| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2040905 | Cell Reports | 2013 | 12 Pages |
SummaryHuntington disease (HD), a dominantly inherited neurodegenerative disorder caused by the expansion of a CAG-encoded polyglutamine (polyQ) repeat in huntingtin (Htt), displays a highly heterogeneous etiopathology and disease onset. Here, we show that the translation of expanded CAG repeats in mutant Htt exon 1 leads to a depletion of charged glutaminyl-transfer RNA (tRNA)Gln-CUG that pairs exclusively to the CAG codon. This results in translational frameshifting and the generation of various transframe-encoded species that differently modulate the conformational switch to nucleate fibrillization of the parental polyQ protein. Intriguingly, the frameshifting frequency varies strongly among different cell lines and is higher in cells with intrinsically lower concentrations of tRNAGln-CUG. The concentration of tRNAGln-CUG also differs among different brain areas in the mouse. We propose that translational frameshifting may act as a significant disease modifier that contributes to the cell-selective neurotoxicity and disease course heterogeneity of HD on both cellular and individual levels.
Graphical AbstractFigure optionsDownload full-size imageDownload as PowerPoint slideHighlights► Expanded CAG stretches are prone to translational frameshifting ► Depletion of the charged, cognate tRNA causes translational frameshifting ► Frequency of translational frameshifting correlates with the CAG repeat length ► Frameshifted species modulate the aggregation course of the parental protein
