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Transcriptome genetics using second generation sequencing in a Caucasian population

国际人类基因组单体型图计划 生物 遗传学 表达数量性状基因座 转录组 DNA微阵列 选择性拼接 单核苷酸多态性 RNA序列 数量性状位点 DNA测序 基因 计算生物学 外显子 基因表达 基因型
作者
Stephen B. Montgomery,Michael Sammeth,María Gutiérrez‐Arcelus,Radosław Lach,Catherine Ingle,James Nisbett,Roderic Guigó,Emmanouil T. Dermitzakis
出处
期刊:Nature [Springer Nature]
卷期号:464 (7289): 773-777 被引量:823
标识
DOI:10.1038/nature08903
摘要

Gene expression is an important phenotype that informs about genetic and environmental effects on cellular state. Many studies have previously identified genetic variants for gene expression phenotypes using custom and commercially available microarrays. Second generation sequencing technologies are now providing unprecedented access to the fine structure of the transcriptome. We have sequenced the mRNA fraction of the transcriptome in 60 extended HapMap individuals of European descent and have combined these data with genetic variants from the HapMap3 project. We have quantified exon abundance based on read depth and have also developed methods to quantify whole transcript abundance. We have found that approximately 10 million reads of sequencing can provide access to the same dynamic range as arrays with better quantification of alternative and highly abundant transcripts. Correlation with SNPs (small nucleotide polymorphisms) leads to a larger discovery of eQTLs (expression quantitative trait loci) than with arrays. We also detect a substantial number of variants that influence the structure of mature transcripts indicating variants responsible for alternative splicing. Finally, measures of allele-specific expression allowed the identification of rare eQTLs and allelic differences in transcript structure. This analysis shows that high throughput sequencing technologies reveal new properties of genetic effects on the transcriptome and allow the exploration of genetic effects in cellular processes.

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