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基于MapID的人类转运RNA化学修饰与表达的定量图谱分析。

MapID-based quantitative mapping of chemical modifications and expression of human transfer RNA.

作者信息

Tepe Mitchel L, Chen Yitan, Carso Allison, Zhou Huiqing

机构信息

Chemistry Department, Boston College, Chestnut Hill, MA 02467, USA.

Chemistry Department, Boston College, Chestnut Hill, MA 02467, USA.

出版信息

Cell Chem Biol. 2025 May 15;32(5):752-766.e7. doi: 10.1016/j.chembiol.2025.04.003. Epub 2025 May 2.

Abstract

Detection and quantification of tRNA chemical modifications are critical for understanding their regulatory functions in biology and diseases. However, tRNA-seq-based methods for modification mapping encountered challenges both experimentally (poor processivity of heavily modified tRNAs during reverse transcription or RT) and bioinformatically (frequent reads misalignment to highly similar tRNA genes). Here, we report "MapID-tRNA-seq" where we deployed an evolved reverse transcriptase (RT-1306) into tRNA-seq and developed "MapIDs" that reduce redundancy of the human tRNA genome and explicitly annotate genetic variances. RT-1306 generated robust mutations against mA and mC, and RT stops against multiple bulky roadblock modifications. MapID-assisted data processing enabled systematic exclusion of false-positive discoveries of modifications which arise from reads misalignment onto similar genes. We applied MapID-tRNA-seq into mapping mA, mC and expression levels of tRNAs in three mammary cell lines, which revealed cell-type dependent modification sites and potential translational regulation of the reduced mitochondrial activities in breast cancer.

摘要

检测和定量tRNA的化学修饰对于理解其在生物学和疾病中的调控功能至关重要。然而,基于tRNA测序的修饰图谱绘制方法在实验方面(反转录过程中高度修饰的tRNA延伸能力差)和生物信息学方面(频繁出现读段与高度相似的tRNA基因错配)都面临挑战。在此,我们报告了“MapID-tRNA-seq”,我们将一种经过进化的逆转录酶(RT-1306)应用于tRNA测序,并开发了“MapIDs”,其减少了人类tRNA基因组的冗余,并明确注释了遗传变异。RT-1306对mA和mC产生了稳定的突变,对多种大体积阻碍性修饰产生了逆转录终止。MapID辅助的数据处理能够系统地排除因读段错配到相似基因上而产生的修饰假阳性发现。我们将MapID-tRNA-seq应用于三种乳腺细胞系中tRNA的mA、mC修饰图谱绘制及表达水平分析,结果揭示了细胞类型依赖性修饰位点以及乳腺癌中线粒体活性降低的潜在翻译调控。

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