Armando Hung scite author profile

Twenty-five isolates of Ornithobacterium rhinotracheale were examined by agar gel precipitation, immunoperoxidase assay, sodium dodecyl sulfate-polyacrylamide gel electrophoresis, western blot analysis, and a polymerase chain reaction. All of the isolates were identified as serotype A. Protein profiles of whole cell extracts were similar for all the isolates, and a polypeptide with a molecular weight of 33 kD was a major component, being present in all the isolates. In the main, proteins of 33, 42, 52, and 66 kD were recognized in immunoblots with sera from chickens naturally exposed to O. rhinotracheale. A modified polymerase chain reaction assay identified O. rhinotracheale DNA from all the isolates and tracheal swabs, producing amplicons of 784 bp, and distinguished O. rhinotracheale from bacterial agents causing similar clinical signs.

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Detection of Vibrio campbellii and V. parahaemolyticus carrying full-length pirAB but only V. campbellii produces Pir toxins

Vicente

Taengphu

Hung

et al. 2020

Aquaculture

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Detection of antibodies to mycoplasmas in South American camelids

Hung

Alvarado

Lopez

et al. 1991

Research in Veterinary Science

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Cytokines expression in alpacas and llamas exposed to cold stress

Arias

Velapatiño

Hung

et al. 2016

Small Ruminant Research

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Armando Hung

Tilapia lake virus (TiLV) from Peru is genetically close to the Israeli isolates

Phenotypic and Molecular Characterization of Isolates of Ornithobacterium rhinotracheale from Peru

Detection of Vibrio campbellii and V. parahaemolyticus carrying full-length pirAB but only V. campbellii produces Pir toxins

Detection of antibodies to mycoplasmas in South American camelids

Cytokines expression in alpacas and llamas exposed to cold stress

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