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. 2014 Oct 14;9(10):e109428. doi: 10.1371/journal.pone.0109428

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© 2014 Wallkamm 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 properly credited.

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A) For studying long-range signaling, Xwnt5A-EGFP transfected HEK293 cells seeded on thinCerts TC chambers were transferred on cells transfected with the ATF2-Luc reporter and cultivated for additional 24 hours. To investigate paracrine signaling, cells transfected with Xwnt5A-EGFP were co-cultured with cells transfected with the ATF2-Luc reporter for 24 hours. To analyze both autocrine and paracrine signaling, the reporter and the Wnt ligand were cotransfected. B) Activation of the non-canonical Wnt reporter ATF2-Luc by co-transfected Wnt8, Wnt11 and Wnt5A. C) Activation of the non-canonical Wnt reporter ATF2-Luc by long-range Wnt8, Wnt11 and Wnt5A in a two-chamber assay. D) Xwnt5A-EGFP triggered ATF2-Luc activation depends on endocytosis. Wnt5A induced ATF2-Luc activation (cotransfection) was inhibited by addition of 5 µg/ml chlorpromazine (Chlo) and 150 µM genistein (Gen) 24 h before the measurement. Given are the mean values ± standard errors and the p-values according to Student's t-test, ns: not significant, n gives the number of transfections.