Human DNA-(Cytosine-5) Methyltransferase-PCNA Complex as a Target for p21
            <sup>WAF1</sup>

Chuang, Linda S.-H.; Ian, Hang-In; Koh, Tong-Wey; Ng, Huck-Hui; Xu, Guoliang; Li, Benjamin F. L.

doi:10.1126/science.277.5334.1996

Cited by 850 publications

(623 citation statements)

References 34 publications

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“…DNMT1 is also recruited to nascent DNA by the essential cofactor UHRF1 (ubiquitin-like, with PHD and RING finger domains 1), which exhibits a high affinity for hemi-methylated DNA through its SRA domain 8,9 and ubiquitinates the histone H3 tail to facilitate DNMT1 recruitment 10 . DNMT1 activity is further directed to the replication fork through its interaction with the proliferating cell nuclear antigen (PCNA) DNA clamp 11 , and deletion of DNMT1s PCNA-binding domain has been reported to delay post replication remethylation 12 . More conceptually, accurate reestablishment of the human methylome requires catalytic activity at ~45 million heterogeneously distributed CpGs (roughly 80% of CpG sites within the diploid genome) that must be completed within a single cell cycle 13 .…”

Section: Introductionmentioning

confidence: 99%

Global delay in nascent strand DNA methylation

Charlton

Downing

Smith

et al. 2018

Nat Struct Mol Biol

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Cytosine methylation is widespread among organisms and essential for mammalian development. In line with early postulations of an epigenetic role in gene regulation, symmetric CpG methylation can be mitotically propagated over many generations with extraordinarily high fidelity. Here, we combine BrdU labeling and immunoprecipitation with genome-wide bisulfite sequencing to explore the inheritance of cytosine methylation onto newly replicated DNA in human cells. Globally, we observe a pronounced lag between the copying of genetic and epigenetic information that is reconsolidated within hours to accomplish faithful mitotic transmission. Populations of arrested cells show a global reduction of lag induced intermediate CpG methylation when compared to proliferating cells, while sites of transcription factor engagement appear cell-cycle invariant. Alternatively, the cancer cell line HCT116 preserves global epigenetic heterogeneity independently of cell-cycle arrest. Taken together, our data suggest that heterogeneous methylation largely reflects asynchronous proliferation, but is intrinsic to actively engaged cis-regulatory elements and cancer.

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Section: Introductionmentioning

confidence: 99%

Global delay in nascent strand DNA methylation

Charlton

Downing

Smith

et al. 2018

Nat Struct Mol Biol

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“…The cell cycle inhibitor p21 CIP1 can disrupt the association between DMT and PCNA, perhaps a ecting the activity of the two proteins (Chuang et al, 1997). Furthermore, levels of DMT and p21 proteins were inversely related in normal and SV-40 transformed human ®broblasts.…”

Section: Discussionmentioning

confidence: 99%

“…In contrast, PCNA expression did not vary greatly among the cell lines, and was not signi®cantly correlated with DMT expression. It has been suggested (Chuang et al, 1997) that the transforming e ect of DMT overexpression observed by others (Wu et al, 1993) may be due in part to the ability of DMT to compete with p21 for PCNA binding, thereby promoting the G 1 -S phase transition. By binding to PCNA in place of p21, excess DMT could increase the level of active cyclin-dependent kinases, promoting Rb phosphorylation and thus progression through the cell cycle.…”

Section: Discussionmentioning

confidence: 99%

“…A recent study reported that DMT can bind to PCNA (proliferating cell nuclear antigen), and that p21 CIP1 can disrupt the association between DMT and PCNA, possibly a ecting the activity of these proteins (Chuang et al, 1997). We therefore examined the levels of PCNA and p21 in the panel of ER-positive andnegative breast cancer cells (Figure 1).…”

Section: Dmt and P21 Are Inversely Correlated In Breast Cancer Cellsmentioning

confidence: 99%

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Expression of DNA methyl-transferase (DMT) and the cell cycle in human breast cancer cells

et al. 1999

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Estrogen receptor (ER)-negative breast cancer cells display extensive methylation of the ER gene CpG island and elevated DNA methyltransferase (DMT) expression compared to ER-positive cells. The present study demonstrates that DMT protein levels tightly correlate with S phase fraction in ER-positive cells, whereas ER-negative cells express DMT throughout the cell cycle. In addition, levels of p21 CIP1 , which disrupts DMT binding to PCNA, are inversely correlated with DMT levels. Therefore increased DMT expression in ER-negative cells is not simply due to elevated S-phase fraction, but rather to more complex changes that allow cells to escape normal cell cycle-dependent controls on DMT expression. Because ER-negative breast tumors often have activated growth factor pathways, the impact of these pathways on DMT expression was examined in ER-positive cells. Stable transfection with ®broblast growth factors (FGFs) 1 and 4 led to increased DMT expression that could not be accounted for by a shift in S phase fraction. Elevated DMT protein expression in FGF-transfectants was accompanied by a signi®cant decrease in p21, again suggesting a reciprocal relationship between these two proteins. However, acquisition of an estrogen-independent phenotype, even in conjunction with elevated DMT levels, was not su cient to promote ER gene silencing via methylation. These results indicate that multiple steps are required for de novo methylation of the ER CpG island.

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“…p21 has several cellular binding partners, including GADD45 damage response protein (Kearsey et al, 1995) and PCNA (Chen et al, 1995). The sequestration of PCNA by p21 from the replication machinery proteins inhibits DNA replication (Flores-Rozas et al, 1994) and interferes with the interaction of PCNA with DNA methyltransferases (Chuang et al, 1997). The loss of p21 leads to defective damage responses and loss of G 1 and mitotic checkpoint control (Brugarolas et al, 1995;Deng et al, 1995).…”

Section: Introductionmentioning

confidence: 99%

Ras induces p21Cip1/Waf1 cyclin kinase inhibitor transcriptionally through Sp1-binding sites

et al. 1999

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p21 Cip1/Waf1 cyclin-dependent kinase inhibitor (p21) is inducible by Raf and mitogen-activated protein kinase kinase (MAPKK), but the level of regulation is unknown. We show here by conditional and transient Rasexpression models that Ras induces p21. Induction of p21 in conditionally Ras-expressing cells is posttranscriptional utilizing mitogen-activated protein kinase (MAPK) pathway. Transient, high-level Ras-expression induces transcriptional activation of p21 mediated by a GC-rich region in p21 promoter -83-54 bp relative to the transcription initiation site containing binding sites for Sp1-family transcription factors. Mutation of either Sp1-binding site 2 or 4 in this region decreases the magnitude of induction of promoter activity by Ras, but only the simultaneous mutation of both sites abolishes fully the induction. Electrophoretic mobility shift assays using an oligonucleotide corresponding to Sp1-binding site 2 indicate that both Sp1 and Sp3 transcription factors bind to this region. The results demonstrate that the central cytosolic growth regulator Ras is a potent transcriptional and posttranscriptional inducer of the nuclear growth inhibitor p21.

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Human DNA-(Cytosine-5) Methyltransferase-PCNA Complex as a Target for p21 ^WAF1

Cited by 850 publications

References 34 publications

Global delay in nascent strand DNA methylation

Global delay in nascent strand DNA methylation

Expression of DNA methyl-transferase (DMT) and the cell cycle in human breast cancer cells

Ras induces p21Cip1/Waf1 cyclin kinase inhibitor transcriptionally through Sp1-binding sites

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Human DNA-(Cytosine-5) Methyltransferase-PCNA Complex as a Target for p21 WAF1

Cited by 850 publications

References 34 publications

Global delay in nascent strand DNA methylation

Global delay in nascent strand DNA methylation

Expression of DNA methyl-transferase (DMT) and the cell cycle in human breast cancer cells

Ras induces p21Cip1/Waf1 cyclin kinase inhibitor transcriptionally through Sp1-binding sites

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Human DNA-(Cytosine-5) Methyltransferase-PCNA Complex as a Target for p21 ^WAF1