常染色体显性视网膜色素变性与不完全外显性由于内含子突变的PRPF31基因。

IF 1.8 3区 医学 Q4 BIOCHEMISTRY & MOLECULAR BIOLOGY
Molecular Vision Pub Date : 2022-01-01
Tahleel Ali-Nasser, Shiri Zayit-Soudry, Eyal Banin, Dror Sharon, Tamar Ben-Yosef
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引用次数: 0

摘要

目的:探讨不完全外显性常染色体显性视网膜色素变性(adRP)在以色列穆斯林阿拉伯家族中的发病机制。方法:对2例adRP患者进行了详细的眼科检查,包括眼底检查、视野测试、光学相干断层扫描和视网膜电图。遗传分析采用全外显子组测序(WES)和Sanger测序。鉴定出的内含子变异的致病性使用几种基于网络的工具进行了计算机评估,在体外使用基于微基因的测定,在体内使用淋巴细胞来源RNA的反转录PCR分析。选择性剪接转录本的相对丰度使用基于扩增子的下一代测序进行评估。采用定量PCR (qPCR)检测PRPF31和CNOT3的相对表达量。结果:本研究纳入的2例患者均为儿童期发病的RP,以夜盲症为首发症状,随后出现视野同心受限。眼底检查结果包括视网膜血管狭窄和周围骨刺色素沉着。到了生命的第三个十年,全视场视网膜电图的发现已经明显减弱。在这些患者中,我们在PRPF31内含子11 +5位置发现了一个新的杂合内含子变异(c.1146+5G>T)。在一名无症状的家庭成员中也检测到相同的变异。通过计算机分析,预测该变异会改变内含子11的剪接。体外剪接实验和淋巴细胞源性RNA的反转录PCR分析显示,突变等位基因主要产生一个较短的转录本,其中外显子11被跳过。预计外显子11的跳过会导致移码和异常截断蛋白(p.Tyr359Serfs*29)。qPCR分析显示突变携带者的PRPF31表达水平降低,受影响患者与其无症状兄弟之间无显著差异。我们评估了与PRPF31突变非外显性相关的几个因素,包括PRPF31核心启动子附近的顺式作用MSR1元件的数量、CNOT3表达水平和CNOT3 rs4806718单核苷酸多态性。在本研究中,这些因素都与家族的非外显性无关。结论:我们报道了一种新的PRPF31内含子突变,该突变是adRP的基础。本报告扩展了PRPF31的致病突变谱,并进一步证明了内含子突变的重要性。此外,它还证明了先前与PRPF31突变相关的不完全外显率现象。在本研究中,该家族的非外显性无法用任何已知机制来解释,这一事实表明,一种新的PRPF31外显性修饰子可能起到了作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Autosomal dominant retinitis pigmentosa with incomplete penetrance due to an intronic mutation of the <i>PRPF31</i> gene.

Autosomal dominant retinitis pigmentosa with incomplete penetrance due to an intronic mutation of the <i>PRPF31</i> gene.

Autosomal dominant retinitis pigmentosa with incomplete penetrance due to an intronic mutation of the <i>PRPF31</i> gene.

Autosomal dominant retinitis pigmentosa with incomplete penetrance due to an intronic mutation of the PRPF31 gene.

Purpose: To identify the molecular mechanisms of the development of autosomal dominant retinitis pigmentosa (adRP) with incomplete penetrance in an Israeli Muslim Arab family.

Methods: Two patients with adRP underwent a detailed ophthalmic evaluation, including funduscopic examination, visual field testing, optical coherence tomography, and electroretinography. Genetic analysis was performed using a combination of whole exome sequencing (WES) and Sanger sequencing. The pathogenicity of the identified intronic variant was evaluated in silico using several web-based tools, in vitro using a minigene-based assay, and in vivo using reverse transcription PCR analysis of lymphocyte-derived RNA. The relative abundance of alternatively spliced transcripts was evaluated using amplicon-based next-generation sequencing. The relative expression levels of PRPF31 and CNOT3 were measured using quantitative PCR (qPCR) analysis.

Results: The two patients recruited in this study had childhood-onset RP, with night blindness as the initial symptom, followed by concentric restriction of the visual field. The funduscopic findings included narrowed retinal blood vessels and peripheral bone spicule pigmentation. By the third decade of life, the full-field electroretinography findings had been remarkably attenuated. In these patients, we identified a novel heterozygous intronic variant at position +5 of PRPF31 intron 11 (c.1146+5G>T). The same variant was also detected in one asymptomatic family member. Through in silico analysis, the variant was predicted to alter the splicing of intron 11. An in vitro splicing assay and a reverse transcription PCR analysis of lymphocyte-derived RNA revealed that the mutant allele yielded mainly a shorter transcript in which exon 11 was skipped. The skipping of exon 11 was expected to cause a frameshift and an aberrant truncated protein (p.Tyr359Serfs*29). The qPCR analysis revealed reduced PRPF31 expression levels in the mutation carriers, without a significant difference between the affected patient and his asymptomatic brother. We evaluated several factors that have been suggested to correlate with non-penetrance of PRPF31 mutations, including the number of cis-acting MSR1 elements adjacent to the PRPF31 core promoter, CNOT3 expression level, and CNOT3 rs4806718 single-nucleotide polymorphism. None of these factors correlated with non-penetrance in the family in this study.

Conclusions: We report a novel intronic mutation in PRPF31 underlying adRP. This report expands the spectrum of pathogenic mutations in PRPF31 and further demonstrates the importance of intronic mutations. Moreover, it demonstrates the phenomenon of incomplete penetrance previously associated with PRPF31 mutations. The fact that the non-penetrance in the family in this study could not be explained by any of the known mechanisms suggests the possible contribution of a novel modifier of PRPF31 penetrance.

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来源期刊
Molecular Vision
Molecular Vision 生物-生化与分子生物学
CiteScore
4.40
自引率
0.00%
发文量
25
审稿时长
1 months
期刊介绍: Molecular Vision is a peer-reviewed journal dedicated to the dissemination of research results in molecular biology, cell biology, and the genetics of the visual system (ocular and cortical). Molecular Vision publishes articles presenting original research that has not previously been published and comprehensive articles reviewing the current status of a particular field or topic. Submissions to Molecular Vision are subjected to rigorous peer review. Molecular Vision does NOT publish preprints. For authors, Molecular Vision provides a rapid means of communicating important results. Access to Molecular Vision is free and unrestricted, allowing the widest possible audience for your article. Digital publishing allows you to use color images freely (and without fees). Additionally, you may publish animations, sounds, or other supplementary information that clarifies or supports your article. Each of the authors of an article may also list an electronic mail address (which will be updated upon request) to give interested readers easy access to authors.
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