Rapid enzymatic detection of Shigatoxin-producingE. coliusing fluorescence-labeled oligonucleotide substrates

Author:

Ramming Isabell,Lang Christina,Hauf Samuel,Krüger Maren,Worbs Sylvia,Peukert Carsten,Fruth Angelika,Dorner Brigitte G.,Brönstrup Mark,Flieger AntjeORCID

Abstract

AbstractShigatoxin-producingE. coli(STEC) are important human pathogens causing disease ranging from diarrhea to severe hemolytic uremic syndrome. As STEC are transmitted via animals, food, and water, and may produce large outbreaks, their timely and qualified detection including isolate recovery is of high importance, but challenging and labor-intense. Thus, the availability of an easy-to-perform rapid test would be a tremendous advance. Since the common feature and major virulence factor of otherwise multifaceted STEC is the Shiga toxin (Stx), we developed a detection method for Stx, specifically for its catalytic RNA-N-glycosidase activity targeting the Sarcin Ricin Loop (SRL) of 28S ribosomal RNA. To this end, synthetic ssDNA substrates mimicking the SRL were designed and linked to a fluorophore and quencher pair, which conferred a fluorescence signal after cleavage by Stx. Optimal results using bacterial culture supernatants or single colonies were achieved for substrateStxSense 4following 30 to 60 minutes incubation. Importantly, different Stx1 and Stx2 subtypes, diverse STEC serotypes, andShigellawere detected. In conclusion, the assay offers rapid and facile detection of STEC based on a real-time readout for Stx activity. Therefore, it may improve STEC risk evaluation, therapy decisions, outbreak and source detection, and simplify research for antimicrobials.

Publisher

Cold Spring Harbor Laboratory

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