RNA-Seq Reveals Novel Transcriptional Reorganization in Human Alcoholic Brain

被引:41
作者
Farris, Sean P. [1 ]
Mayfield, R. Dayne [1 ]
机构
[1] Univ Texas Austin, Waggoner Ctr Alcohol & Addict Res, Austin, TX 78712 USA
来源
BRAIN TRANSCRIPTOME | 2014年 / 116卷
关键词
DIFFERENTIAL EXPRESSION ANALYSIS; LONG NONCODING RNA; SMALL NUCLEOLAR RNAS; GENE-EXPRESSION; MESSENGER-RNA; COEXPRESSION NETWORKS; SYNAPTIC PLASTICITY; LANDSCAPE; GENOME; NORMALIZATION;
D O I
10.1016/B978-0-12-801105-8.00011-4
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
DNA microarrays have been used for over a decade to profile gene expression on a genomic scale. While this technology has advanced our understanding of complex cellular function, the reliance of microarrays on hybridization kinetics results in several technical limitations. For example, knowledge of the sequences being probed is required, distinguishing similar sequences is difficult because of cross-hybridization, and the relatively narrow dynamic range of the signal limits sensitivity. Recently, new technologies have been introduced that are based on novel sequencing methodologies. These next-generation sequencing methods do not have the limitations inherent to microarrays. Next-generation sequencing is unique since it allows the detection of all known and novel RNAs present in biological samples without bias toward known transcripts. In addition, the expression of coding and noncoding RNAs, alternative splicing events, and expressed single nucleotide polymorphisms (SNPs) can be identified in a single experiment. Furthermore, this technology allows for remarkably higher throughput while lowering sequencing costs. This significant shift in throughput and pricing makes low-cost access to whole genomes possible and more importantly expands sequencing applications far beyond traditional uses (Morozova &Marra, 2008) to include sequencing the transcriptome (RNA-Seq), providing detail on gene structure, alternative splicing events, expressed SNPs, and transcript size (Mane et al., 2009; Tang et al., 2009; Walter et al., 2009), in a single experiment, while also quantifying the absolute abundance of genes, all with greater sensitivity and dynamic range than the competing cDNA microarray technology (Mortazavi, Williams, McCue, Schaeffer, & Wold, 2008).
引用
收藏
页码:275 / 300
页数:26
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