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Keywords {🔍}

rna, pubmed, rnaseq, article, expression, ribozero, polya, rnas, reads, google, scholar, intronic, genes, nuclear, table, cas, figure, sequencing, gene, file, methods, total, trizol, rpkm, data, qiagen, additional, analysis, central, extraction, protocols, coding, cells, transcripts, human, fraction, values, expressed, levels, detected, cytoplasmic, noncoding, lncrnas, exonic, differences, number, transcriptome, higher, polyadenylated, method,

Topics {✒️}

13/bioc/vignettes/noiseq/inst/doc/noiseq hans lehrach & marie-laure yaspo rrna-depleted rna-seq procedures strand-specific rna-seq protocols replication-dependent histone cluster marie-laure yaspo x-inactive specific transcript article download pdf rrna depletion-based sequencing u7 snrnp-mediated cleavage open access license polya-selected rna-sequencing replication-dependent histone mrnas replication-dependent histone genes export factor tap/nxf1 microarray quality control nuclear rna metabolism ribo-minus rna-sequencing ribozero rna-seq showed main rna-seq approaches ribozero rna-seq data qiagen rna/ribozero outcomes rna-seq data analysis trizol-ribozero rna-seq related subjects rna-seq selection procedure trizol-based rna extraction silica column-based method qiagen ribozero rna-seq rrna-depleted procedures rna-seq data originating illumina truseq rna strand-specific protocols nuclear-fractionated rna processed full size image rna-seq datasets article sultan statistical tests exploiting qiagen-extracted total rna hek rna-seq experiments privacy choices/manage cookies full access strand master mix st laurent chromatin signature reveals phenol-chloroform based histone cluster genes cell rna reveals rna-seq approaches library preparation protocols

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         headline:Influence of RNA extraction methods and library selection schemes on RNA-seq data
         description:Gene expression analysis by RNA sequencing is now widely used in a number of applications surveying the whole transcriptomes of cells and tissues. The recent introduction of ribosomal RNA depletion protocols, such as RiboZero, has extended the view of the polyadenylated transcriptome to the poly(A)- fraction of the RNA. However, substantial amounts of intronic transcriptional activity has been reported in RiboZero protocols, raising issues regarding their potential nuclear origin and the impact on the actual sequence depth in exonic regions. Using HEK293 human cells as source material, we assessed here the impact of the two commonly used RNA extraction methods and of the library construction protocols (rRNA depletion versus mRNA) on 1) the relative abundance of intronic reads and 2) on the estimation of gene expression values. We benchmarked the rRNA depletion-based sequencing with a specific analysis of the cytoplasmic and nuclear transcriptome fractions, suggesting that the large majority of the intronic reads correspond to unprocessed nuclear transcripts rather than to independent transcriptional units. We show that Qiagen or TRIzol extraction methods retain differentially nuclear RNA species, and that consequently, rRNA depletion-based RNA sequencing protocols are particularly sensitive to the extraction methods. We could show that the combination of Trizol-based RNA extraction with rRNA depletion sequencing protocols led to the largest fraction of intronic reads, after the sequencing of the nuclear transcriptome. We discuss here the impact of the various strategies on gene expression and alternative splicing estimation measures. Further, we propose guidelines and a double selection strategy for minimizing the expression biases, without loss of information.
         datePublished:2014-08-11T00:00:00Z
         dateModified:2014-08-11T00:00:00Z
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            rRNA depletion
            poly(A)+ selection
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            Life Sciences
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            Proteomics
            Animal Genetics and Genomics
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      headline:Influence of RNA extraction methods and library selection schemes on RNA-seq data
      description:Gene expression analysis by RNA sequencing is now widely used in a number of applications surveying the whole transcriptomes of cells and tissues. The recent introduction of ribosomal RNA depletion protocols, such as RiboZero, has extended the view of the polyadenylated transcriptome to the poly(A)- fraction of the RNA. However, substantial amounts of intronic transcriptional activity has been reported in RiboZero protocols, raising issues regarding their potential nuclear origin and the impact on the actual sequence depth in exonic regions. Using HEK293 human cells as source material, we assessed here the impact of the two commonly used RNA extraction methods and of the library construction protocols (rRNA depletion versus mRNA) on 1) the relative abundance of intronic reads and 2) on the estimation of gene expression values. We benchmarked the rRNA depletion-based sequencing with a specific analysis of the cytoplasmic and nuclear transcriptome fractions, suggesting that the large majority of the intronic reads correspond to unprocessed nuclear transcripts rather than to independent transcriptional units. We show that Qiagen or TRIzol extraction methods retain differentially nuclear RNA species, and that consequently, rRNA depletion-based RNA sequencing protocols are particularly sensitive to the extraction methods. We could show that the combination of Trizol-based RNA extraction with rRNA depletion sequencing protocols led to the largest fraction of intronic reads, after the sequencing of the nuclear transcriptome. We discuss here the impact of the various strategies on gene expression and alternative splicing estimation measures. Further, we propose guidelines and a double selection strategy for minimizing the expression biases, without loss of information.
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      dateModified:2014-08-11T00:00:00Z
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         RNA extraction
         rRNA depletion
         poly(A)+ selection
         Intronic reads
         Life Sciences
         general
         Microarrays
         Proteomics
         Animal Genetics and Genomics
         Microbial Genetics and Genomics
         Plant Genetics and Genomics
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