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. 2021 Jan 7;16(1):e0245175. doi: 10.1371/journal.pone.0245175

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© 2021 Janesomboon et al

This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

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Fig 2 — (A) Multiplex PCR amplification of DNA templates from B. thailandensis strains E264, DV1 (lanes 1–2), the BTCV strains E555, SBXPR001 (lanes 3–4), BPBM strains MSHR3326, MSHR4445 (lanes 5–6), B. pseudomallei strains K92643, 1026b (lanes 7–8), B. mallei strains NCTC3709, NCTC12938 (lanes 9–10), and B. humptydooensis strains MSMB43, MSMB1588 (lanes 11–12). (B) Singleplex PCR amplification of B. thailandensis strains E264, DV1 (Bth; lanes 1–2) and B. thailandensis strain E555, SBXPR001 (BTCV; lanes 3–4). Lanes P and N are positive (mixture of Burkholderia spp. DNA) and negative (distilled water) controls, respectively. Lane M is 100 bp DNA ladder.