t(8;21) is a frequent chromosomal translocation in acute myeloid leukemia (AML) and is also reported in lymphoid and biphenotypic acute leukemia.1, 2 t(8;21) fuses the RUNX1 gene (AML1) on chromosome 21 to the ETO gene (RUNX1T1) on chromosome 8, encoding the RUNX1/ETO chimeric transcription factor that represses expression of RUNX1 target genes, promoting self-renewal and blocking myeloid differentiation.3, 4, 5, 6 t(8;21) is insufficient for leukemogenesis and additional co-operating mutations are required for transformation,7 including point mutations that activate and/or over express c-KIT.8 The mechanisms driving the acquisition of co-operating mutations remain unclear, although there is evidence that initiating lesions such as RUNX1/ETO may promote mutagenesis.9, 10 For example, ectopic expression of RUNX1/ETO downregulates several DNA-repair proteins (BRCA2, OGG1 and ATM) and increases the level of phosphorylated TP53 and γH2AX, indicating elevated DNA damage and a possible pro-mutagenic phenotype.10, 11
To test whether expression of RUNX1/ETO is sufficient to increase genomic instability and mutagenesis, we expressed RUNX1/ETO in the non-transformed TK6 lymphoblastoid cell line and measured the acquisition of mutations at the PIGA reporter gene. Cells were transduced with lentivirus carrying either enhanced green fluorescent protein (EGFP) and the RUNX1/ETO fusion or EGFP alone (vector control) (Supplementary Figure 1A; Supplementary Methods) and clones expressing both RUNX1/ETO mRNA and protein were generated (Supplementary Figures 1B and C). For the purposes of measuring RUNX1/ETO-induced mutagenesis, we analysed independent cell clones expressing at least 40% of the fusion transcript found in the Kasumi-1 and SKNO-1 t(8;21)-positive cell lines (Supplementary Figure 1B). Monitoring of RUNX1/ETO-positive clones revealed that expression of the fusion was stable over long culture periods (>12 weeks). Independent vector control clones that expressed equivalent levels of EGFP to RUNX1/ETO-positive cells were used as fusion-protein negative controls (Supplementary Figure 1D).
PIGA encodes a protein essential for production of the glycosylphosphatidylinositol anchor, mediating anchoring of proteins including CD55 and CD59 to the cell membrane.12 Somatic mutations of PIGA are growth neutral and can be determined using flow cytometry analysis measuring CD55 and CD59 expression (Supplementary Figure 2; Supplementary Methods). Using this reporter gene system we determined the mutation frequency (Mf) in several independent RUNX1/ETO-expressing and vector control clones after continuous culture for 8–10 weeks after initial cloning. All clones had a majority population that was positive for CD55 and CD59, confirming that the founding cell was PIGA wild-type (WT). The mean PIGA Mf in RUNX1/ETO clones (7.50 × 10−4) was five times higher than in vector control clones (1.45 × 10−4) (Figure 1a, Supplementary Figure 3A) (P=0.032), with the exception of a single clone that had low expression of the fusion transcript (equivalent to 40% of that in Kasumi-1) (Supplementary Figures 1B and 3A).
The frequency of cells with a mutation (Mf) at a specific gene is determined by the mutation rate per cell division for that gene (μ) and the number of cell divisions (d). Expression of the RUNX1/ETO fusion had a modest but nonsignificant negative effect on cell proliferation (Figure 1b, Supplementary Figure 3B, P=0.812), confirming that the increased Mf in RUNX1/ETO fusion-positive cells was not due to elevated proliferation.
Despite being derived from single cells, EGFP expression in RUNX1/ETO clones was normally distributed in all cell populations (Figure 1c, Supplementary Figure 4), indicating a natural drift in EGFP post cloning. Our data suggest that RUNX1/ETO confers a mutator phenotype in a protein-level-dependent fashion. By using EGFP as a surrogate for RUNX1/ETO we predicted that PIGA-mutant cells would have higher EGFP expression compared with non-mutant cells from the same population. Consistent with this hypothesis, the EGFP geometric mean of fluorescence (GMoF) of PIGA mutant cells derived from RUNX1/ETO cell clones was significantly higher than in non-mutants derived from the same starting population (Figures 1c and d, Supplementary Figure 4, Supplementary Table 1). The only RUNX1/ETO clone that did not show a difference between EGFP GMoF for PIGA WT and mutant cells was that with the lowest RUNX1/ETO expression (clone RE4), which also had no increase in spontaneous PIGA Mf (Supplementary Figure 3A). For vector control clones, the EGFP GMoF was not significantly different between PIGA mutant and WT cells (Figure 1d, Supplementary Figure 4, Supplementary Table 1). These data demonstrate that expression of the RUNX1/ETO fusion oncoprotein confers a mutator phenotype when the transcript is at levels equivalent to at least 60% of that in t(8;21)-positive cell lines.
We next investigated whether RUNX1/ETO transduced cells were particularly sensitive to mutagenesis following exposure to genotoxic anticancer therapies. Fusion protein-positive and vector control clones were exposed to sub-cytotoxic doses of either doxorubicin (100 nM for 4 h) or ionising radiation (3 Gy), and Mf was measured 2 weeks after treatment. The frequency of mutations attributable to doxorubicin or radiation (treatment-induced Mf) was calculated by subtracting the Mf in mock-treated cells from the Mf in doxorubicin- or radiation-treated cells. The mean treatment-induced PIGA Mf was strongly inceased in RUNX1/ETO cell clones compared with vector control clones following either doxorubicin (mean Mf=6.54 × 10−4 vs 0.208 × 10−4, P=0.09) or radiation treatment (mean Mf=5.92 × 10−4 vs 0.209 × 10−4, P=0.008) (Figure 2a, Supplementary Figure 5). As an additional independent measure for treatment-induced Mf we assayed RUNX1/ETO and vector control clones at a second reporter gene, thymidine kinase (TK). The mean treatment-induced TK Mf was also significantly higher in RUNX1/ETO cell clones compared with vector control clones following either doxorubicin (mean Mf=3.53 × 10−6 vs 0.432 × 10−6, P=0.014) or radiation treatment (mean Mf=6.43 × 10−6 vs −0.145 × 10−6, P=0.002) (Figure 2a, Supplementary Figure 5). The only RUNX1/ETO clone that did not show increased sensitivity to doxorubicin or radiation-induced mutation was clone RE4 with low RUNX1/ETO expression (Supplementary Figure 5). For both PIGA and TK, the Mf in vector control clones following doxorubicin or radiation treatment was not significantly different from mock-treated cells (Figure 2a, Supplementary Figure 5), suggesting that, unlike RUNX1/ETO-expressing cells, vector control cells were proficient at repairing treatment-induced DNA damage.
We next investigated whether EGFP expression differed in treatment-induced PIGA mutant cells compared with non-mutant cells derived from the same RUNX1/ETO clonal population. The EGFP GMoF of PIGA mutant cells was significantly higher than in non-mutant cells following treatment with doxorubicin (P=0.03) or ionising radiation (P=0.02) (Figures 2b and c, Supplementary Figure 6). In contrast, the EGFP GMoF was not significantly different between PIGA mutant and WT cells derived from vector control populations following treatment (Figures 2b and c).
These data demonstrate that high levels of RUNX1/ETO sensitise cells to acquisition of mutations following treatment with DNA damage-inducing agents, suggesting that fusion-protein-expressing cells may be compromised in DNA repair. This result is consistent with previously published reports implicating compromised OGG1 DNA glycosylase activity in t(8;21) AML.11, 13 OGG1 functions in base excision repair and initiates repair of oxidised lesions, including 8-hydroxy-2′-deoxyguanosine. We therefore investigated OGG1 expression in 18 independent RUNX1/ETO cell clones and observed that transcript levels were inversely proportional to the expression of the fusion gene (Supplementary Figure 7A). Likewise, OGG1 protein levels were consistently lower in RUNX1/ETO-positive clones compared with vector control clones (Supplementary Figure 7B). We next performed siRNA-mediated depletion of RUNX1/ETO in Kasumi-1, as previously described.5 Two serial electroporations with either RUNX1/ETO or control scrambled siRNA were carried out and OGG1 transcript and protein levels were assessed 72 h after each electroporation. RUNX1/ETO depletion increased OGG1 transcript levels by fourfold and sixfold on days 3 and 6, respectively (Supplementary Figure 7C) with a concomitant increase in OGG1 protein (Supplementary Figures 7C and D). To confirm OGG1 as a RUNX1/ETO target gene we performed ChIP and RNA sequencing after siRNA-mediated RUNX1/ETO depletion. A RUNX1/ETO CHiPseq peak was observed at the OGG1 promoter in control-transfected Kasumi-1 cells, which was lost following siRNA-mediated fusion protein depletion (Supplementary Figure 7E) and was co-localised within a DNaseI hypersensitivity site, as previously reported.6 We also confirmed the increase in OGG1 expression after RUNX1/ETO depletion by RNAseq (Supplementary Figure 7E). Taken together, these data confirm that the RUNX1/ETO fusion protein binds the OGG1 promoter and negatively regulates transcription, suggesting a plausible mechanism by which this common fusion oncoprotein drives mutagenesis. In order to investigate this further, we interrogated whole-genome and exome sequencing data from The Cancer Genome Atlas Project.14 Data were available from 193 AML cases, which included information on 21 386 somatic base substitution mutations, including G>T transversions, the predominant mutation that arises following translesion synthesis of 8-hydroxy-2′-deoxyguanosine and which accumulates following knockdown of OGG1 in experimental systems.15 When stratified by cytogenetic subgroup, 16.13% of all mutations in t(8;21) AML were G>T transversions (16.13%, n=7 cases, Supplementary Table 2), which was higher than any other cytogenetic subgroup and all other AML cases combined (12.14%, n=186 cases), although this did not reach statistical significance (P=0.31, Yates chi-square). These data are consistent with loss of OGG1 contributing to the mutator phenotype in RUNX1/ETO cells by predisposing to G:C>T:A transversions.
By using mutation assays using two independent assays, we have shown that RUNX1/ETO predisposes to the acquisition of mutations, both spontaneously and particularly after treatment with genotoxic agents. We also present evidence that the strength of the mutator phenotype is related to the expression level of the fusion protein. As with all types of AML, relapse is a major cause of mortality in t(8;21) AML. If remission–induction chemotherapy fails to eliminate all the RUNX1/ETO-positive cells, our data suggest that surviving cells are predisposed to mutations that could drive relapse. One consideration for chemotherapy should therefore be to limit mutation of surviving leukemic/preleukemic cells. As such, we hypothesise that targeting the mutator phenotype associated with expression of the RUNX1/ETO fusion gene could impede the acquisition of co-operating mutations required for disease relapse. Our data demonstrate the need to develop novel therapeutic strategies that avoid increasing the mutation burden of AML cells.
References
Wang HY, Tirado CA . t(8;21)(q22;q22) Translocation involving AML1 and ETO in B lymphoblastic leukemia. Hum Pathol 2010; 41: 286–292.
He G, Wu D, Sun A, Xue Y, Jin Z, Qiu H et al. B-Lymphoid and myeloid lineages biphenotypic acute leukemia with t(8;21)(q22;q22). Int J Hematol 2008; 87: 132–136.
Peterson LF, Zhang DE . The 8;21 translocation in leukemogenesis. Oncogene 2004; 23: 4255–4262.
Mulloy JC, Cammenga J, MacKenzie KL, Berguido FJ, Moore MA, Nimer SD . The AML1-ETO fusion protein promotes the expansion of human hematopoietic stem cells. Blood 2002; 99: 15–23.
Martinez Soria N, Tussiwand R, Ziegler P, Manz MG, Heidenreich O . Transient depletion of RUNX1/RUNX1T1 by RNA interference delays tumour formation in vivo. Leukemia 2009; 23: 188–190.
Ptasinska A, Assi SA, Martinez-Soria N, Imperato MR, Piper J, Cauchy P et al. Identification of a dynamic core transcriptional network in t(8;21) AML that regulates differentiation block and self-renewal. Cell Rep 2014; 8: 1974–1988.
Yuan Y, Zhou L, Miyamoto T, Iwasaki H, Harakawa N, Hetherington CJ et al. AML1-ETO expression is directly involved in the development of acute myeloid leukemia in the presence of additional mutations. Proc Natl Acad Sci USA 2001; 98: 10398–10403.
Wang YY, Zhou GB, Yin T, Chen B, Shi JY, Liang WX et al. AML1-ETO and C-KIT mutation/overexpression in t(8;21) leukemia: implication in stepwise leukemogenesis and response to Gleevec. Proc Natl Acad. Sc USA 2005; 102: 1104–1109.
Araten DJ, Krejci O, Ditata K, Wunderlich M, Sanders KJ, Zamecheck L et al. The rate of spontaneous mutations in human myeloid cells. Mutat Res 2013; 749: 49–57.
Krejci O, Wunderlich M, Geiger H, Chou FS, Schleimer D, Jansen M et al. p53 signaling in response to increased DNA damage sensitizes AML1-ETO cells to stress-induced death. Blood 2008; 111: 2190–2199.
Alcalay M, Meani N, Gelmetti V, Fantozzi A, Fagioli M, Orleth A et al. Acute myeloid leukemia fusion proteins deregulate genes involved in stem cell maintenance and DNA repair. J Clin Investig 2003; 112: 1751–1761.
Chen R, Knez JJ, Merrick WC, Medof ME . Comparative efficiencies of C-terminal signals of native glycophosphatidylinositol (GPI)-anchored proproteins in conferring GPI-anchoring. J Cell Biochem 2001; 84: 68–83.
Liddiard K, Hills R, Burnett AK, Darley RL, Tonks A . OGG1 is a novel prognostic indicator in acute myeloid leukaemia. Oncogene 2010; 29: 2005–2012.
The Cancer Genome Atlas Research Network. Genomic and epigenomic landscapes of adult de novo acute myeloid leukemia. N Engl J Med 2013; 368: 2059–2074.
Suzuki T, Harashima H, Kamiya H . Effects of base excision repair proteins on mutagenesis by 8-oxo-7,8-dihydroguanine (8-hydroxyguanine) paired with cytosine and adenine. DNA Repair 2010; 9: 542–550.
Acknowledgements
This work was supported by grants from Leukaemia and Lymphoma Research (#13044 to JMA and #10033, #12055 to OH) and the JGW Patterson Foundation (to JMA and OH). VJF designed and performed research, analysed data and wrote the manuscript. MHN, NM-S, AKB, AP, SEF, HM and SAA performed research. CB and OH designed research and analysed data. JMA conceived the project, designed research, analysed data and wrote the manuscript. All authors approved the final version of the manuscript.
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Forster, V., Nahari, M., Martinez-Soria, N. et al. The leukemia-associated RUNX1/ETO oncoprotein confers a mutator phenotype. Leukemia 30, 251–254 (2016). https://doi.org/10.1038/leu.2015.133
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DOI: https://doi.org/10.1038/leu.2015.133
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