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使用剪接报告基因小基因检测法评估未分类遗传变异对剪接的影响。

Use of splicing reporter minigene assay to evaluate the effect on splicing of unclassified genetic variants.

作者信息

Gaildrat Pascaline, Killian Audrey, Martins Alexandra, Tournier Isabelle, Frébourg Thierry, Tosi Mario

机构信息

Faculty of Medicine Department of Genetics and Institute for Biomedical Research, Rouen University Hospital, Inserm U614, IFRMP, University of Rouen, Northwest Canceropole, Rouen, France.

出版信息

Methods Mol Biol. 2010;653:249-57. doi: 10.1007/978-1-60761-759-4_15.

Abstract

The interpretation of the numerous sequence variants of unknown biological and clinical significance (UV for "unclassified variant") found in genetic screenings represents a major challenge in the molecular diagnosis of genetic disease, including cancer susceptibility. A fraction of UVs may be deleterious because they affect mRNA splicing. Here, we describe a functional splicing assay based on a minigene construct that assesses the impact of sequence variants on splicing. A genomic segment encompassing the variant sequence of interest along with flanking intronic sequences is PCR-amplified from patient genomic DNA and is cloned into a minigene vector. After transient transfection into cultured cells, the splicing patterns of the transcripts generated from the wild-type and from the variant constructs are compared by reverse transcription-PCR analysis and sequencing. This method represents a complementary approach to reverse transcription-PCR analyses of patient RNA, for the identification of pathogenic splicing mutations.

摘要

在包括癌症易感性在内的遗传疾病分子诊断中,解读基因筛查中发现的众多生物学和临床意义未知的序列变异(UV,即“未分类变异”)是一项重大挑战。一部分UV可能是有害的,因为它们会影响mRNA剪接。在此,我们描述了一种基于小基因构建体的功能性剪接检测方法,该方法可评估序列变异对剪接的影响。从患者基因组DNA中通过PCR扩增包含感兴趣变异序列及其侧翼内含子序列的基因组片段,并将其克隆到小基因载体中。在瞬时转染到培养细胞后,通过逆转录PCR分析和测序比较野生型和变异构建体产生的转录本的剪接模式。该方法是对患者RNA进行逆转录PCR分析的一种补充方法,用于鉴定致病性剪接突变。

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