Figure 5
Figure 5. Induction of the anterior hemangioblast program in animal caps requires signaling by activin in the absence of FGF. (A) Embryos at the 1-cell stage were injected in the animal pole with 200 to 400 fg activin mRNA either alone or in combination with 400 pg dominant-negative FGF receptor (XFD) mRNA. Embryos were grown to stage 8, and animal caps were excised and cultured in 1 × MBS to stage 18 and then processed for real-time RT-PCR analysis, probing for Scl (i), Runx1 (ii), SpiB (iii), Mpo (iv), Fli1 (v), and Flk1 (vi). Values represent the average of 3 experiments; error bars represent SD. (B) SpiB, Runx1, and Fli1 expression overlap in animal caps in which the anterior hemangioblast program has been induced by injection of activin and XFD mRNA; 400 fg activin plus 400 pg XFD mRNA were injected into the animal pole at the 1-cell stage, caps were excised at stage 8 and cultured to stage 18/19 as judged by sibling embryos. Caps were fixed, embedded, and sectioned in wax. Alternate 10 × 10-μm sections were probed for SpiB (i,ii), Runx1 (iii,iv), and Fli1 (v,vi) by in situ hybridization on sections. Original magnification ×10 for subpanels i, iii, and v. Original magnification ×20 for panels ii, iv, v, and vi (the same sections).

Induction of the anterior hemangioblast program in animal caps requires signaling by activin in the absence of FGF. (A) Embryos at the 1-cell stage were injected in the animal pole with 200 to 400 fg activin mRNA either alone or in combination with 400 pg dominant-negative FGF receptor (XFD) mRNA. Embryos were grown to stage 8, and animal caps were excised and cultured in 1 × MBS to stage 18 and then processed for real-time RT-PCR analysis, probing for Scl (i), Runx1 (ii), SpiB (iii), Mpo (iv), Fli1 (v), and Flk1 (vi). Values represent the average of 3 experiments; error bars represent SD. (B) SpiB, Runx1, and Fli1 expression overlap in animal caps in which the anterior hemangioblast program has been induced by injection of activin and XFD mRNA; 400 fg activin plus 400 pg XFD mRNA were injected into the animal pole at the 1-cell stage, caps were excised at stage 8 and cultured to stage 18/19 as judged by sibling embryos. Caps were fixed, embedded, and sectioned in wax. Alternate 10 × 10-μm sections were probed for SpiB (i,ii), Runx1 (iii,iv), and Fli1 (v,vi) by in situ hybridization on sections. Original magnification ×10 for subpanels i, iii, and v. Original magnification ×20 for panels ii, iv, v, and vi (the same sections).

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