Current one-pot clustered regularly interspaced short palindromic repeats diagnostics are limited by the cis-cleavage activity of Cas nucleases, which leads to amplicon degradation during amplification. Here, we report a streamlined strategy that overcomes this limitation. By integrating a bipartite split-crRNA into Cas12a (SCas12a), we separate target recognition from PAM dependency and completely eliminate cis-cleavage while preserving robust trans-cleavage. This strategy is broadly applicable
Elimination of cis -cleavage in CRISPR diagnostics for one-pot rapid nucleic acid detection
Wenhao Yin·Yi Liu·Bin Qiao·Jie Qiao·Xianhua Zhang·Qingyuan Jiang·Ruyi He·Zhili Jin·Xinping Wang·Shuqi Jin