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. 2019 Jun 18;10(3):e01138-19. doi: 10.1128/mBio.01138-19

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Copyright © 2019 Vang Nielsen et al.

This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license.

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FIG 1 — hipBST of E. coli O127 encodes a three-component toxin-antitoxin module. (A) Schematic showing a comparison of the hipBA and hipBST operons of E. coli K-12 and O127, respectively. Bent arrows pointing right indicate promoters. The hipBA operon contains two genes, hipB and hipA, while hipBST_O127 contains three genes, hipB_O127, hipS_O127, and hipT_O127. The region of hipA between the dashed lines exhibits sequence similarity to hipS_O127. The 8 amino acid residues of the P loop in HipA (150-VAGAQEKT-158) that binds phosphates of ATP are shown; the autophosphorylated S150 residue is shown in green (35). The homologous P loop and autophosphorylated serine in HipT_O127 were inferred by sequence similarity. (B) Overnight cultures of E. coli MG1655 harboring pSVN1 (pBAD33::hipT_O127) or the empty pBAD33 vector combined with pSVN111 (pNDM220::hipB_O127), pSVN109 (pNDM220::hipS_O127), pSVN110 (pNDM220::hipBS_O127), or the empty low-copy-number pNDM220 vector, as indicated, were diluted to obtain the same values of OD₆₀₀, centrifuged at 5,000 rpm for 5 min, washed in phosphate-buffered saline (PBS), and serially diluted before being spotted onto LB nutrient agar plates containing 0.2% glucose (to repress hipT_O127), 0.2% arabinose (to induce hipT_O127), or 0.2% arabinose plus 200 μM IPTG (to induce hipB_O127, hipS_O127, or hipBS_O127). (C) The strains used in the experiment whose results are shown in panel B were grown in LB medium plus appropriate antibiotics. Overnight cultures were diluted, cells were grown exponentially for at least 3 h until the doubling time appeared constant, and at an OD₆₀₀ of ≈0.3, arabinose (0.2%) was added to induce hipT_O127 (red arrow). After a further 1.5 h, IPTG (200 μM) was added to induce hipS_O127, hipB_O127, or hipBS_O127 (green arrow). (D and E) Viable counts of strains from the experiment whose results are shown in panels B and C before and after the addition of arabinose (0.2%) at an OD₆₀₀ of ≈0.3 (red arrow). At each time point, cell samples (0.5 ml) were washed in PBS before a 10-times dilution series was spotted on agar plates with glucose (0.2%) to repress hipT_O127 expression (D) or with glucose (0.2%) to repress hipT_O127 expression and IPTG (200 μM) to induce hipB_O127, hipS_O127, or hipBS_O127 (E). Plates were incubated for 16 h at 37°C before counting. Data points in panels C, D, and E represent mean values of results from at least three independent experiments, and error bars indicate standard deviations.