Literature DB >> 31268601

Genome-scale, single-cell-type resolution of microRNA activities within a whole plant organ.

Christopher Andrew Brosnan1, Alexis Sarazin1, PeiQi Lim1, Nicolas Gerardo Bologna1, Matthias Hirsch-Hoffmann1, Olivier Voinnet1.   

Abstract

Loaded into ARGONAUTE(AGO) proteins, eukaryotic micro(mi)RNAs regulate gene expression via cleavage, translational repression, and/or accelerated decay of sequence-complementary target transcripts. Despite their importance in development, cell identity maintenance and stress responses, how individual miRNAs contribute to spatial gene regulation within the complex cell mosaics formed in tissues/organs has remained inaccessible in any organism to date. We have developed a non-invasive methodology to examine, at single-cell-type resolution, the AGO-loading and activity patterns of entire miRNA cohorts in intact organs, applied here to the Arabidopsis root tip. A dual miRNAome-targetome analytical interface allowing intuitive data integration/visualization was developed as the basis for in-depth investigations via single-cell-type experimentation. These uncovered an array of so far speculative or hitherto unknown types of spatial miRNA-mediated gene regulation schemes, including via widespread cell-to-cell movement between contiguous layers of distinct identities. This study provides the proof of principle that minimally invasive, genome-scale analysis of miRNA activities within and between single-cell types of whole organs is achievable.
© 2019 The Authors.

Entities:  

Keywords:  AGO1; miRoot; microRNA; targetome; translatome

Mesh:

Substances:

Year:  2019        PMID: 31268601      PMCID: PMC6600646          DOI: 10.15252/embj.2018100754

Source DB:  PubMed          Journal:  EMBO J        ISSN: 0261-4189            Impact factor:   11.598


  62 in total

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10.  Nuclear RNA purification by flow cytometry to study nuclear processes in plants.

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