Your search keyword '"JOHNSON, WM"' showing total 9 results

1. Epidemiologic typing of Salmonella enterica serotype enteritidis in a Canada-wide outbreak of gastroenteritis due to contaminated cheese.

Author

Ahmed R, Soule G, Demczuk WH, Clark C, Khakhria R, Ratnam S, Marshall S, Ng LK, Woodward DL, Johnson WM, and Rodgers FG

Subjects

Bacterial Typing Techniques, Bacteriophage Typing, Canada epidemiology, Electrophoresis, Gel, Pulsed-Field, Gastroenteritis microbiology, Humans, Molecular Epidemiology, Salmonella Food Poisoning microbiology, Cheese microbiology, Disease Outbreaks, Gastroenteritis epidemiology, Salmonella Food Poisoning epidemiology, Salmonella enteritidis classification

Abstract

A major Canada-wide outbreak of gastroenteritis due to Salmonella enterica serotype Enteritidis phage type (PT) 8 occurred in 1998, and this was traced to contaminated cheese in a commercial lunch pack product. Phage typing and pulsed-field gel electrophoresis linked the clinical and cheese isolates of serotype Enteritidis but failed to differentiate outbreak from nonoutbreak PT 8 strains. Further differentiation was made by biotyping based on melibiose fermentation.

Published

2000

2. Multiplex PCR for detection of genes for Staphylococcus aureus enterotoxins, exfoliative toxins, toxic shock syndrome toxin 1, and methicillin resistance.

Author

Mehrotra M, Wang G, and Johnson WM

Subjects

Canada, Exfoliatins genetics, Humans, Nasal Mucosa microbiology, Netherlands, Restriction Mapping, Staphylococcus aureus classification, Staphylococcus aureus isolation & purification, Bacterial Toxins, Enterotoxins genetics, Genes, Bacterial, Methicillin Resistance genetics, Polymerase Chain Reaction methods, Staphylococcus aureus genetics, Superantigens

Abstract

A multiplex PCR assay for detection of genes for staphylococcal enterotoxins A to E (entA, entB, entC, entD, and entE), toxic shock syndrome toxin 1 (tst), exfoliative toxins A and B (etaA and etaB), and intrinsic methicillin resistance (mecA) was developed. Detection of femA was used as an internal positive control. The multiplex PCR assay combined the primers for sea to see and femA in one set and those for eta, etb, tst, mecA, and femA in the other set. Validation of the assay was performed using 176 human isolates of Staphylococcus aureus. This assay offers a very specific, quick, reliable, and inexpensive alternative to conventional PCR assays used in clinical laboratories to identify various staphylococcal toxin genes.

Published

2000

3. Serogroup B, electrophoretic type 15 Neisseria meningitidis in Canada.

Author

Kertesz DA, Coulthart MB, Ryan JA, Johnson WM, and Ashton FE

Subjects

Adult, Canada, Child, Preschool, Electrophoresis, Electrophoresis, Gel, Pulsed-Field, Female, Humans, Infant, Male, Middle Aged, Serotyping, Meningococcal Infections microbiology, Neisseria meningitidis classification

Abstract

Invasive meningococcal disease is nationally reportable in Canada. In recent years, a serogroup C genotype, designated electrophoretic type 15 (ET15), has been the most frequently isolated meningococcal genotype in Canada and has caused epidemics across the country. Between August 1993 and September 1995, there were 9 cases of invasive meningococcal disease caused by a variant of this genotype, expressing group B capsular polysaccharide. The appearance of serogroup B:ET15 was related temporally and geographically to mass immunization campaigns designed to control serogroup C meningococcal disease in Canada. Since there is no vaccine available to control serogroup B meningococcal disease, the appearance of this variant may have public-health significance if it demonstrates the same epidemic potential as its serogroup C counterpart.

Published

1998

4. Human salmonellosis associated with exotic pets.

Author

Woodward DL, Khakhria R, and Johnson WM

Subjects

Animals, Canada, Hedgehogs, Humans, Iguanas, Lizards, Ranidae, Retrospective Studies, Salmonella isolation & purification, Salmonella Infections epidemiology, Serotyping, Turtles, United States epidemiology, Zoonoses epidemiology, Animals, Domestic microbiology, Salmonella classification, Salmonella Infections transmission

Abstract

During the period from 1994 to 1996, an increase in the number of laboratory-confirmed cases of human salmonellosis associated with exposure to exotic pets including iguanas, pet turtles, sugar gliders, and hedgehogs was observed in Canada. Pet turtle-associated salmonellosis was recognized as a serious public health problem in the 1960s and 1970s, and in February 1975 legislation banning the importation of turtles into Canada was enacted by Agriculture Canada. Reptile-associated salmonellosis is once again being recognized as a resurgent disease. From 1993 to 1995, there were more than 20,000 laboratory-confirmed human cases of salmonellosis in Canada. The major source of Salmonella infection is food; however, an estimated 3 to 5% of all cases of salmonellosis in humans are associated with exposure to exotic pets. Among the isolates from these patients with salmonellosis, a variety of Salmonella serotypes were also associated with exotic pets and included the following: S. java, S. stanley, S. poona, S. jangwani, S. tilene, S. litchfield, S. manhattan, S. pomona, S. miami, S. rubislaw, S. marina subsp. IV, and S. wassenaar subsp. IV.

Published

1997

5. Salmonella isolated from humans, animals and other sources in Canada, 1983-92.

Author

Khakhria R, Woodward D, Johnson WM, and Poppe C

Subjects

Animals, Bacterial Typing Techniques, Canada epidemiology, Cattle, Chickens, Disease Outbreaks, Food Microbiology, Humans, Incidence, Meat microbiology, Population Surveillance, Poultry microbiology, Prevalence, Salmonella immunology, Salmonella Infections microbiology, Seroepidemiologic Studies, Swine, Travel, Salmonella isolation & purification, Salmonella Infections epidemiology

Abstract

A total of 89760 human and 22551 non-human isolates of salmonella were serotyped in Canada during the period 1983-92. There were 2180 reported outbreaks associated with 10065 cases during the 10-year period. The most common salmonella serovars isolated from human and non-human sources were S. typhimurium and S. hadar. The third and fourth most common serovars from human sources were S. enteritidis and S. heidelberg, respectively, and from non-human sources they were S. heidelberg and S. infantis. The number of S. typhimurium isolations from human and non-human sources showed a downward trend over the 10-year period. A total of 222 outbreaks of S. typhimurium associated with 1622 cases occurred. The S. hadar isolations from human and non-human sources reached a peak during the years 1987-90 and declined thereafter. The number of human isolates of S. enteritidis increased until 1985 and fluctuated at a level of 8.3-12.8% of all human isolates thereafter. Seventy-three outbreaks of S. enteritidis infection associated with 568 cases occurred. More than 50% of the S. enteritidis infections in humans were caused by phage type (PT) 8. During the review period, infections caused by PT4 were less common and were almost exclusively found in people who had travelled abroad. The annual isolation rates of S. heidelberg from human and non-human sources increased steadily during the period. Bacteriophage typing of serovars from outbreaks showed that contaminated food products of poultry and bovine origin were common sources of human infection. Salmonella typhi was identified as the cause of 43 small outbreaks affecting 116 persons.

Published

1997

6. Identification of epidemiologic markers for Neisseria meningitidis using difference analysis.

Author

Strathdee CA and Johnson WM

Subjects

Bacterial Outer Membrane Proteins genetics, Base Sequence, Canada, Cloning, Molecular methods, DNA Primers chemistry, Dihydropteroate Synthase genetics, Humans, Molecular Sequence Data, Polymorphism, Genetic, DNA, Bacterial genetics, Disease Outbreaks, Genetic Markers, Meningitis, Meningococcal epidemiology, Neisseria meningitidis genetics, Polymerase Chain Reaction methods

Abstract

The feasibility of identifying epidemiologic markers based solely on the identification of DNA fragments present in outbreak-associated isolates was investigated using Neisseria meningitidis (Nm) as a model system. The clonal structure of Nm has been well characterized using multilocus electrophoresis. In Canada, electrophoretic types ET1, ET5, ET9 and ET21 are being displaced from the natural population by type ET15, and the latter type is associated with an increased prevalence of serogroup C meningococcal disease. Difference analysis, which uses subtractive hybridization and polymerase chain reaction (PCR) amplification, was employed to identify amplifiable DNA fragments (amplicons) that differ between the ET15 and the ET1, ET5, ET9 and ET21 genomes. 14 amplicons were cloned which were further characterized by Southern blot analysis to identify six amplicons that represent fragments either unique to or highly polymorphic in the ET15 genome. Oligodeoxyribonucleotide primer pairs were designed for each of the six amplicons, and PCR amplification was used to determine their prevalence across a panel of 167 Nm isolates representative of other serogroups and ETs. Among group C isolates only two of the six amplicons, designated as A and G, were effective in discriminating ET15 from non-ET15 isolates. Amplicon A detects a deletion in the dhps gene which effectively differentiates sulfonamide-sensitive and -resistant serogroup C isolates. The frequency of amplicon A and G detection in the other serogroups and ETs was too great to facilitate their direct use as diagnostic markers for the differentiation of virulent Nm isolates.

Published

1995

7. Genomic fingerprinting of Neisseria meningitidis associated with group C meningococcal disease in Canada.

Author

Strathdee CA, Tyler SD, Ryan JA, Johnson WM, and Ashton FE

Subjects

Canada epidemiology, Electrophoresis, Humans, Meningococcal Infections epidemiology, Neisseria meningitidis classification, DNA Fingerprinting, DNA, Bacterial analysis, Disease Outbreaks, Meningococcal Infections microbiology, Neisseria meningitidis genetics

Abstract

A single electrophoretic type (ET15) of Neisseria meningitidis has been associated with an increased incidence of group C meningococcal disease in Canada. Genomic fingerprinting through pulsed-field gel electrophoresis of chromosomal DNA was used to characterize the clonal relationship among meningococcal isolates of different electrophoretic types and among isolates within ET15. The genomic fingerprints of the ET15 isolates, while similar as a group, were sufficiently distinct to confirm linkage for four pairs of strains from focal outbreaks and differed markedly from those of the other common electrophoretic types, ET5, ET9, and ET21.

Published

1993

8. Streptococcal erythrogenic toxin genes: detection by polymerase chain reaction and association with disease in strains isolated in Canada from 1940 to 1991.

Author

Tyler SD, Johnson WM, Huang JC, Ashton FE, Wang G, Low DE, and Rozee KR

Subjects

Base Sequence, Canada, DNA, Bacterial genetics, Gene Frequency, Genes, Bacterial, Genotype, Humans, Molecular Sequence Data, Oligonucleotide Probes, Pharyngitis microbiology, Polymerase Chain Reaction statistics & numerical data, Scarlet Fever microbiology, Sensitivity and Specificity, Streptococcus pyogenes isolation & purification, Bacterial Proteins, Exotoxins genetics, Membrane Proteins, Streptococcal Infections microbiology, Streptococcus pyogenes genetics

Abstract

The presence of genes encoding pyrogenic exotoxins type A (speA), B (speB), and C (speC) and streptolysin O (slo) was determined by the polymerase chain reaction (PCR) to target specific sequences in 152 strains of group A streptococci. These included reference strains, representative M and T type strains, and strains associated with scarlet fever and pharyngitis collected between 1940 to 1991 and included strains from patients with severe invasive streptococcal infections. PCR amplicons were detected by agarose gel electrophoresis, and specificity was established by restriction fragment analysis. The frequency of occurrence for each target gene among all strains tested was 33.6% for speA, 99.3% for speB, 28.9% for speC, and 100% for slo. Strains of non-group A streptococci, recognized toxigenic bacterial pathogens, and pneumolysin-producing Streptococcus pneumoniae strains were negative for all targeted gene sequences. Detection limits in the PCR were found to be 100 pg of total nucleic acids for the speB and speC genes and 1 ng for the speA and slo genes. Isolates associated with scarlet fever, pharyngitis, and severe invasive infections showed statistically significant differences in the presence of speA, with scarlet fever strains having the highest association (81.3%), severe infections the next highest association (42.9%), and pharyngitis the lowest association (18.4%). Although no significant differences were observed in speC frequencies in isolated associated with the three disease categories, a genotype of speB slo was significantly higher in isolates associated with pharyngitis (54.1%) than in strains associated with scarlet fever (18.8%) or severe invasive disease (23.8%). Streptolysin O targets were present in all the isolates tested, and only a single strain (T-11-M-11) was devoid of targeted speB sequences, thereby demonstrating that neither speB nor slo is associated with any particular clinical presentation.

Published

1992

9. Cytotoxic Escherichia coli O157:H7 associated with haemorrhagic colitis in Canada.

Author

Johnson WM, Lior H, and Bezanson GS

Subjects

Canada, Cytotoxins biosynthesis, Disease Outbreaks epidemiology, Escherichia coli metabolism, Gastrointestinal Hemorrhage etiology, Humans, Colitis etiology, Escherichia coli classification, Escherichia coli Infections

Published

1983