Provost Patrick, Dishart David, Doucet Johanne, Frendewey David, Samuelsson Bengt, Rådmark Olof
Department of Medical Biochemistry and Biophysics, Karolinska Institute, Scheeles väg 2, Stockholm, S-171 77, Sweden.
EMBO J. 2002 Nov 1;21(21):5864-74. doi: 10.1093/emboj/cdf578.
RNA silencing phenomena, known as post-transcriptional gene silencing in plants, quelling in fungi, and RNA interference (RNAi) in animals, are mediated by double-stranded RNA (dsRNA) and mechanistically intersect at the ribonuclease Dicer. Here, we report cloning and expression of the 218 kDa human Dicer, and characterization of its ribonuclease activity and dsRNA-binding properties. The recombinant enzyme generated approximately 21-23 nucleotide products from dsRNA. Processing of the microRNA let-7 precursor by Dicer produced an apparently mature let-7 RNA. Mg(2+) was required for dsRNase activity, but not for dsRNA binding, thereby uncoupling these reaction steps. ATP was dispensable for dsRNase activity in vitro. The Dicer.dsRNA complex formed at high KCl concentrations was catalytically inactive, suggesting that ionic interactions are involved in dsRNA cleavage. The putative dsRNA-binding domain located at the C-terminus of Dicer was demonstrated to bind dsRNA in vitro. Human Dicer expressed in mammalian cells colocalized with calreticulin, a resident protein of the endoplasmic reticulum. Availability of the recombinant Dicer protein will help improve our understanding of RNA silencing and other Dicer-related processes.
RNA沉默现象,在植物中被称为转录后基因沉默,在真菌中称为压制,在动物中称为RNA干扰(RNAi),由双链RNA(dsRNA)介导,并在核糖核酸酶Dicer处发生机制上的交叉。在此,我们报告了218 kDa人Dicer的克隆与表达,及其核糖核酸酶活性和dsRNA结合特性的表征。重组酶从dsRNA产生约21 - 23个核苷酸的产物。Dicer对微小RNA let - 7前体的加工产生了明显成熟的let - 7 RNA。dsRNase活性需要Mg(2+),但dsRNA结合不需要,从而使这些反应步骤解偶联。ATP在体外对dsRNase活性是可有可无的。在高KCl浓度下形成的Dicer.dsRNA复合物没有催化活性,表明离子相互作用参与dsRNA切割。位于Dicer C末端的假定dsRNA结合结构域在体外被证明能结合dsRNA。在哺乳动物细胞中表达的人Dicer与内质网驻留蛋白钙网蛋白共定位。重组Dicer蛋白的可得性将有助于增进我们对RNA沉默及其他与Dicer相关过程的理解。