Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs

Using full-length cDNA sequences, we compared alternative splicing (AS) in humans and mice. The alignment of the human and mouse genomes showed that 86% of 199 426 total exons in human AS variants were conserved in the mouse genome. Of the 20 392 total human AS variants, however, 59% consisted of al...

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Autores principales: Takeda, Jun-ichi, Suzuki, Yutaka, Sakate, Ryuichi, Sato, Yoshiharu, Seki, Masahide, Irie, Takuma, Takeuchi, Nono, Ueda, Takuya, Nakao, Mitsuteru, Sugano, Sumio, Gojobori, Takashi, Imanishi, Tadashi
Formato: Texto
Lenguaje:English
Publicado: Oxford University Press 2008
Materias:
Genomics
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2582632/
https://www.ncbi.nlm.nih.gov/pubmed/18838389
http://dx.doi.org/10.1093/nar/gkn677
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author Takeda, Jun-ichi
Suzuki, Yutaka
Sakate, Ryuichi
Sato, Yoshiharu
Seki, Masahide
Irie, Takuma
Takeuchi, Nono
Ueda, Takuya
Nakao, Mitsuteru
Sugano, Sumio
Gojobori, Takashi
Imanishi, Tadashi
author_facet Takeda, Jun-ichi
Suzuki, Yutaka
Sakate, Ryuichi
Sato, Yoshiharu
Seki, Masahide
Irie, Takuma
Takeuchi, Nono
Ueda, Takuya
Nakao, Mitsuteru
Sugano, Sumio
Gojobori, Takashi
Imanishi, Tadashi
author_sort Takeda, Jun-ichi
collection PubMed
description Using full-length cDNA sequences, we compared alternative splicing (AS) in humans and mice. The alignment of the human and mouse genomes showed that 86% of 199 426 total exons in human AS variants were conserved in the mouse genome. Of the 20 392 total human AS variants, however, 59% consisted of all conserved exons. Comparing AS patterns between human and mouse transcripts revealed that only 431 transcripts from 189 loci were perfectly conserved AS variants. To exclude the possibility that the full-length human cDNAs used in the present study, especially those with retained introns, were cloning artefacts or prematurely spliced transcripts, we experimentally validated 34 such cases. Our results indicate that even retained-intron type transcripts are typically expressed in a highly controlled manner and interact with translating ribosomes. We found non-conserved AS exons to be predominantly outside the coding sequences (CDSs). This suggests that non-conserved exons in the CDSs of transcripts cause functional constraint. These findings should enhance our understanding of the relationship between AS and species specificity of human genes.
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spelling pubmed-25826322008-11-13 Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs Takeda, Jun-ichi Suzuki, Yutaka Sakate, Ryuichi Sato, Yoshiharu Seki, Masahide Irie, Takuma Takeuchi, Nono Ueda, Takuya Nakao, Mitsuteru Sugano, Sumio Gojobori, Takashi Imanishi, Tadashi Nucleic Acids Res Genomics Using full-length cDNA sequences, we compared alternative splicing (AS) in humans and mice. The alignment of the human and mouse genomes showed that 86% of 199 426 total exons in human AS variants were conserved in the mouse genome. Of the 20 392 total human AS variants, however, 59% consisted of all conserved exons. Comparing AS patterns between human and mouse transcripts revealed that only 431 transcripts from 189 loci were perfectly conserved AS variants. To exclude the possibility that the full-length human cDNAs used in the present study, especially those with retained introns, were cloning artefacts or prematurely spliced transcripts, we experimentally validated 34 such cases. Our results indicate that even retained-intron type transcripts are typically expressed in a highly controlled manner and interact with translating ribosomes. We found non-conserved AS exons to be predominantly outside the coding sequences (CDSs). This suggests that non-conserved exons in the CDSs of transcripts cause functional constraint. These findings should enhance our understanding of the relationship between AS and species specificity of human genes. Oxford University Press 2008-11 2008-10-05 /pmc/articles/PMC2582632/ /pubmed/18838389 http://dx.doi.org/10.1093/nar/gkn677 Text en © 2008 The Author(s) http://creativecommons.org/licenses/by-nc/2.0/uk/ This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/2.0/uk/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Genomics
Takeda, Jun-ichi
Suzuki, Yutaka
Sakate, Ryuichi
Sato, Yoshiharu
Seki, Masahide
Irie, Takuma
Takeuchi, Nono
Ueda, Takuya
Nakao, Mitsuteru
Sugano, Sumio
Gojobori, Takashi
Imanishi, Tadashi
Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs
title Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs
title_full Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs
title_fullStr Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs
title_full_unstemmed Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs
title_short Low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cDNAs
title_sort low conservation and species-specific evolution of alternative splicing in humans and mice: comparative genomics analysis using well-annotated full-length cdnas
topic Genomics
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2582632/
https://www.ncbi.nlm.nih.gov/pubmed/18838389
http://dx.doi.org/10.1093/nar/gkn677
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