RPB0340

Pathogen Description

Target Pathogen Pathogen Name NCBI Taxonomy ID Order Family Genus Species Pathogen type
Bordetella pertussis CS Bordetella pertussis CS, Bordetella pertussis str. CS, Bordetella pertussis strain CS 1017264 Burkholderiales Alcaligenaceae Bordetella Bordetella pertussis Bacterium

Primer Description

Primer Name Sequence(5'-3') Length(bp) Primer Final Concentration(μM) GC Content(%) Predicted Melting Temperature(℃) Molecular Weight(g/moles) Positions in GenBank accession number
FP CCTACGGGTCTGTATCACGAGCAAGCGGC 29 10 μM 62.07 68.79 8903.82 \
RP GCGTCTGTCCATAGCGAGCCAGCACGTAGC 30 10 μM 63.33 70.45 9193.01 \

Gene Description

Target Gene GenBank ID
IS1663 gene CP046995.1

Assay Description

Application Assay Primer Designing Software Reaction Time(min) Assay Temperature(℃) Readout System(s) Limit of Detection(LoD) Sensitivity(%) Specificity(%)
The rapid, sensitive and specific Rcod system provides ideas for the establishment of CRISPR-based one-step nucleic acid detection and may aid the development of reliable point-of-care nucleic acid tests. RAA-CRISPR\Cas12b \ 30 min 37°C CRISPR\Cas12b 0.2 copies/μL 0.9796 0.9919

Publication Description

Year of Publication Title Author(s) Journal PMID DOI
2024 Rapid and sensitive detection of nucleic acids using an RAA-CRISPR\Cas12b one-pot detection assay (Rcod) Kangfeng Lin,Kaihu Yao,Xiao Li,Qinghan Li,Xiangju Guo,Weixin You,Wenjing Ren,Ya Bian,Jianguang Guo,Zhen Sun,Rui Zhang,Xiaoqing Yang,Zhiyong Li,Boan Li Talanta 38277969 10.1016/j.talanta.2023.125616

Rapid and sensitive detection of nucleic acids using an RAA-CRISPR\Cas12b one-pot detection assay (Rcod)

Author(s):

Kangfeng Lin,Kaihu Yao,Xiao Li,Qinghan Li,Xiangju Guo,Weixin You,Wenjing Ren,Ya Bian,Jianguang Guo,Zhen Sun,Rui Zhang,Xiaoqing Yang,Zhiyong Li,Boan Li

Journal:

Talanta

Year:

2024

Abstract:

Rapid, sensitive and specific methods are crucial for nucleic acid detection. CRISPR/Cas12b has recently been widely used in nucleic acid detection. However, due to its thermophagic property, DNA isothermal recombinase-aided amplification (RAA) and subsequent CRISPR/Cas12b detection require two separate reactions, which is cumbersome and inconvenient and may cause aerosol pollution. In this study, we propose an RAA-CRISPR/Cas12b one-pot detection assay (Rcod) for Bordetella pertussis detection without additional amplification product transfer steps. The time from sample processing to response time was less than 30 min using nucleic acid extraction-free method, and the sensitivity reached 0.2 copies/μL. In this system, Alicyclobacillus acidoterrestris Cas12b protein (AacCas12b) exhibited strong and specific trans-cleavage activity at a constant temperature of 37 °C, while the cis-cleavage activity was weak. This characteristic reduces the interference of AacCas12b with nucleic acids in the system. Compared with real-time PCR, our Rcod system detected B. pertussis in 221 clinical samples with a sensitivity and specificity of 97.96 % and 99.19 %, respectively, with nucleic acid extraction-free method. The rapid, sensitive and specific Rcod system provides ideas for the establishment of CRISPR-based one-step nucleic acid detection and may aid the development of reliable point-of-care nucleic acid tests. IMPORTANCE: Pertussis is an acute respiratory infection caused by B. pertussis that is highly contagious and potentially fatal, and early diagnosis is essential for the treatment of whooping cough. In this study, we found that AacCas12b has high and strongly specific trans-cleavage activity at lower temperatures. A RAA-CRISPR/Cas12b one-step detection platform (Rcod) without interference with amplification was developed. In addition, the combination of Rcod and nucleic acid extraction-free method can quickly and accurately detect the qualitative detection of B. pertussis, and the detection results are visualized, which makes the pathogen nucleic acid detection and analysis process simpler, and provides a new method for the rapid clinical diagnosis of B. pertussis.