Your search keyword '"Lawes JR"' showing total 12 results

1. Bovine TB infection status in cattle in Great Britain in 2020

Author

Waller, ESL, primary, Brouwer, A, additional, Upton, PA, additional, Harris, KA, additional, Lawes, JR, additional, Duncan, D, additional, Avigad, R, additional, and Dale, J, additional

Published

2022

2. Bovine TB infection status in cattle inGreat Britain in 2018.

Author

Duncan D, Brouwer A, Harris KA, Lawes JR, Avigad R, Dale J, and Upton PA

Subjects

Animals, Cattle, Incidence, Mycobacterium bovis genetics, Prevalence, Tuberculin Test veterinary, United Kingdom epidemiology, Mycobacterium bovis isolation & purification, Sentinel Surveillance veterinary, Tuberculosis, Bovine epidemiology

Published

2020

3. Raw diets for dogs and cats: a review, with particular reference to microbiological hazards.

Author

Davies RH, Lawes JR, and Wales AD

Subjects

Animals, Cats, Diet, Dogs, Europe, Zoonoses, Cat Diseases, Dog Diseases

Abstract

There is a recent trend to feed pet dogs and cats in Britain and other developed countries on raw meat and animal by-products using either commercial preparations or home recipes. This shift from heat-treated processed food has been driven by perceived health benefits to pets and a suspicion of industrially produced pet food. The diets of wild-living related species have been used as a rationale for raw feeding, but differences in biology and lifestyle impose limitations on such comparisons. Formal evidence does exist for claims by raw-feeding proponents of an altered intestinal microbiome and (subjectively) improved stool quality. However, there is currently neither robust evidence nor identified plausible mechanisms for many of the wide range of other claimed benefits. There are documented risks associated with raw feeding, principally malnutrition (inexpert formulation and testing of diets) and infection affecting pets and/or household members. Surveys in Europe and North America have consistently found Salmonella species in a proportion of samples, typically of fresh-frozen commercial diets. Another emerging issue concerns the risk of introducing antimicrobial-resistant bacteria. Raw pet food commonly exceeds hygiene thresholds for counts of Enterobacteriaceae. These bacteria often encode resistance to critically important antibiotics such as extended-spectrum cephalosporins, and raw-fed pets create an elevated risk of shedding such resistant bacteria. Other infectious organisms that may be of concern include Listeria, shiga toxigenic E scherichia coli , parasites such as Toxoplasma gondii and exotic agents such as the zoonotic livestock pathogen Brucella suis, recently identified in European Union and UK raw pet meat imported from Argentina., (© 2019 Crown Copyright. Journal of Small Animal Practice published by John Wiley & Sons Ltd on behalf of British Small Animal Veterinary Association.)

Published

2019

4. Bovine TB infection status in cattle in Great Britain in 2017.

Author

Perrin LD, Harris KA, Reynolds M, Lawes JR, Frost S, Brouwer A, Dale J, Palkopoulou E, and Upton PA

Subjects

Animals, Cattle, Incidence, United Kingdom epidemiology, Sentinel Surveillance veterinary, Tuberculosis, Bovine epidemiology

Published

2019

5. Bovine TB surveillance in Great Britain in 2014.

Author

Lawes JR, Harris KA, Brouwer A, Broughan JM, Smith NH, and Upton PA

Subjects

Abattoirs, Animals, Autopsy veterinary, Cattle, Genotyping Techniques veterinary, Government Agencies, Incidence, Prevalence, Recurrence, Time Factors, Tuberculosis, Bovine microbiology, United Kingdom epidemiology, Sentinel Surveillance veterinary, Tuberculosis, Bovine epidemiology

Abstract

This report, provided by the APHA, summarises the key descriptive epidemiological parameters of bovine TB in cattle in Great Britain from January 1 to December 31, 2014. It summarises some of the temporal trends observed over a longer period and highlights some differences and similarities between Scotland, Wales and the three bovine TB risk areas of England. It updates the previous annual summaries for 2012 and 2013, also published inVeterinary Record(VR, June 14, 2014, vol 174, pp 600-604; March 28, 2015, vol 176, pp 326-330)., (British Veterinary Association.)

Published

2016

6. Bayesian analysis of culture and PCR methods for detection of Campylobacter spp. in broiler caecal samples.

Author

Arnold ME, Jones EM, Lawes JR, Vidal AB, Clifton-Hadley FA, Rodgers JD, and Powell LF

Subjects

Animals, Bayes Theorem, Campylobacter Infections veterinary, DNA, Bacterial analysis, DNA, Bacterial genetics, Campylobacter genetics, Campylobacter isolation & purification, Campylobacter Infections microbiology, Chickens microbiology, Feces microbiology, Polymerase Chain Reaction methods, Poultry Diseases microbiology

Abstract

The objective of this study was to estimate the sensitivity and specificity of a culture method and a polymerase chain reaction (PCR) method for detection of two Campylobacter species: C. jejuni and C. coli. Data were collected during a 3-year survey of UK broiler flocks, and consisted of parallel sampling of caeca from 436 batches of birds by both PCR and culture. Batches were stratified by season (summer/non-summer) and whether they were the first depopulation of the flock, resulting in four sub-populations. A Bayesian approach in the absence of a gold standard was adopted, and the sensitivity and specificity of the PCR and culture for each Campylobacter subtype was estimated, along with the true C. jejuni and C. coli prevalence in each sub-population. Results indicated that the sensitivity of the culture method was higher than that of PCR in detecting both species when the samples were derived from populations infected with at most one species of Campylobacter. However, from a mixed population, the sensitivity of culture for detecting both C. jejuni or C. coli is reduced while PCR is potentially able to detect both species, although the total probability of correctly identifying at least one species by PCR is similar to that of the culture method.

Published

2015

7. The prevalence of Campylobacter spp. in broiler flocks and on broiler carcases, and the risks associated with highly contaminated carcases.

Author

Powell LF, Lawes JR, Clifton-Hadley FA, Rodgers J, Harris K, Evans SJ, and Vidal A

Subjects

Abattoirs, Animals, Campylobacter Infections mortality, Cecum microbiology, Odds Ratio, Prevalence, Risk Factors, Seasons, Skin microbiology, United Kingdom epidemiology, Campylobacter Infections epidemiology, Campylobacter coli isolation & purification, Campylobacter jejuni isolation & purification, Chickens microbiology, Food Microbiology

Abstract

A baseline survey on the prevalence of Campylobacter spp. in broiler flocks and Campylobacter spp. on broiler carcases in the UK was performed in 2008 in accordance with Commission Decision 2007/516/EC. Pooled caecal contents from each randomly selected slaughter batch, and neck and breast skin from a single carcase were examined for Campylobacter spp. The prevalence of Campylobacter in the caeca of broiler batches was 75·8% (303/400) compared to 87·3% (349/400) on broiler carcases. Overall, 27·3% of the carcases were found to be highly contaminated with Campylobacter (≥1000 c.f.u./g). Slaughter in the summer months (June, July, August) [odds ratio (OR) 3·50], previous partial depopulation of the flock (OR 3·37), and an increased mortality at 14 days (≥1·25% to <1·75%) (OR 2·54) were identified as significant risk factors for the most heavily Campylobacter-contaminated carcases. Four poultry companies and farm location were also found to be significantly associated with highly contaminated carcases.

Published

2012

8. Characteristics and comparative performance of direct culture, direct PCR and enumeration methods for detection and quantification of Campylobacter spp. in broiler caeca.

Author

Rodgers JD, Lawes JR, Vidal AB, Ellis-Iversen J, Ridley A, Pleydell EJ, Powell LF, Toszeghy M, Stapleton K, and Clifton-Hadley FA

Subjects

Agar, Animals, Campylobacter growth & development, Campylobacter physiology, Cecum microbiology, Polymerase Chain Reaction methods, Real-Time Polymerase Chain Reaction, Bacterial Load methods, Campylobacter isolation & purification, Campylobacter Infections veterinary, Chickens

Abstract

Detection and enumeration of Campylobacter spp. in broiler chicken flocks are key components of research and surveillance studies aimed at reducing Campylobacter infections in people. Direct culture of caecal contents onto selective agar is the typical method used to confirm flock colonisation. Modified charcoal cefoperazone deoxycholate agar (mCCDA) is commonly used for this method, although alternative selective media have been used. Additionally, PCR methods to detect Campylobacter DNA from caecal contents may provide a rapid alternative. However comparative performance data for these methods is limited and therefore required to ensure optimal detection methods for this sample type. In this study, 306 broiler caeca were tested for Campylobacter using direct culture on mCCDA, Skirrows and Preston agars and two real-time PCR methods, one specific for mapA/ceuE regions and another for the flaA gene region. Additionally, the suitability of spread plating and spiral plating methods for enumeration of Campylobacter and the impact of sample storage were assessed. This study confirmed modified CCDA as an optimal media for detection of Campylobacter in broiler caeca. It was significantly more sensitive than Skirrows or Preston agars. This study also demonstrated that the mapA/ceuE PCR had excellent agreement with culture on mCCDA and is a genuine alternative method. Spread plating and spiral plating methods were suitable for enumeration although spiral plating appeared more sensitive for stored samples (72 h). A 1 log reduction in viable Campylobacters was observed in stored samples, therefore storage effects should be considered for quantitative studies with broiler caeca., (Crown Copyright © 2012. Published by Elsevier B.V. All rights reserved.)

Published

2012

9. Investigation of prevalence and risk factors for Campylobacter in broiler flocks at slaughter: results from a UK survey.

Author

Lawes JR, Vidal A, Clifton-Hadley FA, Sayers R, Rodgers J, Snow L, Evans SJ, and Powell LF

Subjects

Abattoirs, Animals, Prevalence, Risk Factors, Seasons, Survival Analysis, United Kingdom epidemiology, Campylobacter Infections epidemiology, Campylobacter Infections microbiology, Campylobacter jejuni isolation & purification, Chickens, Poultry Diseases epidemiology, Poultry Diseases microbiology

Abstract

During 2007-2009 a UK-wide, 3-year stratified randomized survey of UK chicken broiler flocks was conducted to estimate the prevalence of Campylobacter-infected batches of birds at slaughter. Thirty-seven abattoirs, processing 88·3% of the total UK slaughter throughput, were recruited at the beginning of the survey. Of the 1174 slaughter batches sampled, 79·2% were found to be colonized with Campylobacter, the majority of isolates being C. jejuni. Previous partial depopulation of the flock [odds ratio (OR) 5·21], slaughter in the summer months (categorized as June, July and August; OR 14·27) or autumn months (categorized as September, October and November; OR 1·70) increasing bird age (40-41 days, OR 3·18; 42-45 days, OR 3·56; ⩾46 days, OR 13·43) and higher recent mortality level in the flock (1·00-1·49% mortality, OR 1·57; ⩾1·49% mortality, OR 2·74) were all identified as significant risk factors for Campylobacter colonization of the birds at slaughter. Time in transit to the slaughterhouse of more than 2·5 h was identified as a protective factor (OR 0·52).

Published

2012

10. Strain typing of Mycoplasma cynos isolates from dogs with respiratory disease.

Author

Mannering SA, McAuliffe L, Lawes JR, Erles K, and Brownlie J

Subjects

Animals, Bronchoalveolar Lavage Fluid microbiology, DNA Primers, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Dogs, Electrophoresis, Gel, Pulsed-Field, Female, Male, Mycoplasma genetics, Mycoplasma Infections diagnosis, Random Amplified Polymorphic DNA Technique, Respiratory Tract Infections diagnosis, Species Specificity, Trachea microbiology, Dog Diseases microbiology, Mycoplasma classification, Mycoplasma isolation & purification, Mycoplasma Infections veterinary, Respiratory Tract Infections veterinary

Abstract

The association of Mycoplasma cynos with canine infectious respiratory disease is increasingly being recognised. This study describes the strain typing of 14 M. cynos isolates cultured from trachea and bronchoalveolar lavage samples of six dogs with respiratory disease, from two separate kennels in the United Kingdom. The genetic similarity of the isolates was investigated using pulsed-field gel electrophoresis (PFGE) and random amplified polymorphic DNA (RAPD). Most of the isolates from four dogs housed at a re-homing kennel were genetically similar and some isolates from different dogs were indistinguishable by both PFGE and RAPD. These isolates were cultured from dogs with non-overlapping stays in the kennel, which may indicate maintenance of some strains within kennels. A small number of isolates showed much greater genetic heterogeneity and were genetically distinct from the main group of M. cynos strains. There was also a high degree of similarity of the M. cynos type strain (isolated from a dog with respiratory disease in Denmark in 1971) to at least one of the United Kingdom isolates using PFGE analysis, which may suggest possible conservation of pathogenic strains of M. cynos.

Published

2009

11. VNTR analysis reveals unexpected genetic diversity within Mycoplasma agalactiae, the main causative agent of contagious agalactia.

Author

McAuliffe L, Churchward CP, Lawes JR, Loria G, Ayling RD, and Nicholas RA

Subjects

Animals, DNA Fingerprinting, Electrophoresis, Gel, Pulsed-Field, Genotype, Goat Diseases microbiology, Goats, Molecular Epidemiology methods, Mycoplasma Infections microbiology, Random Amplified Polymorphic DNA Technique, Sheep, Sheep Diseases microbiology, Bacterial Typing Techniques methods, DNA, Bacterial genetics, Minisatellite Repeats, Mycoplasma Infections veterinary, Mycoplasma agalactiae classification, Mycoplasma agalactiae genetics, Polymorphism, Genetic

Abstract

Background: Mycoplasma agalactiae is the main cause of contagious agalactia, a serious disease of sheep and goats, which has major clinical and economic impacts. Previous studies of M. agalactiae have shown it to be unusually homogeneous and there are currently no available epidemiological techniques which enable a high degree of strain differentiation., Results: We have developed variable number tandem repeat (VNTR) analysis using the sequenced genome of the M. agalactiae type strain PG2. The PG2 genome was found to be replete with tandem repeat sequences and 4 were chosen for further analysis. VNTR 5 was located within the hypothetical protein MAG6170 a predicted lipoprotein. VNTR 14 was intergenic between the hypothetical protein MAG3350 and the hypothetical protein MAG3340. VNTR 17 was intergenic between the hypothetical protein MAG4060 and the hypothetical protein MAG4070 and VNTR 19 spanned the 5' end of the pseudogene for a lipoprotein MAG4310 and the 3' end of the hypothetical lipoprotein MAG4320. We have investigated the genetic diversity of 88 M. agalactiae isolates of wide geographic origin using VNTR analysis and compared it with pulsed field gel electrophoresis (PFGE) and random amplified polymorphic DNA (RAPD) analysis. Simpson's index of diversity was calculated to be 0.324 for PFGE and 0.574 for VNTR analysis. VNTR analysis revealed unexpected diversity within M. agalactiae with 9 different VNTR types discovered. Some correlation was found between geographical origin and the VNTR type of the isolates., Conclusion: VNTR analysis represents a useful, rapid first-line test for use in molecular epidemiological analysis of M. agalactiae for outbreak tracing and control.

Published

2008

12. 16S rDNA PCR and denaturing gradient gel electrophoresis; a single generic test for detecting and differentiating Mycoplasma species.

Author

McAuliffe L, Ellis RJ, Lawes JR, Ayling RD, and Nicholas RA

Subjects

Animals, DNA, Ribosomal analysis, Electrophoresis methods, Humans, Mycoplasma genetics, Mycoplasma Infections microbiology, Polymerase Chain Reaction, RNA, Ribosomal, 16S genetics, Mycoplasma classification, RNA, Ribosomal, 16S analysis

Abstract

Diagnosis of Mycoplasma infection is normally based on culture and serological tests, which can be time-consuming and laborious. A number of specific PCRs have been developed but to date there has not been a single generic test capable of detecting and differentiating mycoplasmas to a species level. This report describes the development of a new diagnostic test based on PCR of the 16S rRNA gene with Mycoplasma-specific primers and separation of the PCR product according to primary sequence using denaturing gradient gel electrophoresis (DGGE). DGGE enabled the differentiation of 67 Mycoplasma species of human and veterinary origin and represents a significant improvement on current tests as diagnosis of Mycoplasma infection can be made directly from clinical samples in less than 24 h.

Published

2005