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小鼠胚胎干细胞神经分化过程中视黄酸应答的阶段特异性基因表达特征鉴定

Identification of Stage-Specific Gene Expression Signatures in Response to Retinoic Acid during the Neural Differentiation of Mouse Embryonic Stem Cells.

作者信息

Akanuma Hiromi, Qin Xian-Yang, Nagano Reiko, Win-Shwe Tin-Tin, Imanishi Satoshi, Zaha Hiroko, Yoshinaga Jun, Fukuda Tomokazu, Ohsako Seiichiroh, Sone Hideko

机构信息

Health Risk Research Section, Center for Environmental Risk Research, National Institute for Environmental Studies Tsukuba, Ibaraki, Japan.

出版信息

Front Genet. 2012 Aug 7;3:141. doi: 10.3389/fgene.2012.00141. eCollection 2012.

Abstract

We have previously established a protocol for the neural differentiation of mouse embryonic stem cells (mESCs) as an efficient tool to evaluate the neurodevelopmental toxicity of environmental chemicals. Here, we described a multivariate bioinformatic approach to identify the stage-specific gene sets associated with neural differentiation of mESCs. We exposed mESCs (B6G-2 cells) to 10(-8) or 10(-7) M of retinoic acid (RA) for 4 days during embryoid body formation and then performed morphological analysis on day of differentiation (DoD) 8 and 36, or genomic microarray analysis on DoD 0, 2, 8, and 36. Three gene sets, namely a literature-based gene set (set 1), an analysis-based gene set (set 2) using self-organizing map and principal component analysis, and an enrichment gene set (set 3), were selected by the combined use of knowledge from literatures and gene information selected from the microarray data. A gene network analysis for each gene set was then performed using Bayesian statistics to identify stage-specific gene expression signatures in response to RA during mESC neural differentiation. Our results showed that RA significantly increased the size of neurosphere, neuronal cells, and glial cells on DoD 36. In addition, the gene network analysis showed that glial fibrillary acidic protein, a neural marker, remarkably up-regulates the other genes in gene set 1 and 3, and Gbx2, a neural development marker, significantly up-regulates the other genes in gene set 2 on DoD 36 in the presence of RA. These findings suggest that our protocol for identification of developmental stage-specific gene expression and interaction is a useful method for the screening of environmental chemical toxicity during neurodevelopmental periods.

摘要

我们之前建立了一套用于小鼠胚胎干细胞(mESCs)神经分化的方案,作为评估环境化学物质神经发育毒性的有效工具。在此,我们描述了一种多变量生物信息学方法,以识别与mESCs神经分化相关的阶段特异性基因集。在胚胎体形成过程中,我们将mESCs(B6G - 2细胞)暴露于10⁻⁸或10⁻⁷ M的视黄酸(RA)中4天,然后在分化第8天和第36天进行形态学分析,或在分化第0天、第2天、第8天和第36天进行基因组微阵列分析。通过结合文献知识和从微阵列数据中选择的基因信息,筛选出三个基因集,即基于文献的基因集(集合1)、使用自组织映射和主成分分析的基于分析的基因集(集合2)以及富集基因集(集合3)。然后使用贝叶斯统计对每个基因集进行基因网络分析,以识别mESC神经分化过程中对RA响应的阶段特异性基因表达特征。我们的结果表明,RA在分化第36天时显著增加了神经球、神经元细胞和神经胶质细胞的大小。此外,基因网络分析表明,在存在RA的情况下,神经标记物胶质纤维酸性蛋白在分化第36天时显著上调基因集1和3中的其他基因,而神经发育标记物Gbx2则显著上调基因集2中的其他基因。这些发现表明,我们用于识别发育阶段特异性基因表达和相互作用的方案是筛选神经发育时期环境化学物质毒性的有用方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f916/3413097/98c4809e6f13/fgene-03-00141-g001.jpg

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