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人群暴露于苯的全基因表达反应:探索 RNA 测序技术应用的初步研究。

Global gene expression response of a population exposed to benzene: a pilot study exploring the use of RNA-sequencing technology.

机构信息

School of Public Health, University of California, Berkeley, California 94720-7356, USA.

出版信息

Environ Mol Mutagen. 2013 Aug;54(7):566-73. doi: 10.1002/em.21801. Epub 2013 Aug 1.

Abstract

The mechanism of toxicity of the leukemogen benzene is not entirely known. This pilot study used RNA-sequencing (RNA-seq) technology to examine the effect of benzene exposure on gene expression in peripheral blood mononuclear cells obtained from 10 workers occupationally exposed to high levels of benzene (≥5 ppm) in air and 10 matched unexposed control workers, from a large study (n = 125) in which gene expression was previously measured by microarray. RNA-seq is more sensitive and has a wider dynamic range for the quantification of gene expression. Further, it has the ability to detect novel transcripts and alternative splice variants. The main conclusions from our analysis of the 20 workers by RNA-seq are as follows: The Pearson correlation between the two technical replicates for the RNA-seq experiments was 0.98 and the correlation between RNA-seq and microarray signals for the 20 subjects was around 0.6. 60% of the transcripts with detected reads from the RNA-seq experiments did not have corresponding probes on the microarrays. Fifty-three percent of the transcripts detected by RNA-seq and 99% of those with probes on the microarray were protein-coding. There was a significant overlap (P < 0.05) in transcripts declared differentially expressed due to benzene exposure using the two technologies. About 20% of the transcripts declared differentially expressed using the RNA-seq data were non-coding transcripts. Six transcripts were determined (false-discovery rate < 0.05) to be alternatively spliced as a result of benzene exposure. Overall, this pilot study shows that RNA-seq can complement the information obtained by microarray in the analysis of changes in transcript expression from chemical exposures.

摘要

苯致白血病的毒性机制尚不完全清楚。本初步研究采用 RNA 测序(RNA-seq)技术,检测了 10 名职业性暴露于空气中高浓度苯(≥5ppm)的工人(n=10)和 10 名匹配的未暴露对照工人(n=10)外周血单个核细胞中基因表达的变化。这些工人均来自于一项之前使用微阵列检测过基因表达的大型研究。RNA-seq 技术在检测基因表达方面具有更高的灵敏度和更宽的动态范围,且具有检测新转录本和选择性剪接变体的能力。通过 RNA-seq 对 20 名工人进行分析的主要结论如下:RNA-seq 实验的两个技术重复之间的 Pearson 相关系数为 0.98,20 名受试者的 RNA-seq 和微阵列信号之间的相关性约为 0.6。从 RNA-seq 实验中检测到的具有检测到的读数的转录本中,有 60%没有相应的微阵列探针。RNA-seq 检测到的转录本中有 53%和微阵列上有探针的转录本中有 99%为编码蛋白的转录本。使用两种技术检测到的由于苯暴露而差异表达的转录本之间存在显著重叠(P<0.05)。使用 RNA-seq 数据检测到的约 20%差异表达的转录本是非编码转录本。有 6 个转录本被确定(错误发现率<0.05)为苯暴露导致的选择性剪接。总的来说,这项初步研究表明,RNA-seq 可以补充微阵列分析化学暴露引起的转录本表达变化的信息。

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