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Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb

In mammals, an array of MEF2C proteins is generated by alternative splicing (AS), yet specific functions have not been ascribed to each isoform. Teleost fish possess two MEF2C paralogues, mef2ca and mef2cb. In zebrafish, the Mef2cs function to promote cardiomyogenic differentiation and myofibrilloge...

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Autores principales: Ganassi, M., Badodi, S., Polacchini, A., Baruffaldi, F., Battini, R., Hughes, S.M., Hinits, Y., Molinari, S.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier Pub. Co 2014
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4064114/
https://www.ncbi.nlm.nih.gov/pubmed/24844180
http://dx.doi.org/10.1016/j.bbagrm.2014.05.003
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author Ganassi, M.
Badodi, S.
Polacchini, A.
Baruffaldi, F.
Battini, R.
Hughes, S.M.
Hinits, Y.
Molinari, S.
author_facet Ganassi, M.
Badodi, S.
Polacchini, A.
Baruffaldi, F.
Battini, R.
Hughes, S.M.
Hinits, Y.
Molinari, S.
author_sort Ganassi, M.
collection PubMed
description In mammals, an array of MEF2C proteins is generated by alternative splicing (AS), yet specific functions have not been ascribed to each isoform. Teleost fish possess two MEF2C paralogues, mef2ca and mef2cb. In zebrafish, the Mef2cs function to promote cardiomyogenic differentiation and myofibrillogenesis in nascent skeletal myofibers. We found that zebrafish mef2ca and mef2cb are alternatively spliced in the coding exons 4–6 region and these splice variants differ in their biological activity. Of the two, mef2ca is more abundantly expressed in developing skeletal muscle, its activity is tuned through zebrafish development by AS. By 24 hpf, we found the prevalent expression of the highly active full length protein in differentiated muscle in the somites. The splicing isoform of mef2ca that lacks exon 5 (mef2ca 4–6), encodes a protein that has 50% lower transcriptional activity, and is found mainly earlier in development, before muscle differentiation. mef2ca transcripts including exon 5 (mef2ca 4–5–6) are present early in the embryo. Over-expression of this isoform alters the expression of genes involved in early dorso-ventral patterning of the embryo such as chordin, nodal related 1 and goosecoid, and induces severe developmental defects. AS of mef2cb generates a long splicing isoform in the exon 5 region (Mef2cbL) that predominates during somitogenesis. Mef2cbL contains an evolutionarily conserved domain derived from exonization of a fragment of intron 5, which confers the ability to induce ectopic muscle in mesoderm upon over-expression of the protein. Taken together, the data show that AS is a significant regulator of Mef2c activity.
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spelling pubmed-40641142014-07-01 Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb Ganassi, M. Badodi, S. Polacchini, A. Baruffaldi, F. Battini, R. Hughes, S.M. Hinits, Y. Molinari, S. Biochim Biophys Acta Article In mammals, an array of MEF2C proteins is generated by alternative splicing (AS), yet specific functions have not been ascribed to each isoform. Teleost fish possess two MEF2C paralogues, mef2ca and mef2cb. In zebrafish, the Mef2cs function to promote cardiomyogenic differentiation and myofibrillogenesis in nascent skeletal myofibers. We found that zebrafish mef2ca and mef2cb are alternatively spliced in the coding exons 4–6 region and these splice variants differ in their biological activity. Of the two, mef2ca is more abundantly expressed in developing skeletal muscle, its activity is tuned through zebrafish development by AS. By 24 hpf, we found the prevalent expression of the highly active full length protein in differentiated muscle in the somites. The splicing isoform of mef2ca that lacks exon 5 (mef2ca 4–6), encodes a protein that has 50% lower transcriptional activity, and is found mainly earlier in development, before muscle differentiation. mef2ca transcripts including exon 5 (mef2ca 4–5–6) are present early in the embryo. Over-expression of this isoform alters the expression of genes involved in early dorso-ventral patterning of the embryo such as chordin, nodal related 1 and goosecoid, and induces severe developmental defects. AS of mef2cb generates a long splicing isoform in the exon 5 region (Mef2cbL) that predominates during somitogenesis. Mef2cbL contains an evolutionarily conserved domain derived from exonization of a fragment of intron 5, which confers the ability to induce ectopic muscle in mesoderm upon over-expression of the protein. Taken together, the data show that AS is a significant regulator of Mef2c activity. Elsevier Pub. Co 2014-07 /pmc/articles/PMC4064114/ /pubmed/24844180 http://dx.doi.org/10.1016/j.bbagrm.2014.05.003 Text en © 2014 Elsevier B.V. All rights reserved. https://creativecommons.org/licenses/by-nc-nd/4.0/This work is licensed under a Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License (https://creativecommons.org/licenses/by-nc-nd/4.0/) , which allows reusers to copy and distribute the material in any medium or format in unadapted form only, for noncommercial purposes only, and only so long as attribution is given to the creator.
spellingShingle Article
Ganassi, M.
Badodi, S.
Polacchini, A.
Baruffaldi, F.
Battini, R.
Hughes, S.M.
Hinits, Y.
Molinari, S.
Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
title Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
title_full Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
title_fullStr Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
title_full_unstemmed Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
title_short Distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
title_sort distinct functions of alternatively spliced isoforms encoded by zebrafish mef2ca and mef2cb
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4064114/
https://www.ncbi.nlm.nih.gov/pubmed/24844180
http://dx.doi.org/10.1016/j.bbagrm.2014.05.003
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