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Fig. 1. Cell-cell contact loss of RIE1- ${alpha}$ 5, but not RIE1- ${alpha}$ 5/1, cells after OXO treatment. (A) Stable cell lines ectopically expressing integrin ${alpha}$ 5 (RIE1- ${alpha}$ 5) or tailless ${alpha}$ 5 (RIE1- ${alpha}$ 5/1) were maintained, as described in Materials and Methods. Images for subconfluent cells in normal culture media were taken using a microscope equipped with a digital camera. Both cell lines generally form colonies. (B) Whole cell lysates from subconfluent cells were prepared for immunoblotting using an antibody against an extracellular region ( ${alpha}$ 5exo) or the cytoplasmic tail ( ${alpha}$ 5cyto) of the human integrin ${alpha}$ 5 subunit, or ${alpha}$ -tubulin. Data shown represent at least three independent experiments. (C) Chemical structure of 6-(1-oxobutyl)-5,8-dimethoxy-1,4-naphthoquinone (OXO). (D,E) Cells were seeded onto 10% FBS-DMEM-H-coated glass coverslips. Once confluent monolayers had been formed by incubation in 5% CO₂ at 37°C, cells were treated with either vehicle (DMSO) or OXO (10 µM) for 24 hours, prior to being immunostained for ZO1 (D) or $beta$ -catenin (E). Data shown are representative of three different experiments.

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