Genotyping Brucella canis isolates using a highly discriminatory multilocus variable-number tandem-repeat analysis (MLVA) assay

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作者
Yi Yang
Yin Wang
Elizabeth Poulsen
Russell Ransburgh
Xuming Liu
Baoyan An
Nanyan Lu
Gary Anderson
Chengming Wang
Jianfa Bai
机构
[1] Kansas State University,Kansas State Veterinary Diagnostic Laboratory, College of Veterinary Medicine
[2] Yangzhou University College of Veterinary Medicine,Jiangsu Co
[3] Kansas State University,Innovation Center for the Prevention and Control of Important Animal Infectious Diseases and Zoonoses
[4] Kansas State University,Department of Diagnostic Medicine/Pathobiology, College of Veterinary Medicine
[5] Auburn University,Division of Biology
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Differentiation of Brucella canis from other Brucella species are mainly performed through PCR-based methods and multilocus variable-number tandem-repeat (VNTR) analysis (MLVA) procedures. Both PCR-based and MLVA methods are limited in discriminating B. canis strains. A new MLVA-13Bc method for B. canis genotyping was established by combining eight newly-developed VNTRs with five published ones. During 2010 and 2016, 377 B. canis PCR-positives were identified from 6,844 canine blood samples from 22 U.S. states, resulting in 229 B. canis isolates. The MLVA-13Bc method was able to differentiate each of these 229 isolates. The Hunter-Gaston Discriminatory Index of the individual VNTR loci ranged from 0.516 to 0.934 and the combined discriminatory index reached 1.000. Three major clusters (A, B and C) and 10 genotype groups were identified from the 229 B. canis isolates. Cluster A mainly contains genotype groups 1 and 2, and a few group 3 isolates; nearly all Cluster B isolates were from group 6; other genotype groups were classified into Cluster C. Our newly developed MLVA-13Bc assay is a highly discriminatory assay for B. canis genotyping, and can serve as a useful molecular epidemiological tool, especially for tracing the source of contamination in an event of a B. canis outbreak.
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