Figure 3.
Figure 3. BL-CFC and endothelial potential of Hex-deficient ES cells. (A) BL-CFC potential of Hex+/+, Hex+/-, and Hex-/- EBs at the indicated time points. Numbers represent colonies per 2.5 × 104 cells plated. Data represent means ± SEMs (n = 3). (B) BL-CFC potential of Hex+/+ (□) and Hex-/- (▨) Flk-1+ cells isolated from day-4 EBs. Data represent means ± SEMs (n = 3). (C) RT-PCR expression analysis of Hex+/+ day-4 Flk-1+ cells cultured in VEGF and bFGF for varying periods of time. The 3′ cDNA was prepared by RT-PCR from the Flk-1+ population at the time of isolation (0) or following 3 or 5 days of culture. The cDNA samples were run on a 1.5% agarose gel, blotted, and probed separately with 3′ probes from the indicated genes. L32 was included as an internal control. Control populations include a pool of blast colonies (blast), a pool of primitive erythroid colonies (Ep), and the D4T endothelial cell line. (D) Flk-1+ cells (1 × 104 cells) isolated from day 4 Hex+/+ and Hex-/- were cultured on matrigel-coated wells with VEGF and bFGF. Cells were harvested and counted at days 3 and 5 of culture. Data represent means ± SEMs (n = 3). (E) Immunohistochemistry showing CD31+ endothelial cell clusters (red) and SMA-positive smooth muscle cells (green) (× 50) at 5 days of culture. (F) The size of the CD31+ area in 8 separate fields of each culture was evaluated by image analyzer. The mean size of the CD31+ area in Hex+/+ cultures was adjusted to 1. Data represent means ± SEM.

BL-CFC and endothelial potential of Hex-deficient ES cells. (A) BL-CFC potential of Hex+/+, Hex+/-, and Hex-/- EBs at the indicated time points. Numbers represent colonies per 2.5 × 104 cells plated. Data represent means ± SEMs (n = 3). (B) BL-CFC potential of Hex+/+ (□) and Hex-/- (▨) Flk-1+ cells isolated from day-4 EBs. Data represent means ± SEMs (n = 3). (C) RT-PCR expression analysis of Hex+/+ day-4 Flk-1+ cells cultured in VEGF and bFGF for varying periods of time. The 3′ cDNA was prepared by RT-PCR from the Flk-1+ population at the time of isolation (0) or following 3 or 5 days of culture. The cDNA samples were run on a 1.5% agarose gel, blotted, and probed separately with 3′ probes from the indicated genes. L32 was included as an internal control. Control populations include a pool of blast colonies (blast), a pool of primitive erythroid colonies (Ep), and the D4T endothelial cell line. (D) Flk-1+ cells (1 × 104 cells) isolated from day 4 Hex+/+ and Hex-/- were cultured on matrigel-coated wells with VEGF and bFGF. Cells were harvested and counted at days 3 and 5 of culture. Data represent means ± SEMs (n = 3). (E) Immunohistochemistry showing CD31+ endothelial cell clusters (red) and SMA-positive smooth muscle cells (green) (× 50) at 5 days of culture. (F) The size of the CD31+ area in 8 separate fields of each culture was evaluated by image analyzer. The mean size of the CD31+ area in Hex+/+ cultures was adjusted to 1. Data represent means ± SEM.

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