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Profiling of 2′-O-Me in human rRNA reveals a subset of fractionally modified positions and provides evidence for ribosome heterogeneity

机译:人类rRNA中2-O-Me的分析揭示了部分修饰的位置的子集并提供了核糖体异质性的证据

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摘要

Ribose methylation is one of the two most abundant modifications in human ribosomal RNA and is believed to be important for ribosome biogenesis, mRNA selectivity and translational fidelity. We have applied RiboMeth-seq to rRNA from HeLa cells for ribosome-wide, quantitative mapping of 2′-O-Me sites and obtained a comprehensive set of 106 sites, including two novel sites, and with plausible box C/D guide RNAs assigned to all but three sites. We find approximately two-thirds of the sites to be fully methylated and the remainder to be fractionally modified in support of ribosome heterogeneity at the level of RNA modifications. A comparison to HCT116 cells reveals similar 2′-O-Me profiles with distinct differences at several sites. This study constitutes the first comprehensive mapping of 2′-O-Me sites in human rRNA using a high throughput sequencing approach. It establishes the existence of a core of constitutively methylated positions and a subset of variable, potentially regulatory positions, and paves the way for experimental analyses of the role of variations in rRNA methylation under different physiological or pathological settings.
机译:核糖甲基化是人核糖体RNA中两个最丰富的修饰之一,被认为对核糖体的生物发生,mRNA选择性和翻译保真度很重要。我们已将RiboMeth-seq应用于HeLa细胞的rRNA进行了核糖体范围的2'-O-Me位点的定量作图,并获得了106个位点的完整集合,包括两个新位点,并分配了可能的方框C / D指导RNA除三个站点外。我们发现大约三分之二的位点被完全甲基化,其余部分被部分修饰以支持核糖体异质性在RNA修饰水平上。与HCT116细胞的比较揭示了相似的2'-O-Me谱,在几个位点上存在明显差异。这项研究使用高通量测序方法,构成了人类rRNA中2'-O-Me位点的首个综合图谱。它建立了组成性甲基化位置核心和可变的,潜在的调节位置子集的存在,并为在不同生理或病理环境下rRNA甲基化变异作用的实验分析铺平了道路。

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