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Caenorhabditis elegans PRMT-7 and PRMT-9 Are Evolutionarily Conserved Protein Arginine Methyltransferases with Distinct Substrate Specificities

机译:CaenorhabditiseDeltans PRMT-7和PRMT-9正在进化水保守的蛋白质精氨酸甲基转移酶,具有不同的底物特异性

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Caenorhabditis elegans protein arginine methyltransferases PRMT-7 and PRMT-9 are two evolutionarily conserved enzymes, with distinct orthologs in plants, invertebrates, and vertebrates. Biochemical characterization of these two enzymes reveals that they share much in common with their mammalian orthologs. C. elegans PRMT-7 produces only monomethylarginine (MMA) and preferentially methylates R-X-R motifs in a broad collection of substrates, including human histone peptides and RGrich peptides. In addition, the activity of the PRMT-7 enzyme is dependent on temperature, the presence of metal ions, and the reducing agent dithiothreitol. C. elegans PRMT-7 has a substrate specificity and a substrate preference different from those of mammalian PRMT7, and the available X-ray crystal structures of the PRMT7 orthologs show differences in active site architecture. C. elegans PRMT-9, on the other hand, produces symmetric dimethylarginine and MMA on SFTB-2, the conserved C. elegans ortholog of human RNA splicing factor SF3B2, indicating a possible role in the regulation of nematode splicing. In contrast to PRMT-7, C. elegans PRMT-9 appears to be biochemically indistinguishable from its human ortholog.
机译:胶虫杆菌蛋白质精氨酸甲基转移酶PRMT-7和PRMT-9是两种进化的保守酶,植物,无脊椎动物和脊椎动物中具有明显的突出菌。这两种酶的生化表征揭示它们与哺乳动物的原言相同。 C. Elegans PRMT-7仅生产单体虫碱(MMA),优先甲酸盐甲酸族甲基化物甲基酯,包括人类组蛋白肽和RGRICH肽。此外,PRMT-7酶的活性依赖于温度,金属离子的存在和还原剂二硫醇。 C. Elegans PRMT-7具有与哺乳动物PRMT7不同的底物特异性和基材偏好,并且PRMT7 Orthologs的可用X射线晶体结构显示有源站点架构的差异。另一方面,C. Elegans PRMT-9在SFTB-2上产生对称的Dimethyl垄和MMA,是人RNA剪接因子SF3B2的保守的C. elegans Orthologogog,表明在线虫剪接调节中可能作用。与PRMT-7相比,C. elegans prmt-9似乎与人类的ortholog难以区分。

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