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性别差异在 microRNA-mRNA 网络中的表现:探究性二态新生儿下丘脑中新的表观遗传编程机制。

Sex differences in microRNA-mRNA networks: examination of novel epigenetic programming mechanisms in the sexually dimorphic neonatal hypothalamus.

机构信息

Department of Biomedical Sciences, University of Pennsylvania School of Veterinary Medicine, 380 South University Ave, 410F Hill Pavilion, Philadelphia, PA, 19104, USA.

出版信息

Biol Sex Differ. 2017 Aug 15;8(1):27. doi: 10.1186/s13293-017-0149-3.

Abstract

BACKGROUND

Sexual differentiation of the male brain, and specifically the stress circuitry in the hypothalamus, is primarily driven by estrogen exposure during the perinatal period. Surprisingly, this single hormone promotes diverse programs of sex-specific development that vary widely between different cell types and across the developing male brain. The complexity of this phenomenon suggests that additional layers of gene regulation, including microRNAs (miRNAs), must act downstream of estrogen to mediate this specificity.

METHODS

To identify noncanonical mediators of estrogen-dependent sex-specific neural development, we assayed the miRNA complement of the mouse PN2 hypothalamus by microarray following an injection of vehicle or the aromatase inhibitor, formestane. Initially, multivariate analyses were used to test the influence of sex and experimental group on the miRNA environment as a whole. Then, we utilized traditional hypothesis testing to identify individual miRNA with significantly sex-biased expression. Finally, we performed a transcriptome-wide mapping of Argonaute footprints by high-throughput sequencing of RNA isolated by cross-linking immunoprecipitation (Ago HITS-CLIP) to empirically characterize targeting relationship between estrogen-responsive miRNAs and their messenger RNA (mRNA) targets.

RESULTS

In this study, we demonstrated that the neonatal hypothalamic miRNA environment has robust sex differences and is dynamically responsive to estrogen. Analyses identified 162 individual miRNAs with sex-biased expression, 92 of which were estrogen-responsive. Examining the genomic distribution of these miRNAs, we found three miRNA clusters encoded within a 175-kb region of chromosome 12 that appears to be co-regulated by estrogen, likely acting broadly to alter the epigenetic programming of this locus. Ago HITS-CLIP analysis uncovered novel miRNA-target interactions within prototypical mediators of estrogen-driven sexual differentiation of the brain, including Esr1 and Cyp19a1. Finally, using Gene Ontology annotations and empirically identified miRNA-mRNA connections, we identified a gene network regulated by estrogen-responsive miRNAs that converge on biological processes relevant to sexual differentiation of the brain.

CONCLUSIONS

Sexual differentiation of the perinatal brain, and that of stress circuitry in the hypothalamus specifically, seems to be particularly susceptible to environmental programming effects. Integrating miRNA into our conceptualization of factors, directing differentiation of this circuitry could be an informative next step in efforts to understand the complexities behind these processes.

摘要

背景

雄性大脑的性别分化,特别是下丘脑的应激回路,主要由围产期雌激素暴露驱动。令人惊讶的是,这种单一激素促进了不同的性别特异性发育程序,这些程序在不同的细胞类型和发育中的雄性大脑中差异很大。这种现象的复杂性表明,包括 microRNAs (miRNAs) 在内的其他基因调控层必须在雌激素下游发挥作用,以介导这种特异性。

方法

为了确定雌激素依赖性性别特异性神经发育的非典型介质,我们通过微阵列检测了注射载体或芳香酶抑制剂(formestane)后小鼠 PN2 下丘脑的 miRNA 组成。最初,多元分析用于测试性别和实验组对 miRNA 环境的整体影响。然后,我们利用传统的假设检验来识别具有显著性别偏倚表达的单个 miRNA。最后,我们通过高吞吐量测序对 RNA 进行交联免疫沉淀 (Ago HITS-CLIP) 进行 Argonaute 足迹的全转录组映射,以经验表征雌激素反应性 miRNA 与其信使 RNA (mRNA) 靶标的靶向关系。

结果

在这项研究中,我们证明了新生下丘脑的 miRNA 环境具有强大的性别差异,并对雌激素有动态反应。分析确定了 162 个具有性别偏倚表达的个体 miRNA,其中 92 个是雌激素反应性的。检查这些 miRNA 的基因组分布,我们发现三个 miRNA 簇编码在染色体 12 的 175kb 区域内,这些区域似乎被雌激素共同调节,可能广泛作用于改变该基因座的表观遗传编程。Ago HITS-CLIP 分析揭示了大脑中雌激素驱动性别分化的典型介质内的新 miRNA 靶相互作用,包括 Esr1 和 Cyp19a1。最后,使用基因本体论注释和经验鉴定的 miRNA-mRNA 连接,我们确定了一个受雌激素反应性 miRNA 调控的基因网络,该网络汇聚于与大脑性别分化相关的生物学过程。

结论

围产期大脑的性别分化,特别是下丘脑应激回路的性别分化,似乎特别容易受到环境编程效应的影响。将 miRNA 纳入我们对指导该电路分化的因素的概念化中可能是理解这些过程背后复杂性的一个富有成效的下一步。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a972/5558756/676831058ba5/13293_2017_149_Fig1_HTML.jpg

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