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Peer-reviewed veterinary case report

Identification of Strain-Specific Sequences That Distinguish a Mycoplasma gallisepticum Vaccine Strain from Field Isolates.

Journal:
Journal of clinical microbiology
Year:
2017
Authors:
Ricketts, Camir et al.
Affiliation:
University of Georgia · United States
Species:
bird

Plain-English summary

Mycoplasma gallisepticum is a bacteria that causes serious health problems in poultry, leading to illness and economic losses. Vaccines are used to help control this issue, but sometimes the vaccine strains can become harmful again and are hard to tell apart from the natural strains found in the environment. Researchers studied the genetic differences between a specific vaccine strain and various field strains by sequencing their genomes. They found unique genetic markers in the vaccine strain that can be used to develop tests to quickly identify it, helping to ensure that the right strain is being used in vaccination efforts. This new testing method will improve the ability to differentiate between vaccine strains and field isolates.

Abstract

Despite attempts to control avian mycoplasmosis through management, vaccination, and surveillance, Mycoplasma gallisepticum continues to cause significant morbidity, mortality, and economic losses in poultry production. Live attenuated vaccines are commonly used in the poultry industry to control avian mycoplasmosis; unfortunately, some vaccines may revert to virulence and vaccine strains are generally difficult to distinguish from natural field isolates. In order to identify genome differences among vaccine revertants, vaccine strains, and field isolates, whole-genome sequencing of the M. gallisepticum vaccine strain ts-11 and several "ts-11-like" strains isolated from commercial flocks was performed using Illumina and 454 pyrosequencing and the sequenced genomes compared to the M. gallisepticum Rreference genome. The collective contigs for each strain were annotated using the fully annotated Mycoplasma reference genome. The analysis revealed genetic differences among vlhA alleles, as well as among genes annotated as coding for a cell wall surface anchor protein (mg0377) and a hypothetical protein gene, mg0359, unique to M. gallisepticum ts-11 vaccine strain. PCR protocols were designed to target 5 sequences unique to the M. gallisepticum ts-11 strain: vlhA3.04a, vlhA3.04b, vlhA3.05, mg0377, and mg0359 All ts-11 isolates were positive for the five gene alleles tested by PCR; however, 5 to 36% of field isolates were also positive for at least one of the alleles tested. A combination of PCR tests for vlhA3.04a, vlhA3.05, and mg0359 was able to distinguish the M. gallisepticum ts-11 vaccine strain from field isolates. This method will further supplement current approaches to quickly distinguish M. gallisepticum vaccine strains from field isolates.

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Original publication: https://pubmed.ncbi.nlm.nih.gov/27847370/