An overview of RB1 transcript alterations detected during retinoblastoma genetic screening.

IF 1.2 4区 医学 Q4 GENETICS & HEREDITY
Ophthalmic Genetics Pub Date : 2024-06-01 Epub Date: 2023-11-06 DOI:10.1080/13816810.2023.2270570
Elizabeth A Price, Mandeep S Sagoo, M Ashwin Reddy, Zerrin Onadim
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引用次数: 0

Abstract

Identification of pathogenic RB1 variants aids in the clinical management of families with retinoblastoma. We routinely screen DNA for RB1 variants, but transcript analysis can also be used for variant screening, and to help decide variant pathogenicity. DNA was screened by conformation analysis followed by Sanger sequencing. Large deletion/insertions were detected by polymorphism analysis, MLPA and quantitative-PCR. Methylation-specific PCR was used to detect hypermethylation. RNA screening was performed when a DNA pathogenic variant was missing, or to determine effects on splicing.Two hundred and thirteen small coding variants were predicted to affect splicing in 207 patients. Splice donor (sd) variants were nearly twice as frequent as splice acceptor (sa) with the most affected positions being sd + 1 and sa-1. Some missense and nonsense codons altered splicing, while some splice consensus variants did not. Large deletion/insertions can disrupt splicing, but RNA analysis showed that some of these are more complex than indicated by DNA testing. RNA screening found pathogenic variants in 53.8% of samples where DNA analysis did not. RB1 splicing is altered by changes at consensus splice sites, some missense and nonsense codons, deep intronic changes and large deletion/insertions. Common alternatively spliced transcripts may complicate analysis. An effective molecular screening strategy would include RNA analysis to help determine pathogenicity.

视网膜母细胞瘤基因筛查中检测到的RB1转录物改变综述。
致病性RB1变异体的鉴定有助于视网膜母细胞瘤家族的临床管理。我们常规筛选DNA中的RB1变体,但转录物分析也可用于变体筛选,并有助于确定变体的致病性。通过构象分析和Sanger测序对DNA进行筛选。通过多态性分析、MLPA和定量PCR检测大的缺失/插入。甲基化特异性PCR用于检测高甲基化。当DNA致病性变体缺失时进行RNA筛选,或确定对剪接的影响。213个小编码变体被预测会影响207名患者的剪接。剪接供体(sd)变异的频率几乎是剪接受体(sa)的两倍,受影响最大的位置是sd + 1和sa-1。一些错义和无义密码子改变了剪接,而一些剪接一致变体则没有。大量的缺失/插入会破坏剪接,但RNA分析表明,其中一些比DNA测试显示的更复杂。RNA筛查在53.8%的样本中发现了致病性变异,而DNA分析没有发现。RB1剪接通过共有剪接位点的变化、一些错义和无义密码子、深层内含子变化和大的缺失/插入而改变。常见的选择性剪接转录物可能会使分析复杂化。一种有效的分子筛选策略包括RNA分析,以帮助确定致病性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Ophthalmic Genetics
Ophthalmic Genetics 医学-眼科学
CiteScore
2.40
自引率
8.30%
发文量
126
审稿时长
>12 weeks
期刊介绍: Ophthalmic Genetics accepts original papers, review articles and short communications on the clinical and molecular genetic aspects of ocular diseases.
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