Cheng Flora, De Luca Alana, Hogan Alison L, Rayner Stephanie L, Davidson Jennilee M, Watchon Maxinne, Stevens Claire H, Muñoz Sonia Sanz, Ooi Lezanne, Yerbury Justin J, Don Emily K, Fifita Jennifer A, Villalva Maria D, Suddull Hannah, Chapman Tyler R, Hedl Thomas J, Walker Adam K, Yang Shu, Morsch Marco, Shi Bingyang, Blair Ian P, Laird Angela S, Chung Roger S, Lee Albert
Centre for Motor Neuron Disease Research, Department of Biomedical Sciences, Faculty of Medicine, Health, and Human Sciences, Macquarie University, North Ryde, NSW, Australia.
Illawarra Health and Medical Research Institute (IHMRI), University of Wollongong, Wollongong, NSW, Australia.
Front Mol Neurosci. 2021 Apr 27;14:627740. doi: 10.3389/fnmol.2021.627740. eCollection 2021.
The past decade has seen a rapid acceleration in the discovery of new genetic causes of ALS, with more than 20 putative ALS-causing genes now cited. These genes encode proteins that cover a diverse range of molecular functions, including free radical scavenging (e.g., SOD1), regulation of RNA homeostasis (e.g., TDP-43 and FUS), and protein degradation through the ubiquitin-proteasome system (e.g., ubiquilin-2 and cyclin F) and autophagy (TBK1 and sequestosome-1/p62). It is likely that the various initial triggers of disease (either genetic, environmental and/or gene-environment interaction) must converge upon a common set of molecular pathways that underlie ALS pathogenesis. Given the complexity, it is not surprising that a catalog of molecular pathways and proteostasis dysfunctions have been linked to ALS. One of the challenges in ALS research is determining, at the early stage of discovery, whether a new gene mutation is indeed disease-specific, and if it is linked to signaling pathways that trigger neuronal cell death. We have established a proof-of-concept proteogenomic workflow to assess new gene mutations, using CCNF (cyclin F) as an example, in cell culture models to screen whether potential gene candidates fit the criteria of activating apoptosis. This can provide an informative and time-efficient output that can be extended further for validation in a variety of and models and/or for mechanistic studies. As a proof-of-concept, we expressed cyclin F mutations (K97R, S195R, S509P, R574Q, S621G) in HEK293 cells for label-free quantitative proteomics that bioinformatically predicted activation of the neuronal cell death pathways, which was validated by immunoblot analysis. Proteomic analysis of induced pluripotent stem cells (iPSCs) derived from patient fibroblasts bearing the S621G mutation showed the same activation of these pathways providing compelling evidence for these candidate gene mutations to be strong candidates for further validation and mechanistic studies (such as E3 enzymatic activity assays, protein-protein and protein-substrate studies, and neuronal apoptosis and aberrant branching measurements in zebrafish). Our proteogenomics approach has great utility and provides a relatively high-throughput screening platform to explore candidate gene mutations for their propensity to cause neuronal cell death, which will guide a researcher for further experimental studies.
在过去十年中,肌萎缩侧索硬化症(ALS)新的遗传病因的发现速度迅速加快,目前已有超过20个假定的ALS致病基因被提及。这些基因编码的蛋白质涵盖了广泛的分子功能,包括自由基清除(如超氧化物歧化酶1,SOD1)、RNA稳态调节(如TAR DNA结合蛋白43,TDP - 43和融合蛋白,FUS),以及通过泛素 - 蛋白酶体系统(如泛素连接蛋白2和细胞周期蛋白F)和自噬(TBK1和聚集体蛋白1/p62)进行的蛋白质降解。很可能疾病的各种初始触发因素(无论是遗传、环境和/或基因 - 环境相互作用)必须汇聚到一组共同的分子途径上,这些途径是ALS发病机制的基础。鉴于其复杂性,与ALS相关的分子途径和蛋白质稳态功能障碍的目录众多也就不足为奇了。ALS研究中的挑战之一是在发现的早期阶段确定一个新的基因突变是否确实是疾病特异性的,以及它是否与触发神经元细胞死亡的信号通路相关。我们建立了一个概念验证的蛋白质基因组学工作流程,以评估新的基因突变,以细胞周期蛋白F(CCNF)为例,在细胞培养模型中筛选潜在的基因候选物是否符合激活细胞凋亡的标准。这可以提供一个信息丰富且高效的结果,可进一步扩展到在各种体内和体外模型中进行验证和/或进行机制研究。作为概念验证,我们在人胚肾293(HEK293)细胞中表达了细胞周期蛋白F的突变(K97R、S195R、S509P、R574Q、S621G),用于无标记定量蛋白质组学分析,通过生物信息学预测神经元细胞死亡途径的激活,并通过免疫印迹分析进行了验证。对携带S621G突变的患者成纤维细胞来源的诱导多能干细胞(iPSC)进行蛋白质组学分析,显示这些途径同样被激活,为这些候选基因突变成为进一步验证和机制研究(如E3酶活性测定、蛋白质 - 蛋白质和蛋白质 - 底物研究,以及斑马鱼中的神经元凋亡和异常分支测量)的有力候选者提供了令人信服的证据。我们的蛋白质基因组学方法具有很大的实用性,并提供了一个相对高通量的筛选平台,以探索候选基因突变导致神经元细胞死亡的倾向,这将指导研究人员进行进一步的实验研究。
