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. LAP2ß represses transcriptional activity in a dose-dependent manner. (A) LAP2ß represses the activity of E2F transcription factors. The E2F reporter (0.5 µg) and pCMV-ß-gal (0.5 µg) were co-transfected with expression vectors for E2F1 (0.15 µg), E2F4 (0.15 µg), E2F5 (0.15 µg), DP1 (0.15 µg), DP2 (0.15 µg), DP3 ${alpha}$ (0.3 µg), and LAP2ß (1 µg) into U2OS cells as indicated. (B) LAP2ß represses transcriptional activity of E2F5-DP3, p53, NF- ${kappa}$ B and the constitutive RSV promoter in a dose-dependent manner, but not that of the constitutive CMV promoter. The specific reporters (0.1 µg) and pCMV-ß-gal (0.5 µg), together with expression vectors for E2F5 (0.15 µg) and DP3 ${alpha}$ (0.3 µg, i), p53 (0.1 µg, ii), p65 (0.5 µg, iii), constitutive RSV promoter (0.1 µg, iv), constitutive CMV promoter (0.1 µg, v), and increasing doses of LAP2ß (0.1-2.0 µg) were transfected into U2OS cells as indicated. For each factor, its known endogenous inhibitor was assayed [Rb (1.0 µg), MDM2 (0.5 µg) and I ${kappa}$ B (1 µg)]. (C) LAP2ß represses the activity of p65 upon TNF ${alpha}$ stimulation. U2OS cells were transfected with increasing doses of LAP2ß (0.1-2.0 µg) and I ${kappa}$ B (1.0 µg). 12 hours before harvesting, the cells were stimulated with TNF ${alpha}$ (200 units). For all reporter assays, the values shown represent the averages ± S.D. of duplicate (A) or triplicate (B,C) readings after the luciferase values were normalized to the ß-galactosidase values and compared with the mock control.

Return to article