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Gain of DNA methylation is enhanced in the absence of CTCF at the human retinoblastoma gene promoter

Author: A Doi
A Huarte
AC Bell
B Joseph
Christian Valdes-Quezada
D Farrar
D Garrick
DJ Simpson
DT Butcher
E Soto-Reyes
Edgar González-Buendía
Erandi Ayala-Ortega
F Mohn
F Recillas-Targa
F Recillas-Targa
FJ Calero-Nieto
Félix Recillas-Targa
IA De La Rosa-Velázquez
JE Phillips
JP Issa
KD Robertson
KM McGarvey
KM McGarvey
M Nakamura
M Weber
M Witcher
Mayra Furlan-Magaril
Mercedes Dávalos-Salas
MW Coolen
N Ohtani-Fujita
NP Gomes
P Szabó
PA Jones
R Jothi
RA Gupsta
T Bose
T Guastafierro
VK Tiwari
Y Kondo
Y Kondo
Z Jiang
Publication venue: BioMed Central
Publication date: 01/01/2011
Field of study

Abstract Background Long-term gene silencing throughout cell division is generally achieved by DNA methylation and other epigenetic processes. Aberrant DNA methylation is now widely recognized to be associated with cancer and other human diseases. Here we addressed the contribution of the multifunctional nuclear factor CTCF to the epigenetic regulation of the human <it>retinoblastoma </it>(<it>Rb</it>) gene promoter in different tumoral cell lines. Methods To assess the DNA methylation status of the <it>Rb </it>promoter, genomic DNA from stably transfected human erythroleukemic K562 cells expressing a <it>GFP </it>reporter transgene was transformed with sodium bisulfite, and then PCR-amplified with modified primers and sequenced. Single- and multi-copy integrants with the CTCF binding site mutated were isolated and characterized by Southern blotting. Silenced transgenes were reactivated using 5-aza-2'-deoxycytidine and Trichostatin-A, and their expression was monitored by fluorescent cytometry. <it>Rb </it>gene expression and protein abundance were assessed by RT-PCR and Western blotting in three different glioma cell lines, and DNA methylation of the promoter region was determined by sodium bisulfite sequencing, together with CTCF dissociation and methyl-CpG-binding protein incorporation by chromatin immunoprecipitation assays. Results We found that the inability of CTCF to bind to the <it>Rb </it>promoter causes a dramatic loss of gene expression and a progressive gain of DNA methylation. Conclusions This study indicates that CTCF plays an important role in maintaining the <it>Rb </it>promoter in an optimal chromatin configuration. The absence of CTCF induces a rapid epigenetic silencing through a progressive gain of DNA methylation. Consequently, CTCF can now be seen as one of the epigenetic components that allows the proper configuration of tumor suppressor gene promoters. Its aberrant dissociation can then predispose key genes in cancer cells to acquire DNA methylation and epigenetic silencing.</p

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