Engineering a ribozyme cleavage-induced split fluorescent aptamer complementation assay |
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| Authors: | Simon Ausl?nder David Fuchs Samuel Hürlemann David Ausl?nder Martin Fussenegger |
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| Affiliation: | 1Department of Biosystems Science and Engineering, ETH Zurich, Mattenstrasse 26, CH–4058 Basel, Switzerland; 2Faculty of Science, University of Basel, Mattenstrasse 26, CH-4058 Basel, Switzerland |
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| Abstract: | Hammerhead ribozymes are self-cleaving RNA molecules capable of regulating gene expression in living cells. Their cleavage performance is strongly influenced by intra-molecular loop–loop interactions, a feature not readily accessible through modern prediction algorithms. Ribozyme engineering and efficient implementation of ribozyme-based genetic switches requires detailed knowledge of individual self-cleavage performances. By rational design, we devised fluorescent aptamer-ribozyme RNA architectures that allow for the real-time measurement of ribozyme self-cleavage activity in vitro. The engineered nucleic acid molecules implement a split Spinach aptamer sequence that is made accessible for strand displacement upon ribozyme self-cleavage, thereby complementing the fluorescent Spinach aptamer. This fully RNA-based ribozyme performance assay correlates ribozyme cleavage activity with Spinach fluorescence to provide a rapid and straightforward technology for the validation of loop–loop interactions in hammerhead ribozymes. |
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