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鉴定小鼠精原干细胞中 small RNA 甲基转移酶 Hen1 的底物,并分析其甲基转移酶结构域。

Identification of substrates of the small RNA methyltransferase Hen1 in mouse spermatogonial stem cells and analysis of its methyl-transfer domain.

机构信息

From the State Key Laboratory of Molecular Biology, National Center for Protein Science Shanghai, Shanghai Science Research Center, Shanghai Key Laboratory of Molecular Andrology, CAS Center for Excellence in Molecular Cell Science, Shanghai Institute of Biochemistry and Cell Biology, Chinese Academy of Sciences, University of Chinese Academy of Sciences.

the School of Life Science and Technology, ShanghaiTech University, Shanghai 201210, China.

出版信息

J Biol Chem. 2018 Jun 29;293(26):9981-9994. doi: 10.1074/jbc.RA117.000837. Epub 2018 Apr 27.

Abstract

Small noncoding RNAs (sncRNAs) regulate many genes in eukaryotic cells. Hua enhancer 1 (Hen1) is a 2'--methyltransferase that adds a methyl group to the 2'-OH of the 3'-terminal nucleotide of sncRNAs. The types and properties of sncRNAs may vary among different species, and the domain composition, structure, and function of Hen1 proteins differ accordingly. In mammals, Hen1 specifically methylates sncRNAs called P-element-induced wimpy testis-interacting RNAs (piRNAs). However, other types of sncRNAs that are methylated by Hen1 have not yet been reported, and the structures and the substrates of mammalian Hen1 remain unknown. Here, we report that mouse Hen1 (mHen1) performs 3'-end methylation of classical piRNAs, as well as those of most noncanonical piRNAs derived from rRNAs, small nuclear RNAs and tRNAs in murine spermatogonial stem cells. Moreover, we found that a distinct class of tRNA-derived sncRNAs are mHen1 substrates. We further determined the crystal structure of the putative methyltransferase domain of human Hen1 (HsHen1) in complex with its cofactor AdoMet at 2.0 Å resolution. We observed that HsHen1 has an active site similar to that of plant Hen1. We further found that the putative catalytic domain of HsHen1 alone exhibits no activity. However, an FPP motif at its N terminus conferred full activity to this domain, and additional binding assays suggested that the FPP motif is important for substrate binding. Our findings shed light on its methylation substrates in mouse spermatogonial stem cells and the substrate-recognition mechanism of mammalian Hen1.

摘要

小非编码 RNA(sncRNA)调节真核细胞中的许多基因。Hua 增强子 1(Hen1)是一种 2'-甲基转移酶,它在 sncRNA 的 3'-末端核苷酸的 2'-OH 上添加一个甲基。sncRNA 的类型和性质可能在不同物种之间有所不同,相应地,Hen1 蛋白的结构域组成、结构和功能也有所不同。在哺乳动物中,Hen1 特异性地甲基化称为 P 元素诱导的软弱睾丸相互作用 RNA(piRNA)的 sncRNA。然而,尚未报道 Hen1 甲基化的其他类型的 sncRNA,并且哺乳动物 Hen1 的结构和底物仍然未知。在这里,我们报告小鼠 Hen1(mHen1)在精原干细胞中对经典 piRNA 以及来自 rRNA、小核 RNA 和 tRNA 的大多数非典型 piRNA 进行 3'-末端甲基化。此外,我们发现一类独特的 tRNA 衍生的 sncRNA 是 mHen1 的底物。我们进一步确定了与 AdoMet 共因子复合的人 Hen1(HsHen1)的假定甲基转移酶结构域的晶体结构,分辨率为 2.0 Å。我们观察到 HsHen1 具有与植物 Hen1 相似的活性位点。我们进一步发现 HsHen1 的假定催化结构域单独没有活性。然而,其 N 末端的 FPP 基序赋予该结构域完整的活性,并且额外的结合测定表明该 FPP 基序对底物结合很重要。我们的研究结果揭示了其在小鼠精原干细胞中的甲基化底物和哺乳动物 Hen1 的底物识别机制。

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