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© 2003 The American Society for Nutritional Sciences J. Nutr. 133:3740S-3747S, November 2003


Supplement: International Research Conference on Food, Nutrition, and Cancer

Mechanisms of DNA Damage, DNA Hypomethylation, and Tumor Progression in the Folate/Methyl-Deficient Rat Model of Hepatocarcinogenesis1

S. Jill James*,2, Igor P. Pogribny{dagger}, Marta Pogribna{dagger}, Barbara J. Miller{dagger}, Stefanie Jernigan* and Stepan Melnyk*

* Department of Pediatrics, University of Arkansas for Medical Sciences, Little Rock, AR 72202 and {dagger} Division of Biochemical Toxicology, National Center for Toxicological Research, Jefferson, AR 72079

2 To whom correspondence should be addressed. E-mail: jamesjill{at}uams.edu.

Using the folate/methyl-deficient rat model of hepatocarcinogenesis, we obtained evidence that may provide new insights into a major unresolved paradox in DNA methylation and cancer research: the mechanistic basis for genome-wide hypomethylation despite an increase in DNA methyltransferase activity and gene-specific regional hypermethylation. Previous studies revealed that the methyltransferase binds with higher affinity to DNA strand breaks, gaps, abasic sites, and uracil than it does to its cognate hemimethylated CpG sites, consistent with its ancestral function as a DNA repair enzyme. These same DNA lesions are an early occurrence in models of folate and methyl deficiency and are often present in human preneoplastic cells. We hypothesized that the high-affinity binding of the maintenance DNA methyltransferase to unrepaired lesions in DNA could sequester available enzyme away from the replication fork and promote passive replication-dependent demethylation. In support of this possibility, we found that lesion-containing DNA is less efficiently methylated than lesion-free DNA from folate/methyl-deficient rats and that an increase in DNA strand breaks precedes DNA hypomethylation. Despite an adaptive increase in DNA methyltransferase activity, hemimethylated DNA from folate/methyl-deficient rats is progressively replaced by double-stranded unmethylated DNA that is resistant to remethylation with dietary methyl repletion. In promoter regions, the inappropriate binding of the DNA methyltransferase to unrepaired lesions or mispairs may promote local histone deacetylation, methylation, and regional hypermethylation associated with tumor suppressor gene silencing. These insights in an experimental model are consistent with the possibility that DNA lesions may be a necessary prerequisite for the disruption of normal DNA methylation patterns in preneoplastic and neoplastic cells.


KEY WORDS: • folate deficiency • methyl deficiency • DNA methylation • hepatocarcinogenesis • DNA strand breaks • uracil • deoxynucleotides




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