![Figure 2. Expression of the MFps protein partially restores migration and sprouting response of Flk1 null progenitors in vitro. (A) Schematic depiction of chicken–β-actin promoter-based construct used to overexpress the fpsMF cDNA in ES cells. (B) Western blot analysis of Flk1lacZ/lacZ null ES cell clones demonstrated a 2- to 3-fold increase in MFps in 10 of 11 puro-resistant clones compared with endogenous wild-type Fps protein levels in Flk1 null clones transfected with the empty puromycin construct (protein concentrations were standardized against β-actin levels [lower blot in B]). (C-D) Flk1lacZ/+ embryoid bodies showed endothelial migration and vascular channel formation, indicated by arrows. (E) Flk1GFP/+ embryoid bodies demonstrated angiogenic sprouting activity, indicated by arrows. (F-G) Flk1lacZ/lacZ embryoid bodies demonstrated dramatically reduced numbers of X-gal–stained cells and little migration or sprouting (arrowheads). (H) Similarly, Flk1GFP/GFP embryoid body–derived cells showed little EGFP expression and no migration or sprouting activity (arrowheads). (I-J) MFps-expressing Flk1lacZ/lacZ embryoid bodies showed an increased number of X-gal–stained cells (asterisk in I) and increased sprouting activity (arrow in J). (K) MFps-expressing Flk1GFP/GFP embryoid body–derived cells displayed increased EGFP expression, increased sprouting (arrow), and evidence of aberrant cellular morphology (asterisk). (L) Control Flk1lacZ/lacZ null EB-derived cells incubated with no primary antibody. Indirect PECAM immunofluorescence staining of Flk1lacZ/lacZ EB-derived cells (M) and MFps-expressing, Flk1lacZ/lacZ EB-derived cells (N).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/103/3/10.1182_blood-2003-07-2343/6/zh80030456090002.jpeg?Expires=1724847611&Signature=FRcfcrJGOGyjKaUH~Pwho8BiKuKpbm7WPEiCTVzeifSU9FajZWZxgENacy~IouJCww7jzrFu42WkT45M5sRa7ik0UYnSj2yrZgiODjOS9PK1ajw8SKydA2QMeJ6Xs0UpcmPX~vpI3j8lYSebuJgCiuE4DqkzNyfIV~e~o5yN-nw1tNc0UK2nhW4pGFKgv-pdF~6gfJquCQPQ74Qt-nsGeMj7ckAOJOlZPkA-kXFjUY8t7WV5HjCURs2tmlxu-yLNAlgUXHdPGNRFyBD2RJ6ADm0tkNF3ZBQEdgbbeNXQAMvrGjpA4-2i3tFymzbsdGNtV76mcf~llZa0dMkRRXp9qg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Expression of the MFps protein partially restores migration and sprouting response of Flk1 null progenitors in vitro. (A) Schematic depiction of chicken–β-actin promoter-based construct used to overexpress the fpsMF cDNA in ES cells. (B) Western blot analysis of Flk1lacZ/lacZ null ES cell clones demonstrated a 2- to 3-fold increase in MFps in 10 of 11 puro-resistant clones compared with endogenous wild-type Fps protein levels in Flk1 null clones transfected with the empty puromycin construct (protein concentrations were standardized against β-actin levels [lower blot in B]). (C-D) Flk1lacZ/+ embryoid bodies showed endothelial migration and vascular channel formation, indicated by arrows. (E) Flk1GFP/+ embryoid bodies demonstrated angiogenic sprouting activity, indicated by arrows. (F-G) Flk1lacZ/lacZ embryoid bodies demonstrated dramatically reduced numbers of X-gal–stained cells and little migration or sprouting (arrowheads). (H) Similarly, Flk1GFP/GFP embryoid body–derived cells showed little EGFP expression and no migration or sprouting activity (arrowheads). (I-J) MFps-expressing Flk1lacZ/lacZ embryoid bodies showed an increased number of X-gal–stained cells (asterisk in I) and increased sprouting activity (arrow in J). (K) MFps-expressing Flk1GFP/GFP embryoid body–derived cells displayed increased EGFP expression, increased sprouting (arrow), and evidence of aberrant cellular morphology (asterisk). (L) Control Flk1lacZ/lacZ null EB-derived cells incubated with no primary antibody. Indirect PECAM immunofluorescence staining of Flk1lacZ/lacZ EB-derived cells (M) and MFps-expressing, Flk1lacZ/lacZ EB-derived cells (N).
