Genome‐wide methylation landscape during somatic embryogenesis in Medicago truncatula reveals correlation between Tnt1 retrotransposition and hyperactive methylation regions

Author:

Nandety Raja Sekhar123ORCID,Oh Sunhee1,Lee Hee‐Kyung1,Krom Nick1,Gupta Rajeev23,Mysore Kirankumar S.145ORCID

Affiliation:

1. Noble Research Institute Ardmore Oklahoma 73401 USA

2. Department of Plant Sciences North Dakota State University Fargo North Dakota 58102 USA

3. Cereal Crops Research Unit USDA‐ARS, Edward T. Schafer Agricultural Research Center Fargo North Dakota 58102 USA

4. Institute for Agricultural Biosciences, Oklahoma State University Ardmore Oklahoma 73401 USA

5. Department of Biochemistry and Molecular Biology Oklahoma State University Stillwater Oklahoma 74078 USA

Abstract

SUMMARYMedicago truncatula is a model legume for fundamental research on legume biology and symbiotic nitrogen fixation. Tnt1, a retrotransposon from tobacco, was used to generate insertion mutants in M. truncatula R108. Approximately 21 000 insertion lines have been generated and publicly available. Tnt1 retro‐transposition event occurs during somatic embryogenesis (SE), a pivotal process that triggers massive methylation changes. We studied the SE of M. truncatula R108 using leaf explants and explored the dynamic shifts in the methylation landscape from leaf explants to callus formation and finally embryogenesis. Higher cytosine methylation in all three contexts of CG, CHG, and CHH patterns was observed during SE compared to the controls. Higher methylation patterns were observed in assumed promoter regions (~2‐kb upstream regions of transcription start site) of the genes, while lowest was recorded in the untranslated regions. Differentially methylated promoter region analysis showed a higher CHH methylation in embryogenesis tissue samples when compared to CG and CHG methylation. Strong correlation (89.71%) was identified between the differentially methylated regions (DMRs) and the site of Tnt1 insertions in M. truncatula R108 and stronger hypermethylation of genes correlated with higher number of Tnt1 insertions in all contexts of CG, CHG, and CHH methylation. Gene ontology enrichment and KEGG pathway enrichment analysis identified genes and pathways enriched in the signal peptide processing, ATP hydrolysis, RNA polymerase activity, transport, secondary metabolites, and nitrogen metabolism pathways. Combined gene expression analysis and methylation profiling showed an inverse relationship between methylation in the DMRs (regions spanning genes) and the expression of genes. Our results show that a dynamic shift in methylation happens during the SE process in the context of CG, CHH and CHG methylation, and the Tnt1 retrotransposition correlates with the hyperactive methylation regions.

Funder

Noble Research Institute

Agricultural Research Service

National Science Foundation

Publisher

Wiley

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