Sensitive detection of a bacterial pathogen using allosteric probe-initiated catalysis and CRISPR-Cas13a amplification reaction

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作者
Jinjin Shen
Xiaoming Zhou
Yuanyue Shan
Huahua Yue
Ru Huang
Jiaming Hu
Da Xing
机构
[1] MOE Key Laboratory of Laser Life Science & Institute of Laser Life Science,
[2] South China Normal University,undefined
[3] College of Biophotonics,undefined
[4] South China Normal University,undefined
[5] School of Life Sciences,undefined
[6] South China Normal University,undefined
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The ability to detect low numbers of microbial cells in food and clinical samples is highly valuable but remains a challenge. Here we present a detection system (called ‘APC-Cas’) that can detect very low numbers of a bacterial pathogen without isolation, using a three-stage amplification to generate powerful fluorescence signals. APC-Cas involves a combination of nucleic acid-based allosteric probes and CRISPR-Cas13a components. It can selectively and sensitively quantify Salmonella Enteritidis cells (from 1 to 105 CFU) in various types of samples such as milk, showing similar or higher sensitivity and accuracy compared with conventional real-time PCR. Furthermore, APC-Cas can identify low numbers of S. Enteritidis cells in mouse serum, distinguishing mice with early- and late-stage infection from uninfected mice. Our method may have potential clinical applications for early diagnosis of pathogens.
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