Employment of 16S rDNA gene sequencing techniques for improved identification of difficult-to-identify bacterial veterinary pathogens

被引:0
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作者
John E. Moore
Yasunori Maeda
Jiru Xu
B. Cherie Millar
Peter H. Herold
V. M. J. Browne-Lauwers
Colin E. Goldsmith
Anne Loughrey
Paul J. Rooney
J. Stuart Elborn
Motoo Matsuda
机构
[1] Belfast City Hospital,Northern Ireland Public Health Laboratory, Department of Bacteriology
[2] Xian Jiatong University,Department of Pathogenic Biology
[3] Gortlands Veterinary Clinic,Northern Ireland Regional Adult Cystic Fibrosis Centre, Level 8
[4] Belfast City Hospital,Department of Respiratory Medicine, School of Medicine and Dentistry
[5] Queen’s University,Laboratory of Molecular Biology, School of Environmental Health Sciences
[6] Level 8,undefined
[7] Belfast City Hospital,undefined
[8] Azabu University,undefined
关键词
UPTC; PCR; 16S rRNA; Molecular diagnosis; Pyoderma;
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摘要
To employ 16S rDNA PCR and automated sequencing techniques to identify a collection of bacterial veterinary pathogens from avian, equine, canine and ovine sources, that have proven difficult to identify, employing conventional cultural techniques. Universal or “broad-range” eubacterial PCR was performed on a collection of 46 difficult-to-identify bacterial isolates originating from clinical veterinary specimens. 16S rDNA PCR was performed using two sets of universal primers to successfully generate a composite amplicon of 1,068 bp, which was sequenced to obtain each isolate’s identity. Sequence analysis was able to identify all isolates examined with relative ease. Where the use of molecular identification methods is justified, such as in outbreak control or bioterrorism in animal health, employment of partial 16S rDNA PCR and sequencing employing universal or “broad-range” 16S rDNA, provides a valuable and reliable method of identification of such pathogens.
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页码:1227 / 1232
页数:5
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