Methylome decoding of RdDM-mediated reprogramming effects in the Arabidopsis MSH1 system

Hardik Kundariya; Robersy Sanchez; Xiaodong Yang; Alenka Hafner; Sally A. Mackenzie

doi:10.1186/s13059-022-02731-w

Genome Biology (Aug 2022)

Methylome decoding of RdDM-mediated reprogramming effects in the Arabidopsis MSH1 system

Hardik Kundariya,
Robersy Sanchez,
Xiaodong Yang,
Alenka Hafner,
Sally A. Mackenzie

Affiliations

Hardik Kundariya: Department of Biology, The Pennsylvania State University
Robersy Sanchez: Department of Biology, The Pennsylvania State University
Xiaodong Yang: Department of Biology, The Pennsylvania State University
Alenka Hafner: Department of Biology, The Pennsylvania State University
Sally A. Mackenzie: Department of Biology, The Pennsylvania State University

DOI: https://doi.org/10.1186/s13059-022-02731-w
Journal volume & issue: Vol. 23, no. 1
pp. 1 – 27

Abstract

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Abstract Background Plants undergo programmed chromatin changes in response to environment, influencing heritable phenotypic plasticity. The RNA-directed DNA methylation (RdDM) pathway is an essential component of this reprogramming process. The relationship of epigenomic changes to gene networks on a genome-wide basis has been elusive, particularly for intragenic DNA methylation repatterning. Results Epigenomic reprogramming is tractable to detailed study and cross-species modeling in the MSH1 system, where perturbation of the plant-specific gene MSH1 triggers at least four distinct nongenetic states to impact plant stress response and growth vigor. Within this system, we have defined RdDM target loci toward decoding phenotype-relevant methylome data. We analyze intragenic methylome repatterning associated with phenotype transitions, identifying state-specific cytosine methylation changes in pivotal growth-versus-stress, chromatin remodeling, and RNA spliceosome gene networks that encompass 871 genes. Over 77% of these genes, and 81% of their central network hubs, are functionally confirmed as RdDM targets based on analysis of mutant datasets and sRNA cluster associations. These dcl2/dcl3/dcl4-sensitive gene methylation sites, many present as singular cytosines, reside within identifiable sequence motifs. These data reflect intragenic methylation repatterning that is targeted and amenable to prediction. Conclusions A prevailing assumption that biologically relevant DNA methylation variation occurs predominantly in density-defined differentially methylated regions overlooks behavioral features of intragenic, single-site cytosine methylation variation. RdDM-dependent methylation changes within identifiable sequence motifs reveal gene hubs within networks discriminating stress response and growth vigor epigenetic phenotypes. This study uncovers components of a methylome “code” for de novo intragenic methylation repatterning during plant phenotype transitions.

Published in Genome Biology

ISSN: 1474-760X (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Science: Biology (General): Genetics
Website: https://genomebiology.biomedcentral.com/

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