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Query: UMLS:C0009402 (
colorectal cancer
)
53,228
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The molecular basis of aberrant hypermethylation of CpG islands observed in a subset of human colorectal tumors is unknown. One potential mechanism is the up-regulation of DNA (cytosine-5)-methyltransferases. Recently, two new mammalian DNA methyltransferase genes have been identified, which are referred to as DNMT3A and DNMT3B. The encoded proteins differ from the predominant mammalian DNA methyltransferase
DNMT1
in that they have a substantially higher ratio of de novo to maintenance methyltransferase activity. We have used a highly quantitative 5' nuclease fluorogenic reverse transcription-PCR method (TaqMan) to analyze the expression of all three DNA methyltransferase genes in 25 individual colorectal adenocarcinoma specimens and matched normal mucosa samples. In addition, we examined the methylation patterns of four CpG islands [APC, ESR1 (estrogen receptor), CDKN2A (p16), and MLH1] to determine whether individual tumors show a positive correlation between the level of DNA methyltransferase expression and the frequency of CpG island hypermethylation. All three methyltransferases appear to be up-regulated in tumors when RNA levels are normalized using either ACTB (beta-actin) or POLR2A (RNA pol II large subunit), but not when RNA levels are normalized with proliferation-associated genes, such as H4F2 (histone H4) or PCNA. The frequency or extent of CpG island hypermethylation in individual tumors did not correlate with the expression of any of the three DNA methyltransferases. Our results suggest that deregulation of DNA methyltransferase gene expression does not play a role in establishing tumor-specific abnormal DNA methylation patterns in human
colorectal cancer
.
...
PMID:CpG island hypermethylation in human colorectal tumors is not associated with DNA methyltransferase overexpression. 1034 33
Somatic changes in CpG dinucleotide methylation occur quite commonly in human cancer cell DNA. Relative to DNA from normal human colonic cells, DNA from human
colorectal cancer
cells typically displays regional CpG dinucleotide hypermethylation amid global CpG dinucleotide hypomethylation. The role of the maintenance DNA methyltransferase (
DNMT1
) in the acquisition of such abnormal CpG dinucleotide methylation changes in
colorectal cancer
cells remains controversial; in one study, 60-200-fold increases in
DNMT1
mRNA expression were detected in colorectal polyps and cancers relative to normal colonic tissue [W. S. El-Deiry et al., Proc. Natl. Acad. Sci. USA, 88: 3470-3474, 1991], whereas in another study, only small increases in
DNMT1
mRNA expression, commensurate with differences in cell proliferation accompanying colonic tumorigenesis, were observed [P. J. Lee et al., Proc. Natl. Acad. Sci. USA, 93: 10366-10370, 1996]. To definitively ascertain whether abnormal
DNMT1
expression might accompany human colorectal carcinogenesis, we subjected a series of normal and neoplastic colonic tissues to immunohistochemical staining using a polyclonal antiserum raised against a
DNMT1
polypeptide. A concordance of
DNMT1
expression with the expression of PCNA and other cell proliferation markers, such as Ki-67 and DNA topoisomerase IIalpha, was observed in normal colonic epithelial cells and in cells comprising other normal epithelia and lymphoid tissues. The polypeptide p21, which has been reported to undermine
DNMT1
binding to proliferating cell nuclear antigen at DNA replication sites, was not expressed by normal colonic cells containing
DNMT1
and other cell proliferation markers. In adenomatous polyps, although
DNMT1
expression coincided with the expression of other cell proliferation markers, many
DNMT1
-expressing cells also expressed p21. The fidelity of
DNMT1
expression was further undermined in colorectal carcinomas, in which a striking heterogeneity in
DNMT1
expression, with some carcinoma cells containing very high
DNMT1
levels and others containing very low
DNMT1
levels, was observed. These results indicate that human colorectal carcinogenesis is accompanied by a progressive dysregulation of
DNMT1
expression and suggest that abnormalities in
DNMT1
expression may contribute to the abnormal CpG dinucleotide methylation changes characteristic of human colorectal carcinoma cell DNA.
...
PMID:Abnormal regulation of DNA methyltransferase expression during colorectal carcinogenesis. 1046 69
Inactivation of tumour suppressor genes is central to the development of all common forms of human cancer. This inactivation often results from epigenetic silencing associated with hypermethylation rather than intragenic mutations. In human cells, the mechanisms underlying locus-specific or global methylation patterns remain unclear. The prototypic DNA methyltransferase, Dnmt1, accounts for most methylation in mouse cells, but human cancer cells lacking
DNMT1
retain significant genomic methylation and associated gene silencing. We disrupted the human DNMT3b gene in a
colorectal cancer
cell line. This deletion reduced global DNA methylation by less than 3%. Surprisingly, however, genetic disruption of both
DNMT1
and DNMT3b nearly eliminated methyltransferase activity, and reduced genomic DNA methylation by greater than 95%. These marked changes resulted in demethylation of repeated sequences, loss of insulin-like growth factor II (IGF2) imprinting, abrogation of silencing of the tumour suppressor gene p16INK4a, and growth suppression. Here we demonstrate that two enzymes cooperatively maintain DNA methylation and gene silencing in human cancer cells, and provide compelling evidence that such methylation is essential for optimal neoplastic proliferation.
...
PMID:DNMT1 and DNMT3b cooperate to silence genes in human cancer cells. 1193 49
Epigenomic changes in DNA methylation patterns are evident in a variety of cancers, including
colorectal cancer
(
CRC
). In addition, a large proportion of
CRC
tumors and cell lines harbor genetic mutations in the APC/beta-catenin/TCF transcription activation pathway. While several target genes have been proposed, a causal downstream agent between APC mutation and cancer has not been fully established. Because previous work implicates DNA methyltransferase (DMNT1) as a critical point in tumorigenesis and recent studies suggest that familial
CRC
also exhibits epigenetic alterations, we sought to investigate whether this gene might be regulated by APC in
CRC
. Reconstitution of wild type APC in HT-29
CRC
cell lines reduced the expression of both a reporter gene driven by the minimal
DNMT1
promoter and
DNMT1
mRNA that is independent of cell growth stasis. We also provide evidence for a causal role of
DNMT1
in
CRC
by demonstrating that antisense-driven reduction of
DNMT1
mRNA inhibits anchorage-independent growth, an indicator of tumorigenesis, of
CRC
cells. These data support future consideration of
DNMT1
as a target in the treatment of
CRC
.
...
PMID:Human DNA methyltransferase gene DNMT1 is regulated by the APC pathway. 1253 44
Hypermethylation associated silencing of the CpG islands of tumor suppressor genes is a common hallmark of human cancer. Here we report a functional search for hypermethylated CpG islands using the
colorectal cancer
cell line HCT-116, in which two major DNA methyltransferases,
DNMT1
and DNMT3b, have been genetically disrupted (DKO cells). Using two molecular screenings for differentially methylated loci [differential methylation hybridization (DMH) and amplification of inter-methylated sites (AIMS)], we found that DKO cells, but not the single
DNMT1
or DNMT3b knockouts, have a massive loss of hypermethylated CpG islands that induces the re-activation of the contiguous genes. We have characterized a substantial number of these CpG island associated genes with potentially important roles in tumorigenesis, such as the cadherin member FAT, or the homeobox genes LMX-1 and DUX-4. For other genes whose role in transformation has not been characterized, such as the calcium channel alpha1I or the thromboxane A2 receptor, their re-introduction in DKO cells inhibited colony formation. Thus, our results demonstrate the role of
DNMT1
and DNMT3b in CpG island methylation associated silencing and the usefulness of genetic disruption strategies in searching for new hypermethylated loci.
...
PMID:Genetic unmasking of epigenetically silenced tumor suppressor genes in colon cancer cells deficient in DNA methyltransferases. 1291 69
Chemotherapy using DNA intercalators is one of the most successful approaches to cancer treatment. Although DNA intercalators are believed to inhibit DNA polymerases and topoisomerases, resulting in the induction of apoptosis in tumor cells, other factors potentially inhibited by the anthracycline antibiotics remain to be elucidated. Herein, we show that the enzymatic activity of
DNMT1
, the primary DNA methyltransferase in mammalian cells, is inhibited by DNA intercalators, such as doxorubicin, in an in vitro assay. Enzymatic analyses indicate that doxorubicin inhibits the catalytic activity of
DNMT1
via DNA intercalation. We also found that apoptosis was induced in
DNMT1
(+/+) HCT116 cells by only a limited range of doxorubicin dose, meaning that apoptotic cell death is "conditional" with respect to the concentration of the DNA intercalating drug. It is noteworthy that conditional apoptosis is not observed in human
colorectal cancer
cells lacking
DNMT1
but can be induced in
DNMT1
(-/-) cells by transfection of a plasmid expressing
DNMT1
. Our results suggest that
DNMT1
is one of the major targets of doxorubicin resulting in drug-induced apoptosis in human cancer cells. We propose that expression levels of
DNMT1
in tumor cells may affect the effectiveness of doxorubicin in chemotherapy.
...
PMID:Doxorubicin inhibits DNMT1, resulting in conditional apoptosis. 1534 41
DNA methyltransferase 1
(
DNMT1
)-deficient mice are tumor-prone, and this has been proposed to result from the induction of genomic instability. To address whether loss of
DNMT1
, or the related protein DNMT3b, results in genomic instability in human cancer cells, we used a near-diploid human
colorectal cancer
cell line, HCT116, in which one or both
DNMT
genes were disrupted by homologous recombination. Array-based comparative genomic hybridization analyses indicated that double, but not single,
DNMT
knock-out cells display two specific alterations in regional DNA copy number, suggesting that
DNMT
deficiency and genomic DNA hypomethylation are not associated with widespread genomic amplifications or deletions in human cancer cells. However, spectral karyotype analyses revealed that
DNMT
-deficient HCT116 cells are highly unstable with respect to large-scale chromosomal alterations; furthermore, this effect is characterized by a high degree of individual cell heterogeneity. The induction of chromosomal alterations in
DNMT
-deficient cells was evidenced both by aneuploidy and by large increases in the number of novel chromosomal translocations. Studies of double knock-out cells indicated that the generation of chromosomal alterations is spontaneous and persistent in vitro, meeting the formal definition of genomic instability. In summary, we show that
DNMT
deficiency in human cancer cells results in constitutive genomic instability manifested by chromosomal translocations.
...
PMID:Genetic disruption of cytosine DNA methyltransferase enzymes induces chromosomal instability in human cancer cells. 1620 30
CpG island hypermethylation occurs in most cases of cancer, typically resulting in the transcriptional silencing of critical cancer genes. Procainamide has been shown to inhibit DNA methyltransferase activity and reactivate silenced gene expression in cancer cells by reversing CpG island hypermethylation. We report here that procainamide specifically inhibits the hemimethylase activity of
DNA methyltransferase 1
(
DNMT1
), the mammalian enzyme thought to be responsible for maintaining DNA methylation patterns during replication. At micromolar concentrations, procainamide was found to be a partial competitive inhibitor of
DNMT1
, reducing the affinity of the enzyme for its two substrates, hemimethylated DNA and S-adenosyl-l-methionine. By doing so, procainamide significantly decreased the processivity of
DNMT1
on hemimethylated DNA. Procainamide was not a potent inhibitor of the de novo methyltransferases DNMT3a and DNMT3b2. As further evidence of the specificity of procainamide for
DNMT1
, procainamide failed to lower genomic 5-methyl-2'-deoxycytidine levels in HCT116
colorectal cancer
cells when
DNMT1
was genetically deleted but significantly reduced genomic 5-methyl-2'-deoxycytidine content in parental HCT116 cells and in HCT116 cells where DNMT3b was genetically deleted. Because many reports have strongly linked
DNMT1
with epigenetic alterations in carcinogenesis, procainamide may be a useful drug in the prevention of cancer.
...
PMID:Procainamide is a specific inhibitor of DNA methyltransferase 1. 1623 Mar 60
DNA methylation is an epigenetic mechanism involved in transcriptional silencing of imprinted genes, genes located on the inactive X chromosome, and a number of tumour suppressor genes in cancer. MBD (methyl-CpG-binding domain) proteins selectively bind to methylated DNA and recruit chromatin remodelling and transcriptional repressor complexes, thereby establishing a repressive chromatin state. MBD2, a member of the MBD protein family, binds to methylated promoter CpG islands (clusters of high-density CpG dinucleotides) and acts as a methylation-dependent transcriptional repressor. Previous work has demonstrated that decreased CpG island methylation in mice lacking the DNA methyltransferase
DNMT1
is associated with impaired tumorigenesis when crossed on the tumour-susceptible Apc(Min/+) background. Mbd2 deficiency also dramatically reduces adenoma burden and extends life span in a gene dosage-dependent manner in this mouse model. Mbd2 is therefore essential for tumorigenesis in the murine intestine, although it is dispensable for the viability of the host animals. These findings validate MBD2 as a potential target for therapeutic intervention in
colorectal cancer
.
...
PMID:Role of MBD2 in gene regulation and tumorigenesis. 1624 64
Previous work has shown that DNA hypermethylation of tumor suppressor genes in
colorectal cancer
cells may be maintained in the absence of the major mammalian methyltransferase,
DNA methyltransferase 1
(
DNMT1
). In an effort to dissect the dependency on
DNMT1
to maintain such hypermethylation in different cancer types, we performed a systematic analysis of depletion of
DNMT1
in colorectal (SW48), bladder (T24), and breast (T47D) cancer cells by
DNMT1
-specific small hairpin RNA (shRNA) targeting. We show that although
DNMT1
-deficient SW48 and T24 cells exhibited no observable growth defects and were able to maintain promoter hypermethylation,
DNMT1
-deficient T47D breast cells failed to form comparable numbers of colonies when stably selected for the incorporation of the
DNMT1
-specific shRNA expression vector, suggesting a growth defect with reduced levels of
DNMT1
. Further treatment of T47D cells with transient transfection of small interfering RNA targeting
DNMT1
revealed that severely
DNMT1
-deficient T47D cells could not fully maintain promoter hypermethylation, and gene silencing was partially reversed at two of the three assayed loci. These observations suggest that human cancer cells may differ in their reliance on
DNMT1
for maintaining DNA methylation.
...
PMID:Differential requirement for DNA methyltransferase 1 in maintaining human cancer cell gene promoter hypermethylation. 1642 2
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