Figure 1. Phenotypic analysis of EGF-responsive primary cortical neurospheres.

Primary neurospheres were obtained from cerebral cortex cells isolated from WT and TLR3^−/− embryos at GD14. Cell populations in neurospheres were assayed by using flow cytometry. (a) Percentages of nestin-, GFAP- and Tubulin-β-III-expressing cells in neurospheres cultured for 24 hours or 7 days in proliferation medium supplemented with 20 ng/ml of EGF. Three independent experiments were performed with neurosphere-derived cells isolated from WT and TLR3^−/− embryos (n = 12). Results are expressed as percentages of total gated cells. Values represent mean ± SEM. (b) Dot plots of PAX6, TBR2, and nestin expression in cells derived from WT and TLR3^−/− cortical neurospheres cultured for 7 days. Numbers in quadrants represent the percentages of each subpopulation. Three independent cell culture assays were performed with cells isolated from WT and TLR3^−/− embryos (n = 12); data from one representative assay is shown. (c) Dot plots of TLR3 expression in nestin⁺, PAX6⁺ and TBR2⁺ WT cortical neurosphere cells cultured for 7 days. Numbers in quadrants represent the percentages of each subpopulation. Three independent cell culture assays were performed with cells isolated from WT embryos (n = 12); data from one representative assay is shown.