Abstract
Multiple myeloma (MM) is a plasma cell cancer with poor survival, characterized by the expansion of multiple myeloma cells (MMCs) in the bone marrow. Using a microarray-based genome-wide screen for genes responding to DNA methyltransferases (DNMT) inhibition in MM cells, we identified RECQ1 among the most downregulated genes. RecQ helicases are DNA unwinding enzymes involved in the maintenance of chromosome stability. Here we show that RECQ1 is significantly overexpressed in MMCs compared to normal plasma cells and that increased RECQ1 expression is associated with poor prognosis in three independent cohorts of patients. Interestingly, RECQ1 knockdown inhibits cells growth and induces apoptosis in MMCs. Moreover, RECQ1 depletion promotes the development of DNA double-strand breaks, as evidenced by the formation of 53BP1 foci and the phosphorylation of ataxia-telangiectasia mutated (ATM) and histone variant H2A.X (H2AX). In contrast, RECQ1 overexpression protects MMCs from melphalan and bortezomib cytotoxicity. RECQ1 interacts with PARP1 in MMCs exposed to treatment and RECQ1 depletion sensitizes MMCs to poly(ADP-ribose) polymerase (PARP) inhibitor. DNMT inhibitor treatment results in RECQ1 downregulation through miR-203 deregulation in MMC. Altogether, these data suggest that association of DNA damaging agents and/or PARP inhibitors with DNMT inhibitors may represent a therapeutic approach in patients with high RECQ1 expression associated with a poor prognosis.
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Introduction
Multiple myeloma (MM) is the second most common hematologic malignancy. It is characterized by the accumulation of malignant plasma cells (MMCs) within the bone marrow (BM). MM is a genetically complex disease characterized by altered karyotypes including chromosomal translocations, aneuploidies and DNA copy-number variations.1 In addition to genetic changes, intraclonal heterogeneity of MMCs was recently described as a new level of complexity in MM pathophysiology.2, 3, 4, 5, 6, 7 Epigenetic events could also participate in disease progression and treatment resistance.8 DNA methyltransferase (DNMT) inhibitors and histone deacetylases inhibitors are now being used in the treatment of several hematologic malignancies including MM.9, 10, 11, 12, 13, 14, 15
Recently, we initiated a microarray-based genome-wide screen for genes responding to DNMT inhibition in our large cohort of MM cell lines.16, 17 We identified RECQ1 among the genes downregulated by DNMTi and associated with the worst prognostic value in MM patients.17 RECQ helicases are a family of DNA unwinding enzymes involved in the maintenance of chromosome stability.18 Several functions have been attributed to RECQ proteins, including roles in stabilization and repair of damaged DNA replication forks, homologous recombination and DNA damage checkpoint signaling.19 Mutations in three of the five human RecQ helicases, BLM, WRN and RECQL4, are associated with genetic disorders, respectively, with Bloom’s, Werner and Rothmund–Thomson syndromes, which are characterized by chromosomal instability, premature aging and increased susceptibility to cancer.19 RECQ1 promotes recovery of stalled replication forks.20, 21, 22 Furthermore, RECQ1 accumulates at replication origins in unperturbed cells and at common fragile sites where replication forks have stalled upon cellular exposure to replication inhibitors.23 The role of RECQ1 in replication stress response could be especially important for cancer cells.24 RECQ1 is highly expressed in various types of solid tumors.25, 26, 27, 28 RECQ1 silencing in cancer cells resulted in mitotic catastrophe and prevented tumor growth in murine models.24, 28, 29 Furthermore, RECQ1 depletion induces mitotic cell death in a wide range of solid cancer cell lines but not in normal fibroblasts.24 In glioblastoma cell lines, depletion of RECQ1 results in a significant reduction of cellular proliferation, spontaneous γH2AX foci formation and hypersensitivity to treatments.25 The ability of RECQ1 to support replication recovery could be particularly important for cancer cells. RECQ1 binds G4 motifs in the promoter of genes that are downregulated upon RECQ1 silencing.30 Recent data suggest that RECQ1 could enhance the expression of genes involved in cell migration, invasion and metastasis in solid cancers.30 Accordingly, RECQ1 depletion in breast cancer cell line resulted in a significant inhibition of migration and invasion. Collectively, all these data underline that RECQ1 could play a role in MM pathophysiology and drug resistance with the hallmark feature of oncogene-induced DNA replication stress. γ-histone variant H2A.X (H2AX) analysis demonstrated that MMCs have constitutive ongoing DNA damage.31, 32 High chromosomal instability and replicative stress defines a subgroup of MM patients with poor outcome.33, 34 Furthermore, despite significant advances in MM treatment, including proteasome inhibitors, immunomodulatory agents and novel epigenetic-targeted treatments, that significantly prolonged the median survival, the majority of MM patients relapse with the development of drug resistance.35 Therefore, we intent to explore the impact of RECQ1 in MM pathophysiology.
Materials and methods
Human myeloma cell lines (HMCLs)
XG1, XG2, XG3, XG4, XG5, XG6, XG7, XG10, XG11, XG12, XG13, XG14, XG16, XG19, XG20 and XG21 HMCLs were obtained as previously described.36 AMO-1, LP1, L363, U266, OPM2 and SKMM2 were purchased from DSMZ (Braunschweig, Germany) and RPMI8226 from ATTC (Rockville, MD, USA). HMCLs were authenticated according to their short tandem repeat profiling and their gene expression profiling using Affymetrix U133 plus 2.0 microarrays deposited in the ArrayExpress public database under accession numbers E-TABM-937 and E-TABM-1088.36
Primary multiple myeloma cells
BM samples were collected after patients’ written informed consent in accordance with the Declaration of Helsinki and institutional research board approval from Heidelberg and Montpellier University hospital. In particular, BMs were collected from 206 patients treated with high-dose melphalan and autologous stem cell transplantation and this cohort is termed in the following Heidelberg–Montpellier cohort.37 Patients’ MMCs were purified using anti-CD138 MACS microbeads (Miltenyi Biotech, Bergisch Gladbach, Germany) and their gene expression profile obtained using Affymetrix U133 plus 2.0 microarrays as described (E-MTAB-372).37 The structural chromosomal aberrations, including t(4;14)(p16.3;q32.3) and t(11;14)(q13;q32.3), as well as numerical aberrations including 17p13 and 1q21 gain, were assayed by fluorescence in situ hybridization (iFISH). We also used publicly available Affymetrix gene expression profile (Gene Expression Omnibus, GSE2658) of a cohort of 345 purified MMC from previously untreated patients from the University of Arkansas for Medical Sciences (UAMS, Little Rock, AR, USA), termed in the following UAMS-TT2 cohort.38 We also used total therapy 3 cohort (UAMS-TT3; n=158; E-TABM-1138)39 and data of 152 relapsed MM patients subsequently treated with bortezomib (GSE9782) from the study by Mulligan et al.40
Cell growth assay, cell cycle and apoptosis analyses
HMCLs were cultured for 4 days in 96-well flat-bottom microtiter plates in RPMI 1640 medium, 10% FCS and 2 ng/ml IL-6 (control medium) in the presence of various compounds. Cell growth was evaluated by quantifying intracellular ATP amount with a Cell Titer Glo Luminescent Assay (Promega, Madison, WI, USA) using a Centro LB 960 luminometer (Berthold Technologies, Bad Wildbad, Germany). Doxycycline (1 mg/ml) was added to induce shRECQ1 expression. The cell cycle was assessed using 49,6-diamidino-2-phenylindole (DAPI) staining (Sigma-Aldrich, Munich, Germany), incubation with bromodeoxyuridine (BrdU) for 1 h, and labeling with an anti-BrdU antibody (APC BrdU flow kit, BD Pharmingen, Le Pont De Claix, France) as described.41 Apoptotic cells were detected using phycoerythrin-conjugated Annexin V (PE-annexin V, BD Pharmingen). Apoptosis was measured using caspase-3/7 and caspase-9 luminescence Assay (Caspase Glo Assay (Promega, Madison, WI, USA)) according to the manufacturer’s protocol.
RECQ1 depletion in primary MM cells
BM of patients presenting with previously untreated MM (n=7) at the university hospital of Montpellier was obtained after patients’ written informed consent in accordance with the Declaration of Helsinki and agreement of the Montpellier University Hospital Centre for Biological Resources (DC-2008-417). Mononuclear cells were transfected with shRECQ1 or shRNA scramble lentivirus and MMC cytotoxicity evaluated using anti-CD138-phycoerythrin monoclonal antibody (Immunotech, Marseille, France) as described.17
DNA repair foci—immunofluorescence microscopy
After deposition on slides using a Cytospin centrifuge, cells were fixed with 4% paraformaldehyde, permeabilized with 0.5% Triton in phosphate-buffered saline (PBS) and saturated with 5% bovine milk in PBS. The rabbit anti-53BP1 antibody (clone NB100-304, Novus Biologicals, Cambridge, UK) and the mouse anti-γH2AX (Ser139) antibody (clone JBW301, Merck Millipore, Darmstadt, Germany) were diluted 1/300 and 1/100, respectively, in 5% bovine milk in PBS, and deposited on cytospins for 90 min at room temperature. Slides were washed twice and antibodies to rabbit or mouse immunoglobulins conjugated to alexa 488 (diluted 1/500 in 5% bovine milk in PBS) were added for 45 min at room temperature. Slides were washed and mounted with Vectashield and 1% DAPI. Images and fluorescence were captured with a ZEISS Axio Imager Z2 microscope (× 63 objective), analyzed with Metafer (version3.6, company, town state) and ImageJ software. The number of 53BP1 and γH2AX foci was counted in at least 300 nuclei.
Supplementary informations concerning methodology are included in Supplementary experiment procedures.
Results
RECQ1 is overexpressed in MMCs
RECQ1 expression was analyzed in normal bone marrow plasma cells (BMPCs), primary myeloma cells from newly diagnosed patients (MMCs) and HMCLs using Affymetrix microarrays. RECQ1 gene was significantly overexpressed in MMCs of patients (median=1499; range: 251–6488) compared to normal BMPCs (median=841; range: 523–1519; P<0.001). The expression was even higher in HMCLs (median=3233; range: 811–5873) compared to primary MMCs or BMPCs (P<0.001; Figure 1a). RECQ1 expression was confirmed at protein level in HMCLs, in patients’ primary MMCs (Figure 1b). RECQ1 expression was significantly higher in the poor prognosis proliferation group (P<0.01) and in the CD1 group (P<0.05), and downregulated in the hyperdiploid MM subgroup42 (Supplementary Figure S1A). RECQ1 overexpression in MMCs compared to normal B and plasma cells was also validated by qPCR and western blot (Supplementary Figure S1B and Figure 1b). A high RECQ1 expression in MMCs could predict for both shorter event-free (EFS) and overall survival (OS) in the Heidelberg–Montpellier cohort of 206 previously untreated patients (Figure 1c). These patients could be split in two groups according to RECQ1 expression and patients’ survival using the Maxstat algorithm.16, 43 A group encompassing 17.5% of patients with the highest RECQ1 expression in MMCs had reduced EFS (median=22.7 months) and OS (median=73.3 months) compared to the remaining patients with lower RECQ1 expression (median EFS=34.2 months and median OS=92 months, P⩽0.01) (Figure 1c). A high RECQ1 expression in MMCs was likewise associated with a poor prognosis in the independent UAMS-TT2 (Supplementary Figure S2A, P<0.001) and UAMS-TT3 cohorts of patients (Supplementary Figure S2B, P=0.001). Of note, RECQ1 was significantly overexpressed in patients with del17p, del13 and 1q21 gain (Supplementary Figure S2C), but no correlation was observed with t(4;14) and t(11;14) translocations. The frequency of patients with age⩾65 years, high β-2-microglubuline or high C-reactive protein levels were significantly increased in patients with high RECQ1 expression (P<0.05; Supplementary Table S1). No significant correlation between RECQ1 expression and MMC plasma cell labeling index was found (Supplementary Figure S3).
Interestingly, gene set expression analysis of patients with high RECQ1 expression highlighted a significant enrichment of genes involved in embryonic stem cells transcriptional program and overexpressed in plasmablasts, compared to BM mature plasma cells (Supplementary Figure S4A and Supplementary Tables S2 and S3). In contrast, patients with low RECQ1 expression are characterized by a significant enrichment of genes overexpressed in TACIhigh MMCs and involved in cytokine/cytokine receptor interactions linked with a mature plasma cell gene signature and BM microenvironment dependence44 (Supplementary Figure S4B and Supplementary Tables S4 and S5). Altogether, these data indicate that RECQ1 is significantly overexpressed in MM cells in association with a plasmablastic gene signature and a poor prognosis.
RECQ1 depletion in MMCs affects cell division and induces apoptosis
To investigate the functional significance of RECQ1 overexpression in multiple myeloma cells, XG19, LP1 and XG7 HMCLs were transduced with a doxycycline-inducible lentivirus containing a RECQ1 shRNA. Doxycycline treatment induced a 68–87% reduction of RECQ1 expression at RNA level (P<0.01; Supplementary Figure S5) and a 70–90% reduction at the protein level (P<0.01; Figures 2a and b). RECQ1 depletion induced a progressive death of XG19, LP1 and XG7 TR-shRNA RECQ1 cells, which started 3–4 days after doxycycline addition (Figure 2c, P=0.001 and Supplementary Figure S6A). Doxycycline marginally affected the growth of control HMCL-TRs (Figure 2c and Supplementary Figure S6A). Remarkably, RECQ1 depletion induced apoptosis in HMCL-TR-shRECQ1, which initiated on day 3 and increased on day 7, with 79, 53 and 38% of Annexin-V-positive XG19, LP1 and XG7 TR-shRECQ1 cells, respectively (Supplementary Figure S6B, P<0.05). Apoptosis induced by the depletion of RECQ1 was associated with activation of caspase-9, -3 and -7 (Figure 2d) and could be rescued by adding the Quinoline-Val-Asp-Difluorophenoxymethylketone pan-caspase inhibitor (Supplementary Figure S7). RECQ1 depletion also affected the cell cycle distribution of surviving cells with a blockage of BrdU incorporation and an increase in the G1 and G2/M phases (P<0.05; Figure 3a, P<0.01 and Supplementary Figures S8A and B). These phenotypes were reproduced after RECQ1 suppression using a second shRNA with different targeting sequence (Supplementary Figures S9A, B, C and D) and rescued by the ectopic expression of a shRNA-resistant RECQ1 gene (Supplementary Figures S10A, B and C).
To confirm that RECQ1 is also required for the survival of primary MMCs from patients, BM samples containing malignant MMCs were transduced45, 46 with shRECQ1 lentiviruses and primary MM cells were cultured with their BM environment and recombinant IL-6 as described.17 RECQ1 depletion significantly reduced the median number of viable myeloma cells by 56% (P=0.004; N=7) compared to scramble shRNA (Figure 3b). Of interest, the normal BM non-myeloma cells were not significantly affected by the shRNA (Figure 3b). RECQ1 expression downregulation after transduction was validated in primary MMC of patient using real-time PCR (Supplementary Figure S11). We therefore conclude that viability of MM cell lines and primary MM cells depends on high RECQ1 expression levels.
RECQ1-deficient MMCs show spontaneous DNA breaks and activate the DNA damage response (DDR)
Given the known role of RECQ1 in DNA replication and DDR,21, 47 the effect of RECQ1 depletion on spontaneous DNA damage was investigated. Interestingly, RECQ1 depletion in XG19 HMCLs induced DNA strand breaks as indicated by the alkaline comet assay that detect both single- and double-strand breaks (Figure 4a and Supplementary Figure S12). Indeed, a significant increase in comet tail length and moment was found in XG19-TR-shRECQ1 cells treated with doxycycline compared to control cells (P<0.001, Figure 4a). RECQ1 depletion was also associated with the accumulation of DNA double-strand breaks, as evidenced by increased phosphorylation of the histone variant H2AX and the accumulation of 53BP1 foci (Figures 4b and c and Supplementary Figure S13A). These data were validated after RECQ1 suppression using a second shRNA with different targeting sequence (Supplementary Figure S13B). Finally, RECQ1 depletion induced a DDR associated with an increased phosphorylation of ataxia-telangiectasia mutated (ATM), Chk1, Chk2, P53 and H2AX (Figure 4c). These phenotypes were rescued by the ectopic RECQ1 gene expression (Supplementary Figure S10D). Together, these data indicate that high RECQ1 levels protect MMCs from spontaneous intrinsic DNA damage.
Delayed progression of the replication forks upon RECQ1 depletion
Although it has been reported that RECQ1 plays a role in the maintenance of DNA replication forks,20 we next monitored the role of increased RECQ1 expression on fork progression in MM cells using DNA fiber analysis. To this end, HMCLs were pulse-labeled with 10 μM IdU and 100 μM CldU and the length of CldU tracks was measured to estimate the distance covered by individual forks during the pulse. Interestingly, the length of CldU tracks was significantly shorter in RECQ1-depleted MMCs relative to control cells (P<0.0001; Figure 4d). These data indicate that high RECQ1 levels promote the efficient progression of replication forks in MMCs and suggest that defective fork progression accounts for the increased spontaneous DNA damage in RECQ1-deficient MMCs.
RECQ1 overexpression protects MMCs against melphalan and bortezomib
The results presented above indicate that the overexpression of RECQ1 in MMCs protects them from spontaneous DNA damage and replication stress. Since chemotherapy also induces DNA breaks, we next investigated whether RECQ1 overexpression protects MMCs against dexamethasone, bortezomib or melphalan (Figures 5a and d). Remarkably, the forced expression of RECQ1 in XG7 and XG19 HMCLs (Supplementary Figure S14) resulted in an increased resistance to melphalan and bortezomib-induced cell death, (P<0.05; Figures 5a and d), but had no significant effect on the sensitivity to lenalidomide (Supplementary Figure S15) and dexamethasone (data not shown). Furthermore, a BrdU incorporation assay demonstrated that RECQ1-overexpressing cells surviving after melphalan exposure are still able to proliferate, whereas control myeloma cells are irreversibly blocked in G2/M phase (Figure 5b and Supplementary Figures S16A and B). Interestingly, increased RECQ1 levels did not affect the number of γH2AX foci 24 h after melphalan treatment demonstrating that melphalan induced the same amount of DNA damages in control and myeloma cells overexpressing RECQ1 (Supplementary Figure S17). However, after 72 h of melphalan treatment, the comet assay revealed that cells overexpressing RECQ1 repair DNA breaks induced by melphalan more efficiently than control cells (Figure 5c).
Although RECQ1 overexpression is inhibited by DNMTi such as 5-azacytidine,17 we next tested whether 5-azacitidine treatment sensitize MMCs to melphalan-induced apoptosis. We found that both 5-azacytidine and the direct depletion of RECQ1 with shRNAs sensitized MMCs to melphalan (Supplementary Figures S18A–C). RECQ1 overexpression protects MMCs from bortezomib-induced toxicity (Figure 5d). These observations are consistent with the fact that high RECQ1 expression is associated with a poor prognosis in a cohort of patients at relapse treated by bortezomib monotherapy (Figure 5d). Altogether, these data indicate that RECQ1 plays a central role in the protection of MM cells against both spontaneous DNA damage and DNA lesions induced by chemotherapeutic agents such as bortezomib and melphalan.
Identification of RECQ1-interacting proteins
To identify the proteins that interact with RECQ1 in MMCs, we next immunoprecipitated RECQ1 from the chromatin fraction prepared from XG7 cells. Duplicate mass spectrometry analysis of the SDS-PAGE lanes obtained from RECQ1 immunoprecipitation resulted in a total of 183 proteins after subtraction of the proteins commonly identified with the IgG control antibody (Supplementary Table S6). Among them, several proteins already described as RECQ1-interacting partners were identified, including RPA, PARP1, Ku80, MSH2 and MSH6(refs 48, 49) (Supplementary Table S6). We also observed a significant enrichment in proteins involved in RNA processing and splicing, transcription regulation, regulation of helicase activity and regulation of DDR (Supplementary Table S7), including PARP1, which is consistent with an earlier study.20
RECQ1 interacts with PARP1 and RECQ1 depletion sensitizes MMCs to PARPi
RECQ1 and PARP1 are involved in the control of DNA repair, telomere maintenance and replicative stress responses.50 To further understand the mechanisms of DNA damage induced by RECQ1 depletion in MMCs and validate proteomic results, we analyzed the interactions between PARP1 and RECQ1 in XG7 nuclear extracts. In agreement with mass spectrometry results, we found that PARP1 immunoprecipitates with RECQ1 (Supplementary Figure S19). Of note, the amount of PARP1 bound to RECQ1 was increased after treatment of MMCs with melphalan and bortezomib (Supplementary Figures S19A and B). Given the association of RECQ1 and PARP1 and the clinical development of poly(ADP-ribose) polymerase (PARP) inhibitors in cancer, we next investigated how RECQ1 depletion affects the sensitivity of MMCs to PARP inhibitor. Cells were pulsed with doxycycline for 2 days and treated with increasing PJ34 hydrochloride concentrations for 4 days. RECQ1 depletion significantly sensitized XG7 and XG19 HMCLs to PARPi-induced apoptosis (Figures 6a and b).
DNMTi induces miR-203 expression and targets RECQ1 expression in MMCs
RECQ1 expression was recently described as one of the predicted targets of miR-203 in tongue squamous cell carcinoma.27 Since aberrant methylation of miR-203 promoter region was reported in MMCs but not in normal plasma cells,51 this prompted us to investigate the expression of miR-203 in MMCs exposed to 5-azacytidine. Remarkably, we observed that 5-azacytidine treatment significantly induced miR-203 expression in HMCLs and a concomitant downregulation of RECQ1 (Figure 7a). Moreover, treatment of XG7 and XG19 HMCLs with a specific anti-miR-203 miRNA inhibitor resulted in a significant increase of RECQ1 expression (Figure 7b). Altogether, these data suggest that the epigenetic downregulation of miR-203 in MMCs allows RECQ1 overexpression and increased resistance to melphalan and bortezomib.
Discussion
Here we show that RECQ1 plays a central role in MM biology and in the resistance of MMCs to chemotherapy. Recent studies have pointed out a critical role of RECQ1 in the process of DNA replication, repair and transcription.52 Our data confirm and extend this role to HMCLs and to primary MMCs. In MM, a subset of patients is characterized by chromosomal instability, replicative stress and adverse prognosis.34 Furthermore, MYC dysregulation triggers replicative stress and DNA damage in MM cells.34 In HMCLs, we found that RECQ1 depletion induced a dramatic increase of spontaneous DNA damage, illustrated by the presence of ssDNA breaks in virtually all cells analyzed with the comet assay. Spontaneous DNA double-strand breaks (DSBs) were also detected by immunofluorescence using γ-H2AX and 53BP1 foci as markers of chromosome breaks. These breaks were accompanied with an impaired progression of replication forks and the persistence of surviving MMCs in the G1 or G2 phases of the cell cycle, followed by their progressive death. RECQ1 depletion also induced a massive death of patients’ MMCs without poorly affecting the survival of non-tumor environment cells. Our data demonstrate that RECQ1 contributes to replication stress survival of MM cells.
In spite of effective therapeutic protocols developed in MM, drug resistance remains a major concern. We reported that RECQ1 overexpression was associated with drug resistance in MMC. RECQ1 plays a central role in the protection of MM cells against DNA lesions induced by chemotherapeutic agents such as melphalan and bortezomib. Melphalan is an alkylating agent used in patients receiving high-dose chemotherapy and autologous hematopoietic stem cell transplantation and in non-transplantable patients in combination with other compounds. Bortezomib is a proteasome inhibitor used as a first-in-class drug in MM. Since, protein ubiquitination is essential in regulation and coordination of various pathways of DNA damage recognition, signaling and repair,53 proteasome inhibitors affect DNA repair.54, 55, 56 The protective effect of RECQ1 overexpression against melphalan and bortezomib is associated with the poor prognosis of high RECQ1 expression in MM patients treated with high-dose melphalan and autologous hematopoietic stem cell transplantation (Figure 1c and Supplementary Figures S2A and B) and in relapsing patients treated with bortezomib monotherapy (Figure 5d). Among the RECQ1-interacting proteins, we identified several proteins involved in DNA repair pathways, including PARP1, RPA, Ku80, MSH2 and MSH6. Regression of replication fork appears as a pivotal response mechanism to replication stress and occurs in 15–40% of the forks after exposure to sublethal doses of Top1 inhibitors. Interestingly, this process is regulated by RECQ1 and PARP1.20 PARP activity is dispensable in the formation of reversed forks but is important to maintain and protect them from the counteracting activity of RECQ1 that would cause the restart of reversed forks, leading to DSB formation.20 PARP was shown to signal the presence of lesions on the template and to inhibit RECQ1 locally, thereby restraining the restart of reversed forks until repair of the Top1 cleavage complex is completed.20 These mechanisms could also be involved in MMC resistance to genotoxic agents. Therefore, we reported an increased association of PARP1 and RECQ1 in nuclear extracts of MM cells upon DNA damages induced by melphalan. PARP1 is a target for anticancer therapies and several PARP inhibitors are currently in clinical trials in cancer.57 The effects of PARPi were initially linked to inhibition of the role of PARP1 in base excision repair of DNA damages induced by endogenous or exogenous agents, resulting in accumulation of single-strand breaks, which upon conversion to toxic DSB lesions would kill cancer cells deficient in DSB repair.57 PARPi could also have a therapeutic activity targeting the role of PARP1 in other DNA repair pathways such as NER58 and also via upregulation of NHEJ pathway leading to increased genomic instability due to imprecise repair.59 Our results demonstrate that RECQ1 depletion significantly sensitizes MMCs to PARPi-induced apoptosis. Coupled to the inhibitory effect of PARPi on accumulation of regressed replication forks, it could explain the higher sensitivity of RECQ1-depleted MMCs to PARPi treatment. RECQ1 expression was identified to be inhibited after DNMTi treatment in MM cells.17, 60 We identified RECQ1 as a target of miR-203 in MM cells, as previously reported in tongue carcinoma.27 The aberrant methylation of miR-203 promoter reported in MMCs compared to normal plasma cells51 underlines a mechanism responsible for abnormal RECQ1 overexpression in MM cells (Figure 8). Thus, DNMTi treatment presents therapeutic interest to target RECQ1 expression in MM and induces replicative stress and higher sensitivity to DNA damaging agents (Figure 8 and Supplementary Figure S18). Our data suggest that the association of PARPi to DNMTi and melphalan could act as synthetic lethality treatment in myeloma patients with high expression of RECQ1 and adverse prognosis (Supplementary Figure S20). A study reported that proteasome inhibitor sensitizes MM cells to PARPi treatment.56 According to our results demonstrating the protective effect of RECQ1 overexpression against bortezomib therapy and the cooperation between RECQ1 and PARP1 in DNA replication, combination between DNMTi, proteasome inhibitor and PARPi could be of clinical interest in MM. Interestingly, targeted inhibitors against RECQ1 helicase are currently in development.61
Our data suggest that combination of DNMTi to target RECQ1 expression with melphalan, proteasome inhibitors and/or PARP inhibitors could have a therapeutic interest in RECQ1high myeloma patients associated with a poor survival.
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Acknowledgements
This work was supported by grants from French INCA (Institut National du Cancer) Institute (2012-109/087437 and PLBIO15-256), Languedoc Roussillon CRLR (R14026FF), Fondation de France (201400047510), ITMO Cancer (MM&TT) and Siric Montpellier (INCa-DGOS-Inserm 6045). EV is supported by a grant from Guillaume Espoir association (Saint-Genis-Laval, France).
Author contributions
EV performed research and participated in the writing of the paper. CG, AB and CG participated in the research. HG, AS, LV and DH participated in clinical data analysis and participated in the writing of the paper. LT participated in proteomic analyses. CH supervised proteomic analyses and participated in the writing of the paper. BK, JB, Y-LL, AC and PP participated in the research and in the writing of the paper. JM supervised the research and the writing of the paper.
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Viziteu, E., Klein, B., Basbous, J. et al. RECQ1 helicase is involved in replication stress survival and drug resistance in multiple myeloma. Leukemia 31, 2104–2113 (2017). https://doi.org/10.1038/leu.2017.54
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DOI: https://doi.org/10.1038/leu.2017.54
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