seroconversion against SVA in clinically affected and non-clinically affected sows at early stages of the outbreak as well as maternal SVA antibodies in offspring. Overall, the absence of vesicles (gross lesions) in SVA-infected animals and the variability of RT-qPCR results among specimen type demonstrated that a diagnostic algorithm based on the combination of clinical observations, RT-qPCR in multiple diagnostic specimens, and serology are essential to ensure an accurate diagnosis of SVA.
Published: 2016

38. Antimicrobial Susceptibility Patterns of Brachyspira Species Isolated from Swine Herds in the United States

Author: Nandita S. Mirajkar, Peter R. Davies, and Connie J. Gebhart
Subjects: 0301 basic medicine, Microbiology (medical), Brachyspira, Veterinary medicine, Swine, 040301 veterinary sciences, animal diseases, 030106 microbiology, Tiamulin, Brachyspira pilosicoli, Microbial Sensitivity Tests, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, chemistry.chemical_compound, Antibiotic resistance, Drug Resistance, Bacterial, medicine, Animals, Carbadox, Swine Diseases, biology, Broth microdilution, 04 agricultural and veterinary sciences, Valnemulin, biology.organism_classification, United States, Anti-Bacterial Agents, chemistry, Brachyspira hyodysenteriae, Gram-Negative Bacterial Infections, medicine.drug
Abstract: Outbreaks of swine dysentery, caused by Brachyspira hyodysenteriae and the recently discovered “ Brachyspira hampsonii ,” have reoccurred in North American swine herds since the late 2000s. Additionally, multiple Brachyspira species have been increasingly isolated by North American diagnostic laboratories. In Europe, the reliance on antimicrobial therapy for control of swine dysentery has been followed by reports of antimicrobial resistance over time. The objectives of our study were to determine the antimicrobial susceptibility trends of four Brachyspira species originating from U.S. swine herds and to investigate their associations with the bacterial species, genotypes, and epidemiological origins of the isolates. We evaluated the susceptibility of B. hyodysenteriae , B. hampsonii , Brachyspira pilosicoli , and Brachyspira murdochii to tiamulin, valnemulin, doxycycline, lincomycin, and tylosin by broth microdilution and that to carbadox by agar dilution. In general, Brachyspira species showed high susceptibility to tiamulin, valnemulin, and carbadox, heterogeneous susceptibility to doxycycline, and low susceptibility to lincomycin and tylosin. A trend of decreasing antimicrobial susceptibility by species was observed ( B. hampsonii > B. hyodysenteriae > B. murdochii > B. pilosicoli ). In general, Brachyspira isolates from the United States were more susceptible to these antimicrobials than were isolates from other countries. Decreased antimicrobial susceptibility was associated with the genotype, stage of production, and production system from which the isolate originated, which highlights the roles of biosecurity and husbandry in disease prevention and control. Finally, this study also highlights the urgent need for Clinical and Laboratory Standards Institute-approved clinical breakpoints for Brachyspira species, to facilitate informed therapeutic and control strategies.
Published: 2016

39. Analysis of Humoral Immune Responses to Surface and Virulence-Associated Chlamydiaabortus Proteins in Ovine and Human Abortions by Use of a Newly Developed Line Immunoassay

Author: Katharina Boden, David Longbottom, Andreas Essig, Konrad Sachse, Julia Maile, Ulrike Simnacher, Erwin Soutschek, Juergen Benjamin Hagemann, Morag Livingstone, and Gernot Walder
Subjects: 0301 basic medicine, Microbiology (medical), Virulence Factors, 030106 microbiology, Sheep Diseases, Chlamydiae, Virulence, Abortion, Septic, Clinical Veterinary Microbiology, 03 medical and health sciences, Immune system, Bacterial Proteins, Antigen, Pregnancy, medicine, Animals, Humans, Chlamydia, Immunoassay, Antigens, Bacterial, Sheep, medicine.diagnostic_test, biology, Chlamydia Infections, medicine.disease, biology.organism_classification, Antibodies, Bacterial, Virology, 030104 developmental biology, biology.protein, Female, Antibody, Bacteria
Abstract: The obligate intracellular bacterium Chlamydia abortus is the causative agent of enzootic abortion of ewes and poses a significant zoonotic risk for pregnant women. Using proteomic analysis and gene expression library screening in a previous project, we identified potential virulence factors and candidates for serodiagnosis, of which nine were scrutinized here with a strip immunoassay. We have shown that aborting sheep exhibited a strong antibody response to surface (MOMP, MIP, Pmp13G) and virulence-associated (CPAF, TARP, SINC) antigens. While the latter disappeared within 18 weeks following abortion in a majority of the animals, antibodies to surface proteins persisted beyond the duration of the study. In contrast, nonaborting experimentally infected sheep developed mainly antibodies to surface antigens (MOMP, MIP, Pmp13G), all of which did not persist. We were also able to detect antibodies to these surface antigens in C . abortus -infected women who had undergone septic abortion, whereas a group of shepherds and veterinarians with occupational exposure to C . abortus -infected sheep revealed only sporadic immune responses to the antigens selected. The most specific antigen for the serodiagnosis of human C . abortus infections was Pmp13G, which showed no cross-reactivity with other chlamydiae infecting humans. We suggest that Pmp13G-based serodiagnosis accomplished by the detection of antibodies to virulence-associated antigens such as CPAF, TARP, and SINC may improve the laboratory diagnosis of human and animal C . abortus infections.
Published: 2016

40. Comparison of Culture-Based Methods for Identification of Colonization with Methicillin-Resistant and Methicillin-Susceptible Staphylococcus aureus in the Context of Cocolonization

Author: Irving Nachamkin, Daniel O. Morris, Patrick A. Baron, Warren B. Bilker, Meghan F. Davis, Shelley C. Rankin, Baofeng Hu, Valerie Cluzet, Jacqueline M Ferguson, Karen C. Carroll, Ebbing Lautenbach, and Pam Tolomeo
Subjects: 0301 basic medicine, Microbiology (medical), Staphylococcus aureus, food.ingredient, 030106 microbiology, Context (language use), Biology, Staphylococcal infections, medicine.disease_cause, Clinical Veterinary Microbiology, Microbiology, 03 medical and health sciences, food, medicine, Humans, Mass Screening, Agar, Colonization, Mass screening, Bacteriological Techniques, Staphylococcal Infections, bacterial infections and mycoses, equipment and supplies, medicine.disease, Culture Media, Carrier State, Methicillin Resistance, Methicillin Susceptible Staphylococcus Aureus, Staphylococcus
Abstract: Two screening methods to detect staphylococcal colonization in humans were compared. Direct plating to CHROMagar (BD Diagnostics) was compared to a broth preenrichment followed by plating to Baird-Parker agar. The broth-enrichment method was comparable to CHROMagar for methicillin-resistant Staphylococcus aureas (MRSA) detection, but the enrichment method was optimum for recovery of coagulase-positive Staphylococcus spp.
Published: 2016

41. Detection of the Emerging Picornavirus Senecavirus A in Pigs, Mice, and Houseflies

Author: Scott Dee, Rejane Schaefer, Bryan Myers, Diego G. Diel, Travis Clement, Jane Christopher-Hennings, Eric A. Nelson, L. Caron, Joseph Yaros, Danielle Gava, Lok R. Joshi, Kristin A. Mohr, and Kyle S. Hain
Subjects: 0301 basic medicine, Microbiology (medical), Picornavirus, Swine, Picornaviridae, Disease, Real-Time Polymerase Chain Reaction, Virus, Disease Outbreaks, Clinical Veterinary Microbiology, Mice, 03 medical and health sciences, Swine Vesicular Disease, Houseflies, Environmental Microbiology, medicine, Animals, Housefly, biology, Reverse Transcriptase Polymerase Chain Reaction, Outbreak, biology.organism_classification, Virology, Small intestine, Reverse transcription polymerase chain reaction, 030104 developmental biology, medicine.anatomical_structure, Real-time polymerase chain reaction
Abstract: Senecavirus A (SVA) is an emerging picornavirus that has been recently associated with an increased number of outbreaks of vesicular disease and neonatal mortality in swine. Many aspects of SVA infection biology and epidemiology remain unknown. Here, we present a diagnostic investigation conducted in swine herds affected by vesicular disease and increased neonatal mortality. Clinical and environmental samples were collected from affected and unaffected herds and were screened for the presence of SVA by real-time reverse transcriptase PCR and virus isolation. Notably, SVA was detected and isolated from vesicular lesions and tissues of affected pigs, environmental samples, mouse feces, and mouse small intestine. SVA nucleic acid was also detected in houseflies collected from affected farms and from a farm with no history of vesicular disease. Detection of SVA in mice and housefly samples and recovery of viable virus from mouse feces and small intestine suggest that these pests may play a role on the epidemiology of SVA. These results provide important information that may allow the development of improved prevention and control strategies for SVA.
Published: 2016

42. Staphylococcus chromogenes, a Coagulase-Negative Staphylococcus Species That Can Clot Plasma

Author: Pedro Avellar-Costa, Kátia Regina Netto dos Santos, Marcia Giambiagi-deMarval, C. C. Lange, Maria Aparecida Vasconcelos Paiva Brito, and Danielle Cabral dos Santos
Subjects: Coagulase, 0301 basic medicine, Microbiology (medical), Staphylococcus, Staphylococcus chromogenes, medicine.disease_cause, Clinical Veterinary Microbiology, Microbiology, Plasma, 03 medical and health sciences, medicine, Animals, Staphylococcus species, Blood Coagulation, Mastitis, Bovine, Pathogen, biology, fungi, food and beverages, Plasma Metabolism, biology.organism_classification, medicine.disease, Mastitis, 030104 developmental biology, Staphylococcus aureus, Cattle
Abstract: Staphylococcus chromogenes is one of the main coagulase-negative staphylococci isolated from mastitis of dairy cows. We describe S. chromogenes isolates that can clot plasma. Since the main pathogen causing mastitis is coagulase-positive Staphylococcus aureus , the coagulase-positive phenotype of S. chromogenes described here can easily lead to misidentification.
Published: 2016

43. Seeded Amplification of Chronic Wasting Disease Prions in Nasal Brushings and Recto-anal Mucosa-Associated Lymphoid Tissues from Elk by Real-Time Quaking-Induced Conversion

Author: Ryan J. Monello, Byron Caughey, W. David Walter, Nicholas J. Haley, Margaret A. Wild, Laura L. Hoon-Hanks, Gordon Mitchell, Chris Siepker, Jenny G. Powers, Matteo Manca, Edward A. Hoover, and Jürgen A. Richt
Subjects: Male, 0301 basic medicine, Microbiology (medical), Pathology, medicine.medical_specialty, Time Factors, Lymphoid Tissue, Prions, 040301 veterinary sciences, animal diseases, Biopsy, Mucous membrane of nose, Biology, Sensitivity and Specificity, Clinical Veterinary Microbiology, 0403 veterinary science, 03 medical and health sciences, Intestinal mucosa, medicine, Animals, Intestinal Mucosa, Pathology, Molecular, Rocky Mountain elk, Transmissible spongiform encephalopathy, medicine.diagnostic_test, Diagnostic Tests, Routine, Ruminants, 04 agricultural and veterinary sciences, Chronic wasting disease, medicine.disease, biology.organism_classification, Nasal Mucosa, 030104 developmental biology, Lymphatic system, Wasting Disease, Chronic, Immunohistochemistry, Female
Abstract: Chronic wasting disease (CWD), a transmissible spongiform encephalopathy of cervids, was first documented nearly 50 years ago in Colorado and Wyoming and has since been detected across North America and the Republic of Korea. The expansion of this disease makes the development of sensitive diagnostic assays and antemortem sampling techniques crucial for the mitigation of its spread; this is especially true in cases of relocation/reintroduction or prevalence studies of large or protected herds, where depopulation may be contraindicated. This study evaluated the sensitivity of the real-time quaking-induced conversion (RT-QuIC) assay of recto-anal mucosa-associated lymphoid tissue (RAMALT) biopsy specimens and nasal brushings collected antemortem. These findings were compared to results of immunohistochemistry (IHC) analysis of ante- and postmortem samples. RAMALT samples were collected from populations of farmed and free-ranging Rocky Mountain elk ( Cervus elaphus nelsoni ; n = 323), and nasal brush samples were collected from a subpopulation of these animals ( n = 205). We hypothesized that the sensitivity of RT-QuIC would be comparable to that of IHC analysis of RAMALT and would correspond to that of IHC analysis of postmortem tissues. We found RAMALT sensitivity (77.3%) to be highly correlative between RT-QuIC and IHC analysis. Sensitivity was lower when testing nasal brushings (34%), though both RAMALT and nasal brush test sensitivities were dependent on both the PRNP genotype and disease progression determined by the obex score. These data suggest that RT-QuIC, like IHC analysis, is a relatively sensitive assay for detection of CWD prions in RAMALT biopsy specimens and, with further investigation, has potential for large-scale and rapid automated testing of antemortem samples for CWD.
Published: 2016

44. Development and Validation of an Improved PCR Method Using the 23S-5S Intergenic Spacer for Detection of Rickettsiae in Dermacentor variabilis Ticks and Tissue Samples from Humans and Laboratory Animals

Author: Loganathan Ponnusamy, Steven R. Meshnick, William L. Nicholson, Charles S. Apperson, Haley Sutton, and Madhavi L. Kakumanu
Subjects: 0301 basic medicine, Microbiology (medical), 030106 microbiology, Rickettsiaceae Infections, Polymerase Chain Reaction, Sensitivity and Specificity, Clinical Veterinary Microbiology, law.invention, 03 medical and health sciences, Nucleic acid thermodynamics, law, Animals, Laboratory, Animals, Humans, Dermacentor variabilis, Gene, Polymerase chain reaction, DNA Primers, Dermacentor, Rickettsieae, biology, RNA, Ribosomal, 5S, Nucleic Acid Hybridization, bacterial infections and mycoses, biology.organism_classification, Virology, Molecular biology, 3. Good health, Spotted fever, RNA, Ribosomal, 23S, genomic DNA, bacteria, DNA, Intergenic, Oligonucleotide Probes, Nested polymerase chain reaction
Abstract: A novel nested PCR assay was developed to detect Rickettsia spp. in ticks and tissue samples from humans and laboratory animals. Primers were designed for the nested run to amplify a variable region of the 23S-5S intergenic spacer (IGS) of Rickettsia spp. The newly designed primers were evaluated using genomic DNA from 11 Rickettsia species belonging to the spotted fever, typhus, and ancestral groups and, in parallel, compared to other Rickettsia -specific PCR targets ( ompA , gltA , and the 17-kDa protein gene). The new 23S-5S IGS nested PCR assay amplified all 11 Rickettsia spp., but the assays employing other PCR targets did not. The novel nested assay was sensitive enough to detect one copy of a cloned 23S-5S IGS fragment from “ Candidatus Rickettsia amblyommii.” Subsequently, the detection efficiency of the 23S-5S IGS nested assay was compared to those of the other three assays using genomic DNA extracted from 40 adult Dermacentor variabilis ticks. The nested 23S-5S IGS assay detected Rickettsia DNA in 45% of the ticks, while the amplification rates of the other three assays ranged between 5 and 20%. The novel PCR assay was validated using clinical samples from humans and laboratory animals that were known to be infected with pathogenic species of Rickettsia . The nested 23S-5S IGS PCR assay was coupled with reverse line blot hybridization with species-specific probes for high-throughput detection and simultaneous identification of the species of Rickettsia in the ticks. “ Candidatus Rickettsia amblyommii,” R. montanensis , R. felis , and R. bellii were frequently identified species, along with some potentially novel Rickettsia strains that were closely related to R. bellii and R. conorii .
Published: 2016

45. Development of an Enzyme-Linked Immunosorbent Assay Based on Fusion VP2 332-452 Antigen for Detecting Antibodies against Aleutian Mink Disease Virus

Author: Liandong Qu, Yun Liu, Ming Liu, Cailing Song, Yun Zhang, Dafei Liu, and Xiaowei Chen
Subjects: 0301 basic medicine, Microbiology (medical), viruses, Aleutian Mink Disease, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, Clinical Veterinary Microbiology, law.invention, 03 medical and health sciences, Reference test, Antigen, law, Aleutian Mink Disease Virus, Animals, Humans, Medicine, Antigens, Viral, chemistry.chemical_classification, biology, business.industry, Virology, Recombinant Proteins, Blot, 030104 developmental biology, Enzyme, chemistry, Immunology, biology.protein, Recombinant DNA, Capsid Proteins, Antibody, business, Counterimmunoelectrophoresis
Abstract: For detection of Aleutian mink disease virus (AMDV) antibodies, an enzyme-linked immunosorbent assay (ELISA) was developed using the recombinant VP2 332-452 protein as an antigen. Counterimmunoelectrophoresis (CIEP) was used as a reference test to compare the results of the ELISA and Western blotting (WB); the specificity and sensitivity of the VP2 332-452 ELISA were 97.9% and 97.3%, respectively, which were higher than those of WB. Therefore, this VP2 332-452 ELISA may be a preferable method for detecting antibodies against AMDV.
Published: 2016

46. Changes in the Population of Methicillin-Resistant Staphylococcus pseudintermedius and Dissemination of Antimicrobial-Resistant Phenotypes in the Netherlands

Author: Duim, Birgitta, Verstappen, Koen M., Broens, Els M., Laarhoven, Laura M., Van Duijkeren, Engeline, Hordijk, Joost, De Heus, Phebe, Spaninks, Mirlin, Timmerman, Arjen J., Wagenaar, Jaap A., LS Klinisch Onderzoek Wagenaar, dI&I I&I-4, LS Klinisch Onderzoek Wagenaar, and dI&I I&I-4
Subjects: 0301 basic medicine, Microbiology (medical), Staphylococcus pseudintermedius, Genotype, Staphylococcus, 030106 microbiology, Population, Pyoderma, Microbial Sensitivity Tests, Biology, Staphylococcal infections, Clinical Veterinary Microbiology, 03 medical and health sciences, Dogs, Antibiotic resistance, medicine, Animals, Humans, Life Science, Dog Diseases, education, Alleles, Phylogeny, Netherlands, Retrospective Studies, Host Pathogen Interaction & Diagnostics, Genetics, education.field_of_study, Bacteriologie, Bacteriology, Bacteriology, Host Pathogen Interaction & Diagnostics, Staphylococcal Infections, medicine.disease, biology.organism_classification, Host Pathogen Interactie & Diagnostiek, Multiple drug resistance, Phenotype, Bacteriologie, Host Pathogen Interactie & Diagnostiek, Multilocus sequence typing, Methicillin Resistance, Multilocus Sequence Typing
Abstract: Methicillin-resistant Staphylococcus pseudintermedius (MRSP), which is often multidrug resistant (MDR), has recently emerged as a threat to canine health worldwide. Knowledge of the temporal distribution of specific MRSP lineages, their antimicrobial resistance phenotypes, and their association with clinical conditions may help us to understand the emergence and spread of MRSP in dogs. The aim of this study was to determine the yearly proportions of MRSP lineages and their antimicrobial-resistant phenotypes in the Netherlands and to examine possible associations with clinical conditions. MRSP was first isolated from a canine specimen submitted for diagnostics to the Faculty of Veterinary Medicine of Utrecht University in 2004. The annual cumulative incidence of MRSP among S. pseudintermedius increased from 0.9% in 2004 to 7% in 2013. MRSP was significantly associated with pyoderma and, to a lesser extent, with wound infections and otitis externa. Multilocus sequence typing (MLST) of 478 MRSP isolates yielded 39 sequence types (ST) belonging to 4 clonal complexes (CC) and 15 singletons. CC71 was the dominant lineage that emerged since 2004, and CC258, CC45, and several unlinked isolates became more frequent during the following years. All but two strains conferred an MDR phenotype, but strains belonging to CC258 or singletons were less resistant. In conclusion, our study showed that MDR CC71 emerged as the dominant lineage from 2004 and onward and that less-resistant lineages were partly replacing CC71.
Published: 2016

47. Characterization of Staphylococcus caprae Clinical Isolates Involved in Human Bone and Joint Infections, Compared with Goat Mastitis Isolates

Author: Guillaume Ghislain Aubin, Pascale Bémer, Stéphane Corvec, P. Nicollet, P. Mercier, and J. d'Ersu
Subjects: Adult, Male, 0301 basic medicine, Microbiology (medical), Staphylococcus, 030106 microbiology, Virulence, Mastitis, medicine.disease_cause, Staphylococcal infections, Polymerase Chain Reaction, Clinical Veterinary Microbiology, Microbiology, law.invention, Young Adult, 03 medical and health sciences, law, Staphylococcus epidermidis, Osteoarthritis, medicine, Pulsed-field gel electrophoresis, Animals, Humans, Polymerase chain reaction, Aged, Goat Diseases, biology, Goats, Sequence Analysis, DNA, Middle Aged, Staphylococcal Infections, biology.organism_classification, medicine.disease, Molecular Typing, Staphylococcus aureus, Biofilms, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Female, Staphylococcus caprae
Abstract: Staphylococcus caprae is an emerging microorganism in human bone and joint infections (BJI). The aim of this study is to describe the features of S. caprae isolates involved in BJI (H for human) compared with those of isolates recovered in goat mastitis (A for animal). Fourteen isolates of each origin were included. Identifications were performed using a Vitek 2 GP ID card, tuf gene sequencing, and matrix-assisted laser desorption ionization–time of flight (MALDI-TOF) Vitek MS. Molecular typing was carried out using pulsed-field gel electrophoresis (PFGE) and DiversiLab technology. The crystal violet method was used to determine biofilm-forming ability. Virulence factors were searched by PCR. Vitek MS technology provides an accurate identification for the two types of isolates compared to that of gold-standard sequencing (sensitivity, 96.4%), whereas the Vitek 2 GP ID card was more effective for H isolates. Molecular typing methods revealed two distinct lineages corresponding to the origin despite few overlaps: H and A. In our experimental conditions, no significant difference was observed in biofilm production ability between H and A isolates. Nine isolates (5 H isolates and 4 A isolates) behaved as weak producers while one A isolate was a strong producer. Concerning virulence factors, the autolysin atlC and the serine aspartate adhesin ( sdrZ ) genes were detected in 24 isolates (86%), whereas the lipase gene was always detected, except in one H isolate (96%). The ica operon was present in 23 isolates (82%). Fibrinogen-binding ( fbe ) or collagen-binding ( cna ) genes were not detected by using primers designed for Staphylococcus aureus or Staphylococcus epidermidis , even in low stringency conditions. Although S. caprae probably remains underestimated in human infections, further studies are needed to better understand the evolution and the adaptation of this species to its host.
Published: 2016

48. Characterization of Five Zoonotic Streptococcus suis Strains from Germany, Including One Isolate from a Recent Fatal Case of Streptococcal Toxic Shock-Like Syndrome in a Hunter

Author: Tobias Eisenberg, Khodr Tello, Peter Valentin-Weigand, Christoph Georg Baums, Christoph Hudemann, Hamid Hossain, Angela Hewer, Manfred Rohde, Dirk Bandorski, and Infectious Diseases, College of Veterinary Medicine, University Leipzig, Leipzig.
Subjects: Microbiology (medical), Genotype, Streptococcus suis, Human blood, biology, biology.organism_classification, Shock, Septic, Virology, Clinical Veterinary Microbiology, Microbiology, Proinflammatory cytokine, Germany, Streptococcal Infections, Shock (circulatory), medicine, Animals, Cytokines, Humans, medicine.symptom, STREPTOCOCCAL INFECTIONS, Ex vivo
Abstract: A Streptococcus suis isolate from a German hunter with streptococcal toxic shock-like syndrome (STSLS) and four additional zoonotic isolates were genotyped as mrp + epf * (variant 1890) sly + cps2 + . All five zoonotic German strains were characterized by high multiplication in human blood samples ex vivo , but induction of only low levels of proinflammatory cytokines compared to a Chinese STSLS strain.
Published: 2015

49. Direct Repeat Unit ( dru ) Typing of Methicillin-Resistant Staphylococcus pseudintermedius from Dogs and Cats

Author: Stefan Schwarz, Kristina Kadlec, Richard V. Goering, and J. Scott Weese
Subjects: Microbiology (medical), Meticillin, Staphylococcus pseudintermedius, Genotype, Staphylococcus, Cat Diseases, Staphylococcal infections, Polymerase Chain Reaction, Clinical Veterinary Microbiology, SmaI, Dogs, medicine, Pulsed-field gel electrophoresis, Animals, Dog Diseases, Typing, Repetitive Sequences, Nucleic Acid, Genetics, biology, Sequence Analysis, DNA, Staphylococcal Infections, medicine.disease, biology.organism_classification, Europe, Molecular Typing, North America, Cats, Multilocus sequence typing, Methicillin Resistance, medicine.drug
Abstract: Methicillin-resistant Staphylococcus pseudintermedius (MRSP) has emerged in a remarkable manner as an important problem in dogs and cats. However, limited molecular epidemiological information is available. The aims of this study were to apply direct repeat unit ( dru ) typing in a large collection of well-characterized MRSP isolates and to use dru typing to analyze a collection of previously uncharacterized MRSP isolates. Two collections of MRSP isolates from dogs and cats were included in this study. The first collection comprised 115 well-characterized MRSP isolates from North America and Europe. The data for these isolates included multilocus sequence typing (MLST) and staphylococcal protein A gene ( spa) typing results as well as SmaI macrorestriction patterns after pulsed-field gel electrophoresis (PFGE). The second collection was a convenience sample of 360 isolates from North America. The dru region was amplified by PCR, sequenced, and analyzed. For the first collection, the discriminatory indices of the typing methods were calculated. All isolates were successfully dru typed. The discriminatory power for dru typing ( D = 0.423) was comparable to that of spa typing ( D = 0.445) and of MLST ( D = 0.417) in the first collection. Occasionally, dru typing was able to further discriminate between isolates that shared the same spa type. Among all 475 isolates, 26 different dru types were identified, with 2 predominant types (dt9a and dt11a) among 349 (73.4%) isolates. The results of this study underline that dru typing is a useful tool for MRSP typing, being an objective, standardized, sequence-based method that is relatively cost-efficient and easy to perform.
Published: 2015

50. Development of a Multiplex PCR Assay for Rapid Molecular Serotyping of Haemophilus parasuis

Author: Kate J, Howell, Sarah E, Peters, Jinhong, Wang, Juan, Hernandez-Garcia, Lucy A, Weinert, Shi-Lu, Luan, Roy R, Chaudhuri, Øystein, Angen, Virginia, Aragon, Susanna M, Williamson, Julian, Parkhill, Paul R, Langford, Andrew N, Rycroft, Brendan W, Wren, Duncan J, Maskell, Alexander W, Tucker, and Vanessa S, Terra
Subjects: Microbiology (medical), Bacterial capsule, Serotype, Haemophilus Infections, Time Factors, Genotyping Techniques, Swine, Locus (genetics), Sensitivity and Specificity, Clinical Veterinary Microbiology, Microbiology, Haemophilus parasuis, Genetic variation, Haemophilus, Multiplex polymerase chain reaction, Animals, Serotyping, Bacterial Capsules, Swine Diseases, biology, Pasteurellaceae, biology.organism_classification, Virology, genomic DNA, Genetic Loci, Multiplex Polymerase Chain Reaction
Abstract: Haemophilus parasuis causes Glässer's disease and pneumonia in pigs. Indirect hemagglutination (IHA) is typically used to serotype this bacterium, distinguishing 15 serovars with some nontypeable isolates. The capsule loci of the 15 reference strains have been annotated, and significant genetic variation was identified between serovars, with the exception of serovars 5 and 12. A capsule locus and in silico serovar were identified for all but two nontypeable isolates in our collection of >200 isolates. Here, we describe the development of a multiplex PCR, based on variation within the capsule loci of the 15 serovars of H. parasuis , for rapid molecular serotyping. The multiplex PCR (mPCR) distinguished between all previously described serovars except 5 and 12, which were detected by the same pair of primers. The detection limit of the mPCR was 4.29 × 10 5 ng/μl bacterial genomic DNA, and high specificity was indicated by the absence of reactivity against closely related commensal Pasteurellaceae and other bacterial pathogens of pigs. A subset of 150 isolates from a previously sequenced H. parasuis collection was used to validate the mPCR with 100% accuracy compared to the in silico results. In addition, the two in silico -nontypeable isolates were typeable using the mPCR. A further 84 isolates were analyzed by mPCR and compared to the IHA serotyping results with 90% concordance (excluding those that were nontypeable by IHA). The mPCR was faster, more sensitive, and more specific than IHA, enabling the differentiation of 14 of the 15 serovars of H. parasuis .
Published: 2015

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