1 2665 143 ESTABLISHMENT OF A NOVEL MYELODYSPLASTIC SYNDROME (MDS) XENOTRANSPLANTATION MODEL. BACKGROUND: MYELODYSPLASTIC SYNDROME (MDS) IS A CLONAL DISEASE OF THE ELDERLY CHARACTERIZED BY CHRONIC CYTOPENIA, DYSPLASIA, AND A HIGH RISK OF PROGRESSION TO ACUTE MYELOID LEUKEMIA (AML). UP UNTIL NOW, FEW ANIMAL MODELS THAT FULLY RECAPITULATE CLINICAL FEATURES OF THIS DISEASE HAVE BEEN AVAILABLE. METHODS: THIS STUDY AIMED TO ESTABLISH A NEW MDS XENOGRAFT MODEL UTILIZING A HUMAN MDS-DERIVED CELL LINE WITH HETEROZYGOUS Y641C MUTATION OF EZH2 (SKM-1). 1 X 107 SKM-1 CELLS WERE INOCULATED INTO ANTI-MOUSE CD122 MONOANTIBODY CONDITIONED NONOBESE DIABETIC SEVERE COMBINED IMMUNODEFICIENCY (NOD/SCID) MICE BY INTRAVENOUS INJECTION. DECITABINE WAS INJECTED INTRAPERITONEALLY FOR EVALUATION OF EPIGENETIC DRUGS IN VIVO. RESULTS: IT IS SHOWN THAT THE HETEROZYGOUS Y641C MUTATION IN THE EZH2 GENE MUTATION, WHICH MAY DESTABILIZE THE PROTEIN (??G = 1.46 KCAL/MOL), CAN BE FOUND IN SKM-1 CELLS. MOST MICE PRESENTED ANEMIA AND LEUKOPENIA AT THREE TO FOUR WEEKS AFTER INOCULATION. THE PERIPHERAL BLOOD AND BONE MARROW SMEAR SHOWED PROMINENT DYSPLASIA ON ERYTHROCYTES AND GRANULOCYTES AS WELL AS MONOCYTES. CONCLUSIONS: THESE FINDINGS SUGGEST THAT INTRAVENOUS INOCULATION OF CELLS FROM THE HUMAN MDS-DERIVED CELL LINE PRIOR TO TARGETED DEPLETION OF CD122+ CELLS COULD PROVIDE A NOVEL MDS-LIKE XENOTRANSPLANT MOUSE MODEL. IT IS A USEFUL TOOL FOR EVALUATING POTENTIAL EXISTING AND NOVEL THERAPEUTICS FOR MDS. 2016 2 2462 41 EPIGENETIC THERAPY OF MYELODYSPLASTIC SYNDROMES CONNECTS TO CELLULAR DIFFERENTIATION INDEPENDENTLY OF ENDOGENOUS RETROELEMENT DEREPRESSION. BACKGROUND: MYELODYSPLASTIC SYNDROMES (MDS) AND ACUTE MYELOID LEUKAEMIA (AML) ARE CHARACTERISED BY ABNORMAL EPIGENETIC REPRESSION AND DIFFERENTIATION OF BONE MARROW HAEMATOPOIETIC STEM CELLS (HSCS). DRUGS THAT REVERSE EPIGENETIC REPRESSION, SUCH AS 5-AZACYTIDINE (5-AZA), INDUCE HAEMATOLOGICAL IMPROVEMENT IN HALF OF TREATED PATIENTS. ALTHOUGH THE MECHANISMS UNDERLYING THERAPY SUCCESS ARE NOT YET CLEAR, INDUCTION OF ENDOGENOUS RETROELEMENTS (ERES) HAS BEEN HYPOTHESISED. METHODS: USING RNA SEQUENCING (RNA-SEQ), WE COMPARED THE TRANSCRIPTION OF ERES IN BONE MARROW HSCS FROM A NEW COHORT OF MDS AND CHRONIC MYELOMONOCYTIC LEUKAEMIA (CMML) PATIENTS BEFORE AND AFTER 5-AZA TREATMENT WITH HSCS FROM HEALTHY DONORS AND AML PATIENTS. WE FURTHER EXAMINED ERE TRANSCRIPTION USING THE MOST COMPREHENSIVE ANNOTATION OF ERE-OVERLAPPING TRANSCRIPTS EXPRESSED IN HSCS, GENERATED HERE BY DE NOVO TRANSCRIPT ASSEMBLY AND SUPPORTED BY FULL-LENGTH RNA-SEQ. RESULTS: CONSISTENT WITH PRIOR REPORTS, WE FOUND THAT TREATMENT WITH 5-AZA INCREASED THE REPRESENTATION OF ERE-DERIVED RNA-SEQ READS IN THE TRANSCRIPTOME. HOWEVER, SUCH INCREASES WERE COMPARABLE BETWEEN TREATMENT RESPONSES AND FAILURES. THE EXTENDED VIEW OF HSC TRANSCRIPTIONAL DIVERSITY OFFERED BY DE NOVO TRANSCRIPT ASSEMBLY ARGUED AGAINST 5-AZA-RESPONSIVE ERES AS DETERMINANTS OF THE OUTCOME OF THERAPY. INSTEAD, IT UNCOVERED PRE-TREATMENT EXPRESSION AND ALTERNATIVE SPLICING OF DEVELOPMENTALLY REGULATED GENE TRANSCRIPTS AS PREDICTORS OF THE RESPONSE OF MDS AND CMML PATIENTS TO 5-AZA TREATMENT. CONCLUSIONS: OUR STUDY IDENTIFIES THE DEVELOPMENTALLY REGULATED TRANSCRIPTIONAL SIGNATURES OF PROTEIN-CODING AND NON-CODING GENES, RATHER THAN ERES, AS CORRELATES OF A FAVOURABLE RESPONSE OF MDS AND CMML PATIENTS TO 5-AZA TREATMENT AND OFFERS NOVEL CANDIDATES FOR FURTHER EVALUATION. 2019 3 1901 37 ENGRAFTMENT OF CHRONIC MYELOMONOCYTIC LEUKEMIA CELLS IN IMMUNOCOMPROMISED MICE SUPPORTS DISEASE DEPENDENCY ON CYTOKINES. CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML) IS A CLONAL HEMATOPOIETIC STEM CELL DISORDER THAT TYPICALLY ASSOCIATES WITH MUTATIONS IN EPIGENETIC, SPLICING, AND SIGNALING GENES. GENETICALLY MODIFIED MOUSE MODELS ONLY PARTIALLY RECAPITULATE THE DISEASE PHENOTYPE, WHEREAS XENOTRANSPLANTATION OF CMML CELLS IN IMMUNOCOMPROMISED MICE HAS BEEN RARELY SUCCESSFUL SO FAR. HERE, CMML CD34(+) CELLS SORTED FROM PATIENT BONE MARROW (BM) OR PERIPHERAL BLOOD (PB) WERE INJECTED INTRAVENOUSLY INTO NSG (NOD/LTSZ-SCID IL2RGAMMANULL) MICE AND NSG MICE ENGINEERED TO EXPRESS HUMAN GRANULO-MONOCYTE COLONY-STIMULATING FACTOR, STEM CELL FACTOR, AND INTERLEUKIN-3 (NSGS MICE). FIFTEEN OUT OF 16 PATIENT SAMPLES (94%) SUCCESSFULLY ENGRAFTED INTO NSG OR NSGS OR BOTH MOUSE STRAINS. THE EXPANSION OF HUMAN CELLS, PREDOMINANT IN THE BM, WAS ALSO OBSERVED IN THE SPLEEN AND THE PB AND WAS GREATLY ENHANCED IN MICE PRODUCING THE 3 HUMAN CYTOKINES. GENE MUTATIONS IDENTIFIED IN ENGRAFTED CELLS WERE MOSTLY SIMILAR TO THOSE IDENTIFIED IN PATIENT CELLS BEFORE INJECTION. SUCCESSFUL SECONDARY ENGRAFTMENT WAS OBTAINED IN NSGS MICE IN 3 OUT OF 10 ATTEMPTS. THUS, PRIMARY CMML LEUKEMIC CELLS EXPAND MUCH BETTER IN NSGS COMPARED WITH NSG MICE WITH LIMITED EFFICACY OF SECONDARY TRANSPLANT. 2017 4 2237 43 EPIGENETIC MODIFIERS IN MYELOID MALIGNANCIES: THE ROLE OF HISTONE DEACETYLASE INHIBITORS. MYELOID HEMATOLOGICAL MALIGNANCIES ARE CLONAL BONE MARROW NEOPLASMS, COMPRISING OF ACUTE MYELOID LEUKEMIA (AML), THE MYELODYSPLASTIC SYNDROMES (MDS), CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML), THE MYELOPROLIFERATIVE NEOPLASMS (MPN) AND SYSTEMIC MASTOCYTOSIS (SM). THE FIELD OF EPIGENETIC REGULATION OF NORMAL AND MALIGNANT HEMATOPOIESIS IS RAPIDLY GROWING. IN RECENT YEARS, HETEROZYGOUS SOMATIC MUTATIONS IN GENES ENCODING EPIGENETIC REGULATORS HAVE BEEN FOUND IN ALL SUBTYPES OF MYELOID MALIGNANCIES, SUPPORTING THE RATIONALE FOR TREATMENT WITH EPIGENETIC MODIFIERS. HISTONE DEACETYLASE INHIBITORS (HDACI) ARE EPIGENETIC MODIFIERS THAT, IN VITRO, HAVE BEEN SHOWN TO INDUCE GROWTH ARREST, APOPTOTIC OR AUTOPHAGIC CELL DEATH, AND TERMINAL DIFFERENTIATION OF MYELOID TUMOR CELLS. THESE EFFECTS WERE OBSERVED BOTH AT THE BULK TUMOR LEVEL AND IN THE MOST IMMATURE CD34(+)38(-) CELL COMPARTMENTS CONTAINING THE LEUKEMIC STEM CELLS. THUS, THERE IS A STRONG RATIONALE SUPPORTING HDACI THERAPY IN MYELOID MALIGNANCIES. HOWEVER, DESPITE INITIAL PROMISING RESULTS IN PHASE I TRIALS, HDACI IN MONOTHERAPY AS WELL AS IN COMBINATION WITH OTHER DRUGS, HAVE FAILED TO IMPROVE RESPONSES OR SURVIVAL. THIS REVIEW PROVIDES AN OVERVIEW OF THE RATIONALE FOR HDACI IN MYELOID MALIGNANCIES, CLINICAL RESULTS AND SPECULATIONS ON WHY CLINICAL TRIALS HAVE THUS FAR NOT MET THE EXPECTATIONS, AND HOW THIS MAY BE IMPROVED IN THE FUTURE. 2018 5 4265 37 MICRO-RNA-125A MEDIATES THE EFFECTS OF HYPOMETHYLATING AGENTS IN CHRONIC MYELOMONOCYTIC LEUKEMIA. BACKGROUND: CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML) IS AN AGGRESSIVE HEMATOPOIETIC MALIGNANCY THAT ARISES FROM HEMATOPOIETIC STEM AND PROGENITOR CELLS (HSPCS). PATIENTS WITH CMML ARE FREQUENTLY TREATED WITH EPIGENETIC THERAPEUTIC APPROACHES, IN PARTICULAR THE HYPOMETHYLATING AGENTS (HMAS), AZACITIDINE (AZA) AND DECITABINE (DEC). ALTHOUGH HMAS ARE BELIEVED TO MEDIATE THEIR EFFICACY VIA RE-EXPRESSION OF HYPERMETHYLATED TUMOR SUPPRESSORS, KNOWLEDGE ABOUT RELEVANT HMA TARGETS IS SCARCE. AS SILENCING OF TUMOR-SUPPRESSIVE MICRO-RNAS (MIRS) BY PROMOTER HYPERMETHYLATION IS A CRUCIAL STEP IN MALIGNANT TRANSFORMATION, WE ASKED FOR A ROLE OF MIRS IN HMA EFFICACY IN CMML. RESULTS: INITIALLY, WE PERFORMED GENOME-WIDE MIR-EXPRESSION PROFILING IN A KRAS(G12D)-INDUCED CMML MOUSE MODEL. SELECTED CANDIDATES WITH PROMINENTLY DECREASED EXPRESSION WERE VALIDATED BY QPCR IN CMML MICE AND HUMAN CMML PATIENTS. THESE EXPERIMENTS REVEALED THE CONSISTENT DECREASE IN MIR-125A, A MIR WITH PREVIOUSLY DESCRIBED TUMOR-SUPPRESSIVE FUNCTION IN MYELOID NEOPLASIAS. FURTHERMORE, WE SHOW THAT MIR-125A DOWNREGULATION IS CAUSED BY HYPERMETHYLATION OF ITS UPSTREAM REGION AND CAN BE REVERSED BY HMA TREATMENT. BY EMPLOYING BOTH LENTIVIRAL AND CRISPR/CAS9-BASED MIR-125A MODIFICATION, WE DEMONSTRATE THAT HMA-INDUCED MIR-125A UPREGULATION INDEED CONTRIBUTES TO MEDIATING THE ANTI-LEUKEMIC EFFECTS OF THESE DRUGS. THESE DATA WERE VALIDATED IN A CLINICAL CONTEXT, AS MIR-125A EXPRESSION INCREASED AFTER HMA TREATMENT IN CMML PATIENTS, A PHENOMENON THAT WAS PARTICULARLY PRONOUNCED IN CASES SHOWING CLINICAL RESPONSE TO THESE DRUGS. CONCLUSIONS: TAKEN TOGETHER, WE REPORT DECREASED EXPRESSION OF MIR-125A IN CMML AND DELINEATE ITS RELEVANCE AS MEDIATOR OF HMA EFFICACY WITHIN THIS NEOPLASIA. 2021 6 4547 28 MUTATION ALLELE BURDEN REMAINS UNCHANGED IN CHRONIC MYELOMONOCYTIC LEUKAEMIA RESPONDING TO HYPOMETHYLATING AGENTS. THE CYTIDINE ANALOGUES AZACYTIDINE AND 5-AZA-2'-DEOXYCYTIDINE (DECITABINE) ARE COMMONLY USED TO TREAT MYELODYSPLASTIC SYNDROMES, WITH OR WITHOUT A MYELOPROLIFERATIVE COMPONENT. IT REMAINS UNCLEAR WHETHER THE RESPONSE TO THESE HYPOMETHYLATING AGENTS RESULTS FROM A CYTOTOXIC OR AN EPIGENETIC EFFECT. IN THIS STUDY, WE ADDRESS THIS QUESTION IN CHRONIC MYELOMONOCYTIC LEUKAEMIA. WE DESCRIBE A COMPREHENSIVE ANALYSIS OF THE MUTATIONAL LANDSCAPE OF THESE TUMOURS, COMBINING WHOLE-EXOME AND WHOLE-GENOME SEQUENCING. WE IDENTIFY AN AVERAGE OF 14+/-5 SOMATIC MUTATIONS IN CODING SEQUENCES OF SORTED MONOCYTE DNA AND THE SIGNATURES OF THREE MUTATIONAL PROCESSES. SERIAL SEQUENCING DEMONSTRATES THAT THE RESPONSE TO HYPOMETHYLATING AGENTS IS ASSOCIATED WITH CHANGES IN DNA METHYLATION AND GENE EXPRESSION, WITHOUT ANY DECREASE IN THE MUTATION ALLELE BURDEN, NOR PREVENTION OF NEW GENETIC ALTERATION OCCURENCE. OUR FINDINGS INDICATE THAT CYTOSINE ANALOGUES RESTORE A BALANCED HAEMATOPOIESIS WITHOUT DECREASING THE SIZE OF THE MUTATED CLONE, ARGUING FOR A PREDOMINANTLY EPIGENETIC EFFECT. 2016 7 151 33 ABERRANT METHYLATION AND IMPAIRED EXPRESSION OF THE P15(INK4B) CELL CYCLE REGULATORY GENE IN CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML). THE IMPORTANT CELL CYCLE REGULATORY GENE P15(INK4B) HAS BEEN SHOWN TO BE INACTIVATED IN ACUTE MYELOID LEUKEMIA AND MYELODYSPLASTIC SYNDROME. LITTLE IS KNOWN ABOUT THE EXPRESSION AND EPIGENETIC MODIFICATION OF THIS GENE IN CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML) THAT BELONGS TO THE MYELODYSPLASTIC/MYELOPROLIFERATIVE DISORDERS (MDS/MPD) WITH A HIGH PROPORTION OF BLASTIC TRANSFORMATION. ANALYSIS OF BONE MARROW TREPHINES IN A SERIES OF 33 CMML CASES SHOWED AN ABERRANT P15(INK4B) GENE METHYLATION IN UP TO 58% OF CASES. METHYLATION WAS ANALYZED EMPLOYING DIFFERENT METHYLATION-SPECIFIC PCR AND GENOMIC SEQUENCING PROTOCOLS. IT TURNED OUT TO BE SPREAD OVER A BROAD AREA OF THE 5' REGION AND EXHIBITED SUBSTANTIAL HETEROGENEITY BETWEEN CASES AND EVEN IN INDIVIDUAL PATIENTS. THE DEGREE OF ABERRANT METHYLATION WAS CORRELATED WITH A REDUCED MRNA AS WELL AS REDUCED PROTEIN EXPRESSION, AND WAS ASSOCIATED WITH A HIGHER EXPRESSION OF DNA METHYLTRANSFERASE DNMT 3A. WE CONCLUDE THAT ABERRANT GENE METHYLATION IS A FREQUENT EVENT IN CMML THAT MIGHT CONTRIBUTE TO THE PATHOGENESIS OF THIS MDS/MPD. 2003 8 535 40 ASXL1 MUTATION CORRECTION BY CRISPR/CAS9 RESTORES GENE FUNCTION IN LEUKEMIA CELLS AND INCREASES SURVIVAL IN MOUSE XENOGRAFTS. RECURRENT SOMATIC MUTATIONS OF THE EPIGENETIC MODIFIER AND TUMOR SUPPRESSOR ASXL1 ARE COMMON IN MYELOID MALIGNANCIES, INCLUDING CHRONIC MYELOID LEUKEMIA (CML), AND ARE ASSOCIATED WITH POOR CLINICAL OUTCOME. CRISPR/CAS9 HAS RECENTLY EMERGED AS A POWERFUL AND VERSATILE GENOME EDITING TOOL FOR GENOME ENGINEERING IN VARIOUS SPECIES. WE HAVE USED THE CRISPR/CAS9 SYSTEM TO CORRECT THE ASXL1 HOMOZYGOUS NONSENSE MUTATION PRESENT IN THE CML CELL LINE KBM5, WHICH LACKS ASXL1 PROTEIN EXPRESSION. CRISPR/CAS9-MEDIATED ASXL1 HOMOZYGOUS CORRECTION RESULTED IN PROTEIN RE-EXPRESSION WITH RESTORED NORMAL FUNCTION, INCLUDING DOWN-REGULATION OF POLYCOMB REPRESSIVE COMPLEX 2 TARGET GENES. SIGNIFICANTLY REDUCED CELL GROWTH AND INCREASED MYELOID DIFFERENTIATION WERE OBSERVED IN ASXL1 MUTATION-CORRECTED CELLS, PROVIDING NEW INSIGHTS INTO THE ROLE OF ASXL1 IN HUMAN MYELOID CELL DIFFERENTIATION. MICE XENOGRAFTED WITH MUTATION-CORRECTED KBM5 CELLS SHOWED SIGNIFICANTLY LONGER SURVIVAL THAN UNCORRECTED XENOGRAFTS. THESE RESULTS SHOW THAT THE SOLE CORRECTION OF A DRIVER MUTATION IN LEUKEMIA CELLS INCREASES SURVIVAL IN VIVO IN MICE. THIS STUDY PROVIDES PROOF-OF-CONCEPT FOR DRIVER GENE MUTATION CORRECTION VIA CRISPR/CAS9 TECHNOLOGY IN HUMAN LEUKEMIA CELLS AND PRESENTS A STRATEGY TO ILLUMINATE THE IMPACT OF ONCOGENIC MUTATIONS ON CELLULAR FUNCTION AND SURVIVAL. 2015 9 2911 36 GENE EXPRESSION PROFILING OF LOSS OF TET2 AND/OR JAK2V617F MUTANT HEMATOPOIETIC STEM CELLS FROM MOUSE MODELS OF MYELOPROLIFERATIVE NEOPLASMS. MYELOPROLIFERATIVE NEOPLASMS (MPNS) ARE CLINICALLY CHARACTERIZED BY THE CHRONIC OVERPRODUCTION OF DIFFERENTIATED PERIPHERAL BLOOD CELLS AND THE GRADUAL EXPANSION OF MALIGNANT INTRAMEDULLARY/EXTRAMEDULLARY HEMATOPOIESIS. IN MPNS MUTATIONS IN JAK2 MPL OR CALR ARE DETECTED MUTUALLY EXCLUSIVE IN MORE THAN 90% OF CASES [1,2]. MUTATIONS IN THEM LEAD TO THE ABNORMAL ACTIVATION OF JAK/STAT SIGNALING AND THE AUTONOMOUS GROWTH OF DIFFERENTIATED CELLS THEREFORE THEY ARE CONSIDERED AS "DRIVER" GENE MUTATIONS. IN ADDITION TO THE ABOVE DRIVER GENE MUTATIONS MUTATIONS IN EPIGENETIC REGULATORS SUCH AS TET2 DNMT3A ASXL1 EZH2 OR IDH1/2 ARE DETECTED IN ABOUT 5%-30% OF CASES RESPECTIVELY [3]. MUTATIONS IN TET2 DNMT3A EZH2 OR IDH1/2 COMMONLY CONFER THE INCREASED SELF-RENEWAL CAPACITY ON NORMAL HEMATOPOIETIC STEM CELLS (HSCS) BUT THEY DO NOT LEAD TO THE AUTONOMOUS GROWTH OF DIFFERENTIATED CELLS AND ONLY EXHIBIT SUBTLE CLINICAL PHENOTYPES [4,6-8,5]. IT WAS UNCLEAR HOW MUTATIONS IN SUCH EPIGENETIC REGULATORS INFLUENCED ABNORMAL HSCS WITH DRIVER GENE MUTATIONS HOW THEY INFLUENCED THE DISEASE PHENOTYPE OR WHETHER A SINGLE DRIVER GENE MUTATION WAS SUFFICIENT FOR THE INITIATION OF HUMAN MPNS. THEREFORE WE FOCUSED ON JAK2V617F AND LOSS OF TET2-THE FORMER AS A REPRESENTATIVE OF DRIVER GENE MUTATIONS AND THE LATTER AS A REPRESENTATIVE OF MUTATIONS IN EPIGENETIC REGULATORS-AND EXAMINED THE INFLUENCE OF SINGLE OR DOUBLE MUTATIONS ON HSCS (LINEAGE(-)SCA-1(+)C-KIT(+) CELLS (LSKS)) BY FUNCTIONAL ANALYSES AND MICROARRAY WHOLE-GENOME EXPRESSION ANALYSES [9]. GENE EXPRESSION PROFILING SHOWED THAT THE HSC FINGERPRINT GENES [10] WAS STATISTICALLY EQUALLY ENRICHED IN TET2-KNOCKDOWN-LSKS BUT NEGATIVELY ENRICHED IN JAK2V617F-LSKS COMPARED TO THAT IN WILD-TYPE-LSKS. DOUBLE-MUTANT-LSKS SHOWED THE SAME TENDENCY AS JAK2V617F-LSKS IN TERMS OF THEIR HSC FINGERPRINT GENES BUT THE EXPRESSION OF INDIVIDUAL GENES DIFFERED BETWEEN THE TWO GROUPS. AMONG 245 HSC FINGERPRINT GENES 100 WERE MORE HIGHLY EXPRESSED IN DOUBLE-MUTANT-LSKS THAN IN JAK2V617F-LSKS. THESE ALTERED GENE EXPRESSIONS MIGHT PARTLY EXPLAIN THE MECHANISMS OF INITIATION AND PROGRESSION OF MPNS WHICH WAS OBSERVED IN THE FUNCTIONAL ANALYSES [9]. HERE WE DESCRIBE GENE EXPRESSION PROFILES DEPOSITED AT THE GENE EXPRESSION OMNIBUS (GEO) UNDER THE ACCESSION NUMBER GSE62302 INCLUDING EXPERIMENTAL METHODS AND QUALITY CONTROL ANALYSES. 2015 10 4551 33 MUTATIONAL HIERARCHIES IN MYELODYSPLASTIC SYNDROMES DYNAMICALLY ADAPT AND EVOLVE UPON THERAPY RESPONSE AND FAILURE. CLONAL EVOLUTION IS BELIEVED TO BE A MAIN DRIVER FOR PROGRESSION OF VARIOUS TYPES OF CANCER AND IMPLICATED IN FACILITATING RESISTANCE TO DRUGS. HOWEVER, THE HIERARCHICAL ORGANIZATION OF MALIGNANT CLONES IN THE HEMATOPOIESIS OF MYELODYSPLASTIC SYNDROMES (MDS) AND ITS IMPACT ON RESPONSE TO DRUG THERAPY REMAIN POORLY UNDERSTOOD. USING HIGH-THROUGHPUT SEQUENCING OF PATIENT AND XENOGRAFTED CELLS, WE EVALUATED THE INTRATUMORAL HETEROGENEITY (N= 54) AND RECONSTRUCTED MUTATIONAL TRAJECTORIES (N = 39) IN PATIENTS SUFFERING FROM MDS (N = 52) AND CHRONIC MYELOMONOCYTIC LEUKEMIA-1 (N = 2). WE IDENTIFIED LINEAR AND ALSO BRANCHING EVOLUTION PATHS AND CONFIRMED ON A PATIENT-SPECIFIC LEVEL THAT SOMATIC MUTATIONS IN EPIGENETIC REGULATORS AND RNA SPLICING GENES FREQUENTLY CONSTITUTE ISOLATED DISEASE-INITIATING EVENTS. USING HIGH-THROUGHPUT EXOME- AND/OR DEEP-SEQUENCING, WE ANALYZED 103 CHRONOLOGICALLY ACQUIRED SAMPLES FROM 22 PATIENTS COVERING A CUMULATIVE OBSERVATION TIME OF 75 YEARS MDS DISEASE PROGRESSION. OUR DATA REVEALED HIGHLY DYNAMIC SHAPING OF COMPLEX OLIGOCLONAL ARCHITECTURES, SPECIFICALLY UPON TREATMENT WITH LENALIDOMIDE AND OTHER DRUGS. DESPITE INITIAL CLINICAL RESPONSE TO TREATMENT, PATIENTS' MARROW PERSISTENTLY REMAINED CLONAL WITH RAPID OUTGROWTH OF FOUNDER-, SUB-, OR EVEN FULLY INDEPENDENT CLONES, INDICATING AN INCREASED DYNAMIC RATE OF CLONAL TURNOVER. THE EMERGENCE AND DISAPPEARANCE OF SPECIFIC CLONES FREQUENTLY CORRELATED WITH CHANGES OF CLINICAL PARAMETERS, HIGHLIGHTING THEIR DISTINCT AND FAR-REACHING FUNCTIONAL PROPERTIES. INTRIGUINGLY, INCREASINGLY COMPLEX MUTATIONAL TRAJECTORIES ARE FREQUENTLY ACCOMPANIED BY CLINICAL PROGRESSION DURING THE COURSE OF DISEASE. THESE DATA SUBSTANTIATE A NEED FOR REGULAR BROAD MOLECULAR MONITORING TO GUIDE CLINICAL TREATMENT DECISIONS IN MDS. 2016 11 3532 37 IMATINIB INDEPENDENT ABERRANT METHYLATION OF NOV/CCN3 IN CHRONIC MYELOGENOUS LEUKEMIA PATIENTS: A MECHANISM UPSTREAM OF BCR-ABL1 FUNCTION? BACKGROUND: THE NOV GENE PRODUCT, CCN3, HAS BEEN REPORTED IN A DIVERSE RANGE OF TUMORS TO SERVE AS A NEGATIVE GROWTH REGULATOR, WHILE ACTING AS A TUMOR SUPPRESSOR IN CHRONIC MYELOGENOUS LEUKEMIA (CML). HOWEVER, THE PRECISE MECHANISM OF ITS SILENCING IN CML IS POORLY UNDERSTOOD. IN THE CURRENT STUDY, WE AIMED TO QUERY IF THE GENE REGULATION OF CCN3 IS MEDIATED BY THE PROMOTER METHYLATION IN THE PATIENTS WITH CML. IN ADDITION, TO CLARIFY WHETHER THE EPIGENETIC SILENCING IS AFFECTED BY BCR-ABL1 INHIBITION, WE ASSESSED THE METHYLATION STATUS IN THE PATIENTS AT DIFFERENT TIME INTERVALS FOLLOWING THE TYROSINE KINASE INHIBITION USING IMATINIB THERAPY, AS THE FIRST-LINE TREATMENT FOR THIS TYPE OF LEUKEMIA. METHODS: TO ADDRESS THIS ISSUE, WE APPLIED BISULFITE-SEQUENCING TECHNIQUE AS A HIGH-RESOLUTION METHOD TO STUDY THE REGULATORY SEGMENT OF THE CCN3 GENE. THE RESULTS WERE ANALYZED IN NEWLY DIAGNOSED CML PATIENTS AS WELL AS FOLLOWING IMATINIB THERAPY. WE ALSO EVALUATED THE CORRELATION OF CCN3 PROMOTER METHYLATION WITH BCR-ABL1 LEVELS. RESULTS: OUR FINDINGS REVEALED THAT THE METHYLATION OCCURS FREQUENTLY IN THE PROMOTER REGION OF CML PATIENTS SHOWING A SIGNIFICANT INCREASE OF THE METHYLATED PERCENTAGE AT THE CPG SITES COMPARED TO NORMAL INDIVIDUALS. INTERESTINGLY, THIS HYPERMETHYLATION WAS INDICATED TO BE INDEPENDENT OF BCR-ABL1 TITERS IN BOTH GROUPS, WHICH MIGHT SUGGEST A MECHANISM BEYOND THE BCR-ABL1 FUNCTION. CONCLUSION: DESPITE SUGGESTING THAT THE CCN3 HYPERMETHYLATION ACTS AS A MOLECULAR MECHANISM INDEPENDENT OF BCR-ABL1 FUNCTION IN CML PATIENTS, THIS SCENARIO REQUIRES FURTHER VALIDATION BY COMPLEMENTARY EXPERIMENTS. IN THE CASE OF ACTING UPSTREAM OF BCR-ABL1 SIGNALING, THE METHYLATION MARKER CAN PROVIDE EARLY DETECTION AND A NOVEL PLATFORM FOR TARGETED EPIGENETIC MODIFIERS FOR EFFICIENT TREATMENT IN IMATINIB RESISTANT PATIENTS. 2019 12 4681 34 NEW OPTIONS IN THE TREATMENT OF MYELODYSPLASTIC SYNDROME. MYELODYSPLASTIC SYNDROME (MDS) IS A HETEROGENEOUS GROUP OF PROGRESSIVE CHRONIC HEMATOPOIETIC DISORDERS, USUALLY PRESENTING AS REFRACTORY ANEMIA OR CYTOPENIA, WITH AN APPROXIMATELY 25% RISK OF PROGRESSION TOWARD ACUTE MYELOID LEUKAEIMA (AML), AND NO PROVEN CURATIVE TREATMENT. NOVEL BIOLOGICAL TREATMENT STRATEGIES TARGETING BOTH THE MALIGNANT BLOOD CELL AND ITS MICROENVIRONMENT CAN OVERCOME RESISTANCE TO CURRENT THERAPIES, AND REPRESENT A PROMISING TREATMENT PARADIGM FOR IMPROVING PATIENT OUTCOME. MANY OF THESE AGENTS HAVE MULTIPLE BIOLOGIC ACTIVITIES. THE OBJECTIVE OF THIS ARTICLE IS TO PRESENT A COMPARATIVE REVIEW OF CLASSIFICATION SYSTEMS IN MDS AND TO DISCUSS THE EVOLVING TRENDS IN THE TREATMENT OF MDS (IMMUNOSUPPRESIVE THERAPY, IMMUNOMODULATORY DRUGS, ARSENIC TRIOXIDE, PROTEASOME INHIBITORS, EPIGENETIC THERAPY). 2005 13 1070 31 CLONAL ARCHITECTURE OF CHRONIC MYELOMONOCYTIC LEUKEMIAS. GENOMIC STUDIES IN CHRONIC MYELOID MALIGNANCIES, INCLUDING MYELOPROLIFERATIVE NEOPLASMS (MPN), MYELODYSPLASTIC SYNDROMES (MDS), AND MPN/MDS, HAVE IDENTIFIED COMMON MUTATIONS IN GENES ENCODING SIGNALING, EPIGENETIC, TRANSCRIPTION, AND SPLICING FACTORS. IN THE PRESENT STUDY, WE INTERROGATED THE CLONAL ARCHITECTURE BY MUTATION-SPECIFIC DISCRIMINATION ANALYSIS OF SINGLE-CELL-DERIVED COLONIES IN 28 PATIENTS WITH CHRONIC MYELOMONOCYTIC LEUKEMIAS (CMML), THE MOST FREQUENT MPN/MDS. THIS ANALYSIS REVEALS A LINEAR ACQUISITION OF THE STUDIED MUTATIONS WITH LIMITED BRANCHING THROUGH LOSS OF HETEROZYGOSITY. SERIAL ANALYSIS OF UNTREATED AND TREATED SAMPLES DEMONSTRATES A DYNAMIC ARCHITECTURE ON WHICH MOST CURRENT THERAPEUTIC APPROACHES HAVE LIMITED EFFECTS. THE MAIN DISEASE CHARACTERISTICS ARE EARLY CLONAL DOMINANCE, ARISING AT THE CD34(+)/CD38(-) STAGE OF HEMATOPOIESIS, AND GRANULOMONOCYTIC DIFFERENTIATION SKEWING OF MULTIPOTENT AND COMMON MYELOID PROGENITORS. COMPARISON OF CLONAL EXPANSIONS OF TET2 MUTATIONS IN MDS, MPN, AND CMML, TOGETHER WITH FUNCTIONAL INVALIDATION OF TET2 IN SORTED PROGENITORS, SUGGESTS A CAUSATIVE LINK BETWEEN EARLY CLONAL DOMINANCE AND SKEWED GRANULOMONOCYTIC DIFFERENTIATION. ALTOGETHER, EARLY CLONAL DOMINANCE MAY DISTINGUISH CMML FROM OTHER CHRONIC MYELOID NEOPLASMS WITH SIMILAR GENE MUTATIONS. 2013 14 6680 35 USING PERIPHERAL BLOOD CIRCULATING DNAS TO DETECT CPG GLOBAL METHYLATION STATUS AND GENETIC MUTATIONS IN PATIENTS WITH MYELODYSPLASTIC SYNDROME. MYELODYSPLASTIC SYNDROME (MDS) IS A HEMATOPOIETIC STEM CELL DISORDER. SEVERAL GENETIC/EPIGENETIC ABNORMALITIES ARE DEEPLY ASSOCIATED WITH THE PATHOGENESIS OF MDS. ALTHOUGH BONE MARROW (BM) ASPIRATION IS A COMMON STRATEGY TO OBTAIN MDS CELLS FOR EVALUATING THEIR GENETIC/EPIGENETIC ABNORMALITIES, BM ASPIRATION IS DIFFICULT TO PERFORM REPEATEDLY TO OBTAIN SERIAL SAMPLES BECAUSE OF PAIN AND SAFETY CONCERNS. HERE, WE REPORT THAT CIRCULATING CELL-FREE DNAS FROM PLASMA AND SERUM OF PATIENTS WITH MDS CAN BE USED TO DETECT GENETIC/EPIGENETIC ABNORMALITIES. THE PLASMA DNA CONCENTRATION WAS FOUND TO BE RELATIVELY HIGH IN PATIENTS WITH HIGHER BLAST CELL COUNTS IN BM, AND ACCUMULATION OF DNA FRAGMENTS FROM MONO-/DI-NUCLEOSOMES WAS CONFIRMED. USING SERIAL PERIPHERAL BLOOD (PB) SAMPLES FROM PATIENTS TREATED WITH HYPOMETHYLATING AGENTS, GLOBAL METHYLATION ANALYSIS USING BISULFITE PYROSEQUENCING WAS PERFORMED AT THE SPECIFIC CPG SITES OF THE LINE-1 PROMOTER. THE RESULTS CONFIRMED A DECREASE OF THE METHYLATION PERCENTAGE AFTER TREATMENT WITH AZACITIDINE (DAYS 3-9) USING DNAS FROM PLASMA, SERUM, AND PB MONO-NUCLEAR CELLS (PBMNC). PLASMA DNA TENDS TO SHOW MORE RAPID CHANGE AT DAYS 3 AND 6 COMPARED WITH SERUM DNA AND PBMNC. FURTHERMORE, THE TET2 GENE MUTATION IN DNAS FROM PLASMA, SERUM, AND BM CELLS WAS QUANTITATED BY PYROSEQUENCING ANALYSIS. THE EXISTENCE RATIO OF MUTATED GENES IN PLASMA AND SERUM DNA SHOWED ALMOST EQUIVALENT LEVEL WITH THAT IN THE CD34+/38- STEM CELL POPULATION IN BM. THESE DATA SUGGEST THAT GENETIC/EPIGENETIC ANALYSES USING PB CIRCULATING DNA CAN BE A SAFER AND PAINLESS ALTERNATIVE TO USING BM CELLS. 2012 15 4549 32 MUTATION ANALYSIS OF THERAPY-RELATED MYELOID NEOPLASMS. WE ANALYZED THE GENETIC MUTATION STATUS OF 13 PATIENTS WITH THERAPY-RELATED MYELOID NEOPLASMS (T-MN). CONSISTENT WITH PREVIOUS REPORTS, T-MN CELLS PREFERENTIALLY ACQUIRED MUTATIONS IN TP53 AND EPIGENETIC MODIFYING GENES, INSTEAD OF MUTATIONS IN TYROSINE KINASE AND SPLICEOSOME GENES. FURTHERMORE, WE COMPARED THE MUTATION STATUS OF THREE T-MN CELLS WITH EACH OF THE INITIAL LYMPHOID MALIGNANT CELLS, AND IDENTIFIED COMMON MUTATIONS AMONG T-MN AND THE INITIAL MALIGNANT CELLS IN TWO PATIENTS. IN A PATIENT WHO DEVELOPED CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML) AFTER FOLLICULAR LYMPHOMA (FL), TET2 MUTATION WAS IDENTIFIED IN BOTH CMML AND FL CELLS. NOTABLY, THE TET2 MUTATION WAS ALSO IDENTIFIED IN PERIPHERAL BLOOD CELLS IN THE DISEASE-FREE PERIOD WITH THE SAME ALLELIC FREQUENCY AS CMML AND FL CELLS, BUT NOT IN A GERM-LINE CONTROL, INDICATING THAT THE TET2 MUTATION OCCURRED SOMATICALLY IN THE INITIATING CLONE FOR BOTH MALIGNANT CELLS. ON THE OTHER HAND, A GERM-LINE MYB MUTATION WAS IDENTIFIED IN A PATIENT WHO DEVELOPED MYELODYSPLASTIC SYNDROMES (MDS) AFTER FL. THESE RESULTS SUGGEST THAT GERM-LINE DEPOSITION AND CLONAL HEMATOPOIESIS ARE CLOSELY ASSOCIATED WITH T-MN SUSCEPTIBILITY; HOWEVER, FURTHER ANALYSIS IS NECESSARY TO CLARIFY THE MECHANISM REQUIRED TO PROVIDE THE INITIATING CLONE WITH LINEAGE COMMITMENT AND CLONAL EXPANSION. 2018 16 4530 34 MULTILAYER INTRACLONAL HETEROGENEITY IN CHRONIC MYELOMONOCYTIC LEUKEMIA. THE FUNCTIONAL DIVERSITY OF CELLS THAT COMPOSE MYELOID MALIGNANCIES, I.E., THE RESPECTIVE ROLES OF GENETIC AND EPIGENETIC HETEROGENEITY IN THIS DIVERSITY, REMAINS POORLY UNDERSTOOD. THIS QUESTION IS ADDRESSED IN CHRONIC MYELOMONOCYTIC LEUKEMIA, A MYELOID NEOPLASM IN WHICH CLINICAL DIVERSITY CONTRASTS WITH LIMITED GENETIC HETEROGENEITY. TO GENERATE INDUCED PLURIPOTENT STEM CELL CLONES, WE REPROGRAMMED CD34(+) CELLS COLLECTED FROM A PATIENT WITH A CHRONIC MYELOMONOCYTIC LEUKEMIA IN WHICH WHOLE EXOME SEQUENCING OF PERIPHERAL BLOOD MONOCYTE DNA HAD IDENTIFIED 12 GENE MUTATIONS, INCLUDING A MUTATION IN KDM6A AND TWO HETEROZYGOUS MUTATIONS IN TET2 IN THE FOUNDING CLONE AND A SECONDARY KRAS(G12D) MUTATION. CD34(+) CELLS FROM AN AGE-MATCHED HEALTHY DONOR WERE ALSO REPROGRAMMED. WE CAPTURED A PART OF THE GENETIC HETEROGENEITY OBSERVED IN THE PATIENT, I.E. WE ANALYZED FIVE CLONES WITH TWO GENETIC BACKGROUNDS, WITHOUT AND WITH THE KRAS(G12D) MUTATION. HEMATOPOIETIC DIFFERENTIATION OF THESE CLONES RECAPITULATED THE MAIN FEATURES OF THE PATIENT'S DISEASE, INCLUDING OVERPRODUCTION OF GRANULOMONOCYTES AND DYSMEGAKARYOPOIESIS. THESE ANALYSES ALSO DISCLOSED SIGNIFICANT DISCREPANCIES IN THE BEHAVIOR OF HEMATOPOIETIC CELLS DERIVED FROM INDUCED PLURIPOTENT STEM CELL CLONES WITH SIMILAR GENETIC BACKGROUND, CORRELATING WITH LIMITED EPIGENETIC CHANGES. THESE ANALYSES SUGGEST THAT, BEYOND THE CODING MUTATIONS, SEVERAL LEVELS OF INTRACLONAL HETEROGENEITY MAY PARTICIPATE IN THE YET UNEXPLAINED CLINICAL HETEROGENEITY OF THE DISEASE. 2020 17 1046 40 CLINICAL DEVELOPMENT OF DECITABINE AS A PROTOTYPE FOR AN EPIGENETIC DRUG PROGRAM. THIS REVIEW HIGHLIGHTS DECITABINE AS A PROTOTYPE EPIGENETIC MODIFYING DRUG TO SHOW HOW THE CLINICAL DEVELOPMENT OF EPIGENETIC AGENTS DIFFERS FROM THAT OF TRADITIONAL CYTOTOXIC CHEMOTHERAPIES. DECITABINE, A CYTOSINE ANALOGUE, IS CYTOTOXIC AT HIGH DOSES BUT HAS SELECTIVE DNA DEMETHYLATING ACTIVITY AT LOW DOSES. THE FOCUS OF CURRENT DECITABINE INVESTIGATIONS IS TWOFOLD: TO ELUCIDATE ALL OF THE MECHANISMS OF ACTION AND TO DETERMINE THE OPTIMAL DOSE, SCHEDULE, AND CONCOMITANT THERAPIES. NEW PHASE I TRIALS HAVE IDENTIFIED A "BIOLOGICALLY EFFECTIVE DOSE," WHICH IS 1 TO 2 LOGS LOWER THAN THE CYTOTOXIC DOSE. A CLINICAL DEVELOPMENT PROGRAM WITH LOW-DOSE DECITABINE IN MALIGNANT DISEASES IS FOCUSED ON MYELODYSPLASTIC SYNDROME (MDS), ACUTE MYELOGENOUS LEUKEMIA (AML), AND CHRONIC MYELOGENOUS LEUKEMIA (CML). A PHASE III TRIAL IN MDS SHOWED OBJECTIVE RESPONSES (COMPLETE [CR] PLUS PARTIAL [PR] REMISSION) AND LONGER MEDIAN TIME TO PROGRESSION TO AML OR DEATH WITH DECITABINE THAN WITH SUPPORTIVE CARE ALONE. THE OPTIMAL USE OF DECITABINE MAY BE IN COMBINATION WITH OTHER AGENTS THAT PROMOTE GENE EXPRESSION, NAMELY, HISTONE DEACETYLASE (HDAC) INHIBITORS. OPTIMIZED DECITABINE DOSES AND COMBINATIONS WITH OTHER EPIGENETIC THERAPIES THAT CAN BE USED AT MINIMALLY TOXIC DOSES PROVIDE POTENTIALLY SAFER THERAPEUTIC OPTIONS AND INTRODUCE NOVEL COMBINATION THERAPIES. 2005 18 5983 39 TET2 RESTRAINS INFLAMMATORY GENE EXPRESSION IN MACROPHAGES. TET METHYLCYTOSINE DIOXYGENASE 2 (TET2) IS ONE OF THE EARLIEST AND MOST FREQUENTLY MUTATED GENES IN CLONAL HEMATOPOIESIS OF INDETERMINATE POTENTIAL (CHIP) AND MYELOID CANCERS, INCLUDING MYELODYSPLASTIC SYNDROMES (MDS) AND CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML). TET2 CATALYZES THE OXIDATION OF 5-METHYLCYTOSINE TO 5-HYDROXYMETHYLCYTOSINE, LEADING TO DNA DEMETHYLATION, AND ALSO AFFECTS TRANSCRIPTION BY RECRUITING HISTONE MODIFIERS. INACTIVATING TET2 MUTATIONS CAUSE EPIGENETIC DYSREGULATION, CLONAL HEMATOPOIETIC STEM CELL (HSC) DOMINANCE, AND MONOCYTIC LINEAGE SKEWING. HERE, WE FOUND THAT TET2 WAS THE MOST HIGHLY EXPRESSED TET ENZYME IN MURINE MACROPHAGE (MPHI) DIFFERENTIATION. TET2 TRANSCRIPTION WAS FURTHER INDUCED BY LIPOPOLYSACCHARIDE (LPS), BUT NOT INTERLEUKIN (IL)-4, STIMULATION, POTENTIALLY IN A NUCLEAR FACTOR KAPPABETA-DEPENDENT MANNER. TET2 LOSS DID NOT AFFECT EARLY LPS GENE RESPONSES IN VITRO, BUT INCREASED IL-1B, IL-6, AND ARGINASE 1 (ARG1) MRNA EXPRESSION AT LATER STAGES OF STIMULATION IN BONE-MARROW-DERIVED MPHIS (BMMPHIS). TET2-DEFICIENT PERITONEAL MPHIS, HOWEVER, DEMONSTRATED PROFOUND, CONSTITUTIVE EXPRESSION OF LPS-INDUCED GENES ASSOCIATED WITH AN INFLAMMATORY STATE IN VIVO. IN CONTRAST, TET2 DEFICIENCY DID NOT AFFECT ALTERNATIVE MPHI GENE EXPRESSION SIGNIFICANTLY IN RESPONSE TO IL-4. THESE RESULTS SUGGESTED IMPAIRED RESOLUTION OF INFLAMMATION IN THE ABSENCE OF TET2 BOTH IN VITRO AND IN VIVO. FOR THE FIRST TIME, WE ALSO DETECTED TET2 MUTATIONS IN BMMPHIS FROM MDS AND CMML PATIENTS AND ASSAYED THEIR EFFECTS ON LPS RESPONSES, INCLUDING THEIR POTENTIAL INFLUENCE ON HUMAN IL-6 EXPRESSION. OUR RESULTS SHOW THAT TET2 RESTRAINS INFLAMMATION IN MURINE MPHIS AND MICE, RAISING THE POSSIBILITY THAT LOSS OF TET2 FUNCTION IN MPHIS MAY ALTER THE IMMUNE ENVIRONMENT IN THE LARGE ELDERLY POPULATION WITH TET2-MUTANT CHIP AND IN TET2-MUTANT MYELOID CANCER PATIENTS. 2017 19 4876 37 OVEREXPRESSION OF ARGINASE 1 IS LINKED TO DNMT3A AND TET2 MUTATIONS IN LOWER-GRADE MYELODYSPLASTIC SYNDROMES AND CHRONIC MYELOMONOCYTIC LEUKEMIA. IMMUNE DYSREGULATION IS A COMMON FEATURE OF MYELODYSPLASTIC SYNDROMES (MDS) AND CHRONIC MYELOMONOCYTIC LEUKEMIA (CMML), PARTICULARLY IN EARLY STAGES. HOWEVER, THE GENETIC BASIS REMAINS POORLY UNDERSTOOD. WE RECENTLY REPORTED THAT MACROPHAGES FROM MICE DEFICIENT IN TET METHYLCYTOSINE DIOXYGENASE 2 (TET2), A MODEL OF MDS/CMML, ARE HYPERINFLAMMATORY AND HAVE INCREASED EXPRESSION OF ARGINASE 1 (ARG1). IN MACROPHAGES AND MYELOID DERIVED SUPPRESSOR CELLS (MDSCS) EXPRESSION OF ARG1 CONTRIBUTES TO T-CELL SUPPRESSION AND IMMUNE EVASION BY L-ARGININE DEPLETION, IN THE SETTING OF CHRONIC INFLAMMATION AND CANCER. SINCE HUMAN MDS AND CMML ARE DRIVEN BY TET2 MUTATIONS AND ASSOCIATED WITH CHRONIC INFLAMMATION, WE HYPOTHESIZED THAT ARGINASE ENZYMATIC ACTIVITY AND ARG1 EXPRESSION WOULD BE INCREASED IN HUMAN MDS/CMML BONE MARROW. ELEVATED ARGINASE ACTIVITY WAS OBSERVED IN BONE MARROW MONONUCLEAR CELLS OF MDS AND CMML PATIENTS WITH LOWER-GRADE FEATURES. IMMUNOHISTOCHEMICAL STUDIES CONFIRMED THAT MYELOMONOCYTIC CELLS OVEREXPRESS ARG1. ADDITIONALLY, MUTATIONS IN THE EPIGENETIC REGULATORS TET2 AND DNMT3A CORRESPONDED TO HIGH ARG1 EXPRESSION AND ACTIVITY. THESE FINDINGS SUGGEST ARG1 IS A BIOMARKER OF IMMUNE DYSREGULATION IN EARLY MDS AND CMML. RECENT MURINE FINDINGS HAVE IMPLICATED TET2 AND DNMT3A IN REGULATION OF INNATE IMMUNITY. OUR STUDY SUGGESTS SIMILAR CHANGES MAY BE DRIVEN BY HUMAN TET2 AND DNMT3A MUTATIONS. 2018 20 825 34 CHARACTERIZATION OF FUNCTIONAL TRANSPOSABLE ELEMENT ENHANCERS IN ACUTE MYELOID LEUKEMIA. TRANSPOSABLE ELEMENTS (TES) HAVE BEEN SHOWN TO HAVE IMPORTANT GENE REGULATORY FUNCTIONS AND THEIR ALTERATION COULD LEAD TO DISEASE PHENOTYPES. ACUTE MYELOID LEUKEMIA (AML) DEVELOPS AS A CONSEQUENCE OF A SERIES OF GENETIC CHANGES IN HEMATOPOIETIC PRECURSOR CELLS, INCLUDING MUTATIONS IN EPIGENETIC FACTORS. HERE, WE SET OUT TO STUDY THE GENE REGULATORY ROLE OF TES IN AML. WE FIRST EXPLORED THE EPIGENETIC LANDSCAPE OF TES IN AML PATIENTS USING ATAC-SEQ DATA. WE SHOW THAT A LARGE NUMBER OF TES IN GENERAL, AND MORE SPECIFICALLY MAMMALIAN-WIDE INTERSPERSED REPEATS (MIRS), ARE MORE ENRICHED IN AML CELLS THAN IN NORMAL BLOOD CELLS. WE OBTAINED A SIMILAR FINDING WHEN ANALYZING HISTONE MODIFICATION DATA IN AML PATIENTS. GENE ONTOLOGY ENRICHMENT ANALYSIS SHOWED THAT GENES NEAR MIRS IN OPEN CHROMATIN REGIONS ARE INVOLVED IN LEUKEMOGENESIS. TO FUNCTIONALLY VALIDATE THEIR REGULATORY ROLE, WE SELECTED 19 MIR REGIONS IN AML CELLS, AND TESTED THEM FOR ENHANCER ACTIVITY IN AN AML CELL LINE (KASUMI-1) AND A CHRONIC MYELOID LEUKEMIA (CML) CELL LINE (K562); THE RESULTS REVEALED SEVERAL MIRS TO BE FUNCTIONAL ENHANCERS. TAKEN TOGETHER, OUR RESULTS SUGGEST THAT TES ARE POTENTIALLY INVOLVED IN MYELOID LEUKEMOGENESIS AND HIGHLIGHT THESE SEQUENCES AS POTENTIAL CANDIDATES HARBORING AML-ASSOCIATED VARIATION. 2020