Figure 4
Development and analysis of Cdh5−/−GFP+/+: Cdh5+/+GFP−/− chimeric mice embryos. (A) Schematic representation of the Cdh5 chimeric mouse development and analysis. Identification of Cdh5−/−GFP+/+ mES cells after electroporation of Cdh5 CRISPRs targeting exons 1 to 12 of the Cdh5 gene followed by karyotyping to exclude aneuploidy. Injection of Cdh5−/−GFP+ mES cells into WT mouse embryo of foster mothers and harvesting chimeric AGM at E10.5 for immunohistochemistry (GFP, Runx1, DAPI) and at E11.5 for cd41/c-Kit/cd45.2 expression, CFU analysis, transplant into sublethally irradiated mice as well as at E13.5 fetal liver for Lineage−Sca1+c-Kit+ expression, CFU analysis, and reconstitution capacity of fetal liver transplants. (B) Western analysis for Cdh5 and Hsp60 protein expression in E13.5 Cdh5−/−GFP+:Cdh5+/+GFP−-fetal liver–derived GFP− and GFP+ cells. To demonstrate the absence of Cdh5 at protein level, we sorted GFP+ and GFP− cells from fetal liver of E13.5 Cdh5−/−GFP+/+:Cdh5+/+GFP−/− chimeric mice embryos. Our western blot data confirmed the absence of Cdh5 protein in GFP+ cells. (C) The percentage of GFP chimerism in 11 E11.5 AGM, 6 E13.5 fetal liver, and 3 live pups. (D) Immunostaining of GFP (green), Runx1 (red), and DAPI (violet) in transverse sections of E10.5 AGM region, indicating that Cdh5−/− GFP+ cells produced Runx1+ GFP+ hematopoietic clusters in the ventral wall of the E10.5 dorsal aorta. Magnification, 40×.

Development and analysis of Cdh5−/−GFP+/+: Cdh5+/+GFP−/− chimeric mice embryos. (A) Schematic representation of the Cdh5 chimeric mouse development and analysis. Identification of Cdh5−/−GFP+/+ mES cells after electroporation of Cdh5 CRISPRs targeting exons 1 to 12 of the Cdh5 gene followed by karyotyping to exclude aneuploidy. Injection of Cdh5−/−GFP+ mES cells into WT mouse embryo of foster mothers and harvesting chimeric AGM at E10.5 for immunohistochemistry (GFP, Runx1, DAPI) and at E11.5 for cd41/c-Kit/cd45.2 expression, CFU analysis, transplant into sublethally irradiated mice as well as at E13.5 fetal liver for LineageSca1+c-Kit+ expression, CFU analysis, and reconstitution capacity of fetal liver transplants. (B) Western analysis for Cdh5 and Hsp60 protein expression in E13.5 Cdh5−/−GFP+:Cdh5+/+GFP-fetal liver–derived GFP and GFP+ cells. To demonstrate the absence of Cdh5 at protein level, we sorted GFP+ and GFP cells from fetal liver of E13.5 Cdh5−/−GFP+/+:Cdh5+/+GFP−/− chimeric mice embryos. Our western blot data confirmed the absence of Cdh5 protein in GFP+ cells. (C) The percentage of GFP chimerism in 11 E11.5 AGM, 6 E13.5 fetal liver, and 3 live pups. (D) Immunostaining of GFP (green), Runx1 (red), and DAPI (violet) in transverse sections of E10.5 AGM region, indicating that Cdh5−/− GFP+ cells produced Runx1+ GFP+ hematopoietic clusters in the ventral wall of the E10.5 dorsal aorta. Magnification, 40×.

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