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Development and evaluation of temperature-sensitive Mycoplasma anserisalpingitidis clones as vaccine candidates.
Beko, Katinka; Grózner, Dénes; Mitter, Alexa; Udvari, Lilla; Földi, Dorottya; Wehmann, Eniko; Kovács, Áron B; Domán, Marianna; Bali, Krisztina; Bányai, Krisztián; Gyuris, Éva; Thuma, Ákos; Kreizinger, Zsuzsa; Gyuranecz, Miklós.
Afiliación
  • Beko K; Veterinary Medical Research Institute, Budapest, Hungary.
  • Grózner D; Veterinary Medical Research Institute, Budapest, Hungary.
  • Mitter A; MolliScience Ltd., Biatorbágy, Hungary.
  • Udvari L; Veterinary Medical Research Institute, Budapest, Hungary.
  • Földi D; MolliScience Ltd., Biatorbágy, Hungary.
  • Wehmann E; Veterinary Medical Research Institute, Budapest, Hungary.
  • Kovács ÁB; Veterinary Medical Research Institute, Budapest, Hungary.
  • Domán M; Veterinary Medical Research Institute, Budapest, Hungary.
  • Bali K; Veterinary Medical Research Institute, Budapest, Hungary.
  • Bányai K; Veterinary Medical Research Institute, Budapest, Hungary.
  • Gyuris É; Veterinary Medical Research Institute, Budapest, Hungary.
  • Thuma Á; Veterinary Medical Research Institute, Budapest, Hungary.
  • Kreizinger Z; Department of Pharmacology and Toxicology, University of Veterinary Medicine, Budapest, Hungary.
  • Gyuranecz M; Veterinary Diagnostic Directorate, National Food Chain Safety Office, Budapest, Hungary.
Avian Pathol ; 51(6): 535-549, 2022 Dec.
Article en En | MEDLINE | ID: mdl-35866306
Mycoplasma anserisalpingitidis is economically the most important pathogenic Mycoplasma species of waterfowl in Europe and Asia. The lack of commercially available vaccines against M. anserisalpingitidis had prompted this study with the aim to produce temperature-sensitive (ts+) clones as candidates for an attenuated live vaccine. The production of ts+ clones was performed by N-methyl-N'-nitro-N-nitrosoguanidine (NTG)-induced mutagenesis of Hungarian M. anserisalpingitidis field isolates. The clones were administered via eye-drop and intracloacally to 33-day-old geese. Colonization ability was examined by PCR and isolation from the trachea and cloaca, while the serological response of the birds was tested by ELISA. Pathological and histopathological examinations were performed in the eighth week after inoculation. Whole-genome sequence (WGS) analysis of the selected clone and its parent strain was also performed. NTG-treatment provided three ts+ mutants (MA177/1/11, MA177/1/12, MA271). MA271 was detected at the highest rate from cloacal (86.25%) and tracheal (30%) samples, while MA177/1/12 and MA271 elicited remarkable serological responses with 90% of the birds showing seroconversion. Re-isolates of MA271 remained ts+ throughout the experiment. Based on these properties, clone MA271 was found to be the most promising vaccine candidate. WGS analysis revealed 59 mutations in the genome of MA271 when compared to its parent strain, affecting both polypeptides involved in different cellular processes and proteins previously linked to bacterial fitness and virulence. Although further studies are needed to prove that MA271 is in all aspects a suitable vaccine strain, it is expected that this ts+ clone will contribute to the control of M. anserisalpingitidis infection.RESEARCH HIGHLIGHTS Three M. anserisalpingitidis ts+ vaccine candidates were produced by NTG-mutagenesis.Clone MA271 was able to colonize geese and induce a serological response.MA271 re-isolates remained ts+ during the 8-week-long experiment.WGS analysis revealed 59 mutations in the genome of MA271.
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Texto completo: 1 Banco de datos: MEDLINE Asunto principal: Enfermedades de las Aves de Corral / Mycoplasma / Infecciones por Mycoplasma Tipo de estudio: Diagnostic_studies Límite: Animals Idioma: En Revista: Avian Pathol Año: 2022 Tipo del documento: Article País de afiliación: Hungria

Texto completo: 1 Banco de datos: MEDLINE Asunto principal: Enfermedades de las Aves de Corral / Mycoplasma / Infecciones por Mycoplasma Tipo de estudio: Diagnostic_studies Límite: Animals Idioma: En Revista: Avian Pathol Año: 2022 Tipo del documento: Article País de afiliación: Hungria