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. Author manuscript; available in PMC: 2013 Apr 22.

Published in final edited form as: Dev Dyn. 2012 Jun 23;241(8):1274–1288. doi: 10.1002/dvdy.23817

Neural crest cells were cultured in vitro and chemically transfected with GFP. A Bar graph scoring cell shape of neural crest cells after electroporation (T-test: p<0.005, N=680 per each treatment). There were far fewer neural crest cells showing a migratory/mesenchymal morphology compared with GFP cells. B Morphology of neural crest cells chemically transfected with GFP, Slit2-GFP or MIF-GFP. C Graph showing individual cell area (y axis corresponds to μm² of cell surface) for neural crest cells after transfection. Cells expressing Slit2-GFP were significantly smaller than control-GFP or MIF-GFP expressing cells (T-test: p<0.0004 T-test, N=60 cells per each treatment).

Neural crest cells were cultured in vitro and chemically transfected with GFP. A Bar graph scoring cell shape of neural crest cells after electroporation (T-test: p<0.005, N=680 per each treatment). There were far fewer neural crest cells showing a migratory/mesenchymal morphology compared with GFP cells. B Morphology of neural crest cells chemically transfected with GFP, Slit2-GFP or MIF-GFP. C Graph showing individual cell area (y axis corresponds to μm² of cell surface) for neural crest cells after transfection. Cells expressing Slit2-GFP were significantly smaller than control-GFP or MIF-GFP expressing cells (T-test: p<0.0004 T-test, N=60 cells per each treatment).