Pathogens (Jan 2023)

A Multiplex PCR Assay for Differential Identification of Wild-type and Vaccine Strains of <i>Mycoplasma gallisepticum</i>

  • Sung-Il Kang,
  • O-Mi Lee,
  • Hye-Jin Lee,
  • Yong-Kuk Kwon,
  • Myeong Ju Chae,
  • Ji-Yeon Jeong,
  • Min-Su Kang

DOI
https://doi.org/10.3390/pathogens12010111
Journal volume & issue
Vol. 12, no. 1
p. 111

Abstract

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Mycoplasma gallisepticum (MG) can cause respiratory disease in chickens and result in serious economic losses in the chicken industry. The use of live vaccines has been a favorable option for the control of MG infection in multi-age commercial layers and broiler breeders. There are three live vaccines, including ts-11, 6/85, and F strain, that have been commonly used in various parts of the world, including South Korea. The definitive diagnosis of the infection, therefore, requires the differentiation of wild-type field strains of MG from the vaccine strains used. Thus, we aimed to develop a novel multiplex PCR assay to discriminate between vaccine strains (ts-11, 6/85, and F strain) and wild-type field strains of MG isolated from infected chickens. We designed four novel primer sets that are each specific to MG species, ts-11, 6/85, and F strain. The multiplex PCR assay using the primer sets differentially identified wild-type and vaccine strains of MG but did not detect other avian bacteria. The detection limit of this assay was 250 fg/μL of genomic DNA of each strain tested. In addition, this assay was applied to 36 MG strains isolated from chickens over the past 20 years in South Korea. As a result, the assay identified 22 wild-type strains and 14 vaccine strains. Consequently, the novel multiplex PCR assay can discriminate between vaccine and wild-type field strains of MG and could be a valuable tool for the diagnosis of MG infection in MG-vaccinated chicken flocks.

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