4.7 Article

5-Methylcytosine RNA Methylation in &ITArabidopsis Thaliana&IT

Journal

MOLECULAR PLANT
Volume 10, Issue 11, Pages 1387-1399

Publisher

CELL PRESS
DOI: 10.1016/j.molp.2017.09.013

Keywords

5-methylcytosine (m(5)C); Arabidopsis; RNA methylation; TRM4B; root development

Funding

  1. Chinese academy of Agricultural Sciences
  2. National University of Singapore Temasek Life Sciences Laboratory
  3. Elite Youth Program of the Chinese Academy of Agricultural Science
  4. Recruitment program of Global Youth Expert of China
  5. Singapore National Research Foundation Investigatorship Program [NRF-NRFI2016-02]
  6. Academic Research Fund from the Ministry of Education - Singapore [MOE2015-T2-1-002]

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5-Methylcytosine (m(5)C) is a well-characterized DNA modification, and is also predominantly reported in abundant non-coding RNAs in both prokaryotes and eukaryotes. However, the distribution and biological functions of m(5)C in plant mRNAs remain largely unknown. Here, we report transcriptome-wide profiling of RNA m(5)C in Arabidopsis thaliana by applying m(5)C RNA immunoprecipitation followed by a deep-sequencing approach (m(5)C-RIP-seq). LC-MS/MS and dot blot analyses reveal a dynamic pattern of m(5)C mRNA modification in various tissues and at different developmental stages. m(5)C-RIP-seq analysis identified 6045 m(5)C peaks in 4465 expressed genes in young seedlings. We found that m(5)C is enriched in coding sequences with two peaks located immediately after start codons and before stop codons, and is associated with mRNAs with low translation activity. We further demonstrated that an RNA (cytosine-5)-methyl-transferase, tRNA-specific methyltransferase 4B (TRM4B), exhibits m(5)C RNA methyltransferase activity. Mutations in TRM4B display defects in root development and decreased m(5)C peaks. TRM4B affects the transcript levels of the genes involved in root development, which is positively correlated with their mRNA stability and m(5)C levels. Our results suggest that m(5)C in mRNA is a new epitranscriptome marker in Arabidopsis, and that regulation of this modification is an integral part of gene regulatory networks underlying plant development.

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