The structure and mechanism of action of a distinct class of dicistrovirus intergenic region IRESs

Author:

Abaeva Irina S1,Young Christina2,Warsaba Reid2,Khan Nadiyah2,Tran Lan Vy2,Jan Eric2,Pestova Tatyana V1ORCID,Hellen Christopher U T1ORCID

Affiliation:

1. Department of Cell Biology, SUNY Downstate Health Sciences University , Brooklyn, NY 11203, USA

2. Department of Biochemistry and Molecular Biology, Life Sciences Institute, University of British Columbia , Vancouver , BC V6T 1Z3, Canada

Abstract

Abstract Internal ribosomal entry sites (IRESs) engage with the eukaryotic translation apparatus to promote end-independent initiation. We identified a conserved class of ∼150 nt long intergenic region (IGR) IRESs in dicistrovirus genomes derived from members of the phyla Arthropoda, Bryozoa, Cnidaria, Echinodermata, Entoprocta, Mollusca and Porifera. These IRESs, exemplified by Wenling picorna-like virus 2, resemble the canonical cricket paralysis virus (CrPV) IGR IRES in comprising two nested pseudoknots (PKII/PKIII) and a 3′-terminal pseudoknot (PKI) that mimics a tRNA anticodon stem–loop base-paired to mRNA. However, they are ∼50 nt shorter than CrPV-like IRESs, and PKIII is an H-type pseudoknot that lacks the SLIV and SLV stem–loops that are primarily responsible for the affinity of CrPV-like IRESs for the 40S ribosomal subunit and that restrict initial binding of PKI to its aminoacyl (A) site. Wenling-class IRESs bound strongly to 80S ribosomes but only weakly to 40S subunits. Whereas CrPV-like IRESs must be translocated from the A site to the peptidyl (P) site by elongation factor 2 for elongation to commence, Wenling-class IRESs bound directly to the P site of 80S ribosomes, and decoding begins without a prior translocation step. A chimeric CrPV clone containing a Wenling-class IRES was infectious, confirming that the IRES functioned in cells.

Funder

National Institutes of Health

Canadian Institutes of Health Research

Publisher

Oxford University Press (OUP)

Subject

Genetics

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