DEAD-box基因家族在拟南芥生长发育中的作用

在RNA代谢过程中,需要许多蛋白和核酸的参与,其中一类蛋白就是RNA解旋酶。RNA解旋酶通过水解ATP获得能量来参与RNA代谢的多个方面,包括核内转录、pre-mRNA的剪切、核糖体发生、核质运输、蛋白质翻译、RNA降解、细胞器内基因的表达。DEAD-box蛋白家族是RNA解旋酶中最大的亚家族,它具有9个保守结构域,因motifyⅡ的保守氨基酸序列Asp-Glu-Ala-Asp(DEAD)而命名。该家族在酵母、拟南芥(Arabidopsis thaliana Heynh.)和人类基因组中都有较多的家庭成员。近年来,研究者对拟南芥DEAD-box蛋白家族的结构和功能进行了一些研究,本文着重总结DEAD-box基因家族对拟南芥生长发育的影响。     

RNA结合蛋白与神经退行性疾病

神经退行性疾病是一类导致神经元细胞退化、功能丧失的疾病。随着RNA结合蛋白TDP-43和FUS被发现与神经退行性疾病渐冻人症(amyotrophic lateral sclerosis,ALS)密切相关,人们越来越多地关注RNA结合蛋白与神经退行性疾病的关系。大多数RNA结合蛋白都存在一个类似于prion的结构域,这个结构域使其容易发生积聚,并与神经毒性的产生相关。RNA结合蛋白参与应激颗粒的形成,应激颗粒的形成可能与神经退行性疾病相关,这进一步揭示了RNA结合蛋白在这类疾病中可能发挥作用。     

DDX21 RNA解旋酶不同结构域的功能特点解析

DEAD-box家族是在生物体内普遍存在的一类高度保守的RNA解旋酶,在RNA的合成和加工、细胞发育和细胞代谢等过程中都发挥着重要作用。DDX21 RNA解旋酶是DEAD-box家族成员之一,而目前为止DDX21的酶学功能及结构特征尚未被完全了解。本研究运用生物化学与生物物理学前沿技术,系统地研究了DDX21各结构域在不同功能中发挥的作用。首先重组构建并纯化了人的DDX21 RNA解旋酶及不同的截短蛋白质,利用动态激光散射和凝胶层析技术分析各蛋白质的寡聚形态,发现N-端的非功能区（N-端181aa）与C-端的4个FRGQR重复结构域对其结构有较大的影响;利用荧光偏振技术比较分析了各蛋白质与单链RNA的结合反应,结果显示,仅保留DEADc和HELICc结构域的截短蛋白质与单链RNA完全没有亲和性,缺失N-端181aa的截短蛋白质对ssRNA的结合能力与全长蛋白质基本一致,而仅缺失C-端的4个重复FRGQR结构域的截短蛋白质与单链RNA的亲和能力将显著下降;利用快速停流检测技术分析各截短蛋白质的解旋及退火活性,发现DEADc、HELICc及GUCT_RHII三个结构域共同参与DDX21的解旋功能,另一方面,缺失C-端4个FRGQR重复结构域的截短蛋白质导致退火能力的丧失。本研究揭示了DDX21的GUCT_RHII结构域及C-端4个FRGQR重复结构域在其结构及功能中发挥的重要作用,为今后研究DDX21的结构及其细胞功能提供了重要的理论依据。     

vasa基因研究进展

DEAD-box家族基因编码一类ATP依赖的RNA解旋酶。经系统进化分析可将该家族蛋白分为VASA、PL10和p68三个亚家族。其中,vasa基因最先在果蝇(Drosophila melanogaster)中被发现,在许多动物中都已经克隆得到其同源基因,研究显示,vasa基因在生殖细胞系中特异性表达,在许多生物中为生殖细胞形成和配子发生所需。有趣的是在果蝇中VASA蛋白是生殖质的组成部分,而在斑马鱼(Danio rerio)中vasa mRNA才是生殖质的组成部分。本文主要综述了vasa基因及其蛋白的结构、功能、表达和作为原生殖细胞分子标记物的应用等方面的内容,并展望了其研究前景。     

几种不同细胞系之间P68 RNA解旋酶表型差异的研究

对分别来自4种不同细胞系的细胞,在生长期间胞内P68 RNA解旋酶的动态变化进行了蛋白质和mRNA的比较研究。结果发现随着细胞培养时间的延长,各系细胞中P68 RNA解旋酶均呈现出有规律的改变,并且这种规律具有明显的细胞系特征:肿瘤细胞系之间表现出P68 RNA解旋酶蛋白条带单一的一致性;非肿瘤细胞系P68 RNA解旋酶蛋白出现多条带变化,并表现出明显的适应性;肿瘤细胞系与非肿瘤细胞系之间P68 RNA解旋酶的表型存在着明显的差异,这种差异从分子水平上揭示出P68 RNA解旋酶与细胞生长密切相关,并可能与细胞癌化有关。对产生这种差异的可能原因及其生物学意义进行了讨论。     

小热应激蛋白与动物繁殖机能的关系研究进展

热应激是指机体受到超过本身体温调节能力的高温刺激而产生的非特异性防御反应,热应激蛋白是机体热应激反应发生后细胞新合成或合成数量增加的一类蛋白质,小分子热应激蛋白是热应激蛋白家族中重要的一类成员,作为分子伴侣在细胞的正常代谢和生理条件下表达和发挥作用。目前已证实小热应激蛋白还参与调控细胞增殖和凋亡、生物膜膜脂的流动性、核质穿梭作用、免疫应答和疾病治疗等。本综述分别就小热应激蛋白在雄性动物生精细胞发育过程中参与的增殖、分化及凋亡调控作用以及在雌性动物卵母细胞发育、成熟、妊娠维持和生育调节功能的研究进展做一概述,旨在为小热应激蛋白生物学功能深入研究提供参考。     

受体相互作用蛋白3——细胞凋亡与坏死的调节阀

综述了受体相互作用蛋白(RIPs)蛋白结构和RIP3调控细胞凋亡与坏死机制的研究进展．受体相互作用蛋白3(receptor-interacting protein 3, RIP3)是丝/苏氨酸蛋白激酶家族成员之一,该蛋白质家族包含一类高度保守的丝/苏氨酸激酶结构域．RIP家族激酶作为细胞应激传感分子,在调控细胞凋亡、细胞坏死和存活通路中发挥重要作用．近年发现,RIP3参与肿瘤坏死因子TNFα诱导的细胞程序化坏死的生物学过程．认识RIP3调控TNFα诱导的细胞凋亡与坏死不同死亡途径转换的分子机制,有助于发现肿瘤治疗的新策略．     

piRNA通路中调控蛋白质研究进展

piRNA是一类与Argonaute蛋白家族的PIWI亚家族蛋白结合的非编码小RNA,其在沉默转座子、维持基因组的稳定性和保证生物体生殖细胞的正常发育中起着重要作用。piRNA通路包括piRNA的生成、piRISC的形成,以及由piRISC介导的转座子沉默。现总结了目前发现的参与调控果蝇和小鼠中piRNA通路的蛋白质因子。     

hnRNP A1的功能研究进展

核不均一核糖核蛋白(heterogeneous nuclear ribonucleoprotein,hnRNP)是一类多功能RNA结合蛋白家族,能与RNA聚合酶Ⅱ合成的新生转录本结合,并以复合体形式参与转录本稳定与成熟调控过程. hnRNP A1是hnRNPs家族重要成员,不仅广泛参与癌症与神经系统疾病相关基因的可变剪接调控,还在病毒侵染、细胞衰老及应激恢复中发挥重要作用.此外,hnRNP A1作为典型的RNA结合蛋白,在转录与可变剪接调控过程中,可通过动态三维结构识别特定序列.本文总结了hnRNP A1的最新研究进展,以期为进一步探究hnRNP A1在疾病发生中的功能研究提供参考.     

DEAD-box解旋酶在植物非生物胁迫响应中的功能研究进展

解旋酶广泛存在于从病毒到人类几乎所有已知的原核和真核生物体中,它们能利用NTP水解获得能量促进双链DNA/RNA解链。DEAD-box解旋酶是最大的解旋酶家族,在DNA复制、修复、重组、转录、核糖体发生和翻译起始等几乎所有涉及DNA/RNA代谢的细胞过程中均发挥重要作用。近年研究表明,DEAD-box解旋酶除具有持家基因功能外,还广泛参与植物生长发育及胁迫响应过程。目前,由解旋酶介导的胁迫应答具体机制依然不清晰。现重点介绍近年来高等植物DEAD-box解旋酶在非生物胁迫响应中的功能研究进展,同时探讨解旋酶参与胁迫应答的可能机制。     

Inhibition of cytoplasmic mRNA stress granule formation by a viral proteinase

Mammalian cells form dynamic cytoplasmic mRNA stress granules (SGs) in response to environmental stresses including viral infections. SGs are involved in regulating host mRNA function and metabolism, although their precise role during viral infection is unknown. SGs are thought to assemble based on functions of the RNA-binding proteins TIA-1/TIAR or Ras-GAP SH3 domain-binding protein (G3BP). Here, we investigated the relationship between a prototypical plus-strand RNA virus and SGs. Early during poliovirus infection, SG formation is induced, but as infection proceeds this ability is lost, and SGs disperse. Infection resulted in cleavage of G3BP, but not TIA-1 or TIAR, by poliovirus 3C proteinase. Expression of a cleavage-resistant G3BP restored SG formation during poliovirus infection and significantly inhibited virus replication. These results elucidate a mechanism for viral interference with mRNP metabolism and gene regulation and support a critical role of G3BP in SG formation and restriction of virus replication.     

The cold-inducible RNA-binding protein migrates from the nucleus to cytoplasmic stress granules by a methylation-dependent mechanism and acts as a translational repressor

The cold-inducible RNA-binding protein (CIRP) is a nuclear 18-kDa protein consisting of an amino-terminal RNA Recognition Motif (RRM) and a carboxyl-terminal domain containing several RGG motifs. First characterized for its overexpression upon cold shock, CIRP is also induced by stresses such as UV irradiation and hypoxia. Here, we investigated the expression as well as the subcellular localization of CIRP in response to other stress conditions. We demonstrate that oxidative stress leads to the migration of CIRP to stress granules (SGs) without alteration of expression. Stress granules are dynamic cytoplasmic foci at which stalled translation initiation complexes accumulate in cells subjected to environmental stress. Relocalization of CIRP into SGs also occurs upon other cytoplasmic stresses (osmotic pressure or heat shock) as well as in response to stresses of the endoplasmic reticulum. CIRP migration into SGs is independent from TIA-1 which has been previously reported to be a general mediator of SG formation, thereby suggesting the existence of multiple pathways leading to SG formation. Moreover, deletion mutants revealed that both RGG and RRM domains can independently promote CIRP migration into SGs. However, the methylation of arginine residues in the RGG domain is necessary for CIRP to exit the nucleus to be further recruited into SGs. By RNA-tethering experiments, we also show that CIRP down-regulates mRNA translation and that this activity is carried by the carboxyl-terminal RG-enriched domain. Altogether, our findings further reveal the diversity of mechanisms by which CIRP is regulated by environmental stresses and provide new insights into CIRP cytoplasmic function.     

Sequestration of G3BP coupled with efficient translation inhibits stress granules in Semliki Forest virus infection

Dynamic, mRNA-containing stress granules (SGs) form in the cytoplasm of cells under environmental stresses, including viral infection. Many viruses appear to employ mechanisms to disrupt the formation of SGs on their mRNAs, suggesting that they represent a cellular defense against infection. Here, we report that early in Semliki Forest virus infection, the C-terminal domain of the viral nonstructural protein 3 (nsP3) forms a complex with Ras-GAP SH3-domain–binding protein (G3BP) and sequesters it into viral RNA replication complexes in a manner that inhibits the formation of SGs on viral mRNAs. A viral mutant carrying a C-terminal truncation of nsP3 induces more persistent SGs and is attenuated for propagation in cell culture. Of importance, we also show that the efficient translation of viral mRNAs containing a translation enhancer sequence also contributes to the disassembly of SGs in infected cells. Furthermore, we show that the nsP3/G3BP interaction also blocks SGs induced by other stresses than virus infection. This is one of few described viral mechanisms for SG disruption and underlines the role of SGs in antiviral defense.     

The involvement of stress granules in aging and aging‐associated diseases

Stress granules (SGs) are nonmembrane assemblies formed in cells in response to stress conditions. SGs mainly contain untranslated mRNA and a variety of proteins. RNAs and scaffold proteins with intrinsically disordered regions or RNA‐binding domains are essential for the assembly of SGs, and multivalent macromolecular interactions among these components are thought to be the driving forces for SG assembly. The SG assembly process includes regulation through post‐translational modification and involvement of the cytoskeletal system. During aging, many intracellular bioprocesses become disrupted by factors such as cellular environmental changes, mitochondrial dysfunction, and decline in the protein quality control system. Such changes could lead to the formation of aberrant SGs, as well as alterations in their maintenance, disassembly, and clearance. These aberrant SGs might in turn promote aging and aging‐associated diseases. In this paper, we first review the latest progress on the molecular mechanisms underlying SG assembly and SG functioning under stress conditions. Then, we provide a detailed discussion of the relevance of SGs to aging and aging‐associated diseases.     

Regulation of stress granule dynamics by Grb7 and FAK signalling pathway

Cells form stress granules (SGs) in response to environmental stresses, which constitute cytoplasmic domains where mRNAs are stored and translation is halted. Although several components are found in SGs, it is poorly understood as to how SGs are formed and dissolved. We identified growth factor receptor-bound protein 7 (Grb7), an RNA-binding, translational regulator, as an integral component of SGs, which directly interacts with Hu antigen R (HuR) and is required for cells to form SGs. When stress is terminated, Grb7 is hyperphosphorylated by focal adhesion kinase (FAK), loses its ability to directly interact with HuR and is dissociated from SG components, thereby disrupting SGs in recovering cells. Consistently, dominant-negative hypophospho mutants of FAK and Grb7 significantly attenuate SG disassembly during recovery. FAK activation followed by its phosphorylating Grb7 constitutes a cell-autonomous signalling pathway that regulates the disassembly of SGs and translational stimulation during recovery. This is the first reported pathway actively regulating the dynamics of SGs.     

Stress Granule Formation is One of the Early Antiviral Mechanisms for Host Cells Against Coxsackievirus B Infection

Stress granules (SGs) are intracellular granules formed when cellular translation is blocked and have been reported to be involved in a variety of viral infections. Our previous studies revealed that SGs are involved in the coxsackievirus B (CVB) infection process, but the role of SGs in CVB infection has not been fully explored. In this study, we found that CVB type 3 (CVB3) could induce SG formation in the early phase of infection. Results showed that levels of CVB3 RNA and protein were significantly inhibited during the early stage of CVB3 infection by the elevated formation of SGs, while viral RNA and protein synthesis were significantly promoted when SG formation was blocked. Our findings suggest that SG formation is one of the early antiviral mechanisms for host cells against CVB infection.     

Response to stress in biological disorders: Implications of stress granule assembly and function

It is indispensable for cells to adapt and respond to environmental stresses, in order for organisms to survive. Stress granules (SGs) are condensed membrane‐less organelles dynamically formed in the cytoplasm of eukaryotes cells to cope with diverse intracellular or extracellular stress factors, with features of liquid‐liquid phase separation. They are composed of multiple constituents, including translationally stalled mRNAs, translation initiation factors, RNA‐binding proteins and also non‐RNA‐binding proteins. SG formation is triggered by stress stimuli, viral infection and signal transduction, while aberrant assembly of SGs may contribute to tissue degenerative diseases. Recently, a growing body of evidence has emerged on SG response mechanisms for cells facing high temperatures, oxidative stress and osmotic stress. In this review, we aim to summarize factors affecting SGs assembly, present the impact of SGs on germ cell development and other biological processes. We particularly emphasize the significance of recently reported RNA modifications in SG stress responses. In parallel, we also review all current perspectives on the roles of SGs in male germ cells, with a particular focus on the dynamics of SG assembly.     

Characterizing mRNA interactions with RNA granules during translation initiation inhibition

When cells experience environmental stresses, global translational arrest is often accompanied by the formation of stress granules (SG) and an increase in the number of p-bodies (PBs), which are thought to play a crucial role in the regulation of eukaryotic gene expression through the control of mRNA translation and degradation. SGs and PBs have been extensively studied from the perspective of their protein content and dynamics but, to date, there have not been systematic studies on how they interact with native mRNA granules. Here, we demonstrate the use of live-cell hybridization assays with multiply-labeled tetravalent RNA imaging probes (MTRIPs) combined with immunofluorescence, as a tool to characterize the polyA+ and β-actin mRNA distributions within the cytoplasm of epithelial cell lines, and the changes in their colocalization with native RNA granules including SGs, PBs and the RNA exosome during the inhibition of translational initiation. Translation initiation inhibition was achieved via the induction of oxidative stress using sodium arsenite, as well as through the use of Pateamine A, puromycin and cycloheximide. This methodology represents a valuable tool for future studies of mRNA trafficking and regulation within living cells.