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Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration

Here, we identify a role for the matrilin-2 (Matn2) extracellular matrix protein in controlling the early stages of myogenic differentiation. We observed Matn2 deposition around proliferating, differentiating and fusing myoblasts in culture and during muscle regeneration in vivo. Silencing of Matn2...

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Autores principales: Deák, Ferenc, Mátés, Lajos, Korpos, Éva, Zvara, Ágnes, Szénási, Tibor, Kiricsi, Mónika, Mendler, Luca, Keller-Pintér, Anikó, Ózsvári, Béla, Juhász, Hajnalka, Sorokin, Lydia, Dux, László, Mermod, Nicolas, Puskás, László G., Kiss, Ibolya
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Company of Biologists 2014
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4117230/
https://www.ncbi.nlm.nih.gov/pubmed/24895400
http://dx.doi.org/10.1242/jcs.141556
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author Deák, Ferenc
Mátés, Lajos
Korpos, Éva
Zvara, Ágnes
Szénási, Tibor
Kiricsi, Mónika
Mendler, Luca
Keller-Pintér, Anikó
Ózsvári, Béla
Juhász, Hajnalka
Sorokin, Lydia
Dux, László
Mermod, Nicolas
Puskás, László G.
Kiss, Ibolya
author_facet Deák, Ferenc
Mátés, Lajos
Korpos, Éva
Zvara, Ágnes
Szénási, Tibor
Kiricsi, Mónika
Mendler, Luca
Keller-Pintér, Anikó
Ózsvári, Béla
Juhász, Hajnalka
Sorokin, Lydia
Dux, László
Mermod, Nicolas
Puskás, László G.
Kiss, Ibolya
author_sort Deák, Ferenc
collection PubMed
description Here, we identify a role for the matrilin-2 (Matn2) extracellular matrix protein in controlling the early stages of myogenic differentiation. We observed Matn2 deposition around proliferating, differentiating and fusing myoblasts in culture and during muscle regeneration in vivo. Silencing of Matn2 delayed the expression of the Cdk inhibitor p21 and of the myogenic genes Nfix, MyoD and Myog, explaining the retarded cell cycle exit and myoblast differentiation. Rescue of Matn2 expression restored differentiation and the expression of p21 and of the myogenic genes. TGF-β1 inhibited myogenic differentiation at least in part by repressing Matn2 expression, which inhibited the onset of a positive-feedback loop whereby Matn2 and Nfix activate the expression of one another and activate myoblast differentiation. In vivo, myoblast cell cycle arrest and muscle regeneration was delayed in Matn2(−/−) relative to wild-type mice. The expression levels of Trf3 and myogenic genes were robustly reduced in Matn2(−/−) fetal limbs and in differentiating primary myoblast cultures, establishing Matn2 as a key modulator of the regulatory cascade that initiates terminal myogenic differentiation. Our data thus identify Matn2 as a crucial component of a genetic switch that modulates the onset of tissue repair.
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spelling pubmed-41172302014-08-19 Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration Deák, Ferenc Mátés, Lajos Korpos, Éva Zvara, Ágnes Szénási, Tibor Kiricsi, Mónika Mendler, Luca Keller-Pintér, Anikó Ózsvári, Béla Juhász, Hajnalka Sorokin, Lydia Dux, László Mermod, Nicolas Puskás, László G. Kiss, Ibolya J Cell Sci Research Article Here, we identify a role for the matrilin-2 (Matn2) extracellular matrix protein in controlling the early stages of myogenic differentiation. We observed Matn2 deposition around proliferating, differentiating and fusing myoblasts in culture and during muscle regeneration in vivo. Silencing of Matn2 delayed the expression of the Cdk inhibitor p21 and of the myogenic genes Nfix, MyoD and Myog, explaining the retarded cell cycle exit and myoblast differentiation. Rescue of Matn2 expression restored differentiation and the expression of p21 and of the myogenic genes. TGF-β1 inhibited myogenic differentiation at least in part by repressing Matn2 expression, which inhibited the onset of a positive-feedback loop whereby Matn2 and Nfix activate the expression of one another and activate myoblast differentiation. In vivo, myoblast cell cycle arrest and muscle regeneration was delayed in Matn2(−/−) relative to wild-type mice. The expression levels of Trf3 and myogenic genes were robustly reduced in Matn2(−/−) fetal limbs and in differentiating primary myoblast cultures, establishing Matn2 as a key modulator of the regulatory cascade that initiates terminal myogenic differentiation. Our data thus identify Matn2 as a crucial component of a genetic switch that modulates the onset of tissue repair. The Company of Biologists 2014-08-01 /pmc/articles/PMC4117230/ /pubmed/24895400 http://dx.doi.org/10.1242/jcs.141556 Text en © 2014. Published by The Company of Biologists Ltd http://creativecommons.org/licenses/by/3.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/3.0), which permits unrestricted use, distribution and reproduction in any medium provided that the original work is properly attributed.
spellingShingle Research Article
Deák, Ferenc
Mátés, Lajos
Korpos, Éva
Zvara, Ágnes
Szénási, Tibor
Kiricsi, Mónika
Mendler, Luca
Keller-Pintér, Anikó
Ózsvári, Béla
Juhász, Hajnalka
Sorokin, Lydia
Dux, László
Mermod, Nicolas
Puskás, László G.
Kiss, Ibolya
Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
title Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
title_full Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
title_fullStr Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
title_full_unstemmed Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
title_short Extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
title_sort extracellular deposition of matrilin-2 controls the timing of the myogenic program during muscle regeneration
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4117230/
https://www.ncbi.nlm.nih.gov/pubmed/24895400
http://dx.doi.org/10.1242/jcs.141556
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