| Literature DB >> 33406971 |
Sangrea Shim1,2, Hong Gil Lee1,2, Ok-Sun Park3, Hosub Shin4, Kyounghee Lee3, Hongwoo Lee1, Jin Hoe Huh2,4, Pil Joon Seo1,2,3.
Abstract
Plant somatic cells can be reprogrammed into pluripotent cell mass, called callus, through a two-step in vitro tissue culture method. Incubation on callus-inducing medium triggers active cell proliferation to form a pluripotent callus. Notably, DNA methylation is implicated during callus formation, but a detailed molecular process regulated by DNA methylation remains to be fully elucidated. Here, we compared genome-wide DNA methylation profiles between leaf and callus tissues in Arabidopsis using whole-genome bisulphite-sequencing. Global distribution of DNA methylation showed that CHG methylation was increased, whereas CHH methylation was reduced especially around transposable element (TE) regions during the leaf-to-callus transition. We further analysed differentially expressed genes around differentially methylated TEs (DMTEs) during the leaf-to-callus transition and found that genes involved in cell cycle regulation were enriched and also constituted a coexpression gene network along with pluripotency regulators. In addition, a conserved DNA sequence analysis for upstream cis-elements led us to find a putative transcription factor associated with cell fate transition. CIRCADIAN CLOCK-ASSOCIATED 1 (CCA1) was newly identified as a regulator of plant regeneration, and consistently, the cca1lhy mutant displayed altered phenotypes in callus proliferation. Overall, these results suggest that DNA methylation coordinates cell cycle regulation during callus formation, and CCA1 may act as a key upstream coordinator at least in part in the processes.Entities:
Keywords: Arabidopsis; CCA1; DNA methylation; TE; callus
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Year: 2021 PMID: 33406971 PMCID: PMC8812807 DOI: 10.1080/15592294.2021.1872927
Source DB: PubMed Journal: Epigenetics ISSN: 1559-2294 Impact factor: 4.528