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. 2015 Jul 16;5:11944. doi: 10.1038/srep11944

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a) Linear control peptide and L and D cyclic peptides to form LDn6–8, respectively b) CHO-K1 were treated with ten-fold serial dilutions of LDn6–8 and LF_N-DTA in the presence of 20 nM PA for 30 minutes. The same experimental conditions were used as previously described. c) CHO-K1 were treated with 100 nM LD6–8 in the presence of 20 nM PA for 12 hours then subjected to cytosolic extraction for western blot, as previously described. Cropped blots are used in western blot data (c).