| Literature DB >> 33595922 |
Qingzhou Meng1,2, Xinjie Wang1,3,4, Yanqun Wang1, Lu Dang2, Xinyi Liu5, Xiaodong Ma4, Tian Chi6, Xian Wang3,6, Qin Zhao7, Guang Yang3, Ming Liu1, Xingxu Huang1,6, Peixiang Ma1,3.
Abstract
Detection of pathogens with single-nucleotide variations is indispensable for the disease tracing, but remains technically challenging. The D614G mutation in the SARS-CoV-2 spike protein is known to markedly enhance viral infectivity but is difficult to detect. Here, we report an effective approach called "synthetic mismatch integrated crRNA guided Cas12a detection" (symRNA-Cas12a) to detect the D614 and G614 variants effectively. Using this method, we systemically screened a pool of crRNAs that contain all the possible nucleotide substitutions covering the -2 to +2 positions around the mutation and identify one crRNA that can efficiently increase the detection specificity by 13-fold over the ancestral crRNA. With this selected crRNA, the symRNA-Cas12a assay can detect as low as 10 copies of synthetic mutant RNA and the results are confirmed to be accurate by Sanger sequencing. Overall, we have developed the symRNA-Cas12a method to specifically, sensitively and rapidly detect the SARS-CoV-2 D614G mutation.Entities:
Keywords: COVID-19; CRISPR-based detection; CRISPR/Cas12a; D614G; SARS-CoV-2
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Year: 2021 PMID: 33595922 DOI: 10.1002/biot.202100040
Source DB: PubMed Journal: Biotechnol J ISSN: 1860-6768 Impact factor: 4.677