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Internal ribosome entry sites enhance translation in trans in antisense non-coding SINEUP and circular RNAs

Nucleic Acids Research. 2025-08; 
Sabrina D'Agostino, Abraham Tettey-Matey, Massimiliano Volpe, Bianca Pierattini, Mattia D'Agostino, Denisa Smělá, Federico Ansaloni, Laura Broglia, Pierre Lau, Omar Peruzzo, Clarissa Braccia, Andrea Armirotti, Margherita Scarpato, Devid Damiani, Gloria Ros, Valerio Di Carlo, Federica Maniscalco, Elias Bechara, Gian Gaetano Tartaglia, Piero Carninci, Claudio Santoro, Francesca Persichetti, Luca Pandolfini, Angelita Simonetti, Stefano Espinoza, Silvia Zucchelli, Remo Sanges, Carlotta Bon, Stefano Gustincich Center for Human Technologies, Non-coding RNAs and RNA-based therapeutics, Istituto Italiano di Tecnologia (IIT), Via Enrico Melen 83, Genova 16152, Italy.
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Custom Vector Construction Synthetic SINEUP constructs were designed to evaluate the regulatory activity of invSINEB2 and IRES elements on target mRNA translation in cis and trans. All studied inserts, unless purchased from GenScript Biotech (Netherlands) B.V. Get A Quote

摘要

Sequences in the 5'-untranslated regions of cellular and viral mRNAs can function as internal ribosome entry sites (IRESs), driving cis-acting translation of the downstream protein-coding open reading frame. Here we demonstrate that RNA sequences with either newly identified or well-characterized IRES activity can also induce trans-acting translation of an independent mRNA species through an antisense sequence. SINEUPs are antisense long non-coding RNAs that enhance the translation of overlapping sense mRNAs in trans by employing two critical domains: the invSINEB2 sequence, which up-regulates translation (effector domain), and an antisense region providing target specificity (binding domain). First, we show th... More

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