The double homeodomain protein DUX4c is associated with regenerating muscle fibers and RNA-binding proteins

Clothilde Claus; Moriya Slavin; Eugénie Ansseau; Céline Lancelot; Karimatou Bah; Saskia Lassche; Manon Fiévet; Anna Greco; Sara Tomaiuolo; Alexandra Tassin; Virginie Dudome; Benno Kusters; Anne-Emilie Declèves; Dalila Laoudj-Chenivesse; Baziel G M van Engelen; Denis Nonclercq; Alexandra Belayew; Nir Kalisman; Frédérique Coppée

doi:10.1186/s13395-022-00310-y

The double homeodomain protein DUX4c is associated with regenerating muscle fibers and RNA-binding proteins

Skelet Muscle. 2023 Mar 7;13(1):5. doi: 10.1186/s13395-022-00310-y.

Authors

Clothilde Claus¹, Moriya Slavin², Eugénie Ansseau¹, Céline Lancelot¹, Karimatou Bah¹, Saskia Lassche^{3

4}, Manon Fiévet¹, Anna Greco³, Sara Tomaiuolo¹, Alexandra Tassin^{1

5}, Virginie Dudome¹, Benno Kusters⁶, Anne-Emilie Declèves¹, Dalila Laoudj-Chenivesse⁷, Baziel G M van Engelen³, Denis Nonclercq⁸, Alexandra Belayew¹, Nir Kalisman², Frédérique Coppée⁹

Affiliations

¹ Laboratory of Metabolic and Molecular Biochemistry, Research Institute for Health Sciences and Technology, University of Mons, 6, Avenue du Champs de Mars, B-7000, Mons, Belgium.
² Department of Biological Chemistry, the Alexander Silberman Institute of Life Sciences, Hebrew University of Jerusalem, Jerusalem, Israel.
³ Department of Neurology, Donders Institute for Brain, Cognition and Behaviour, Radboud University Medical Center, 6525 GA, Nijmegen, The Netherlands.
⁴ Department of Neurology, Zuyderland Medical Center, Heerlen, the Netherlands.
⁵ Laboratory of Respiratory Physiology and Rehabilitation, Research Institute for Health Sciences and Technology, University of Mons, 6, Avenue du Champs de Mars, B-7000, Mons, Belgium.
⁶ Department of Pathology, Donders Institute for Brain, Cognition and Behaviour, Radboud University Medical Center, 6525 GA, Nijmegen, The Netherlands.
⁷ PhyMedExp, University of Montpellier, INSERM, CNRS, Montpellier, France.
⁸ Laboratory of Histology, Research Institute for Health Sciences and Technology, University of Mons, 6, Avenue du Champs de Mars, B-7000, Mons, Belgium.
⁹ Laboratory of Metabolic and Molecular Biochemistry, Research Institute for Health Sciences and Technology, University of Mons, 6, Avenue du Champs de Mars, B-7000, Mons, Belgium. Frederique.coppee@umons.ac.be.

Abstract

Background: We have previously demonstrated that double homeobox 4 centromeric (DUX4C) encoded for a functional DUX4c protein upregulated in dystrophic skeletal muscles. Based on gain- and loss-of-function studies we have proposed DUX4c involvement in muscle regeneration. Here, we provide further evidence for such a role in skeletal muscles from patients affected with facioscapulohumeral muscular dystrophy (FSHD).

Methods: DUX4c was studied at RNA and protein levels in FSHD muscle cell cultures and biopsies. Its protein partners were co-purified and identified by mass spectrometry. Endogenous DUX4c was detected in FSHD muscle sections with either its partners or regeneration markers using co-immunofluorescence or in situ proximity ligation assay.

Results: We identified new alternatively spliced DUX4C transcripts and confirmed DUX4c immunodetection in rare FSHD muscle cells in primary culture. DUX4c was detected in nuclei, cytoplasm or at cell-cell contacts between myocytes and interacted sporadically with specific RNA-binding proteins involved, a.o., in muscle differentiation, repair, and mass maintenance. In FSHD muscle sections, DUX4c was found in fibers with unusual shape or central/delocalized nuclei (a regeneration feature) staining for developmental myosin heavy chain, MYOD or presenting intense desmin labeling. Some couples of myocytes/fibers locally exhibited peripheral DUX4c-positive areas that were very close to each other, but in distinct cells. MYOD or intense desmin staining at these locations suggested an imminent muscle cell fusion. We further demonstrated DUX4c interaction with its major protein partner, C1qBP, inside myocytes/myofibers that presented features of regeneration. On adjacent muscle sections, we could unexpectedly detect DUX4 (the FSHD causal protein) and its interaction with C1qBP in fusing myocytes/fibers.

Conclusions: DUX4c upregulation in FSHD muscles suggests it contributes not only to the pathology but also, based on its protein partners and specific markers, to attempts at muscle regeneration. The presence of both DUX4 and DUX4c in regenerating FSHD muscle cells suggests DUX4 could compete with normal DUX4c functions, thus explaining why skeletal muscle is particularly sensitive to DUX4 toxicity. Caution should be exerted with therapeutic agents aiming for DUX4 suppression because they might also repress the highly similar DUX4c and interfere with its physiological role.

Keywords: DUX genes; Differentiation; FUS; Fibrosis; HA-binding protein C1qBP; M1/M2 macrophages; Muscle regeneration; RNA-binding interactors; SFPQ; Testis.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Carrier Proteins
Cytoplasm
Desmin
Homeodomain Proteins* / genetics
Humans
Mitochondrial Proteins
Muscle Fibers, Skeletal
Muscular Dystrophy, Facioscapulohumeral* / genetics
RNA-Binding Proteins* / genetics
Transcription Factors* / genetics

Substances

C1QBP protein, human
Carrier Proteins
Desmin
Homeodomain Proteins
Mitochondrial Proteins
DUX4L9 protein, human
Transcription Factors
RNA-Binding Proteins