Endogenous Shoc2 localizes with active EGFR.

Abstract

<p><b>A</b>, Serum-starved Cos1 cells were treated with 10 ng/ml of EGF for 12 min at 37°C, fixed, permeabilized and stained with Shoc2 and EGFR (Ab528) antibodies followed by secondary Alexa548 donkey anti-rabbit and Alexa488 donkey anti-mouse antibodies were used. Insets show high magnification images of the regions of the cell indicated by white rectangles. Scale bars, 10 µm. <b>B</b>, High magnification images of the regions similar to those presented in <i>(</i><b><i>A</i></b><i>)</i> with examples of co-localization of Shoc2 and EGFR. Filter channels used for imaging of living cells as in <i>(</i><b><i>A</i></b><i>)</i> insets. Scale bars, 5 µm.</p

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