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Unraveling the Bivalent and Rapid Interactions Between a Multivalent RNA Recognition Motif and RNA: A Kinetic Approach
Uppsala University, Disciplinary Domain of Science and Technology, Chemistry, Department of Chemistry - BMC, Biochemistry. Ridgeview Instruments AB, SE-75643 Uppsala, Sweden..ORCID iD: 0000-0001-7595-4851
Univ Florence, Ugo Schiff & Magnet Resonance Ctr CERM, Dept Chem, I-50019 Florence, Italy.;Giotto Biotech srl, I-50019 Florence, Italy.;Univ Dundee, MRC Prot Phosphorylat & Ubiquitylat Unit, Dundee DD1 5EH, Scotland..
Univ Florence, Ugo Schiff & Magnet Resonance Ctr CERM, Dept Chem, I-50019 Florence, Italy.;Giotto Biotech srl, I-50019 Florence, Italy..
Uppsala University, Disciplinary Domain of Science and Technology, Chemistry, Department of Chemistry - BMC, Biochemistry. Uppsala University, Science for Life Laboratory, SciLifeLab.ORCID iD: 0000-0003-2728-0340
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2024 (English)In: Biochemistry, ISSN 0006-2960, E-ISSN 1520-4995, Vol. 63, no 21, p. 2816-2829Article in journal (Refereed) Published
Abstract [en]

The kinetics of the interaction between Musashi-1 (MSI1) and RNA have been characterized using surface plasmon resonance biosensor analysis. Truncated variants of human MSI1 encompassing the two homologous RNA recognition motifs (RRM1 and RRM2) in tandem (aa 1-200), and the two RRMs in isolation (aa 1-103 and aa 104-200, respectively) were produced. The proteins were injected over sensor surfaces with immobilized RNA, varying in sequence and length, and with one or two RRM binding motifs. The interactions of the individual RRMs with all RNA variants were well described by a 1:1 interaction model. The interaction between the MSI1 variant encompassing both RRM motifs was bivalent and rapid for all RNA variants. Due to difficulties in fitting this complex data using standard procedures, we devised a new method to quantify the interactions. It revealed that two RRMs in tandem resulted in a significantly longer residence time than a single RRM. It also showed that RNA with double UAG binding motifs and potential hairpin structures forms less stable bivalent complexes with MSI1 than the single UAG motif containing linear RNA. Substituting the UAG binding motif with a CAG sequence resulted in a reduction of the affinity of the individual RRMs, but for MSI1, this reduction was strongly enhanced, demonstrating the importance of bivalency for specificity. This study has provided new insights into the interaction between MSI1 and RNA and an understanding of how individual domains contribute to the overall interaction. It provides an explanation for why many RNA-binding proteins contain dual RRMs.
Place, publisher, year, edition, pages
American Chemical Society (ACS), 2024. Vol. 63, no 21, p. 2816-2829
National Category
Biochemistry Molecular Biology
Identifiers
URN: urn:nbn:se:uu:diva-547901DOI: 10.1021/acs.biochem.4c00301ISI: 001336862700001PubMedID: 39397705Scopus ID: 2-s2.0-85206470797OAI: oai:DiVA.org:uu-547901DiVA, id: diva2:1929205
Funder
European Commission, 813239Available from: 2025-01-20 Created: 2025-01-20 Last updated: 2025-03-06Bibliographically approved
In thesis
1. Insights into Musashi-1 interactions with RNA: From in vitro kinetics to cell biology
Open this publication in new window or tab >>Insights into Musashi-1 interactions with RNA: From in vitro kinetics to cell biology
2025 (English)Doctoral thesis, comprehensive summary (Other academic)
Abstract [en]

The interaction between proteins and RNA has gained increased attention as a key regulatory mechanism of RNA translation beyond conventional postulated mechanisms. It is also involved in various pathologies, including cancer and neurodegenerative disorders. In this thesis, the interactions between the RNA-binding protein Musashi-1 (MSI1) and both linear and hairpin-like RNA strands have been investigated using time-resolved and structural technologies, such as SPR biosensors, LigandTracer, and NMR.

Initially, the interactions of the two RNA recognition motifs (RRM1 and RRM2) in MSI1 were characterized separately. Both motifs exhibited high affinity for the UAG motif, with no significant difference between linear and hairpin-like RNA. These interactions followed a 1:1 binding mechanism, with relatively fast, but well-defined association and dissociation rate constants. Next, the interaction of the N-terminal region of MSI1, containing both RRMs, was analyzed, revealing a bivalent binding mechanism. Commercial software was not suitable for distinguishing the fast monovalent and slow bivalent interactions. Therefore, a novel method was developed to quantify kinetic rate constants and binding affinities.

To explore the determinants for the specificity of the interaction, RNA mutants and protein variants were designed to shift RRM2 recognition from the UAG to the CAG motifs. Comprehensive characterization confirmed the impact of these mutations and RNA structural modifications on the interaction.

Additionally, to examine MSI1 regulatory role in synthetic biology, a post-transcriptionally controlled circuit was engineered in E. coli using MSI1 binding to RNA strands. This system, developed on solid media, utilized sfGFP fluorescence as a reporter. Data analysis using the Gompertz growth model correlated well with previously published data on bacteria in suspension. The regulatory effect of oleic acid, a potential MSI1 allosteric inhibitor, was confirmed using this assay. Similarly, MSI1 inhibition effects were assessed in HCT-116 colorectal cancer cells, revealing that both oleic acid and luteolin impacted cell proliferation and CD44v6 receptor expression.

In conclusion, this work has resulted in novel methods and insights for studying and understanding the kinetics and mechanisms of protein-RNA interactions.
Place, publisher, year, edition, pages
Uppsala: Acta Universitatis Upsaliensis, 2025. p. 78
Series
Digital Comprehensive Summaries of Uppsala Dissertations from the Faculty of Science and Technology, ISSN 1651-6214 ; 2508
Keywords
Interaction kinetics, biochemistry, RNA-protein interactions, RNA binding proteins, synthetic biology
National Category
Biochemistry Biophysics Cell and Molecular Biology
Research subject
Biochemistry
Identifiers
urn:nbn:se:uu:diva-552069 (URN)978-91-513-2408-1 (ISBN)
Public defence
2025-04-25, A1:107, BMC, Husargatan 3, Uppsala, 09:00 (English)
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Supervisors
Available from: 2025-04-02 Created: 2025-03-06 Last updated: 2025-04-02

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Pérez-Ropero, GuillermoDanielson, U. HelenaBuijs, Jos

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