QUICK SEARCH:

[advanced]

	Author:		Keyword(s):

Home Help Feedback Subscriptions Archive Search Table of Contents

	Help viewing high resolution images
	Return to article

(Downloading may take up to 30 seconds.
If the slide opens in your browser, select File -> Save As to save it.)
Click on image to view larger version.

Fig. 1. An intact PI3K pathway is required for Hgf-induced Mdm2 translocation. (A) Upon Hgf stimulation, wild-type (+/+) Met induces Mdm2 translocation from the cytoplasm into the nucleus of cultured primary embryonic hepatocytes. By contrast, Met^2P, which has intact PI3K activity but reduced Akt signaling (met^2P/2P), does not trigger Mdm2 translocation. (B) Quantitative analysis of Mdm2 translocation in wild-type (+/+) and mutant (2P/2P) embryonic hepatocytes. Mdm2 translocation in wild-type hepatocytes is abolished in the presence of the PI3K inhibitor LY 294002 (10 µM). (C) In vivo inactivation of p53 restores hepatocyte survival in met^2P/2P mutant embryos. TUNEL staining of liver cryosections from E12.5 wild-type (+/+), met^2P/2P treated (met^2P/2P+PFT) or not (met^2P/2P) with the p53 inhibitor pifithrin- ${alpha}$ and double-homozygous met^2P/2P; p53^-/- embryos. (D) Quantitative analysis of TUNEL-positive cells in E12.5 liver sections of the indicated genotypes. The proportion of apoptotic cells is represented as fold increase compared with wild-type livers. The numbers of embryos analyzed in these studies are indicated (n). Arrows indicate nuclei. ^**P<0.001.

Return to article