IKAROS is required for the measured response of NOTCH target genes upon external NOTCH signaling
Authors:
Maud Lemarié aff001; Stefania Bottardi aff001; Lionel Mavoungou aff001; Helen Pak aff001; Eric Milot aff001
Authors place of work:
Maisonneuve-Rosemont Hospital Research Center; CIUSSS de l’est de l’Île de Montréal, Montréal, QC, Canada
aff001; Department of Medicine, Université de Montréal, Montréal, Québec, Canada
aff002
Published in the journal:
IKAROS is required for the measured response of NOTCH target genes upon external NOTCH signaling. PLoS Genet 17(3): e1009478. doi:10.1371/journal.pgen.1009478
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1009478
Summary
The tumor suppressor IKAROS binds and represses multiple NOTCH target genes. For their induction upon NOTCH signaling, IKAROS is removed and replaced by NOTCH Intracellular Domain (NICD)-associated proteins. However, IKAROS remains associated to other NOTCH activated genes upon signaling and induction. Whether IKAROS could participate to the induction of this second group of NOTCH activated genes is unknown. We analyzed the combined effect of IKAROS abrogation and NOTCH signaling on the expression of NOTCH activated genes in erythroid cells. In IKAROS-deleted cells, we observed that many of these genes were either overexpressed or no longer responsive to NOTCH signaling. IKAROS is then required for the organization of bivalent chromatin and poised transcription of NOTCH activated genes belonging to either of the aforementioned groups. Furthermore, we show that IKAROS-dependent poised organization of the NOTCH target Cdkn1a is also required for its adequate induction upon genotoxic insults. These results highlight the critical role played by IKAROS in establishing bivalent chromatin and transcriptional poised state at target genes for their activation by NOTCH or other stress signals.
Keywords:
DNA transcription – Gene expression – Gene regulation – Chromatin – Chromatin immunoprecipitation – Immunoprecipitation – Notch signaling – Tumor suppressor genes
Introduction
NOTCH signaling controls cell proliferation, differentiation, and apoptosis. It is required for hematopoietic stem/progenitor cells (HS/PC) interactions with their environment [1,2]. Disruption or abnormal expression of NOTCH receptors (NOTCH 1 to 4), particularly NOTCH 1, affects hematopoietic cell homeostasis and is common in hematological malignancies including T-cell Acute Lymphocytic Leukemia (T-ALL) [3,4]. NOTCH signaling/induction triggers sequential proteolytic cleavage events that promote nuclear localization of the NOTCH Intracellular Cleaved Domain (NICD). The nuclear NICD forms a ‘ternary complex’ with the transcription factor RBP-Jκ (CBF1) and the coactivator Mastermind-like, thereby favoring the activation of NOTCH target genes. In order to induce transcriptional activation, this ternary complex also recruits co-activators like p300 [5]. Chromatin recruitment of NICD and RBP-Jκ to different target genes can be unstable and may require other transcription factors to be efficiently bound [6]. In mammalian cells different transcription factors including members of the IKZF family such as IKAROS (IKZF1), HELIOS (IKZF2) and AIOLOS (IKZF3) were reported to interact with NICD [7,8]. However, whether these interactions can be functional and stabilize RBP-Jκ/NICD at specific genes is not known.
IKAROS has been identified as an important repressor of NOTCH target genes in lymphoid, myeloid and erythroid cells [7,9–13]. NOTCH target genes downregulated by IKAROS are marked by histone H3K27me3, which is a post-translational modification mainly catalyzed by the Polycomb Repressive Complex 2 (PRC2) methyltransferase enzyme, EZH2. IKAROS, in association with the Nucleosome Remodeling and Deacetylase (NuRD) complex, favors the recruitment of PRC2 to the chromatin [7,13,14] and in erythroid cells, EZH2 is required for IKAROS-dependent repression of Notch1 and Hes1 genes [13]. IKAROS can also repress activation of the NOTCH target genes pTα and Hes1 by preventing the recruitment of RBP-Jκ [13,15]. Thus, the repression of NOTCH target genes imposed by IKAROS is likely to be complementary to the canonical mechanism of such repression, which is mediated by chromatin recruitment of RBP-Jκ along with various corepressors [16].
Interestingly, genome wide analyses of transcription factors binding to chromatin suggest that IKAROS can be recruited with NICD to specific NOTCH target genes [7]. However, it remains unclear whether IKAROS participates to the activation of these NOTCH targets upon signaling. Indeed, IKAROS can also act as a transcriptional activator [17–19]. Unlike observed for other transcription factors capable to participate to both transcriptional repression and activation [20], proteomic analyses and target gene characterization have failed to fully clarify how IKAROS can either inhibit or promote transcription, even though this duality may depend on IKAROS ability to associate with several cofactors and complexes on chromatin [21,22]. For instance, the interaction between IKAROS and the NuRD complex, which is critical for chromatin organization of multiple gene regulatory regions in hematopoietic cells [22,23], can lead to either transcriptional repression [24,25] or activation when IKAROS conjointly associates with the NuRD and the Positive-Transcription Elongation Factor b (P-TEFb) complexes [18,23]. P-TEFb must be activated to release CDK9 from the inactive 7SK snRNP complex and promote transcription elongation. Once activated, CDK9 phosphorylates the Pol II C-terminal domain (CTD) at Ser-2, along with the negative elongation factors NELF and DSIF [26] and the conformational changes that follow allow Pol II to enter the productive phase of transcription elongation [27]. IKAROS interacts with CDK9 and PP1 [23,28] and thereby, facilitates their joined recruitment to specific genes [23]. IKAROS mutants with low affinity for PP1 no longer favor proficient transcriptional elongation [23], suggesting that the IKAROS-PP1 interaction promotes P-TEFb activation and, thereby, productive transcriptional elongation. Hence, by associating with different cofactors IKAROS can activate or repress target genes and control the rate of transcriptional elongation [18,23,29].
Homozygous IKAROS knockout mice (IkNull) are characterized by severe lymphopoietic defects [30] and succumb to leukemia or lymphoma with 100% penetrance [31]. IKAROS controls gene expression in HS/PC and several hematopoietic lineage cells [12,29,32–37]. Overexpression of dominant negative IKAROS isoforms frequently characterizes childhood B- and T-ALL [38]. IKAROS is also implicated in erythroid cell gene regulation [13,18,29,39,40] and IkNull mice develop anemia due to impairment of erythroid cell homeostasis [41,42]. However, it remains to be determined whether the IkNull effect on these cells is the consequence of the absence of IKAROS regulation imposed on NOTCH target genes.
In this work, we define the crosstalk between IKAROS and NOTCH signaling in erythroid cells. First, we compared the transcriptomes of IKAROS proficient (IkWT) vs IKAROS knockout (IkNull) erythroid cells co-cultured with the bone marrow-derived stroma cell line OP9 (control) or OP9-DL1, which ectopically expresses the NOTCH ligand DELTA-like 1 (DL1) [43]. We demonstrate that IKAROS is required for repression of multiple NOTCH target genes and, unexpectedly, is required for activation of others. The molecular characterization of several NOTCH regulated genes indicates that IKAROS and the ATP-dependent chromodomain helicase CHD4 of the NuRD complex are needed to establish bivalent chromatin and poised transcription of NOTCH target genes. Finally, we show that IKAROS is critical for poised transcription and for the controlled expression of the NOTCH target gene Cdkn1a (which encodes the P21WAF1/CIP1 protein) upon genotoxic insults.
Results
Experimental design and gene expression profiles upon IKAROS ablation and NOTCH induction
The main objective of this study was to define whether IKAROS could play a role in activation and repression of NOTCH target genes upon signaling in erythroid cells. To this purpose, embryonic day 14.5 (e14.5) mouse fetal livers were harvested from IKAROS wild type (IkWT) or knockout (IkNull) embryos and co-cultured for 48h with murine bone marrow stromal OP9 or OP9-DL1 cells [43–45]. Since OP9-DL1 cells have been engineered to constitutively express the NOTCH ligand Delta-like 1 (DL1; S1 Fig), they were used to trigger NOTCH signaling. After co-culture, the erythroid cells were isolated by FACS using the erythroid-specific marker Ter119 [46]. RNA was then extracted from IkWT/OP9; IkWT/OP9-DL1; IkNull/OP9; IkNull/OP9-DL1 Ter119+ cells and RNA-sequencing (RNA-seq) was performed in biological triplicate. The RNA-seq results were normalized with the DESeq package [47]. Briefly, the read count was normalized by size factor that was calculated by median ratio of gene counts relative to geometric mean per gene. If not otherwise stated, we retained differentially expressed genes displaying log2 fold change ≥ 0.8 or ≤ -0.8 and a False Discovery rate (FDR) < 0.05. A pilot assay revealed that the profile of the Ter119+ cells comprised within the P3 and P4 populations (S2 Fig and [13]) does not show variation, regardless of IKAROS expression or co-culture with OP9 or OP9-DL1 cells. Thus, like previously reported [48,49], the absence of IKAROS or induction of the NOTCH pathway only have minor effect on the fetal liver Ter119+ erythroid cells population and hence, will allow us to perform comparative analyses.
Although IKAROS is described as a repressor of NOTCH target genes [7,10,11,13,50], our results revealed two opposing patterns of gene regulation imposed by the absence of IKAROS in IkNull cells upon the induction of the NOTCH pathway, i.e., overexpression and downregulation. This outcome suggests that upon NOTCH induction, IKAROS can either repress or activate NOTCH target genes (Fig 1A).
We first analyzed genes overexpressed upon the loss of IKAROS. Comparative analysis of RNA-seq results of IkNull and IkWT cells co-cultured with either OP9 or OP9-DL1 cells revealed that 3130 genes were overexpressed in IkNull Ter119+ cells (Figs 1B and S3 and S1 File). As expected, and confirming the robustness of our experimental model, the expression of multiple NOTCH target genes increased upon DL1 mediated activation, in IkWT/OP9-DL1 vs IkWT/OP9 (S3 Table). These differentially expressed genes were analyzed with the bioinformatic software clustering DAVID [51,52] and regrouped according to cellular function (S4 Table). Analysis of the transcriptome in IkNull/OP9 vs IkWT/OP9 indicated that 2286 genes were overexpressed in IkNull/OP9 (χ+β; Figs 1B and S3 and S1 File), whereas analysis of IkNull/OP9-DL1 vs IkWT/OP9-DL1 revealed that 2631 genes were overexpressed in IkNull/OP9-DL1 (χ+α; Figs 1B and S3 and S1 File). The majority of the overexpressed genes was common to both comparative analyses (1787 genes: χ; Figs 1B and S3 and S1 File), suggesting that their expression is enhanced by the absence of IKAROS independently of extracellular NOTCH signaling. Functional annotation analysis of these genes revealed that regardless of NOTCH induction, IKAROS deletion has a dominant effect on the erythroid transcriptome and could affect the formation and functionality of erythroid cells since genes associated with cellular differentiation, homeostasis, signaling or iron transport are affected in IkNull cells (Fig 1C and 1D). The comparative analysis of gene expression profiles indicates that 499 genes are specifically overexpressed in IkNull/OP9 vs IkWT/OP9 and 844 genes are uniquely overexpressed in IkNull/OP9-DL1 vs IkWT/OP9-DL1 (respectively, β and α sets; Fig 1B and S1 File). Most of the 499 genes specifically overexpressed in IkNull/OP9 cells can be functionally annotated as cell proliferation, homeostasis, cell-to-cell communication, signaling and metabolism (S5 Table). Alternatively, IkNull/OP9-DL1 overexpressed genes are among others, annotated as regulators of gene transcription, inflammation, lymphoid cell activity and cell death (S6 Table). Thus, it can be assumed that the effect of IKAROS depletion and NOTCH induction further affects the transcriptome and, most likely, the function of erythroid cells.
The role of IKAROS as a repressor of NOTCH target genes has been well described [7,9–11,13]. Our RNA-seq analysis highlighted this repressive effect and, interestingly, allowed the identification of 223 genes whose overexpression requires the conjoint removal of IKAROS and induction of the NOTCH pathway (overexpression in IkNull/OP9-DL1 above all other conditions; Fig 2A and S2 File). We named this phenomenon the ‘additive effect’. Overexpression of two randomly selected genes (Il6 and Zfp446) in IkNull e14.5 fetal liver erythroid cells was confirmed by qRT-PCR (S4A Fig). The biological processes affected by the ‘additive effect’ include signaling, transcription control, metabolism, cellular growth, and proliferation (Fig 2B). Importantly, several genes characterized by the ‘additive effect’ encode tumor suppressors or oncogenes (S7 Table). Their abnormal expression can perturb hematopoietic cell homeostasis, contribute to malignant transformation, modify cell interactions with the niche, and/or affect cellular capacity to provide an adaptive immune response.
RNA-seq analysis also suggests that IKAROS deletion can transcriptionally desensitize NOTCH target genes to NOTCH induction (repressed genes; Fig 1A). Indeed, our data indicate that among genes activated by NOTCH (IkWT/OP9-DL1 vs IkWT/OP9), 21 are characterized by a significant decrease of their expression levels when IKAROS is missing (IkNull/OP9-DL1 vs IkWT/OP9-DL1), hence revealing that IKAROS can also contribute to NOTCH-associated gene transcriptional activation (Fig 2C). We named this phenomenon the ‘desensitize effect’. Functional annotation analysis of these genes was performed and indicated that 3 of the genes affected by IKAROS deletion in the context of NOTCH induction are involved in response to stimulus (Fig 2D). Oncogenes and tumor suppressor genes are also among the 21 genes requiring IKAROS to be properly stimulated upon NOTCH induction (S8 Table). In summary, these results suggest that IKAROS is required to prime and favor the physiological activation of different NOTCH target genes upon NOTCH induction.
IKAROS is required to attain a physiological response upon NOTCH induction
To elucidate the mechanism(s) used by IKAROS to either repress or prime NOTCH target genes, we studied the regulation of representative genes from either ‘groups’ i.e., those characterized by the ‘additive effect’ or the ‘desensitize effect’.
Among the 223 genes repressed by IKAROS and overexpressed upon joint NOTCH induction and IKAROS ablation (additive effect: Fig 2A and S9 Table), we chose Cdkn1a and Tp53, which encode respectively P21WAF1/CIP1 and TP53. TP53 and its downstream effector P21WAF1/CIP1 are critical factors in cancer biology (S7 Table). The expression levels of Cdkn1a and Tp53 as well as P21WAF1/CIP1 but not TP53, increase in IkNull erythroid cells (Fig 3A and 3B). Unchanged TP53 level in IkNull cells most likely relates to the fact that TP53 is highly regulated by post-translational mechanisms [53,54] that can mask the contribution of IKAROS.
Cdkn1a and Tp53 genes were previously identified as NOTCH target genes [55–57]. To determine whether IKAROS can directly regulate Cdkn1a and Tp53 genes, we performed chromatin immunoprecipitation (ChIP) with antibodies directed against IKAROS or NICD. IKAROS and NICD were detected at the Transcription Start Site (TSS) region and Open Reading Frame (ORF) of both genes (Fig 3C and 3E) in IkWT erythroid cells, thus indicating their recruitment to Cdkn1a and Tp53 NOTCH target genes in these cells. Since NICD binding to chromatin in freshly isolated erythroid cells was unexpected, we investigated NICD recruitment levels upon NOTCH induction in IkNull/OP9-DL1 cells (S4B Fig), whereby the expression of Cdkn1a and Tp53 is optimal. The results of ChIP performed in erythroid cells co-cultured with OP9-DL1 indicate that the recruitment of NICD to the chromatin of target genes dramatically increases, when compared to the 1-to-4-fold enrichment level observed in fetal liver erythroid cells (Figs S4B and 3C and 3D). Therefore, the weak NICD recruitment observed in fetal liver (Fig 3C and 3D) and in IkNull/OP9 (S4B Fig), might not be biologically significant and might be related to background detection associated with this specific antibody under our experimental conditions (i.e., double HCHO-EGS fixation; see Materials and Methods). Altogether, these results are reminiscent of those reported in thymocytes where IKAROS and RBP-Jκ can be recruited to the same regulatory regions of NOTCH activated genes [7]. Whether IKAROS can be co-recruited with RBP-Jκ and influence NICD recruitment to Cdkn1a and Tp53 in erythroid cells remains to be determined.
We further analyzed the additive effect of IKAROS abrogation and NOTCH induction by means of the OP9/OP9-DL1 co-culture system. In accordance with RNA-seq results, qRT-PCR analysis indicated that the expression levels of Cdkn1a and Tp53 significantly increase in IkNull/OP9-DL1 cells (Fig 4A and 4B), suggesting that the interplay between IKAROS and NOTCH is biologically relevant and particularly important to control the expression of P21WAF1/CIP1 (Figs 4C and 4D and S5), which is a critical regulator of cellular stress response [58,59].
IKAROS can influence transcriptional activation and elongation at selected target genes [17,36,60]. Hence, we employed ChIP assays to analyze the role of IKAROS for transcription control of Cdkn1a and Tp53 genes, by studying the distribution of histone post-translational modifications. IKAROS synergizes with the PRC2 enzyme EZH2 [13,14] and with the transcription elongation licensing factor P-TEFb [18,61]. Thus, H3K27me3 (deposited by EZH2) as well as H3K4me3 and H3K79me2, which are typical marks of productive elongation [62], were studied to define the role of IKAROS as transcriptional repressor and/or activator. In IkWT/OP9 and IkWT/OP9-DL1 cells, Cdkn1a TSS and ORF are marked with H3K4me3, H3K79me2 and H3K27me3 (Figs 5A and S6A). This chromatin state closely resembles bivalent chromatin of hematopoietic stem/progenitor cells harboring H3K4me3 and H3K27me3 [63] and marking genes poised or primed for rapid transcriptional activation [64]. Cdkn1a overexpression (Fig 4A), higher H3K79me2 and lower H3K27me3 levels at Cdkn1a regulatory regions in IkNull/OP9 and IkNull/OP9-DL1 cells, suggest that IKAROS is required for the bivalent organization of the chromatin and the poised state of this gene (Fig 5A). To test whether IKAROS could be required for the establishment of a bivalent chromatin characterized by the simultaneous co-occupancy of H3K4me3 and H3K27me3 to the Cdkn1a TSS, sequential ChIP (re-ChIP) [65] assays were carried out. The results obtained indicate that these histone post-translational modifications are simultaneously enriched at Cdkn1a TSS (S6B Fig), hence suggesting that IKAROS favors bivalent chromatin organization of the Cdkn1a gene prior to its induction by NOTCH. Finally, the peak of H3K79me2 levels at Cdkn1a TSS and ORF in IkNull/OP9-DL1 cells (Fig 5A), strengthened the additive effect imposed by IKAROS ablation and NOTCH induction.
In IkWT cells, chromatin at Tp53 contains H3K4me3 and H3K79me2 but not H3K27me3 marks (Fig 5B). The latter suggests that IKAROS does not contribute to PRC2 recruitment, bivalent chromatin organization (S6B Fig) or repression of this gene. Indeed, Tp53 is transcriptionally active in erythroid cells and we have shown that conjoint IKAROS deletion and NOTCH induction lead to Tp53 overexpression (Fig 4B). Thus, IKAROS may not trigger Tp53 repression, but the increase of H3K79 methylation and the ‘additive effect’ observed in IkNull/OP9-DL1 suggest that, by controlling H3K79me2 levels, IKAROS prevents the NOTCH-dependent induction of Tp53 transcriptional overexpression, which is likely linked to a variation in the control of transcriptional elongation.
To further investigate the importance of H3K79me2 deposition for occurrence of the additive effect, the cells were treated with EPZ004777, a known inhibitor of DOT1L (inhDOT1L), which is the unique methyltransferase capable of H3K79 methylation in mammalian cells [62]. The erythroid model cell line G1E-ER4 was used to define the lowest concentration of EPZ004777 (3μM) capable to decrease DOT1L activity and hence, H3K79me2 deposition (S7A Fig). G1E-ER4 are ES-derived pro-erythroblast GATA-1null cells expressing an inducible GATA-1-estrogen receptor (GATA-1-ER) fusion protein, which accumulates in the nucleus upon Tamoxifen induction and allows differentiation into erythroid cells [66–68]. Treatment with 3μM EPZ004777 severely reduced the cellular levels (S7B Fig) as well as the deposition of H3K79me2 to Cdkn1a and Tp53 TSS region (S7C Fig) in erythroid IkWT and IkNull Ter119+ cells co-cultured with OP9-DL1. The inhibition of DOT1L disrupts the additive effect imposed by IKAROS deletion and NOTCH induction on Tp53 but does not significantly change the additive effect detected at Cdkn1a (S7D Fig vs Fig 4A). This suggests that DOT1L activity is requested for Tp53 overexpression imposed by the additive effect of IKAROS deletion and NOTCH induction. Currently, it is unclear why DOT1L inhibition and H3K79 methylation reduction do not correlate with a lower expression levels of Cdkn1a and Tp53 in the absence of NOTCH induction. However, it is known that a direct link between H3K79 methylation and expression levels is not common to all genes [69] and, herein, it might be influenced by specific regulatory mechanisms occurring when IKAROS-CHD4 vs NICD or BRG1 complexes are alternatively recruited to these genes.
Disruption of IKAROS-dependent recruitment of the CHD4/NuRD complex leads to the abnormal expression of NOTCH target genes
The implication of chromatin remodeling activities for the ‘additive’ and ‘desensitize’ effects of IKAROS depletion and NOTCH induction was also explored. IKAROS can interact with NuRD and BAF subunits in lymphoid and erythroid cells thereby, controlling gene expression [19,23,70–72]. Interestingly, NICD was also reported to interact with NuRD and PBAF [8]. Therefore, we assessed the recruitment of the remodeling ATPases CHD4 and BRG1, respectively included in NuRD and P/BAF (BAF or PBAF) complex, to genes characterized by the ‘additive’ (Cdkn1a and Tp53) or ‘desensitize’ (Prdm16 and Nrarp, as described below; S2 File) effect in erythroid cells.
As expected, CHD4 of the NuRD complex, was recruited to Cdkn1a and Tp53 TSS and ORF in IkWT/OP9 and IkWT/OP9-DL1 cells. CHD4 recruitment to these genes was IKAROS-dependent and higher in IkWT/OP9-DL1 than IkWT/OP9 cells (Fig 6A and 6C), suggesting that it is facilitated by conjoint NICD binding to these genes (Fig 3C–3E). Conversely, the BAF component BRG1 was more efficiently recruited to Cdkn1a and Tp53 regions in IkNull/OP9-DL1 cells (Fig 6B and 6D). Thus, the ‘additive effect’ observed upon IKAROS ablation and NOTCH induction might be due to lower CHD4/NuRD and higher BRG1-P/BAF recruitment to chromatin.
Next, we assessed the recruitment of IKAROS, CHD4 and BRG1 to genes characterized by the ‘desensitize effect’, whereby IKAROS deletion impairs the NOTCH-associated gene activation. Prdm16 and Nrarp genes were selected for this analysis. PRDM16 is an important factor involved in the homeostasis of hematopoietic stem/progenitor cells [73]. It has been identified as a fusion partner in AML [74,75] and its oncogenic behavior seems to be highly dependent of its N-terminal PR-domain [76]. NRARP is a negative feedback regulator of the NOTCH pathway [77]. It also behaves as an oncogene, being overexpressed in breast, liver, thyroid and non-small cell lung cancers [78–81] and in several T-ALL and CLL cell lines upon NOTCH induction [82,83]. Interestingly, IKAROS and NICD can associate with Nrarp and Prdm16 TSS (S8A and S4B Figs). RNA-seq analysis revealed that Nrarp and Prdm16 belong to the group of genes whose expression upon NOTCH induction is affected by IKAROS deletion (Fig 7A). ChIP assays with CHD4 and BRG1 antibodies demonstrated that CHD4 is recruited to Nrarp and Prdm16 TSS, and that this binding is enhanced in IkWT cells upon NOTCH pathway activation (IkWT/OP9-DL1; Fig 7B), whereas BRG1 recruitment is higher in IKAROS-deleted and NOTCH-activated cells (IkNull/OP9-DL1; Fig 7C). These results suggest that CHD4 and BRG1 are needed to enhance Prdm16 and Nrarp gene expression upon NOTCH induction in IkWT cells, but that in IkNull cells, the absence of IKAROS prevents CHD4 recruitment to these genes and their expression upon NOTCH induction. The recruitment of IKAROS-CHD4 to Prdm16 and Nrarp TSS in IkWT Ter119+ cells (Figs S8A and 7B) suggests that IKAROS and CHD4 are required to organize chromatin at regulatory regions for rapid transcriptional activation. Bivalent chromatin characterized by H3K4me3 and H3K27me3 marks, is associated to poised transcription and thereby, rapid transcriptional activation [64]. ChIP assays showed H3K4me3 and H3K27me3 enrichment at Prdm16 and Nrarp chromatin, and significant reduction of H3K4me3 (but not H3K27me3) levels in IkNull/OP9 as well as IkNull/OP9-DL1 cells (S8B Fig). Furthermore, sequential ChIP analysis indicates that IKAROS is important for the organization of bivalent chromatin characterized by the co-occupancy of H3K4me3 and H3K27me3 to the TSS region of these desensitized genes (S8C Fig).
Thus, based on our results we propose that, at genes characterized by the desensitize effect, IKAROS favours the organization of a poised transcription structure marked by bivalent chromatin and thereby, promotes rapid transcriptional activation upon NOTCH signaling.
IKAROS influences NOTCH targets genes in hematopoietic progenitors and in erythroid cells
Bivalent chromatin and priming of transcriptional activation can be set in hematopoietic stem/progenitor cells (HS/PC) and maintained during cellular differentiation [84–89]. IKAROS is expressed and is an important regulator of genes in HS/PC [37,41]. Accordingly, we observed that IKAROS controls Cdkn1a and Prdm16 gene expression in fetal liver-derived hematopoietic progenitor (lin-) cells (S9A Fig). Thus, we tested whether the additive and desensitize effects observed in the IkNull erythroid cells originate from the absence of IKAROS in HS/PC or can be triggered by the ablation of IKAROS at later stages of erythroid differentiation. To address this issue, non-target siRNA (IkNT: expressing IKAROS at wild type level) or IKAROS knock-down (IkKD) e14.5 fetal liver erythroid cells were co-cultured for 48h on OP9 or OP9-DL1 cells. Less than 40% of Ikaros mRNA remains in the IkKD/OP9 or IkKD/OP9-DL1 vs IkNT/OP9 or IkNT/OP9-DL1 cells (S9B Fig). Next, we performed a comparative analysis of the expression levels of Cdkn1a, Tp53, Nrarp and Prdm16 genes in IkKD/OP9 or IkKD/OP9-DL1 vs IkNT/OP9 or IkNT/OP9-DL1 cells. The results obtained indicate that, as observed in erythroid cells derived from IkNull mice, IKAROS knock-down induced by siRNA transfection in erythroid cells favors the additive (Cdkn1a and Tp53 genes) or the desensitize (Nrarp and Prdm16 genes) effect upon NOTCH induction (S9C Fig).
To confirm that the NOTCH induction worked as expected in the siRNA ‘nucleofected’ erythroid cells, the expression levels of Cxcl1 and Mmp23, two gene responding to NOTCH pathway induction but not to variation of IKAROS expression levels (RNA-seq analysis; GEO accession ID: GSE122951), were investigated. The expression of these two genes does not vary between IkNT (wild type IKAROS expression levels) and IKAROS knock-down cells, and their overexpression solely depends on NOTCH induction upon OP9-DL1 co-culture (S9D and S9E Fig).
Together, these results suggest that IKAROS provides the adequate regulation of NOTCH target genes in hematopoietic progenitor as well erythroid cells.
IKAROS is required to prevent the overexpression of P21WAF1/CIP1 upon DNA damage induction
Having established the role of IKAROS as regulator of Tp53 and Cdkn1a genes, we then questioned the biological relevance of such regulation upon induction of DNA damage signaling that induces TP53 and P21WAF1/CIP1 activation [90]. The levels of IKAROS, TP53 and P21WAF1/CIP1 were analyzed in IkWT and IkNull Ter119+ cells co-cultured with OP9 or OP9-DL1 cells exposed to ionizing radiation (IR; 3.5 Gy). P21WAF1/CIP1 levels increased in IKAROS depleted cells whether or not exposed to IR, although IR exposure and NOTCH signaling induced the highest protein levels (Figs 3B and 8A). To address the importance of TP53 for IKAROS-induced P21WAF1/CIP1 overexpression, we knocked down Tp53 or Tp53 together with Ikaros in the erythroid model cell line G1E-ER4 (Fig 8B and 8C). As in IkNull Ter119+ cells, Ikaros knock-down in G1E-ER4 cells results in overexpression of P21WAF1/CIP1, particularly upon cell irradiation (Fig 8C). Though to a lesser extent, Tp53 and Ikaros double knock-down induced P21WAF1/CIP1 overexpression, when compared with Tp53 knock-down only. Thus, TP53 is required for maximal P21WAF1/CIP1 overexpression after irradiation, but IKAROS has an effect by itself on P21WAF1/CIP1 regulation in TP53 depleted cells (Fig 8C). To assess the potential clinical importance of IKAROS for P21WAF1/CIP1 expression, we tested the effect of lenalidomide on P21WAF1/CIP1 levels. Lenalidomide is a thalidomide homologue that promotes ubiquitination and proteasomal degradation of IKAROS as well as other IKZF family members [91,92], and is used for the treatment of patients with myelodysplastic syndrome or multiple myeloma [93,94]. As presented in Fig 8D, lenalidomide treatment of our erythroid cell models (G1E-ER4 and erythroid cells) led to IKAROS depletion and P21WAF1/CIP1 overexpression, suggesting that the induction of apoptosis imposed by lenalidomide treatment of hematopoietic cells [81] is likely related to the regulation of Cdkn1a/P21WAF1/CIP1 forced by IKAROS.
Thus, IKAROS regulation of Cdkn1a/P21WAF1/CIP1 (i) can occur in association with TP53 or be mediated by IKAROS alone; (ii) is important upon NOTCH induction but is also highly relevant to control Cdkn1a induction upon genotoxic insults, e.g., IR exposure.
Discussion
The IKAROS-mediated repression of NOTCH target genes is critical at early stages of lymphopoiesis. In here, we demonstrate that IKAROS, not only represses NOTCH target genes in the absence of NOTCH signaling, it can also restrain their activation upon NOTCH induction. This phenomenon was termed the ‘additive effect’ since the absence of IKAROS added to NOTCH induction results in the atypical overexpression of these genes. Our study also revealed the existence of another group of NOTCH target genes, which require IKAROS for transcriptional activation upon NOTCH signaling. These genes, which are not responsive to NOTCH induction in IKAROS depleted cells, are characterized by what we named the ‘desensitize effect’. To both groups of genes IKAROS is required for efficient recruitment of the remodeling ATPase CHD4 and bivalent chromatin organization associated with priming of transcriptional activation. Thus, IKAROS controls NOTCH target gene expression and promotes an adequate response to stress imposed by NOTCH induction or genotoxic insults.
IKAROS influences the recruitment of chromatin remodelers to NOTCH target genes
Gene expression is precisely regulated to maintain cell functions, specificity, and viability. Cellular stress, imposed by modification of cell homeostasis, infection, or genotoxic agents, activates intracellular signaling pathways including NOTCH, and provides the adequate response to protect the cell. Nonetheless, uncontrolled activation of NOTCH target genes, especially oncogenes, can disrupt cell functions and favor carcinogenesis. IKAROS is known to downregulate or silence many NOTCH target genes. It then prevents their activation in the absence of signaling. Moreover, the additive effect described in here and detected at multiple NOTCH targets, indicates that IKAROS controls the extent of the activation/expression levels of these genes upon NOTCH induction. This view is supported by ChIP-seq data, which indicate that recruitment of IKAROS to multiple NOTCH target genes can be maintained upon NOTCH signaling and gene activation [7]. The mechanism(s) used by IKAROS to control the expression levels of NOTCH target genes upon signaling remains to be fully elucidated. Nonetheless, the fluctuation of CHD4 and BRG1 recruitment to the NOTCH target genes studied suggests that: (i) IKAROS largely controls recruitment of these chromatin remodelers; and (ii) the timely recruitment of both remodelers is required for gene-controlled activation and expression. Indeed, the overexpression imposed by the additive effect of IKAROS depletion and NOTCH signaling is linked to variations in the recruitment of chromatin remodeling activities to NOTCH target genes. According to this view, IKAROS and CHD4 are required to prevent atypical gene overexpression upon NOTCH induction by restraining BRG1 recruitment to genes characterized by the additive effect. However, to Nrarp and Prdm16 genes, which are characterized by the desensitize effect, IKAROS and CHD4 recruitment precedes and is maintained upon BRG1 recruitment and gene activation. Then, the simultaneous presence of CHD4 and BRG1 is associated to full transcriptional activation upon NOTCH induction. Together with chromatin studies, these results reinforce the importance of IKAROS-mediated CHD4 activity for chromatin remodeling and promoter organization, which cannot be compensated by BRG1 recruitment. Hence, for both classes of genes, chromatin remodeling and transcriptional priming imposed by IKAROS and CHD4 are required for the physiological transcriptional activation of target genes upon induction of the NOTCH pathway.
The proximity between the nucleosome remodeling ATPases CHD4 and BRG1, which are best described as components of the NuRD and P/BAF complexes, has been demonstrated in osteosarcoma and hematopoietic cells [95,96]. Furthermore, genome wide analysis of CHD4 and BRG1 chromatin binding suggests their potential co-recruitment to genes repressed in embryonic stem cells [97–99]. However, in other cells, their sequential recruitment is required for the timely regulation of multiple genes [100]. For instance, the epithelial-mesenchymal transition in oral cancer cells is regulated by the sequential recruitment of these remodeling complexes to common genes, which facilitates the switching of their transcriptional state [101]. Similar to what we observed at Cdkn1a and Tp53 genes (Fig 6), NuRD was reported to antagonize recruitment and activation of the BAF complex [101]. The opposing activities of CHD4/NuRD and BRG1/BAF could therefore contribute to fine-tune gene expression in response to external signals [97,102]. However, the co-recruitment of CHD4 and BRG1 to genes displaying the desensitize effect does not corroborate with these observations whereby CHD4/NuRD acts as a transcriptional repressor and prevents the recruitment/activity of BRG1/BAF. The proximity and co-localization of these remodelers to transcriptionally active genes rather suggest that they might exert complementary actions to regulate gene expression. The cooperation between remodelers is required for proper chromatin organization and is best described during DNA repair (reviewed in [103]). Different remodelers including CHD4, BRG1 and SNF2H are recruited to DNA double strand breaks (DSBs) and participate to DSB detection and repair by homologous recombination. The joint recruitment of remodelers has also been described to transcriptionally active genes, such as hsp70 gene in Drosophila whereby the SWI/SNF complex and an ISWI-related complex are simultaneously located at the active promoter [104]. The complementary activity of remodelers can indeed be required for recruitment of different transcription factors or to control specific steps of transcription including poised organization, transcriptional initiation, elongation and/or termination [105–107].
IKAROS establishes bivalent chromatin and poised transcription of NOTCH target genes
Histone post-translational modifications were tested to define the mechanism(s) used by IKAROS to influence the chromatin organization and regulation of the NOTCH target genes of both above-mentioned groups. With the exception of the transcriptionally active Tp53 gene, Cdkn1a, Nrarp and Prdm16 genes were characterized by H3K4me3 and H3K27me3, which are histone post-translational modifications that usually characterize bivalent chromatin and mark genes primed/poised for transcriptional activation [64]. According to the canonical model, NOTCH activation leads to NICD translocation to the nucleus where the binding to NOTCH target genes is dynamic and frequently influenced by IKAROS [7,11,13,14,108]. In the absence of IKAROS, NOTCH activation per se associates with increased H3K79me2 levels at Cdkn1a and Tp53 TSS and ORF. However, NOTCH activation does not perturb the levels of H3K4me3 or H3K27me3 marks, which require the additional effect of IKAROS deletion to significantly change. According with this observation, Cdkn1a and Tp53 gene expression increases upon NOTCH pathway activation, although their overexpression is more important in cells that also lack IKAROS protein. Of note, sequential ChIP analyses demonstrate the importance of IKAROS for the establishment of bivalent chromatin domains characterized by the co-occupancy of H3K4me3 and H3K27me3 to Cdkn1a, Nrarp and Prdm16 genes, prior to their activation upon NOTCH induction. Previous reports suggested that IKAROS could be associated to bivalent chromatin at the CD8 locus in CD8-/CD4- double negative thymocytes, hence before transcriptional activation of the CD8 gene [109]. IKAROS then remains associated with chromatin during thymocyte differentiation to CD8+/CD4+ double positive stage, when CD8 is transcriptionally activated. Furthermore, Ding et al. [110] proposed that IKAROS can have a pioneering activity by favoring chromatin organization granting accessibility of other regulators to enhancers and gene promoters during lymphoid cell differentiation. Whether IKAROS could influence the timely recruitment of CHD4 and BRG1 to these genes remains unclear.
Unlike the other NOTCH target genes that we have characterized, Tp53 has a transcriptional activity that is further enhanced by NOTCH induction. The overexpression of Tp53 related to the additive effect is characterized by an increase of H3K79 methylation, which is associated with productive transcriptional elongation [69,111,112]. H3K79 methylation is mediated by DOT1L, a methyltransferase important for transcription elongation [113]. The importance of DOT1L for the additive effect was demonstrated upon treatment with the DOT1L inhibitor EPZ004777. DOT1L inhibition affects Tp53 and also Cdkn1a overexpression in NOTCH-activated cells whereby IKAROS had been deleted, thus suggesting that IKAROS can restrain DOT1L activity and productive transcription elongation of these genes. In support of this finding, it has been shown that DOT1L activity can correlate with high-level gene expression and the DOT1L yeast homolog, Dot1, genetically and physically interacts with PAF1, a potent regulator of transcription elongation [113]. How IKAROS can provide a rate limiting DOT1L activity to NOTCH targets is presently unknown, but could be related to the composition of the Pol II transcriptional elongation complex or to the chromatin organization at transcribed region of target genes. Indeed, IKAROS modulation of CHD4/NuRD and BRG1/BAF recruitment to chromatin could be pivotal since in addition to their well described function in regulating gene activation and repression, both remodeling complexes are reported to directly influence transcriptional elongation [17,23,104,114]. In fact, the CHD4/NuRD complex can interact with P-TEFb, which enhances the release of promoter-proximal paused Pol II [18,23] and BRG1/BAF, which promotes chromatin remodeling associated with Pol II transcription elongation of the HSF1 target gene Hsp70 in mammalian fibroblasts [104,114].
In summary, our results support a model whereby the IKAROS-CHD4 association does not account for individual gene activation or repression, but rather assures appropriate chromatin conformation and poised transcriptional organization required for transcriptional activation upon NOTCH induction (Fig 9). Without the dominant contribution of IKAROS, chromatin ‘pre-setting’ either before NOTCH induction or genotoxic insults, will be abnormal and most likely influenced by other regulatory elements that can: (i) promote BRG1 recruitment and atypical overexpression (additive effect); or (ii) preclude BRG1 recruitment and transcriptional activation (desensitize effect) of the NOTCH target genes. At NOTCH target genes, IKAROS largely controls the timely recruitment of the chromatin remodelers CHD4 and BRG1, and thereby, gene activation/expression levels. The results presented here provide a new perspective on the critical role played by IKAROS to promote adequate and controlled cell response to stress, whether imposed by NOTCH induction or genotoxic insults.
Materials and methods
Ethics statement
Animal experiments were conducted in accordance with the Canadian Council on Animal Care (CCAC) guidelines and approved by the Maisonneuve-Rosemont Hospital animal care committee (protocol number: 2015–15).
Mouse line
The IkNull mouse model is characterized by the deletion of the last translated exon of the Ikaros (Ikzf1) gene, which results in protein instability and the absence of IKAROS protein in all tissues [30]. Heterozygous male and female were bred, embryonic day 14.5 (e14.5) homozygote IkWT (IKAROS wild-type) or IkNull embryos were harvested and fetal livers were isolated. Since at this developmental stage the fetal liver contains nearly exclusively (~80%) erythroid cells [115,116], e14.5 fetal liver-derived cells are referred to as erythroid cells throughout the paper. Animals were sacrificed by cervical dislocation. All mutant embryos were compared with wild type littermates, to reduce difference in genetic background or developmental stage. Fetal liver DNA was extracted with DNAzol reagent (ThermoFisher) and samples were genotyped by PCR as described [30]. Animal experiments were conducted in accordance with the Canadian Council on Animal Care (CCAC) guidelines and approved by the Maisonneuve-Rosemont Hospital animal care committee.
RNA-sequencing and analysis
IkWT or IkNull e14.5 fetal liver cells were co-cultured for 48h on OP9 or OP9-DL1 stromal cell lines. Cells were then washed, resuspended in PBS-5% heat-inactivated FBS and Ter119+ cells were sorted by high-speed fluorescence-activated cell sorting (FACS). RNA from IkWT/OP9, IkWT/OP9-DL1, IkNull/OP9 and IkNull/OP9-DL1 Ter119+ cells was isolated by Trizol (ThermoFisher) extraction and purified with the RNeasy column kit (Qiagen) according to manufacturer instructions. RNA was further purified with mRNA enrichment with oligodT beads. The library was performed with the TruSeq RNA Sample Preparation kit (Illumina). Samples were sequenced on the HiSeq2000 Illumina sequencer following standard procedures. mRNA profiles were generated in biological triplicate, using Illumina cBot 2 System. The quality of the raw reads was assessed with FASTQC. Reports show no pool imbalance. After examining the quality of the raw reads, no trimming was deemed necessary. The reads were aligned to the GRCm38/mm10 genome with TopHat. The raw alignment counts were calculated with htseq-count. The RNA-seq results were normalized with the DESeq package [47]. Briefly, the read count was normalized by size factor that was calculated by median ratio of gene counts relative to geometric mean per gene. The log2 fold change is an estimate of the fold change between the conditions, based on the distribution of the reads. qRT-PCR validation was performed using specific primer sets in real-time PCR with SYBR Green.
Cell culture
G1E-ER4 (GATA-1 knockout ES-derived pro-erythroblast cell line expressing an inducible GATA-1-ER protein) cells [66–68] were cultured in Iscove’s modified Dulbecco’s medium (IMDM; ThermoFisher) containing 13% fetal bovine serum (FBS; Sigma), 1.7% penicillin-streptomycin (Wisent), 1.8 U/ml erythropoietin (Eprex), 1.1 mM 1-thioglycerol (Sigma), and 0.5% conditioned medium from a Kit ligand-producing CHO cell line.
To produce IKAROS knock-down clones, G1E-ER4 cells were infected with MISSION pLKO.1-puro vector (Sigma) containing short hairpin RNA (shRNA) specific to Ikaros mRNA (shIK) or a nonspecific scrambled shRNA (scrCTL). Positive cells were selected with Puromycin (2 μg/ml). OP9-DL1 cells are murine bone marrow stromal OP9 cells engineered to express constitutively the NOTCH ligand DELTA-like 1 (DL1). These cells were used in a co-culture system to activate the NOTCH signaling in e14.5 mouse fetal liver erythroid cells. OP9 and OP9-DL1 cells were seeded in α-Minimum Essential Medium (α-MEM; ThermoFisher) for four days. Then, IkWT or IkNull fetal liver cells were layered onto OP9 and OP9-DL1 in α-MEM added with 2 U/ml erythropoietin (Eprex) and cultured for 48h. Where indicated, cells were treated with the DOT1L inhibitor EPZ004777 (Calbiochem), at a concentration of 3 μM for 48h or with equal volume of DMSO (diluent control).
siRNA nucleofection
Knock-down experiments with small interfering RNA (siRNA) were performed in G1E-ER4 cells or e14.5 fetal liver erythroid cells (IkKD cells). The non-target control siRNA (siNT) and Tp53 siRNA (siP53) were purchased from Dharmacon (siGENOME SMARTpool siRNA); Ikaros pre-designed siRNA (siIK) (SASI_Mm01_00065776; SASI_Mm01_00065777; SASI_Mm02_00287954) were purchased from MilliporeSigma. For each nucleofection, 3×106 G1E-ER4 cells or 106 erythroid cells were washed PBS and resuspended in 100 μl of Ingenio Solution (Mirus). Next, 25 μl (20 μM) of either siNT or siP53 (for G1E-ER4 cells) or 5 μg of siNT or siIK (for erythroid cells) were added to the cell suspension, which was immediately nucleofected (Amaxa Nucleofector II, Lonza) with program G-016 (G1E-ER4 cells) or X-001 (erythroid cells) according to the literature [117] and manufacturer’ instructions.
Cell irradiation
E14.5 fetal liver or G1E-ER4 cells were irradiated with a dose of 3.5 Gy, using a gamma cell irradiator. Cells were maintained at 37°C and 5% CO2 and harvested after 3h-incubation.
Protein analysis
For Western blot assays, cells were lysed in Laemmli buffer (1 mM PMSF, 150 mM NaCl, 50 mM Tris HCl pH 6.8, 10% glycerol, 2% sodium dodecyl sulfate, 0.1% bromophenol blue, 2.5% β-mercaptoethanol), then sonicated, boiled for 10 minutes, migrated on SDS-polyacrylamide gel and transferred to nitrocellulose membrane (Bio-Rad). IKAROS (Cell signaling #D6N9Y), P21WAF1/CIP1 (BD Biosciences #556431), TP53 (Santa Cruz #393031), GAPDH (MilliporeSigma) or ACTIN (NeoMarkers) and horseradish peroxidase (HRP)-conjugated antibody (Jackson) were used for immunoblotting. Proteins were detected with Clarity Western enhanced chemiluminescence substrate (ECL; Bio-Rad) with a Fujifilm LAS-4000 luminescent image analyzer (GE Healthcare).
Quantitative reverse transcription PCR (qRT-PCR)
One to three million cells were washed in PBS and total RNA was isolated with TRIzol reagent (ThermoFisher). cDNA was generated using the All-in-One cDNA Synthesis SuperMix according to manufacturer’s instructions (Bimake). Quantitative PCR was carried out on an Applied Biosystems machine (Thermo-Fisher) using SYBR Green qPCR Master Mix (Biotool). Relative transcript levels were calculated using Hprt or Actin as control. To compare gene expression levels between conditions, results are presented as the ratio of the expression of each gene relative to the control expression. Where indicated, results were expressed as a fold change relative to the control. Quantitative analysis was performed according to Pfaffl’s method [118]. Primer sequences are detailed in S1 Table.
ChIP-qPCR assay
Cells were fixed in PBS/1.5 mM Ethylene glycol bis(succinimidyl succinate) (EGS) for 30 minutes, at room temperature, with gentle agitation and protected from light. Cells were complementary cross-linked for 5 minutes with 1% formaldehyde (Sigma) and fixation was stopped with Glycine (20 mM final) for 10 minutes. Cells were resuspended in SDS lysis buffer (1% SDS; 10 mM EDTA; 50 mM Tris-HCl pH 8.1) for 10 minutes and sonicated (Branson-Digital Sonifier) in order to obtain chromatin shear ranging 300 to 500 bp. Samples were then centrifuged, diluted in dilution buffer (0.01% SDS; 1.1% Triton; 1.2 mM EDTA; 16.7 mM Tris-HCl pH 8.0; 165 mM NaCl), pre-cleared with protein A Sepharose beads (MilliporeSigma) and incubated overnight with H3K4me3 (Abcam#8580), H3K27me3 (Milipore#17–622), H3K36me3 (Milipore#17100–32), H3K79me2 (Cell Signaling#5427), IKAROS (Santa-Cruz#13039), NOTCH/NICD (Abcam#8925) antibodies or isotype-matched immunoglobulins. Protein-DNA complexes were retrieved with protein A Sepharose beads (MilliporeSigma) and sequentially washed with the following buffers: low salt (0.1% SDS; 1% Triton; 2 mM EDTA; 20 mM Tris HCl pH 8; 150 mM NaCl), high salt (0.1% SDS; 1% Triton; 2 mM EDTA; 20 mM Tris HCl pH 8.0; 500 mM NaCl), LiCl (0.25 M LiCl; 1% NP-40; 1% Sodium Deoxycholate; 1 mM EDTA; 10 mM Tris-HCl pH 8.0) and TE (1 mM EDTA; 10 mM Tris HCl pH 8.0). After de-crosslinking and proteinase K digestion, the genomic DNA was purified and used as template in qPCR reactions.
Quantitative PCR (qPCR) were carried out as reported in Bottardi et al. [119] with minor modifications. About 1/30 of immunoprecipitated and 1/10 of unbound (input) material was used as a template for qPCR using SYBR Green (Bimake) on an ABI 7300 Fast real-time PCR system (Applied Biosystem). Quantification was performed according to the 2-ΔΔCt method [120] where ΔΔCt = ΔCt (test)—ΔCt (reference); ΔCt (test) = Ct (ChIP test)–Ct (input test); ΔCt (reference) = Ct (ChIP reference); test corresponds to the gene of interest; reference, to Thp promoter. All data showed are the results of at least four independent ChIP experiments with qPCR from each ChIP performed in triplicate and averaged (standard deviation). To correctly interpret the amplification values obtained by qPCR, the efficiency of all primer sets was carefully checked and primer pairs displaying an amplification efficiency ranging from 95 to 102% were chosen. Primer sequences are detailed in S2 Table.
Ter119/CD71 fetal liver cell sorting
IkWT or IkNull e14.5 fetal liver cells were washed and resuspended in PBS-5% heat-inactivated FBS. Cells were sequentially incubated for 30 minutes on ice with rat anti-Ter119 hybridoma, anti-rat Fluorescein Isothiocyanate (FITC)-conjugated (BD-Pharmingen) and Phycoerythrin (PE)-conjugated anti-CD71 (BioLegends) antibodies. Cells were sorted by high-speed fluorescence-activated cell sorting (FACS Vantage; Becton, Dickinson).
Lineage negative hematopoietic progenitor (lin-) cell purification
IkWT or IkNull e14.5 embryos were harvested, and fetal livers were collected and mechanically dissociated in 1X PBS, 5% FBS to generate a single-cell suspension and then centrifuged. Mature erythrocytes were lysed as follows: cell pellet was resuspended in 10 ml of 0.2% NaCl and after 40 second, 10 ml of 1.6% NaCl was added to re-establish osmolarity. Cells were centrifuged at 400g for 10 minutes, resuspended in 1X PBS, 5% FBS, passed through a 40 μm strainer to remove debris and then centrifuged for 5 minutes at 250g at 4°C. Lin- cells were obtained using the easySep mouse hematopoietic progenitor enrichment kit (StemCell Technology). RNA extraction and qRT-PCR analysis were carried out as described above (‘Quantitative reverse transcription PCR (qRT-PCR)’). Lin- cell purity and composition was assessed by ex-vivo clonogenic assays in complete methylcellulose medium (MethoCult M3434 StemCell Technology) and scored under contrast microscopy at day 14 [23].
Sequential ChIP (re-ChIP)
IkWT or IkNull e14.5 embryos were harvested, and fetal livers were isolated. Erythroid cells (20 X 106 cells per re-ChIP) were fixed in PBS, 1% formaldehyde (MilliporeSigma) for 10 minutes at room temperature with gentle agitation and fixation was quenched with Glycine (20 mM final) for 10 minutes. The first round of precipitation was carried out as described above (‘ChIP-qPCR assay’). After the second wash in TE buffer, immunoprecipitated complexes were eluted twice in buffer E (50 mM Tris-HCl pH 8.0; 10 mM EDTA; 1% SDS) by gentle shacking at 42°C for 20 min. Eluates were pooled, diluted 1:10 in ChIP dilution buffer and subject to the second round of immunoprecipitation. After an overnight incubation at 4°C, washes, chromatin elution, de-crosslinking, proteinase K digestion and qPCR were carried out as described above (‘ChIP-qPCR assay’). Re-ChIP assays were carried out with H3K4me3, H3K27me3 antibodies or isotype-matched IgG. Fold enrichment levels were calculated according to the “percentage input method” (https://www.thermofisher.com/ca/en/home/life-science/epigenetics-noncoding-rnaresearch/chromatin-remodeling/chromatin-immunoprecipitation-chip/chip-analysis.html).
Supporting information
S1 Table [docx]
Oligonucleotides used for qRT-PCR analysis.
S2 Table [docx]
Oligonucleotides used for ChIP analysis.
S3 Table [docx]
Genes overexpressed in Ik Ter119 upon NOTCH induction.
S4 Table [docx]
Principal functional annotations of genes listed in .
S5 Table [docx]
Principal functional annotations of the 499 genes specifically overexpressed in Ik/OP9 cells; log2 ≥ 0.08; < 0.05.
S6 Table [docx]
Principal functional annotations of the 844 genes specifically overexpressed in Ik/OP9-DL1 . Ik/OP9-DL1 cells; log2 ≥ 0.08; < 0.05.
S7 Table [docx]
Tumor suppressors and oncogenes included in the list of the 223 genes characterized by the ‘additive effect’ (see ).
S8 Table [docx]
Tumor suppressors and oncogenes included in the list of the 21 genes characterized by the ‘desensitize effect’ (see ).
S9 Table [docx]
List of the 223 genes characterized by the ‘additive effect’ (see ).
S1 Fig [dl1]
Expression of the Delta-like 1 ligand in OP9 cells.
S2 Fig [tif]
Distribution of the erythroid populations in Ik and Ik e14.5 mouse fetal livers co-cultured with OP9 or OP9-DL1 cells.
S3 Fig [tif]
Heatmaps corresponding to the genes overexpressed in Ik/OP9 or OP9-DL1 vs Ik/OP9 or OP9-DL1.
S4 Fig [a]
Gene expression and NICD recruitment in Ik and Ik Ter119 cells upon NOTCH induction.
S5 Fig [tif]
Western blot quantification presented in .
S6 Fig [a]
Determination of histone post-translational modifications and sequential ChIP analysis carried out to test the co-occupancy of H3K4me3 and H3K27me3 at and TSS.
S7 Fig [a]
Effect of DOT1L inhibition on and gene expression in G1E-ER4 cells or Ik and Ik Ter119 cells upon NOTCH induction.
S8 Fig [blue]
Histone post-translational modifications at and genes in Ik and Ik Ter119 cells upon NOTCH induction.
S9 Fig [a]
Effect of IKAROS abrogation on , , and gene expression in lineage negative hematopoietic progenitor (lin) and erythroid cells.
S1 File [xlsx]
Genes overexpressed in IkNull/OP9 or OP9-DL1 vs IkWT/OP9 or OP9-DL1.
S2 File [xlsx]
Genes characterized by the additive or the desensitize effect imposed by the absence of IKAROS and the induction of NOTCH.
Zdroje
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