![BCL11A-dependent and independent cooperativities after combinatorial HRI depletion and HbF pharmacologic induction. (A) BCL11A transcript levels (normalized to DMSO control) in healthy CD34+ donors, as measured by qRT-PCR after shRNA scrambled control or HRI depletion with 2 independent shRNAs combined with either vehicle control or HbF pharmacologic induction (50 μM hydroxyurea [HU], 1 μM pomalidomide [Pom], or 0.125 μM UNC0638). (B) LRF/ZBTB7A transcript levels (normalized to DMSO control) as measured by qRT-PCR. Each symbol (circle, square, triangle) represents a biologically independent sample. (C) Representative western blot after shRNA scrambled control or HRI depletion with HRI shRNA #2 combined with HbF pharmacologic inducers. (D) Western blot quantification of BCL11A protein levels and LRF/ZBTB7A protein levels from 3 independent biological samples, normalized to total protein levels. Statistical analyses by 2-way analysis of variance. Significance vs DMSO control. Three independent biological replicates for all experiments. Error bars represent standard deviation. ***P < .001. (E) Hierarchical clustering using all genes (unsupervised) of RNA-Seq data after shRNA-mediated HRI depletion combined with vehicle control, 1 μM pomalidomide, or 0.125 μM UNC0638. (F) Principal component analysis of RNA-Seq data (red, donor replicate #1; blue, donor replicate #2). Percentage variance represented by each principal component axis. (G) RNA-Seq data visualized as log2 fold change in expression of known HbF regulators. DMSO served as the pharmacologic vehicle control. Two independent biological replicates for RNA-Seq analysis. **Absolute change >1.5-fold and adjusted P < .05.](https://ash.silverchair-cdn.com/ash/content_public/journal/bloodadvances/4/18/10.1182_bloodadvances.2020002475/2/advancesadv2020002475f3.png?Expires=1720301161&Signature=it7sd~D~fApgEOUWu~-d~gdmxRw5X3GdWYeMlq3LtMrmmFdc7DXrB3~doZ5XqPeB5xfEnZEj3n9pWoBdKQ~urFZHhHQ5ofm6QGlbhb6VbVph8lOaDT-mJ~ia0hpPXKYmbk3qUpmkqo8Ag4IEvlf4WGuT92~4ZBJsaOOPt5y-TRedAk4Ma77l~oSpihU~r4YmdR~ojNMMQN8RV1Hvl8X6BqcIi7OXpDCO~PQ5vTAFWoGgWfFIftNA2Q6Ll9t31LD9-Xtcq3xueDP6TMt~SSGdINqL3eGRfOT5vcB7SAqq-X~9cfaUR8geU~SwP9jpI1iJZm9cTd6tjx1IMNUYIGd5qw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
BCL11A-dependent and independent cooperativities after combinatorial HRI depletion and HbF pharmacologic induction. (A) BCL11A transcript levels (normalized to DMSO control) in healthy CD34+ donors, as measured by qRT-PCR after shRNA scrambled control or HRI depletion with 2 independent shRNAs combined with either vehicle control or HbF pharmacologic induction (50 μM hydroxyurea [HU], 1 μM pomalidomide [Pom], or 0.125 μM UNC0638). (B) LRF/ZBTB7A transcript levels (normalized to DMSO control) as measured by qRT-PCR. Each symbol (circle, square, triangle) represents a biologically independent sample. (C) Representative western blot after shRNA scrambled control or HRI depletion with HRI shRNA #2 combined with HbF pharmacologic inducers. (D) Western blot quantification of BCL11A protein levels and LRF/ZBTB7A protein levels from 3 independent biological samples, normalized to total protein levels. Statistical analyses by 2-way analysis of variance. Significance vs DMSO control. Three independent biological replicates for all experiments. Error bars represent standard deviation. ***P < .001. (E) Hierarchical clustering using all genes (unsupervised) of RNA-Seq data after shRNA-mediated HRI depletion combined with vehicle control, 1 μM pomalidomide, or 0.125 μM UNC0638. (F) Principal component analysis of RNA-Seq data (red, donor replicate #1; blue, donor replicate #2). Percentage variance represented by each principal component axis. (G) RNA-Seq data visualized as log2 fold change in expression of known HbF regulators. DMSO served as the pharmacologic vehicle control. Two independent biological replicates for RNA-Seq analysis. **Absolute change >1.5-fold and adjusted P < .05.