A synthetic RNA editing factor edits its target site in chloroplasts and bacteria

Author:

Royan Santana,Gutmann Bernard,Colas des Francs-Small CatherineORCID,Honkanen SuviORCID,Schmidberger Jason,Soet Ashley,Sun Yueming Kelly,Vincis Pereira Sanglard Lilian,Bond Charles S.,Small IanORCID

Abstract

AbstractMembers of the pentatricopeptide repeat (PPR) protein family act as specificity factors in C-to-U RNA editing. The expansion of the PPR superfamily in plants provides the sequence variation required for design of consensus-based RNA-binding proteins. We used this approach to design a synthetic RNA editing factor to target one of the sites in the Arabidopsis chloroplast transcriptome recognised by the natural editing factor CHLOROPLAST BIOGENESIS 19 (CLB19). We show that our synthetic editing factor specifically recognises the target sequence in in vitro binding assays. The designed factor is equally specific for the target rpoA site when expressed in chloroplasts and in the bacterium E. coli. This study serves as a successful pilot into the design and application of programmable RNA editing factors based on plant PPR proteins.

Funder

Department of Education and Training | Australian Research Council

Publisher

Springer Science and Business Media LLC

Subject

General Agricultural and Biological Sciences,General Biochemistry, Genetics and Molecular Biology,Medicine (miscellaneous)

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