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. 2015 Jul 30;2(8):288–298. doi: 10.15698/mic2015.08.217

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This is an open-access article released under the terms of the Creative Commons Attribution (CC BY) license, which allows the unrestricted use, distribution, and reproduction in any medium, provided the original author and source are acknowledged.

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(A) Cells treated with 30 µM LeuLeu-OMe were fixed and stained with PI and annexin-FITC, and analyzed by flow cytometry. Digitonin-permeabilized cells were used as a positive control for the stains.

(B, C) Cell stably expressing YFP-TbATG8.2 were cultivated in medium with or without 30 µM LeuLeu-OMe. Autophagosome formation was monitored by relocalization of YFP-TbATG8.2 from a cytoplasmic distribution in control cells to a punctate structures using fluorescence microscopy. Autophagosome formation was quantitated and the results are shown as mean ± SD from 3 independent experiments. Cells starved in cytomix for 2 h were used as a positive control.