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               <dc:title>Dynamic interplay between RPL3- and RPL3L-containing ribosomes modulates mitochondrial activity in the mammalian heart</dc:title>
               <dc:creator>Milenkovic, Ivan</dc:creator>
               <dc:creator>Santos Vieira, Helaine Graziele</dc:creator>
               <dc:creator>Lucas, Morghan C.</dc:creator>
               <dc:creator>Ruiz-Orera, Jorge</dc:creator>
               <dc:creator>Patone, Giannino</dc:creator>
               <dc:creator>Kesteven, Scott</dc:creator>
               <dc:creator>Wu, Jianxin</dc:creator>
               <dc:creator>Feneley, Michael</dc:creator>
               <dc:creator>Espadas, Guadalupe</dc:creator>
               <dc:creator>Sabidó Aguadé, Eduard, 1981-</dc:creator>
               <dc:creator>Hübner, Norbert</dc:creator>
               <dc:creator>van Heesch, Sebastiaan</dc:creator>
               <dc:creator>Völkers, Mirko</dc:creator>
               <dc:creator>Novoa, Eva Maria</dc:creator>
               <dc:description>The existence of naturally occurring ribosome heterogeneity is now a well-acknowledged phenomenon. However, whether this heterogeneity leads to functionally diverse &amp;apos;specialized ribosomes&amp;apos; is still a controversial topic. Here, we explore the biological function of RPL3L (uL3L), a ribosomal protein (RP) paralogue of RPL3 (uL3) that is exclusively expressed in skeletal muscle and heart tissues, by generating a viable homozygous Rpl3l knockout mouse strain. We identify a rescue mechanism in which, upon RPL3L depletion, RPL3 becomes up-regulated, yielding RPL3-containing ribosomes instead of RPL3L-containing ribosomes that are typically found in cardiomyocytes. Using both ribosome profiling (Ribo-seq) and a novel orthogonal approach consisting of ribosome pulldown coupled to nanopore sequencing (Nano-TRAP), we find that RPL3L modulates neither translational efficiency nor ribosome affinity towards a specific subset of transcripts. In contrast, we show that depletion of RPL3L leads to increased ribosome-mitochondria interactions in cardiomyocytes, which is accompanied by a significant increase in ATP levels, potentially as a result of fine-tuning of mitochondrial activity. Our results demonstrate that the existence of tissue-specific RP paralogues does not necessarily lead to enhanced translation of specific transcripts or modulation of translational output. Instead, we reveal a complex cellular scenario in which RPL3L modulates the expression of RPL3, which in turn affects ribosomal subcellular localization and, ultimately, mitochondrial activity.</dc:description>
               <dc:description>The European Union&amp;apos;s Horizon 2020 Research and Innovation Program under the Marie Skodowska-Curie grant agreement [713673]; the Australian Research Council [DE170100506 to E.M.N.]; the Spanish Ministry of Economy, Industry and Competitiveness (MEIC) [PGC2018-098152-A-100 to E.M.N.]; the European Union Horizon 2020 Research and Innovation Program ERC advanced grant [AdG788970 to N.H.] and ERC starting grant [StG101042103 to E.M.N.]; the Leducq Foundation [16CVD03 to N.H.]; the Chan Zuckerberg Foundation [2019-20266 to N.H.]; and ‘la Caixa’ INPhINIT PhD fellowship [LCF/BQ/DI18/11660028 to I.M.]. We acknowledge the support of the MEIC to the EMBL partnership, Centro de Excelencia Severo Ochoa and CERCA Programme/Generalitat de Catalunya. The CRG/UPF Proteomics Unit is part of the Spanish Infrastructure for Omics Technologies (ICTS OmicsTech) and it is a member of the ProteoRed PRB3 consortium which is supported by grant PT17/0019 of the PE I + D + i 2013-2016 from the Instituto de Salud Carlos III (ISCIII) and ERDF. Conflict of interest statement. E.M.N. has received travel expenses from ONT to participate in nanopore conferences. I.M. has received a travel bursary from ONT to present his work in international conferences. E.M.N. is Scientific Advisory Board member for IMMAGINA Biotech. The authors declare that they have no competing interests.</dc:description>
               <dc:date>2023-09-26T06:30:54Z</dc:date>
               <dc:date>2023-09-26T06:30:54Z</dc:date>
               <dc:date>2023</dc:date>
               <dc:type>info:eu-repo/semantics/article</dc:type>
               <dc:type>info:eu-repo/semantics/publishedVersion</dc:type>
               <dc:relation>Nucleic Acids Res. 2023;51(11):5301-24</dc:relation>
               <dc:relation>info:eu-repo/grantAgreement/EC/H2020/713673</dc:relation>
               <dc:relation>info:eu-repo/grantAgreement/ES/2PE/PGC2018-098152-A-100</dc:relation>
               <dc:relation>info:eu-repo/grantAgreement/EC/H2020/788970</dc:relation>
               <dc:rights>© The Author(s) 2023. This is an Open Access article distributed under the terms of the Creative Commons Attribution-NonCommercial License (http://creativecommons.org/licenses/by-nc/4.0/), which permits non-commercial re-use, distribution, and reproduction in any medium, provided the original work is properly cited. For commercial re-use, please contact journals.permissions@oup.com</dc:rights>
               <dc:rights>http://creativecommons.org/licenses/by-nc/4.0/</dc:rights>
               <dc:rights>info:eu-repo/semantics/openAccess</dc:rights>
               <dc:publisher>Oxford University Press</dc:publisher>
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