Programmable RNA detection with CRISPR-Cas12a

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作者
Santosh R. Rananaware
Emma K. Vesco
Grace M. Shoemaker
Swapnil S. Anekar
Luke Samuel W. Sandoval
Katelyn S. Meister
Nicolas C. Macaluso
Long T. Nguyen
Piyush K. Jain
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[1] University of Florida,Department of Chemical Engineering
[2] University of Florida,Department of Biology, CLAS
[3] University of Florida,Department of Molecular Genetics and Microbiology
[4] University of Florida,UF Health Cancer Center
[5] Baylor College of Medicine,Department of Molecular and Human Genetics
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Cas12a, a CRISPR-associated protein complex, has an inherent ability to cleave DNA substrates and is utilized in diagnostic tools to identify DNA molecules. We demonstrate that multiple orthologs of Cas12a activate trans-cleavage in the presence of split activators. Specifically, the PAM-distal region of the crRNA recognizes RNA targets provided that the PAM-proximal seed region has a DNA target. Our method, Split Activator for Highly Accessible RNA Analysis (SAHARA), detects picomolar concentrations of RNA without sample amplification, reverse-transcription, or strand-displacement by simply supplying a short DNA sequence complementary to the seed region. Beyond RNA detection, SAHARA outperforms wild-type CRISPR-Cas12a in specificity towards point-mutations and can detect multiple RNA and DNA targets in pooled crRNA/Cas12a arrays via distinct PAM-proximal seed DNAs. In conclusion, SAHARA is a simple, yet powerful nucleic acid detection platform based on Cas12a that can be applied in a multiplexed fashion and potentially be expanded to other CRISPR-Cas enzymes.
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