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Satellite cell-specific ablation of Cdon impairs integrin activation, FGF signalling, and muscle regeneration

Authors
Bae, Ju-HyeonHong, MingiJeong, Hyeon-JuKim, HyebeenLee, Sang-JinRyu, DongryeolBae, Gyu-UnCho, Sung ChunLee, Young-SamKrauss, Robert S.Kang, Jong-Sun
Issue Date
Aug-2020
Publisher
WILEY
Keywords
Satellite cell; Muscle regeneration; Cdon; Cellular senescence; FGFR; Growth factor signalling
Citation
JOURNAL OF CACHEXIA SARCOPENIA AND MUSCLE, v.11, no.4, pp 1089 - 1103
Pages
15
Journal Title
JOURNAL OF CACHEXIA SARCOPENIA AND MUSCLE
Volume
11
Number
4
Start Page
1089
End Page
1103
URI
https://scholarworks.sookmyung.ac.kr/handle/2020.sw.sookmyung/1334
DOI
10.1002/jcsm.12563
ISSN
2190-5991
2190-6009
Abstract
Background Perturbation in cell adhesion and growth factor signalling in satellite cells results in decreased muscle regenerative capacity. Cdon (also called Cdo) is a component of cell adhesion complexes implicated in myogenic differentiation, but its role in muscle regeneration remains to be determined. Methods We generated inducible satellite cell-specific Cdon ablation in mice by utilizing a conditional Cdon allele and Pax7 (CreERT2). To induce Cdon ablation, mice were intraperitoneally injected with tamoxifen (tmx). Using cardiotoxin-induced muscle injury, the effect of Cdon depletion on satellite cell function was examined by histochemistry, immunostaining, and 5-ethynyl-2'-deoxyuridine (EdU) incorporation assay. Isolated myofibers or myoblasts were utilized to determine stem cell function and senescence. To determine pathways related to Cdon deletion, injured muscles were subjected to RNA sequencing analysis. Results Satellite cell-specific Cdon ablation causes impaired muscle regeneration with fibrosis, likely attributable to decreased proliferation, and senescence, of satellite cells. Cultured Cdon-depleted myofibers exhibited 32 +/- 9.6% of EdU-positive satellite cells compared with 58 +/- 4.4% satellite cells in control myofibers (P < 0.05). About 32.5 +/- 3.7% Cdon-ablated myoblasts were positive for senescence-associated beta-galactosidase (SA-beta-gal) while only 3.6 +/- 0.5% of control satellite cells were positive (P < 0.001). Transcriptome analysis of muscles at post-injury Day 4 revealed alterations in genes related to mitogen-activated protein kinase signalling (P < 8.29 e(-5)) and extracellular matrix (P < 2.65 e(-24)). Consistent with this, Cdon-depleted tibialis anterior muscles had reduced phosphorylated extracellular signal-regulated kinase (p-ERK) protein levels and expression of ERK targets, such as Fos (0.23-fold) and Egr1 (0.31-fold), relative to mock-treated control muscles (P < 0.001). Cdon-depleted myoblasts exhibited impaired ERK activation in response to basic fibroblast growth factor. Cdon ablation resulted in decreased and/or mislocalized integrin beta 1 activation in satellite cells (weak or mislocalized integrin1 in tmx = 38.7 +/- 1.9%, mock = 21.5 +/- 6%, P < 0.05), previously linked with reduced fibroblast growth factor (FGF) responsiveness in aged satellite cells. In mechanistic studies, Cdon interacted with and regulated cell surface localization of FGFR1 and FGFR4, likely contributing to FGF responsiveness of satellite cells. Satellite cells from a progeria model, Zmpste24(-/-) myofibers, showed decreased Cdon levels (Cdon-positive cells in Zmpste24(-/-) = 63.3 +/- 11%, wild type = 90 +/- 7.7%, P < 0.05) and integrin beta 1 activation (weak or mislocalized integrin beta 1 in Zmpste24(-/-) = 64 +/- 6.9%, wild type = 17.4 +/- 5.9%, P < 0.01). Conclusions Cdon deficiency in satellite cells causes impaired proliferation of satellite cells and muscle regeneration via aberrant integrin and FGFR signalling.
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