Enzymatic cleavage of RNA by RNA

The catalytic activity of E. coli RNase P, an enzyme essential for tRNA biosynthesis in vivo, resides in the RNA subunit of the enzyme. This RNA, which has all the properties of a classical enzyme, can cleave precursor tRNAs in vitro in the total absence of proteins.     

Enzymatic cleavage of RNA by RNA

The discovery and characterization of the catalytic RNA subunit of the enzyme ribonuclease P ofEscherichia coli is described.Nobel lecture given on December 8, 1989, by Professor Sidney Altman, and published in LES PRIX NOBEL 1989, printed in Sweden by Norstedts Tryckeri, Stockholm, Sweden, 1990, republished here with the permission of the Nobel Foundation, the copyright holder.     

Moving RNA moves RNA forward

Cell communication affects all aspects of cell structure and behavior, such as cell proliferation, differentiation, division, and coordination of various physiological functions. The moving RNA in plants and mammalian cells indicates that nucleic acid could be one of the various types of messengers for cell communication. The microvesicle is a critical pathway that mediates RNA moving and keeps moving RNA stable in body fluids. When moving miRNA enters the target cell, it functions by altering the gene expression profile and significantly inhibiting mRNA translation in recipient cells. Thus, moving RNA may act as a long-range modulator during development, organogenesis, and tumor metastasis.     

Catalytic RNA and RNA Splicing

The capacity of Watson-Crick base-pair complementarity to directinformational transactions basic to gene expression has longbeen appreciated. Among RNA molecules, it mediates mRNA-tRNAcodon-anticodon pairing and the 16S rRNA-mRNA Shine-Dalgarnointeraction. More recently, we have come to realize that therole of RNA may transcend that of intermolecular recognition,per se, to include catalysis. Following the tour-de-force studiesof the self-splicing Tetrahymena rRNA precursor, the stage isnow set for the primary role of RNA to be revealed in nuclearpre-RNA splicing, which is catalyzed by a large ribonucleoprotein(RNP) complex in the cell nucleus, called the spliceosome. Theremoval of introns from nuclear pre-messenger RNA (pre-mRNA)shares fundamental properties with certain RNA self-splicingreactions. It therefore seems likely that the major catalyticstrategies in nuclear pre-mRNA splicing are carried out by thesmall nuclear RNAs (snRNAs), which are major constituents ofthe spliceosome.     

非编码RNA和RNA沉默

生物体内存在大量的非编码RNA ,它们形态各异 ,功能也千差万别 ,在生物的生长、发育、分化进程中扮演着不同的角色 ,尤其是siRNA ,它是RNA沉默的诱因。RNA沉默是真核生物特有的现象 ,它需要一系列因子的参与 ,其中RNA依赖性的RNA聚合酶是沉默起始的关键 ,Dicer酶是形成siRNA的基础 ,而RNA沉默诱导复合体 (RSIC)等是发生RNA沉默“链式反应”的关键因子     

RNA编辑功能和RNA干扰

RNA编辑被认为是生命体一种新的基因加工与修饰现象,是指DNA转录成RNA后除RNA剪切外的其他加工过程,以核苷酸的删除、插入或替换等方式改变遗传信息,揭示生物进化过程中基因修饰和调控的另一个重要途径,是对中心法则的重要补充.而RNAi是一种由dsRNA介导的,在转录水平、转录后水平和翻译水平上阻断基因表达的基因调节途径.着重介绍 RNA编辑功能、RNA编辑与RNA干扰关系.     

RNA helicases: modulators of RNA structure

RNA molecules play an essential role in many cellular processes, often as components of ribonucleoprotein complexes. Like proteins, RNA molecules adopt sequence-specific secondary and tertiary structures that are essential for function; alteration of these structures therefore provides a means of regulating RNA function. The discovery of DEAD box proteins, a large family of proteins that share several highly conserved motifs and have known or putative ATP-dependent RNA helicase activity, has provoked growing interest in the concept that regulation of RNA function may occur through local unwinding of complex RNA structures.     

Sephadex-binding RNA ligands: rapid affinity purification of RNA from complex RNA mixtures

Sephadex-binding RNA ligands (aptamers) were obtained through in vitro selection. They could be classified into two groups based on their consensus sequences and the aptamers from both groups showed strong binding to Sephadex G-100. One of the highest affinity aptamers, D8, was chosen for further characterization. Aptamer D8 bound to dextran B512, the soluble base material of Sephadex, but not to isomaltose, isomaltotriose and isomaltotetraose, suggesting that its optimal binding site might consist of more than four glucose residues linked via alpha-1,6 linkages. The aptamer was very specific to the Sephadex matrix and did not bind appreciably to other supporting matrices, such as Sepharose, Sephacryl, cellulose or pustulan. Using Sephadex G-100, the aptamer could be purified from a complex mixture of cellular RNA, giving an enrichment of at least 60 000-fold, compared with a non-specific control RNA. These RNA aptamers can be used as affinity tags for RNAs or RNA subunits of ribonucleoproteins to allow rapid purification from complex mixtures of RNA using only Sephadex.     

Completion of RNA synthesis by viral RNA replicases

How the 5′-terminus of the template affects RNA synthesis by viral RNA replicases is poorly understood. Using short DNA, RNA and RNA–DNA chimeric templates that can direct synthesis of replicase products, we found that DNA templates tend to direct the synthesis of RNA products that are shorter by 1 nt in comparison to RNA templates. Template-length RNA synthesis was also affected by the concentration of nucleoside triphosphates, the identity of the bases at specific positions close to the 5′-terminus and the C2′-hydroxyl of a ribose at the third nucleotide from the 5′-terminal nucleotide. Similar requirements are observed with two bromoviral replicases, but not with a recombinant RNA-dependent RNA polymerase. These results begin to define the interactions needed for the viral replicase to complete synthesis of viral RNA.     

Suppression of RNA interference by adenovirus virus-associated RNA

We show that human adenovirus inhibits RNA interference (RNAi) at late times of infection by suppressing the activity of two key enzyme systems involved, Dicer and RNA-induced silencing complex (RISC). To define the mechanisms by which adenovirus blocks RNAi, we used a panel of mutant adenoviruses defective in virus-associated (VA) RNA expression. The results show that the virus-associated RNAs, VA RNAI and VA RNAII, function as suppressors of RNAi by interfering with the activity of Dicer. The VA RNAs bind Dicer and function as competitive substrates squelching Dicer. Further, we show that VA RNAI and VA RNAII are processed by Dicer, both in vitro and during a lytic infection, and that the resulting short interfering RNAs (siRNAs) are incorporated into active RISC. Dicer cleaves the terminal stem of both VA RNAI and VA RNAII. However, whereas both strands of the VA RNAI-specific siRNA are incorporated into RISC, the 3' strand of the VA RNAII-specific siRNA is selectively incorporated during a lytic infection. In summary, our work shows that adenovirus suppresses RNAi during a lytic infection and gives insight into the mechanisms of RNAi suppression by VA RNA.