Figure 6.
BAHD1 interacts functionally and physically with the PRC2 complex. (A) Cas9-expressing F11KO HUDEP-2 cells were transduced with a lentiviral vector library encoding sgRNAs against 496 epigenetic modifier genes, selected in puromycin, then induced to undergo maturation for 5 days. Band3high and Band3low erythroblasts were FACS purified and analyzed by deep sequencing to compare the sgRNA representation. (B) Differential gene rank by RRA score from MAGeCK analysis32,33 of Band3high and Band3low erythroblasts. The PRC2 complex genes EED, EZH2, and RBBP4 are indicated. (C) WT and F11KO (clone F11KO #2) HUDEP-2 cells expressing Cas9 plus individual EZH2, SUZ12, EED, or control (Ctrl) sgRNAs were analyzed for Band3 expression after 5 days of induced erythroid maturation. The graph shows the mean ± SEM from 4 biological replicate experiments. (D) Pellets of cells described in panel C after 5 days of induced maturation. (E) 293T cells were transfected with plasmids encoding BAHD1-MYC and EZH2 (left panel) or BAHD1-MYC and EED (right panel). After 48 hours, cell lysates were immunoprecipitated with anti-MYC or IgG antibody, and western blot analysis was performed with the antibodies indicated at the right of each panel. The input represents 10% of the immunoprecipitated samples. (F) GSEA of differentially expressed genes in F11KO vs WT HUDEP-2 cells (left panel) or BAHD1-OE vs control HUDEP-2 cells (right panel), showing enrichment for a PRC2 target gene set. (G) Model showing the regulation of erythroid gene expression by FBXO11-mediated degradation of BAHD1. In early-stage erythroblasts, many erythroid genes are maintained in a bivalent state associated with concomitant H3K4me3 and H3K27me3 promoter marks and low-level expression. The heterochromatin-associated protein BAHD1 binds H3K3me3, recruits repressor proteins, and physically interacts with the PRC2 complex (an H3K27me3 writer). Recruitment of the erythroid transcription factor GATA1 is inhibited by BAHD1-induced heterochromatin. FBXO11 relieves transcriptional repression, facilitates GATA1 binding and promotes transition to a monovalent activating state by stimulating ubiquitin-mediated proteolysis of BAHD1, either before or after its binding to DNA and/or its interaction with corepressor proteins. NGS, next-generation sequencing. **P < .01; ***P < .001; ****P < .0001 (unpaired Student t test).

BAHD1 interacts functionally and physically with the PRC2 complex. (A) Cas9-expressing F11KO HUDEP-2 cells were transduced with a lentiviral vector library encoding sgRNAs against 496 epigenetic modifier genes, selected in puromycin, then induced to undergo maturation for 5 days. Band3high and Band3low erythroblasts were FACS purified and analyzed by deep sequencing to compare the sgRNA representation. (B) Differential gene rank by RRA score from MAGeCK analysis32,33  of Band3high and Band3low erythroblasts. The PRC2 complex genes EED, EZH2, and RBBP4 are indicated. (C) WT and F11KO (clone F11KO #2) HUDEP-2 cells expressing Cas9 plus individual EZH2, SUZ12, EED, or control (Ctrl) sgRNAs were analyzed for Band3 expression after 5 days of induced erythroid maturation. The graph shows the mean ± SEM from 4 biological replicate experiments. (D) Pellets of cells described in panel C after 5 days of induced maturation. (E) 293T cells were transfected with plasmids encoding BAHD1-MYC and EZH2 (left panel) or BAHD1-MYC and EED (right panel). After 48 hours, cell lysates were immunoprecipitated with anti-MYC or IgG antibody, and western blot analysis was performed with the antibodies indicated at the right of each panel. The input represents 10% of the immunoprecipitated samples. (F) GSEA of differentially expressed genes in F11KO vs WT HUDEP-2 cells (left panel) or BAHD1-OE vs control HUDEP-2 cells (right panel), showing enrichment for a PRC2 target gene set. (G) Model showing the regulation of erythroid gene expression by FBXO11-mediated degradation of BAHD1. In early-stage erythroblasts, many erythroid genes are maintained in a bivalent state associated with concomitant H3K4me3 and H3K27me3 promoter marks and low-level expression. The heterochromatin-associated protein BAHD1 binds H3K3me3, recruits repressor proteins, and physically interacts with the PRC2 complex (an H3K27me3 writer). Recruitment of the erythroid transcription factor GATA1 is inhibited by BAHD1-induced heterochromatin. FBXO11 relieves transcriptional repression, facilitates GATA1 binding and promotes transition to a monovalent activating state by stimulating ubiquitin-mediated proteolysis of BAHD1, either before or after its binding to DNA and/or its interaction with corepressor proteins. NGS, next-generation sequencing. **P < .01; ***P < .001; ****P < .0001 (unpaired Student t test).

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