Sensitive and multiplexed RNA detection with Cas13 droplets and kinetic barcoding

Author:

Son Sungmin,Lyden Amy,Shu Jeffrey,Stephens Stephanie I.,Fozouni Parinaz,Knott Gavin J.,Smock Dylan C. J.,Liu Tina Y.ORCID,Boehm Daniela,Simoneau Camille,Kumar G. Renuka,Doudna Jennifer A.ORCID,Ott Melanie,Fletcher Daniel A.ORCID

Abstract

SUMMARYRapid and sensitive quantification of RNA is critical for detecting infectious diseases and identifying disease biomarkers. Recent direct detection assays based on CRISPR-Cas13a1–4 avoid reverse transcription and DNA amplification required of gold-standard PCR assays5, but these assays have not yet achieved the sensitivity of PCR and are not easily multiplexed to detect multiple viruses or variants. Here we show that Cas13a acting on single target RNAs loaded into droplets exhibits stochastic nuclease activity that can be used to enable sensitive, rapid, and multiplexed virus quantification. Using SARS-CoV-2 RNA as the target and combinations of CRISPR RNA (crRNA) that recognize different parts of the viral genome, we demonstrate that reactions confined to small volumes can rapidly achieve PCR-level sensitivity. By tracking nuclease activity within individual droplets over time, we find that Cas13a exhibits rich kinetic behavior that depends on both the target RNA and crRNA. We demonstrate that these kinetic signatures can be harnessed to differentiate between different human coronavirus species as well as SARS-CoV-2 variants within a single droplet. The combination of high sensitivity, short reaction times, and multiplexing makes this droplet-based Cas13a assay with kinetic barcoding a promising strategy for direct RNA identification and quantification.

Publisher

Cold Spring Harbor Laboratory

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