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盒 C/D RNA 引导的 RNA 甲基转移酶的功能组织。

Functional organization of box C/D RNA-guided RNA methyltransferase.

机构信息

Key Laboratory of RNA Biology, CAS Center for Excellence in Biomacromolecules, Institute of Biophysics, Chinese Academy of Sciences, Beijing 100101, China.

Institute of Chinese Integrative Medicine, Hebei Medical University, Shijiazhuang 050017, Hebei, China.

出版信息

Nucleic Acids Res. 2020 May 21;48(9):5094-5105. doi: 10.1093/nar/gkaa247.

Abstract

Box C/D RNA protein complexes (RNPs) catalyze site-specific 2'-O-methylation of RNA with specificity determined by guide RNAs. In eukaryotic C/D RNP, the paralogous Nop58 and Nop56 proteins specifically associate with terminal C/D and internal C'/D' motifs of guide RNAs, respectively. We have reconstituted active C/D RNPs with recombinant proteins of the thermophilic yeast Chaetomium thermophilum. Nop58 and Nop56 could not distinguish between the two C/D motifs in the reconstituted enzyme, suggesting that the assembly specificity is imposed by trans-acting factors in vivo. The two C/D motifs are functionally independent and halfmer C/D RNAs can also guide site-specific methylation. Extensive pairing between C/D RNA and substrate is inhibitory to modification for both yeast and archaeal C/D RNPs. N6-methylated adenine at box D/D' interferes with the function of the coupled guide. Our data show that all C/D RNPs share the same functional organization and mechanism of action and provide insight into the assembly specificity of eukaryotic C/D RNPs.

摘要

盒 C/D RNA 蛋白复合物 (RNP) 以指导 RNA 决定的特异性催化 RNA 的特异性 2'-O-甲基化。在真核 C/D RNP 中,两个类似的 Nop58 和 Nop56 蛋白分别与指导 RNA 的末端 C/D 和内部 C'/D' 基序特异性结合。我们已经用嗜热酵母 Chaetomium thermophilum 的重组蛋白重新组成了活性 C/D RNP。Nop58 和 Nop56 不能区分重组酶中的两种 C/D 基序,这表明组装特异性是由体内的反式作用因子决定的。这两个 C/D 基序在功能上是独立的,半 C/D RNA 也可以指导特异性甲基化。C/D RNA 与底物之间的广泛配对对酵母和古菌 C/D RNP 的修饰均有抑制作用。盒 D/D' 处的 N6-甲基腺嘌呤干扰了偶联指导的功能。我们的数据表明,所有 C/D RNP 都具有相同的功能组织和作用机制,并为真核 C/D RNP 的组装特异性提供了深入的了解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/daef/7229835/a058b8d27458/gkaa247fig1.jpg

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