For the 24 hr Matrigel outgrowth assays, MatTek dishes were coated (24 hr at 37°C) with 10% Matrigel mixed with either human IgG-Fc (Jackson Immunoresearch) or EphA4-Fc
(R&D Systems). To precluster the Fc fusion proteins for some experiments, we combined each Fc protein with mouse-anti-human Fc (Jackson Immunoresearch) for 1 hr at a 1:10 molar ratio. For each experiment, the spiral ganglion was removed at E12.5 and placed onto a precoated dish with normal culture medium and permitted to grow for 24 hr. For neuron and mesenchyme coculture experiments, a spiral ganglion and an equivalent-sized portion Selleck Talazoparib of otic mesenchyme were removed from the cochlea at E12.5 and transferred to Matrigel-coated MatTek dishes (5% for 1 hr at 37°C), containing solutions of either standard control MO or a Pou3f4-specific MO (GATCCTCTACTAGTTATAATGTGGC). Neuron and mesenchyme explants were plated approximately 1 mm from each other before receiving Endo-Porter (0.6% final; Gene Tools) to facilitate delivery of the MOs. After 2 days at 37°C, the MO and Endo-Porter-containing medium was NVP-BGJ398 replaced with normal culture medium and grown an additional 3 days. For some experiments, soluble preclustered
human IgG-Fc or EphA4-Fc was added to cultures following 2 days Morpholino exposure. Both IgG-Fc and EphA4-Fc were used at 10 nM based on a previous report (Brors et al., 2003). For culture experiments comparing Fc versus ephrin-B2-Fc (R&D Systems), we did not perform preclustering. ChIP was performed as described Phosphoribosylglycinamide formyltransferase previously (Jhingory et al., 2010) but with minor modification. E15.5 cochleae were isolated in
chilled PBS and then fixed for 20 min using 4% paraformaldehyde. The Agarose ChIP Kit (Pierce) was used for subsequent DNA digestion and precipitation. Approximately 8 μg of chicken anti-Pou3f4 or chicken IgY (negative control) and PrecipHen beads (Aves Labs) was used for IP. With resulting DNAs, we performed qPCR using SYBR Green. For each primer set, a standard curve was generated using mouse genomic DNA; control and experimental Ct values were compared to this standard curve for quantification. The data here represent at least two independent ChIPs and three qPCR analyses for each primer set. Please see Supplemental Experimental Procedures for lists of the antibodies, in situ hybridization probes, qPCR primers, quantification methods used in the study, and a description of the microarray that identified Epha4. We thank the members of the Kelley laboratory for their valuable discussions and technical assistance during this work. We thank Dr. Lisa Cunningham (NIH/National Institute on Deafness and other Communication Disorders [NIDCD]), Dr. Doris Wu (NIH/NIDCD), and Dr. Maria J. Donoghue (Georgetown University) for the critical reading of this manuscript. Epha4 null tissue was a kind gift from Dr. Maria J. Donoghue. Mr. Jonathan Stuckey was very helpful with the illustration in Figure 8.