Thermodynamic profiles for cotranslational trigger factor substrate recognition

Author:

Herling Therese W.1ORCID,Cassaignau Anaïs M. E.2ORCID,Wentink Anne S.2ORCID,Peter Quentin A. E.1ORCID,Kumar Pavan C.1,Kartanas Tadas1ORCID,Schneider Matthias M.1ORCID,Cabrita Lisa D.2ORCID,Christodoulou John2ORCID,Knowles Tuomas P. J.1ORCID

Affiliation:

1. Yusuf Hamied Department of Chemistry, University of Cambridge, Cambridge CB2 1EW, UK.

2. Institute of Structural and Molecular Biology, University College London and Birkbeck College, London WC1 6BT, UK.

Abstract

Molecular chaperones are central to the maintenance of proteostasis in living cells. A key member of this protein family is trigger factor (TF), which acts throughout the protein life cycle and has a ubiquitous role as the first chaperone encountered by proteins during synthesis. However, our understanding of how TF achieves favorable interactions with such a diverse substrate base remains limited. Here, we use microfluidics to reveal the thermodynamic determinants of this process. We find that TF binding to empty 70S ribosomes is enthalpy-driven, with micromolar affinity, while nanomolar affinity is achieved through a favorable entropic contribution for both intrinsically disordered and folding-competent nascent chains. These findings suggest a general mechanism for cotranslational TF function, which relies on occupation of the exposed TF-substrate binding groove rather than specific complementarity between chaperone and nascent chain. These insights add to our wider understanding of how proteins can achieve broad substrate specificity.

Publisher

American Association for the Advancement of Science (AAAS)

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