Your search keyword '"Serotyping veterinary"' showing total 904 results

1. Research progress into the principles and methods underlying capsular typing of Glaesserella parasuis.

Author

Zhu Y, Guan L, Zhang J, Xue Y, and Zhao Z

Subjects

Animals, Bacterial Capsules genetics, Hemagglutination Tests veterinary, Immunodiffusion veterinary, Swine, Haemophilus Infections diagnosis, Haemophilus Infections microbiology, Haemophilus Infections veterinary, Haemophilus parasuis genetics, Haemophilus parasuis classification, Polymerase Chain Reaction veterinary, Serotyping veterinary, Serotyping methods, Swine Diseases diagnosis, Swine Diseases microbiology

Abstract

Glaesserella parasuis (GPS) is an important bacterial pathogen of swine. Serotype identification has presented a bottleneck in GPS research since it was first identified as the pathogen causing Glässer's disease in pigs in 1910. This paper presents a systematic review of the history of the development and application of gel immunodiffusion (GID), indirect hemagglutination assay (IHA), and polymerase chain reaction (PCR) typing methods for GPS, and the discovery of their shared antigenic basis. It provides a systematic theoretical overview of the immunology and principles underlying the three typing methods and offers new ideas for research into the prevention and control of Glässer's disease. In 1992, GPS was first classified into serotypes 1-15 using GID based on GPS heat-stable antigens, but about 25% of the strains were found to be non-typeable, and the composition of their antigens for serotyping was unclear. In 2003, the IHA method was established based on saline-extracted antigens of GPS, whose sensitivity and typing rate were higher than for GID, although about 15% of strains were still found to be non-typeable. The results of IHA and GID typing are roughly consistent, since they share the same GPS surface polysaccharide serotyping antigens, although whether these are capsular polysaccharides, lipopolysaccharides, or other polysaccharides, remains to be determined. In 2013, the Capsular polysaccharide (CPS) synthetic gene clusters from GPS serotypes 1-15 were successfully analyzed, confirming that CPS is essential for the formation of antigens for serotyping. In 2015, primers were designed based on the specific target genes of GPS capsules to establish a PCR typing method (H-PCR) for GPS, which, however, could not identify serotypes 5 and 12. In 2017, a new PCR typing method (J-PCR) was established based on the specific target genes of GPS capsules, which could identify serotypes 5 and 12. A combination of the two PCR typing methods enables the typing of almost all GPS strains, and the consistency with GID and IHA was verified using molecular biological methods. The antigenic basis of the three typing methods was shown to involve the GPS capsule. PCR typing methods are characterized by simple operation, fast speed, and low cost, and can successfully solve many problems in GID and IHA serotyping, and so have become widely adopted., (© 2024. The Author(s).)

Published

2024

2. Characterization of Tenacibaculum maritimum isolated from diseased salmonids farmed in Chile reveals high serological and genetic heterogeneity.

Author

Avendaño-Herrera R, Lopez P, Echeverría-Bugueño M, Araya-León H, and Irgang R

Subjects

Animals, Chile epidemiology, Genetic Variation, Serotyping veterinary, Genetic Heterogeneity, Aquaculture, Fish Diseases microbiology, Tenacibaculum genetics, Tenacibaculum isolation & purification, Flavobacteriaceae Infections veterinary, Flavobacteriaceae Infections microbiology, Salmo salar, Oncorhynchus mykiss microbiology

Abstract

The diversity of Tenacibaculum maritimum in Chile remains poorly understood, particularly in terms of antigenic and genetic diversity. This information is crucial for the future development of a vaccine against tenacibaculosis and would increase understanding of this important fish pathogen. With this aim, the biochemical, antigenic, and genetic characteristics were analysed for 14 T. maritimum isolates, recovered from diseased Atlantic salmon (Salmo salar) and rainbow trout (Oncorhynchus mykiss) farmed in Chile between 1998 and 2022. Biochemical analysis showed a homogeneity among all the Chilean T. maritimum isolates and all four other strains included for comparison purposes. Serological characterization using dot-blot assaying revealed antigenic heterogeneity with the use of unabsorbed antisera. The majority of isolates showed cross-reactions, identifying three main serological patterns. When the PCR-based serotyping scheme was performed, the existence of antigenic heterogeneity was confirmed. Four Atlantic salmon isolates were 4-0; and most isolates, including the rainbow trout isolate, were 3-1 (n = 9). A turbot (Scophthalmus maximus) isolate was 1-0. Using an existing Multilocus Sequence Typing system, two newly identified sequence types (ST193 and ST198) in the database were detected. ST193 encompassed nine isolates obtained from Atlantic salmon and rainbow trout, while ST198 regrouped four isolates, all retrieved from diseased Atlantic salmon in 2022. These findings highlight significant antigenic and genetic diversity among the Chilean isolates. This information is useful for epizootiology and the selection of suitable candidate strain(s) for vaccine development against tenacibaculosis caused by T. maritimum in Chilean salmon farming., (© 2024 John Wiley & Sons Ltd.)

Published

2024

3. Salmonella carriage and change in serovar distribution in broiler giblets at slaughterhouse level in Turkiye: first report using ISO 6579-1:2017 and ISO 6579-3:2014.

Author

Akgun Z, Coskun AG, Cetin E, Temelli S, and Eyigor A

Subjects

Animals, Prevalence, Real-Time Polymerase Chain Reaction veterinary, Salmonella isolation & purification, Salmonella genetics, Gizzard, Avian microbiology, Serotyping veterinary, Carrier State veterinary, Carrier State microbiology, Salmonella typhimurium isolation & purification, Salmonella typhimurium genetics, Salmonella enteritidis isolation & purification, Salmonella enteritidis genetics, Chickens, Abattoirs, Salmonella Infections, Animal microbiology, Salmonella Infections, Animal epidemiology, Poultry Diseases microbiology, Poultry Diseases epidemiology, Serogroup

Abstract

This study aimed to determine the prevalence and serovar distribution of salmonellae in liver, heart, and spleen (LHS) and gizzard (G) of slaughtered broilers. For this, a total of 60 sample units, comprised of 30 LHS and 30 G collected from 3 slaughterhouses, were analysed by reference methods for detection and serotyping as revised ISO 6579-1:2017 and ISO 6579-3:2014, respectively. Also, Salmonella-specific real-time PCR (Salm-PCR) was used for species confirmation, while Salmonella Enteritidis (S. Enteritidis) and Salmonella Typhimurium (S. Typhimurium) specific real-time PCR (SE/ST-PCR) was evaluated to determine its efficiency for rapid detection of the serovars mandated in current legal regulations compared to standard serotyping. All LHS (100%-30/30) and 90% (27/30) of G samples harbored Salmonella with an overall prevalence of 95% (57/60) in samples examined, where all isolates were confirmed as Salmonella by Salm-PCR. The most prevalent serovar in broiler giblets was S. Virchow (80.70%-46/57) followed by S. Enteritidis (19.30%-11/57). SE/ST-PCR (%17.54-10/57) could not detect one G isolate, which was serotyped as S. Enteritidis by standard serotyping. High relative accuracy (98.25%), sensitivity (100%) and specificity (100%), and agreement between methods (κ: 0.94) verified SE/ST-PCR's potential to be used as an alternative in rapid detection of S. Enteritidis and S. Typhimurium. Data on high Salmonella prevalence in broiler giblets of slaughterhouse origin, and detection of the pathogen by the implementation of all requirements indicated in the revised ISO 6579-1:2017 standard method, enabling the determination of actual prevalence in the samples with high sensitivity and specificity is of significance for public health. Additionally, identification of S. Virchow as the dominant serovar followed by S. Enteritidis with a relatively lower prevalence, and absence of S. Typhimurium in broiler giblets are important findings for Turkiye. This up to date data, obtained by strict application of ISO 6579-3:2014 procedures, indicated a shift in circulating serovars in the broiler industry. The objective findings in this study would bring awareness to national/international literature, and may be of use in future improvements in legal regulations., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

4. Molecular characterization of Escherichia coli isolates recovered from broilers with cellulitis.

Author

Müller A, Schulze Bernd K, Seinige D, Braun AS, Kumm F, and Kehrenberg C

Subjects

Animals, Germany, Phylogeny, Drug Resistance, Bacterial, Genotype, Anti-Bacterial Agents pharmacology, Electrophoresis, Gel, Pulsed-Field veterinary, Serotyping veterinary, Chickens microbiology, Poultry Diseases microbiology, Cellulitis veterinary, Cellulitis microbiology, Escherichia coli Infections veterinary, Escherichia coli Infections microbiology, Escherichia coli genetics, Escherichia coli isolation & purification, Escherichia coli drug effects

Abstract

Avian cellulitis in broilers, caused by avian pathogenic Escherichia coli, is a major cause for carcass rejections during meat inspection, resulting in significant economic losses. In this study, we analysed E. coli isolates obtained from broiler chickens affected by cellulitis for their genetic relatedness and antimicrobial resistance phenotype and genotype. The objective was to determine whether there is a clonal spread or whether these clinical isolates differ. For this purpose, E. coli was isolated from swab samples collected from diseased broilers across 77 poultry farms in Germany, resulting in 107 isolates. These isolates were subjected to serotyping, PCR-based phylotyping and macrorestriction analysis with subsequent pulsed-field gel-electrophoresis for typing purposes. In addition, the presence of virulence genes associated with avian pathogenic E. coli (APEC) was investigated by PCR. Antimicrobial susceptibility of the isolates was examined by the disk diffusion method according to CLSI guidelines and subsequently, the presence of corresponding resistance genes was investigated by PCR. Typing results revealed that a significant proportion of the isolates belonged to serotype O78:K80, which is one of the major APEC serotypes. Phylogenetic grouping showed that phylogenetic group D was most commonly represented (n = 49). Macrorestriction analysis showed overall heterogenous results, however, some clustering of closely related isolates was observed. The level of antimicrobial resistance was high, with 83.8% of isolates non-susceptible to at least one class of antimicrobial agents and 40% of isolates showing resistance to at least three classes. The most frequently observed resistance was to ampicillin, mediated by bla TEM (n = 56). However, few isolates were non-susceptible to ciprofloxacin (n = 8) and none of the isolates was resistant to 3rd generation cephalosporins or carbapenems. Overall, the results show that genetically diverse APEC associated with avian cellulitis can be found among and within German poultry farms. While most isolates were antimicrobial resistant, resistance levels to high(est) priority critically important antimicrobials were low., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

5. High Salmonella load with serovar virchow dominance pose major public safety risk in postchill broiler carcasses.

Author

Demircioglu A, Coskun AG, Kanar TS, Eyigor A, and Temelli S

Subjects

Animals, Meat microbiology, Food Handling methods, Bacterial Load veterinary, Cold Temperature, Real-Time Polymerase Chain Reaction veterinary, Serotyping veterinary, Chickens microbiology, Salmonella isolation & purification, Serogroup, Food Microbiology

Abstract

The objective of this study was to determine Salmonella contamination levels, presence and serovar distribution in broiler carcasses before and after chilling, as well as to evaluate the effectiveness of chilling process. A total of 96 pooled neck skin samples (PNSS) of 48 prechill (PreC) and 48 postchill (PosC) carcasses, representing 480 broilers collected in 6 mo' period were analyzed using ISO 6579-2:2012 Miniaturized Most Probable Number (ISO-mMPN) technique. Species confirmation and serovar identification was performed by Salmonella-specific real-time PCR (Salm-PCR) and conventional serotyping, respectively. Mean Salmonella count was 1.84 log 10 MPN/g in PreC, and 1.48 log 10 MPN/g in PosC samples, indicating a statistically significant reduction of 0.36 log 10 MPN/g (p < 0.05) in the counts by plant's air chill system. Salmonella positivity reduced from 97.9% (47/48) in PreC to 85.42% (41/48) in PosC samples, confirmed by Salm-PCR with identified serovars as S. Virchow (89.77 %) followed by S. Schwarzengrund (9.09%) and S. Bredeney (1.14%). Persistence of high load and prevalence of Salmonella with serovar Virchow dominance (other than the ones mandated in current guidelines) in the final product contributes significant and up to date data to relevant literature, and provides unbiased epidemiological reference to legal authorities for future relevant revisions., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2024

6. Serotype diversity and antimicrobial susceptibility profiles of Actinobacillus pleuropneumoniae isolated in Italian pig farms from 2015 to 2022.

Author

Guarneri F, Romeo C, Scali F, Zoppi S, Formenti N, Maisano AM, Catania S, Gottschalk M, and Alborali GL

Subjects

Swine, Animals, Serogroup, Microbial Sensitivity Tests veterinary, Enrofloxacin, Farms, Retrospective Studies, Anti-Bacterial Agents pharmacology, Sulfamethoxazole pharmacology, Trimethoprim pharmacology, Italy epidemiology, Serotyping veterinary, Actinobacillus pleuropneumoniae, Pleuropneumonia epidemiology, Pleuropneumonia veterinary, Pleuropneumonia microbiology, Swine Diseases epidemiology, Swine Diseases microbiology, Actinobacillus Infections epidemiology, Actinobacillus Infections veterinary, Actinobacillus Infections microbiology, Thiamphenicol analogs & derivatives

Abstract

Actinobacillus pleuropneumoniae (APP) is a bacterium frequently associated with porcine pleuropneumonia. The acute form of the disease is highly contagious and often fatal, resulting in significant economic losses for pig farmers. Serotype diversity and antimicrobial resistance (AMR) of APP strains circulating in north Italian farms from 2015 to 2022 were evaluated retrospectively to investigate APP epidemiology in the area. A total of 572 strains isolated from outbreaks occurring in 337 different swine farms were analysed. The majority of isolates belonged to serotypes 9/11 (39.2%) and 2 (28.1%) and serotype diversity increased during the study period, up to nine different serotypes isolated in 2022. The most common resistances were against tetracycline (53% of isolates) and ampicillin (33%), followed by enrofloxacin, florfenicol and trimethoprim/sulfamethoxazole (23% each). Multidrug resistance (MDR) was common, with a third of isolates showing resistance to more than three antimicrobial classes. Resistance to the different classes and MDR varied significantly depending on the serotype. In particular, the widespread serotype 9/11 was strongly associated with florfenicol and enrofloxacin resistance and showed the highest proportion of MDR isolates. Serotype 5, although less common, showed instead a concerning proportion of trimethoprim/sulfamethoxazole resistance. Our results highlight how the typing of circulating serotypes and the analysis of their antimicrobial susceptibility profile are crucial to effectively manage APP infection and improve antimicrobial stewardship., (© 2024. The Author(s).)

Published

2024

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

Author

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

Subjects

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

Abstract

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

Published

2024

8. Shiga toxin-producing Escherichia coli isolated from hunted wild boar (Sus scrofa) in Switzerland.

Author

Nüesch-Inderbinen M, Barmettler K, Stevens MJA, and Cernela N

Subjects

Animals, Humans, Swine, Switzerland epidemiology, Serotyping veterinary, Animals, Wild, Shiga Toxin genetics, Sus scrofa, Shiga-Toxigenic Escherichia coli genetics, Escherichia coli Proteins genetics, Escherichia coli Infections epidemiology, Escherichia coli Infections veterinary, Swine Diseases epidemiology

Abstract

Introduction: Shiga toxin-producing Escherichia (E.) coli (STEC) are zoonotic foodborne pathogens of significant public health importance. While ruminants are considered the main reservoir, wild animals are increasingly acknowledged as carriers and potential reservoirs of STEC. The aim of this study was to determine the occurrence of STEC in a total of 59 faecal samples of hunted wild boars (Sus scrofa) from two different regions in Switzerland (canton Thurgau in northern Switzerland and canton Ticino in southern Switzerland), and to characterise the isolates using a whole genome sequencing approach. After an enrichment step, Shiga-toxin encoding genes (stx) were detected by real-time PCR in 41 % (95 % confidence interval (95 %CI) 0,29 - 0,53) of the samples, and STEC were subsequently recovered from 22 % (95 %CI 0,13 - 0,34) of the same samples. Seven different serotypes and six different sequence types (STs) were found, with O146:H28 ST738 (n = 4) and O100:H20 ST2514 (n = 4) predominating. Subtyping of stx identified isolates with stx1c/stx2b (n = 1), stx2a (n = 1), stx2b (n = 6), and stx2e (n = 6). No isolate contained the eae gene, but all harboured additional virulence genes, most commonly astA (n = 10), hlyE (n = 9), and hra (n = 9). STEC O11:H5, O21:H21, and O146:H28 harboured virulence factors associated with extra-intestinal pathogenic E. coli (ExPEC), and STEC O100:H20 and O155:H26 possessed sta1 and/or stb and were STEC/enterotoxigenic E. coli (ETEC) hybrid pathotypes. Our results show that wild boars are carriers of STEC which may be distributed in the environment, possibly leading to the contamination of agricultural crops and water sources. The serogroups included STEC O146 which belongs to the most common non-O157 serogroups associated with human illness in Europe, with implications for public health. Since Stx2e-producing STEC have frequently been reported in swine and pork, STEC O100:H20 harbouring stx2e in faeces of wild boars may be relevant to free-range systems of pig farming because of the potential risk of transmission events at the wildlife-livestock interface.

Published

2024

9. Molecular identification and characterisation of Mannheimia haemolytica.

Author

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

Subjects

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

Abstract

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

Published

2024

10. Molecular characterization of the HMTp210 gene of Avibacterium paragallinarum and the proposition of a new genotyping method as alternative for classical serotyping.

Author

Buter R, Feberwee A, de Wit S, Heuvelink A, da Silva A, Gallardo R, Soriano Vargas E, Swanepoel S, Jung A, Tödte M, and Dijkman R

Subjects

Animals, Serotyping veterinary, Genotype, Phylogeny, Chickens, Haemophilus Infections veterinary, Haemophilus Infections microbiology, Haemophilus paragallinarum genetics, Poultry Diseases microbiology

Abstract

Avibacterium paragallinarum (A. paragallinarum) is the aetiological agent of infectious coryza (IC) in chickens and characterized by acute respiratory distress and severe drop in egg production. Vaccination is important in the control of IC outbreaks and the efficacy of vaccination is dependent on A. paragallinarum serovars included in the vaccine. Classical serotyping of A. paragallinarum is laborious and hampered by poor availability of antigens and antisera. The haemagglutinin, important in classical serotyping, is encoded by the HMTp210 gene. HMTp210 gene analysis has been shown to have potential as alternative to classical serotyping. The aim of the present study was to further investigate the potential of sequence analyses of partial region 1 of the HMTp210 gene, the HMTp210 hypervariable region and the concatenated sequences of both fragments. For this analysis, 123 HMTp210 gene sequences (field isolates, A. paragallinarum serovar reference strains and vaccine strains) were included. Evaluation of serovar references and vaccine strains revealed a need for critical evaluation, especially within Page serovar B and C. Phylogenetic analysis of HMTp210 region 1 resulted in a separation of Page serovar A, B and C strains. Analysis of the HMTp210 HVR alone was not sufficient to discriminate all nine different Kume serovar references. The concatenated sequences of HMTp210 region 1 and HMTp210 HVR resulted in 14 clusters with a high correlation with Page serovar and with the nine currently known Kume serovars and is therefore proposed as a novel genotyping method that could be used as an alternative for classical serotyping of A. paragallinarum .

Published

2023

11. Molecular characterization of Glaesserella parasuis strains circulating in North American swine production systems.

Author

Mugabi R, Silva APSP, Hu X, Gottschalk M, Aragon V, Macedo NR, Sahin O, Harms P, Main R, Tucker AW, Li G, and Clavijo MJ

Subjects

Animals, Swine, Multilocus Sequence Typing veterinary, Phylogeny, Serogroup, Serotyping veterinary, North America, Haemophilus parasuis genetics

Abstract

Background: Glaesserella parasuis is the causative agent of Glässer's disease in pigs. Serotyping is the most common method used to type G. parasuis isolates. However, the high number of non-typables (NT) and low discriminatory power make serotyping problematic. In this study, 218 field clinical isolates and 15 G. parasuis reference strains were whole-genome sequenced (WGS). Multilocus sequence types (MLST), serotypes, core-genome phylogeny, antimicrobial resistance (AMR) genes, and putative virulence gene information was extracted., Results: In silico WGS serotyping identified 11 of 15 serotypes. The most frequently detected serotypes were 7, 13, 4, and 2. MLST identified 72 sequence types (STs), of which 66 were novel. The most predominant ST was ST454. Core-genome phylogeny depicted 3 primary lineages (LI, LII, and LIII), with LIIIA sublineage isolates lacking all vtaA genes, based on the structure of the phylogenetic tree and the number of virulence genes. At least one group 1 vtaA virulence genes were observed in most isolates (97.2%), except for serotype 8 (ST299 and ST406), 15 (ST408 and ST552) and NT (ST448). A few group 1 vtaA genes were significantly associated with certain serotypes or STs. The putative virulence gene lsgB, was detected in 8.3% of the isolates which were predominantly of serotype 5/12. While most isolates carried the bcr, ksgA, and bacA genes, the following antimicrobial resistant genes were detected in lower frequency;  blaZ (6.9%), tetM (3.7%), spc (3.7%), tetB (2.8%), bla-ROB-1 (1.8%), ermA (1.8%), strA (1.4%), qnrB (0.5%), and aph3''Ia (0.5%).   CONCLUSION: This study showed the use of WGS to type G. parasuis isolates and can be considered an alternative to the more labor-intensive and traditional serotyping and standard MLST. Core-genome phylogeny provided the best strain discrimination. These findings will lead to a better understanding of the molecular epidemiology and virulence in G. parasuis that can be applied to the future development of diagnostic tools, autogenous vaccines, evaluation of antibiotic use, prevention, and disease control., (© 2023. BioMed Central Ltd., part of Springer Nature.)

Published

2023

12. Phenotypic and genotypic characterization of Listeria monocytogenes in clinical ruminant cases in Korea.

Author

Kim J, Kim JW, and Kim HY

Subjects

Cattle, Animals, Humans, Virulence genetics, Ruminants, Serotyping veterinary, Goats, Republic of Korea epidemiology, Food Microbiology, Electrophoresis, Gel, Pulsed-Field veterinary, Listeria monocytogenes, Listeriosis epidemiology, Listeriosis veterinary, Cattle Diseases epidemiology, Goat Diseases

Abstract

Listeria monocytogenes, a foodborne human and veterinary pathogen, is associated with high mortality rates in ruminants. However, no studies have investigated the antimicrobial resistance of L. monocytogenes isolates from clinical ruminant cases. This study aimed to determine the phenotypic and genotypic characteristics of L. monocytogenes isolates from clinical cases of Korean ruminants. We collected 24 L. monocytogenes isolates from aborted bovine fetuses and goats presenting with listeriosis-related symptoms. The isolates were subjected to PCR serogrouping, conventional serotyping, virulence gene detection, and antimicrobial susceptibility testing. Furthermore, pulsed-field gel electrophoresis and multilocus sequence typing were used to classify and compare genetic diversity among the isolates, including human L. monocytogenes isolates. The most prevalent L. monocytogenes serotypes were 4b (Ⅳ b ), 1/2a (Ⅱ a ; Ⅱ c ), and 1/2b (Ⅱ b ). All isolates harbored the virulence genes; however, llsX-encoding listeriolysin were identified only in serotypes 4b and 1/2b. All isolates, including two found in humans, formed three genetically diverse pulsed-field gel electrophoresis clusters according to serotype, lineage, and sequence type. The most prevalent sequence type was ST1, followed by ST365 and ST91. The isolates from ruminants with listeriosis were resistant to oxacillin and ceftriaxone and showed diverse lineage, serotype (serogroup), and sequence type characteristics. Considering that the atypical sequence types exhibited clinical manifestations and histopathological lesions, further study is needed to elucidate the pathogenicity of genetically diverse ruminant L. monocytogenes isolates. Furthermore, continuous monitoring of antimicrobial resistance is required to prevent the emergence of L. monocytogenes strains resistant to common antimicrobials., Competing Interests: Competing interests The authors declare that they have no competing interests., (Copyright © 2023 Elsevier B.V. All rights reserved.)

Published

2023

13. Novel pan-lineage VP1 specific degenerate primers for precise genetic characterization of serotype O foot and mouth disease virus circulating in India.

Author

Khulape SA, Biswal JK, Jana C, Subramaniam S, and Singh RP

Subjects

Animals, Serogroup, Serotyping veterinary, Genetic Heterogeneity, Foot-and-Mouth Disease Virus genetics, Foot-and-Mouth Disease epidemiology

Abstract

Analysis of the VP1 gene sequence of the foot and mouth disease virus (FMDV) is critical to understanding viral evolution and disease epidemiology. A standard set of primers have been used for the detection and sequence analysis of the VP1 gene of FMDV directly from suspected clinical samples with limited success. The study validated VP1-specific degenerate primer-based reverse transcription polymerase chain reaction (RT-PCR) for the qualitative detection and sequencing of serotype O FMDV lineages circulating in India. The novel degenerate primer-based RT-PCR amplifying the VP1 gene can circumvent the genetic heterogeneity observed in viruses after cell culture adaptation and facilitate precise viral gene sequence analysis from clinical samples., Competing Interests: The authors declare no conflicts of interest., (© 2023 The Korean Society of Veterinary Science.)

Published

2023

14. Molecular analysis of enteropathogenic Escherichia coli (EPEC) isolates from healthy food-producing animals and humans with diarrhoea.

Author

Beraldo LG, Borges CA, Maluta RP, Cardozo MV, and de Ávila FA

Subjects

Humans, Animals, Swine, Sheep, Adhesins, Bacterial genetics, Diarrhea veterinary, Serotyping veterinary, Enteropathogenic Escherichia coli genetics, Escherichia coli Infections epidemiology, Escherichia coli Infections veterinary, Escherichia coli Proteins genetics, Sheep Diseases, Swine Diseases

Abstract

Enteropathogenic Escherichia coli (EPEC) is a pathogen associated with acute diarrhoea in humans. To determine whether EPEC isolated from healthy food-producing animals possesses the same virulence gene repertoire as EPEC isolated from human with diarrhoea, we compared six typical EPEC (tEPEC) and 20 atypical EPEC (aEPEC) from humans with diarrhoea and 42 aEPEC from healthy animals (swine, sheep and buffaloes), using pulsed-field gel electrophoresis (PFGE), virulence markers, serotyping and subtyping of eae and tir genes. We found that human and animal isolates shared virulence genes, including nleB, nleE and nleF, which were associated with human diarrhoea. Serogroups and serotypes identified in isolates of food-producing animals such as O26:H11, O128:H2, O76:H7, O103, O108, O111 and O145, have previously been implicated in human disease. The subtypes eae and tir were also shared between human and animal isolates, being eae-γ1 and eae-β1 the most prevalent in both groups, while the most common tir subtypes were α and β. Despite PFGE analysis demonstrating that EPEC strains are heterogeneous and there was no prevalent clone identified, EPEC isolated from humans and food-producing animals shared some characteristics, such as virulence genes associated with human diarrhoea, indicating that food-producing animals could play a role as reservoirs for those genes., (© 2022 Wiley-VCH GmbH.)

Published

2023

15. Characterization of an atypical Actinobacillus pleuropneumoniae serovar 2 isolate with a rough-type lipopolysaccharide.

Author

To H, Akaike Y, Kon M, Koike F, Shibuya K, Sasakawa C, and Nagai S

Subjects

Swine, Animals, Lipopolysaccharides, Serogroup, Polysaccharides, Serotyping veterinary, Actinobacillus pleuropneumoniae genetics, Actinobacillus Infections veterinary, Swine Diseases

Abstract

We describe phenotypic and genetic characterization of an atypical Japanese Actinobacillus pleuropneumoniae isolate OT761. Nucleotide sequence analysis revealed that gene clusters involved in capsular polysaccharide and O-polysaccharide (O-PS) biosynthesis of the isolate were nearly identical to those of serovar 2 reference strain. The main difference found between the O-PS loci is the shortening of 31 amino acids from the C terminus of WcaJ in the atypical isolate due to a 93 bp deletion at the 3' end of wcaJ gene. Immunoblot analysis revealed that this isolate could not produce O-PS. Taken together, our results showed that the C-terminal domain of the A. pleuropneumoniae WcaJ plays a critical role in enzyme function of WcaJ involved in the biosynthesis of O-PS.

Published

2023

16. Using genetic markers for detection and subtyping of the emerging Salmonella enterica subspecies enterica serotype Muenchen.

Author

Arnold K, Lim S, Rakler T, Rovira A, Satuchne C, Yechezkel E, Wiseman A, Pima Y, Yakunin E, Rokney A, and Elnekave E

Subjects

Humans, Animals, Serogroup, Genetic Markers, Chickens, Salmonella, Serotyping veterinary, Poultry, Salmonella enterica

Abstract

Non-typhoidal Salmonella (NTS) poses a global threat to public health. Poultry, one of the main reservoirs of NTS, is usually not clinically affected by most NTS, yet the economic losses to the poultry industry due to control and mitigation efforts, and due to negative publicity can be tremendous. NTS strains are routinely characterized into serotypes in a time-consuming, labor-intensive multistep process that requires skilled personnel. Moreover, the discriminatory power of serotyping is limited compared to other subtyping methods. Whole-genome sequence data enable the identification of genetic variation within serotypes. However, sequencing is often limited by available resources, and analyzing and interpreting the genetic data may be time-consuming. Source tracing during epidemiological outbreak investigations requires rapid and efficient characterization of strains to control pathogen spread. Here we designed a multiplex polymerase chain reaction (PCR) assay for the detection of genetic variants of Salmonella Muenchen, a serotype that has emerged in Israel in the last 3 yr in both clinical human cases and different hosts. Test sensitivity of 99.21% and specificity of 94 to 100% were determined using in-silico PCR with a dataset of 18,282 NTS assemblies from 37 NTS serotypes. Similarly, test sensitivity of 100% and specificity of 96.2 to 100% were determined in-vitro with 120 NTS isolates of 52 serotypes. Moreover, the test enabled differentiation between the common sequence types of serotype Muenchen using both approaches. As opposed to traditional serotyping and other subtyping methods, the designed test allows for rapid and cost-efficient detection of the emerging S. Muenchen serotype and its variants in a single step. Future development of similar assays for other dominant serotypes may help reduce the time and cost required for detection and initial characterization of dominant NTS strains. Overall, these tests will be beneficial to both public health and for reducing of the economic losses to the poultry industry due to NTS infections., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

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

Author

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

Subjects

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

Abstract

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

Published

2022

18. Enhanced detection and serotyping of foot-and-mouth disease virus serotype O, A, and Asia1 using a novel multiplex real-time RT-PCR.

Author

Lim DR, Ryoo S, Kang H, Oh SH, Jang SH, Kang B, Park HJ, Hwang H, Kim JM, Park CK, and Cha SH

Subjects

Animals, DNA Primers, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sensitivity and Specificity, Serogroup, Serotyping veterinary, Foot-and-Mouth Disease diagnosis, Foot-and-Mouth Disease epidemiology, Foot-and-Mouth Disease Virus

Abstract

Rapid and accurate detection and serotyping of foot-and-mouth disease (FMD) virus (FMDV) is essential for implementing control policies against emergent FMD outbreaks. Current serotyping assays, such as VP1 reverse transcription-polymerase chain reaction (RT-PCR)/sequencing (VP1 RT-PCR/sequencing) and antigen detection enzyme-linked immunosorbent assay (ELISA), have problems with increasing serotyping failure of FMDVs from FMD outbreaks. This study was conducted to develop a multiplex real-time RT-PCR for specific detection and differential serotyping of FMDV serotype O, A, and Asia 1 directly from field clinical samples. Primers and probes were designed based on 571 VP1 coding region sequences originated from seven pools. Multiplex real-time RT-PCR using these primers and probes demonstrated serotype-specific detection with enhanced sensitivity compared to VP1 RT-PCR/sequencing for reference FMDV (n = 24). Complete serotyping conformity between the developed multiplex real-time RT-PCR and previous VP1 RT-PCR/sequencing was demonstrated using FMDV field viruses (n = 113) prepared in cell culture. For FMDV field clinical samples (n = 55), the serotyping rates of multiplex real-time RT-PCR and VP1 RT-PCR/sequencing were 92.7% (51/55) and 72.7% (40/55), respectively. Moreover, the developed multiplex real-time RT-PCR demonstrated improved FMDV detection (up to 33.3%) and serotyping (up to 67.7%) capabilities for saliva samples when compared with 3D real-time RT-PCR and VP1 RT-PCR/sequencing, during 10 days of challenge infection with FMDV serotype O, A, and Asia 1. Collectively, this study suggests that the newly developed multiplex real-time RT-PCR assay may be useful for the detection and differential serotyping of FMDV serotype O, A, and Asia 1 in the field., (© 2022 The Authors. Transboundary and Emerging Diseases published by Wiley-VCH GmbH.)

Published

2022

19. Characterisation and epidemiological subtyping of Shiga toxin-producing Escherichia coli isolated from the beef production chain in Gauteng, South Africa.

Author

Onyeka LO, Adesiyun AA, Keddy KH, Hassim A, Smith AM, and Thompson PN

Subjects

Abattoirs, Animals, Cattle, Electrophoresis, Gel, Pulsed-Field veterinary, Serotyping veterinary, South Africa epidemiology, Cattle Diseases epidemiology, Escherichia coli Infections epidemiology, Escherichia coli Infections veterinary, Shiga-Toxigenic Escherichia coli genetics

Abstract

In South Africa, there is a shortage of epidemiologic data on Shiga toxin-producing Escherichia coli (STEC) in the beef production chain. This study was conducted to characterise STEC isolates originating from three studies conducted in a cattle feedlot, beef abattoirs and retail outlets in Gauteng province, South Africa. Polymerase chain reaction was used to detect virulence genes, the Epsilometer test to assess antimicrobial susceptibility, pulsed-field gel electrophoresis (PFGE) to investigate genetic relatedness of isolates, and conventional serotyping for phenotypic identification. Amongst the 86 STEC isolates, the eaeA gene was detected in 20 (23%), and 26 different serogroups were identified, including the clinically important O8, O174, O2, 020 and O117. The majority of the isolates (95%; 82/86) exhibited resistance to one or more antimicrobial agents, and 30 of the isolates (35%) exhibited multi-drug resistance (MDR), being resistant to at least three antimicrobial classes. The PFGE patterns showed a highly diverse but related STEC population, with 45 distinct patterns and evidence of horizontal transmission along the beef production chain. This is significant because it demonstrates continual environmental contamination and risk of contamination along the beef production chain and the food chain. To our knowledge, this is the first study that provides evidence of horizontal transmission of STEC along the beef production chain in South Africa. This epidemiological information could facilitate the development of a proactive strategy for reducing potential foodborne outbreaks and transmission of antimicrobial resistant pathogens in the food chain., (Copyright © 2022 Elsevier B.V. All rights reserved.)

Published

2022

20. Assessing Salmonella prevalence and complexity through processing using different culture methods.

Author

Rasamsetti S, Berrang ME, Cox NA, and Shariat NW

Subjects

Animals, Food Microbiology, Prevalence, Salmonella, Serotyping veterinary, Anti-Infective Agents, Chickens

Abstract

Conventional Salmonella surveillance requires a week for isolation, confirmation, and subsequent serotyping. We previously showed that this could be reduced by 24 h by combining the pre-enrichment and enrichment steps into a single selective pre-enrichment step and was tested on directly after picking. The goal of this study was 2-fold: 1) to evaluate the use of selective pre-enrichment through each step of processing, including postintervention when the Salmonella load is reduced, and 2) to assess any changes in serovar populations in Salmonella positive samples. Duplicate carcass drip samples, each representative of 500 broiler carcasses, were collected by catching processing water drip under moving carcass shackle lines in each of three commercial broiler slaughter plants. Samples were collected post-pick, post-inside-outside bird wash (IOBW), and post-chill; duplicate wing rinses were performed pre- and post-antimicrobial parts dip. Each processing plant was sampled 6 times for a total of 180 samples collected. The number of Salmonella positives identified with selective pre-enrichment conditions (48/180) was similar to traditional selective enrichment culture conditions (52/180), showed good concordance in recovery rate between the 2 culture methods (Fisher's exact test, P = 0.72). We also found that the incidence of Salmonella reduced dramatically after antimicrobial intervention (post-pick 66.7% vs. post chill 8.3%). When serovar populations were evaluated in Salmonella positive samples using CRISPR-SeroSeq, we detected four different Salmonella serovars, Kentucky, Infantis, Schwarzengrund, and Typhimurium, and their incidence rose between post-pick and post-IOBW. The relative abundance of Infantis within individual samples increased between post-pick and post-IOBW while the relative abundance of the other 3 serovars decreased. These results suggest that a selective pre-enrichment step reduces the time required for Salmonella isolation without negatively affecting detection and serovar profiles in culture positive samples were not altered between culture conditions used., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

21. Salmonella enterica subsp. enterica serotypes isolated for the first time in feral cats: The impact on public health.

Author

Rosario I, Calcines MI, Rodríguez-Ponce E, Déniz S, Real F, Vega S, Marin C, Padilla D, Martín JL, and Acosta-Hernández B

Subjects

Animals, Animals, Wild, Cats, Public Health, Salmonella, Serogroup, Serotyping veterinary, Cat Diseases epidemiology, Salmonella Infections, Animal epidemiology, Salmonella enterica

Abstract

Stray cat populations can represent a significant threat of the transmission of zoonotic diseases such as salmonellosis. The objective of this study was to assess Salmonella carriage by free-living cats in Gran Canaria island and the Salmonella serovars involved, in order to inform to those responsible for the colonies about the possible risk factors. One hundred rectal swabs of feral cats were taken. Salmonella strains were serotyped in accordance with Kauffman-White-Le-Minor technique. Of a total of 100 animals under study, 19% were found to be positive to Salmonella spp. This is the first report that described the zoonotic serovars S. Nima, S. Bredeney, S. Grancanaria and S. Kottbus in cats. The present study demonstrates that feral cats may represent a source of risk for the spread of different Salmonella zoonotic serovars. It has been reported that there is a certain correlation between Salmonella isolates from pets and wild animals. Further studies are needed from other animal species and environmental sources to make this correlation., (Copyright © 2022 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2022

22. Identification, serotyping, and antimicrobial susceptibility of Riemerella anatipestifer isolated from ducks in Vietnam.

Author

Vo TT, Dang VT, Le DH, and Nguyen TH

Subjects

Agar, Animals, Ducks microbiology, RNA, Ribosomal, 16S genetics, Riemerella, Serotyping veterinary, Vietnam, Anti-Infective Agents, Poultry Diseases, Sepsis veterinary

Abstract

Background: Septicemia caused by Riemerella anatipestifer ( R. anatipestifer ) is a serious problem in the duck industry worldwide, and it is currently one of the major concerns for duck farming in Vietnam.., Aim: This study was conducted to identify the causative agent of septicemia in ducks in Vietnam. The antimicrobial susceptibility and serotypes of R. anatipestifer isolates were also determined to provide valuable information for disease treatment and vaccine development., Methods: Riemerella anatipestifer was isolated using blood agar and chocolate agar media. The commercial API 20NE microtest system and the partial nucleotide sequence analysis of the 16s rRNA were used to identify R. anatipestifer strains. Serotypes were determined by slide agglutination test using standard antisera against R. anatipestifer . The disk diffusion method was utilized to investigate the antimicrobial susceptibility of R. anatipestifer isolated strains., Results: A total of 408 samples were collected from ducks with typical symptoms of septicemia for R. anatipestifer isolation. Sixty-nine R. anatipestifer strains were identified. Serotyping results showed that 30 out of 69 bacterial strains were classified as serotypes 1, 6, 8, 10, and 20, with serotype 10 being the most prevalent. The antimicrobial susceptibility test revealed that 100% of the bacterial isolates were susceptible to Amoxicillin/clavulanic acid and Imipenem. On the contrary, the majority of R. anatipestifer strains were resistant to Nalidixic acid (89.9%), Streptomycin (75.4%), and Norfloxacin (72.5%)., Conclusion: This is the first ever report in terms of identification, serotyping, and antimicrobial susceptibility tests of R. anatipestifer causing septicemia in ducks of Vietnam, providing useful scientific information for treatment as well as vaccine development to control the disease.

Published

2022

23. Molecular detection, biotyping and serotyping of Yersinia enterocolitica isolated from chicken livers in Tabriz.

Author

Hassanzadeh P, Ghasemzadeh Limoee E, and Nouri Gharajalar S

Subjects

Animals, Chickens, Liver, Serotyping veterinary, Yersinia Infections epidemiology, Yersinia Infections veterinary, Yersinia enterocolitica genetics

Abstract

Introduction and Purpose: Yersinia enterocolitica belongs to the family of Enterobacteriaceae and is a psychrophilic pathogen that is associated with foodborne infections. It usually causes gastroenteritis, mesenteric lymphadenitis, and septicemia. This study aimed to molecular detection, biotyping, and serotyping of Yersinia enterocolitica isolated from chicken livers in Tabriz., Materials and Methods: One hundred chicken liver samples were collected randomly from poultry slaughterhouses in Tabriz for three months. After enrichment process, the presence of Yersinia enterocolitica in studied samples was determined through culture-based methods, biochemical and molecular tests. Then the biotype and serotype of the isolates were determined., Results: 31 samples (31%) were positive for Yersinia enterocolitica by both phenotypic and molecular assays. Among positive samples, 25 (80.64%) had non-pathogenic biotype 1 A with serotype O: 5 (23 samples) and O: 8 (2 samples). 6 (19.36%) had biotype 1B and all of them had O: 3 serotype. The serotype Yersinia enterocolitica O: 9 was not found., Conclusion: the present study highlighted the significance of chicken liver as potential source of Yersinia enterocolitica infection in Tabriz city., (Copyright © 2022. Published by Elsevier Ltd.)

Published

2022

24. Characterization of Shiga toxin-producing Escherichia coli isolated from Cattle and Sheep in Xinjiang province, China, using whole-genome sequencing.

Author

Liu Y, Li H, Chen X, Tong P, Zhang Y, Zhu M, Su Z, Yao G, Li G, and Cai W

Subjects

Animals, Cattle, Serogroup, Serotyping veterinary, Sheep, Virulence genetics, Virulence Factors genetics, Cattle Diseases epidemiology, Escherichia coli Infections epidemiology, Escherichia coli Infections veterinary, Escherichia coli Proteins, Sheep Diseases epidemiology, Shiga-Toxigenic Escherichia coli genetics

Abstract

Shiga toxin-producing Escherichia coli (STEC) is an important food-borne pathogen capable of causing severe gastrointestinal diseases in humans. Cattle and sheep are the natural reservoir hosts of STEC strains. Previously, we isolated 56 STEC strains from anal and carcass swab samples of cattle and sheep in farms and slaughterhouses. In this study, we performed whole-genome sequencing of these isolates and determined their serotypes, virulence profiles, sequence types (STs) and genetic relationships. Our results showed that the 56 isolates belong to 20 different STs, 29 O:H serotypes and 8 stx subtype combinations. The highly prevalent serotypes for bovine and ovine isolates were O8:H25 and O87:H16, respectively. Five serotypes of cattle or sheep isolates are novel. The majority (63%) of cattle isolates contain stx1 + stx2, subtyped into stx1a, stx2a and stx2c. In contrast, most of the sheep isolates contain stx1 only, primarily subtyped into stx1a and stx1c. None of the isolates tested eae-positive, but virulence factors such as ehxA and espP were present with variable prevalence rates. The prevalence of saa (19.6%) and espP (12.5%) in cattle isolates is much higher than that in sheep isolates, whereas that of subA (34%), katP (14.3%) and ireA (28.6%) in sheep isolates is considerably higher than that in cattle isolates. Core-genome SNP analysis revealed that the majority of isolates could be clustered based on their serotypes or STs, whereas some clustering is associated with more than one ST or serotype. Five sheep isolates (4 belonging to ST675 and serotype O76:H19 and 1 belonging to ST25 and serotype O128:H2) share STs, serotypes and stx profiles with two hemolytic uremic syndrome-associated enterohemorrhagic E. coli (HUSEC) isolates; a cattle isolate belonging to the same ST as HUSEC isolate HUSEC001 contains all the nine virulence genes tested. These data suggest a potential of the six isolates for causing severe human infections. Collectively, we described the characteristics of cattle and sheep STEC isolates from Xinjiang, China, which may be utilized in comparative studies of other geographic regions and sources of isolation, and for surveillance as well., (© 2021 Wiley-VCH GmbH.)

Published

2022

25. Distribution and characterization of Streptococcus suis serotypes isolated from January 2015 to June 2020 from diseased pigs in Québec, Canada.

Author

Lacouture S, Olivera YR, Mariela S, and Gottschalk M

Subjects

Animals, Quebec, Serogroup, Serotyping veterinary, Swine, Streptococcal Infections microbiology, Streptococcal Infections veterinary, Streptococcus suis genetics, Streptococcus suis isolation & purification, Swine Diseases microbiology

Abstract

Streptococcus suis is one of the most important swine bacterial pathogens causing economic losses. This report presents the serotype distribution of S. suis recovered from diseased pigs in Québec from January 2015 to June 2020. Serotypes 1/2 and 2 predominated, followed by serotypes 7, 3, 5, 4, 9, 1, and 14. Compared to previously reported data, very few changes could be observed concerning the serotype distribution, indicating a relative stability. Half of the untypable isolates did not belong to the species S. suis sensu stricto , as determined by recN polymerase chain reaction. Less than 10% of "real S. suis " isolates were untypable. The genetic diversity of S. suis serotypes 1, 2, and 14, as analyzed by multilocus sequence typing, was mainly represented by sequence type (ST)1, ST28, ST25, and ST94. All ST1 isolates (considered highly virulent) belonged to either serotype 1 or 14., (Copyright and/or publishing rights held by the Canadian Veterinary Medical Association.)

Published

2022

26. Proposal of a subtype of serovar 4, K4b:O3, of Actinobacillus pleuropneumoniae based on serological and genotypic analysis.

Author

To H, Kon M, Koike F, Shibuya K, Nagai S, Gottschalk M, Frey J, and Sasakawa C

Subjects

Actinobacillus Infections veterinary, Animals, Genotype, Pleuropneumonia microbiology, Pleuropneumonia veterinary, Serogroup, Serotyping veterinary, Swine, Swine Diseases microbiology, Actinobacillus pleuropneumoniae classification, Actinobacillus pleuropneumoniae genetics, Bacterial Typing Techniques veterinary

Abstract

The aim of this study was to investigate an isolate of Actinobacillus pleuropneumoniae, named 14-760, which was serologically not classifiable among the recognised serovars of A. pleuropneumoniae. It reacted with the antisera raised against serovars 3, 6, 8, 15 and 17 in the agar gel precipitation (AGP) test, and was positive in the capsular serovar 4-specific PCR (cps4B PCR) assay. The isolate contains a type II capsule locus similar to serovar 4 but with variations in the length of four intergeneric regions (modF-cpxA, cpxD-cpsA, cpsC-a 114 bp orf, and lysA-ydeN), and three gene sequences (modF, cpsC and ydeN). The main difference found between the K4 and K4b cps genes is the additional 35 AAs found in type 4b due to a 4 bp insert in cps4bC. The LPS O-Ag locus is highly similar to that of reference strains of serovars 3, 6, 8, 15, 17 and 19. Isolate 14-760 is biovar 1 and contains solely the structural genes required for toxin ApxII production (apxIICA), and the type I secretion system (apxIBD) for the export of ApxII. Antiserum against isolate 14-760 adsorbed with antigen prepared from serovars 8, 15 or 17 reference strains remained reactive with isolate 14-760, but not with antigens prepared from serovars 1-18. Taken together, our results indicate the existence of a subtype of A. pleuropneumoniae, serovar 4, that we called "K4b:O3″, and we propose isolate 14-760 as the reference strain., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

27. Molecular characterization and in vivo pathogenicity study of Listeria monocytogenes isolated from fresh and frozen local and imported fish in Jordan.

Author

Tarazi Y, El-Sukhon S, Al-Rahbi A, and Ismail ZB

Subjects

Animals, Jordan epidemiology, Mice, Polymerase Chain Reaction veterinary, Serotyping veterinary, Virulence, Listeria monocytogenes genetics

Abstract

Background: Listeria monocytogenes (L. monocytogenes) is a serious zoonotic and food transmitted human pathogen causing meningitis and abortions. Several outbreaks of listeriosis have been associated with the consumption of ready-to-eat food products; dairy, meat, fish, and contaminated fruits and vegetables worldwide., Aim: This study was designed to detect and characterize L. monocytogenes isolated from local and imported fish in Jordan., Methods: A total of 170 fish (70 local and 100 imported), of which 140 fresh and 30 frozen samples were used in this study. Listeria monocytogenes was cultured and initially identified using conventional microbiological methods. For confirmation and serotyping of the L. monocytogenes isolates, PCR techniques were used. Using oral and intraperitoneal administration, mice were used to determine the pathogenicity and LD 50 of the isolated L. monocytogenes ., Results: A total of 72 Listeria spp. isolates were cultured from fish. Of those, 24 were positively identified as L. monocytogenes. Other strains of Listeria spp. were L. ivanovii (21), L. innocua (11), and L. grayi (16). Serotyping of the L. monocytogenes indicated that 14 isolates belonged to the 1/2b, 3b serotypes whereas 10 isolates belonged to the 4a and 4c serotypes. All isolates were virulent to mice with an LD 50 dose ranging from 3 × 10 10 CFU/ml to 3 × 10 7.5 CFU/ml. All the virulent isolates belonged to the serotype 1/2b. Histopathologically, dead mice showed multiple necrotic lesions in the liver and spleen., Conclusion: Results of this study showed the presence of potentially pathogenic L. monocytogenes in fresh and frozen, local, and imported fish in Jordan. Strict monitoring and quality control regulatory measures must be adopted to prevent future outbreaks of food poisoning associated with fish consumption., Competing Interests: The authors declare that they have no conflicts of interests.

Published

2021

28. Shiga toxin-producing Escherichia coli isolated from pasteurized dairy products from Bahia, Brazil.

Author

Rosario AILS, Castro VS, Santos LF, Lisboa RC, Vallim DC, Silva MCA, Figueiredo EES, Conte-Junior CA, and Costa MP

Subjects

Animals, Brazil, Dairy Products, Serotyping veterinary, Escherichia coli Infections veterinary, Escherichia coli O157, Escherichia coli Proteins, Shiga-Toxigenic Escherichia coli genetics

Abstract

The presence of pathogenic Shiga toxin-producing Escherichia coli (STEC) in dairy products represents a public health concern because of its ability to produce the toxins Stx1 and Stx2, which cause intestinal diseases. Monitoring the stages of milk production and checking dairy products for contamination are crucial steps to ensure dairy safety. This study aimed to report the occurrence of thermotolerant coliforms, E. coli, and STEC strains in pasteurized dairy products and to evaluate the antibiotic resistance profiles, serotypes, and characterizations of the STEC isolates by pulsed-field gel electrophoresis. We obtained a total of 138 pasteurized dairy products from 15 processing plants in Bahia, Brazil, to examine coliforms, E. coli, and STEC strains. We found that 43% of samples (59/138) contained thermotolerant coliforms, and 30% (42/138) did not comply with Brazilian regulations. Overall, 6% (9/138) were positive for E. coli and 4% (5/138) were positive for STEC. We recovered 9 STEC isolates from pasteurized cream (2/9), Minas Padrão cheese (2/9), Minas Frescal cheese (4/9), and ricotta (1/9). All isolates were stx2-positive, and 2 were eae-positive. All isolates were negative for the "big 6" STEC serogroups, belonging instead to serotypes ONT:HNT, ONT:H12, O148:H-, OR:H40, OR:HNT, and O148:HNT. Pulsed-field gel electrophoresis revealed 100% genetic similarity among 3 isolates from 2 different samples produced in the same production facility, which may suggest cross-contamination. As well, we found isolates that were 98% similar but in samples produced in different production facilities, suggesting a mutual source of contamination or a circulating strain. Two STEC strains exhibited resistance to streptomycin. Although the isolates presented a low resistance profile and no strain belonged to the "big 6" pathogenic group, the circulation of stx2-positive STEC strains in ready-to-eat products highlights the importance of epidemiological surveillance inside the Brazilian dairy chain., (Copyright © 2021 American Dairy Science Association. Published by Elsevier Inc. All rights reserved.)

Published

2021

29. Molecular characterization of Glaesserella parasuis strains isolated from North America, Europe and Asia by serotyping PCR and LS-PCR.

Author

Macedo N, Gottschalk M, Strutzberg-Minder K, Van CN, Zhang L, Zou G, Zhou R, Marostica T, Clavijo MJ, Tucker A, and Aragon V

Subjects

Animals, Asia epidemiology, Europe epidemiology, Haemophilus Infections epidemiology, Haemophilus Infections microbiology, North America epidemiology, Polymerase Chain Reaction veterinary, Prevalence, Seroepidemiologic Studies, Serotyping veterinary, Sus scrofa, Swine, Swine Diseases microbiology, Haemophilus Infections veterinary, Haemophilus parasuis genetics, Swine Diseases epidemiology

Abstract

Glaesserella parasuis strains were characterized by serotyping PCR, vtaA virulence marker Leader Sequence (LS)-PCR, clinical significance, and geographic region. Overall, the serovars 4, 5/12, 7, 1, and 13 were the most commonly detected. Serovars of greatest clinical relevance were systemic isolates that had a higher probability of being serovar 5/12, 13, or 7. In comparison, pulmonary isolates had a higher likelihood of being serovars 2, 4, 7, or 14. Serovars 5/12 and 13 have previously been considered disease-associated, but this study agrees with other recent studies showing that serovar 7 is indeed associated with systemic G. parasuis disease. Serovar 4 strains illustrated how isolates can have varying degrees of virulence and be obtained from pulmonary, systemic, or nasal sites. Serovars 8, 9, 15, and 10 were predominantly obtained from nasal samples, which indicates a limited clinical significance of these serovars. Additionally, most internal G. parasuis isolates were classified as virulent by LS-PCR and were disease-associated isolates, including serovars 1, 2, 4, 5/12, 7, 13, and 14. Isolates from the nasal cavity, including serovars 6, 9, 10, 11, and 15, were classified as non-virulent by LS-PCR. In conclusion, the distribution of G. parasuis serovars remains constant, with few serovars representing most of the strains isolated from affected pigs. Moreover, it was confirmed that the LS-PCR can be used for G. parasuis virulence prediction of field strains worldwide.

Published

2021

30. Salmonella in the processing line of farmed Tambatinga (Colossoma macropomum x Piaractus brachypomus) in Mato Grosso, Brazil: serotypes of occurrence and antimicrobial profile.

Author

Fernandes DVGS, Carvalho RCT, Castro VS, Cunha-Neto A, Muller B, Carvalho FT, Dos Prazeres Rodrigues D, Vieira BS, and de Souza Figueiredo EE

Subjects

Animals, Anti-Bacterial Agents pharmacology, Brazil, Microbial Sensitivity Tests veterinary, Serogroup, Serotyping veterinary, Salmonella, Salmonella Infections, Animal epidemiology

Abstract

The objective of this study was to evaluate the dispersion dynamics and antimicrobial resistance profiles of Salmonella in the processing of Tambatinga (Colossoma macropomum x Piaractus brachypomus). Thirty fish were monitored during four processing stages (reception, first wash, evisceration, and prepackage area) in a fish slaughterhouse. One hundred and twenty fish surface samples were collected and tested through bacteriological analysis, PCR, serotyping, and antimicrobial resistance profile (disk-diffusion). Of these samples, 7.5% (9/120) were positive for Salmonella, with 0.83% being observed in the pre-packaging phase, indicating a low occurrence at this stage. All the analyzed stages were positive for Salmonella, with the prevalent serovars being Ndolo, Mbandaka, Typhimurium, Rough, and O:16. All strains were sensitive to various antimicrobials. Improvements in microbiological control during all processing stages should be implemented to ensure a Salmonella-free product.

Published

2021

31. Sero- and apx-typing of German Actinobacillus pleuropneumoniae field isolates from 2010 to 2019 reveals a predominance of serovar 2 with regular apx-profile.

Author

Schuwerk L, Hoeltig D, Waldmann KH, Valentin-Weigand P, and Rohde J

Subjects

Actinobacillus Infections microbiology, Actinobacillus pleuropneumoniae isolation & purification, Animals, Genotype, Genotyping Techniques veterinary, Germany, Pleuropneumonia microbiology, Serogroup, Serotyping veterinary, Sus scrofa, Swine, Actinobacillus Infections veterinary, Actinobacillus pleuropneumoniae genetics, Pleuropneumonia veterinary, Swine Diseases microbiology

Abstract

Serotyping is the most common method to characterize field isolates of Actinobacillus (A.) pleuropneumoniae, the etiological agent of porcine pleuropneumonia. Based on serology, many farms seem to be infected and antibodies against a wide variety of serovars are detectable, but, so far it is unknown to what degree respective serovars contribute to outbreaks of clinical manifest disease. In this study, 213 German A. pleuropneumoniae field isolates retrieved for diagnostic purposes from outbreaks of porcine pleuropneumonia between 2010 and 2019 were genetically serotyped and analyzed regarding their apx-toxin gene profile using molecular methods. Serotyping revealed a prominent role of serovar 2 in clinical cases (64% of all isolates) and an increase in the detection of this serovar since 2010 in German isolates. Serovar 9/11 followed as the second most frequent serovar with about 15% of the isolates. Furthermore, very recently described serovars 16 (n = 2) and 18 (n = 8) were detected. Most isolates (93.4%) showed apx-profiles typical for the respective serovar. However, this does not hold true for isolates of serovar 18, as 75% (n = 6) of all isolates of this serovar deviated uniformly from the "typical" apx-gene profile of the reference strain 7311555. Notably, isolates from systemic lesions such as joints or meninges did not harbor the complete apxICABD operon which is considered typical for highly virulent strains. Furthermore, the extremely low occurrence (n = 1) of NAD independent (biovar II) isolates in German A. pleuropneumoniae was evident in our collection of clinical isolates.

Published

2021

32. Long-chain LPS-based enzyme-linked immunosorbent assay to detect swine herds infected by Actinobacillus pleuropneumoniae serotype 17.

Author

Gottschalk M, Lacouture S, Blackwell T, and Bossé J

Subjects

Animals, Antibodies, Bacterial, Enzyme-Linked Immunosorbent Assay veterinary, Lipopolysaccharides, North America, Serogroup, Serotyping veterinary, Swine, Actinobacillus Infections diagnosis, Actinobacillus Infections veterinary, Actinobacillus pleuropneumoniae, Swine Diseases diagnosis

Abstract

Actinobacillus pleuropneumoniae serotype 17, one of the two most recent serotypes described, has been isolated from diseased pigs in North America. Yet, no serological test for surveillance has been developed so far. An enzyme-linked immunosorbent assay (ELISA) using the long-chain lipopolysaccharide antigen (LC-LPS) of this serotype is described. As predicted by previous genetic data on the O-antigen locus, cross reactions were observed between this serotype and serotypes 3, 6, 8, and 15. Although animals infected by serotype 17 would be detected using the current serotype 3 LC-LPS ELISA, better results may be obtained when plates are coated with the antigen purified from the homologous serotype., (Copyright and/or publishing rights held by the Canadian Veterinary Medical Association.)

Published

2021

33. Serotyping versus genotyping in infected sheep and goats with small ruminant lentiviruses.

Author

Acevedo Jiménez GE, Tórtora Pérez JL, Rodríguez Murillo C, Arellano Reynoso B, and Ramírez Álvarez H

Subjects

Animals, Enzyme-Linked Immunosorbent Assay veterinary, Genotype, Goats, Lentivirus genetics, Lentivirus isolation & purification, Lentivirus Infections virology, Phylogeny, Polymerase Chain Reaction veterinary, Ruminants, Sensitivity and Specificity, Serotyping veterinary, Sheep, Antibodies, Viral blood, Goat Diseases virology, Lentivirus immunology, Lentivirus Infections veterinary, Sheep Diseases virology

Abstract

Despite SRLV infection being endemic in Mexico, there is little information regarding which genotypes are present. We compared serotyping and PCR-sequencing results from sheep and goats infected with SRLV. We separated plasma and peripheral blood leukocytes (PBL) from 1940 blood samples from sheep and goats from 12 states across Mexico. To detect SRLV infection, we tested plasma samples using two commercial ELISA kits (VMRD and Eradikit SRLV Screening). Then, we serotyped the infecting virus (A/ B) using Eradikit SRLV Genotyping. PBL DNA was used to detect the proviral genome via PCR. Positive amplicons were sequenced to identify viral genotypes using a phylogenetic analysis. Also, we analysed for residues differences in the sequences of a capsid epitope between genotypes. The serological results indicated a higher detection of seropositive animals using the VMRD ELISA compared to Eradikit, with 21 % and 15.3 % more in sheep and goats respectively. Only 25.7 % of the ELISA serotyping results matched those from PCR-sequencing. PCR-sequencing was able to identify genotype A, B and coinfections in animals classified as indeterminate by the ELISA test. This lack of sensitivity may be related to the lack of epitopes from the matrix and transmembrane peptides used by ELISA screening. Sequences analysis revealed that SRLVs found in sheep cluster with genetic subtypes A2 and B1, while those in goats cluster with subtypes A1 and B1. Serotyping did not prove to be an adequate method for predicting the viral genotype (A and / or B) in infections caused by SRLV., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2021

34. Serotyping and pathotyping of Glaesserella parasuis isolated 2012-2019 in Germany comparing different PCR-based methods.

Author

Schuwerk L, Hoeltig D, Waldmann KH, Strutzberg-Minder K, Valentin-Weigand P, and Rohde J

Subjects

Animals, Germany, Haemophilus Infections microbiology, Polymerase Chain Reaction methods, Serogroup, Serotyping veterinary, Sus scrofa, Swine, Haemophilus Infections veterinary, Haemophilus parasuis genetics, Haemophilus parasuis pathogenicity, Polymerase Chain Reaction veterinary, Swine Diseases microbiology, Virulence genetics

Abstract

Glaesserella parasuis is an important pathogen in swine production. It acts as a primary pathogen in systemic Glässer´s disease and as a secondary pathogen in Porcine Respiratory Disease Complex. In this study, a collection of 308 isolates from carrier animals and individuals with respiratory or Glässer´s disease isolated 2012-2019 in Germany was analysed. Isolates were characterized for serovar implementing two different PCR methods. Additionally, two different PCR methods for pathotyping isolates were applied to the collection and results compared. Serovar 6 (p < 0.0001) and 9 (p = 0.0007) were correlated with carrier isolates and serovar 4 was associated with isolates from animals with respiratory disease (p = 0.015). In systemic isolates, serovar 13 was most frequently detected (18.9%). Various other serovars were isolated from all sites and the ratio of serovar 5 to serovar 12 was approximately 1:2. These two serovars together represented 14.3% of the isolates; only serovar 4 was isolated more frequently (24.7%). The pathotyping method based on the leader sequence (LS = ESPR of vta) was easy to perform and corresponded well to the clinical background information. Of the carrier isolates 72% were identified as non-virulent while 91% of the systemic isolates were classified as virulent (p < 0.0001). Results of the pathotyping PCR based on 10 different marker genes overall were in good agreement with clinical metadata as well as with results of the LS-PCR. However, the pathotyping PCR was more complicated to perform and analyze. In conclusion, a combination of the serotyping multiplex-PCR and the LS-PCR could improve identification of clinically relevant G. parasuis isolates, especially from respiratory samples.

Published

2020

35. Development and validation of a simplified serotyping ELISA based on monoclonal antibodies for the diagnosis of foot-and-mouth disease virus serotypes O, A, C and Asia 1.

Author

Grazioli S, Ferris NP, Dho G, Pezzoni G, Morris AS, Mioulet V, and Brocchi E

Subjects

Animals, Antibodies, Monoclonal analysis, Cattle, Cattle Diseases virology, Enzyme-Linked Immunosorbent Assay methods, Foot-and-Mouth Disease virology, Serotyping veterinary, Sus scrofa, Swine, Swine Diseases virology, Cattle Diseases diagnosis, Enzyme-Linked Immunosorbent Assay veterinary, Foot-and-Mouth Disease diagnosis, Foot-and-Mouth Disease Virus isolation & purification, Serotyping methods, Swine Diseases diagnosis

Abstract

This study describes the development and validation of a simplified enzyme-linked immunosorbent assay (ELISA) for the detection and discrimination of foot-and-mouth disease virus (FMDV) serotypes O, A, C and Asia 1. The multiplex ELISA was designed using selected, type-specific monoclonal antibodies (MAbs) coated onto ELISA plates as catching antibodies and a unique pan-FMDV MAb (1F10) as detector conjugate. Capture MAbs with the broadest intratypic reactivity were selected for each of the four FMDV serotypes by screening large panels of candidate MAbs with a wide spectrum of representative FMDV isolates. An additional pan-FMDV ELISA using 1F10 MAb for both capture and detection was used to complement the specific typing ELISAs to detect virus isolates, which might escape binding to the selected serotype-specific MAbs. This multiplex ELISA was prepared in a stabilized format, with immunoplates pre-coated with six MAbs and positive antigen controls already trapped by the relevant MAb, with the view to make available a diagnostic kit. Diagnostic performance of the MAbs-multiplex ELISA was analysed using 299 FMDV-positive epithelial suspensions representative of the antigenic and genomic variability within each serotype. Overall, the results provided evidence that the diagnostic performance of this assay platform is improved compared to the more complex polyclonal-based antigen detection ELISA; combining data from different serotypes and referring to the gold standard tests (i.e. virus isolation and/or RT-PCR), the MAbs-multiplex ELISA showed a sensitivity of 79% for the serotype-specific ELISA, compared to 72% for the polyclonal ELISA. The absence of reactivity of a minority of FMDV strains using the MAbs-multiplex ELISA can largely be attributed to deteriorated or low antigen concentration in the sample. This multiplex ELISA is simple, rapid and stable. FMDV antigenic diversity was adequately covered by the selected MAbs. Therefore, it can be used to replace existing polyclonal ELISAs for FMDV detection and serotyping., (© 2020 Blackwell Verlag GmbH.)

Published

2020

36. Serogroups of Dichelobacter nodosus, the cause of footrot in sheep, are randomly distributed across England.

Author

Prosser NS, Monaghan EM, Green LE, and Purdy KJ

Subjects

Animals, England epidemiology, Female, Foot Rot epidemiology, Polymerase Chain Reaction veterinary, Serotyping veterinary, Sheep microbiology, Sheep Diseases epidemiology, Dichelobacter nodosus genetics, Foot Rot microbiology, Serogroup, Sheep Diseases microbiology

Abstract

We present the largest and most representative study of the serological diversity of Dichelobacter nodosus in England. D. nodosus causes footrot and is one of the top five globally important diseases of sheep. The commercial vaccine, containing nine serogroups, has low efficacy compared with bivalent vaccines. Our aim was to investigate the prevalence and distribution of serogroups of D. nodosus in England to elucidate whether a bivalent vaccine could protect the national flock. Farmers from 164 flocks submitted eight interdigital swabs from eight, preferably diseased, sheep. All serogroups, A-I, were detected by PCR in 687/1150 D. nodosus positive swabs, with a prevalence of 2.6-69.3% of positive swabs per serogroup. There was a median of two serogroups per flock (range 0-6). Serogroups were randomly distributed between, but clustered within, flocks, with 50 combinations of serogroups across flocks. H and B were the most prevalent serogroups, present in > 60% of flocks separately but in only 27% flocks together. Consequently, a bivalent vaccine targeting these two serogroups would protect 27% of flocks fully (if only H and B present) and partially, if more serogroups were present in the flock. We conclude that one bivalent vaccine would not protect the national flock against footrot and, with 50 combinations of serogroups in flocks, flock-specific vaccines are necessary.

Published

2020

37. Genetic analysis of an Erysipelothrix rhusiopathiae swine isolate determined to be serovar 2 by a gel double diffusion test but serovar 1a/2 by a serotyping PCR assay.

Author

Shiraiwa K, Ogawa Y, Nishikawa S, Nakayama M, Eguchi M, and Shimoji Y

Subjects

Animals, Genetic Testing veterinary, Serogroup, Serotyping veterinary, Swine, Erysipelothrix genetics, Erysipelothrix Infections, Swine Diseases

Abstract

We previously developed a multiplex PCR assay for the differentiation of serovar 1a, 1b, 2 and 5 strains of Erysipelothrix rhusiopathiae. In this study, we analyzed the serovar-defining chromosomal region of a serovar 2 swine isolate, which was PCR-positive for both serovars 1a and 2 by the multiplex PCR assay. Genetic analysis of the chromosomal region revealed that, as in serovar 1a strains, the ERH&#95;1440 gene, which is usually truncated or missing in serovar 2 strains, was intact in this strain. This paper first shows an E. rhusiopathiae serovar 2 strain possessing an intact ERH&#95;1440 gene and suggests that care may be needed when determining the serovar of such rare strains by PCR assay.

Published

2020

38. Urban birds: An important source of antimicrobial resistant Salmonella strains in Central Spain.

Author

Martín-Maldonado B, Vega S, Mencía-Gutiérrez A, Lorenzo-Rebenaque L, de Frutos C, González F, Revuelta L, and Marin C

Subjects

Animals, Anti-Bacterial Agents pharmacology, Drug Resistance, Bacterial, Microbial Sensitivity Tests veterinary, Salmonella drug effects, Serotyping veterinary, Spain epidemiology, Bird Diseases epidemiology, Bird Diseases microbiology, Birds microbiology, Drug Resistance, Multiple, Bacterial, Salmonella classification, Salmonella Infections, Animal epidemiology

Abstract

Antimicrobial resistance (AMR) is one of the most important threats of the 21 st century. Wild birds have been described as reservoirs of AMR in different bacterial species, such as Salmonella spp. Privation of food, climate change and overpopulation have forced many wild species to modify their feeding habits, attending urban areas. In this context, the aim of this study was to study Salmonella presence, as well as related AMR in urban birds that inhabit the city and its surroundings. A total of 300 urban birds were sampled for Salmonella detection according to the ISO 6579-1:2017 (Annex D) recommendations, and serotyping was carried out according to the White-Kauffman-Le Minor scheme. Antimicrobial susceptibility was tested following 2013/652/EU Decision guides. Wild birds analysed were positive for Salmonella in 12.3 % of cases, with white storks fed in landfills as the most Salmonella prevalent species (p < 0.05). The most common serovars isolated were zoonotic (S. Enteritidis, S. Typhimurium and S. Typhimurium monophasic variant). From Salmonella isolated strains, 40.5 % were resistant to the most prevalent AMRs found in urban birds were ciprofloxacin (36.4 %), nalidixic acid (36.4 %) and colistin (27.3 %). The scientific community, public administration and population in general should work together to control antimicrobial administration and drug waste management in order to decrease the development and spread of AMR., (Copyright © 2020 Elsevier Ltd. All rights reserved.)

Published

2020

39. Public health aspects of Shiga toxin-producing Escherichia coli (STEC) strains in sheep and goats of Bakhtiari pastoral tribe, Iran.

Author

Zaheri H, Ghanbarpour R, Jajarmi M, Bagheri M, Ghanadian A, and Askari Badouei M

Subjects

Animals, Escherichia coli Infections epidemiology, Escherichia coli Infections microbiology, Escherichia coli Proteins genetics, Feces microbiology, Female, Iran epidemiology, Male, Polymerase Chain Reaction veterinary, Public Health, Serogroup, Serotyping veterinary, Sheep Diseases epidemiology, Sheep Diseases microbiology, Shiga Toxin genetics, Shiga-Toxigenic Escherichia coli isolation & purification, Transients and Migrants, Virulence genetics, Escherichia coli Infections veterinary, Goats microbiology, Sheep microbiology, Shiga-Toxigenic Escherichia coli genetics, Virulence Factors genetics

Abstract

Nomadic populations do not have permanent settlements as they move their livestock between grazing areas in different seasons; such movements may have great impact on dissemination of food-borne pathogens in various regions. The aim of this study was to characterize Shiga toxin-producing Escherichia coli (STEC) strains as a food-borne pathogen in sheep and goats of Bakhtiari pastoral tribe in Iran. In the present study, 72 fecal samples were obtained from 26 sheep and 46 goats. First, all recovered E. coli isolates were screened for stx gene. After detection of stx-positive isolates, the virulence genes including stx1, stx2, eae, ehly, saa, astA, subAB, terD, and the genetic markers of O Island 57 (Z2098 and Z2099) were investigated. Also fifteen important STEC O-serogroups were determined using PCR assays. Results showed that 27 animals (27/72; 37.5%) carried STEC strains including 16/26 (61.6%) sheep and 11/46 (23.9%) goats. All STECs were eae-negative but 81.4% (22/27) were positive for saa. The most prevalent virulence profile was stx1/stx2/ehly/saa/subAB (37%; 10/27). Most STECs (24/27) were positive for at least one of the selected OI-57 markers. The O91 (n = 6), O5 (n = 3), O113 (n = 1), O128 (n = 1), and O104 (n = 1) were the detected O-serogroups in this study. It is concluded that such moving animal populations could have public health concerns which have to be addressed in the future.

Published

2020

40. A case report of sporadic ovine listerial meningoencephalitis in Kosovo.

Author

Hamidi A, Bisha B, Goga I, Wang B, Robaj A, and Sylejmani DS

Subjects

Animals, Anti-Bacterial Agents pharmacology, Brain microbiology, Female, Kosovo, Listeriosis diagnosis, Listeriosis microbiology, Meningoencephalitis diagnosis, Meningoencephalitis microbiology, Microbial Sensitivity Tests veterinary, Serotyping veterinary, Sheep, Sheep Diseases, Sheep, Domestic, Drug Resistance, Bacterial, Listeria monocytogenes drug effects, Listeria monocytogenes isolation & purification, Listeriosis veterinary, Meningoencephalitis veterinary

Abstract

In 2018, a case of neural disease suspected of listeriosis was reported in a flock of sheep in Kosovo with the death of ewes and 5 lambs. Samples from the brain of only three dead animals were subjected to histopathological and bacteriological analysis. MALDI-TOF MS was applied to confirm suspected Listeria spp. isolates from culture and multiplex PCR was applied for molecular serotyping. All isolates were tested for antimicrobial susceptibility by microdilution broth method. The histopathological analysis of the brain specimens showed typical changes for Listeria monocytogenes. Listeria spp. was isolated in brain samples from all three animals, and all the isolates were confirmed using MALDI-TOF MS and PCR down to the species level (Listeria monocytogenes). The molecular characterisation using multiplex PCR revealed all isolates as Listeria monocytogenes serotype 4b. All L. monocytogenes isolates were found to be susceptible to penicillin, erythromycin, tetracycline, streptomycin, trimethoprim/sulfamethosazole, quinupristin/dalfopristin, kanamycin, vancomycin, and gentamicin but resistant to nitrofurantoin and lincomycin. This study shows the emergence of a highly virulent strain in sheep farms in Kosovo and a possible threat to public health.

Published

2020

41. Comparative genomics of Streptococcus parauberis: new target for molecular identification of serotype III.

Author

Torres-Corral Y and Santos Y

Subjects

Animals, Bacterial Capsules genetics, Fish Diseases microbiology, Fishes, Genetic Loci, Genomics, Multiplex Polymerase Chain Reaction, Real-Time Polymerase Chain Reaction, Sensitivity and Specificity, Serogroup, Serotyping methods, Streptococcal Infections microbiology, Streptococcal Infections veterinary, Streptococcus classification, Genome, Bacterial genetics, Serotyping veterinary, Streptococcus genetics, Streptococcus isolation & purification

Abstract

This paper describes the predicted structure for the cps loci involved in capsule biosynthesis for Streptococcus parauberis serotypes III, IV, and V. Based on the specific serotype regions I, II, and III, a multiplex PCR protocol (mPCR) was designed to differentiate the main serotypes causing fish diseases. A real-time PCR method (qPCR) is also described to identify S. parauberis of serotype III in bacterial cultures and fish tissues. In silico and in vitro analyses revealed that both methods have a 100% specificity. The mPCR assay was optimized for the detection of S. parauberis strains of subtypes Ia (amplicon size 213 bp), subtypes Ib and Ic (both amplicon size 303 bp), serotype II (amplicon size 403 bp), and serotype III (amplicon size 130 bp) from bacterial cultures. The qPCR assay was optimized for the identification and quantification of S. parauberis serotype III strains in bacterial cultures and fish tissues. This assay achieved a sensitivity of 2.67 × 10 2 gene copies (equivalent to 3.8 × 10 -9  ng/μl) using pure bacterial cultures of S. parauberis serotype III and 1.76 × 10 2 gene copies in fish tissues experimentally and naturally infected with S. parauberis of the serotype III. The specificity and sensitivity of the protocols described in this study suggest that these methods could be used for diagnostic and/or epidemiological purposes in clinical diagnostic laboratories. KEY POINTS: • Structure of loci cps for S. parauberis of serotypes III, IV and V was described. • mPCR to differentiate S. parauberis serotypes causing disease in fish was optimized. • qPCR assay to quantify strains of S. parauberis serotype III in fish tissues.

Published

2020

42. Development of a mismatch amplification mutation assay to correctly serotype isolates of Streptococcus suis serotypes 1, 2, 1/2, and 14.

Author

Lacouture S, Okura M, Takamatsu D, Corsaut L, and Gottschalk M

Subjects

Animals, Mutation, Polymerase Chain Reaction methods, Serogroup, Serotyping methods, Streptococcus suis classification, Polymerase Chain Reaction veterinary, Serotyping veterinary, Streptococcus suis genetics

Abstract

Streptococcus suis is one of the most important bacterial swine pathogens worldwide and is an emerging pathogen in humans. There are 29 serotypes, and serotyping, which is based on the antigenicity of the capsular polysaccharide (CPS) or on its coding genes, is often part of routine identification and provides further information regarding S. suis virulence and zoonotic potential. Serotypes 2 and 14 possess high zoonotic potential, and serotype 1/2 is the serotype most frequently isolated from diseased pigs in North America. PCR has replaced antibody-based techniques to perform serotyping. However, traditional PCR is not able to differentiate serotype 2 from 1/2 and serotype 1 from 14, given that the only difference in the cps loci of those serotype pairs is a nonsynonymous single-nucleotide polymorphism. We developed a mismatch amplification mutation assay (MAMA)-PCR that was able to correctly serotype 148 isolates previously known to be serotypes 1, 2, 1/2, or 14. This technique will be highly useful in animal and human health laboratories performing PCR serotyping of S. suis isolates.

Published

2020

43. Research Note: Repetitive element-based polymerase chain reaction genotyping improves efficiency of Salmonella surveillance in a model broiler production system.

Author

Walker GK, Suyemoto MM, Borst LB, and Brake J

Subjects

Animals, Anti-Bacterial Agents pharmacology, Genotyping Techniques veterinary, Polymerase Chain Reaction veterinary, Poultry Diseases microbiology, Prevalence, Salmonella genetics, Salmonella Infections, Animal microbiology, Serotyping veterinary, Chickens, DNA Fingerprinting veterinary, Drug Resistance, Bacterial genetics, Epidemiological Monitoring veterinary, Poultry Diseases epidemiology, Salmonella isolation & purification, Salmonella Infections, Animal epidemiology

Abstract

The genetic relatedness and antimicrobial susceptibility profiles of Salmonella isolated from poultry and their environment were determined. One broiler breeder flock (BBF1) and 2 broiler flocks (BF1 and BF2) were reared over a 1.75-year period on the same poultry research farm. Hatching eggs were obtained from BBF1 to produce BF1 chicks, while BF2 chicks were progeny of a separate, unsampled broiler breeder flock. BF1 and BF2 were reared in the same housing facilities but 6 mo apart. Salmonella isolates were collected via litter sock sampling (BF1), cecal excision (BF1 and BF2), or cloacal swabs (BBF1). Serotyping identified Salmonella enterica subsp. enterica serovar Altona (SA) in BBF1 and S. enterica subsp. enterica serovar Senftenberg (SS) in BF1 and BF2. Genotypic fingerprinting was achieved with Rep-PCR using the (GTG) 5 primer and revealed sequence homology among Senftenberg isolates from BF1 and BF2. For each isolate, the minimum inhibitory concentration was determined for 27 antimicrobial agents using Sensititre plates with formularies specific to antimicrobials used in poultry production or those used to control gram negative pathogens. Isolates from the 3 flocks were resistant to clindamycin, erythromycin, novobiocin, penicillin, and tylosin tartrate and demonstrated intermediate resistance to azithromycin, florfenicol, and spectinomycin. These data demonstrated that serovar Altona and Senftenberg were harbored by poultry, the latter appeared to persist in broiler flocks, and both serotypes shared similar patterns of antimicrobial susceptibility in an integrated research operation. In the case of multiple Salmonella isolates, combining genotypic fingerprinting methods with serotyping of representative isolates would reduce the number of samples required for serotyping and more clearly identify relatedness of isolates. These methods facilitate effective surveillance in poultry production systems, thus allowing for implementation of precise Salmonella control measures., (Copyright © 2020. Published by Elsevier Inc.)

Published

2020

44. Immunohistochemical and molecular analysis of Pasteurella multocida in a rabbit with suppurative pleuropneumonia.

Author

Uenoyama K, Ueno Y, Tosaki K, Abeto Y, Ito H, Katsuda K, and Shibahara T

Subjects

Animals, Antibodies, Chickens, Multilocus Sequence Typing methods, Multilocus Sequence Typing veterinary, Pasteurella Infections epidemiology, Pasteurella Infections pathology, Pasteurella multocida genetics, Pasteurella multocida pathogenicity, Pleuropneumonia microbiology, Pleuropneumonia pathology, Pleuropneumonia veterinary, Serotyping veterinary, Taiwan epidemiology, Pasteurella Infections veterinary, Pasteurella multocida isolation & purification, Rabbits microbiology

Abstract

A 1-month-old rabbit, imported as a pet by a distributor, died suddenly in the quarantine period in Japan due to suppurative pleuropneumonia. A bacterial isolate from its right lung was identified as Pasteurella multocida serotype A: 11. The isolate was classified as ST204 using the RIRDC scheme of multilocus sequence typing, suggesting that the isolate was genetically related to European isolates of the same sequence type listed in the PubMLST database and not to four other isolates that originated from past imported rabbits. In the immunohistochemical assay, an antiserum recognizing the somatic serotype 11 antigen generated from chicken could specifically detect P. multocida, indicating that the antiserum for somatic serotyping was useful for immunohistochemical diagnosis of rabbit pasteurellosis.

Published

2020

45. Identification and characterization of Dutch Avibacterium paragallinarum isolates and the implications for diagnostics.

Author

Feberwee A, Dijkman R, Buter R, Soriano-Vargas E, Morales-Erasto V, Heuvelink A, Fabri T, Bouwstra R, and de Wit S

Subjects

Animals, Disease Outbreaks veterinary, Enterobacteriaceae isolation & purification, Female, Molecular Typing veterinary, Netherlands epidemiology, Pasteurellaceae isolation & purification, Pasteurellaceae pathogenicity, Pasteurellaceae Infections epidemiology, Pasteurellaceae Infections microbiology, Polymerase Chain Reaction veterinary, Poultry Diseases diagnosis, Poultry Diseases epidemiology, Serogroup, Serotyping veterinary, Species Specificity, Virulence, Chickens microbiology, Enterobacteriaceae genetics, Pasteurellaceae genetics, Pasteurellaceae Infections veterinary, Poultry Diseases microbiology

Abstract

This study reports the results of diagnostic and molecular typing methods for 18 Avibacterium paragallinarum isolates obtained from outbreaks of infectious coryza in commercial layer flocks in the Netherlands. Isolation, biochemical identification, species-specific PCR tests and classical serotyping were performed. In addition, molecular typing by Enterobacterial Repetitive Intergenic Consensus-Based Polymerase Chain Reaction (ERIC-PCR) and sequence analysis of the partial HPG2 region of A. paragallinarum were applied and results of both techniques were compared. Moreover, the pathogenicity of an isolate of the most common genotype detected in the Netherlands was determined in an animal experiment. All 18 Avibacterium isolates were nicotinamide adenine dinucleotide-dependent . All isolates were detected by the species-specific conventional PCR while 33% of the isolates were missed by the species-specific real-time PCR. Sequence analysis showed a probe mismatch as a result of a single nucleotide polymorphism (G1516A). Modification of the probe of the real-time PCR was necessary to overcome false negative results. Molecular typing showed that sequence analysis of the partial HPG2 region was in concordance with ERIC-PCR results and indicated the presence of two major genotypes. Serotyping showed the presence of serovars A-1, A-2 and B-1. There was no correlation between genotyping results and serotyping results. Inoculation of an isolate of the most prevalent genotype, and belonging to serovar A-1, into brown layer hens demonstrated the pathogenicity of this isolate.

Published

2019

46. Emergence of Salmonella enterica serovar 4,[5],12:i:- as the primary serovar identified from swine clinical samples and development of a multiplex real-time PCR for improved Salmonella serovar-level identification.

Author

Naberhaus SA, Krull AC, Bradner LK, Harmon KM, Arruda P, Arruda BL, Sahin O, Burrough ER, Schwartz KJ, and Kreuder AJ

Subjects

Animals, Multiplex Polymerase Chain Reaction methods, Multiplex Polymerase Chain Reaction veterinary, Real-Time Polymerase Chain Reaction methods, Salmonella Infections, Animal microbiology, Salmonella enterica pathogenicity, Serogroup, Serotyping methods, Swine, Swine Diseases microbiology, United States, Virulence, Real-Time Polymerase Chain Reaction veterinary, Salmonella Infections, Animal diagnosis, Salmonella enterica classification, Serotyping veterinary, Swine Diseases diagnosis

Abstract

Rapid identification of the infecting Salmonella serovar from porcine diagnostic samples is vital to allow implementation of appropriate on-farm treatment and management decisions. Although identification at the serogroup level can be rapidly achieved at most veterinary diagnostic laboratories, final Salmonella serovar identification often takes several weeks because of the limited number of reference laboratories performing the complex task of serotyping. Salmonella serogroup B, currently the dominant serogroup identified from swine clinical samples in the United States, contains serovars that vary from highly pathogenic to minimally pathogenic in swine. We determined the frequency of detection of individual group B serovars at the Iowa State Veterinary Diagnostic Laboratory from 2008 to 2017, and validated a multiplex real-time PCR (rtPCR) to distinguish pathogenic serogroup B serovars from those of lesser pathogenicity. Our results indicate that, since 2014, Salmonella enterica ssp. enterica serovar 4,[5],12:i:- has been the dominant serovar identified from swine clinical samples at the ISU-VDL, with S. Typhimurium now the second most common serovar identified. We developed a rtPCR to allow rapid differentiation of samples containing S. 4,[5],12:i:- and S. Typhimurium from samples containing serovars believed to be of less pathogenicity, such as S. Agona and S. Derby. When combined with enrichment culture, this rtPCR has the ability to significantly improve the time to final serovar identification of the 2 most commonly identified pathogenic Salmonella serovars in swine, and allows rapid implementation of serovar-specific intervention strategies.

Published

2019

47. Salmonella serotype assignment by sequencing analysis of intergenic regions of ribosomal RNA operons.

Author

Kipper D, Hellfeldt RM, De Carli S, Lehmann FKM, Fonseca ASK, Ikuta N, and Lunge VR

Subjects

Operon, Salmonella genetics, Sequence Analysis, RNA methods, Serogroup, Serotyping veterinary, DNA, Intergenic analysis, RNA, Ribosomal analysis, Salmonella classification, Sequence Analysis, RNA veterinary

Abstract

Salmonella laboratorial detection is usually carried out by bacteriological culture and serological methods. Salmonella isolates are then classified into more than 2,650 serotypes with different somatic (O) and flagellar (H) antigenic combinations. More recently, DNA analysis methods were developed and applied for the identification of Salmonella serotypes, including intergenic spacer regions (ISRs) that separates DNA-encoding ribosomal subunits (rRNA gene) in Salmonella genomes. The present study aimed to evaluate the nucleotide diversity of the ISRs in 2 rRNA operons (rrnB and rrnH) for the assignment of Salmonella serotypes. A total of 63 Salmonella isolates (bacterial cultures) from 21 serotypes were obtained in the period of 2014 to 2017. DNA was extracted, and PCRs were used to detect the genus Salmonella and 4 important serotypes: Enteritidis, Gallinarum, Heidelberg, and Typhimurium. ISRs of the operons rrnB and rrnH were amplified by PCR and then sequenced. All sequence results were submitted to BLASTn search and were aligned in comparison to 72 Salmonella reference nucleotide sequences. The results demonstrated that 60 (95.2%) samples returned a sequence of the same serotype (determined by the traditional serological procedure) after searching in BLASTn and/or in the alignment with the reference sequences for both operons (rrnB and rrnH). These PCR-sequencing procedures had a general agreement index of 0.792 based on the Kappa analysis, 98.7% sensitivity value, 100% specificity, and 98.4% accuracy. Three different phylogenetic trees were generated from the alignments with the sequences of rrnH, rrnB, and rrnH plus rrnB and isolates clustered in specific branches according to the serotypes., (© 2019 Poultry Science Association Inc.)

Published

2019

48. Serotyping and antimicrobial resistance of Mannheimia haemolytica strains from European cattle with bovine respiratory disease.

Author

Andrés-Lasheras S, Zaheer R, Klima C, Sanderson H, Ortega Polo R, Milani MRM, Vertenten G, and McAllister TA

Subjects

Animals, Anti-Bacterial Agents pharmacology, Bovine Respiratory Disease Complex microbiology, Cattle, Europe epidemiology, Mannheimia haemolytica physiology, Pasteurellaceae Infections epidemiology, Pasteurellaceae Infections microbiology, Prevalence, Bovine Respiratory Disease Complex epidemiology, Drug Resistance, Bacterial immunology, Mannheimia haemolytica drug effects, Pasteurellaceae Infections veterinary, Serotyping veterinary

Abstract

The objective of this study was to assess the prevalence of three serotypes, A1, A2, and A6 in 98 M. haemolytica isolates collected from clinical BRD cases in European cattle and assess their antimicrobial resistance profiles. Isolates were characterized by serotyping (plate agglutination and serotype specific PCR) and antimicrobial susceptibility testing. The study identified a predominance of serotypes A1 (59%) and A6 (22%) in European M. haemolytica isolates exhibiting a relatively low level of antimicrobial resistance. A comprehensive understanding of the relative prevalence of different M. haemolytica serotypes in Europe informs a targeted approach for vaccine design against BRD., (Crown Copyright © 2019. Published by Elsevier Ltd. All rights reserved.)

Published

2019

49. The first report on serotyping of bluetongue virus in small ruminants of Khyber Pakhtunkhwa province, Pakistan.

Author

Malik AI, Ijaz M, Yaqub T, Shabir MZ, Avais M, Ghaffar A, Ali A, Farooqi SH, and Mehmood K

Subjects

Animals, Bluetongue virology, Bluetongue virus isolation & purification, Enzyme-Linked Immunosorbent Assay veterinary, Goat Diseases virology, Goats, Pakistan epidemiology, Prevalence, Real-Time Polymerase Chain Reaction veterinary, Seroepidemiologic Studies, Serotyping veterinary, Sheep, Sheep Diseases virology, Sheep, Domestic, Bluetongue epidemiology, Bluetongue virus classification, Goat Diseases epidemiology, Sheep Diseases epidemiology

Abstract

Bluetongue virus (BTV), a member of Orbivirus genus (family Reoviridae), is a non-contagious infection of domestic and wild ruminants. The current study was designed to detect various serotypes of BTV in small ruminants of Khyber Pakhtunkhwa (KPK) province of Pakistan, along with their effects on hemato-biochemical parameters. A total of 408 serum samples in four districts (Mansehra, Abbottabad, Swabi, and Kohat) of KPK from small ruminants were screened based on competitive ELISA (cELISA). A total of 204 (50%) samples were found positive for BTV group-specific antibodies. The seropositive samples were processed for the detection of BTV serotypes through real-time polymerase chain reaction (qPCR). Out of 204 cELISA-positive samples, 60 (29.41%) were found positive through qPCR. Three serotypes [6, 8, 9] were detected from Mansehra District and two from Kohat [2, 8] and Abbottabad [6, 8], while only one from Swabi [8]. The serotype "8" was found consistently in all the four study districts. A significant (p < 0.05) increase in the level of blood urea nitrogen (BUN) and alkaline phosphatase (ALP) was recorded in goats, whereas aspartate aminotransferase (AST) in sheep infected with BTV, compared to healthy animals. The hematological parameters showed significantly (p < 0.05) raised total leucocyte count (TLC) in both sheep and goats, whereas only hematocrit (HCT) value was increased significantly (p < 0.05) in infected sheep. This is the first report on serotyping of BTV among small ruminants in Pakistan.

Published

2019

50. Generation of monoclonal antibodies against foot-and-mouth disease virus SAT 2 and the development of a lateral flow strip test for virus detection.

Author

Yang M, Mudabuka B, Quizon K, and Nfon C

Subjects

Africa epidemiology, Animals, Female, Foot-and-Mouth Disease epidemiology, Foot-and-Mouth Disease virology, Foot-and-Mouth Disease Virus classification, Foot-and-Mouth Disease Virus isolation & purification, Livestock, Mice, Mice, Inbred BALB C, Sensitivity and Specificity, Serogroup, Serotyping veterinary, Antibodies, Monoclonal immunology, Antibodies, Viral immunology, Chromatography, Affinity veterinary, Foot-and-Mouth Disease diagnosis, Foot-and-Mouth Disease Virus immunology

Abstract

Foot-and-mouth disease (FMD) remains a major economic concern for the livestock productivity in many developing countries and a continued threat to countries that are disease free because of its potential devastating impact on agricultural, food chain and tourism sectors. FMD virus (FMDV) is recognized as having seven serotypes: O, A, C, Asia 1, South African Territories (SAT) 1, 2, 3 and multiple subtypes within each serotype. FMD outbreaks due to SAT 2 have been reported in many African countries. The development of a rapid and easily performed test for FMD detection is critical for controlling FMD outbreaks and containing its spread. The present project developed a lateral flow immunochromatographic (LFI) strip test for the rapid detection of FMDV SAT 2. A panel of monoclonal antibodies (mAbs) against FMDV serotype SAT 2 was produced and characterized. One mAb (#10) was selected as the capture mAb because it reacted to all 23 SAT 2 isolates archived at the National Center for Foreign Animal Disease. The LFI strip test was developed using biotin-conjugated mAb #10, and the colloid gold-conjugated FMDV serotype-independent mAb as the detection mAb. A generic Rapid Assay Device (gRAD) with one test line and a control line was used for the test. The LFI strip test detected all 23 tested SAT 2 isolates and recent outbreak strains. The results indicated that the diagnostic specificity and sensitivity of the LFI strip test were greater than the double antibody sandwich (DAS) DAS ELISA. The ability of the LFI strip test to produce rapid diagnostic results will be useful for early on-site diagnosis during FMD outbreaks., (© 2018 Blackwell Verlag GmbH.)

Published

2019