Abnormal Mitosis and Genetic Instability Induced by Downregulation of Candidate Myeloid Tumor Suppressor Genes Isolated from the Long Arm of Chromosome 7.

Abstract To isolate myeloid tumor suppressor genes from 7q, we tried to detect microdeletions (< 100 Kb) that might be present in MDS/AML cells carrying apparently normal chromosome 7. For this purpose, we developed our original microarray-based CGH technology. In this system, instead of BAC clones generally used as probes, we applied short (3–5 Kb) genomic DNA fragments containing strictly no repetitive sequences. We made 235 probes in a region spanning 21.7 Mb within 7q21.3–7q31.1. Although we selected MDS/AML patients whose marrow did not show cytogenetically visible 7q deletions, gross copy number changes frequently observed in adult patients prevented us from identification of common microdeletions. By investigation of 21 childhood myeloid leukemia patients with normal karyotype, we successfully identified a common microdeletion spanning approximately 120 Kb. Eight (38%) patients shared this microdeletion, which was not detected in normal individuals. Database search revealed that this region contains three hypothetical genes. Only vertebrates have these genes that likely evolved from one common ancestral gene of fish. Real-time quantitative PCR revealed that 9 (29%) out of 31 adult MDS/AML harbors microdeletions in at least one of these three genes. None of these genes had been well characterized nor has known motifs that would suggest function of the gene products. We named them Miki, Titan and Kasumi. Immunoblot analysis revealed expression of all three genes at high levels in most lymphoid leukemia cell lines, while half of myeloid cell lines lacked at least one of their expression. In leukemia cells carrying monosomy 7, expression levels were generally low. Miki, a heavily glycosylated protein, co-localized with centrosomes and spindles in the mitotic phase. To test the function of Miki, we used si-RNAs to downregulate Miki expression in HeLa and K562 cells, both of which show basically normal metaphase and nuclear morphology. Cells expressing Miki at reduced levels showed small and fragmented centrosomes, loss of spindle tension, tripolar mitosis or even completely disturbed spindle formation. As a result, anaphase lagging, colchicine-mitosis (C-mitosis), premature chromosome decondensation and chromatid bridges were observed in virtually all cells in the mitotic phase. In the interphase, bi- or tri-nuclear or even multinuclear cells with micronuclei, all of which are characteristic to MDS, were frequently observed. On the other hand, proteomic analysis revealed that Titan and Kasumi bind to the DNA-PK complex, which plays critical roles in the non-homologous end joining (NHEJ) of double stranded DNA (dsDNA) breaks. Indeed, these proteins were translocated from cytoplasm to nucleus by ionizing radiation (IR) or by treatment of drugs that yield dsDNA breaks. Cells expressing Kasumi at reduced levels by si-RNA showed increased radiosensitivity, sister chromatid exchange, and number of background-level phosphorylated histone H2AX foci (i.e., foci formed without IR), which are co-localized with dsDNA breaks. These results indicate that the genes we isolated are promising candidates for anti-leukemic genes located in 7q, because downregulation of these gene products by 7q deletions would cause the abnormal morphology of MDS and genetic instability.

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Methylation Status of Tumor Suppressor Genes BEX2, IGSF4, RARB and TIMP3 Is Indicative for AML with Translocations of the MLL Gene.

Blood ◽

10.1182/blood.v110.11.2115.2115 ◽

2007 ◽

Vol 110 (11) ◽

pp. 2115-2115

Author(s):

Hilmar Quentmeier ◽

Willy G. Dirks ◽

Stefan Nagel ◽

Sonja Röhrs ◽

Björn Schneider ◽

...

Keyword(s):

Tumor Suppressor ◽

Cell Lines ◽

Promoter Methylation ◽

Tumor Suppressor Genes ◽

Lymphoblastic Leukemia ◽

Methylation Status ◽

Leukemia Cell ◽

Human Leukemia ◽

Expression Array ◽

Suppressor Genes

Abstract The methylation of CpG islands leads to the abnormal silencing of tumor suppressor genes and thus supposedly contributes to tumorigenesis. Recently, brain expressed X-linked-2 (BEX2) was described as candidate tumor suppressor gene in malignant glioma. With tissue expression array analyses, we could show that BEX2 was highly expressed in various brain-derived tissues, but not in hematopoetic cells of healthy donors. Also acute lymphoblastic leukemia (ALL) and acute myeloid leukemia (AML) cell lines usually did not show high levels of BEX2. However, we found BEX2 highly expressed in those AML cell lines that carried aberrations of the mixed lineage leukemia gene (MLLmu). While MLL wild-type (MLLwt) cell lines showed hypermethylation of a CpG rich area within the BEX2 promoter, the BEX2 expressing, MLLmu cell lines did not show methylation of the BEX2 promoter. Confirming that BEX2 is an epigenetically regulated gene, aza-2′deoxycytidine increased the expression of BEX2 mRNA in MLLwt cells. Hypermethylation profiles of tumor suppressor genes may be used to identify subtypes of leukemia/lymphoma. To find out whether silencing and activation patterns of BEX2 in leukemia correlate with those of other tumor suppressor genes, we performed a polymerase-chain reaction (PCR) based assay (MLPA) that allowed us to simultaneously verify methylation- and ploidy status of 24 tumor suppressor genes. Twenty-eight human leukemia cell lines were tested, fourteen AML- and ALL-derived cell lines, half of them with MLL translocations. In summary, 7/24 tumor suppressor genes (plus BEX2) appear to be promising markers allowing for the distinction between ALL and AML, and between MLLmu and MLLwt AML. All AML and ALL cell lines were affected by methylation or deletion of CKDN2B and/or ESR1. Analysis of the methylation status of DAPK1 and FHIT allowed to distinguish between ALL and AML. The promoters of both genes, DAPK1 and FHIT were methylated in the majority of ALL cell lines: 11/14 ALL vs. 1/14 AML cell lines showed methylation of DAPK1, 13/14 ALL vs. 2/14 AML showed methylation of FHIT. There was no correlation between the methylation status of tumor suppressor genes and the MLL status in ALL cell lines. In contrast, MLLmu and wt AML cell lines showed differential promoter methylation patterns of IGSF4, RARB and TIMP3. At least two of these genes were methylated in every MLLwt AML cell line, but not in MLLmu AML. Quantitative real-time PCR demonstrated that expression of BEX2 and IGSF4 was silenced in cells carrying the methylated promoters. For RARB and TIMP3, additional mechanisms besides promoter methylation appear to be involved in gene regulation. These results show that methylation status of as few as four tumor suppressor genes (BEX2, IGSF4, RARB and TIMP3) may allow conclusions about the MLLmu/wt status of AML cells. Our results raise the question whether MLLmu proteins are directly or indirectly responsible for the hypomethylation of BEX2, IGSF4, RARB and TIMP3. If this is the case, tissue-specific effectors must play important additional roles as MLLmu ALL cells do not show this phenomenon.

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Promoter Methylation of RASSF1A Associates to Adult Secondary Glioblastomas and Pediatric Glioblastomas

ISRN Neurology ◽

10.5402/2012/576578 ◽

2012 ◽

Vol 2012 ◽

pp. 1-10 ◽

Cited By ~ 7

Author(s):

Jorge Muñoz ◽

María del Mar Inda ◽

Paula Lázcoz ◽

Idoya Zazpe ◽

Xing Fan ◽

...

Keyword(s):

Tumor Suppressor ◽

Cell Lines ◽

Tumor Suppressor Genes ◽

Promoter Hypermethylation ◽

Suppressor Genes ◽

Primary Tumors ◽

Specific Pcr ◽

Inactivation Mechanism ◽

Altered Gene ◽

Homozygous Deletions

While allelic losses and mutations of tumor suppressor genes implicated in the etiology of astrocytoma have been widely assessed, the role of epigenetics is still a matter of study. We analyzed the frequency of promoter hypermethylation by methylation-specific PCR (MSP) in five tumor suppressor genes (PTEN, MGMT, RASSF1A, p14ARF, and p16INK4A), in astrocytoma samples and cell lines. RASSF1A was the most frequently hypermethylated gene in all grades of astrocytoma samples, in cell lines, and in adult secondary GBM. It was followed by MGMT. PTEN showed a slight methylation signal in only one GBM and one pilocytic astrocytoma, and in two cell lines; while p14ARF and p16INK4A did not show any evidence of methylation in primary tumors or cell lines. In pediatric GBM, RASSF1A was again the most frequently altered gene, followed by MGMT; PTEN, p14 and p16 showed no alterations. Lack or reduced expression of RASSF1A in cell lines was correlated with the presence of methylation. RASSF1A promoter hypermethylation might be used as a diagnostic marker for secondary GBM and pediatric GBM. Promoter hypermethylation might not be an important inactivation mechanism in other genes like PTEN, p14ARF and p16INK4A, in which other alterations (mutations, homozygous deletions) are prevalent.

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Inactivation of tumor suppressor genes and deregulation of the c-myc gene in urothelial cancer cell lines

Urological Research ◽

10.1007/bf00300017 ◽

1995 ◽

Vol 23 (5) ◽

pp. 293-300 ◽

Cited By ~ 31

Author(s):

M.-O. Grimm ◽

B. J�rgens ◽

W. A. Schulz ◽

K. Decken ◽

D. Makri ◽

...

Keyword(s):

Tumor Suppressor ◽

Cell Lines ◽

Cancer Cell ◽

Tumor Suppressor Genes ◽

Urothelial Cancer ◽

Cancer Cell Lines ◽

Suppressor Genes ◽

Myc Gene ◽

Urothelial Cancer Cell

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Downregulation of a Candidate Myeloid Tumor Suppressor Gene Isolated from 7q21 Induces Abnormal Mitosis Due to Insufficient Centrosome Maturation.

Blood ◽

10.1182/blood.v110.11.2638.2638 ◽

2007 ◽

Vol 110 (11) ◽

pp. 2638-2638

Author(s):

Hiroya Asou ◽

Hirotaka Matsui ◽

Yuko Ozaki ◽

Akiko Nagamachi ◽

Daisuke Aki ◽

...

Keyword(s):

Tumor Suppressor ◽

Tumor Suppressor Gene ◽

Cell Lines ◽

Myeloid Leukemia ◽

Leukemia Cell ◽

Suppressor Gene ◽

Monosomy 7 ◽

Leukemia Cell Lines ◽

Abnormal Mitosis ◽

Tankyrase 1

Abstract To isolate myeloid tumor suppressor gene(s) in 7q, we searched microdeletions in a region spanning 21.7 Mb within 7q21.2–7q31.1 using a microarray-based CGH system. By investigation of 21 childhood myeloid leukemia patients with normal karyotype, we identified a common microdeletion cluster spanning approximately 120 Kb in the 7q21.3 subband. Eight (38%) patients shared this microdeletion, which was not detected in normal individuals. Real-time quantitative PCR revealed that this region is also deleted in 9 (29%) out of 31 adult RAEB and AML patients. Database search revealed that this region contains three hypothetical genes. Among them, we chose one previously uncharacterized gene for further investigation and named Miki (mitotic kinetics regulator) for the function of its gene product, described below. Immunoblot analysis revealed high levels of Miki expression in most lymphoid leukemia cell lines, while half of myeloid leukemia cell lines expressed Miki at reduced levels. In six leukemia lines carrying monosomy 7, expression levels were generally low. Miki co-localized with the Golgi apparatus in the interphase and with centrosomes and spindles in the mitotic phase. To test the function of Miki, we used si-RNAs to downregulate Miki expression in HeLa and K562 cells, both of which show basically normal metaphase and nuclear morphology. Cells expressing Miki at reduced levels showed insufficient maturation and disturbed positioning of centrosomes, resulting in unorganized spindles including loss of spindle tension, curled and fragile spindles, or even completely disturbed spindle formation. Time-lapse observation revealed prometaphase and/or metaphase delay with unaligned or even totally scattered chromosomes in prometaphase in virtually all cells in the mitotic phase. As a result, cells underwent pre-anaphase arrest and exited mitosis in the absence of chromosome segregation or terminated mitosis by cell death. In the interphase, there were many cells with chromatid bridges and/or bi- or tri-nuclear or even multinuclear cells with micronuclei that resembled pathological cells routinely observed in the bone marrow pictures of MDS patients. Interestingly, myeloid cell lines with low Miki expression, including those with monosomy 7, generally showed abnormal mitosis such as scattered chromosomes and abnormal nuclear morphologies (multi-nuclear cells with small nuclei) at higher frequency than cell lines expressing Miki at high levels. Moreover, induction of Miki restores normal mitosis in leukemia cells with monosomy 7. Miki was poly(ADP-ribosyl)ated (PARsylated) in late G2 to M phase by tankyrase-1, one of PAR polymerase (PARP), and tankyrase-1 activity was required for the binding of Miki to spindles and centrosomes. These data suggest that loss of Miki gene contributes to the development and progression of MDS by disturbing mitosis.

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Strategies to Re-Express Epigenetically-Silenced Tumor Suppressor Genes Converge on the Requirement for Inhibition of the Histone Methyltransferase SUV39H1.

Blood ◽

10.1182/blood.v112.11.3357.3357 ◽

2008 ◽

Vol 112 (11) ◽

pp. 3357-3357

Author(s):

Asha Lakshmikuttyamma ◽

Stuart Scott ◽

David P. Sheridan ◽

John DeCoteau ◽

Ron Geyer

Keyword(s):

Tumor Suppressor ◽

Cell Lines ◽

Tumor Suppressor Genes ◽

Fold Increase ◽

Dna Demethylation ◽

Dna Hypermethylation ◽

Suppressor Genes ◽

Promoter Dna Methylation ◽

Promoter Dna ◽

E Cadherin

Abstract Gene silencing mediated by aberrant promoter DNA hypermethylation represents a key mechanism by which tumor suppressor gene expression is silenced in cancer and it is associated with multiple repressive histone modifications. Histone H3 lysine 9 (H3K9) methylation is a key repressive chromatin modification with important implications for regulating cell proliferation, differentiation, and gene expression. SUV39H1 is a methyltransferase that catalyzes the addition of trimethyl groups to H3K9. SUV39H1 is associated with regions of hypermethylated CpG islands, with repressive complexes, such as RB/E2F, and with DNA-binding proteins involved in leukemogenesis, such as AML1 and PML-RAR, where its H3K9 trimethylation activity promotes heterochromatin formation and gene silencing. We studied the requirement of SUV39H1 in the epigenetic silencing of heavily methylated tumor suppressor genes p15INK4B and E-cadherin in acute myeloid leukemia (AML). Treatment of AML cell lines AML193, KG1a, and Kasumi with the DNA methyltransferase (DNMT) inhibitor 5-Aza-2’-deoxycytidine (5-Aza-dC) induces p15INK4B and E-cadeherin re-expression in association with dramatic decreases in p15INK4B and E-cadherin promoter DNA methylation and marked reductions in the levels of SUV39H1 and H3K9 trimethylation at these promoters. Interestingly, treatment of these cell lines with SUV39H1 shRNA, or the SUV39H1 inhibitor chaetocin, also induces p15INK4B and E-cadherin re-expression and H3K9 demethylation, without affecting promoter DNA methylation. Thus, re-expression of hypermethylated tumor suppressors requires histone H3K9 demethylation, which can be achieved indirectly by decreasing the amount of SUV39H1 associated with the promoter using 5-Aza-dC, or directly by inhibiting SUV39H1 expression or activity without requiring promoter DNA demethylation. Furthermore, we found that SUV39H1 shRNA or chaetocin in combination with 5-Aza-dC acts synergistically to re-express epigenetically silenced p15INK4B and E-cadherin in AML cell lines. Treatment of primary human AML blasts obtained from two patients with combinations of 5-Aza-C and chaetocin also results in synergistic re-expression of p15INK4B and E-cadherin (2–6 fold increase with 5-Aza-C or chaetocin treatment vs. 11–14 fold increase with co-treatment). Our study has important implications for developing novel epigenetic therapies of relevance to AML as it suggests that the re-expression of tumor suppressor genes silenced by aberrant promoter DNA hypermethylation converges on the requirement for SUV39H1 and H3K9 methylation inhibition but not promoter DNA demethylation. Our finding that SUV39H1 inhibition may function synergistically with DNMT inhibitors to enhance gene reactivation and chromatin changes also highlights the needs for developing more inhibitors of histone methyltransferases and for performing detailed drug interaction studies to identify the best drug combinations for optimal epigenetic therapies.

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Genome-Wide Methylation Analysis of Primary Mantle Cell Lymphomas Identifies Novel Gene Targets for Epigenetic Drug Therapy.

Blood ◽

10.1182/blood.v114.22.673.673 ◽

2009 ◽

Vol 114 (22) ◽

pp. 673-673

Author(s):

Violetta Leshchenko ◽

Pei-Yu Kuo ◽

Rita Shaknovich ◽

Tobias Gellen ◽

Yvonne Remache ◽

...

Keyword(s):

Tumor Suppressor ◽

Cell Lines ◽

Tumor Suppressor Genes ◽

Gene Promoter ◽

Fold Increase ◽

Therapeutic Benefit ◽

Mrna Levels ◽

Gene Promoters ◽

Suppressor Genes ◽

Epigenetic Drug

Abstract Abstract 673 Mantle Cell Lymphoma (MCL) is an aggressive and incurable malignancy arising from naïve B cells (NBC) in the mantle zone of lymph node follicles. Murine models over-expressing Cyclin D1, the putative oncogene implicated in the majority of MCL, do not fully recapitulate the disease phenotype. We therefore hypothesize that there are additional mechanisms contributing to MCL pathogenesis and undertook an integrative approach by studying genome-wide DNA methylation and gene expression in primary MCL to uncover additional genes and pathways involved in MCL pathogenesis. We therefore compared and contrasted the DNA methylation levels of 14,000 gene promoters in MCL patients and normal tonsillar NBC controls using the HELP (HPA II tiny fragment Enrichment by Ligation mediated PCR) assay. All patient samples were obtained prior to any treatment from peripheral blood or apheresis specimens from newly diagnosed patients with histologically confirmed MCL. We found significant hypo-methylation of gene promoters in the MCL patients as compared to normal NBCs. Integrating genomic methylation data from HELP and gene expression data from Affymetrix U133 arrays, we determined a signature of differentially methylated genes with reciprocal changes in mRNA levels. Using pathway analysis and gene ontogeny, we selected genes for validation by choosing loci that were differentially methylated and fulfilling the following characteristics (i) demonstrating a clear methylation state change (from hypomethylated in normal B cells to methylated in MCL or vice-versa) using a threshold of 0.0 on the log ratio scale, (ii) Genes that function as tumor suppressors and were hypermethylated and suppressed in MCLs in our data (iii) Overexpressed/ hypomethylated genes with existing therapeutic options available or in clinical trial (iv) involved in pathways controlling biological processes with known relevance to MCL i.e. cell cycle control, apoptosis. Our panel included four differentially hypermethylated genes CDKN2B, MLF-1, PCDH8, HOXD8 and four differentially hypomethylated genes CD37, HDAC1, NOTCH1 and CDK5. MassArray Epityper analysis confirmed the presence of differential methylation at the promoter region of these genes, which was consistent between MCL patients and cell lines in all 8 genes studied. Remarkably, PCDH8 and CDKN2B have previously been shown to be silenced by methylation at their gene promoters and transfection of PCDH8 and CDKN2B have been shown to reduce tumor growth in breast cancer and MCL cell line models respectively. Based on these data, we hypothesized that the aberrantly hypermethylated and thereby silenced tumor suppressor genes in MCL could be pharmacologically induced by DNA hypomethylating agents and HDAC inhibitors for therapeutic benefit. We therefore next treated MCL cell lines MINO and Z138 with the DNA methyltransferase inhibitor Decitabine alone and in combination with the HDAC inhibitor SAHA. HELP analysis of MINO and Z138 cells treated with hypomethylating doses of decitabine (0.5uM × 3days) showed widespread reversal of aberrant gene promoter hypermethylation. Hypomethylation in these cell lines was accompanied with 3-7 fold increase in mRNA levels of tumor suppressor genes CDKN2B, MLF-1, PCDH8 and HOXD8. Concurrent treatment with SAHA (1 uM x 1 dose) synergized with Decitabine leading to 5-15 fold increase in mRNA of these tumor suppressor genes in Z138 cells. Importantly, treatment with Decitabine and SAHA as single agents decreased MCL cell viability by 60% and 40% respectively and the combination synergised in anti-MCL cytotoxicity with > 90% decrease in cell viability. In conclusion, our analysis shows prominent aberrant gene promoter methylation patterns in MCL genome and identifies novel differentially methylated and expressed genes in MCL cell lines and primary MCLs. Furthermore, we demonstrate that reversal of aberrant hypermethylated and silenced genes can be targeted for therapeutic benefit using epigenetic drugs in MCL. We are currently modeling our combination epigenetic drug therapy in primary MCL cells in culture and murine xenograft systems. We expect these results to support the development of clinical trials investigating the prospective use of combination epigenetic therapy in MCL. Disclosures: No relevant conflicts of interest to declare.

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Loss of Heterozygosity at the Ink4a/ArfLocus Facilitates Abelson Virus Transformation of Pre-B Cells

Journal of Virology ◽

10.1128/jvi.74.20.9479-9487.2000 ◽

2000 ◽

Vol 74 (20) ◽

pp. 9479-9487 ◽

Cited By ~ 4

Author(s):

Justin Mostecki ◽

Anne Halgren ◽

Arash Radfar ◽

Zohar Sachs ◽

James Ravitz ◽

...

Keyword(s):

B Cells ◽

Tumor Suppressor ◽

Loss Of Heterozygosity ◽

Cell Lines ◽

Tumor Suppressor Genes ◽

Single Copy ◽

Transformation Process ◽

Suppressor Genes ◽

Abelson Virus

ABSTRACT In many tumor systems, analysis of cells for loss of heterozygosity (LOH) has helped to clarify the role of tumor suppressor genes in oncogenesis. Two important tumor suppressor genes, p53 and the Ink4a/Arf locus, play central roles in the multistep process of Abelson murine leukemia virus (Ab-MLV) transformation. p53 and the p53 regulatory protein, p19Arf, are required for the apoptotic crisis that characterizes the progression of primary transformed pre-B cells to fully malignant cell lines. To search for other tumor suppressor genes which may be involved in the Ab-MLV transformation process, we used endogenous proviral markers and simple-sequence length polymorphism analysis to screen Abelson virus-transformed pre-B cells for evidence of LOH. Our survey reinforces the role of the p53-p19 regulatory pathway in transformation; 6 of 58 cell lines tested had lost sequences on mouse chromosome 4, including theInk4a/Arf locus. Consistent with this pattern, a high frequency of primary pre-B-cell transformants derived fromInk4a/Arf +/− mice became established cell lines. In addition, half of them retained the single copy of the locus when the transformation process was complete. These data demonstrate that a single copy of the Ink4a/Arf locus is not sufficient to fully mediate the effects of these genes on transformation.

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