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TIN: An R Package for Transcriptome Instability Analysis

机译:TIN:用于转录组稳定性分析的R包

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Alternative splicing is a key regulatory mechanism for gene expression, vital for the proper functioning of eukaryotic cells. Disruption of normal pre-mRNA splicing has the potential to cause and reinforce human disease. Owing to rapid advances in high-throughput technologies, it is now possible to identify novel mRNA isoforms and detect aberrant splicing patterns on a genome scale, across large data sets. Analogous to the genomic types of instability describing cancer genomes (eg, chromosomal instability and microsatellite instability), transcriptome instability (TIN) has recently been proposed as a splicing-related genome-wide characteristic of certain solid cancers. We present the R package TIN, available from Bioconductor, which implements a set of methods for TIN analysis based on exon-level microarray expression profiles. TIN provides tools for estimating aberrant exon usage across samples and for analyzing correlation patterns between TIN and splicing factor expression levels.
机译:替代剪接是基因表达的关键调节机制,对于真核细胞的适当功能至关重要。正常前mRNA剪接的破坏具有引起和增强人类疾病的可能性。由于高通量技术的快速进展,现在可以在大型数据集中识别新型mRNA同种型并检测基因组规模的异常剪接模式。类似于描述癌症基因组(例如,染色体不稳定性和微卫星不稳定性)的不稳定性的基因组类型,最近已经提出了转录组不稳定性(锡)作为某些固体癌的剪接相关基因组特征。我们介绍了从生物导体中获得的R包锡,其利用基于外显子级微阵列表达谱的锡分析方法。锡提供用于估计样品的异常外显子使用的工具,并用于分析锡和剪接因子表达水平之间的相关模式。

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