Dynamic rRNA methylation regulates translation in the hematopoietic system and is essential for stem cell fitness

生物 翻译(生物学) 甲基化 造血干细胞 干细胞 平动调节 DNA甲基化 细胞生物学 遗传学 造血 调节器 表观遗传学 核糖体 RNA甲基化 翻译效率 细胞分化 核糖体RNA 基因表达调控 核糖核酸 计算生物学 信使核糖核酸 真核翻译 多形体 RNA结合蛋白
作者
Ofri Rabany,Sivan Ben Dror,Maram Arafat,Hadar Aharoni levitanus,Yudit Halperin,Virginie Marchand,Nikolai Romanovski,Noga Ussishkin,Maayan Livneh Golany,Adi Reches,J. Wexler,Nina Mayorek,Galya Monderer‐Rothkoff,Sagiv Shifman,Widad Mâmmer Bouhou,Michael VanInsberghe,Cornelius Pauli,Carsten Müller‐Tidow,Ola Karmi,Yoav Livneh
出处
期刊:Blood [Elsevier BV]
卷期号:147 (5): 520-533 被引量:1
标识
DOI:10.1182/blood.2024028300
摘要

Self-renewal and differentiation are at the basis of hematopoiesis. Although it is known that tight regulation of translation is vital for hematopoietic stem cells' (HSC) biology, the mechanisms underlying translation regulation across the hematopoietic system remain obscure. Here, we reveal a novel mechanism of translation regulation in the hematopoietic hierarchy, which is mediated by rRNA methylation dynamics. Using ultralow-input ribosome profiling, we characterized cell-type-specific translation capacity during erythroid differentiation. We found that translation efficiency (TE) changes progressively with differentiation and can distinguish between discrete cell populations, as well as define differentiation trajectories. To reveal the underlying mechanism, we performed comprehensive mapping of the most abundant rRNA modification, 2'-O-methyl (2'OMe). We found that, such as TE, 2'OMe dynamics followed a distinct trajectory during erythroid differentiation. Genetic perturbation of individual 2'OMe sites demonstrated their distinct roles in modulating proliferation and differentiation. By combining CRISPR screening, molecular, and functional analyses, we identified a specific methylation site, 28S-Gm4588, which is progressively lost during differentiation, as a key regulator of HSC self-renewal. We showed that low methylation at this site led to translational skewing, mediated mainly by codon frequency, which promoted differentiation. Functionally, HSC with diminished 28S-Gm4588 methylation exhibited impaired self-renewal capacity ex vivo, and loss of fitness in vivo in bone marrow transplants. Extending our findings beyond the hematopoietic system, we also found distinct dynamics of 2'OMe profiles during differentiation of non-HSC. Our findings reveal rRNA methylation dynamics as a general mechanism for cell-type-specific translation, required for cell function and differentiation.
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