Myc-binding-site recognition in the human genome is determined by chromatin context

被引:303
作者
Guccione, Ernesto
Martinato, Francesca
Finocchiaro, Giacomo
Luzi, Lucilla
Tizzoni, Laura
Dall'Olio, Valentina
Zardo, Giuseppe
Nervi, Clara
Bernard, Loris
Amati, Bruno
机构
[1] European Inst Oncol, Dept Expt Oncol, I-20139 Milan, Italy
[2] IFOM, FIRC, Inst Mol Oncol, I-20139 Milan, Italy
[3] Real Time PCR Facil, I-20139 Milan, Italy
[4] Univ Roma La Sapienza, Dept Cellular Biotechnol & Hematol, I-00128 Rome, Italy
[5] San Raffaele BioMed Pk Fdn, I-00128 Rome, Italy
[6] Univ Roma La Sapienza, Dept Histol & Med Embryol, Rome, Italy
关键词
D O I
10.1038/ncb1434
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Large-scale chromatin immunoprecipitation ( ChIP) studies have been effective in unravelling the distribution of DNA-binding transcription factors along eukaryotic genomes(1), but specificity determinants remain elusive. Gene-regulatory regions display distinct histone variants and modifications ( or marks)(2-15). An attractive hypothesis is that these marks modulate protein recognition(16-18), but whether or not this applies to transcription factors remains unknown. Based on large-scale datasets(2,19-21) and quantitative ChIP, we dissect the correlations between 35 histone marks and genomic binding by the transcription factor Myc. Our data reveal a relatively simple combinatorial organization of histone marks in human cells, with a few main groups of marks clustering on distinct promoter populations. A stretch of chromatin bearing high H3 K4/K79 methylation and H3 acetylation ( or 'euchromatic island'), which is generally associated with a pre-engaged basal transcription machinery(12,13), is a strict prerequisite for recognition of any target site by Myc ( whether the consensus CACGTG or an alternative sequence)(22). These data imply that tethering of a transcription factor to restricted chromatin domains is rate-limiting for sequence-specific DNA binding in vivo.
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收藏
页码:764 / U225
页数:10
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