Monoallelic de novo variants in DDX17 cause a neurodevelopmental disorder

基因敲除 生物 表型 神经突 轴突引导 轴突 神经科学 遗传学 基因 细胞生物学 体外
作者
Eleanor G. Seaby,Annie Godwin,Géraldine Meyer-Dilhet,Valentine Clerc,Xavier Grand,Tia Fletcher,Laloé Monteiro,Martijn Kerkhofs,Valério Carelli,Flavia Palombo,Marco Seri,Giulia Olivucci,Mina Grippa,Claudia Ciaccio,Stefano D’Arrigo,Maria Iascone,Marion Bermudez,J. Fischer,Nataliya Di Donato,Sophie Goesswein,Marco L. Leung,Daniel C. Koboldt,Cortlandt Myers,Gudny A. Arnadottir,Kári Stéfansson,Patrick Sulem,Ethan M. Goldberg,Ange-Line Bruel,Frédéric Tran Mau‐Them,Marjolaine Willems,Hans T. Björnsson,Hakon Bjorn Hognason,Eirny Tholl Thorolfsdottir,Emanuele Agolini,Antonio Novelli,Giuseppe Zampino,Roberta Onesimo,Katherine Lachlan,Diana Baralle,Heidi L. Rehm,Anne O’Donnell‐Luria,Julien Courchet,Matthew Guille,Cyril F. Bourgeois,Sarah Ennis
出处
期刊:Brain [Oxford University Press]
标识
DOI:10.1093/brain/awae320
摘要

Abstract DDX17 is an RNA helicase shown to be involved in critical processes during the early phases of neuronal differentiation. Globally, we compiled a case-series of 11 patients with neurodevelopmental phenotypes harbouring de novo monoallelic variants in DDX17. All 11 patients in our case series had a neurodevelopmental phenotype, whereby intellectual disability, delayed speech and language, and motor delay predominated. We performed in utero cortical electroporation in the brain of developing mice, assessing axon complexity and outgrowth of electroporated neurons, comparing wild-type and Ddx17 knockdown. We then undertook ex vivo cortical electroporation on neuronal progenitors to quantitatively assess axonal development at a single cell resolution. Mosaic ddx17 crispants and heterozygous knockouts in Xenopus tropicalis were generated for assessment of morphology, behavioural assays, and neuronal outgrowth measurements. We further undertook transcriptomic analysis of neuroblastoma SH-SY5Y cells, to identify differentially expressed genes in DDX17-KD cells compared to controls. Knockdown of Ddx17 in electroporated mouse neurons in vivo showed delayed neuronal migration as well as decreased cortical axon complexity. Mouse primary cortical neurons revealed reduced axon outgrowth upon knockdown of Ddx17 in vitro. The axon outgrowth phenotype was replicated in crispant ddx17 tadpoles and in heterozygotes. Heterozygous tadpoles had clear neurodevelopmental defects and showed an impaired neurobehavioral phenotype. Transcriptomic analysis identified a statistically significant number of differentially expressed genes involved in neurodevelopmental processes in DDX17-KD cells compared to control cells. We have identified potential neurodevelopment disease-causing variants in a gene not previously associated with genetic disease, DDX17. We provide evidence for the role of the gene in neurodevelopment in both mammalian and non-mammalian species and in controlling the expression of key neurodevelopment genes.
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