Chd4 a301 081a

The following antibodies were used: α-Tubulin (T9026); Acetyl-Histone H4 (06–866 lot#2554112, EMD Millipore (Billerica, MA)); CHD4 (A301-081A, Bethyl Laboratories (Montgomery, TX)); FITC anti-mouse (715-095-150 lot#115855, Jackson ImmunoResearch (West Grove, PA)); FLAG M2 (F1804 lot#SLBG5673V and lot#124K6106); FLAG M2 (F3165 lot#SLBL1237V); HDAC2 (ab7029, lot#GR88809-7, Abcam (Cambridge, UK)); HRP anti-mouse (115-035-146, Jackson ImmunoResearch); MBD2 (A301-632A, Bethyl); mouse IgG (315-005-003 lot#120058, Jackson ImmunoResearch); MTA2 (ab8106 lot#GR185489-3, Abcam); TRITC anti-rabbit (711-025-152 lot#114768, Jackson ImmunoResearch); rabbit monoclonal antibodies against DUX4 (E5-5 and E14-3) were produced in collaboration with Epitomics and are described elsewhere (Geng et al., 2012 (link)).

For denaturing PAGE, samples were separated in NuPAGE Bis-Tris 4–12% gels (Life Technologies) using MOPS running buffer according to manufacturer's instructions. Gels were transferred to nitrocellulose membranes (Bio-Rad, Hercules, CA) using XCell Transfer Kit and Transfer Buffer (Life Technologies) according to manufacturer's instructions. BN-PAGE gels were first incubated in 8% acetic acid prior to transfer to PVDF membranes (Life Technologies). Protein detection was performed using the following antibodies: FLAG (M2-peroxidase labeled, A8592, Sigma-Aldrich), Sall4 (ab29112, Abcam, Cambridge, UK), Chd4 (A301–081A, Bethyl Laboratories Inc., Montgomery, TX), Hdac2 (sc-7899, Santa Cruz, Biotechnology Inc., Dallas, TX), Wdr5 (A302–430A, Bethyl Laboratories Inc.), Wdr5 (A302–429A, Bethyl Laboratories Inc.), and Rbbp4 (ab1765, Abcam).