Issue 76, 2024

High-contrast imaging of cellular non-repetitive drug-resistant genes via in situ dead Cas12a-labeled PCR

Abstract

In situ imaging of genes of pathogenic bacteria can profile cellular heterogeneity, such as the emergence of drug resistance. Fluorescence in situ hybridization (FISH) serves as a classic approach to image mRNAs inside cells, but it remains challenging to elucidate genomic DNAs and relies on multiple fluorescently labeled probes. Herein, we present a dead Cas12a (dCas12a)-labeled polymerase chain reaction (CasPCR) assay for high-contrast imaging of cellular drug-resistant genes. We employed a syncretic dCas12a-green fluorescent protein (dCas12a–GFP) to tag the amplicons, thereby enabling high-contrast imaging and avoiding multiple fluorescently labeled probes. The CasPCR assay can quantify quinolone-resistant Salmonella enterica in mixed populations and identify them isolated from poultry farms.

Graphical abstract: High-contrast imaging of cellular non-repetitive drug-resistant genes via in situ dead Cas12a-labeled PCR

Supplementary files

Article information

Article type
Communication
Submitted
24 Jun 2024
Accepted
23 Aug 2024
First published
28 Aug 2024

Chem. Commun., 2024,60, 10524-10527

High-contrast imaging of cellular non-repetitive drug-resistant genes via in situ dead Cas12a-labeled PCR

R. Deng, X. Zhang, J. Cao, X. Liu, Y. Zhang, F. Wang and X. Xia, Chem. Commun., 2024, 60, 10524 DOI: 10.1039/D4CC03059A

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