It is a fast, reproducible, simple, specific and sensitive way to detect
nucleic acids, which could be used in clinical diagnostic tests in the future. The design of the assay gives it potential to be used for quantification, for detection of multiple other serotypes of Salmonella or to be modified for the detection of other bacterial samples. Also, more significantly, the sensitivity of the test and its confirmed low limit of detection, are promising factors for the important switch to direct detection from real clinical and environmental samples which have not been previously cultured and have low find more numbers of bacteria. Acknowledgements The authors would like to thank the staff at the Department of Veterinary Services, Nicosia Selleck Pembrolizumab for assisting in sample collection; S. Gilliland and J. Hezka for technical assistance. This work was supported by research funds from the University of Cyprus (awarded to L. G. Kostrikis) and the Birch Biomedical Research LLC. Electronic supplementary material Additional File 1: Oligonucleotide primers and molecular beacons in the real-time PCR assay. Table of primer and molecular beacon sequences used in this study. (DOC 63 KB) References 1. Gorman R, Adley CC: Characterization of Salmonella enterica serotype Typhimurium isolates from human, food, and animal sources in the Republic of Ireland. J Clin Microbiol 2004,42(5):2314–2316.CrossRefPubMed
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