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. 2016 Nov 15;2016:8905675. doi: 10.1155/2016/8905675

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Copyright © 2016 Yuan Xin Goay et al.

This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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Analytical specificity of the PCR assay for detection of (a) STY2020 and (b) STY2021 genes, respectively (representative figures). Lane: M = 100 bp DNA ladder (Promega); N = negative control; 1 = S. Typhi; 2 = S. Paratyphi A; 3 = S. Paratyphi B; 4 = S. Paratyphi C; 5 = S. Enteritidis; 6 = S. Typhimurium; 7 = S. Weltevreden; 8 = S. Agona; 9 = S. Heidelberg; 10 = S. Poona; 11 = S. Hadar; 12 = S. Braenderup; 13 = S. Albany; 14 = S. Oslo; 15 = S. Kibi; 16 = S. Newport; 17 = S. Tshiongwe; 18 = S. Uppsala; 19 = S. Richmond; 20 = S. Bardo; 21 = S. Emek; 22 = S. Kissi; 23 = S. Virchow; 24 = S. Bordeaux; 25 = S. Regent; 26 = S. Java; 27 = S. Farsta; 28 = Shigella dysenteriae; 29 = Shigella flexneri; 30 = Shigella sonnei; 31 = Shigella boydii; 32 = Vibrio cholerae; 33 = Enterohemorrhagic Escherichia coli; 34 = Enteropathogenic Escherichia coli; 35 = Aeromonas hydrophila; 36 = Yersinia enterocolitica; and 37 = Klebsiella pneumonia. The PCR amplicon sizes for genes 16S rRNA, STY2020, and STY2021 were 1,326 bp, 429 bp, and 732 bp, respectively.