| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2041683 | Cell Reports | 2014 | 12 Pages |
•S-Nitrosylation of MEF2 at conserved cysteine residues occurs in plants and animal•S-Nitrosylation of MEF2 inhibits its DNA binding and transcriptional activity•S-Nitrosylation of MEF2 inhibits both neurogenesis and neuronal survival
SummaryRedox-mediated posttranslational modifications represent a molecular switch that controls major mechanisms of cell function. Nitric oxide (NO) can mediate redox reactions via S-nitrosylation, representing transfer of an NO group to a critical protein thiol. NO is known to modulate neurogenesis and neuronal survival in various brain regions in disparate neurodegenerative conditions. However, a unifying molecular mechanism linking these phenomena remains unknown. Here, we report that S-nitrosylation of myocyte enhancer factor 2 (MEF2) transcription factors acts as a redox switch to inhibit both neurogenesis and neuronal survival. Structure-based analysis reveals that MEF2 dimerization creates a pocket, facilitating S-nitrosylation at an evolutionally conserved cysteine residue in the DNA binding domain. S-Nitrosylation disrupts MEF2-DNA binding and transcriptional activity, leading to impaired neurogenesis and survival in vitro and in vivo. Our data define a molecular switch whereby redox-mediated posttranslational modification controls both neurogenesis and neurodegeneration via a single transcriptional signaling cascade.
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