Inhibition of de novo ceramide synthesis upregulates phospholipase D and enhances myogenic differentiation

Author:

Mebarek Saïda123,Komati Hiba123,Naro Fabio4,Zeiller Caroline123,Alvisi Monica4,Lagarde Michel123,Prigent Annie-France123,Némoz Georges123

Affiliation:

1. INSERM, Unit 585, Villeurbanne, F-69621 France

2. INSA-Lyon, Laboratoire de Physiopathologie des Lipides et Membranes, Villeurbanne, F-69621 France

3. IMBL, Villeurbanne, F-69621 France

4. Università di Roma-La Sapienza, Dipartimento di Istologia ed Embriologia Medica, Roma, Italy

Abstract

In L6 skeletal myoblasts induced to differentiate by Arg8-vasopressin treatment, a short-lived lowering of ceramide levels was observed, followed by a long-lasting elevation that was prevented by inhibitors of the de novo synthesis pathway, fumonisin B1 and myriocin. Both inhibitors increased the expression of myogenic differentiation markers and cell fusion rate, whereas short-chain ceramides inhibited these responses. Similar drug effects were observed on primary mouse satellite cell differentiation. Furthermore, bacterial sphingomyelinase overexpression suppressed myogenin nuclear accumulation in L6 cells. These data suggested that endogenous ceramide mediates a negative feedback mechanism limiting myogenic differentiation, and that inhibitors of ceramide synthesis promoted myogenesis by removing this control. Phospholipase D (PLD), a recognized target of ceramide, is required for myogenesis, as shown by the negative effects of PLD1 isoform depletion obtained by siRNA treatment. Fumonisin induced an increase in PLD activity of L6 cells, whereas C6-ceramide decreased it. The expression of PLD1 mRNA transcripts was selectively decreased by C6-ceramide, and increased by ceramide synthesis inhibitors. An early step of myogenic response is the PLD1-dependent formation of actin stress fiber-like structures. C6-ceramide addition or overexpression of sphingomyelinase impaired actin fiber formation. Ceramide might thus regulate myogenesis through downregulation of PLD1 expression and activity.

Publisher

The Company of Biologists

Subject

Cell Biology

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