Sahar Al Seesi scite author profile

Mutation in minor spliceosome components is linked to the developmental disorder microcephalic osteodysplastic primordial dwarfism type 1 (MOPD1). Here, we inactivated the minor spliceosome in the developing mouse cortex (pallium) by ablating , which encodes the crucial minor spliceosome small nuclear RNA (snRNA) U11. conditional knockout mice were born with microcephaly, which was caused by the death of self-amplifying radial glial cells (RGCs), while intermediate progenitor cells and neurons were produced. RNA sequencing suggested that this cell death was mediated by upregulation of p53 (Trp53 - Mouse Genome Informatics) and DNA damage, which were both observed specifically in U11-null RGCs. Moreover, U11 loss caused elevated minor intron retention in genes regulating the cell cycle, which was consistent with fewer RGCs in S-phase and cytokinesis, alongside prolonged metaphase in RGCs. In all, we found that self-amplifying RGCs are the cell type most sensitive to loss of minor splicing. Together, these findings provide a potential explanation of how disruption of minor splicing might cause microcephaly in MOPD1.

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Bootstrap-based differential gene expression analysis for RNA-Seq data with and without replicates

Seesi

Tiagueu

Zelikovsky

et al. 2014

BMC Genomics

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A major application of RNA-Seq is to perform differential gene expression analysis. Many tools exist to analyze differentially expressed genes in the presence of biological replicates. Frequently, however, RNA-Seq experiments have no or very few biological replicates and development of methods for detecting differentially expressed genes in these scenarios is still an active research area.In this paper we introduce a novel method, called IsoDE, for differential gene expression analysis based on bootstrapping. We compared IsoDE against four existing methods (Fisher's exact test, GFOLD, edgeR and Cuffdiff) on RNA-Seq datasets generated using three different sequencing technologies, both with and without replicates. Experiments on MAQC RNA-Seq datasets without replicates show that IsoDE has consistently high accuracy as defined by the qPCR ground truth, frequently higher than that of the compared methods, particularly for low coverage data and at lower fold change thresholds. In experiments on RNA-Seq datasets with up to 7 replicates, IsoDE has also achieved high accuracy. Furthermore, unlike GFOLD and edgeR, IsoDE accuracy varies smoothly with the number of replicates, and is relatively uniform across the entire range of gene expression levels.The proposed non-parametric method based on bootstrapping has practical running time, and achieves robust performance over a broad range of technologies, number of replicates, sequencing depths, and minimum fold change thresholds.

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Fast bootstrapping-based estimation of confidence intervals of expression levels and differential expression from RNA-Seq data

Mandric

Temate‐Tiagueu

Shcheglova

et al. 2017

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Sahar Al Seesi

Key Parameters of Tumor Epitope Immunogenicity Revealed Through a Consortium Approach Improve Neoantigen Prediction

Genomic and bioinformatic profiling of mutational neoepitopes reveals new rules to predict anticancer immunogenicity

Minor spliceosome inactivation causes microcephaly, owing to cell cycle defects and death of self-amplifying radial glial cells

Bootstrap-based differential gene expression analysis for RNA-Seq data with and without replicates

Fast bootstrapping-based estimation of confidence intervals of expression levels and differential expression from RNA-Seq data

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