J Integr Plant Biol.

• Research Article •    

UBA2A regulates seed dormancy and the stability of chromatin-retained DOG1 messenger RNA

Ce Wang1,2,3, Lien Brzezniak1, Sebastian Sacharowski1, Michal Krzyszton1, Veena Halale Manjunath1,2, Mateusz Jan Olechowski2,4, Anna Kulik4 and Szymon Swiezewski1*   

  1. 1. Laboratory of Seeds Molecular Biology, Institute of Biochemistry and Biophysics, Polish Academy of Sciences, Warsaw 02‐106, Poland
    2. Doctoral School of Molecular Biology and Biological Chemistry, Institute of Biochemistry and Biophysics of the Polish Academy of Sciences, Warsaw 02‐106, Poland
    3. Department of Biology, University of Fribourg, Fribourg 1700, Switzerland
    4. Laboratory of Plant Protein Phosphorylation, Institute of Biochemistry and Biophysics, Polish Academy of Sciences, Warsaw 02‐106, Poland

    *Correspondence: Szymon Swiezewski (sswiez@ibb.waw.pl)
  • Received:2023-11-22 Accepted:2025-08-01 Online:2025-10-23
  • Supported by:
    The authors would like to acknowledge the help of Krzysztof Kokoszka with glasshouse and lab maintenance support, and all the members of the Swiezewski lab for discussions. M.K. was supported by the National Science Centre, Poland (Grant Nos. OPUS UMO‐2021/41/B/NZ3/02605 and OPUS UMO‐2024/53/B/NZ3/02252). V.H.M. was supported by the National Science Centre, Poland (Grant No. PRELUDIUM UMO‐2024/53/N/NZ3/02320). Se.S. was supported by the National Science Centre, Poland (Grant No. NCN OPUS 2024/53/B/NZ1/03741). S.S. was supported by Foundation for Polish Science (Grant No. FNP TEAM POIR.04.04.00‐00‐3C97/16). L.B. was supported by Foundation for Polish Science (Grant No. FNP POWROTY POIR.04.04.00‐00‐3F86/17‐00). S.S. and L.B. were supported by the National Science Centre, Poland (Grant No. 2023/50/E/NZ3/00043). N.G.S. was performed thanks to the Genomics Core Facility CeNT UW (Grant No. RRID:SCR_022718), using the NovaSeq. 6000 platform financed by the Polish Ministry of Science and Higher Education (decision No. 6817/IA/SP/2018 of 2018‐04‐10). This study was supported by the Institute of Biochemistry and Biophysics PAS Internal Grant MG‐05‐22‐02.

Abstract: Multiple factors control primary seed dormancy established during seed maturation and secondary seed dormancy initiated when a non-dormant imbibed seed is exposed to adverse conditions. A key player in the control of primary and secondary dormancy in Arabidopsis thaliana is the Delay of Germination 1 (DOG1) gene, the expression of which is extensively regulated at the transcriptional and co-transcriptional levels. Despite its importance, the influence of post-transcriptional messenger RNA (mRNA) processing and mRNA storage of DOG1 on the determination of dormancy depth remains elusive. Here, we show that the UBA2A protein, a member of the heterogeneous nuclear ribonucleoprotein (hnRNP) family, negatively regulates primary and secondary seed dormancy through the regulation of the DOG1 gene expression at the post-transcriptional level. uba2a mutants show higher levels of the DOG1 mRNA. Surprisingly, DOG1 gene transcription is not affected, as demonstrated by single-molecule fluorescent in situ hybridization, chromatin-attached mRNA analysis and Pol II chromatin immunoprecipitation (ChIP). Instead, our results show that the UBA2A protein decreases the stability of both chromatin-bound and cytoplasmic DOG1 mRNA pools, and results in higher chromatin retention of DOG1 mRNA in the uba2a mutant. Our study highlights chromatin retention and mRNA stability as important features of DOG1 gene expression regulation with a profound impact on dormancy establishment and shows that UBA2A protein, like its human homolog hnRNPAB, is most likely implicated in mRNA transport in the cell.

Key words: DOG1 regulation, post‐transcriptional regulation, seed dormancy

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