Development of a duplex TaqMan Real-Time Polymerase Chain Reaction for accurate identification and quantification of Salmonella enteritidis from laboratory samples and contaminated chicken eggs

Journal Article
Published on
byMDPI

Abstract

Salmonella enteritidis is a major causative agent of foodborne illnesses worldwide. As the traditional serotyping and quantification methods are labor-intensive, time-consuming, and expensive, faster and more convenient molecular diagnostic methods are needed. In this study, we developed and validated a rapid duplex TaqMan real-time polymerase chain reaction (PCR) for the accurate identification and quantification of S. enteritidis. The primers and TaqMan probes were designed based on the S. enteritidis-specific gene lygD and the Salmonella genus-specific gene invA. The melt curve and gel electrophoresis analysis showed that the designed primers had potent specificity for the amplification of lygD and invA. The duplex real-time PCR specifically identified S. enteritidis from a panel of 40 Salmonella strains that represented 29 serovars and 12 non-Salmonella organisms. The duplex real-time PCR assay detected four copies of S. enteritidis DNA per reaction. The intra- and inter- assays indicated a high degree of reproducibility. The real-time PCR could accurately detect and quantify S. enteritidis in chicken organs after Salmonella infection. Furthermore, the assay identified 100% of the S. enteritidis and Salmonella genus isolates from chicken egg samples with superior sensitivity after 6 h of pre-enrichment compared to the traditional culture method. Additionally, the most-probable-number (MPN) combined with qPCR and a shortened incubation time (MPN-qPCR-SIT) method was developed for the population determination of S. enteritidis and compared with various enumeration methods. Thus, we have established and validated a new duplex real-time PCR assay and MPN-qPCR-SIT method for the accurate detection and quantification of S. enteritidis, which could contribute to meeting the need for fast detection and identification in prevention and control measures for food safety.

Citation

Xiong, D., Zhou, Y., Song, L., Liu, B., Matchawe, C., Chen, X., Pelle, R., Jiao, X. and Pan, Z. 2022. Development of a duplex TaqMan Real-Time Polymerase Chain Reaction for accurate identification and quantification of Salmonella enteritidis from laboratory samples and contaminated chicken eggs. Foods 11:742.

Authors

  • Xiong, D.
  • Zhou, Y.
  • Song, L.
  • Liu, B.
  • Matchawe, C.
  • Chen, X.
  • Pelle, Roger
  • Jiao, X.
  • Pan, Z.

Related Publications

ILRI publication cover

Morphometric differentiation of three chicken ecotypes of Ethiopia using multivariate analysis

  • Markos, S.
  • Belay, Berhanu
  • Dessie, Tadelle

Training curriculum to underpin the development of training courses for chicken value chain actors

  • Yami, A.
  • Esatu, Wondmeneh
  • Rege, Ed
  • Hoa Hoang
  • Ngo Thi Kim Cuc
  • Sothyra Tum
  • Chhay Ty
  • Dessie, Tadelle
ILRI publication cover

Genomic analysis of Nigerian indigenous chickens reveals their genetic diversity and adaptation to heat-stress

  • Rachman, M.P.
  • Bamidele, O.
  • Dessie, Tadelle
  • Smith, J.
  • Hanotte, Olivier H.
  • Gheyas, A.A.

Diversity of Salmonella enterica phages isolated from chicken farms in Kenya

  • Gunathilake, K.M.D.
  • Makumi, Angela
  • Loignon, S.
  • Tremblay, D.
  • Labrie, S.
  • Svitek, Nicholas
  • Moineau, S.

Establishing farmer groups and linking smallholder farmers with input and output markets: A guide for smallholder based poultry production in the tropics

  • Yitayih, Mulugeta
  • Kassie, Girma T.
  • Dessie, Tadelle

Enhancing technical capacity on smallholder poultry development: Guidelines for developing a capacity development roadmap in SAPLING and other Tropical Poultry Genetics Solution (TPGS) countries

  • Yitayih, Mulugeta
  • Getachew, Fasil
  • Dessie, Tadelle