Evolution of motif variants and positional bias of the cyclic-AMP response element

From National Research Council Canada

DOI	Resolve DOI: https://doi.org/10.1186/1471-2148-7-S1-S15
Author	Search for: Smith, Brandon¹; Search for: Fang, Hung¹; Search for: Pan, Youlian²; Search for: Walker, P. Roy¹; Search for: Famili, A. Fazel²; Search for: Sikorska, Marianna¹
Affiliation	National Research Council of Canada. NRC Institute for Biological Sciences National Research Council of Canada. NRC Institute for Information Technology
Format	Text, Article
Subject	base sequence; binding; binding sites; Canada; chromosome mapping; consensus sequence; CpG Islands; cyclic AMP; cyclic AMP response element-binding protein; deamination; difference; DNA; DNA methylation; evolution, molecular; gene; gene expression; genome; mammals; metabolism; methylation; protein; region; response elements; sequence; sequence analysis, DNA; sequences; site; transcription factors; variation (genetics)
Abstract	BACKGROUND: Transcription factors regulate gene expression by interacting with their specific DNA binding sites. Some transcription factors, particularly those involved in transcription initiation, always bind close to transcription start sites (TSS). Others have no such preference and are functional on sites even tens of thousands of base pairs (bp) away from the TSS.The Cyclic-AMP response element (CRE) binding protein (CREB) binds preferentially to a palindromic sequence (TGACGTCA), known as the canonical CRE, and also to other CRE variants. CREB can activate transcription at CREs thousands of bp away from the TSS, but in mammals CREs are found far more frequently within 1 to 150 bp upstream of the TSS than in any other region. This property is termed positional bias.The strength of CREB binding to DNA is dependent on the sequence of the CRE motif. The central CpG dinucleotide in the canonical CRE (TGACGTCA) is critical for strong binding of CREB dimers. Methylation of the cytosine in the CpG can inhibit binding of CREB. Deamination of the methylated cytosines causes a C to T transition, resulting in a functional, but lower affinity CRE variant, TGATGTCA. RESULTS: We performed genome-wide surveys of CREs in a number of species (from worm to human) and showed that only vertebrates exhibited a CRE positional bias. We performed pair-wise comparisons of human CREs with orthologous sequences in mouse, rat and dog genomes and found that canonical and TGATGTCA variant CREs are highly conserved in mammals. However, when orthologous sequences differ, canonical CREs in human are most frequently TGATGTCA in the other species and vice-versa. We have identified 207 human CREs showing such differences CONCLUSION: Our data suggest that the positional bias of CREs likely evolved after the separation of urochordata and vertebrata. Although many canonical CREs are conserved among mammals, there are a number of orthologous genes that have canonical CREs in one species but the TGATGTCA variant in another. These differences are likely due to deamination of the methylated cytosines in the CpG and may contribute to differential transcriptional regulation among orthologous genes
Publication date	2007-02-08
In	BMC Evolutionary Biology 7, no. Suppl 1 (8 February 2007): S15–.
Language	English
NRC number	SMITH2007A
NPARC number	9363345
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Record identifier	7ecf6fdf-64ca-4b50-acdb-3843929b6335
Record created	2009-07-10
Record modified	2020-05-10

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