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Fibroblast growth factor 21 is expressed and secreted from skeletal muscle following electrical stimulation <i>via</i> extracellular ATP activation of the PI3K/Akt/mTOR signaling pathway
Indexado
WoS WOS:000945875800001
Scopus SCOPUS_ID:85149892841
DOI 10.3389/FENDO.2023.1059020
Año 2023
Tipo artículo de investigación

Citas Totales

Autores Afiliación Chile

Instituciones Chile

% Participación
Internacional

Autores
Afiliación Extranjera

Instituciones
Extranjeras


Abstract



Fibroblast growth factor 21 (FGF21) is a hormone involved in the regulation of lipid, glucose, and energy metabolism. Although it is released mainly from the liver, in recent years it has been shown that it is a "myokine", synthesized in skeletal muscles after exercise and stress conditions through an Akt-dependent pathway and secreted for mediating autocrine and endocrine roles. To date, the molecular mechanism for the pathophysiological regulation of FGF21 production in skeletal muscle is not totally understood. We have previously demonstrated that muscle membrane depolarization controls gene expression through extracellular ATP (eATP) signaling, by a mechanism defined as "Excitation-Transcription coupling". eATP signaling regulates the expression and secretion of interleukin 6, a well-defined myokine, and activates the Akt/mTOR signaling pathway. This work aimed to study the effect of electrical stimulation in the regulation of both production and secretion of skeletal muscle FGF21, through eATP signaling and PI3K/Akt pathway. Our results show that electrical stimulation increases both mRNA and protein (intracellular and secreted) levels of FGF21, dependent on an extracellular ATP signaling mechanism in skeletal muscle. Using pharmacological inhibitors, we demonstrated that FGF21 production and secretion from muscle requires the activation of the P2YR/PI3K/Akt/mTOR signaling pathway. These results confirm skeletal muscle as a source of FGF21 in physiological conditions and unveil a new molecular mechanism for regulating FGF21 production in this tissue. Our results will allow to identify new molecular targets to understand the regulation of FGF21 both in physiological and pathological conditions, such as exercise, aging, insulin resistance, and Duchenne muscular dystrophy, all characterized by an alteration in both FGF21 levels and ATP signaling components. These data reinforce that eATP signaling is a relevant mechanism for myokine expression in skeletal muscle.

Revista



Revista ISSN
Frontiers In Endocrinology 1664-2392

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Disciplinas de Investigación



WOS
Endocrinology & Metabolism
Scopus
Sin Disciplinas
SciELO
Sin Disciplinas

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Publicaciones WoS (Ediciones: ISSHP, ISTP, AHCI, SSCI, SCI), Scopus, SciELO Chile.

Colaboración Institucional



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Autores - Afiliación



Ord. Autor Género Institución - País
1 ARIAS-CALDERON, MANUEL ANDRES Hombre Universidad de Chile - Chile
2 CASAS-ATALA, MARIANA VICTORIA Mujer Universidad de Chile - Chile
3 Balanta-Melo, Julian Hombre Universidad de Chile - Chile
UNIV VALLE - Colombia
Universidad del Valle, Cali - Colombia
4 Morales, Camilo Hombre Universidad de Chile - Chile
Pontificia Univ Javeriana - Colombia
Pontificia Universidad Javeriana, Cali - Colombia
5 Hernández, Nadia Mujer Universidad de Chile - Chile
6 LLANOS-VIDAL, PAOLA ANDREA Mujer Universidad de Chile - Chile
7 JAIMOVICH-PEREZ, ENRIQUE ZACARIAS Hombre Universidad de Chile - Chile
8 BUVINIC-RADIC, SONJA Mujer Universidad de Chile - Chile

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Financiamiento



Fuente
Fondef
Fondo Nacional de Desarrollo Científico y Tecnológico
Comisión Nacional de Investigación Científica y Tecnológica
Universidad del Valle
Conicyt Chile
FONDECYT Chile
Pontificia Universidad Javeriana
Redes
Universidad de Chile VID-Enlace Fondecyt
Program Professor Scholarship Semillero Docente 2014 of the Universidad del Valle, Colombia
Academic Development Program of the Pontificia Universidad Javeriana Cali (CM-J)

Muestra la fuente de financiamiento declarada en la publicación.

Agradecimientos



Agradecimiento
This research was funded by the FONDECYT Chile Grants No.1151353 (SB, PL, MC), 1201385 (SB, PL) and 1190406 (PL, SB). Universidad de Chile VID-Enlace Fondecyt 2019 VIDENL29/19 (SB) and VIDENL09 (EJ). FONDEF ID16/10101(MC, EJ, SB). REDES 180209 (MC, EJ, SB). CONICYT Chile Scholarship No. 21170015 (JB-M), No. 63140009 (CM-J), No.21151035 (MA-C). Academic Development Program of the Pontificia Universidad Javeriana Cali (CM-J) and the Program Professor Scholarship Semillero Docente 2014 of the Universidad del Valle, Colombia (JB-M).
This research was funded by the FONDECYT Chile Grants No.1151353 (SB, PL, MC), 1201385 (SB, PL) and 1190406 (PL, SB). Universidad de Chile VID-Enlace Fondecyt 2019 VIDENL29/19 (SB) and VIDENL09 (EJ). FONDEF ID16/10101(MC, EJ, SB). REDES 180209 (MC, EJ, SB). CONICYT Chile Scholarship No. 21170015 (JB-M), No. 63140009 (CM-J), No.21151035 (MA-C). Academic Development Program of the Pontificia Universidad Javeriana Cali (CM-J) and the Program Professor Scholarship Semillero Docente 2014 of the Universidad del Valle, Colombia (JB-M).
This research was funded by the FONDECYT Chile Grants No.1151353 (SB, PL, MC), 1201385 (SB, PL) and 1190406 (PL, SB). Universidad de Chile VID-Enlace Fondecyt 2019 VIDENL29/19 (SB) and VIDENL09 (EJ). FONDEF ID16/10101(MC, EJ, SB). REDES 180209 (MC, EJ, SB). CONICYT Chile Scholarship No. 21170015 (JB-M), No. 63140009 (CM-J), No.21151035 (MA-C). Academic Development Program of the Pontificia Universidad Javeriana Cali (CM-J) and the Program Professor Scholarship Semillero Docente 2014 of the Universidad del Valle, Colombia (JB-M).

Muestra la fuente de financiamiento declarada en la publicación.