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. 2016 Jan 11;11(1):e0145831. doi: 10.1371/journal.pone.0145831

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© 2016 Mallela 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 5 — A. Cells growing exponentially in YPD were further incubated without (upper plot) or with 20 μg ml^-1 myriocin (lower plot) for 4 hrs and LCB levels in the lipid extracts were determined by ESI-MS. A similar pretreatment with 2 μg ml^-1 of myriocin repressed LCB levels of ypr114w∆ and WT to the same degree, albeit less strongly (not shown). B. Plates containing myriocin with or without 20 mM NAC were incubated for 2 days (top sections W303 background, bottom sections BY4742 background). C. Strains in the W303 background were grown in YPD with or without myriocin (1.2 μg ml^-1) for 24 h and superoxide anions were detected by staining with DHE. After 24 h all strains had grown to the same density.