An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning

Loading of mRNA onto the ribosomal 43S pre-initiation complex (PIC) and its subsequent scanning require the removal of the secondary structure of the by RNA helicases such as eIF4A. However, the topology and mechanics of the scanning complex bound to mRNA (48S-PIC) and the influence of its solvent-s...

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Main Authors: Irene Díaz-López, René Toribio, Juan José Berlanga, Iván Ventoso
Format: Article
Language:English
Published: eLife Sciences Publications Ltd 2019-12-01
Series:eLife
Subjects:
Online Access:https://elifesciences.org/articles/48246
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spelling doaj-1bdedf8ed2854ed0849d75dd8957a7142021-05-05T18:08:23ZengeLife Sciences Publications LtdeLife2050-084X2019-12-01810.7554/eLife.48246An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanningIrene Díaz-López0René Toribio1Juan José Berlanga2https://orcid.org/0000-0002-2408-6561Iván Ventoso3https://orcid.org/0000-0001-7887-3520Centro de Biología Molecular “Severo Ochoa” (CSIC-UAM), Departamento de Biología Molecular, Universidad Autónoma de Madrid (UAM), Madrid, SpainCentro de Biotecnología y Genómica de Plantas, Madrid, SpainCentro de Biología Molecular “Severo Ochoa” (CSIC-UAM), Departamento de Biología Molecular, Universidad Autónoma de Madrid (UAM), Madrid, SpainCentro de Biología Molecular “Severo Ochoa” (CSIC-UAM), Departamento de Biología Molecular, Universidad Autónoma de Madrid (UAM), Madrid, SpainLoading of mRNA onto the ribosomal 43S pre-initiation complex (PIC) and its subsequent scanning require the removal of the secondary structure of the by RNA helicases such as eIF4A. However, the topology and mechanics of the scanning complex bound to mRNA (48S-PIC) and the influence of its solvent-side composition on the scanning process are poorly known. Here, we found that the ES6S region of the 48S-PIC constitutes an extended binding channel for eIF4A-mediated unwinding of mRNA and scanning. Blocking ES6S inhibited the cap-dependent translation of mRNAs that have structured 5′ UTRs (including G-quadruplexes), many of which are involved in signal transduction and growth, but it did not affect IRES-driven translation. Genome-wide analysis of mRNA translation revealed a great diversity in ES6S-mediated scanning dependency. Our data suggest that mRNA threading into the ES6S region makes scanning by 48S PIC slower but more processive. Hence, we propose a topological and functional model of the scanning 48S-PIC.https://elifesciences.org/articles/48246ES6S regiontranslationscanningmRNA secondary structureG quadruplex
collection DOAJ
language English
format Article
sources DOAJ
author Irene Díaz-López
René Toribio
Juan José Berlanga
Iván Ventoso
spellingShingle Irene Díaz-López
René Toribio
Juan José Berlanga
Iván Ventoso
An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning
eLife
ES6S region
translation
scanning
mRNA secondary structure
G quadruplex
author_facet Irene Díaz-López
René Toribio
Juan José Berlanga
Iván Ventoso
author_sort Irene Díaz-López
title An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning
title_short An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning
title_full An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning
title_fullStr An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning
title_full_unstemmed An mRNA-binding channel in the ES6S region of the translation 48S-PIC promotes RNA unwinding and scanning
title_sort mrna-binding channel in the es6s region of the translation 48s-pic promotes rna unwinding and scanning
publisher eLife Sciences Publications Ltd
series eLife
issn 2050-084X
publishDate 2019-12-01
description Loading of mRNA onto the ribosomal 43S pre-initiation complex (PIC) and its subsequent scanning require the removal of the secondary structure of the by RNA helicases such as eIF4A. However, the topology and mechanics of the scanning complex bound to mRNA (48S-PIC) and the influence of its solvent-side composition on the scanning process are poorly known. Here, we found that the ES6S region of the 48S-PIC constitutes an extended binding channel for eIF4A-mediated unwinding of mRNA and scanning. Blocking ES6S inhibited the cap-dependent translation of mRNAs that have structured 5′ UTRs (including G-quadruplexes), many of which are involved in signal transduction and growth, but it did not affect IRES-driven translation. Genome-wide analysis of mRNA translation revealed a great diversity in ES6S-mediated scanning dependency. Our data suggest that mRNA threading into the ES6S region makes scanning by 48S PIC slower but more processive. Hence, we propose a topological and functional model of the scanning 48S-PIC.
topic ES6S region
translation
scanning
mRNA secondary structure
G quadruplex
url https://elifesciences.org/articles/48246
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