mRNA adenosine methylase (MTA) deposits m6A on pri-miRNAs to modulate miRNA biogenesis inArabidopsis thaliana

Author:

Bhat Susheel SagarORCID,Bielewicz DawidORCID,Gulanicz TomaszORCID,Bodi Zsuzsanna,Yu XiangORCID,Anderson Stephen J.ORCID,Szewc LukaszORCID,Bajczyk MateuszORCID,Dolata JakubORCID,Grzelak Natalia,Smolinski Dariusz J.ORCID,Gregory Brian D.ORCID,Fray Rupert G.ORCID,Jarmolowski Artur,Szweykowska-Kulinska Zofia

Abstract

InArabidopsis thaliana, the METTL3 homolog, mRNA adenosine methylase (MTA) introducesN6-methyladenosine (m6A) into various coding and noncoding RNAs of the plant transcriptome. Here, we show that an MTA-deficient mutant (mta) has decreased levels of microRNAs (miRNAs) but accumulates primary miRNA transcripts (pri-miRNAs). Moreover, pri-miRNAs are methylated by MTA, and RNA structure probing analysis reveals a decrease in secondary structure within stem–loop regions of these transcripts inmtamutant plants. We demonstrate interaction between MTA and both RNA Polymerase II and TOUGH (TGH), a plant protein needed for early steps of miRNA biogenesis. Both MTA and TGH are necessary for efficient colocalization of the Microprocessor components Dicer-like 1 (DCL1) and Hyponastic Leaves 1 (HYL1) with RNA Polymerase II. We propose that secondary structure of miRNA precursors induced by their MTA-dependent m6A methylation status, together with direct interactions between MTA and TGH, influence the recruitment of Microprocessor to plant pri-miRNAs. Therefore, the lack of MTA inmtamutant plants disturbs pri-miRNA processing and leads to the decrease in miRNA accumulation. Furthermore, our findings reveal that reduced miR393b levels likely contributes to the impaired auxin response phenotypes ofmtamutant plants.

Funder

Narodowe Centrum Nauki

Ministerstwo Nauki i Szkolnictwa Wyższego

RCUK | Biotechnology and Biological Sciences Research Council

National Science Foundation

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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