长链非编码RNA与肿瘤和干细胞

人类基因组包含20 000多种蛋白质编码基因,只占总基因的2%左右,而90%以上的转录子是长链非编码RNA(Long non-coding RNAs,lnc RNAs)。lnc RNAs是广泛存在于哺乳动物基因组中的长度在200-100 000 nt之间,且不具有蛋白质编码功能的转录本。研究发现其在许多类型的肿瘤中存在异常表达,具有潜在的致癌或抑癌作用,并作为重要的调控分子参与各种生物学过程,与肿瘤的发生、发展密不可分。此外,lnc RNAs在维持干细胞全能性、调控干细胞基因表达、调节干细胞自我更新和分化等方面发挥了至关重要的作用,是继micro RNA后肿瘤研究的新热点。针对lnc RNAs在肿瘤和干细胞生物学中的功能及相关机制作一综述,旨在为肿瘤的诊断、治疗、预后等方面提供新思路。     

长非编码RNA与造血谱系分化

全基因组测序分析显示,人类基因组中蛋白质编码基因所占比例不足2%,但高达80%的基因位点可以转录出RNA。在这些非编码RNA(non-coding RNA,nc RNA)中,长度超过200个核苷酸的RNA分子被称为长非编码RNA(long non-coding RNA,lnc RNA)。在血液系统中,基于造血不同分化阶段的转录组测序和分析发现,几乎在造血分化各个阶段都有lnc RNA参与。lnc RNA在维持造血干细胞未分化状态、诱导红细胞脱核成熟、粒细胞定向分化以及淋巴细胞迁移等谱系分化过程中均发挥了不可或缺的作用。lnc RNA作为调控因子在转录、转录后以及翻译等多个水平参与造血谱系分化调控。该文综述了近年来lnc RNA在造血分化领域的研究现状,为后续进一步揭示lnc RNA介导的造血调控网络奠定基础。     

长链非编码RNA AFAP1-AS1促进肿瘤侵袭转移

<正>人类基因组计划及其后续的DNA元件百科全书计划(The Encyclopedia of DNA Elements Project,ENCODE)研究成果表明,蛋白质编码基因序列仅占人类基因组序列的1%~3%,人基因组中绝大部分可转录的序列为长链非编码RNA(long non-coding RNA,lnc RNAs)[1].Lnc RNA广泛地存在于各种生物中,且随着生物复杂程度的升高,基因组中lnc RNA序列的比例也相应地增大,提示lnc RNA在生物进化过程中可能有着重要意义[2-4].随着     

LncRNA在神经发育及神经性疾病中作用的研究进展

长链非编码RNA(long non-coding RNA,lnc RNA)是指不具有编码蛋白能力且长度大于200nt的RNA,近年来,越来越多的lnc RNAs在多种生命活动中发挥着重要的作用。已有研究发现lnc RNAs在神经发育过程中起着重要的作用,lnc RNAs可以调控神经干细胞定向分化为神经元、胶质细胞、星状细胞,lnc RNAs,还参与调控神经干细胞的分化进程;lnc RNAs表达异常与神经疾病也有密切关系。本文就lnc RNAs在调控神经细胞分化进程和在神经性疾病作用的研究新进展进行综述。     

DLK1-DIO3印记区域的miRNAs与疾病的发生

哺乳动物的基因组以发育调控模式进行转录,生成长的和短的非编码RNAs(non-coding RNA,ncRNAs).ncRNAs占到人类转录组的98%,与生物体进化复杂程度显著相关.MicroRNAs(miRNAs)是目前研究比较透彻的,长度大约为20~24个核苷酸的ncRNAs,其通过与靶基因mRNA的结合在转录后水平负调控基因的表达.人类基因组中一个最大的miRNA簇位于14号染色体(14q32)的DLK1-DIO3印记区域,包括了54个miRNAs.这些miRNAs通过参与调节重要的信号通路在许多病理过程中发挥作用.充分了解DLK1-DIO3印记区域中这个大的miRNA簇,在病理生理过程中的重要性将有助于为相关疾病的治疗提供新的策略.本文比较深入地分析了DLK1-DIO3印记区域中的miRNAs在调控组织动态平衡以及多种癌症发生中的作用,同时对其潜在的临床应用价值进行了讨论.     

植物长链非编码RNA的研究进展

长链非编码RNA(long non-coding RNAs,lnc RNAs)是真核生物中一类长度大于200个核苷酸、无蛋白编码能力或编码能力极低的RNA转录本。lnc RNA种类和功能的多样性导致了对其进行研究的复杂性,特别是对植物中lnc RNA的认识相当有限。该文就近年来植物中已发现的lnc RNA的种类、相关转录酶、参与的生物学过程、发挥功能的分子机制以及其相关的研究策略等方面进行综述和展望,以期为深入认识植物lnc RNA提供借鉴。     

基因印记与lncRNA

基因印记是一种表观遗传调控机制,在二倍体哺乳动物的发育过程中,基因印记可以调控来自亲代的等位基因差异表达。非编码RNA是不编码蛋白质的RNA,它在RNA水平调控基因表达。研究表明大多数印记基因中存在长非编码RNA（长度>200nt的非编码RNA）的转录,长非编码RNA主要通过顺式的转录干扰作用来实现基因印记。同时基因印记及其相关的长非编码RNA异常表达与许多先天疾病相关,迄今已发现数十种人类遗传疾病与基因印记有关,而lncRNA引起的基因印记在疾病的发生和治疗中起着重要作用。     

Emerging similarities in epigenetic gene silencing by long noncoding RNAs

Long noncoding RNAs (lncRNAs) such as Xist, Air, and Kcnq1ot1 are required for epigenetic silencing of multiple genes in cis within large chromosomal domains, including distant genes located hundreds of kilobase pairs away. Recent evidence suggests that all three of these lncRNAs are functional and that they silence gene expression, in part, through an intimate interaction with chromatin. Here we provide an overview of lncRNA-dependent gene silencing, focusing on recent findings for the Air and Kcnq1ot1 lncRNAs. We review molecular evidence indicating that these lncRNAs interact with chromatin and correlate their presence with specific histone modifications associated with gene silencing. A general model for a lncRNA-dependent gene-silencing mechanism is presented based on the apparent ability of lncRNAs to recruit histone-modifying activities to chromatin. However, alternate mechanisms may be required to explain the silencing of some lncRNA-dependent genes. Finally, we discuss unanswered questions and future perspectives associated with these enigmatic lncRNA molecules.     

A differentially methylated imprinting control region within the Kcnq1 locus harbors a methylation-sensitive chromatin insulator

The mechanisms underlying the phenomenon of genomic imprinting remain poorly understood. In one instance, a differentially methylated imprinting control region (ICR) at the H19 locus has been shown to involve a methylation-sensitive chromatin insulator function that apparently partitions the neighboring Igf2 and H19 genes in different expression domains in a parent of origin-dependent manner. It is not known, however, if this mechanism is unique to the Igf2/H19 locus or if insulator function is a common feature in the regulation of imprinted genes. To address this question, we have studied an ICR in the Kcnq1 locus that regulates long range repression on the paternally derived p57Kip2 and Kcnq1 alleles in an imprinting domain that includes Igf2 and H19. We show that this ICR appears to possess a unidirectional chromatin insulator function in somatic cells of both mesodermal and endodermal origins. Moreover, we document that CpG methylation regulates this insulator function suggesting that a methylation-sensitive chromatin insulator is a common theme in the phenomenon of genomic imprinting.     

Polycomb group proteins Ezh2 and Rnf2 direct genomic contraction and imprinted repression in early mouse embryos

Genomic imprinting regulates parental-specific expression of particular genes and is required for normal mammalian development. How imprinting is established during development is, however, largely unknown. To address this question, we studied the mouse Kcnq1 imprinted cluster at which paternal-specific silencing depends on expression of the noncoding RNA Kcnq1ot1. We show that Kcnq1ot1 is expressed from the zygote stage onward and rapidly associates with chromatin marked by Polycomb group (PcG) proteins and repressive histone modifications, forming a discrete repressive nuclear compartment devoid of RNA polymerase II, a configuration also observed at the Igf2r imprinted cluster. In this compartment, the paternal Kcnq1 cluster exists in a three-dimensionally contracted state. In vivo the PcG proteins Ezh2 and Rnf2 are independently required for genomic contraction and imprinted silencing. We propose that the formation of a parental-specific higher-order chromatin organization renders imprint clusters competent for monoallelic silencing and assign a central role to PcG proteins in this process.     

Long noncoding RNA Airn protects podocytes from diabetic nephropathy lesions via binding to Igf2bp2 and facilitating translation of Igf2 and Lamb2

Diabetic nephropathy (DN) is a severe diabetic microvascular complication with high mortality. Long noncoding RNAs (lncRNAs) are characterized as important regulators of various biological processes by emerging researches, whereas the molecular mechanisms by which lncRNAs participate in DN progression need to be further clarified. Herein, we conducted a study on the regulatory role in DN of an lncRNA named antisense of Igf2r non‐protein‐coding RNA (Airn). Airn expression was downregulated in renal tissues of diabetic mice, and was negatively related with DN development. Besides, Airn downregulation was detected in high‐glucose‐stimulated podocytes, resulting in poorer cell viability, a higher tendency to cell apoptosis, and a deficiency of laminin level, while Airn overexpression could significantly alleviate these deleterious effects. Mechanistically, using RNA immunoprecipitation and RNA pull‐down assays, we found that Airn could bind to the RNA‐binding protein Igf2bp2, thus facilitating translation of Igf2 and Lamb2 to maintain normal podocyte viability and glomerular barrier function. Collectively, our results demonstrate the protective role of lncRNA Airn in podocytes against DN, providing a new insight into DN pathogenesis and molecular therapy.     

Towards unravelling the Igf2/H19 imprinted domain

Genomic imprinting is an epigenetic marking process that confers parent-of-origin-dependent expression on certain genes. These imprinted genes are sometimes found in clusters, suggesting a possible involvement of higher order regulatory elements controlling expression and imprinting of genes organised in such clusters. In the distal chromosome 7 there are at least four imprinted genes: Mash2, Ins2, Igf2 and H19. Recent evidence⁽¹⁾ suggests that imprinting and expression of at least Igf2 and H19 may be mechanistically linked.     

Genomic Imprinting in Mammals

Genomic imprinting affects a subset of genes in mammals and results in a monoallelic, parental-specific expression pattern. Most of these genes are located in clusters that are regulated through the use of insulators or long noncoding RNAs (lncRNAs). To distinguish the parental alleles, imprinted genes are epigenetically marked in gametes at imprinting control elements through the use of DNA methylation at the very least. Imprinted gene expression is subsequently conferred through lncRNAs, histone modifications, insulators, and higher-order chromatin structure. Such imprints are maintained after fertilization through these mechanisms despite extensive reprogramming of the mammalian genome. Genomic imprinting is an excellent model for understanding mammalian epigenetic regulation.     

Aberrant expression of imprinted lncRNA MEG8 causes trophoblast dysfunction and abortion

Long noncoding RNAs (lncRNAs) are a group of noncoding RNAs whose nucleotides are longer than 200 bp. Previous studies have shown that they play an important regulatory role in many developmental processes and biological pathways. However, the contributions of lncRNAs to placental development are largely unknown. Here, our study aimed to investigate the lncRNA expression signatures in placental development by performing a microarray lncRNA screen. Placental samples were obtained from pregnant C57BL/6 female mice at three key developmental time points (embryonic day E7.5, E13.5, and E19.5). Microarrays were used to analyze the differential expression of lncRNAs during placental development. In addition to the genomic imprinting region and the dynamic DNA methylation status during placental development, we screened imprinted lncRNAs whose expression was controlled by DNA methylation during placental development. We found that the imprinted lncRNA Rian may play an important role during placental development. Its homologous sequence lncRNA MEG8 (RIAN) was abnormally highly expressed in human spontaneous abortion villi. Upregulation of MEG8 expression in trophoblast cell lines decreased cell proliferation and invasion, whereas downregulation of MEG8 expression had the opposite effect. Furthermore, DNA methylation results showed that the methylation of the MEG8 promoter region was increased in spontaneous abortion villi. There was dynamic spatiotemporal expression of imprinted lncRNAs during placental development. The imprinted lncRNA MEG8 is involved in the regulation of early trophoblast cell function. Promoter methylation abnormalities can cause trophoblastic cell defects, which may be one of the factors that occurs in early unexplained spontaneous abortion.