De Ritis Daniele, Ferrè Laura, De Winter Jonathan, Tremblay-Desbiens Clémence, Blais Mathieu, Bassi Maria Teresa, Dupré Nicolas, Baets Jonathan, Filippi Massimo, Maltecca Francesca
Mitochondrial Dysfunctions in Neurodegeneration Unit, IRCCS Ospedale San Raffaele, 20132 Milan, Italy.
Department of Neurology, IRCCS Ospedale San Raffaele, 20132 Milan, Italy.
Brain Commun. 2024 Jul 18;6(4):fcae243. doi: 10.1093/braincomms/fcae243. eCollection 2024.
Autosomal recessive spastic ataxia of Charlevoix-Saguenay is a rare neurodegenerative disease caused by biallelic variants in the gene encoding for sacsin. More than 200 pathogenic variants have been identified to date, most of which are missense. It is likely that the prevalence of autosomal recessive spastic ataxia of Charlevoix-Saguenay is underestimated due to the lack of an efficient diagnostic tool able to validate variants of uncertain significance. We have previously shown that sacsin is almost absent in fibroblasts of patients with autosomal recessive spastic ataxia of Charlevoix-Saguenay regardless of the type of variant, because sacsin carrying missense variants is cotranslationally degraded. In this work, we aimed to establish the pathogenicity of variants by quantifying sacsin protein in blood samples, with relevant implications for autosomal recessive spastic ataxia of Charlevoix-Saguenay diagnosis. We developed a protocol to assess sacsin protein levels by western blot using small amounts of peripheral blood mononuclear cells, which can be propagated in culture and cryopreserved. The study involves eight patients with autosomal recessive spastic ataxia of Charlevoix-Saguenay (including a novel case) carrying variants of different types and positions along the gene and two parents who are carriers of heterozygous missense variants. We show that patients with autosomal recessive spastic ataxia of Charlevoix-Saguenay (carrying either missense or truncating variants) almost completely lacked sacsin in peripheral blood mononuclear cells. Moreover, both carriers of a missense variant showed 50% reduction in sacsin protein levels compared to controls. We also describe a patient with uniparental isodisomy carrying a homozygous nonsense variant near the 3' end of the gene. This resulted in a stable sacsin protein lacking the last 202 amino acids, probably due to escape of nonsense-mediated decay of mRNA. In conclusion, we have optimized a minimally invasive diagnostic tool for autosomal recessive spastic ataxia of Charlevoix-Saguenay in blood samples based on sacsin protein level assessment. Indeed, our results provide definite evidence that sacsin carrying missense pathogenic variants undergoes cotranslational degradation. The quantitative reduction in sacsin levels in the case of missense variants of uncertain significance allows defining them as pathogenic variants, something which cannot be predicted bioinformatically with high certainty.
夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调是一种罕见的神经退行性疾病,由编码 sacsin 的基因双等位基因变异引起。迄今为止已鉴定出200多种致病变异,其中大多数是错义变异。由于缺乏能够验证意义不确定变异的有效诊断工具,夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调的患病率可能被低估。我们之前已经表明,无论变异类型如何,夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调患者的成纤维细胞中几乎不存在 sacsin,因为携带错义变异的 sacsin 在共翻译过程中被降解。在这项工作中,我们旨在通过定量血液样本中的 sacsin 蛋白来确定变异的致病性,这对夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调的诊断具有重要意义。我们开发了一种方案,使用少量外周血单个核细胞通过蛋白质印迹法评估 sacsin 蛋白水平,这些细胞可以在培养中增殖并冷冻保存。该研究涉及八名患有夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调的患者(包括一个新病例),他们携带沿该基因不同类型和位置的变异,以及两名携带杂合错义变异的携带者父母。我们表明,患有夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调的患者(携带错义或截短变异)在外周血单个核细胞中几乎完全缺乏 sacsin。此外,与对照组相比,两个携带错义变异的携带者的 sacsin 蛋白水平降低了50%。我们还描述了一名单亲二体患者,其在该基因3'端附近携带纯合无义变异。这导致了一种稳定的 sacsin 蛋白,缺少最后202个氨基酸,可能是由于 mRNA 的无义介导衰变逃逸所致。总之,我们基于 sacsin 蛋白水平评估优化了一种用于夏尔沃 - 萨格奈常染色体隐性痉挛性共济失调血液样本的微创诊断工具。确实,我们的结果提供了确凿的证据,表明携带错义致病变异的 sacsin 会经历共翻译降解。对于意义不确定的错义变异,sacsin 水平的定量降低使其能够被定义为致病变异,而这是无法通过生物信息学高度确定地预测的。
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