double strand breaks can initiate gene silencing and sirt1-dependent onset of dna methylation in an exogenous promoter cpg island可以启动基因沉默和sirt1-dependent双链断裂的dna甲基化在一个外生发起人cpg岛.pdfVIP
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double strand breaks can initiate gene silencing and sirt1-dependent onset of dna methylation in an exogenous promoter cpg island可以启动基因沉默和sirt1-dependent双链断裂的dna甲基化在一个外生发起人cpg岛
Double Strand Breaks Can Initiate Gene Silencing and
SIRT1-Dependent Onset of DNA Methylation in an
Exogenous Promoter CpG Island
Heather M. O’Hagan, Helai P. Mohammad, Stephen B. Baylin*
The Sidney Kimmel Comprehensive Cancer Center at Johns Hopkins, Baltimore, Maryland, United States of America
Abstract
Chronic exposure to inducers of DNA base oxidation and single and double strand breaks contribute to tumorigenesis. In
addition to the genetic changes caused by this DNA damage, such tumors often contain epigenetically silenced genes with
aberrant promoter region CpG island DNA hypermethylation. We herein explore the relationships between such DNA
damage and epigenetic gene silencing using an experimental model in which we induce a defined double strand break in
an exogenous promoter construct of the E-cadherin CpG island, which is frequently aberrantly DNA hypermethylated in
epithelial cancers. Following the onset of repair of the break, we observe recruitment to the site of damage of key proteins
involved in establishing and maintaining transcriptional repression, namely SIRT1, EZH2, DNMT1, and DNMT3B, and the
appearance of the silencing histone modifications, hypoacetyl H4K16, H3K9me2 and me3, and H3K27me3. Although in most
cells selected after the break, DNA repair occurs faithfully with preservation of activity of the promoter, a small percentage
of the plated cells demonstrate induction of heritable silencing. The chromatin around the break site in such a silent clone is
enriched for most of the above silent chromatin proteins and histone marks, and the region harbors the appearance of
increasing DNA methylation in the CpG island of the promoter. During the acute break, SIRT1 appears to be required for the
transient recruitment of DNMT3B and subsequent methylation of the promoter in the silent clones. Taken together, our
data suggest th
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