Abstract
Isocitrate dehydrogenase 1 (IDH1) is the key enzyme that was involved in the modulation of cellular metabolism, epigenetic modification and redox states homeostasis. Gain-of-function mutations and decreased expression of IDH1 have been demonstrated to be tightly associated with the pathogenesis of various myeloid malignancies characterized by ineffective erythropoiesis, such as acute myeloid leukemia (AML) and myelodysplastic syndrome (MDS). However, the function and mechanism of IDH1 in human erythropoiesis still remains to be further explored. Here, utilizing the human erythropoiesis system, we present an innovative perspective of nuclear IDH1-mediated chromatin state reprogramming, besides its well-characterized metabolism effects. We showed that Knockdown of IDH1 induced chromatin reorganization and subsequently led to abnormalities of various key biological events in erythroid precursors, which could not be rescued by addition of reactive oxygen species (ROS) scavengers or supplementation of α-ketoglutarate (α-KG). Further analyzing indicated that IDH1 partially translocated into nuclear and acting as chromatin-binding protein. These findings strongly suggest nuclear located IDH1 elicited its effect in an enzymatic activity independent manner. We further revealed that deficiency of IDH1 induces genome-wide changes in distribution and intensity of multiple histone marks, among which H3K79me3 was identified as a critical factor in chromatin state reprogramming. Integrated analysis of ChIP-seq, ATAC-seq and RNA-seq recognized that SIRT1 was the key gene affected by IDH1 deficiency. Thus, our current work provided novel insights for further clarifying fundamental biological function of IDH1 which has substantial implications for an in-depth understanding of pathogenesis of diseases with IDH1 dysfunction and accordingly development of therapeutic strategies.
Graphical Abstract
Key Points
Nuclear located IDH1 regulates human erythropoiesis in a metabolism independent manner;
IDH1 deficiency leads to chromatin states reprogramming by causing aberrant accumulation and genome-wide re-distribution of H3K79me3;
Dyserythropoiesis is caused by downregulation of SIRT1 induced by H3K79me3 accumulation.
Introduction
Isocitrate dehydrogenase 1 (IDH1) is a key enzyme involved in regulation of redox homeostasis by catalyzing oxidative decarboxylation of isocitrate to α-ketoglutarate (α-KG), also known as 2-oxoglutarate (2-OG), simultaneously reducing NAD(P)+ to NAD(P)H and liberating CO 1. Growing evidence suggests that, in addition to metabolism regulation, IDH1 is also involved in regulation of epigenetic landscape 2. IDH1 mutations are known to cause dysregulation of chromatin modifications, such as DNA methylation, histone acetylation and methylation, which are associated with the occurrence and development of various myeloid malignancies characterized by ineffective erythropoiesis, such as acute myeloid leukemia (AML) and myelodysplastic syndromes (MDS) 3,4. Notably, recent research work also revealed that decreased expression of IDH1 are also contributed to the onset of AML and MDS 5,6.
Previous studies found that IDH1 mutations led to loss of normal catalytic activity 7 and gain of function, causing accumulation of the rare metabolite 2-hydroxyglutarate (2-HG) 8,9. 2-HG acts as an “oncometabolite” by competitively inhibiting multiple α-KG-dependent dioxygenases10–12, consequently altering cells epigenetic state and leading to pathogenesis of myeloid malignancies 1,9. However, several recent studies have shown that suppression of mutant IDH1 expression and/or inhibition of 2-HG production is not sufficient to reverse mutant IDH1-induced epigenetic changes 13,14. Blocking production of 2-HG did not inhibit the growth of many solid cancers with IDH1 mutations 13. Importantly, although IDH1 mutations lead to gradual accumulation of DNA and histone methylation markers, inhibition of IDH1 mutation expression did not lead to complete restoration of epigenome and transcriptome to initial state 14. Moreover, it has been reported that high concentration of 2-HG produced by mutant IDH1 also has antineoplastic activity in glioma 15. All these findings strongly suggested that the roles of IDH1 mutations in the pathogenesis of AML and MDS might not only be attributed to its capability to produce 2-HG.
Recently, the decreased expression of IDH1 induced by the expression of PIM2 was found to result in aberrant upregulation of proliferation of MDS cells 5. In addition, there is another study showed that the upregulation expression of IDH1 evoked by TFEB plays critical roles in the maintenance of epigenetic programs of myeloid progenitor cells and thus contribute in the suppression of the growth and survival of AML cells 6. These findings strongly suggest that aberrant expression of IDH1 is also an important factor in the pathogenesis of AML and MDS.
Considering that genetic mutations may lead to the loss of original functions while acquiring new roles, we speculate that the roles of IDH1 mutations in the pathogenesis of myeloid disorder diseases might not only be attributed to the gain of function-dependent manner, but also attributed to an enzymatic independent loss of function manner, which has not been recognized previously. It also should be noted that most previous studies focused primarily on the pathogenic roles of mutated IDH1, whereas the biological function of IDH1 and underlying mechanisms remain largely unknown.
In this study, by using an in vitro human erythropoiesis system, during which cell morphology and chromatin architecture are dramatically altered 16, 17, we presented an innovative perspective that nuclear IDH1 is involved in chromatin state reprogramming in an enzymatic activity independent manner to regulate terminal erythropoiesis.
Methods
Culture of CD34+ cells and shRNA or siRNA mediated knockdown of IDH1
Primary human CD34+ cells were acquired from cord blood by positive selection using CD34+ magnetic selective beads system according to the manufacturers protocol 18. The detailed methods have been described previously including culture medium composition, the culture protocol, preparation of lentivirus 19. The sequence of IDH1-shRNA and IDH1-siRNA in experiments were shown in Supplemental Table 2.
Drug treatment
The drugs for cell treatment were as follows. N-Acetyl-L-cysteine (MCE, HY-B0215) used at a final concentration of 10μM. Glutathione (Selleck Chemicals, S4606) was dissolved in DMSO, and used at a final concentration of 50 μM. α-ketoglutanic acid (MilliporeSigma, K1128) was used at a final concentration of 50 μM. EX527 (Selleck, S1541) used at final concentrations of 10 and 200 nM and SRT1720 (MCE, HY10532) used at final concentrations of 0.1, 0.5 nM and 2.5μM.
Immunofluorescent staining of AML or MDS patients Paraffin-Embedded bone marrow cells
Formalin-fixed, paraffin-embedded tissues blocks of bone marrow samples from AML and MDS patients bearing IDH1 mutation were sectioned at a thickness of about 4-5 µm. Slides were floated in a 40°C water bath and then transferred onto glass slides. After drying for 12 hours, slides were deparaffinized with xylene and rehydrated with alcohol. Then, slides were incubated in 10 mM citrate buffer (pH 6.0) at 95-100°C for 10 minutes. 3% BSA in PBS were added onto slides and incubated at 25°C for 30 minutes. Slides were incubated with primary antibodies at 4°C for 12 hours and with secondary antibody at 25°C for 30 minutes. Nuclear was stained with Hoechst 33342 (blue). The following primary antibodies were used as follows: rabbit polyclonal antibody to IDH1(#12332-1-AP, Proteintech), mouse monoclonal antibody to Histone H3 (Tri methyl K79) (BSM-33098M, Thermo Fisher Scientific). Secondary antibodies were goat anti-rabbit or goat anti-mouse labeled with Alexa Fluor 488 or Cy5(Servicebio). Pannoramic MIDI (3DHISTECH) slice scanner was used to acquire images.
DNA pull-down assay
The sequence of the biotin labeled probes for SIRT1 was as follows (Forward oligo: TCCCAAAGTGCTGGGATTACAG; Reverse oligo: GCACCTCGGTACCCAATCG). Genomic DNA containing the target DNA sequence was used as a template, the promoter region of SIRT1 was amplified by PCR, including biotin-labeled and non-biotin-labeled. 2 ug probes (target gene biotin-labeled probe set and non-labeled probe set, Empty magnetic beads group) were added in EP tube and incubated for 8 hours in a 4°C refrigerator. 300 μL cell lysates (empty beads group without lysis solution) were added into magnetic bead-probe mixture and incubated in a 4°C refrigerator for 12 hours, 30 μL (10%) of the remaining lysates were taken as the input group. Incubation mixture was centrifuged at 3000rpm for 2 minutes and washed 5 times. Loading buffer was added into each group (including input group and beads group). Tubes were input into boiling water bath for 10 minutes and centrifuged at 3000rpm for 5 minutes. The obtained production can be directly used for WB experiment.
Data analysis
We performed chromatin immunoprecipitation (ChIP)-seq, ATAC-seq and RNA-seq, detailed description of data analysis was provided in supplemental Data.
Results
IDH1 deficiency impaired terminal erythropoiesis in an enzymatic activity independent manner
To further explore the roles of IDH1 during human erythropoiesis, we performed shRNA/siRNA-mediated knockdown of IDH1 on days 7, 11, and 15. ShRNA and siRNA mediated knockdown efficiency were confirmed by qRT-PCR (Supplemental Figure 1A) and western blot (Supplemental Figure 1B, C and Supplemental Figure 5A, B). Consistent with our previous results, we found that loss of IDH1 had a slight effect on cell growth (Supplemental Figure 1D) but not on apoptosis at late stages of erythropoiesis (Supplemental Figure 1E, F and Supplemental Figure 5C, D). Although the differentiation of colony-forming unit-erythroid (CFU-E) cells into terminal stage, characterized by glycoprotein A expression, was not affected by lack of IDH1 (Supplemental Figure 3A, B and Supplemental Figure 5E, F), the generation of orthochromatic cells, defined as GPAposα4-integrinlowband3hi 21, was delayed by IDH1 deficiency (Supplemental Figure 3C, D and Supplemental Figure 6A, B). This delay of differentiation was also confirmed by morphological observation using cytospin assay (Supplemental Figure 3E). Since chromatin condensation and enucleation are distinguished cellular events of polychromatic and orthochromatic cells 21, we also evaluated cell morphology and enucleation. We observed a remarkable accumulation of polychromatic and orthochromatic erythroblasts with abnormal nuclei in IDH1-deficient erythroblasts (Figure 1A; Supplemental Figure 6C, D) and severely impaired enucleation (Figure 1B; Supplemental Figure 6E, F). In addition, we found that IDH1 deletion resulted in distinctly larger nuclei compared to controls, with the ratio of nucleus/plasma increased more than 2-fold in IDH1-deficient erythroid cells (Supplemental Figure 4A, B), indicating that IDH1 knockdown impaired nuclear condensation.
IDH1, a critical modulator of redox homeostasis and metabolism, catalyzes the conversion of isocitrate into α-KG in metabolism13. We have recently reported that IDH1 can regulate terminal stage human erythropoiesis by interacting with vitamin C 22, 23. Interestingly, former study revealed that defect in erythropoiesis caused by IDH1 deficiency could not be rescued by reactive oxygen species (ROS) scavenging or α-KG supplementation, which indicates that IDH1 might perform its function partially in an enzyme-independent manner. To gain a better understanding of mechanism underlying effects of IDH1, we detected ROS and α-KG production. Firstly, we measured ROS production by flow cytometry using DCFHDA dye for quantitative and qualitative assessment of ROS based on the mean fluorescence intensity (MFI) of GFP. Results showed that MFI in IDH1-deficient group increased about 2-fold on day 15 (Supplemental Figure 7A). Although aberrant upregulation of ROS could be attenuated using ROS scavengers N-acetyl-L-cysteine (NAC, 10 μM) and glutathione (GSH, 50 μM) (Supplemental Figure 7B, C), generation of erythroblasts with abnormal nuclei or reduction of enucleation efficiency caused by IDH1 deficiency was not rescued (Figure 1C, D). In addition, we conducted colorimetric detection assay to determine α-KG levels 24, and found that lack of IDH1 resulted in a significant decrease in α-KG levels to 20 nmol compared to 35 nmol in control group on day 15 (Supplemental Figure 7D). However, supplementation with 50 μM of α-KG could not rescue aberrant cell events induced by lack of IDH1 (Supplemental Figure 7E; Figure 1E, F). These findings confirmed that IDH1 plays a crucial role in regulation of terminal human erythropoiesis in an enzymatic activity-independent manner. In addition, IDH1 deficiency led to the generation of erythroid cells with abnormal nuclei and reduction of mature red blood cells, which is consistent with dyserythropoietic features in myelodysplastic syndrome (MDS) and acute myeloid leukemia (AML) with erythroid dysplasia.
IDH1 localizes to nucleus of human erythroid cells
IDH1 has been widely studied as a key metabolic enzyme localized in cytoplasm or peroxisome. In recent years, it has also been reported that IDH1 localized in nucleoplasm and chromatin of embryonic stem cells (ESCs) 20. However, the subcellular localization of IDH1 during human erythropoiesis still remain largely unknown. To address this, we systematically analyzed the subcellular location of IDH1 in erythroid cells at different time points on umbilical cord blood-derived CD34+ cells induced to normal human terminal erythroid development. Immunofluorescence analysis revealed that IDH1 localized within nucleus as cells matured (Figure 2A, B). We also examined location of IDH1 in human umbilical cord blood-derived erythroid progenitor 2 (HUDEP-2), K562 and HEL cell lines and found that IDH1 also localized within nucleus (Figure 2C and Supplemental Figure 2A, B). In addition, we obtained paraffin-embedded bone marrow samples from 10 patients with IDH1-mutant AML/MDS, including 4 MDS and 6 AML samples (Supplemental Table1). IDH1 mutation sites were reported in previous studies, including R132C, R132G, and R132H 2. We further detected localization of IDH1 by immunofluorescence staining assay, IDH1 was also expressed in both nucleus and cytoplasm of erythroblasts characterized as GPA positive expression (Figure 2D and Supplemental Figure 2C). In contrast, IDH1 was exclusively localized in cytoplasm of 293T cell line (Figure 2E). Western blot analyses further confirmed nuclear location of IDH1 in erythroblast but not in 293T cells (Figure 2F). The unique subcellular localization pattern of IDH1 in erythroid cells suggests that it may play a role in erythropoiesis through enzymatic independent manner.
Nuclear IDH1 maintains nuclear morphological on terminal erythropoiesis
Previously, presence of IDH1 in nucleus has been mentioned 20, but it has not been specifically proven that the function of IDH1 relies on its nuclear localization. To further test whether nuclear IDH1 is prominent in maintaining nucleus morphology independent of its enzymatic activity, we knocked out IDH1 in nucleus while retaining cytoplasmic IDH1 (Figure 3A). Firstly, as shown in Figure 3B, we knocked out IDH1 using CRISPR-Cas9 technology by infecting with viral particles carrying small guide RNA (sgRNA) sequences targeting IDH1 and sorted with GFP to get Sg-IDH1 HUDEP2 cells, in which IDH1 was totally depleted. Cells overexpressing nuclear export signal (NES)-IDH1 were then transduced into Sg-IDH1 HUDEP2 to deplete nuclear IDH1 while preserving IDH1 in cytoplasm in HUDEP2 cells. After expansion and differentiation 25, we further confirmed the selective localization of IDH1 to nucleus by confocal microscopy. As shown in Figure 3C, there is no presence of IDH1 in nucleus while the cytoplasm localization of IDH1 was still retaining. Selective knockdown of nuclear IDH1 caused a significant increase of the proportion of HUDEP2 cells with abnormal nuclei (Figure 3D). While, as it was shown in Figure 3E, statistical analysis showed that proportion of cell nuclear malformations of Sg-NES-IDH1 cells was as similar as Sg-IDH1 cells. Taken together, these results demonstrated that nuclear IDH1 plays critical roles in maintaining of nuclear morphology during terminal erythropoiesis.
Deficiency of IDH1 reshaped chromatin landscape in late-stage erythroblasts
Given that nuclear located chromatin-binding proteins play crucial roles in maintaining chromatin structure and gene expression 26, we further checked the distribution of IDH1 in nucleus of erythroid cells cultivated on day 15. We found that IDH1 is detected in chromatin fraction of erythroid cells on day 15 (Figure 4A). To explore the role of IDH1 in maintaining chromatin architecture, we evaluated the effect of IDH1 on the chromatin structure of erythroid cells using transmission electron microscopy. As expected, IDH1 deficiency led to aberrant dynamic transition between euchromatin and heterochromatin state. In mixed late erythroblasts on day 15 as well as purified polychromatic and orthochromatic cells, the proportion of euchromatin increased by 2-3 folds in IDH1-deficient cells compared to control cells (Figure 4B, C). There is growing evidence that metabolites drive chromatin dynamics through post-translational modifications (PTMs) that alter chromatin structure and function 27, 28. Moreover, it has been well established that dynamic changes in methylation and demethylation of histone proteins could modify their interaction with DNA, consequently changing the ratio of heterochromatin and euchromatin 29. Thus, we next detected histone modification marks using immunofluorescence imaging and western blotting. For most histone modifications, such as H3K36me2, H3K4me3, H3K4me2, and H3K36me3, there were no significant differences between IDH1-deficient groups and control group on day 15 (Supplemental Figure 8A, B). However, abundance and subcellular location of specific histone modifications altered dramatically, including H3K27me2, H3K79me3, and H3K9me3. In control group, the majority of histone modification markers were released to cytoplasm for final degradation. While in IDH1-deficient groups, H3K27me2, H3K79me3, and H3K9me3 were still arrested in nucleus (Figure 4D-F). Taken together, all these results strongly suggested that nuclear IDH1 played critical roles in maintaining chromatin state dynamics by affecting accumulation and distribution of specific histone modifications.
Identification of H3K79me3 as the critical factor in response to IDH1 deficiency
Previous studies have reported that mutant-IDH1 induced chromatin state altering and thus drive development of gliomas and other human malignancies. To further define chromatin state reprogramming induced by IDH1 deficiency during erythropoiesis, we used chromatin immunoprecipitation followed by ChIP-seq to investigate genome-wide distribution of three key histone modifications in IDH1-deficient groups on day 15. Firstly, heatmaps and corresponding profile plots of ChIP-seq data showed that there was the greatest increase in recruitment of H3K79me3 to chromosome (Figure 5A, B). In addition, there were 21,169 peaks of H3K79me3 identified, which were significantly larger than 91 peaks of H3K27me2 and 1740 peaks of H3K9me3 (Figure 5C). We further analyzed the peak localization of H3K79me3, H3K27me2, and H3K9me3. Around 45% peaks of H3K79me3 were located in promoter regions. While for H3K27me2 and H3K9me3, peaks covered a large proportion in the distal intergenic region, approximately ∼70% (Figure 5D). In fact, there were 8602 peaks with H3K79me3 in promoter region, which was ∼800-fold more than that of H3K27me2 and H3K9me3 (Figure 5E). We subsequently conducted Gene Ontology (GO) analysis on the differential peaks. GO terms from biological processes, cellular components, and molecular functions consistently showed that H3K79me3 peaks were predominantly enriched with promoters of genes involved in RNA splicing and chromatin modification pathway (Figure 5F). Taken together, these results indicated that IDH1 deficiency reshaped chromatin states and subsequently altered gene expression pattern, especially for genes regulated by H3K79me3, which was the mechanism underlying roles of IDH1 in modulation of terminal erythropoiesis.
We further detected location of H3K79me3 in control and Sg-NES-IDH1 HUDEP-2 cell line and found that deletion of nuclear IDH1 induced H3K79me3 accumulation in nucleus (Supplemental Figure 9A). Since the generation of erythroid with abnormal nucleus and reduction of mature red blood cells caused by IDH1 absence are notable characteristics of MDS and AML. In addition, pathogenesis of AML/MDS is significantly associated with IDH1 mutation 30. Therefore, we speculated that aberrant accumulation and distribution of H3K79me3 caused by dysfunction of IDH1 were also another characteristic of MDS/AML bearing IDH1 mutation. Thus, we performed immunofluorescence microscopy observation to further investigate the clinical significance of H3K79me3 in progression of IDH1-mut AML/MDS. Notably, an interesting finding was that H3K79me3 colocalized with IDH1 mutants in nucleus (Supplemental Figure 9B).
IDH1 deletion increased chromatin accessibility in late-stage erythroblasts
Histone post-modifications are important epigenetic markers involved in multiple cellular processes via regulation of gene transcription or remodeling of chromatin structure 31, 32. Since previous studies have identified H3K79me3 as a transcriptional activating marker 33, we speculated that accumulation of H3K79me3 in IDH1-deficient erythroblasts would subsequently lead to switch of closed chromatin into open chromatin. To test our hypothesis, we performed Assay for Transposase-Accessible Chromatin with high-throughput sequencing (ATAC-Seq) to identify alterations in chromatin accessibility (Supplemental Figure 10A, B). Heatmaps and corresponding profile plots displayed chromatin accessibility of Luciferase-shRNA and IDH1-shRNA at peak centers. We found that IDH1-deficient cells showed higher ATAC peak signals compared to control cells (Figure 6A, B). Volcano plot showed that there were 2,637 ATAC peaks gained and 442 ATAC peaks lost in presence of IDH1 deficiency (Figure 6C). Analysis of localization of ATAC peaks showed that differential peaks were mainly located in promoter regions (Figure 6D; Supplemental Figure 10C). GO analysis showed that gained ATAC peaks were mainly enriched with promoters of genes involved in various chromatin regulation pathways (Figure 6E). To identify which specific DNA binding motifs were enriched in differential peaks, we performed motif analysis using HOMER and found that gained ATAC promoter peaks were enriched with KLF1 binding motifs (p<0.001), which was identified as an erythroid-specific transcription factor (Figure 6F). Therefore, these results further confirmed that nuclear IDH1 plays a critical role in chromatin structure modulation as determined by accumulation and distribution of H3K79me3.
Integrated analysis of ChIP-seq, ATAC-seq and RNA-seq identified SIRT1 as one of the key genes affected by IDH1 deficiency
To further elucidate mechanisms underlying effects of IDH1 deficiency on changes in chromatin landscape and transcriptional state, we conducted integration analysis of ChIP-seq, ATAC-seq and RNA-seq. RNA-seq analysis was performed to get widespread gene expression in control and IDH1-deficient erythroid cells (Supplemental Figure 11A). Volcano plot and heatmap of differentially expressed genes revealed that 3,543 genes were upregulated and 3,295 genes were downregulated after IDH1 knockdown (Supplemental Figure 11B-C, E). GO analysis showed that upregulated genes mainly enriched in pathway associated with chromatin, such as chromatin organization and chromatin remodeling (Supplemental Figure 11D). We further displayed chromatin-related genes, including TSPYL1, SIRT1 and others (Supplemental Figure 11F). Further integrated analysis of RNA-seq and ChIP-seq showed that gene expression levels of H3K79me3-marked genes were upregulated in IDH1-deficient cells (Supplemental Figure 12A, B). Furthermore, integrated analysis of ChIP-seq and ATAC-seq confirmed that IDH1 loss resulted in a greater proportion of open chromatin regions in H3K79me3-enriched sites (Supplemental Figure 12C). Gene Set Enrichment Analysis (GSEA) showed that chromatin structure modulating pathway, including chromatin silencing and gene expression epigenetics (Figure 7A). We found that there were 93 genes overlap in ATAC-seq, ChIP-seq and RNA-seq (Figure 7B), of which 3 genes shared in chromatin-associated pathways, including SIRT1, NUCKS1 and KMT5A (Figure 7C). Transcription factors (TFs) play key roles in regulation of transcription by recognizing and binding to target gene promoter region. Due to deficiency of IDH1, gained ATAC promoter peaks were enriched with KLF1 binding motifs (Figure 6F). KLF1 has been characterized as one of the most significant TFs involved in regulation of human erythropoiesis. We thus detected TFs bound on SIRT1, NUCKS1 and KMT5A locus. ChIP-seq results showed that KLF1 could bind to promoter regions of SIRT1, NUCKS1 and KMT5A, with the highest peak signal at promoter of SIRT1 (Figure 7D). This finding was further confirmed with DNA pull-down assay (Figure 7E). IDH1 deficiency caused alteration of chromatin landscape, characterized by aberrant accumulation and distribution of H3K79me3, which led to dysregulation of terminal erythropoiesis. Thus, we speculated that H3K79me3 was involved in SIRT1 up-regulation. Using DNA pull-down assay, we found that H3K79me3 binds to SIRT1 gene promoter region in response to IDH1 knockdown (Figure 7E). Representatively, gene expression levels and ATAC peak signals at SIRT1 locus were elevated in IDH1-shRNA group and were accompanied by enrichment of H3K9me3 (Figure 7F). These findings strongly suggested that IDH1 deletion can lead to increased accumulation of H3K79me3 in SIRT1 promoter region and thus switch region into open state, thereby recruiting KLF1 to promote SIRT1 expression.
SIRT1 plays a critical role in mediating the regulatory effect of IDH1 during terminal stage erythropoiesis
Further integrated analysis also provided evidence to support our forementioned findings. As shown in Figure 7F, RNA-seq, ATAC-seq and ChIP-seq signal tracks annotated to SIRT1 gene loci showed H3K79me3/ATAC-seq overlap and corresponding upregulation of SIRT1 in IDH1 knockdown group. Based on these results, we speculated that SIRT1 was the key factor that mediated the role of IDH1 in regulation of terminal erythropoiesis. Therefore, we performed verification and rescue experiments by treatment of normal erythroid cells with a SIRT1 activator or treatment of IDH1-deficient cells with a SIRT1 inhibitor, respectively. First, we confirmed that the application of SRT1720 on normal erythroid cells and treatment of IDH1-deficient erythroid cells with IDH1-EX527 does not induce apoptosis (Supplemental Figure 13A-D). The addition of SRT1720 led to nuclear malformations in a dose-dependent manner, in approximately 40% of cells (Figure 8A). Importantly, we observed a significant enucleation reduction after addition of SRT1720. In control group, the percentage of enucleated cells was 30% and 45% on day 13 and day 15, respectively, compared to < 20% in SRT1720 group (Figure 8B). Therefore, SIRT1 activation mimicked the cell dysfunction caused by IDH1 knockdown. Morphological images of IDH1-deficient erythroid cells treated with EX527 showed that malformed nuclei were partially rescued (Figure 8C). In addition, treatment with SIRT1 inhibitor EX527 also partially increased enucleation efficiency to 25% and 35% on day 13 and day 15, respectively (Figure 8D). In conclusion, these findings prove that SIRT1 is a key regulatory factor that mediates roles of IDH1 in regulation of nuclear morphology and enucleation of terminal stage erythropoiesis.
Discussion
The effective diagnosis and treatment of tumors bearing IDH1 mutations relies on an understanding of the fundamental biological and physiological roles of IDH1. In this study, we delineated an enzyme activity-independent role of IDH1 in regulation of human erythropoiesis through remodeling chromatin state. We demonstrated that deficient nuclear IDH1 led to dramatic accumulation of multi-histone modifications, among which H3K79me3 was identified as the crucial factor, resulting in SIRT1 upregulation and consequently leading to defects in various critical cell events during terminal stage erythropoiesis.
Recent advances in understanding non-catalytic activity of metabolism enzymes have provided insights into roles of IDH1 34. Change in subcellular distribution of metabolism enzymes is associated with distinct non-canonical functions. It has been reported that metabolic intermediates such as acetyl CoA, α-KG, S-adenosylmethionine, and nicotinamide adenine dinucleotide can act as cofactors of epigenetic modification of nuclear genes to regulate stem cell function and differentiation 35. Interestingly, as a metabolic enzyme, hexokinase 2 (HK2) localizes to nucleus of AML and normal hematopoietic stem and progenitor cells, and nuclear HK2 has a non-canonical mechanism by which mitochondrial enzymes influence stem cell function independently of their metabolic function 34. In addition, glycolytic enzymes that are translocated to nucleus have independent catalytic roles, such as kinase activity and DNA-binding ability that are associated with regulation of gene expression and DNA repair. For instance, nuclear translocated glyceraldehyde 3-phosphate dehydrogenase can bind to E3 ubiquitin ligase SIAH1 and initiate apoptosis, as well as bind to telomeres to maintain their length 36. In this study, we found that IDH1, as one of key metabolism enzymes, localizes to nucleus in erythroid cells of healthy person and AML/MDS patients, and plays critical roles in maintaining cell morphology and chromatin dynamics in an enzymatic activity-independent manner.
Although a few studies have reported that IDH1 is located in nucleus, most studies have focused on the metabolism and RNA binding of IDH1 located in cytoplasm 20. In line with previous findings, our study confirmed the critical role of IDH1 in regulation of human erythropoiesis, which could not be rescued by addition of ROS scavengers or supplementation with α-KG 22, 23. Previous work reported that IDH1 regulate human erythropoiesis modulating metabolism, based on the finding that defective erythropoiesis induced by IDH1 deficiency could be reversed by application of vitamin C. It should be noted that Vitamin C is a critical metabolic regulator that plays important biological and physiological roles, as well as epigenetic modulatory roles, but underlying mechanism still remains to be well illustrated 37, 38. Based on diverse outcomes of vitamin C treatment and metabolism restoration, we proposed that IDH1 might elicit its effect partially in an enzymatic activity-independent manner.
Interestingly, we found that IDH1 deficiency had no obvious effect on differentiation and proliferation of proerythroblasts and basophils but affected unique cell events of polychromatic and orthochromatic erythroblasts, including cell morphology, chromatin condensation, and enucleation. Terminal stage erythropoiesis is a highly dynamic and complex process during which chromatin structure undergoes significant changes 39. Current and previous studies showed that in addition to chromatin condensation, majority of histones were released into cytoplasm for decomposition during late stage of terminal erythropoiesis and is crucial for chromatin condensation and subsequent enucleation 40. Chromatin reorganization, histone release, and redistribution are essential for chromatin reprogramming on terminal erythroid development. In present study, our finding showed that IDH1 deficiency led to accumulation of multiple histone modification markers in nucleus, particularly in polychromatic and orthochromatic cells, might explain effects of IDH1 deficiency at specific development stages. In addition, we found that IDH1 deficiency caused methylated histones accumulation on chromatin and increased accessibility to generate open chromatin state for transcription activation, which further exacerbates defective terminal erythropoiesis. Present study is first to report that nuclear IDH1 has important roles in maintenance of dynamic changes in chromatin states. Our findings suggest synergistic actions of nuclear IDH1 and cytoplasmic on regulation of human erythropoiesis by modulating metabolism and chromatin architecture.
Our results also suggested that IDH1 deficiency was related to aberrant accumulation of H3K79me3 and SIRT1 upregulation. Although disturbed methylation catalyzed by DOT1 is a well-recognized target for diagnosis and treatment of leukemia and its transformation, the majority of previous studies mainly focused on the role of H3K79 demethylation 41–43. In this study, in vitro and in vivo (patient samples) experiments showed that IDH1 deficiency led to significant H3K79me3 accumulation, which could be used to diagnose dyserythropoiesis with IDH1 functional defect. SIRT1 is important for catalyzing removal of acetyl groups from non-histone and histone proteins. Previous studies have demonstrated that SIRT1 is involved in a wide range of physiological functions, including regulation of gene expression, cell growth, DNA repair 44, oxidative stress 45, metabolism 46 and aging47. In addition, SIRT1 activates expression of fetal hemoglobin genes in adult human erythroblasts 48. Notably, SIRT1 is also involved in regulation of higher-order chromatin structure and various pathways related to pathogenesis and transformation of various dyserythropoiesis-related hematopoietic diseases 49. Overexpression and underexpression of SIRT1 are strongly associated with pathogenesis of AML and MDS. Both inhibitory and activatory strategies have been proposed for diagnosis and treatment of these diseases 50. In current study, we proved that IDH1 deficiency leads to significantly increased SIRT1 expression. Series of phenotypes caused by IDH1 deficiency, such as nuclear malformation, aberrant nuclear condensation, and impaired enucleation, could be partially rescued by addition of specific SIRT1 inhibitor. These findings confirm that inhibitory strategy is promising for diagnosis and treatment of dyserythropoiesis-related diseases, particularly in patients with IDH1 mutation.
In conclusion, our work provides a novel insight into the role of IDH1 in the regulation of chromatin states. The findings related to IDH1-H3K79me3-SIRT1 regulatory axis indicates that H3K79me3 and SIRT1 may be targeted for the diagnosis and treatment of diseases with IDH1 mutations.
Data availability
The data underlying this article are available in article and in its online supplementary material. RNA-seq data have been deposited in the GEO under accession code GSE223141. ChIP-seq data have been deposited in the GEO under accession code GSE222296. ATAC-seq have been deposited in the GEO under accession code GSE222401.
Author contributions
X.A. and L.C. designed the overall project, analyzed the results and prepared the manuscript, with input from all co-authors. M.L. performed the experiments with assistance from M.Y., Q.Y. and L.S.; H.C.Z. and X.W. performed the integrated bioinformatics analysis under the supervision of T. W.; W.L., Z.J. and F.X. performed the analysis of the samples from patients bearing IDH1 mutation; K. R. and N. Y. provide support in the culture and maintaining of HUDEP-2 cells.
Acknowledgements
This work was supported by grants from the Natural Science Foundation of China (82170116, 81870094, 81570099 and 82300134).
Conflict of interest
The authors declare that they have no competing financial interests.
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