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. 2021 Sep 17;40(20):e107680. doi: 10.15252/embj.2021107680

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©2021 The Authors. Published under the terms of the CC BY 4.0 license

This is an open access article under the terms of the http://creativecommons.org/licenses/by/4.0/ License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.

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Figure EV5 — Quantification of the size of the T47D^DsRed cells within MDA‐MB‐231^{CFP;Cre;Control} or MDA‐MB‐231^{CFP;Cre;HA‐RASSF1C} tumors indicating equal contribution to tumor volume.

Representative 3 h migration paths of T47D^eGFP reporter cells within a single intravital imaging field of tumors co‐injected with MDA‐MB‐231^{CFP;Cre;Control} (Control, left) or MDA‐MB‐231^{CFP;Cre;HA‐RASSF1C} (RASSF1C, right).

Representative confocal images of lungs of mice with mammary gland tumors initiated by either the co‐injection of T47D^DsRed reporter cells with MDA‐MB‐231^{CFP;Cre;Control} or MDA‐MB‐231^{CFP;Cre;HA‐RASSF1C}. Scale bars represent 200 μm.

Quantification of the number of T47D^DsRed metastatic events found in the lungs of mice with mammary gland tumors initiated by MDA‐MB‐231^{CFP;Cre;Control} (Control) or MDA‐MB‐231^{CFP;Cre;HA‐RASSF1C} (RASSF1C) cells. Whole lung tile images were used for quantification, 6 of 10 μm sections each, 100 μm apart.

Data information: Data are analyzed by Student’s t‐test and represented as mean ± SEM.