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Mammalian promoters can be separated into two classes, conserved TATA box–enriched promoters, which initiate at a welldefined site, and more plastic, broad and evolvable CpG-rich promoters. We have sequenced tags corresponding to several hundred thousand transcription start sites (TSSs) in the mouse and human genomes, allowing precise analysis of the sequence architecture and evolution of distinct promoter classes. Different tissues and families of genes differentially use distinct types of promoters. Our tagging methods allow quantitative analysis of promoter usage in different tissues and show that differentially regulated alternative TSSs are a common feature in protein-coding genes and commonly generate alternative N termini. Among the TSSs, we identified new start sites associated with the majority of exons and with 3’ UTRs. These data permit genome-scale identification of tissue-specific promoters and analysis of the cis-acting elements associated with them.

Genome-wide analysis of mammalian promoter architecture and evolution / Carninci, P; Sandelin, A; Lenhard, B; Katayama, S; Shimokawa, K; Ponjavic, J; Semple, Ca; Taylor, Ms; Engström, Pg; Frith, Mc; Forrest, Ar; Alkema, Wb; Tan, Sl; Plessy, C; Kodzius, R; Ravasi, T; Kasukawa, T; Fukuda, S; KANAMORI KATAYAMA, M; Kitazume, Y; Kawaji, H; Kai, C; Nakamura, M; Konno, H; Nakano, K; MOTTAGUI TABAR, S; Arner, P; Chesi, A; Gustincich, Stefano; Persichetti, F; Suzuki, H; Grimmond, Sm; Wells, Ca; Orlando, V; Wahlestedt, C; Liu, Et; Harbers, M; Kawai, J; Bajic, Vb; Hume, Da; Hayashizaki, Y.. - In: NATURE GENETICS. - ISSN 1061-4036. - 38:(2006), pp. 626-635. [10.1038/ng1789]

Genome-wide analysis of mammalian promoter architecture and evolution

Gustincich, Stefano;
2006-01-01

Abstract

Mammalian promoters can be separated into two classes, conserved TATA box–enriched promoters, which initiate at a welldefined site, and more plastic, broad and evolvable CpG-rich promoters. We have sequenced tags corresponding to several hundred thousand transcription start sites (TSSs) in the mouse and human genomes, allowing precise analysis of the sequence architecture and evolution of distinct promoter classes. Different tissues and families of genes differentially use distinct types of promoters. Our tagging methods allow quantitative analysis of promoter usage in different tissues and show that differentially regulated alternative TSSs are a common feature in protein-coding genes and commonly generate alternative N termini. Among the TSSs, we identified new start sites associated with the majority of exons and with 3’ UTRs. These data permit genome-scale identification of tissue-specific promoters and analysis of the cis-acting elements associated with them.
2006
NATURE GENETICS
38
626
635
Carninci, P; Sandelin, A; Lenhard, B; Katayama, S; Shimokawa, K; Ponjavic, J; Semple, Ca; Taylor, Ms; Engström, Pg; Frith, Mc; Forrest, Ar; Alkema, Wb; Tan, Sl; Plessy, C; Kodzius, R; Ravasi, T; Kasukawa, T; Fukuda, S; KANAMORI KATAYAMA, M; Kitazume, Y; Kawaji, H; Kai, C; Nakamura, M; Konno, H; Nakano, K; MOTTAGUI TABAR, S; Arner, P; Chesi, A; Gustincich, Stefano; Persichetti, F; Suzuki, H; Grimmond, Sm; Wells, Ca; Orlando, V; Wahlestedt, C; Liu, Et; Harbers, M; Kawai, J; Bajic, Vb; Hume, Da; Hayashizaki, Y.
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/20.500.11767/16237
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