Animal Biology Department, Faculty of Natural Sciences, University of Tabriz, Tabriz, Iran.
Center of Excellence for Biodiversity, Faculty of Natural Sciences, University of Tabriz, Tabriz, Iran.
J Neurogenet. 2024 Mar;38(1):19-25. doi: 10.1080/01677063.2024.2365634. Epub 2024 Jun 17.
HERC2-associated neurodevelopmental-disorders(NDD) encompass a cluster of medical conditions that arise from genetic mutations occurring within the gene. These disorders can manifest a spectrum of symptoms that impact the brain and nervous system, including delayed psychomotor development, severe mental retardation, seizures and autistic features. Whole-Exome-Sequencing(WES) was performed on a ten-year-old male patient referred to the genetic center for genetic analysis. Blood samples were collected from the proband, his parents, and his sister to extract DNA. PCR-Sanger-sequencing was utilized to validate the findings obtained from WES. In order to obtain a more thorough understanding of the impact of the mutation, an extensive analysis was conducted using bioinformatics tools. WES data analysis identified a homozygous single nucleotide change(C > T) at position c14215 located in exon ninety-two of the gene (NC_000015.10(NM_004667.6):c.14215C > T). The absence of this mutation among our cohort composed of four hundred normal healthy adults from the same ethnic group, and its absence in any other population database, confirms the pathogenicity of the mutation. This study revealed that the substitution of arginine with a stop codon within the Hect domain caused a premature stop codon at position 4739(p.Arg4739Ter). This mutation significantly results in the production of a truncated HERC2 protein with an incomplete HECT domain. In the final stage of ubiquitin attachment, HECT E3 ubiquitin ligases play a catalytic role by creating a thiolester intermediate using their conserved catalytic cysteine (Cys4762). This intermediate is formed before ubiquitin is transferred to a substrate protein. The truncation of the HERC2 protein is expected to disrupt its ability to perform this function, which could potentially hinder important regulatory processes related to the development and maintenance of synapses. The identification of a novel pathogenic variant, NC_000015.10(NM_004667.6):c.14215C > T, located within the ninety-two exon of the gene, is notable for its association with an autosomal recessive inheritance pattern in cases of Intellectual Developmental Disorder(IDD). In the end, this variant could potentially play a part in the underlying mechanisms leading to the onset of intellectual developmental disorder.
HERC2 相关神经发育障碍 (NDD) 涵盖了一组由基因内发生的基因突变引起的疾病。这些疾病可能表现出一系列影响大脑和神经系统的症状,包括精神运动发育迟缓、严重智力障碍、癫痫发作和自闭症特征。对一名十岁男性患者进行了全外显子组测序 (WES),该患者被转介至遗传中心进行基因分析。从先证者、其父母和姐姐采集血液样本以提取 DNA。利用 PCR-Sanger 测序验证从 WES 获得的发现。为了更全面地了解突变的影响,使用生物信息学工具对其进行了广泛分析。WES 数据分析在 基因的外显子 92 中发现了一个纯合单核苷酸变化 (C > T),位置为 c14215(NC_000015.10(NM_004667.6):c.14215C > T)。在我们的 400 名来自同一族群的正常健康成年人组成的队列中,没有发现该突变,在任何其他人群数据库中也没有发现该突变,这证实了该突变的致病性。这项研究表明,在 Hect 结构域内精氨酸被替换为一个终止密码子,导致 4739 位提前出现终止密码子 (p.Arg4739Ter)。该突变显著导致 HERC2 蛋白产生截短,其 HECT 结构域不完整。在泛素附着的最后阶段,HECT E3 泛素连接酶通过其保守的催化半胱氨酸 (Cys4762) 形成硫酯中间体,发挥催化作用。在泛素转移到底物蛋白之前形成该中间体。HERC2 蛋白的截断预计会破坏其执行此功能的能力,这可能会阻碍与突触发育和维持相关的重要调节过程。鉴定出一种新的致病性变体,NC_000015.10(NM_004667.6):c.14215C > T,位于 基因的外显子 92 内,与常染色体隐性遗传模式相关,与智力发育障碍 (IDD) 有关。最后,该变体可能在导致智力发育障碍的潜在机制中发挥作用。
