Epigenome analyses using BAC microarrays identify evolutionary conservation of tissue-specific methylation of SHANK3

CpG islands are present in one-half of all human and mouse genes and typically overlap with promoters or exons. We developed a method for high-resolution analysis of the methylation status of CpG islands genome-wide, using arrays of BAC clones and the methylation-sensitive restriction enzyme NotI. H...

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Veröffentlicht in:Nature genetics 2005-06, Vol.37 (6), p.645-651
Hauptverfasser: Costello, Joseph F, Ching, Tsui-Ting, Maunakea, Alika K, Jun, Peter, Hong, Chibo, Zardo, Giuseppe, Pinkel, Daniel, Albertson, Donna G, Fridlyand, Jane, Mao, Jian-Hua, Shchors, Ksenya, Weiss, William A
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Sprache:eng
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Zusammenfassung:CpG islands are present in one-half of all human and mouse genes and typically overlap with promoters or exons. We developed a method for high-resolution analysis of the methylation status of CpG islands genome-wide, using arrays of BAC clones and the methylation-sensitive restriction enzyme NotI. Here we demonstrate the accuracy and specificity of the method. By computationally mapping all NotI sites, methylation events can be defined with single-nucleotide precision throughout the genome. We also demonstrate the unique expandability of the array method using a different methylation-sensitive restriction enzyme, BssHII. We identified and validated new CpG island loci that are methylated in a tissue-specific manner in normal human tissues. The methylation status of the CpG islands is associated with gene expression for several genes, including SHANK3, which encodes a structural protein in neuronal postsynaptic densities. Defects in SHANK3 seem to underlie human 22q13 deletion syndrome. Furthermore, these patterns for SHANK3 are conserved in mice and rats.
ISSN:1061-4036
1546-1718
DOI:10.1038/ng1563