The FoxO3/type 2 deiodinase pathway is required for normal mouse myogenesis and muscle regeneration
Monica Dentice, … , P. Reed Larsen, Domenico Salvatore
Monica Dentice, … , P. Reed Larsen, Domenico Salvatore
Published October 11, 2010
Citation Information: J Clin Invest. 2010;120(11):4021-4030. https://doi.org/10.1172/JCI43670.
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Research Article Muscle biology

The FoxO3/type 2 deiodinase pathway is required for normal mouse myogenesis and muscle regeneration

Abstract

The active thyroid hormone 3,5,3′ triiodothyronine (T3) is a major regulator of skeletal muscle function. The deiodinase family of enzymes controls the tissue-specific activation and inactivation of the prohormone thyroxine (T4). Here we show that type 2 deiodinase (D2) is essential for normal mouse myogenesis and muscle regeneration. Indeed, D2-mediated increases in T3 were essential for the enhanced transcription of myogenic differentiation 1 (MyoD) and for execution of the myogenic program. Conversely, the expression of T3-dependent genes was reduced and after injury regeneration markedly delayed in muscles of mice null for the gene encoding D2 (Dio2), despite normal circulating T3 concentrations. Forkhead box O3 (FoxO3) was identified as a key molecule inducing D2 expression and thereby increasing intracellular T3 production. Accordingly, FoxO3-depleted primary myoblasts also had a differentiation deficit that could be rescued by high levels of T3. In conclusion, the FoxO3/D2 pathway selectively enhances intracellular active thyroid hormone concentrations in muscle, providing a striking example of how a circulating hormone can be tissue-specifically activated to influence development locally.

Authors

Monica Dentice, Alessandro Marsili, Raffaele Ambrosio, Ombretta Guardiola, Annarita Sibilio, Ji-Hye Paik, Gabriella Minchiotti, Ronald A. DePinho, Gianfranco Fenzi, P. Reed Larsen, Domenico Salvatore

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Figure 2

Blocking D2 impairs myogenic differentiation of mpc.

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Blocking D2 impairs myogenic differentiation of mpc. (A) Primary pp6 fro...
(A) Primary pp6 from wild-type or Dio2–/– mice and C2C12 mock-transfected (shCTR) or shD2 cells were cultured in proliferative or differentiating conditions as indicated. Scale bar: 100 μm. (B) cDNAs were prepared from pp6 cells from wild-type or Dio2–/– mice and cultured in proliferative and differentiating conditions in the presence of vehicle or 30 nM T3 as indicated. cDNAs were analyzed for MyoD, myogenin, and Myh2 expression by RT-PCR. For each gene, normalized copies of the target gene in proliferating wild-type pp6 cells were set as 1. Values are mean ± SEM of 4 independent experiments (C) Western blot analysis of total lysates from pp6 cells cultured as in B. Tubulin levels were measured as loading control.