1 3396 115 HOST SHP1 PHOSPHATASE ANTAGONIZES HELICOBACTER PYLORI CAGA AND CAN BE DOWNREGULATED BY EPSTEIN-BARR VIRUS. MOST IF NOT ALL GASTRIC CANCERS ARE ASSOCIATED WITH CHRONIC INFECTION OF THE STOMACH MUCOSA WITH HELICOBACTER PYLORI CAGA-POSITIVE STRAINS(1-4). APPROXIMATELY 10% OF GASTRIC CANCERS ALSO HARBOUR EPSTEIN-BARR VIRUS (EBV) IN THE CANCER CELLS(5,6). FOLLOWING DELIVERY INTO GASTRIC EPITHELIAL CELLS VIA TYPE IV SECRETION(7,8), THE CAGA-ENCODED CAGA PROTEIN UNDERGOES TYROSINE PHOSPHORYLATION ON THE GLU-PRO-ILE-TYR-ALA (EPIYA) MOTIFS INITIALLY BY SRC FAMILY KINASES (SFKS) AND THEN BY C-ABL(9,10). TYROSINE-PHOSPHORYLATED CAGA BINDS TO THE PRO-ONCOGENIC PROTEIN TYROSINE PHOSPHATASE SHP2 AND THEREBY DEREGULATES THE PHOSPHATASE ACTIVITY(11,12), WHICH HAS BEEN CONSIDERED TO PLAY AN IMPORTANT ROLE IN GASTRIC CARCINOGENESIS(13). HERE WE SHOW THAT THE SHP2 HOMOLOGUE SHP1 INTERACTS WITH CAGA INDEPENDENTLY OF THE EPIYA MOTIF. THE INTERACTION POTENTIATES THE PHOSPHATASE ACTIVITY OF SHP1 THAT DAMPENS THE ONCOGENIC ACTION OF CAGA BY DEPHOSPHORYLATING THE CAGA EPIYA MOTIFS. IN VITRO INFECTION OF GASTRIC EPITHELIAL CELLS WITH EBV INDUCES SHP1 PROMOTER HYPERMETHYLATION, WHICH STRENGTHENS PHOSPHORYLATION-DEPENDENT CAGA ACTION VIA EPIGENETIC DOWNREGULATION OF SHP1 EXPRESSION. CLINICAL SPECIMENS OF EBV-POSITIVE GASTRIC CANCERS ALSO EXHIBIT SHP1 HYPERMETHYLATION WITH REDUCED SHP1 EXPRESSION. THE RESULTS REVEAL THAT SHP1 IS THE LONG-SOUGHT PHOSPHATASE THAT CAN ANTAGONIZE CAGA. AUGMENTED H. PYLORI CAGA ACTIVITY, VIA SHP1 INHIBITION, MIGHT ALSO CONTRIBUTE TO THE DEVELOPMENT OF EBV-POSITIVE GASTRIC CANCER. 2016 2 4176 27 MELATONIN RELIEVES NEUROPATHIC ALLODYNIA THROUGH SPINAL MT2-ENHANCED PP2AC AND DOWNSTREAM HDAC4 SHUTTLING-DEPENDENT EPIGENETIC MODIFICATION OF HMGB1 TRANSCRIPTION. MELATONIN (MLT; N-ACETYL-5-METHOXYTRYPTAMINE) EXHIBITS ANALGESIC PROPERTIES IN CHRONIC PAIN CONDITIONS. WHILE RESEARCHES LINKING MLT TO EPIGENETIC MECHANISMS HAVE GROWN EXPONENTIALLY OVER RECENT YEARS, VERY FEW STUDIES HAVE INVESTIGATED THE CONTRIBUTION OF MLT-ASSOCIATED EPIGENETIC MODIFICATION TO PAIN STATES. HERE, WE REPORT THAT TOGETHER WITH BEHAVIORAL ALLODYNIA, SPINAL NERVE LIGATION (SNL) INDUCED A DECREASE IN THE EXPRESSION OF CATALYTIC SUBUNIT OF PHOSPHATASE 2A (PP2AC) AND ENHANCED HISTONE DEACETYLASE 4 (HDAC4) PHOSPHORYLATION AND CYTOPLASMIC ACCUMULATION, WHICH EPIGENETICALLY ALLEVIATED HDAC4-SUPPRESSED HMGB1 GENE TRANSCRIPTION, RESULTING IN INCREASED HIGH-MOBILITY GROUP PROTEIN B1 (HMGB1) EXPRESSION SELECTIVELY IN THE IPSILATERAL DORSAL HORN OF RATS. FOCAL KNOCK-DOWN OF SPINAL PP2AC EXPRESSION ALSO RESULTED IN BEHAVIORAL ALLODYNIA IN ASSOCIATION WITH SIMILAR PROTEIN EXPRESSION AS OBSERVED WITH SNL. NOTABLY, INTRATHECAL ADMINISTRATION WITH MLT INCREASED PP2AC EXPRESSION, HDAC4 DEPHOSPHORYLATION AND NUCLEAR ACCUMULATION, RESTORED HDAC4-MEDIATED HMGB1 SUPPRESSION AND RELIEVED SNL-SENSITIZED BEHAVIORAL PAIN; THESE EFFECTS WERE ALL INHIBITED BY SPINAL INJECTION OF 4P-PDOT (A MT2 RECEPTOR ANTAGONIST, 30 MINUTES BEFORE MLT) AND OKADAIC ACID (OA, A PP2A INHIBITOR, 3 HR AFTER MLT). OUR FINDINGS DEMONSTRATE A NOVEL MECHANISM BY WHICH MLT AMELIORATES NEUROPATHIC ALLODYNIA VIA EPIGENETIC MODIFICATION. THIS MLT-EXHIBITED ANTI-ALLODYNIA IS MEDIATED BY MT2-ENHANCED PP2AC EXPRESSION THAT COUPLES PP2AC WITH HDAC4 TO INDUCE HDAC4 DEPHOSPHORYLATION AND NUCLEAR IMPORT, HEREIN INCREASES HDAC4 BINDING TO THE PROMOTER OF HMGB1 GENE AND UPREGULATES HMGB1 EXPRESSION IN DORSAL HORN NEURONS. 2016 3 3982 31 LONG-TERM EXPOSURE OF LEUKEMIA CELLS TO MULTI-TARGETED TYROSINE KINASE INHIBITOR INDUCES ACTIVATIONS OF AKT, ERK AND STAT5 SIGNALING VIA EPIGENETIC SILENCING OF THE PTEN GENE. IMATINIB INDUCES COMPLETE MOLECULAR RESPONSE IN PATIENTS WITH CHRONIC MYELOID LEUKEMIA (CML) AND CHRONIC EOSINOPHILIC LEUKEMIA (CEL). HOWEVER, DEVELOPMENT OF RESISTANCE TO IMATINIB HAS EMERGED AS AN IMPORTANT CLINICAL PROBLEM FOR MOLECULAR-TARGETED THERAPY IN CML AND CEL. IN THIS STUDY, WE HAVE ESTABLISHED THE IMATINIB-RESISTANT CEL EOL-1 SUB-LINES (DESIGNATED AS EOL-1R) BY CULTURING CELLS WITH INCREASING CONCENTRATIONS OF IMATINIB FOR 6 MONTHS. INTERESTINGLY, EOL-1R CELLS SHOWED EPIGENETIC SILENCING OF THE PHOSPHATASE AND TENSIN HOMOLOG DELETED ON CHROMOSOME TEN (PTEN) GENE. EXPOSURE OF EOL-1R CELLS TO IMATINIB FAILED TO DEPHOSPHORYLATE AKT, ERK AND STAT5, ALTHOUGH PDGFRALPHA WAS EFFECTIVELY INACTIVATED. THE FORCED EXPRESSION OF PTEN NEGATIVELY REGULATED THESE SIGNAL PATHWAYS AND SENSITIZED EOL-1R CELLS TO IMATINIB. NOTABLY, HYPERMETHYLATION OF THE PROMOTER REGION OF THE PTEN GENE IN ASSOCIATION WITH THE DOWNREGULATION OF THIS GENE'S TRANSCRIPTS WAS IDENTIFIED IN IMATINIB-RESISTANT LEUKEMIA CELLS ISOLATED FROM INDIVIDUALS WITH CEL, CML AND PHILADELPHIA-POSITIVE ACUTE LYMPHOBLASTIC LEUKEMIA. IN ADDITION, ANTI-EPIGENETIC AGENTS RESTORED PTEN EXPRESSION, RESULTING IN THE SENSITIZATION OF EOL-1R CELLS TO IMATINIB. TAKEN TOGETHER, EPIGENETIC SILENCE OF PTEN IS ONE OF THE MECHANISMS THAT CAUSE DRUG RESISTANCE IN INDIVIDUALS WITH LEUKEMIA AFTER EXPOSURE TO IMATINIB. ANTI-EPIGENETIC AGENTS MAY BE USEFUL FOR OVERCOMING DRUG RESISTANCE IN SUCH A CASE. 2010 4 5301 21 PROTEIN PHOSPHATASE 2A CATALYTIC SUBUNIT ALPHA PLAYS A MYD88-DEPENDENT, CENTRAL ROLE IN THE GENE-SPECIFIC REGULATION OF ENDOTOXIN TOLERANCE. MYD88, THE INTRACELLULAR ADAPTOR OF MOST TLRS, MEDIATES EITHER PROINFLAMMATORY OR IMMUNOSUPPRESSIVE SIGNALING THAT CONTRIBUTES TO CHRONIC INFLAMMATION-ASSOCIATED DISEASES. ALTHOUGH GENE-SPECIFIC CHROMATIN MODIFICATIONS REGULATE INFLAMMATION, THE ROLE OF MYD88 SIGNALING IN ESTABLISHING SUCH EPIGENETIC LANDSCAPES UNDER DIFFERENT INFLAMMATORY STATES REMAINS ELUSIVE. USING QUANTITATIVE PROTEOMICS TO ENUMERATE THE INFLAMMATION-PHENOTYPIC CONSTITUENTS OF THE MYD88 INTERACTOME, WE FOUND THAT IN ENDOTOXIN-TOLERANT MACROPHAGES, PROTEIN PHOSPHATASE 2A CATALYTIC SUBUNIT ALPHA (PP2AC) ENHANCES ITS ASSOCIATION WITH MYD88 AND IS CONSTITUTIVELY ACTIVATED. KNOCKDOWN OF PP2AC PREVENTS SUPPRESSION OF PROINFLAMMATORY GENES AND RESISTANCE TO APOPTOSIS. THROUGH SITE-SPECIFIC DEPHOSPHORYLATION, CONSTITUTIVELY ACTIVE PP2AC DISRUPTS THE SIGNAL-PROMOTING TLR4-MYD88 COMPLEX AND BROADLY SUPPRESSES THE ACTIVITIES OF MULTIPLE PROINFLAMMATORY/PROAPOPTOTIC PATHWAYS AS WELL, SHIFTING PROINFLAMMATORY MYD88 SIGNALING TO A PROSURVIVAL MODE. CONSTITUTIVELY ACTIVE PP2AC TRANSLOCATED WITH MYD88 INTO THE NUCLEI OF TOLERANT MACROPHAGES ESTABLISHES THE IMMUNOSUPPRESSIVE PATTERN OF CHROMATIN MODIFICATIONS AND REPRESSES CHROMATIN REMODELING TO SELECTIVELY SILENCE PROINFLAMMATORY GENES, COORDINATING THE MYD88-DEPENDENT INFLAMMATION CONTROL AT BOTH SIGNALING AND EPIGENETIC LEVELS UNDER ENDOTOXIN-TOLERANT CONDITIONS. 2013 5 3352 29 HISTONE DEMETHYLASE RBP2 MEDIATES THE BLAST CRISIS OF CHRONIC MYELOID LEUKEMIA THROUGH AN RBP2/PTEN/BCR-ABL CASCADE. EPIGENETIC DISORDERS PLAY A KEY ROLE IN TUMORIGENESIS AND DEVELOPMENT, AMONG WHICH HISTONE METHYLATION ABNORMALITIES ARE COMMON. WHILE PATIENTS LIVING WITH CHRONIC MYELOID LEUKEMIA IN THE CHRONIC PHASE (CML-CP) HAVE A GOOD RESPONSE TO TKI, BLASTIC PHASE (CML-BP) PATIENTS DEMONSTRATE POOR EFFICACY AND HIGH FATALITY RATES. HOWEVER, WHILE THE MECHANISM OF BLAST CRISIS OF CHRONIC MYELOID LEUKEMIA REMAINS UNCLEAR, HIGH EXPRESSION AND ACTIVATION OF BCR-ABL ARE USUALLY RELATED TO CML BLAST CRISIS TRANSITION. WE FOUND THAT HISTONE H3 LYSINE 4 (H3K4) DEMETHYLASE RBP2 EXPRESSION IS NEGATIVELY CORRELATED WITH BCR-ABL EXPRESSION, WHICH SUGGESTS A REGULATORY LINK BETWEEN THESE TWO GENES. WE ALSO DISCOVERED THAT RBP2 MEDIATES THE DEPHOSPHORYLATION OF BCR-ABL BY DIRECTLY DOWNREGULATING PTEN EXPRESSION, DEPENDING ON HISTONE DEMETHYLASE ACTIVITY, WHILE PTEN TARGETS PROTEIN PHOSPHATASE ACTIVITY OF BCR-ABL, A PHOSPHATASE WHICH DIRECTLY DEPHOSPHORYLATES BCR-ABL. IN CLINICAL SPECIMENS, THE MRNA EXPRESSION OF RBP2 WAS FOUND TO BE POSITIVELY CORRELATED WITH THAT OF PTEN. THESE DATA SUGGEST THAT THE UNDER-EXPRESSION OF RBP2 PROMOTES BLAST CRISIS TRANSITION BY ACTIVATING AN RBP2/PTEN/BCR-ABL CASCADE. 2019 6 574 26 BCR/ABL INCREASES EZH2 LEVELS WHICH REGULATES XIAP EXPRESSION VIA MIRNA-219 IN CHRONIC MYELOID LEUKEMIA CELLS. IN THIS STUDY, WE SHOWED THAT THE LEVELS OF EZH2 IN BONE MARROW MONONUCLEAR CELLS (BMMNCS) ISOLATED FROM INDIVIDUALS WITH CHRONIC MYELOID LEUKEMIA (CML) (N=12) WERE SIGNIFICANTLY GREATER THAN THOSE IN BMMNCS ISOLATED FROM HEALTHY VOLUNTEERS (N=6) AS WELL AS INDIVIDUALS WITH PHILADELPHIA CHROMOSOME-NEGATIVE MYELOPROLIFERATIVE NEOPLASMS. LENTIVIRAL TRANSDUCTION OF THE BCR/ABL GENE IN BA/F3 CELLS INCREASED EZH2 LEVELS IN PARALLEL WITH PHOSPHORYLATION OF STAT5. NOTABLY, CHROMATIN IMMUNOPRECIPITATION ASSAYS SHOWED THAT STAT5A BOUND TO A PROMOTER REGION OF THE EZH2 GENE, RESULTING IN AN INCREASE IN THE TRANSCRIPTIONAL ACTIVITY OF EZH2 IN LEUKEMIA CELLS. IMPORTANTLY, DOWNREGULATION OF EZH2 BY SHORT HAIRPIN RNAS (SHRNAS) INHIBITED THE EXPRESSION OF XIAP AND INCREASED THE MIR-219 LEVELS ASSOCIATED WITH A DECREASE IN HYPERMETHYLATION OF MIR-219-1 CPG ISLANDS. MOREOVER, OVEREXPRESSION OF MIR-219 DECREASED THE LEVELS OF XIAP IN CML CELLS. SINCE THE 3'-UNTRANSLATED REGION (3'-UTR) OF XIAP CONTAINS MIR219-5P-COMPLEMENTARY BINDING SITE, MIR-219 MIGHT MODULATE THE EXPRESSION OF XIAP THROUGH BINDING OF MIR-219 ON THE 3'-UTR OF XIAP. TAKEN TOGETHER, BCR/ABL POSITIVELY REGULATES THE EXPRESSION OF EZH2 VIA STAT5 SIGNALING. EZH2 MODULATES EPIGENETIC CHANGES AT DNA METHYLATED REGIONS ENCODING MIR-219 AND DOWNREGULATES THE LEVEL OF MIR-219, RESULTING IN UPREGULATION OF XIAP. 2016 7 3531 23 IMATINIB CAUSES EPIGENETIC ALTERATIONS OF PTEN GENE VIA UPREGULATION OF DNA METHYLTRANSFERASES AND POLYCOMB GROUP PROTEINS. WE HAVE RECENTLY REPORTED THE POSSIBLE IMATINIB-RESISTANT MECHANISM; LONG-TERM EXPOSURE OF LEUKEMIA CELLS TO IMATINIB DOWNREGULATED LEVELS OF PHOSPHATASE AND TENSIN HOMOLOG DELETED ON CHROMOSOME 10 (PTEN) VIA HYPERMETHYLATION OF ITS PROMOTER REGION (LEUKEMIA 2010; 24: 1631). THE PRESENT STUDY EXPLORED THE MOLECULAR MECHANISMS BY WHICH IMATINIB CAUSED METHYLATION ON THE PROMOTER REGION OF THIS TUMOR SUPPRESSOR GENE IN LEUKEMIA CELLS. REAL-TIME REVERSE TRANSCRIPTION PCR FOUND THAT LONG-TERM EXPOSURE OF CHRONIC EOSINOPHILIC LEUKEMIA EOL-1 CELLS EXPRESSING FIP1L1/PLATELET-DERIVED GROWTH FACTOR RECEPTOR-ALPHA TO IMATINIB INDUCED EXPRESSION OF DNA METHYLTRANSFERASE 3A (DNMT3A) AND HISTONE-METHYLTRANSFERASE ENHANCER OF ZESTE HOMOLOG 2 (EZH2), A FAMILY OF POLYCOMB GROUP, THEREBY INCREASING METHYLATION OF THE GENE. IMMUNOPRECIPITATION ASSAY FOUND THE INCREASED COMPLEX FORMATION OF DNMT3A AND EZH2 PROTEINS IN THESE CELLS. MOREOVER, CHROMATIN IMMUNOPRECIPITATION ASSAY SHOWED THAT AMOUNTS OF BOTH DNMT3A AND EZH2 PROTEINS BOUND AROUND THE PROMOTER REGION OF PTEN GENE WERE INCREASED IN EOL-1 CELLS AFTER EXPOSURE TO IMATINIB. FURTHERMORE, WE FOUND THAT LEVELS OF DNMT3A AND EZH2 WERE STRIKINGLY INCREASED IN LEUKEMIA CELLS ISOLATED FROM INDIVIDUALS WITH CHRONIC MYELOGENOUS LEUKEMIA (N=1) AND PHILADELPHIA CHROMOSOME-POSITIVE ACUTE LYMPHOBLASTIC LEUKEMIA (N=2), WHO RELAPSED AFTER TREATMENT WITH IMATINIB COMPARED WITH THOSE ISOLATED AT THEIR INITIAL PRESENTATION. TAKEN TOGETHER, IMATINIB COULD CAUSE DRUG-RESISTANCE VIA RECRUITMENT OF POLYCOMB GENE COMPLEX TO THE PROMOTER REGION OF THE PTEN AND DOWNREGULATION OF THIS GENE'S TRANSCRIPTS IN LEUKEMIA PATIENTS. 2011 8 3781 23 INTERFERON SIGNATURE IN PATIENTS WITH STAT1 GAIN-OF-FUNCTION MUTATION IS EPIGENETICALLY DETERMINED. STAT1 GAIN-OF-FUNCTION (GOF) VARIANTS LEAD TO DEFECTIVE TH17 CELL DEVELOPMENT AND CHRONIC MUCOCUTANEOUS CANDIDIASIS (CMC), BUT FREQUENTLY ALSO TO AUTOIMMUNITY. STIMULATION OF CELLS WITH STAT1 INDUCING CYTOKINES LIKE INTERFERONS (IFN) RESULT IN HYPERPHOSPHORYLATION AND DELAYED DEPHOSPHORYLATION OF GOF STAT1. HOWEVER, THE MECHANISM HOW THE DELAYED DEPHOSPHORYLATION EXACTLY CAUSES THE INCREASED EXPRESSION OF STAT1-DEPENDENT GENES, AND HOW THE INTRACELLULAR SIGNAL TRANSDUCTION FROM CYTOKINE RECEPTORS IS AFFECTED, REMAINS UNKNOWN. IN THIS STUDY WE SHOW THAT THE CIRCULATING LEVELS OF IFN-ALPHA WERE NOT PERSISTENTLY ELEVATED IN STAT1 GOF PATIENTS. NEVERTHELESS, THE EXPRESSION OF INTERFERON SIGNATURE GENES WAS EVIDENT EVEN IN THE PATIENT WITH LOW OR UNDETECTABLE SERUM IFN-ALPHA LEVELS. CHROMATIN IMMUNOPRECIPITATION (CHIP) EXPERIMENTS REVEALED THAT THE ACTIVE CHROMATIN MARK TRIMETHYLATION OF LYSINE 4 OF HISTONE 3 (H3K4ME3), WAS SIGNIFICANTLY ENRICHED IN AREAS ASSOCIATED WITH INTERFERON-STIMULATED GENES IN STAT1 GOF CELLS IN COMPARISON TO CELLS FROM HEALTHY DONORS. THIS SUGGESTS THAT THE CHROMATIN BINDING OF GOF STAT1 VARIANT PROMOTES EPIGENETIC CHANGES COMPATIBLE WITH HIGHER GENE EXPRESSION AND ELEVATED REACTIVITY TO TYPE I INTERFERONS, AND POSSIBLY PREDISPOSES FOR INTERFERON-RELATED AUTOIMMUNITY. THE RESULTS ALSO SUGGEST THAT EPIGENETIC REWIRING MAY BE RESPONSIBLE FOR TREATMENT FAILURE OF JANUS KINASE 1/2 (JAK1/2) INHIBITORS IN CERTAIN PATIENTS. 2019 9 1693 31 DUSP4 DEFICIENCY CAUSED BY PROMOTER HYPERMETHYLATION DRIVES JNK SIGNALING AND TUMOR CELL SURVIVAL IN DIFFUSE LARGE B CELL LYMPHOMA. THE EPIGENETIC DYSREGULATION OF TUMOR SUPPRESSOR GENES IS AN IMPORTANT DRIVER OF HUMAN CARCINOGENESIS. WE HAVE COMBINED GENOME-WIDE DNA METHYLATION ANALYSES AND GENE EXPRESSION PROFILING AFTER PHARMACOLOGICAL DNA DEMETHYLATION WITH FUNCTIONAL SCREENING TO IDENTIFY NOVEL TUMOR SUPPRESSORS IN DIFFUSE LARGE B CELL LYMPHOMA (DLBCL). WE FIND THAT A CPG ISLAND IN THE PROMOTER OF THE DUAL-SPECIFICITY PHOSPHATASE DUSP4 IS ABERRANTLY METHYLATED IN NODAL AND EXTRANODAL DLBCL, IRRESPECTIVE OF ABC OR GCB SUBTYPE, RESULTING IN LOSS OF DUSP4 EXPRESSION IN 75% OF >200 EXAMINED CASES. THE DUSP4 GENOMIC LOCUS IS FURTHER DELETED IN UP TO 13% OF AGGRESSIVE B CELL LYMPHOMAS, AND THE LACK OF DUSP4 IS A NEGATIVE PROGNOSTIC FACTOR IN THREE INDEPENDENT COHORTS OF DLBCL PATIENTS. ECTOPIC EXPRESSION OF WILD-TYPE DUSP4, BUT NOT OF A PHOSPHATASE-DEFICIENT MUTANT, DEPHOSPHORYLATES C-JUN N-TERMINAL KINASE (JNK) AND INDUCES APOPTOSIS IN DLBCL CELLS. PHARMACOLOGICAL OR DOMINANT-NEGATIVE JNK INHIBITION RESTRICTS DLBCL SURVIVAL IN VITRO AND IN VIVO AND SYNERGIZES STRONGLY WITH THE BRUTON'S TYROSINE KINASE INHIBITOR IBRUTINIB. OUR RESULTS INDICATE THAT DLBCL CELLS DEPEND ON JNK SIGNALING FOR SURVIVAL. THIS FINDING PROVIDES A MECHANISTIC BASIS FOR THE CLINICAL DEVELOPMENT OF JNK INHIBITORS IN DLBCL, IDEALLY IN SYNTHETIC LETHAL COMBINATIONS WITH INHIBITORS OF CHRONIC ACTIVE B CELL RECEPTOR SIGNALING. 2015 10 3175 27 H2AX PHOSPHORYLATION REGULATED BY P38 IS INVOLVED IN BIM EXPRESSION AND APOPTOSIS IN CHRONIC MYELOGENOUS LEUKEMIA CELLS INDUCED BY IMATINIB. INCREASING EVIDENCE SUGGESTS THAT HISTONE H2AX PLAYS A CRITICAL ROLE IN REGULATION OF TUMOR CELL APOPTOSIS AND ACTS AS A NOVEL HUMAN TUMOR SUPPRESSOR PROTEIN. HOWEVER, THE ACTION OF H2AX IN CHRONIC MYELOGENOUS LEUKEMIA (CML) CELLS IS UNKNOWN. THE DETAILED MECHANISM AND EPIGENETIC REGULATION BY H2AX REMAIN ELUSIVE IN CANCER CELLS. HERE, WE REPORT THAT H2AX WAS INVOLVED IN APOPTOSIS OF CML CELLS. OVEREXPRESSION OF H2AX INCREASED APOPTOTIC SENSITIVITY OF CML CELLS (K562) INDUCED BY IMATINIB. HOWEVER, OVEREXPRESSION OF SER139-MUTATED H2AX (BLOCKING PHOSPHORYLATION) DECREASED SENSITIVITY OF K562 CELLS TO APOPTOSIS. SIMILARLY, KNOCKDOWN OF H2AX MADE K562 CELLS RESISTANT TO APOPTOTIC INDUCTION. THESE RESULTS REVEALED THAT THE FUNCTION OF H2AX INVOLVED IN APOPTOSIS IS STRICTLY RELATED TO ITS PHOSPHORYLATION (SER139). OUR DATA FURTHER INDICATED THAT IMATINIB MAY STIMULATE MITOGEN-ACTIVATED PROTEIN KINASE (MAPK) FAMILY MEMBER P38, AND H2AX PHOSPHORYLATION FOLLOWED A SIMILAR TIME COURSE, SUGGESTING A PARALLEL RESPONSE. H2AX PHOSPHORYLATION CAN BE BLOCKED BY P38 SIRNA OR ITS INHIBITOR. THESE DATA DEMONSTRATED THAT H2AX PHOSPHORYLATION WAS REGULATED BY P38 MAPK PATHWAY IN K562 CELLS. HOWEVER, THE P38 MAPK DOWNSTREAM, MITOGEN- AND STRESS-ACTIVATED PROTEIN KINASE-1 AND -2, WHICH PHOSPHORYLATED HISTONE H3, WERE NOT REQUIRED FOR H2AX PHOSPHORYLATION DURING APOPTOSIS. FINALLY, WE PROVIDED EPIGENETIC EVIDENCE THAT H2AX PHOSPHORYLATION REGULATED APOPTOSIS-RELATED GENE BIM EXPRESSION. BLOCKING OF H2AX PHOSPHORYLATION INHIBITED BIM GENE EXPRESSION. TAKEN TOGETHER, THESE DATA DEMONSTRATED THAT H2AX PHOSPHORYLATION REGULATED BY P38 IS INVOLVED IN BIM EXPRESSION AND APOPTOSIS IN CML CELLS INDUCED BY IMATINIB. 2014 11 3877 27 KDM6A PROMOTES IMATINIB RESISTANCE THROUGH YY1-MEDIATED TRANSCRIPTIONAL UPREGULATION OF TRKA INDEPENDENTLY OF ITS DEMETHYLASE ACTIVITY IN CHRONIC MYELOGENOUS LEUKEMIA. RATIONALE: DESPITE LANDMARK THERAPY OF CHRONIC MYELOGENOUS LEUKEMIA (CML) WITH TYROSINE KINASE INHIBITORS (TKIS), DRUG RESISTANCE REMAINS PROBLEMATIC. CANCER PATHOGENESIS INVOLVES EPIGENETIC DYSREGULATION AND IN PARTICULAR, HISTONE LYSINE DEMETHYLASES (KDMS) HAVE BEEN IMPLICATED IN TKI RESISTANCE. WE SOUGHT TO IDENTIFY KDMS WITH ALTERED EXPRESSION IN CML AND DEFINE THEIR CONTRIBUTION TO IMATINIB RESISTANCE. METHODS: BIOINFORMATICS SCREENING COMPARED KDM EXPRESSION IN CML VERSUS NORMAL BONE MARROW WITH SHRNA KNOCKDOWN AND FLOW CYTOMETRY USED TO MEASURE EFFECTS ON IMATINIB-INDUCED APOPTOSIS IN K562 CELLS. TRANSCRIPTOMIC ANALYSES WERE PERFORMED AGAINST KDM6A CRISPR KNOCKOUT/SHRNA KNOCKDOWN K562 CELLS ALONG WITH GENE RESCUE EXPERIMENTS USING WILDTYPE AND MUTANT DEMETHYLASE-DEAD KDM6A CONSTRUCTS. CO-IMMUNOPRECIPITATION, LUCIFERASE REPORTER AND CHIP WERE EMPLOYED TO ELUCIDATE MECHANISMS OF KDM6A-DEPENDENT RESISTANCE. RESULTS: AMONGST FIVE KDMS UPREGULATED IN CML, ONLY KDM6A DEPLETION SENSITIZED CML CELLS TO IMATINIB-INDUCED APOPTOSIS. RE-INTRODUCTION OF DEMETHYLASE-DEAD KDM6A AS WELL AS WILD-TYPE KDM6A RESTORED IMATINIB RESISTANCE. RNA-SEQ IDENTIFIED NTRK1 GENE DOWNREGULATION AFTER DEPLETION OF KDM6A. MOREOVER, NTRK1 EXPRESSION POSITIVELY CORRELATED WITH KDM6A IN A SUBSET OF CLINICAL CML SAMPLES AND KDM6A KNOCKDOWN IN FRESH CML ISOLATES DECREASED NTRK1 ENCODED PROTEIN (TRKA) EXPRESSION. MECHANISTICALLY, KDM6A WAS RECRUITED TO THE NTRK1 PROMOTER BY THE TRANSCRIPTION FACTOR YY1 WITH SUBSEQUENT TRKA UPREGULATION ACTIVATING DOWN-STREAM SURVIVAL PATHWAYS TO INVOKE IMATINIB RESISTANCE. CONCLUSION: CONTRARY TO ITS REPORTED ROLE AS A TUMOR SUPPRESSOR AND INDEPENDENT OF ITS DEMETHYLASE FUNCTION, KDM6A PROMOTES IMATINIB-RESISTANCE IN CML CELLS. THE IDENTIFICATION OF THE KDM6A/YY1/TRKA AXIS AS A NOVEL IMATINIB-RESISTANCE MECHANISM REPRESENTS AN UNEXPLORED AVENUE TO OVERCOME TKI RESISTANCE IN CML. 2021 12 3633 27 INCREASE IN HDAC9 SUPPRESSES MYOBLAST DIFFERENTIATION VIA EPIGENETIC REGULATION OF AUTOPHAGY IN HYPOXIA. EXTREMELY REDUCED OXYGEN (O(2)) LEVELS ARE DETRIMENTAL TO MYOGENIC DIFFERENTIATION AND MULTINUCLEATED MYOTUBE FORMATION, AND CHRONIC EXPOSURE TO HIGH-ALTITUDE HYPOXIA HAS BEEN REPORTED TO BE AN IMPORTANT FACTOR IN SKELETAL MUSCLE ATROPHY. HOWEVER, HOW CHRONIC HYPOXIA CAUSES MUSCLE DYSFUNCTION REMAINS UNKNOWN. IN THE PRESENT STUDY, WE FOUND THAT SEVERE HYPOXIA (1% O(2)) SIGNIFICANTLY INHIBITED THE FUNCTION OF C2C12 CELLS (FROM A MYOBLAST CELL LINE). IMPORTANTLY, THE IMPAIRMENT WAS CONTINUOUSLY MANIFESTED EVEN DURING CULTURE UNDER NORMOXIC CONDITIONS FOR SEVERAL PASSAGES. MECHANISTICALLY, WE REVEALED THAT HISTONE DEACETYLASES 9 (HDAC9), A MEMBER OF THE HISTONE DEACETYLASE FAMILY, WAS SIGNIFICANTLY INCREASED IN C2C12 CELLS UNDER HYPOXIC CONDITIONS, THEREBY INHIBITING INTRACELLULAR AUTOPHAGY LEVELS BY DIRECTLY BINDING TO THE PROMOTER REGIONS OF ATG7, BECLIN1, AND LC3. THIS PHENOMENON RESULTED IN THE SEQUENTIAL DEPHOSPHORYLATION OF GSK3BETA AND INACTIVATION OF THE CANONICAL WNT PATHWAY, IMPAIRING THE FUNCTION OF THE C2C12 CELLS. TAKEN TOGETHER, OUR RESULTS SUGGEST THAT HYPOXIA-INDUCED MYOBLAST DYSFUNCTION IS DUE TO ABERRANT EPIGENETIC REGULATION OF AUTOPHAGY, AND OUR EXPERIMENTAL EVIDENCE REVEALS THE POSSIBLE MOLECULAR PATHOGENESIS RESPONSIBLE FOR SOME MUSCLE DISEASES CAUSED BY CHRONIC HYPOXIA AND SUGGESTS A POTENTIAL THERAPEUTIC OPTION. 2019 13 6402 20 THE ROLES OF EPIGENETIC MODIFICATIONS OF PROAPOPTOTIC BID AND BIM GENES IN IMATINIB-RESISTANT CHRONIC MYELOID LEUKEMIA CELLS. IN CHRONIC MYELOID LEUKEMIA (CML), EPIGENETIC MODIFICATIONS SUCH AS PROMOTER HYPERMETHYLATION AND INACTIVE HISTONE MODIFICATION ARE KNOWN MECHANISMS OF DRUG RESISTANCE. IN OUR STUDY, WE INVESTIGATED THE ROLES OF PROMOTER HYPERMETHYLATION OF BIM AND BID GENES AND H3K27ME3 HISTONE MODIFICATION ON IMATINIB RESISTANCE. WE DETECTED HIGHER EXPRESSION LEVELS OF BIM AND BID GENES AND LOWER EXPRESSION LEVELS OF EZH2, EED2, SIRT1, AND SUZ12 GENES IN IMATINIB-RESISTANT K562/IMA-3 CELLS COMPARED TO IMATINIB-NON-RESISTANT K562 CELLS. WHILE WE DETERMINED THE EZH2 AND DNMT ENZYMES AS BOUNDED TO THE PROMOTER OF THE BIM GENE, WE DID NOT DETECT HYPERMETHYLATION OF THIS PROMOTER. WE ALSO FOUND THE H3K27ME3 HISTONE MODIFICATION PROMOTER OF BIM AND BID GENES IN BOTH CELL LINES. IN CONCLUSION, OUR RESULTS SUPPORT THE NOTION THAT DNA PROMOTER METHYLATION MAY BE FORMED INDEPENDENTLY FROM EZH2-H3K27ME3 AND PRO-APOPTOTIC BIM AND BID GENES ARE NOT METHYLLATED IN THE IMATINIB RESISTANCE OF CML CELLS. 2013 14 3475 21 IDENTIFICATION OF A STAT5 TARGET GENE, DPF3, PROVIDES NOVEL INSIGHTS IN CHRONIC LYMPHOCYTIC LEUKEMIA. STAT5 CONTROLS ESSENTIAL CELLULAR FUNCTIONS AND IS ENCODED BY TWO GENES, STAT5A AND STAT5B. TO PROVIDE INSIGHT TO THE MECHANISMS LINKING HEMATOLOGIC MALIGNANCY TO STAT5 ACTIVATION/REGULATION OF TARGET GENES, WE IDENTIFIED STAT5 TARGET GENES AND FOCUSED ON DPF3 GENE, WHICH ENCODES FOR AN EPIGENETIC FACTOR. DPF3 EXPRESSION WAS INDUCED UPON IL-3 STIMULATION IN BA/F3 CELLS, WHILE STRONG BINDING OF BOTH STAT5A AND STAT5B WAS DETECTED IN ITS PROMOTER. REDUCED EXPRESSION OF DPF3 WAS DETECTED IN BA/F3 CELLS WITH STAT5A AND STAT5B KNOCK-DOWN, SUGGESTING THAT THIS GENE IS POSITIVELY REGULATED BY STAT5, UPON IL-3 STIMULATION. FURTHERMORE, THIS GENE WAS SIGNIFICANTLY UP-REGULATED IN CLL PATIENTS, WHERE DPF3 GENE/PROTEIN UP-REGULATION AND STRONG STAT5 BINDING TO THE DPF3 PROMOTER, CORRELATED WITH INCREASED STAT5 ACTIVATION, MAINLY IN NON-MALIGNANT MYELOID CELLS (GRANULOCYTES). OUR FINDINGS PROVIDE INSIGHTS IN THE STAT5 DEPENDENT TRANSCRIPTIONAL REGULATION OF DPF3, AND DEMONSTRATE FOR THE FIRST TIME INCREASED STAT5 ACTIVATION IN GRANULOCYTES OF CLL PATIENTS. NOVEL ROUTES OF INVESTIGATION ARE OPENED TO FACILITATE THE UNDERSTANDING OF THE ROLE OF STAT5 ACTIVATION IN THE COMMUNICATION BETWEEN NON-MALIGNANT MYELOID AND MALIGNANT B-CELLS, AND THE FUNCTIONS OF STAT5 TARGET GENES NETWORKS IN CLL BIOLOGY. 2013 15 3261 27 HEPATITIS C VIRUS-INDUCED UP-REGULATION OF PROTEIN PHOSPHATASE 2A INHIBITS HISTONE MODIFICATION AND DNA DAMAGE REPAIR. THE MOLECULAR MECHANISMS UNDERLYING HEPATOCARCINOGENESIS IN CHRONIC VIRAL HEPATITIS ARE POORLY UNDERSTOOD. A POTENTIAL TUMORIGENIC PATHWAY COULD INVOLVE PROTEIN PHOSPHATASE 2A (PP2A) AND PROTEIN ARGININE METHYLTRANSFERASE 1 (PRMT1), BECAUSE BOTH ENZYMES ARE DYSREGULATED IN CHRONIC HEPATITIS C, AND BOTH ENZYMES HAVE BEEN INVOLVED IN CHROMATIN REMODELING AND DNA DAMAGE REPAIR. WE USED CELL LINES THAT ALLOW THE INDUCIBLE EXPRESSION OF HEPATITIS C VIRUS PROTEINS (UHCV57.3) AND OF THE CATALYTIC SUBUNIT OF PP2A (UPP2A-C8) AS WELL AS HUH7.5 CELLS INFECTED WITH RECOMBINANT CELL CULTURE-DERIVED HEPATITIS C VIRUS (HCVCC) TO STUDY EPIGENETIC HISTONE MODIFICATIONS AND DNA DAMAGE REPAIR. THE INDUCTION OF VIRAL PROTEINS, THE OVEREXPRESSION OF PP2AC, OR THE INFECTION OF HUH7.5 CELLS WITH HCVCC RESULTED IN AN INHIBITION OF HISTONE H4 METHYLATION/ACETYLATION AND HISTONE H2AX PHOSPHORYLATION, IN A SIGNIFICANTLY CHANGED EXPRESSION OF GENES IMPORTANT FOR HEPATOCARCINOGENESIS, AND INHIBITED DNA DAMAGE REPAIR. OVEREXPRESSION OF PP2AC IN NIH-3T3 CELLS INCREASED ANCHORAGE-INDEPENDENT GROWTH. THESE CHANGES WERE PARTIALLY REVERSED BY THE TREATMENT OF CELLS WITH THE METHYL-GROUP DONOR S-ADENOSYL-L-METHIONINE (SAME). CONCLUSION: HEPATITIS C VIRUS-INDUCED OVEREXPRESSION OF PP2AC CONTRIBUTES TO HEPATOCARCINOGENESIS THROUGH DYSREGULATION OF EPIGENETIC HISTONE MODIFICATIONS. THE CORRECTION OF DEFECTIVE HISTONE MODIFICATIONS BY S-ADENOSYL-L-METHIONINE MAKES THIS DRUG A CANDIDATE FOR CHEMOPREVENTIVE THERAPIES IN PATIENTS WITH CHRONIC HEPATITIS C WHO ARE AT RISK FOR DEVELOPING HEPATOCELLULAR CARCINOMA. 2010 16 5459 23 RESEARCH ON THE EPIGENETIC REGULATION MECHANISM OF THE PTPN6 GENE IN ADVANCED CHRONIC MYELOID LEUKAEMIA. PTPN6, A TYROSINE PHOSPHATASE PROTEIN, PLAYS A NEGATIVE ROLE IN CELL SIGNAL TRANSDUCTION AND IS NEGATIVELY CORRELATED WITH TUMOUR FORMATION AND GROWTH. HOWEVER, EPIGENETIC REGULATION MECHANISM OF THE PTPN6 GENE IN ADVANCED CHRONIC MYELOID LEUKAEMIA (CML) REMAINS UNCLEAR. THIS STUDY INVESTIGATED BONE MARROW OR BLOOD SAMPLES FROM 44 CML PATIENTS AND 10 HEALTHY VOLUNTEERS. KCL22 AND K562 CELLS WERE CULTURED AND TREATED WITH DEMETHYLATION DRUGS AND HISTONE DEACETYLASE INHIBITORS. REAL TIME QUANTITATIVE POLYMERASE CHAIN REACTION (QPCR), METHYLATION-SPECIFIC PCR, BISULFITE SEQUENCING PCR, WESTERN BLOTTING, CO-IMMUNOPRECIPITATION AND CHROMATIN IMMUNOPRECIPITATION (CHIP) WAS PERFORMED. PTPN6 WAS DOWN-REGULATED IN CELL LINES AND PATIENTS WITH ADVANCED PHASE CML, WHEREAS DNMT1, DNMT3A, MECP2, MBD2 AND HDAC1 WERE UP-REGULATED. TREATMENT WITH 5-AZACYTIDINE, DECITABINE, SODIUM VALPROATE AND LBH589 INCREASED PTPN6 EXPRESSION, BUT DECREASED THAT OF DNMT1, DNMT3A, MECP2, MBD2 AND HDAC1. IMMUNOPRECIPITATION AND MASS SPECTROMETRY SHOWED THAT HDAC1 COMBINED DIRECTLY WITH PTPN6. CHIP-SEQ SHOWED THAT HDAC1 DID NOT COMBINE WITH THE PROMOTER REGION OF PTPN6, WHILE MAPK, AKT, STAT5, JAK2 AND MYC PROMOTER REGIONS ALL COMBINED WITH HDAC1. PTPN6 IS ASSOCIATED WITH PROGRESSION OF CML. LOW EXPRESSION LEVEL OF PTPN6 WAS ASSOCIATED WITH DNA METHYLATION AND REGULATED BY HISTONE ACETYLATION. HDAC1 PARTICIPATES IN THE REGULATION OF PTPN6. 2017 17 4172 20 MELATONIN IMPEDES TET1-DEPENDENT MGLUR5 PROMOTER DEMETHYLATION TO RELIEVE PAIN. MELATONIN (N-ACETYL-5-METHOXYTRYPTAMINE)/MT2 RECEPTOR-DEPENDENT EPIGENETIC MODIFICATION REPRESENTS A NOVEL PATHWAY IN THE TREATMENT OF NEUROPATHIC PAIN. BECAUSE SPINAL TEN-ELEVEN TRANSLOCATION METHYLCYTOSINE DIOXYGENASE 1 (TET1)-DEPENDENT EPIGENETIC DEMETHYLATION HAS RECENTLY BEEN LINKED TO PAIN HYPERSENSITIVITY, WE HYPOTHESIZED THAT MELATONIN/MT2-DEPENDENT ANALGESIA INVOLVES SPINAL TET1-DEPENDENT DEMETHYLATION. HERE, WE SHOWED THAT SPINAL TET1 GENE TRANSFER BY INTRATHECAL DELIVERY OF TET1-ENCODING VECTORS TO NAIVE RATS PRODUCED PROFOUND AND LONG-LASTING NOCICEPTIVE HYPERSENSITIVITY. IN ADDITION, ENHANCED TET1 EXPRESSION, TET1-METABOTROPIC GLUTAMATE RECEPTOR SUBTYPE 5 (MGLUR5) PROMOTER COUPLING, DEMETHYLATION AT THE MGLUR5 PROMOTER, AND MGLUR5 EXPRESSION IN DORSAL HORN NEURONS WERE OBSERVED. RATS SUBJECTED TO SPINAL NERVE LIGATION AND INTRAPLANTAR COMPLETE FREUND'S ADJUVANT INJECTION DISPLAYED TACTILE ALLODYNIA AND BEHAVIORAL HYPERALGESIA ASSOCIATED WITH SIMILAR CHANGES IN THE DORSAL HORN. NOTABLY, INTRATHECAL MELATONIN INJECTION REVERSED THE PROTEIN EXPRESSION, PROTEIN-PROMOTER COUPLING, PROMOTER DEMETHYLATION, AND PAIN HYPERSENSITIVITY INDUCED BY TET1 GENE TRANSFER, SPINAL NERVE LIGATION, AND INTRAPLANTAR COMPLETE FREUND'S ADJUVANT INJECTION. ALL THE EFFECTS CAUSED BY MELATONIN WERE BLOCKED BY PRETREATMENT WITH A MT2 RECEPTOR-SELECTIVE ANTAGONIST. IN CONCLUSION, MELATONIN RELIEVES PAIN BY IMPEDING TET1-DEPENDENT DEMETHYLATION OF MGLUR5 IN DORSAL HORN NEURONS THROUGH THE MT2 RECEPTOR. OUR FINDINGS LINK MELATONIN/MT2 SIGNALING TO TET1-DEPENDENT EPIGENETIC DEMETHYLATION OF NOCICEPTIVE GENES FOR THE FIRST TIME AND SUGGEST MELATONIN AS A PROMISING THERAPY FOR THE TREATMENT OF PAIN. 2017 18 5458 24 RESEARCH ON EPIGENETIC MECHANISM OF SFRP2 IN ADVANCED CHRONIC MYELOID LEUKEMIA. SECRETED FRIZZLED-RELATED PROTEIN 2 (SFRP2) HAS BEEN REPORTED TO ACT AS A TUMOR SUPPRESSORS. THIS STUDY AIMS TO DETECT THE BIOLOGICAL ROLE OF SFRP2 IN ADVANCED CHRONIC MYELOID LEUKEMIA (CML). IN THIS STUDY WE EXAMINED BONE MARROW SAMPLES FROM 45 CML PATIENTS AND 10 HEALTHY DONORS. K562 AND KCL22 CELLS WERE CULTURED AND TREATED WITH DEMETHYLATION DRUG AND HISTONE DEACETYLASE INHIBITOR (HDACI). KCL22 AND K562 CELLS WERE TRANSFECTED WITH LENTIVIRAL VECTOR (LV)-SFRP2, LV-CONTROL. THE CELLS WERE THEN SUBJECTED TO PROLIFERATION AND APOPTOSIS ASSAYS, REAL TIME POLYMERASE CHAIN REACTION (PCR), METHYLATION-SPECIFIC PCR (MSP), WESTERN BLOTTING, CO-IMMUNOPRECIPITATION (COIP) AND CHROMATIN IMMUNOPRECIPITATION (CHIP), WE FOUND THAT SFRP2 WAS DOWN-REGULATED IN THE ACCELERATED AND BLAST PHASE OF CML, WHEREAS, THE LEVELS OF WNT1, WNT3 AND WNT5A WERE UP-REGULATED IN THE ACCELERATED AND BLAST PHASE OF CML. OVEREXPRESSION SFRP2 INHIBITED PROLIFERATION, PROMOTED APOPTOSIS AND ACTIVATED THE WNT PATHWAY. COIP-MS RESULTS SHOWED THAT SFRP2 INTERACTED WITH WNT1 AND WNT5A. CHIP-SEQ RESULT INDICATED THAT THE PROMOTER OF H3K4ME3 AND H3K27ME3 WERE ABLE TO INTERACT WITH SFRP2. IN CONCLUSION, OUR FINDINGS DEMONSTRATED THE SFRP2 ACT AS A POTENTIAL THERAPEUTIC TARGET FOR ADVANCED CML. FURTHERMORE, OUR RESULTS SUPPORT THE USE OF DEMETHYLATION DRUGS AND HDACI AS A POTENTIAL CML TREATMENT STRATEGY. 2018 19 6028 20 THE BMI1 POLYCOMB PROTEIN REPRESSES CYCLIN G2-INDUCED AUTOPHAGY TO SUPPORT PROLIFERATION IN CHRONIC MYELOID LEUKEMIA CELLS. THE BMI1 POLYCOMB PROTEIN REGULATES SELF-RENEWAL, PROLIFERATION AND SURVIVAL OF CANCER-INITIATING CELLS ESSENTIALLY THROUGH EPIGENETIC REPRESSION OF THE CDKN2A TUMOR SUPPRESSOR LOCUS. WE DEMONSTRATE HERE FOR THE FIRST TIME THAT BMI1 ALSO PREVENTS AUTOPHAGY IN CHRONIC MYELOID LEUKEMIA (CML) CELL LINES, TO SUPPORT THEIR PROLIFERATION AND CLONOGENIC ACTIVITY. USING CHROMATIN IMMUNOPRECIPITATION, WE IDENTIFIED CCNG2/CYCLIN G2 (CCNG2) AS A DIRECT BMI1 TARGET. BMI1 DOWNREGULATION IN CD34+ CML CELLS BY PTC-209 PHARMACOLOGICAL TREATMENT OR SHBMI1 TRANSDUCTION TRIGGERED CCNG2 EXPRESSION AND DECREASED CLONOGENIC ACTIVITY. ALSO, ECTOPIC EXPRESSION OF CCNG2 IN CD34+ CML CELLS STRONGLY DECREASED THEIR CLONOGENICITY. CCNG2 WAS SHOWN TO ACT BY DISRUPTING THE PHOSPHATASE 2A COMPLEX, WHICH ACTIVATES A PKCZETA-AMPK-JNK-ERK PATHWAY THAT ENGAGES AUTOPHAGY. WE OBSERVED THAT BMI1 AND CCNG2 LEVELS EVOLVED INVERSELY DURING THE PROGRESSION OF CML TOWARDS AN ACUTE DEADLY PHASE, AND THEREFORE HYPOTHESIZED THAT BMI1 COULD SUPPORT ACUTE TRANSFORMATION OF CML THROUGH THE SILENCING OF A CCNG2-MEDIATED TUMOR-SUPPRESSIVE AUTOPHAGY RESPONSE. 2015 20 2441 22 EPIGENETIC SILENCING OF TUMOR SUPPRESSOR MIR-3151 CONTRIBUTES TO CHINESE CHRONIC LYMPHOCYTIC LEUKEMIA BY CONSTITUTIVE ACTIVATION OF MADD/ERK AND PIK3R2/AKT SIGNALING PATHWAYS. WE HYPOTHESIZE THAT MIR-3151, LOCALIZED TO A GWAS-IDENTIFIED CHRONIC LYMPHOCYTIC LEUKEMIA (CLL) RISK LOCUS (8Q22.3), IS A TUMOR SUPPRESSOR MIRNA SILENCED BY PROMOTER DNA METHYLATION IN CLL. THE PROMOTER OF MIR-3151 WAS METHYLATED IN 5/7 (71%) CLL CELL LINES, 30/98 (31%) DIAGNOSTIC PRIMARY SAMPLES, BUT NOT NORMAL CONTROLS. METHYLATION OF MIR-3151 CORRELATED INVERSELY WITH EXPRESSION. TREATMENT WITH 5-AZA-2'-DEOXYCYTIDINE LED TO PROMOTER DEMETHYLATION AND MIR-3151 RE-EXPRESSION. LUCIFERASE ASSAY CONFIRMED MAP-KINASE ACTIVATING DEATH DOMAIN (MADD) AND PHOSPHOINOSITIDE-3-KINASE, REGULATORY SUBUNIT 2 (PIK3R2) AS DIRECT TARGETS OF MIR-3151. MOREOVER, RESTORATION OF MIR-3151 RESULTED IN INHIBITION OF CELLULAR PROLIFERATION AND ENHANCED APOPTOSIS, REPRESSION OF MADD AND PIK3R2, DOWNREGULATION OF MEK/ERK AND PI3K/AKT SIGNALING, AND REPRESSION OF MCL1. LASTLY, MIR-3151 METHYLATION WAS SIGNIFICANTLY ASSOCIATED WITH METHYLATION OF MIR-203 AND MIR-34B/C IN PRIMARY CLL SAMPLES. THEREFORE, THIS STUDY SHOWED THAT MIR-3151 IS A TUMOR SUPPRESSIVE MIRNA FREQUENTLY HYPERMETHYLATED AND HENCE SILENCED IN CLL. MIR-3151 SILENCING BY DNA METHYLATION PROTECTED CLL CELLS FROM APOPTOSIS THROUGH OVER-EXPRESSION OF ITS DIRECT TARGETS MADD AND PIK3R2, HENCE CONSTITUTIVE ACTIVATION OF MEK/ERK AND PI3K/AKT SIGNALING RESPECTIVELY, AND CONSEQUENTLY OVER-EXPRESSION OF MCL1. 2015