Epigenetic malleability at core promoter initiates tobacco PR-1a expression post salicylic acid treatment

Niraj Lodhi; Mala Singh; Rakesh Srivastava; Samir V Sawant; Rakesh Tuli

doi:10.1007/s11033-022-08074-w

Epigenetic malleability at core promoter initiates tobacco PR-1a expression post salicylic acid treatment

Mol Biol Rep. 2023 Jan;50(1):417-431. doi: 10.1007/s11033-022-08074-w. Epub 2022 Nov 6.

Authors

Niraj Lodhi^{1

2}, Mala Singh³, Rakesh Srivastava³, Samir V Sawant³, Rakesh Tuli^{3

4}

Affiliations

¹ National Botanical Research Institute, Council of Scientific and Industrial Research, Rana Pratap Marg, Lucknow, 226001, India. lodhinirajp@gmail.com.
² Mirna Analytics, New York, NY, 19047, USA. lodhinirajp@gmail.com.
³ National Botanical Research Institute, Council of Scientific and Industrial Research, Rana Pratap Marg, Lucknow, 226001, India.
⁴ University Institute of Engineering & Technology (UIET), Sector 25, Panjab University, Chandigarh, 160014, India.

PMID: 36335522
DOI: 10.1007/s11033-022-08074-w

Abstract

Background: Tobacco's PR-1a gene is induced by pathogen attack or exogenous application of salicylic acid (SA). Nucleosome mapping and chromatin immunoprecipitation assay were used to delineate the histone modifications on the PR-1a promoter. However, the epigenetic modifications of the inducible promoter of the PR-1a gene are not fully understood yet.

Methods and results: Southern approach was used to scan the promoter of PR-1a to identify presence of nucleosomes, ChIP assays were performed using anti-histones antibodies of repressive chromatin by di- methylated at H3K9 and H4K20 or active chromatin by acetylated H3K9/14 and H4K16 to find epigenetic malleability of nucleosome over core promoter in uninduced or induced state post SA treatment. Class I and II mammalian histone deacetylase (HDAC) inhibitor TSA treatment was used to enhance the expression of PR-1a by facilitating the histone acetylation post SA treatment. Here, we report correlated consequences of the epigenetic modifications correspond to disassembly of the nucleosome (spans from - 102 to + 55 bp, masks TATA and transcription initiation) and repressor complex from core promoter, eventually initiates the transcription of PR-1a gene post SA treatment. While active chromatin marks di and trimethylation of H3K4, acetylation of H3K9 and H4K16 are increased which are associated to the transcription initiation of PR-1a following SA treatment. However, in uninduced state constitutive expression of a negative regulator (SNI1) of AtPR1, suppresses AtPR1 expression by six-fold in Arabidopsis thaliana. Further, we report 50-to-1000-fold increased expression of AtPR1 in uninduced lsd1 mutant plants, up to threefold increased expression of AtPR1 in uninduced histone acetyl transferases (HATs) mutant plants, SNI1 dependent negative regulation of AtPR1, all together our results suggest that inactive state of PR-1a is indeed maintained by a repressive complex.

Conclusion: The study aimed to reveal the mechanism of transcription initiation of tobacco PR-1a gene in presence or absence of SA. This is the first study that reports nucleosome and repressor complex over core promoter region maintains the inactivation of gene in uninduced state, and upon induction disassembling of both initiates the downstream gene activation process.

Keywords: Epigenetics; Histone modifications; LSD1; Nucleosome; PR-1a; Salicylic acid; Transcription; Trichostatin A.

MeSH terms

Acetylation
Animals
Arabidopsis Proteins* / genetics
Arabidopsis Proteins* / metabolism
Arabidopsis* / genetics
Arabidopsis* / metabolism
Chromatin / metabolism
Epigenesis, Genetic
Mammals / metabolism
Nicotiana / genetics
Nicotiana / metabolism
Nuclear Proteins / genetics
Nucleosomes / genetics
Nucleosomes / metabolism
Promoter Regions, Genetic / genetics
Salicylic Acid / metabolism
Salicylic Acid / pharmacology

Substances

Nucleosomes
Salicylic Acid
Chromatin
SNI1 protein, Arabidopsis
Nuclear Proteins
Arabidopsis Proteins