Fig. 2.

ERG controls the expression of multiple regulators of coagulation in a tissue-specific manner. a qPCR screen analysis of genes involved in the regulation of coagulation in HUVEC was performed at 48 h after ERG inhibition by siRNA (n = 4–6 independent experiments). Data were normalised to GAPDH. b, c qPCR analysis of selected targets genes directly or indirectly involved in coagulation and endothelial markers in whole liver (b) and lung (c) lysates from adult control (Erg^fl/fl) and ERG-deficient (Erg^iEC-KO) mice (n = 4–5 per genotype). Data were normalised to 18S. d–e qPCR analysis of thrombomodulin (TM) mRNA expression in whole liver (d) and lung (e) lysates from adult Erg^fl/fl and Erg^iEC-KO mice (n = 5 per genotype). Data were normalised to 18S. f Immunoblot and quantification of WB for TM in protein extracts of lung samples from adult Erg^fl/fl and Erg^iEC-KO mice 30 days after tamoxifen injection (n = 3 mice per group). Data were normalized to GAPDH. All graphical data are mean ± s.e.m, *P < 0.05, Student’s t-test. Source data are provided as a Source Data file