组蛋白修饰在卵母细胞发育中功能和调控机制的研究进展

组蛋白修饰作为表观遗传调控网络的重要组成部分,其主要的修饰类型包括乙酰化、甲基化、磷酸化等,在卵母细胞减数分裂过程中呈现动态变化.在卵母细胞发育过程中,表观遗传调控因子涉及的乙酰化、甲基化维持、磷酸化和组蛋白置换调控着卵母细胞减数分裂过程中基因的表达、纺锤体的组装、染色体的排列和基因组的稳定性,确保了卵母细胞减数分裂的...     

表观遗传药物对体细胞核移植胚胎发育的促进作用

体细胞核移植(somatic cell nuclear transfer,SCNT)是利用卵母细胞胞质中的重编程物质对高度分化体细胞核进行重编程作用使其恢复全能性并发育为新个体的技术。在SCNT过程中,表观遗传修饰参与卵母细胞的重编程,如DNA甲基化修饰和组蛋白的翻译后修饰。这些重编程的异常修饰会对SCNT胚胎的发育产生不良影响。表观遗传药物,如DNA甲基转移酶抑制剂和组蛋白去乙酰基酶抑制剂,可改善表观遗传修饰的异常现象,促进体细胞核移植重构胚的重编程。该文对SCNT胚胎重编程过程中的异常表观遗传修饰以及近年来报道的表观遗传相关药物进行综述,并进一步探讨了这些药物对SCNT胚胎发育的促进作用。     

组蛋白乙酰化与卵母细胞及胚胎的体外发育

组蛋白乙酰化及去乙酰化是表观遗传修饰一个重要部分,其对哺乳动物卵母细胞成熟和胚胎发育具有重要的调节作用。因此深入研究组蛋白乙酰化的发生机制,对于改善卵母细胞和早期胚胎的发育具有重要意义。对哺乳动物卵母细胞及胚胎发育过程中的组蛋白乙酰化动态修饰进行综述。     

精子表观遗传修饰及其在胚胎发育过程中的潜在作用

精子发生(Spermatogenesis) 是一高度复杂的过程, 包括有丝分裂、减数分裂和精子形成。精母细胞经过独特而广泛的染色质与表观遗传修饰重塑之后, 最终分化产生了具有特定表观遗传修饰的精子。最近研究表明, 成熟精子中的表观遗传修饰在发育的胚胎中发挥了重要作用, 其表观遗传模式的改变会导致某些疾病风险提高, 如受精失败、胚胎发生机能障碍、早产、出生体重低、先天畸形、新生儿死亡以及其他在辅助生殖技术后代中发现的发生频率较高的妊娠相关并发症。文章通过评价成熟精子中DNA甲基化、保留组蛋白修饰、RNAs和精蛋白等表观遗传修饰的重要意义及其在胚胎发育过程中的潜在作用, 阐述了成熟精子中改变的表观遗传修饰与相关疾病之间的关系, 为不育症的防治、精子表观遗传质量评价以及降低辅助生殖技术后代表观遗传疾病风险等提供基础资料。     

表观遗传修饰与肿瘤

肿瘤的形成受遗传学修饰和表观遗传修饰的影响。长期以来人们一直认为基因突变参与肿瘤的形成,近年来越来越多的证据表明,表观遗传修饰在肿瘤进展中同样具有非常重要的作用。表观遗传调控可以影响基因转录活性而不涉及DNA序列的改变。本文介绍了肿瘤发生发展过程中出现的表观遗传修饰异常,以及通过干预表观遗传修饰治疗肿瘤的应用前景。     

表观遗传修饰在糖脂代谢中的作用

表观遗传学是研究没有DNA序列变化的、可遗传的基因表达改变。表观遗传修饰可以参与多种生命过程,其在糖脂代谢中也发挥了重要的作用。生物体内的糖脂代谢关系密切,糖脂代谢紊乱会导致多种代谢性疾病的发生。文章主要从DNA甲基化、组蛋白修饰、非编码RNA调控等方面综述了表观遗传修饰在糖脂代谢中的研究进展。     

表观遗传对炎症的调控机制及其在奶牛乳房炎抗病育种中的应用前景

炎症受遗传和非遗传因素(环境或表观遗传)的共同影响, 其中表观遗传(Epigenetic)在炎症的发生发展过程中发挥重要调控作用。表观遗传修饰是指DNA序列没有改变, 而基因表达却发生了可遗传的变化, 主要包括DNA甲基化和组蛋白修饰等。表观遗传为病原微生物与炎症反应间关系的研究架起了重要桥梁。炎症反应中T辅助细胞的分化, 细胞因子、趋化因子等基因的表达都受到表观遗传的调控。文章主要综述了DNA甲基化、组蛋白修饰等对炎症尤其是乳房炎的调控机制, 并就表观遗传调控在奶牛乳房炎治疗及抗病育种中的应用前景进行了展望。     

表观遗传修饰在胰腺β细胞分化和功能中的作用

表观遗传是指在不改变DNA核苷酸序列的前提下,通过DNA甲基化、组蛋白修饰和非编码RNA等形式引起基因表达的可遗传性改变,并参与多种生命过程。最新研究发现,多种表观遗传修饰形式可影响胰腺β细胞的发育和功能,从而导致糖代谢紊乱,在糖尿病的发生发展中起到了重要的作用。现将对β细胞分化与功能中的表观遗传调控机制进行综述。     

母源物质对重编程作用研究进展

卵母细胞发生过程中会积累大量的物质,即所谓的母源物质(maternal materials),自然状态下,这些母源物质对受精以及之后的发育具有重要的生物学功能。雌雄配子融合后,精子核与卵母细胞中单倍体染色体组均会发生剧烈的表观遗传修饰变化,这个过程也同样发生在体细胞核移植到卵母细胞质之后,这种变化被称之为重编程。重编程奠定了新个体发生发育全部程序的基础,因此是一个备受重视的生物学过程。重编程包括DNA去甲基化、染色质重塑和组蛋白修饰等。受精后,卵母细胞与精子的基因组均会在一定时间和空间范围内经历相应的重编程过程,清除各自基因组在配子形成中保留的表观遗传学修饰,调控基因表达并形成正常发育的全能性胚胎。受精后,卵母细胞成熟中积累的多种母源物质聚集在雄原核周围,调控其基因组的重编程。体细胞核移植胚胎中供体细胞核注到去核卵母细胞后也将在卵母细胞中蛋白质、mRNA、酶类等母源物质的作用下进行重编程。现总结了母源物质对雄原核及供体细胞核重编程作用的研究进展,并探讨了母源物质作用的可能机制。     

表观遗传调控在糖尿病及其并发症中的作用

表观遗传(epigenetics)是指DNA序列不发生变化但基因表达却发生了可遗传的改变．表观遗传调控过程十分复杂,主要包括DNA甲基化、组蛋白修饰和微小RNA(miRNA)等．糖尿病是一种慢性代谢性疾病,常伴随大血管和微血管并发症．糖尿病的发生、发展不仅取决于遗传因素,而且也受到表观遗传修饰的调控．因此,对表观遗传调控的研究将为糖尿病及其并发症的预防和治疗提供新的思路和方法．     

The Epigenetic Reprogramming Roadmap in Generation of iPSCs from Somatic Cells

Reprogramming of somatic cells to induced pluripotent stem cells(iPSCs) is a comprehensive epigenetic process involving genome-wide modifications of histones and DNA methylation. This process is often incomplete, which subsequently affects i PSC reprograming,pluripotency, and differentiation capacity. Here, we review the epigenetic changes with a focus on histone modification(methylation and acetylation) and DNA modification(methylation) during i PSC induction. We look at changes in specific epigenetic signatures, aberrations and epigenetic memory during reprogramming and small molecules influencing the epigenetic reprogramming of somatic cells. Finally,we discuss how to improve i PSC generation and pluripotency through epigenetic manipulations.     

长链非编码RNA相关表观遗传修饰在癌症中的进展*

长链非编码RNA(lncRNA)是一类转录本长度大于200 nt的RNA分子,编码蛋白质的功能有限,但其功能多样且复杂。已有研究报道lncRNA与肿瘤的发展进程密切相关,lncRNA可以通过不同方式参与细胞内生物学进程的调控,是潜在的癌症调节因子,其中,调节表观遗传修饰水平是其影响癌症进程的主要手段;癌症发病过程中细胞内存在着不同程度的表观遗传修饰,其主要为包括甲基化、乙酰化、磷酸化、糖基化、泛素化等修饰方式在内的DNA修饰、RNA修饰以及蛋白质的翻译后修饰,在癌症的不同阶段其修饰的异常程度不同,从而影响肿瘤发生的生物学进程。研究表明,lncRNA可以通过自身修饰或参与其他生物大分子的表观遗传修饰进程参与癌症的发生发展。因此,回顾了lncRNA所参与的表观遗传修饰形式和lncRNA在表观遗传修饰方面所起到的作用,并概述了lncRNA通过影响表观遗传修饰水平从而调控癌症进程的方法。旨在总结癌症细胞内表观遗传修饰方面所涉及lncRNA的研究进展,为癌症诊断和治疗提供潜在的靶标和生物学标志物。     

Current advances in epigenetic modification and alteration during mammalian ovarian folliculogenesis

During the growth and development of mammalian ovarian follicles, the activation and deactivation of mass genes are under the synergistic control of diverse modifiers through genetic and epigenetic events. Many factors regulate gene activity and functions through epigenetic modification without altering the DNA sequence, and the common mechanisms may include but are not limited to: DNA methylation, histone modifications (e.g., acetylation, deacetylation, phosphorylation, methylation, and ubiquitination), and RNA-associated silencing of gene expression by noncoding RNA. Over the past decade, substantial progress has been achieved in studies involving the epigenetic alterations during mammalian germ cell development. A number of candidate regulatory factors have been identified. This review focuses on the current available information of epigenetic alterations (e.g., DNA methylation, histone modification, noncoding-RNA-mediated regulation) during mammalian folliculogenesis and recounts when and how epigenetic patterns are differentially established, maintained, or altered in this process. Based on different types of epigenetic regulation, our review follows the temporal progression of events during ovarian folliculogenesis and describes the epigenetic changes and their contributions to germ cell-specific functions at each stage (i.e., primordial folliculogenesis (follicle formation), follicle maturation, and follicular atresia).     

A novel role for the Aurora B kinase in epigenetic marking of silent chromatin in differentiated postmitotic cells

Combinatorial modifications of the core histones have the potential to fine-tune the epigenetic regulation of chromatin states. The Aurora B kinase is responsible for generating the double histone H3 modification tri-methylated K9/phosphorylated S10 (H3K9me3/S10ph), which has been implicated in chromosome condensation during mitosis. In this study, we have identified a novel role for Aurora B in epigenetic marking of silent chromatin during cell differentiation. We find that phosphorylation of H3 S10 by Aurora B generates high levels of the double H3K9me3/S10ph modification in differentiated postmitotic cells and also results in delocalisation of HP1beta away from heterochromatin in terminally differentiated plasma cells. Microarray analysis of the H3K9me3/S10ph modification shows a striking increase in the modification across repressed genes during differentiation of mesenchymal stem cells. Our results provide evidence that the Aurora B kinase has a role in marking silent chromatin independently of the cell cycle and suggest that targeting of Aurora B-mediated phosphorylation of H3 S10 to repressed genes could be a mechanism for epigenetic silencing of gene expression.     

转基因克隆牛胎盘中印迹基因PEG10的DNA甲基化水平

低效率的体细胞核移植技术显著制约着该技术在转基因动物生产上的广泛应用。目前认为供体细胞核不能被受体卵母细胞胞质完全的表观重编程是其效率低下的最主要原因,而DNA甲基化是基因表观修饰的主要方式之一。为了探求转基因克隆牛的死亡是否与其胎盘中印迹基因的甲基化的重编程程度相关,文章通过亚硫酸氢盐测序法(Bisulfite sequencing PCR,BSP)和亚硫酸氢盐联合限制性内切酶分析法(Combined bisulfite restriction analysis,COBRA),对印迹基因PEG10在围产期死亡且存在发育缺陷的转基因克隆牛的胎盘(死亡组)和存活的转基因克隆牛的胎盘(存活组)与正常对照牛胎盘(对照组)的DNA甲基化水平进行了详细的比较。结果发现,与对照组相比,PEG10基因在死亡组上表现出异常的超甲基化水平,而存活组与对照组相比无显著性差异。研究结果显示,胎盘中印迹基因的DNA甲基化表观重编程不彻底可能是导致转基因克隆牛发育异常进而死亡的主要原因之一。     

Chromatin modification and epigenetic reprogramming in mammalian development

The developmental programme of embryogenesis is controlled by both genetic and epigenetic mechanisms. An emerging theme from recent studies is that the regulation of higher-order chromatin structures by DNA methylation and histone modification is crucial for genome reprogramming during early embryogenesis and gametogenesis, and for tissue-specific gene expression and global gene silencing. Disruptions to chromatin modification can lead to the dysregulation of developmental processes, such as X-chromosome inactivation and genomic imprinting, and to various diseases. Understanding the process of epigenetic reprogramming in development is important for studies of cloning and the clinical application of stem-cell therapy.     

Genome-wide analysis of epigenetic dynamics across human developmental stages and tissues

Background

Epigenome is highly dynamic during the early stages of embryonic development. Epigenetic modifications provide the necessary regulation for lineage specification and enable the maintenance of cellular identity. Given the rapid accumulation of genome-wide epigenomic modification maps across cellular differentiation process, there is an urgent need to characterize epigenetic dynamics and reveal their impacts on differential gene regulation.

Methods

We proposed DiffEM, a computational method for differential analysis of epigenetic modifications and identified highly dynamic modification sites along cellular differentiation process. We applied this approach to investigating 6 epigenetic marks of 20 kinds of human early developmental stages and tissues, including hESCs, 4 hESC-derived lineages and 15 human primary tissues.

Results

We identified highly dynamic modification sites where different cell types exhibit distinctive modification patterns, and found that these highly dynamic sites enriched in the genes related to cellular development and differentiation. Further, to evaluate the effectiveness of our method, we correlated the dynamics scores of epigenetic modifications with the variance of gene expression, and compared the results of our method with those of the existing algorithms. The comparison results demonstrate the power of our method in evaluating the epigenetic dynamics and identifying highly dynamic regions along cell differentiation process.

     

表观遗传跨代继承表型研究进展

表观基因组在配子发生和早期胚胎发育中经历一个重编程过程。因此, 人们认为表观遗传信息不可能代间传递。表观遗传跨代继承表型的出现, 说明某些表观遗传标志可能逃脱了重编程。尽管该观点尚存争议, 但日益增多的实验证据表明表观遗传记忆确实存在于哺乳动物中。由于表观遗传修饰具有可逆性, 表观基因组易受各种环境因子(如化学物质、营养和行为等)的影响而改变。因此, 表观基因组提供了跨代传递环境影响的可能机制。文章介绍了表观遗传跨代继承表型的概念, 论述了表观遗传重编程和表观遗传信息跨代传递的分子机制, 列举了一些环境因子与表观遗传跨代继承性疾病。     

鲫鱼Dnmt1基因cDNA的克隆及表达分析

研究克隆了编码鲫鱼Dnmt1蛋白的cDNA序列,并对Dnmt1基因的时空表达模式和表达丰度差异进行了分析。该cDNA全长4912bp,编码1503个氨基酸。鲫鱼Dnmt1蛋白与其他物种Dnmt1蛋白的同源性分析表明,N端调节区的保守性较低,但C端的催化区是高度保守的。整胚原位杂交显示,Dnmt1 mRNA在胚胎发育早期是广泛分布的,随着胚胎的发育,Dnmt1 mRNA在眼睛、脑部和已成熟体节的信号较强烈,显示了明显的区域性差异。实时定量PCR结果显示在鲫鱼胚胎发育早期有丰富的母源Dnmt1 mRNA存在,在早期发育过程中其丰度逐渐降低,在胚胎发育至2d后,Dnmt1 mRNA丰度又升到较高水平。RT-PCR检测表明在肝、心、脾、肾、脑、肌肉、视网膜等成体组织中都有Dnmt1的表达,但实时定量PCR结果显示在细胞分裂增殖旺盛的组织中表达水平明显较高。上述结果提示鲫鱼Dnmt1可能参与了胚胎基因组DNA甲基化的重编程,甲基化表观遗传学式样的确立和合子核基因正确时空表达模式形成的调节控制。