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Mitochondrial glutamate dehydrogenase from Leishmania tarentolae is a guide RNA-binding protein.

机译:来自塔氏利什曼原虫的线粒体谷氨酸脱氢酶是一种指导性RNA结合蛋白。

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To identify specific proteins interacting with guide RNAs (gRNAs) in mitochondrial ribonucleoprotein complexes from Leishmania tarentolae, fractionated and unfractionated mitochondrial extracts were subjected to UV cross-linking with added labeled gRNA and also with [alpha-32P]UTP-labeled endogenous RNA. An abundant 110-kDa protein (p110) localized in the T-V complex, which sediments in glycerol gradients at the leading edge of the 10S terminal uridylyltransferase peak, was found to interact with both types of labeled RNAs. The p110 protein was gel isolated and subjected to microsequence analysis, and the gene was cloned. The sequence revealed significant similarity with mitochondrial glutamate dehydrogenases. A polyclonal antiserum was raised against a recombinant fragment of the p110 gene and was used to demonstrate a stable and specific gRNA-binding activity by coimmunoprecipitation and competitive gel shift analyses. Complex formation was strongly inhibited by competition with poly(U) or by deletion or substitution of the gRNA 3' oligo(U) tail. Also, addition of a 3' oligo(U) tail to an unrelated transcript was sufficient for p110 binding. Both the gRNA-binding activity of the p110 protein and in vitro gRNA-independent and gRNA-dependent uridine insertion activities in the mitochondrial extract were inhibited by high concentrations of dinucleotides.
机译:为了鉴定与来自塔氏利什曼原虫的线粒体核糖核蛋白复合物中的指导RNA(gRNA)相互作用的特定蛋白质,将分级和未分级的线粒体提取物与添加的标记gRNA以及[α-32P] UTP标记的内源RNA进行UV交联。发现存在于T-V复合物中的大量110-kDa蛋白(p110)沉积在10S末端uridylyltransferase峰前沿的甘油梯度中,与两种类型的标记RNA相互作用。凝胶分离p110蛋白并进行微序列分析,并克隆该基因。该序列显示出与线粒体谷氨酸脱氢酶的显着相似性。产生了针对p110基因重组片段的多克隆抗血清,并用于通过免疫共沉淀和竞争性凝胶位移分析证明稳定且特异性的gRNA结合活性。与poly(U)竞争或gRNA 3'oligo(U)尾部的缺失或取代强烈抑制了复合物的形成。同样,在无关的转录本上添加3'oligo(U)尾部足以结合p110。高浓度的二核苷酸会抑制p110蛋白的gRNA结合活性以及线粒体提取物中的体外gRNA依赖性和gRNA依赖性尿苷插入活性。

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